BIOLOGICAL CHARACTERIZATION OF TRITRICHOMONAS FOETUS OF BOVINE AND FELINE ORIGIN Except where reference is made to the work of others, the work described in this dissertation is my own or was done in collaboration with my advisory committee. This dissertation does not include proprietary or classified information. __________________________________ Heather Dawn Stockdale Certificate of Approval: _______________________________ ______________________________ M. Daniel Givens Byron L. Blagburn, Chair Associate Professor Distinguished University Professor Pathobiology Pathobiology _______________________________ ______________________________ Christine C. Dykstra Jennifer A. Spencer Associate Professor Instructor Pathobiology Pathobiology _______________________________ ______________________________ David S. Lindsay Joe F. Pittman Profesor Interim Dean Biomedical Sciences & Pathobiology Graduate School Virginia-Maryland Regional College of Veterinary Medicine BIOLOGICAL CHARACTERIZATION OF TRITRICHOMONAS FOETUS OF BOVINE AND FELINE ORIGIN Heather Dawn Stockdale A Dissertation Submitted to the Graduate Faculty of Auburn University in Partial Fulfillment of the Requirements for the Degree of Doctor of Philosophy Auburn, Alabama May 10, 2008 iii BIOLOGICAL CHARACTERIZATION OF TRITRICHOMONAS FOETUS OF BOVINE AND FELINE ORIGIN Heather Dawn Stockdale Permission is granted to Auburn University to make copies of this dissertation at its discretion, upon request of individuals or institutions and at their expense. The author reserves all publication rights. ______________________________ Signature of Author ______________________________ Date of Graduation iv VITA Heather Dawn Stockdale is the daughter of Ernest Neil and Penny Stockdale of Milton, Kentucky. She was born on November 19, 1976 in Madison, Indiana and graduated with honors from Trimble County High School in 1995. She began her undergraduate studies at the University of Kentucky, graduating in 1999 with a Bachelor?s of Science degree in Biology. In 2002, she enrolled in the graduate program at Appalachian State University. She graduated summa cum laude in 2004 with a Master?s of Science degree in Biology and was nominated and accepted to the Alpha Epsilon Lambda Graduate and Professional Honor Society. In 2004, she began her Doctoral work in Parasitology at Auburn University College of Veterinary Medicine, graduating cum laude with a Doctorate degree in Biomedical Sciences on May 10, 2008. v DISSERTATION ABSTRACT BIOLOGICAL CHARACTERIZATION OF TRITRICHOMONAS FOETUS OF BOVINE AND FELINE ORIGIN Heather Dawn Stockdale Doctor of Philosophy, May 10, 2008 (M.S., Appalachian State University, 2004) (B.S., University of Kentucky, 1999) 120 Typed Pages Directed by Byron L. Blagburn Tritrichomonas foetus is a causative agent of venereal trichomoniasis in cattle characterized by early fetal death and post-coital pyometra. Reports have suggested that T. foetus (or a similar organism) is also the causative agent of large-bowel diarrhea in cats, characterized by large bowel inflammation, flatulence, tenesmus and fecal incontinence. Diagnosis of feline trichomoniasis is based upon observation of live organisms in direct smears, cultured feces or by amplification of specific genes using polymerase chain reaction (PCR). No documented treatment successfully eliminates T. foetus consistently from naturally infected cats. Certain drugs may reduce clinical signs and numbers of trichomonads from feces, but relapses of diarrhea commonly occur. In the first study I attempted to estimate the prevalence of feline trichomoniasis within the pet population in the United States. To do so, 173 fecal samples were collected from cats in 16 states. Feces were scored for consistency and subjected to vi culture and PCR analysis. Seventeen of 173 (10%) were positive for T. foetus by both fecal culture and PCR. Results indicate that T. foetus is prevalent in the pet population and that its presence correlates with the presence of diarrhea. Experimental infections were conducted to determine if T. foetus, whether of bovine or feline origin, are biologically distinct. In the second study, two groups of virgin Angus heifers were inoculated with either T. foetus isolated from a pyometritic cow or a naturally infected cat. Vaginal, cervical, and uterine mucus samples were analyzed over an 11-week period and a single transcervical uterine biopsy sample was obtained from each animal, revealing severe damage to the endometrium in heifers infected with the bovine isolate of T. foetus. This was not observed in heifers infected with the feline isolate. In the third study, 6 cats were inoculated with a bovine (D-1) isolate of T. foetus and one cat was inoculated with a feline (AUTf-1) isolate of T. foetus. Fecal samples from each cat were collected and subjected to culture over a period of five weeks. By PI day 15 the cat infected with the feline (AUTf-1) isolate had become culture positive for trichomonads while only one of six cats infected with the bovine (D-1) isolate was positive by PI day 32. At necropsy, the intestine of each cat was divided into five sections and the contents were collected and subjected to culture. The cat that received the feline (AUTf-1) isolate was positive in 4 of 5 intestinal sections and two cats infected with the bovine (D-1) isolate were positive in only one intestinal section. The combined results of studies two and three indicate that the disease caused by feline and bovine isolates of T. foetus in cattle are not identical and the susceptibility of cats to the feline (AUTf-1) and bovine (D-1) isolates T. foetus also appears demonstrably different. vii ACKNOWLEDGMENTS I would like to thank my mentor, Dr. Byron L. Blagburn, for his guidance and support during my time at Auburn University. Additionally, thanks are due to my committee members, Dr. M. Daniel Givens, Dr. Jennifer A. Spencer, Dr. Christine C. Dykstra and Dr. David S. Lindsay. The experimental infection studies would not have been possible without the help of Dr. Soren Rodning, Dr. Ron H. BonDurant, Dr. Ray Dillon, Ellie Gripshover, Charles Price, Jamie Butler, Tracey Land, Sharon Barney, Dr. David Stringfellow and the caretakers at the North Auburn Beef Unit, Dr. Nancy Cox and Dr. Henry Baker. I would also like to thank Dr. Mark Carpenter for assistance with statistical analysis and Drs. Stephen Lenz, Joseph Newton and Elizabeth Welles for assistance with histopathological analysis. Thanks are due to Dr. Richard Bird, Patricia Deinnocentes and Scott Lenaghan for assistance with molecular analysis and photomicrographs taken throughout the studies were possible with the assistance of Drs. David Miller, Maria Toivio-Kinnucan, John Dennis and Pete Christopherson. Finally, thanks and gratitude are due to my parents, Neil and Penny, my brother Jonathan and fianc? Trey for their unconditional love and support during this challenging time in my life. viii Journal used The Journal of Parasitology Computer software used Microsoft? Windows? XP Professional SAS? Statistical Software Vector NTI? Advance 10 Phylogeny Inference Package (PHYLIP) ver. 3.67 Phylodraw ver. 0.8 ix TABLE OF CONTENTS LIST OF TABLES xii LIST OF FIGURES xiii CHAPTER I. LITERATURE REVIEW: TRITRICHOMONAS FOETUS AND TRICHOMONIASIS 1 The Trichomonads 1 Figure 1.1 2 Table 1.1 4 Bovine Trichomoniasis 5 Figure 1.2 8 Figure 1.3 9 Feline Trichomoniasis 11 Research Objectives 14 CHAPTER II. TRITRICHOMONAS FOETUS INFECTIONS IN SURVEYED PET CATS 16 Introduction 16 Materials and Methods 17 Study population 17 Sample collection 17 Sample analysis 18 Figure 2.1 19 Results 20 Table 2.1 21 Table 2.2 22 Discussion 24 CHAPTER III. EXPERIMENTAL INFECITON OF CATTLE WITH A FELINE ISOLATE OF TRITRICHOMONAS FOETUS 28 Introduction 28 Materials and Methods 29 Heifers and estrus synchronization 29 Organisms and inoculation 31 Sampling procedures 31 Sample evaluations 33 Statistical analysis 33 x Results 34 Trichomonads recovered from samples 34 Figure 3.1 35 Figure 3.2 36 Uterine biopsies 37 Table 3.1 38 Discussion 39 Figure 3.3 40 CHAPTER IV. EXPERIMENTAL INFECTION OF CATS (FELIS CATUS) WITH TRITRICHOMONAS FOETUS ISOLATED FROM CATTLE 44 Introduction 44 Materials and Methods 45 Protozoal isolates 45 Cats 45 DNA isolation and PCR 46 Inoculation 46 Collection of fecal samples and culture 47 Euthanasia and necropsy 47 Results 49 Fecal cultures 49 Intestinal cultures 49 Table 4.1 50 Table 4.2 51 Histopathological analysis 52 Discussion 52 Table 4.3 53 Figure 4.1 54 CHAPTER V. FURTHER BIOLOGICAL CHARACTERIZATION OF TRITRICHOMONAS FOETUS OF FELINE ORIGIN 57 Introduction 57 Materials and Methods 58 Sources of organisms and maintenance 58 Light microscopy 59 Scanning electron microscopy (SEM) 59 Transmission electron microscopy (TEM) 60 Molecular characterization of Tritrichomonas foetus 60 Random amplification of polymorphic DNA (RAPD) 61 Table 5.1 62 Phylogenetic analysis 63 Internal transcribed spacer regions and ribosomal RNA genes 63 RAPD analysis 63 xi Results 64 Microscopic analysis 64 Molecular Comparisons 64 Figure 5.1 65 Figure 5.2 66 Table 5.2 67 Table 5.3 68 Table 5.4 70 Figure 5.3 71 Figure 5.4 72 Figure 5.5 73 Figure 5.6 74 Discussion 75 Figure 5.7 76 CHAPTER VI. OVERALL CONCLUSIONS 80 CUMULATIVE BIBLIOGRAPHY 83 APPENDIX A. COMPLETE DATA RESULTS OBTAINED FROM VETERINARIANS PARTICIPATING IN THE SURVEY OF THE PET CAT POPULATION 90 APPENDIX B. ALIGNED SEQUENCES FOR ALL ISOLATES USED IN GENETIC COMPARISONS OF THE ITS-1, ITS-2 AND 5.8 S rRNA GENES 97 APPENDIX C. SEQUENCES OF FELINE ISOLATES REGISTERED IN GENBANK WITH CORRESPONDING ACCESSION NUMBERS 101 APPENDIX D. MATRIX RESULTING FROM RAPD PCR BANDING PATTERN ANALYSIS 105 xii LIST OF TABLES 1.1 Selected trichomonads of human and veterinary importance. 4 2.1 Signalment and treatment outcomes for cats positive for Tritrichomonas 21 foetus. 2.2 Homologous sequence identity values comparing Tritrichomonas foetus 22 isolates submitted to Auburn University College of Veterinary Medicine to published feline (AF466751) and bovine (AF339736) T. foetus sequences registered in GenBank. 3.1 Inflammatory response of Tritrichomonas foetus infection determined 38 from transcervical, uterine biopsies of endometrial tissue. 4.1 Results of the fecal sample cultures and health observations of cats over 50 the 5 week study period. 4.2 Culture results of material washed from individual sections of intestine 51 from each cat. 4.3 Histopathological analysis results of intestinal sections recovered from 53 each cat at necropsy. 5.1 Oligonucleotide primers used for amplification of random DNA markers of various trichomonads. 62 5.2 Accession numbers given to feline (AUTf) trichomonad isolates registered in GenBank. 67 5.3 Genetic sequences differences between 12 feline trichomonad isolates and the bovine (AF339736) isolate of T. foetus found in GenBank. 68 5.4 Sequence identities (%) obtained from nucleotide BLASTn analysis between the 12 feline isolates (EU569301-EU569312, respectively) and 5 other trichomonads from GenBank. 70 xiii LIST OF FIGURES 1.1 Tritrichomonas foetus morphological characteristics. 2 1.2 Muco-purulent vaginal discharge from a heifer experimentally infected with Tritrichomonas foetus. 8 1.3 Material collected from the uterus of a heifer experimentally infected with Tritrichomonas foetus. 9 2.1 Fecal scoring system used to determine consistency of stool samples acquired from surveyed cats. 19 3.1 Cumulative weekly vaginal, cervical and uterine positive cultures taken from heifers inoculated with the bovine isolate of Tritrichomonas foetus. 35 3.2 Cumulative weekly vaginal, cervical and uterine positive cultures taken from heifers inoculated with the feline isolate of Tritrichomonas foetus. 36 3.3 Transcervical uterine biopsy samples from three heifers taken six weeks PI. 40 4.1 Tissue samples taken at necropsy from the intestine of cats infected with 54 Tritrichomonas foetus. 5.1 Photomicrographs taken of the feline AUTf-1 isolate of Tritrichomonas 65 foetus. 5.2 Transmission electron micrographs (TEM) taken of the feline AUTf-1 66 isolate of Tritrichomonas foetus. 5.3 Phylogenetic tree depicting genetic sequence comparisons of the 5.8SrRNA gene and ITS-1 and ITS-2 regions between AUTf sequences and published GenBank sequences. 71 5.4 Phylogenetic tree depicting genetic sequence comparisons of the ITS-2 region between AUTf sequences and published GenBank sequences. 72 5.5 Phylogenetic tree depicting genetic sequence comparisons of the ITS-1 region between AUTf sequences and published GenBank sequences. 73 xiv 5.6 RAPD PCR results using 9 oligonucleotide 12-mer primers to compare genetic sequence banding patterns between AUTf feline trichomonad isolates and other trichomonad isolates. 74 5.7 Phylogenetic tree depicting genetic sequence comparisons of the RAPD PCR results between AUTf sequences and published GenBank sequences. 76 1 CHAPTER I. LITERATURE REVIEW: TRITRICHOMONAS FOETUS AND TRICHOMONIASIS The Trichomonads The trichomonads are anaerobic protozoan parasites placed in the phylum Parabasalia, order Trichomonadida and family Trichomonadidae (Brugerolle and Lee, 2000). A new rank system classifies trichomonads as [Excavata: Parabasalia: Trichomonadida] (Adl, et al., 2005). They are comprised of a unique complement and arrangement of organelles and intricate cytoskeletal features (Figure 1.1). Trichomonads have a single nucleus located at the anterior end of the cell body, which is pyriform, or pear shaped. They replicate via binary longitudinal fission, undergoing closed mitosis in which there is no breakdown of the nuclear envelope; the spindle is extranuclear. The Golgi apparatus is quite large, and does not divide during replication. The cytoskeleton includes an axostyle, pelta and costa. The axostyle, comprised of microtubules, supports the cell body, and extends beyond the length of the cell. The pelta serves as the originating point and supportive structure for the flagella. The flagella include three to five anterior flagella, and often a posterior recurrent flagellum, each emerging from basal bodies composed of nine microtubule triplets. The basal bodies are made up of contractile centrin fibers, allowing internalization of flagella during formation of the pseudocyst. The costa is a structure unique to trichomonads, and supports the posterior 2 Figure 1.1. Tritrichomonas foetus morphological characteristics. External features and internal organelles include anterior flagella (AF), posterior recurrent flagellum (PF), axostyle (AX), costa (C), hydrogenosomes (H), undulating membrane (UM), nucleus (N) and pelta (PL). Note sketch is not to scale. AF PF AX C H UM N PL 3 recurrent flagellum and the resulting undulating membrane which extends one-half to three-fourths the length of the cell body. Trichomonads do not have traditional mitochondria, and rely on spherical organelles known as hydrogenosomes to synthesize ATP (Honigberg, 1963, Roberts and Janovy, 2000, Benchimol, 2004). There are several genera and species of trichomonads affecting humans and animals (Table 1.1). The trichomonad most commonly encountered in veterinary medicine is Tritrichomonas foetus. The cytoskeleton and internal organelles of T. foetus are similar to other trichomonads; however this genus has three anterior flagella, a recurrent flagellum that extends from an undulating membrane three-fourths the length of the cell body. Additionally, the axostyle continues beyond the posterior end of the cell body. The approximate size of T. foetus is 10?m x 6?m (Kofoid, 1920, Wenrich and Emmerson, 1933, BonDurant and Honigberg, 1994, Benchimol, 2004). Tritrichomonas foetus is the causative agent of venereal trichomoniasis in cattle, documented on six continents (Morgan, 1947) and intestinal trichomoniasis in cats (Kessel, 1928, Jordan, 1956, BonDurant and Honigberg, 1994, BonDurant, 1997, Gookin, et al., 1999, Levy, et al., 2003). There has also been a report of T. foetus causing diarrhea in dogs (Gookin, et al., 2005) and a questionable report of human infection (Okamoto, et al., 1998). Recently, attempts were made to synonymize Tritrichomonas suis, a commensal trichomonad that infects the stomach, colon and nasal passages of swine, with T. foetus after molecular analysis of shared genetic sequences and detailed comparisons of morphological characteristics (Tachezy, et al., 2002). 4 Table 1.1. Selected trichomonads of human and veterinary importance (Jordan, 1956, BonDurant and Honigberg, 1994, Honigberg and Burgess, 1994, Gookin, et al., 1999, Roberts and Janovy, 2000, Levy, et al., 2003, Gookin, et al., 2005). Trichomonad species Host Location Disease Trichomonas tenax humans oral cavity none Trichomonas vaginalis humans vagina, urethra urethritis vaginits Pentatrichomonas hominis humans intestine none dogs large intestine diarrhea Trichomonas gallinae birds upper digestive caseous tract nodules, fluid in crop Trichomonas canistomae dogs oral cavity none Trichomonas felistomae cats oral cavity none Tritrichomonas foetus cattle vagina, uterus abortion, prepuce metritis balanoposthitis swine stomach, colon none nasal pasages cats large intestine diarrhea dogs large intestine diarrhea 5 Bovine Trichomoniasis Trichomonas foetus (Riedm?ller, 1928) syn. Trichomonas spp. reported by Kunstler (1888) syn. Trichomonas utero-vaginalis vitulae reported by Mazzanti (1900) was first described in cows and aborted fetuses in Europe, however pathogenicity was not fully realized until the research of Riedm?ller between 1928 and 1933 (Morgan, 1944, Laing, 1956). Kunstler described Trichomonas in the vagina of a cow and intestine of a pig, while Mazzanti found trichomonads in the reproductive tract of sterile cows in a slaughterhouse and described a uterus containing ?fluid resembling sour milk?. Riedm?ller (1928) later published results describing aborted bovine fetuses containing trichomonads. In 1929, Abelein demonstrated evidence that Trichomonas foetus had the ability to cause reproductive disease in cattle (Morgan, 1944). Infection with T. foetus results in venereal disease in cattle; trichomonads are found in the reproductive tract of the cow and prepucial cavity of the bull. A T. foetus infection may result in infertility, abortions and pyometra in the cow, as well as vaginitis, cervicitis, endometritis and salpingitis (Laing, 1956, Parsonson, et al., 1976, BonDurant, 1997, Felleisen, 1999). Infected bulls are usually mature, greater than three to four years of age, and are commonly asymptomatic (BonDurant, et al., 1990, Rae, et al., 1999). However, inflammation of the prepuce and glans penis (balanoposthitis) can occur since trichomonads are found in smegma within the crypts of the penile midshaft and caudal regions, and prepucial cavity of infected bulls, (Laing, 1956, Parsonson, et al., 1976, BonDurant, 1997, Felleisen, 1999, Rae, et al., 1999, Rhyan, et al., 1999). The abortions are usually early in the pregnancy, but can be midterm or late-term, and it is unclear how they occur (BonDurant, 1997). Hypotheses include (1) the 6 possibility of large organism numbers in the maternal uterus, (2) surface antigens released from the trichomonad that bind to neighboring host cells, triggering opsonization and phagocytosis or antibody-dependent cell cytotoxicity (ADCC), (3) adherence to either the fetus or maternal endometrium resulting in severe cytotoxicity previously thought to not exist, and (4) trichomonad enzymes may affect surface proteins of host cells that provide communication between the fetus and maternal endometrium (BonDurant, 1997). Trichomonads have been found in the chorionic stroma of the placentas of aborted fetuses, in addition to the alveoli and bronchioles (Rhyan, et al., 1988). Trichomonads are lumen-dwellers, actually adhering to vaginal epithelial cells (Corbeil, et al., 1989) and in order to enter the fetus they would have to cross one or more membranes. It is believed that the trichomonads are caught up in the amniotic fluid and amniotic sac during development. The fetus then ingests this fluid, allowing the trichomonads to enter areas such as the fetal stomach, intestine and lung, but the trichomonads would still have to penetrate the chorion (BonDurant, 1997). In vitro research using bovine oocytes, zygotes and embryos in the presence of T. foetus showed no effect on mobility or function of spermatozoa. Fertilization and embryonic development still occurred and there were no significant differences in the number or percentage of hatched embryos when compared to T. foetus-free controls (Bielanski, et al., 2004). These conclusions are supported by previous work in which virgin heifers were mated with infected bulls. This resulted in a 61% pregnancy rate, with two heifers demonstrating signs of future abortion when examined at necropsy 60 and 95 days after mating (Parsonson, et al., 1976). 7 However recent in vitro studies indicate that T. foetus severely damages and infiltrates the zona pellucida, reaches the oocyte and induce apoptosis (Benchimol, et al., 2007). Many cattle infected with T. foetus, both bulls and cows, may be asymptomatic. Sometimes the most prominent symptom is low fertility rates or an increase in aborted fetuses. However, T. foetus can be diagnosed using samples from a bull, cow or even a freshly aborted fetus. Diagnosis involving bulls is accomplished by a prepucial scraping, allowing any parasites collected to proliferate at room temperature in a culture media such as the InPouch TF? culture system (Biomed Diagnostics, White City, OR) or trypticase-yeast-maltose (TYM) Diamond?s medium (Diamond, 1983). After a period of 1-3 days, flagellates, if present in the original sample, will be visible under a microscope. When diagnosing trichomoniasis in cows there is usually a muco-purulent vaginal discharge which can be collected and examined for flagellates (Figure 1.2). Since trichomoniasis can also cause pyometra, the uterine discharge can also be used (Figure 1.3). Lastly, in instances where infection has spread throughout a herd and there are an increased number of aborted fetuses, necropsy of a fresh fetus can aid in diagnosis of this disease (BonDurant, 1997). Observing flagellates under the microscope will allow a morphological assessment. Once the organisms are cultured, T. foetus DNA can be extracted and a PCR assay can be performed to verify the cause of the infection (Grahn, et al., 2005). There is no approved treatment for T. foetus in cattle. Some have suggested that imidazoles can be used; however, they are not FDA approved compounds. The best treatment is prevention through artificial insemination and herd management (Laing, 1956, BonDurant, 1997). The use of virgin bulls, maiden cows or the acquisition of 8 Figure 1.2. Muco-purulent vaginal discharge from a heifer experimentally infected with Tritrichomonas foetus. The vaginal discharge can be collected and used for diagnosis of venereal trichomoniasis. Detection of trichomonads can be accomplished by direct smear or culture and viewing organisms using light microscopy at 100X magnification. 9 Figure 1.3. Material collected from the uterus of a heifer experimentally infected with Tritrichomonas foetus. The vial on the right is the uterine contents of a negative control heifer, not infected with T. foetus. The vial on the left is the uterine contents of a heifer infected with T. foetus. The uterine material can be collected and used for diagnosis of venereal trichomoniasis. Detection of trichomonads can be accomplished by direct smear or culture and viewing organisms using light microscopy at 100X magnification. 10 pregnant cows can reduce the prevalence of infection (Laing, 1956). It is also important to keep herds confined as much as possible (BonDurant, 1997). A vaccine has been introduced for use in heifers (Trich Guard? V5L, Fort Dodge Laboratories, Overland Park, KS). It contains killed T. foetus, Campylobacter and Leptospira cells (BonDurant, 1997), and while it is not a cure for bovine trichomoniasis, studies indicate that it may shorten the duration of infection and decrease the severity of the disease (Kvasnicka, et al., 1999) . Many infected bulls are lifelong carriers of the parasite, while cows may clear the infection after a few months (Skirrow and BonDurant, 1990a, Felleisen, et al., 1998). Once infected with T. foetus, cows develop a strong humoral immune response. After seven to nine weeks post-infection, research has shown that IgA and IgG1 levels increase in vaginal, cervical and uterine secretions (Skirrow and BonDurant, 1990b). Transient IgM responses were also detected, mainly in cervical secretions. Transient IgG2 responses were detected throughout the reproductive tract during later stages of the infection (Skirrow and BonDurant, 1990b). Research has also shown that trichomoniasis in bulls induces a humoral response. As with infected cows, the primary antibodies detected in the serum, smegma and prepucial washings of infected bulls were IgA, IgG1, IgG2 and IgM (Campero, et al., 1990, Rhyan, et al., 1999). Chronic infections in bulls are believed to result from larger trichomonad populations in the smegma verses those adhering to the surface epithelium of the penis which can be readily accessed by antibodies (Campero, et al., 1990). It is estimated that the beef industry in the United States loses millions of dollars each year due to trichomoniasis (Fitzgerald, et al., 1958, Wilson, et al., 1979). In one 11 epidemiological simulation model of disease dynamics in T. foetus infected herds, calf revenues decreased 4-10% due to lower calf numbers and weaning weights. Additionally, cow revenues decreased 5-35% when compared to uninfected herds (Rae, 1989). Infection by T. foetus is predominantly found in the western United States due to large, free-roaming herds that are allowed to mate freely (BonDurant, 1997). However, studies have shown a mean prevalence of T. foetus infection in approximately 11.9% of bulls on beef cattle ranches in central Florida, with a prevalence of 35.9% in one of eleven ranch units (Rae, et al., 1999). Feline Trichomoniasis Trichomonas felis was the name given to trichomonads recovered from a South American cat in 1922 by Da Cunha and Muniz (Kessel, 1928). In 1926, Tanabe referred to these trichomonads as Pentatrichomonas felis since they were found in both dogs and cats (Kessel, 1928). There was debate regarding the number of anterior flagella, and appeared to be mixed populations of trichomonads with three, four or five anterior flagella (Kessel, 1928). Differences in the numbers of anterior flagella were attributed to either the loss of extra flagella, adherence to debris or obscuring of flagella by the cell body. In 1956, Jordan published the first case report documenting Trichomonas spp. as a possible cause of diarrhea in cats. The cat in this case suffered from chronic diarrhea containing blood and mucus, anorexia, weight loss and lethargy. The cat died within days of admission. Years later, there were reports of Pentatrichomonas hominis infecting kittens and young cats. These cats presented with similar symptoms including 12 malodorous mucoid diarrhea and frequent defecation outside the litter box, lethargy and dyschezia (Romatowski, 1996, 2000). It was later suggested that Tritrichomonas foetus was the causative agent of chronic diarrhea in cats, and not P. hominis (Levy, et al., 2003). Light microscopy confirmed the presence of three anterior flagella and rRNA genes from both T. foetus and P. hominis were compared and found to be dissimilar. The results indicating that T. foetus was the causative agent of chronic diarrhea in cats led to further investigative studies. Results of research indicated that cats infected with T. foetus suffered from large-bowel diarrhea that was pasty, malodorous and usually associated with blood or mucus. Incontinence, flatulence and tenesmus were also common symptoms (Gookin, et al., 1999). The diarrhea persisted from two days to three years. The average age of diagnosis was nine months, with the majority less than one year. There also appeared to be no differences in susceptibility between males or females, or pure or mixed breed cats (Gookin, et al., 1999). Additional studies found that diarrhea usually resolved within two years, but relapses were common (Foster, et al., 2004). A prevalence survey of 117 cats representing 89 catteries at an international cat show found that 31% (36/117 cats and 28/89 catteries) were positive for T. foetus infection (Gookin, et al., 2004). Many of the positive cats were from multi-cat households however the exact route of transmission remains unknown. The majority of positive samples were confirmed by polymerase chain reaction (PCR) of fecal specimens utilizing primers specific for rRNA (Gookin, et al., 2002, Gookin, et al., 2004). Additional methods used for T. foetus detection include identification of motile trophozoites by direct examination of fresh feces, culture using TYM Diamond?s medium 13 and the InPouch TF? culture system (Biomed Diagnostics, White City, OR) (Diamond, 1983, Gookin, et al., 2003, Gookin, et al., 2004). Treatment of feline trichomoniasis is problematic and often unsuccessful. One of the initial treatments attempted was 0.5% carbarsone in a 2.5% sodium bicarbonate solution (Jordan, 1956). In this case trichomonads were no longer detected in feces, but hemorrhagic diarrhea developed followed, by death only days after treatment. Other attempted treatments with limited success include metronidazole alone or in combination with enrofloxacin, resulting in resolution of diarrhea and trichomonads only to be followed by relapse (Romatowski, 1996, 2000). Treatment with fenbendazole, furazolidone and metronidazole was found to control bacterial growth in the colon however trichomonads remained detectable in feces (Gookin, et al., 1999). Treatments which utilized prescription diets or home remedies including plain turkey and rice were unsuccessful. Supplements including yogurt, slippery elm, pumpkin, or glutamine, frequent bathing and litter box changes also did not resolve diarrhea (Foster, et al., 2004). Some treatment regimes have demonstrated efficacy against feline trichomoniasis. Metronidazole, fenbendazole and enrofloxacin used in combination has been shown to resolve diarrhea and trichomonad infection in several cases without relapse (Stockdale, et al., 2006). Ronidazole has shown greater efficacy than metronidazole for treatment of feline trichomoniasis, effectively eradicating trichomonads and resolving diarrhea without relapse (Gookin, et al., 2006). The results of ronidazole were dosage dependent, and cats receiving the lowest concentration of drug relapsed within 20 weeks (Gookin, et al., 2006). Tinidazole has shown some efficacy against feline trichomoniasis, decreasing detection of T. foetus in fecal samples and increasing resistance to later infections in 14 experimentally infected cats. However, tinidazole was not able to eradicate T. foetus infections in all cats (Gookin, et al., 2007). Research Objectives There is still little known regarding T. foetus infection in cats. Is this organism identical to T. foetus found in the reproductive tract of cattle? If so, how is does it gain entry into and survive the large intestine of a cat? The reproductive tract and large intestine are two distinctly different environments and the ability to thrive in both would require unique adaptive mechanisms. In addition to extensive characterization of the trichomonads recovered from the feces of naturally infected cats, it is necessary to conduct cross-transmission studies to determine host susceptibilities using trichomonad organisms isolated from both cattle and felids. It also remains unclear whether bacteria or other flora/fauna within the large intestine contribute to the ability of T. foetus to establish infection or induce diarrhea in cats, or whether concurrent infections with other parasites or infectious agents such as feline immunodeficiency virus (FIV) or feline leukemia virus (FeLV) could enhance susceptibility to T. foetus infection. There is an additional possibility that certain breed susceptibilities to T. foetus infection exist in the feline population. Many reported clinical cases of feline trichomoniasis include Pixie-bob tails, Siamese, and Russian blue breeds (Romatowski, 1996, Felleisen, 1999, Lappin, 2000). However, infections also were reported from domestic long-hair and domestic short-hair breeds. The cases documented to date appear to represent an equal mix of males and females, as well. The objectives of this research are to first, obtain information on the occurrence of T. foetus in the pet cat population via arbitrary fecal samples obtained by practicing 15 veterinarians from client-owned cats in different geographic regions in the United States. Second, characterize the comparative infectivity and pathogenicity of bovine and feline isolates of T. foetus in virgin heifers. Third, determine the infectivity of a bovine isolate of T. foetus in cats and fourth, compare genetic and morphologic characteristics of bovine and feline isolates of T. foetus using light microscopy, electron microscopy and gene sequencing methodologies. 16 CHAPTER II. TRITRICHOMONAS FOETUS INFECTIONS IN SURVEYED PET CATS Introduction Feline trichomoniasis is a large-bowel disease in cats thought to be caused by Tritrichomonas foetus (Gookin, et al., 2001, Levy, et al., 2003, Foster, et al., 2004). Reported clinical signs of trichomoniasis may include chronic diarrhea associated with blood or mucus, flatulence, tenesmus and anal irritation (Gookin, et al., 1999, Foster, et al., 2004, Stockdale, et al., 2006). Since 1996, reports of feline trichomoniasis have increased dramatically. The increase in diagnosis is most likely due to increased awareness and improved diagnostic techniques. Tritrichomonas foetus is often misdiagnosed as Giardia spp. (Gookin, et al., 2004) or Pentatrichomonas hominis (Romatowski, 1996, 2000, Levy, et al., 2003) or underdiagnosed in an outdoor cat whose daily bowel movements are usually not observed by the owner. A prevalence study of purebred cats at an international cat show revealed that 31% of 117 surveyed cats and 89 catteries sampled were positive for T. foetus infection (Gookin, et al., 2004). However this represented only 12% of total cats and 16% of total catteries present at the cat show. Among the cats testing positive for T. foetus, only 24 had reported loose stools or diarrhea and 36 were co-infected with Giardia spp. or coccidia (5). Specific breeds for each positive cat were not given. 17 Statistics reported by the 2007-2008 National Pet Owners Survey (APPMA, 2008) indicate that there are over 90 million pet cats in American households (HSUS, 2008). These pet cats include both pure and mixed breeds living in multi- or single cat households. These cats can also harbor additional pathogens that may cause or contribute to large-bowel disease. The goal of this survey was to estimate the prevalence of T. foetus in pet cats representing three geographic regions of the United States. Additionally, the prevalence of cats concurrently infected with other pathogens will also be noted along with presence of reported clinical signs of feline trichomoniasis. Materials and Methods Study Population Cats were chosen arbitrarily by participating veterinarians who were instructed to choose cats as they were presented to the clinic and not based on presence or absence of disease however there is the possibility of inherent bias in the selection process. Selected cats presented with or without signs of trichomoniasis. The study population included male and female cats, purebred and mixed breed varieties, and comprised all age groups. Sample Collection Fresh fecal samples were taken from each cat directly from the litter box or by use of a fecal loop. Samples were added to the InPouch TF? culture system (BioMed Diagnostics, White City, OR) and shipped overnight to the Auburn University College of Veterinary Medicine. The following information was obtained from each cat when possible: age, breed, sex, geographic location, origin of acquisition by owner (i.e. shelter, stray, cattery), concurrent infections and past treatments. Veterinarians were asked to score fecal consistency using a scale of 0, 33, 66, and 100 as follows: 0=diarrhea, watery, 18 loose or possibly blood; 33= no form, loose, puddles or piles; 66= formed, soft or wet; 100= formed and hard (Purina? Fecal Scoring System for Cats, Nestl? Purina PetCare Co., St. Louis, MO) (Figure 2.1). Some positive cats were successfully treated with fenbendazole 50mg/kg PO q24h for 5 days, metronidazole 75mg PO q24h for 10 days and enrofloxacin 5mg PO q24h for 21 days, taken concurrently (Stockdale, et al., 2006), or ronidazole 30-50mg/kg PO q12h for 14 days (Gookin, et al., 2006). When possible, veterinarians were contacted for a follow-up sample after completion of the selected treatment regimen. Sample analysis Fecal specimens were examined immediately upon arrival at the Auburn University College of Veterinary Medicine. The contents of the InPouch TF? were examined by light microscopy at 100X magnification and cultured at 37?C in trypticase- yeast-maltose (TYM) media without agar (Diamond, 1983). Cultured samples were evaluated two days after incubation at 37?C for the presence of motile trophozoites. Negative cultures were kept for 10 days, and reevaluated every two days. Positive cultures were verified by polymerase chain reaction (PCR) (Grahn, et al., 2005) using DNA that was extracted from each sample (Billeter, et al., 2007). Conserved 5.8S rRNA gene sequences and internal transcribed spacer (ITS) regions were used to verify the presence of T. foetus. This PCR procedure utilized the primers TFR-3 and TFR-4 (Felleisen, et al., 1998, Grahn, et al., 2005). Amplified PCR gene sequences from each positive sample were compared against other acquired positive samples of both bovine and feline origin. 19 Figure 2.1. Fecal scoring system used to determine consistency of stool samples acquired from surveyed cats. Veterinarians were advised to use this as their evaluation guide when needed. 20 The analysis included gene sequences from feline isolates collected from naturally infected cats, (accession numbers EU569301-EU569312), and gene sequences in GenBank from trichomonads isolated from felines (accession number AF466750) (Levy, et al., 2003) and bovines (accession number AF339736) (Walker, et al., 2003). Additionally, the analysis included trichomonad DNA sequences isolated from porcine, Tritrichomonas suis (accession number AY349190) (Kleina, et al., 2004), a lizard, Anolis bartschi, Tritrichomonas nonconforma (accession number AY886845) and a tree shrew, Tupaia belangeri, Tritrichomonas mobilensis (accession number AY886842) (Cepicka, et al., 2006) Results One hundred seventy-three feline fecal samples were submitted for examination from veterinarians throughout the United States. Total samples included pure (32) and mixed breed (141) cats. Samples were received from Alabama (69), California (10), Delaware (4), Florida (2), Georgia (2), Hawaii (14), Indiana (1), Kentucky (20), Louisiana (10), Missouri (1), New Jersey (1), North Carolina (22), Ohio (2), Tennessee (13), Texas (1) and Virginia (1). Seventeen of the 173 (10%) samples were positive for T. foetus using both culture and PCR procedures (Tables 2.1 and 2.2). Positive cats were between the ages of 6 weeks and 12 years and were reported to have chronic diarrhea, with blood or mucus. Positive surveyed cats were pure (12) and mixed breed (5), male (10) and female (7). Positive pure bred cats included Siamese (1), Russian Blue (1), Bengal (1), Japanese Bobtail (1), Scottish Fold (1), Toyger (5), Himalayan-x (1) and Abyssinian (1). Several cats were infected concurrently with Giardia spp. (5), 21 T a bl e 2. 1. S i g n a l m e n t an d t r ea t m e n t o u t c o m es f o r cat s p o s i t i v e f o r Tr itr ichomonas f o etus . I s o l at e A g e S e x Br eed L o cat i o n T r ea t m e n t * Out c o m e Co n c ur r e n t I n f ect i o n 1 11 m o M S i a m es e Al a b a m a m e t , f e n , en r o c l ear ; T. f o etus cul t ur e ( - ) ri n g w o r m 2 2 y o M R u s s i a n B l ue Al a b a m a m e t , f e n , en r o T. f o etus cul t ur e ( - ) ; d i ar r h ea C r y p tos p o r idium s pp. 3 1 7 w o F B e n g al A l ab am a m e t , f e n , e n r o , ro n eut h ani z ed F I P 4 2 y o F J a pa n e s e B o bt a il No r t h C a r o lin a m e t , f e n , en r o c l ear ; T. f o e t us cul t ur e ( - ) 5 6wo M DS H Hawa i i r o n c l ear ; T. f o e t us cul t ur e ( - ) Giar dia s p p ., ri n g w o r m 6 7wo M DS H Hawa i i r o n c l ear ; T. f o e t us cul t ur e ( - ) Giar dia s p p ., ri n g w o r m 7 7wo M DS H Hawa i i r o n c l ear ; T. f o e t us cul t ur e ( - ) Giar dia s p p ., ri n g w o r m 8 12wo M Scott i s h f o l d C a l i f o r n i a r o n c l ear ; T. f o e t us cul t ur e ( - ) 9 7m o M T o y g e r C a l i f o r n i a u n kn ow n u n kn ow n 10 1. 5y o F T o y g er C a l i f o r n i a un k n o w n un k n o w n 1 1 7m o F T o y g e r C a l i f o r n i a u n kn ow n u n kn ow n 1 2 8m o M T o y g e r C a l i f o r n i a u n kn ow n u n kn ow n 13 10 m o M T o y g er T e x a s m e t , f e n , en r o , ro n u n kn ow n I s os por a s pp. 1 4 9 m o F H i m a l a y a n ? X A l a b a m a m e t , f e n , e n ro c l e a r ; T. f o e t us cul t ur e ( - ) Giar dia s pp. 15 11 m o F DS H T e nn es s ee m e t , f e n , en r o c l ear Giar dia s pp. 16 4 y o M DM H Ohi o un a b l e t o t r ea t eut h ani z ed co cci d i a 17 12 y o F Aby s s i n i a n New J e r s e y m e t , f e n , en r o un k n o w n * T r e at me n t ab b r e v iatio n s : me t = me t r o n id a z o l e , f e n = f e n b en d azo le , e n r o = e n r o f l o x ac in , r o n = r o n i d azo le ( S to c k d a le e t al ., 2 0 0 6 ; G o o k i n e t a l . , 2 006) 22 Table 2.2 Numerical breakdown of survey results collected from pet cats by participating veterinarians. Population percentage is also given. Complete results are given in Appendix A. Total cats surveyed 173 Total cats with diarrhea* 77 45% culture positive 17 10% culture negative 60 35% Total cats without diarrhea* 69 40% no information available (NIA) 27 15% culture positive 0 0% culture negative 96 55% Total pure bred cats 30 17% pure bred cross 2 culture positive 12 38% culture negative 20 62% Total mixed breed cats 141 82% culture positive 5 4% culture negative 136 96% Total culture positive cats with concurrent infection 9 53% Giardia 5 Cryptosporidium 1 coccidia 2 ringworm 4 FIP 1 without concurrent infection 7 41% Age range culture positive cats 6 weeks old ? 12 years old Age range culture negative cats 4 weeks old ? 13 years old *If only the fecal scoring system was used in stool evaluation, out of 0, 33, 66 or 100, 0-33 was considered diarrhea; 66-100 was considered normal stool (Figure 2.1). 23 Cryptosporidium spp. (1), coccidia (2) or dermatophytes (4) or also diagnosed with Feline Infectious Peritonitis (FIP) (1) (Tables 2.1 and 2.2). Sixty surveyed cats were culture negative and reported to have diarrhea. The remaining 96 surveyed cats that were culture negative had no reports of diarrhea (69) or no information was given (27). Negative cats were between the ages of 4 weeks and 13 years old, representing both pure (20) and mixed (136) breeds (Table 2.2). Negative pure bred cats included Himalayan (2), Himalayan-x (1), Ragdoll (1), Persian (7), Siamese (2), Toyger (3), Scottish Fold (3) and Bengal (2). Negative surveyed cats were also reported to be diagnosed with diabetes (3), gingivitis (1), tapeworms (3), allergies (1), roundworm (4), upper respiratory infection (2), coccidia (7), FIV (1), Giardia spp. (3) and fleas (1) at the time of fecal collection (Appendix A). Eight of the 17 positive surveyed cats cleared the trichomonad infection concurrent with resolution of diarrhea. Four of these cats were treated with a combination of enrofloxacin (5 mg PO q24h for 21 days), metronidazole (75 mg PO q24h for 10 days) and fenbendazole (50 mg/kg PO q24h for 5 days) (Stockdale, et al., 2006), and four cats were treated with ronidazole (30-50 mg BID for 14 days) (Gookin, et al., 2006). One cat was T. foetus negative after treatment and Cryptosporidium spp. positive but did not resolve diarrhea. Two cats were euthanized, one due to an additional FIP diagnosis and one due to an inability to administer treatment. The outcome of six cats is unknown (Table 2.1). Of the 17 positive surveyed cats, genetic DNA was successfully extracted from 12 fecal samples (GenBank accession numbers EU569301-EU569312) collected at Auburn University. The PCR products amplified from conserved 5.8S rRNA, ITS-1 and ITS-2 24 genes were compared to similar known trichomonad sequences in GenBank. These comparisons showed 97-100% sequence identity between the feline trichomonad isolates collected at Auburn University and published bovine and feline T. foetus isolates (AF339736 and AF466750, respectively). Further genetic sequence analyses between these feline trichomonad isolates and various bovine, feline, porcine and reptilian trichomonads are described in detail in Chapter V. Discussion This survey revealed that 10% (17/173) of the surveyed feline pet population was positive for T. foetus. Of the 17 positive cats, 12 were pure bred and included Siamese (1), Russian Blue (1), Bengal (1), Japanese bobtail (1), Scottish fold (1), Toyger (5), Himalayan-x (1) and Abyssinian (1). This prevalence rate is lower than the prevalence rate reported by Gookin et al., 2004 at an international cat show, 31%. However, cats in the Gookin et al. study were all purebred representing only 12% of total cats and 16% of total catteries present at the cat show. Among the 36 cats testing positive for T. foetus at the international cat show, only 24 had reported loose stools or diarrhea and 14 were also co-infected with Giardia spp. or coccidia (5) (Gookin, et al., 2004). All 17 of our positive cats presented with chronic diarrhea, but not always associated with blood or mucus (Appendix A). Many of the cats surveyed by Gookin et al. were kept in densely populated catteries (1-59 cats/household) and of 89 catteries sampled, 62 reported cats with loose stool while only 28 were T. foetus positive. Another survey conducted in the United Kingdom reported 16 out of 111 cats positive for T. foetus, 14 of which were pure bred. Breeds included Siamese (6), Bengal (6), Ragdoll (1) and Persian (1) (Gunn- Moore, et al., 2007). Additionally, a survey conducted in the United States found that of 25 32 cats presenting with diarrhea, 12 were pure bred and included Abyssinian (7), Bengal (2), Persian (1), Tokinese (1) and Pixie Bob (1) (Gookin, et al., 1999). It is evident that feline trichomoniasis is not a disease of only pedigreed cats however the possibility that these cats are at greater risk has not been ruled out. The infected cats in our survey displayed some common signs of trichomoniasis, including chronic large-bowel diarrhea associated with blood or mucus, vomiting and weight loss. Concurrent infections in our surveyed cats infected with T. foetus reported by the veterinarian included Cryptosporidium spp (1), Giardia spp. (5), Isospora spp. (1), coccidia (1), dermatophytes (ringworm) (4) and FIP (1). The question still remains as to whether T. foetus is the single cause of large-bowel diarrhea in infected cats or if a concurrent infection or impaired immune system leave younger cats more vulnerable to a potentially opportunistic parasite. In our survey, of the 17 positive cats 10 had additional pathogens or disease present. Studies investigating the pathogenicity and infectivity of T. foetus in cats have observed concurrent infection or disease when T. foetus is present. In one study, 32 cats presented with diarrhea associated with blood or mucus and 8 had coexisting enteric infections. Two were diagnosed with severe or mild lymphoplasmacytic colitis, typhlitis and enteritis, additional infections included Isospora spp. (3), Toxascaris leonina (1), Giardia spp. (1) and Giardia spp. and Cryptosporidium spp. (1) (Gookin, et al., 1999). In an experimental infection study, eight cats were inoculated with a feline isolate of T. foetus (Gookin, et al., 2001). Four cats were already infected with Cryptosporidium spp. and four were specific pathogen-free (SPF). The investigators reported increased frequency and intensity of diarrhea in Cryptosporidium spp. positive cats with stool 26 samples ranging from semi-formed (score, 2) to cow-pat or liquid (score, 3 and 4). The SPF cats were reported to have stool samples ranging from formed (score, 1) to semi- formed (score, 2) and were labeled diarrhea. Comparing this fecal scoring system to the one used in our survey, samples that were formed (score, 100) to semi-formed (score, 66) were considered normal since stress or small dietary changes could cause softer stool, while samples that were cow-pat (score, 33) to liquid (score, 0) were considered to be diarrhea. Differences in stool consistency can differ between individuals? opinions or between score systems utilized in the experiments. With this in mind, the experimental infection of SPF cats with T. foetus demonstrated disease that was significantly less severe than that exhibited by cats concurrently infected with Cryptosporidium. According to our scoring system, SPF cats exhibiting semi-formed stools would have been considered normal. The authors report no increase in Cryptosporidium oocysts shed in feces and that cats had normal stools before infection with T. foetus. Trichomonads were also recovered from feces at an earlier time point and from more cats in those concurrently infected with Cryptosporidium spp. (3 of 4 by post-inoculation day 4) than the SPF cats (2 of 4 by post-inoculation day 7). Although the authors state the addition of T. foetus did not contribute to symptoms of cryptosporidiosis, differences in experimental outcomes between the two groups suggest T. foetus alone may not be sufficient to cause chronic diarrhea with the close association of blood or mucus. Again, differences in opinion regarding fecal consistency can sway results. The average age of the infected cats in this study (12 months) was similar to the average age (9 months) of infected cats previously reported (Gookin, et al., 1999). Studies to date support that feline trichomoniasis appears to be a disease of younger cats 27 and kittens, with the rare exception of a cat older than six years (Gookin, et al., 1999, Foster, et al., 2004, Stockdale, et al., 2006). Infection with T. foetus and resulting symptoms have been shown to resolve after two years in some cats (Foster, et al., 2004). At present, there is no approved treatment for feline trichomoniasis and responses to therapies mentioned previously may vary. Many cats infected with T. foetus may resolve diarrhea only to relapse weeks or months later (Foster, et al., 2004). Consequently, elimination of the parasite is problematic for those cats that do not spontaneously recover. The method(s) of transmission of T. foetus infection in cats remains unknown. It is unclear whether it is transmitted through shared litter boxes or between queens and kittens. It also remains unclear whether T. foetus is the only pathogen causing disease in these cats or playing the role of opportunist in cats on the fringe of disease. The methodologies used in this study may leave room for inherent bias however does give limited insight into the prevalence of T. foetus in the pet cat population. 28 CHAPTER III. EXPERIMENTAL INFECTION OF CATTLE WITH A FELINE ISOLATE OF TRITRICHOMONAS FOETUS Introduction Tritrichomonas foetus is a flagellated, protozoan parasite that causes bovine trichomoniasis, a venereal disease resulting in infertility and abortion, pyometra, endometritis, vaginitis, and cervicitis in infected cows. In bovines, T. foetus inhabits the vagina, cervix, and uterus of cows and the prepucial cavity of bulls (BonDurant, 1985, 1997, Felleisen, 1999). Tritrichomonas foetus appears to be a cosmopolitan organism. Experimental data demonstrate that T. foetus infections can be sustained in mice for at least 26 wk (Hook, et al., 1995) and may be a causative agent of diarrhea in dogs (Gookin et al., 2005). There has been an attempt to synonymize T. foetus and Tritrichomonas suis, a gastrointestinal trichomonad of pigs (Tachezy et al., 2002). One case report described trichomonad organisms resembling T. foetus in the cerebral spinal fluid of a human patient that underwent a peripheral blood stem cell transplant (Okamoto et al., 1998). Numerous reports have appeared recently in the scientific literature in which a species of Tritrichomonas was reported as a cause of large bowel diarrhea in cats (Stockdale et al., 2006). Structural, morphological, and molecular data suggest the causative agent is T. foetus (Gookin et al., 2002; Levy et al., 2003; Yeager and Gookin, 2005). Cats infected with T. foetus may present with flatulence, tenesmus, and chronic 29 diarrhea that may contain blood or mucus (Gookin et al., 1999; Gookin et al., 2001; Foster et al., 2004). These cats also come from a variety of backgrounds, which may or may not include contact with cattle (Gookin et al., 1999; Gookin et al., 2004; Stockdale et al., 2006). Tritrichomonas foetus is found in the large intestine of cats, commonly along the mucosal surface of the colon; it may also be found in the ileum and cecum (Gookin et al., 2001, Yeager and Gookin, 2005). Determination of the species of Tritrichomonas responsible for diarrhea in cats may help clarify host susceptibilities and routes of transmission for parasites within this genus. This research reports the results of experimental infection of heifers with T. foetus obtained from naturally infected cats. We also attempted to infect a cohort of heifers with T. foetus obtained from naturally infected cattle to serve as a positive control. Results from this study may help support or refute the synonymy of species infecting the 2 different hosts. Materials and Methods Heifers and estrus synchronization Twenty virgin Angus heifers, ranging in age from 15- to 29-mo-old, were obtained from a reproductive herd maintained at the Auburn University College of Veterinary Medicine. These heifers were randomly divided into 2 groups of 10, and a vaginal sample was taken from each heifer and cultured to ensure no prior infection with T. foetus. The average age of heifers in the first group was 19.8 mo; heifers in this group were inoculated with a bovine isolate of T. foetus obtained from a naturally infected cow. The average age of heifers in the second group was 23 mo; heifers in this group were inoculated with a feline isolate of T. foetus obtained from a naturally infected cat. The group receiving the bovine isolate was inoculated and monitored first. After sampling 30 completion, the group receiving the feline isolate was inoculated and monitored. These were not concurrent experiments. Infections with the bovine isolate were conducted April 2006 thru September 2006, and infections with the feline isolate were conducted October 2006 thru April 2007. To improve the chances of successful infection, inoculations with T. foetus were carried out during estrus, which was synchronized among heifers in each group to mimic natural infection during coitus (Skirrow and BonDurant, 1990a, BonDurant, 1997). Estrus synchronization was achieved using an EAZI- BREED? CIDR ? (controlled vaginal drug release) insert (Pfizer, InterAg, Hamilton, New Zealand), delivering 1.38 g of progesterone over a 7-day period. At the time of progesterone device insertion, each heifer also received 2 ml (100 ?g) of Cystorelin ? (gonadorelin diacetate tetrahydrate) (Merial, Duluth, Georgia) by intramuscular injection with an 18-gauge, 40-mm needle. After 7 days, the CIDR inserts were removed and the heifers were given 5 ml (25 mg) of Lutalyse ? (dinoprost tromethamine) (Pfizer, Pharmacia & Upjohn Co., New York, New York) by intramuscular injection with an 18-gauge, 40-mm needle. Time of estrus for each heifer was determined using the HeatWatch? Estrus Detection System (CowChips, LCC, Denver, Colorado). The radio frequency transmitters for HeatWatch? were placed in nylon patches and glued to the caudal dorsal midline of each heifer on day 7 using cattle backtag cement (H.B. Fuller Company, St. Paul, Minnesota) as described in the HeatWatch? user?s manual. The system data, i.e., mounting frequency, was evaluated during the first 5 days to determine inoculation times for each heifer with T. foetus. When estrus was confirmed, 8 heifers in each group of 10 were inoculated with 10 6 T. foetus organisms of either bovine or feline origin. The 2 remaining heifers in each group 31 were used as negative controls and were inoculated with sterile, parasite-free phosphate buffered saline solution (PBSS). Organisms and inoculation A previously cloned (Skirrow and BonDurant, 1990a) bovine isolate of T. foetus (D-1) was originally cultured from a naturally infected cow. A feline isolate of T. foetus (AUTf-1) was obtained from the feces of a naturally infected cat that presented with diarrhea to the Auburn University College of Veterinary Medicine (Stockdale, et al., 2006). The feline isolate was cultured in Trypticase-Yeast Extract-Maltose Medium (TYM) without agar (Diamond, 1983). A single cell clone of the feline isolate was obtained by limiting dilution and both the feline and bovine isolates were stored in freezing media in liquid nitrogen until 1 wk prior to infection. The freezing media was made under sterile conditions using FCS, DMSO and TYM at 3:2:5, respectively. Immediately prior to inoculation, each isolate was thawed and maintained in TYM at 37? C. Isolates were washed and suspended in sterile PBSS at a concentration of 10 6 trichomonads/ml. Approximately 1 ml of this suspension was inoculated into the cranial lumen of the vagina of 8 of the 10 heifers in the group using a 52.5-cm infusion pipette equipped with a flex adaptor (Continental? Plastic Co., Delavan, Wisconsin). The 2 remaining heifers in each group were inoculated with 1 ml of sterile, parasite-free PBSS. Sampling procedures At 24 hr post-inoculation (PI), samples were taken from the cranial vagina and cervix of each heifer. One control heifer was sampled first to assure the absence of cross- infections between the heifers. The second control heifer was randomly placed among the remaining 8 infected heifers to assure trichomonads were not transmitted by our 32 sampling techniques. Vaginal mucus samples were collected from each heifer using a sterile 52.5-cm infusion pipette with a flex adaptor and 20-ml syringe. Cervical mucus samples were collected using a sterile, stainless steel ? ml French-style straw gun (Nasco, Fort Atkinson, Wisconsin) covered by a plastic French-style sheath (Nasco), further covered by a plastic 52.5-cm oversleeve sanitary chemise (Agtech, Inc., Manhattan, Kansas) to prevent contamination with vaginal contents. Cervical mucus was aspirated using a 20-ml syringe. Vaginal and cervical mucus samples were each suspended in 2-ml TYM. Vaginal and cervical mucus samples were collected daily for 7 days, and then bi-weekly for 10 wk. Beginning 1 wk PI, samples were collected from one uterine horn of each heifer once weekly for 10 wk. Prior to uterine sampling, each heifer was administered a low caudal epidural of 2% lidocaine HCl (0.5 ml/45.5 kg) (Hospira, Inc., Lake Forest, Illinois) using an 18-gauge, 35-mm needle to facilitate sample collection. Also prior to uterine sampling, the perineal region was washed 3 times with water and T-Scrub? povidone-iodine cleansing solution (Thatcher Co., Salt Lake City, Utah). A sterile 14-, 16-, 18-, or 20-F catheter was passed through the cervical canal and into the uterine horn. Uterine mucus samples were collected by flushing approximately 20 ml of sterile PBSS into and out of the uterine horn. Samples were evaluated by culture as described below. All heifers were sampled until trichomonads were no longer recovered from cultured samples. During wk 6 PI, a transcervical uterine biopsy was performed and endometrial samples were obtained from each heifer after administering low caudal epidural anesthesia as previously described. This procedure was performed using Jackson uterine 33 biopsy forceps. The endometrial biopsy samples were fixed in 10% neutral buffered formalin and processed using routine histologic techniques. Sample evaluation Vaginal and cervical samples were returned to the laboratory and maintained in TYM at 37? C for 1 wk. Uterine samples (2 ml) were resuspended in TYM and maintained at 37? C for 1 wk. All samples were examined after 2 days in culture using standard light microscopy at 100x magnification. Samples were designated as positive (+) or negative (-) based on the presence of motile T. foetus trophozoites. All samples were discarded after T. foetus was observed or after 2 consecutive negative examinations. Biopsy specimens were scored in a blinded fashion for periglandular and interstitial inflammation, the presence of an intact epithelium, and endometrial edema. Inflammation was characterized based on the presence of neutrophils, lymphocytes, plasma cells, macrophages, and eosinophils, and their distribution, along with edema, throughout the sample. Each specimen was scored using a scale of increasing severity: 1=minimal, 2=slight, 3=moderate, 4=marked, 5=severe, extensive. Surface epithelium and uterine glands were noted as present (P) or absent (A). Overall scores were calculated by taking the product of a leukocyte score and the distribution score, followed by addition of the edema score. Statistical analysis All statistical analyses were performed using SAS? Statistical Software (SAS Institute, Inc., Cary, North Carolina). Statistical test results with a P-value less than 0.05 were reported as significant. Two-sample t-tests were used to analyze total vaginal and cervical positives between each experimental group during the first wk of sampling, as 34 well as total days vaginal, cervical, and uterine positives during sampling wk 1 through 10. This test was also used to compare inflammatory scores between the 2 groups. A log-rank test, using the Lifetest procedure in SAS?, was used to analyze the time until a positive uterine sample was detected. Fisher?s exact tests, using the Freq procedure in SAS?, were used to compare the numbers of heifers of each group retaining an intact surface epithelium and the numbers of each group that had cleared the trichomonad infection by wk 19 PI. Results Trichomonads recovered from samples Motile trichomonads were detected in cultures of vaginal and cervical mucus from heifers infected with both bovine D-1 (Fig. 3.1) and feline AUTf-1 (Fig. 3.2) T. foetus isolates. We observed both vaginal and cervical positive cultures in both groups beginning from day 1 PI through day 7 PI. The mean numbers of vaginal positive and cervical positive days were 4.5 and 3.9, respectively, for heifers inoculated with the bovine isolate of T. foetus, and 4.3 and 3.0 respectively, for heifers inoculated with the feline isolate of T. foetus. These means were not statistically significantly different between the groups infected with bovine or feline T. foetus isolates with respect to the number of vaginal (P=0.587) or cervically positive (P=0.213) days during the first wk. During the remaining 10 wk of sampling, motile trichomonads were detected in cultures of vaginal and cervical mucus in 7 of 8 inoculated heifers from both groups (Figs. 3.1, 3.2). There were no statistically significant differences in the total number of vaginal days positive (P=0.3495) or cervical days positive (P=0.4313) for infected heifers 35 Figure 3.1. Cumulative weekly vaginal, cervical and uterine positive cultures taken from heifers inoculated with the bovine isolate of Tritrichomonas foetus. Sampling was performed daily during the initial week (W0) and bi-weekly for the remaining ten weeks (W1-W10). 36 Figure 3.2. Cumulative weekly vaginal, cervical and uterine positive cultures taken from heifers inoculated with the feline isolate of Tritrichomonas foetus. Sampling was performed daily during the initial week (W0) and bi-weekly for the remaining ten weeks (W1-W10). 37 between each group during the 10 sampling weeks. A thick, yellow vaginal discharge was observed in many of the infected heifers. Heifers from each group had uterine samples positive for motile trichomonads. Positive uterine samples also contained a thick, yellow muco-purulent exudate. Uterine samples were positive in 7 of 8 heifers inoculated with the bovine T. foetus isolate at 1, or more, collection points during the 10 wk sampling period (Fig. 3.1), while uterine samples were positive in 5 of 8 heifers inoculated with the feline T. foetus isolate (Fig. 3.2). There were no statistically significant differences in the number of uterine positive heifers between each group (P= 0.4980). The time until development of a uterine infection in heifers inoculated with the bovine isolate ranged from 1 wk PI to 6 wk PI, while heifers inoculated with the feline isolate ranged from 2 to 3 wk PI. There were no statistically significant differences in time required to establish a uterine infection between the 2 groups (P=0.385). The mean time to detection of positive uterine samples was 3 wk PI for both groups. Uterine biopsies Examination of endometrial biopsies revealed endometritis, with both periglandular and interstitial inflammation, in heifers from each infection group. A mixed infiltrate of inflammatory cells was present, along with varying degrees of edema and decreased glandular density. Heifers infected with the bovine T. foetus isolate demonstrated more variability in severity of endometritis than those infected with the feline T. foetus isolate with respect to periglandular (P=0.004) and interstitial inflammation (P=0.009). This was evident in calculated histologic scores of each uterine biopsy sample (Table 3.1). Overall mean histological scores for heifers infected with the 38 T a bl e 3. 1. I n f l a m m a t o r y r e s p o n s e o f Tr itr ichomon as f o etus i n f ect i o n det e r m i n ed f r o m t r an s c er vi c a l , ut er i n e bi o p s i e s o f e n do m e t r i a l t i s s ue. U t er i n e s a m p l e s wer e t a ken f r o m he i f er s i n f ect ed w i t h t h e b o vi ne i s o l at e ( D - 1 ) an d f e l i ne i s o l at e ( A UT f - 1) o f T. foe t us . Sco r es f r o m eac h h e i f er ( 1 = m i n im a l , 2=s l i g h t , 3=m o der a t e , 4=m a r k ed, 5=s e v e r e , ex t e ns i v e ; dat a n o t s h o w n ) wer e t a ken an d i n d i v i dua l l e uko c y t e s c o r es wer e cal cu l a t e d by t a k i n g t h e pr o duc t o f eac h l e uko c y t e s c o r e an d t h e di s t r i b u t i o n s c o r e g i v e n f o r each s a m p l e . I n di v i d u a l s c or e s a r e s h ow n b e l o w . T h e m a x i m u m an d m i ni m u m ov e r al l s c or e s a r e c a l c ul ate d b y ta k i n g th os e i n di vi d u a l s c o r es an d add i n g t h e ede m a s c o r e. A ( - ) den o t e s t h at s a m p l e s wer e n o t av a i l a bl e due t o i n a b i l i t y t o p e n e t r at e cer v i x . L e uko c y t e He i f er # ( D - 1 i s o l at e) He i f er # ( A UT f - 1 i s o l at e) 1 2 3 4 5 6 7 8 9 10 1 2 3 4 5 6 7 8 9 10 P erig l a n d u la r n e ut r o p h i l s 4 0 0 2 0 - 0 0 - 0 0 0 0 0 0 - 0 2 0 0 l y m p h o c y t e s 6 0 0 1 0 - 0 1 - 1 1 1 1 0 1 - 0 1 1 2 pl a s m a c e l l s 4 0 0 1 - - 0 1 - 1 1 1 1 0 2 - 0 1 1 2 m a c r o pha ge s 0 0 0 0 - - 0 0 - 0 0 0 0 0 0 - 0 0 0 0 e o s i n o p h i l s 4 0 0 0 - - 0 0 - 0 0 1 0 0 1 - 0 0 0 0 e d e m a 4 0 4 2 1 - 3 2 - 3 2 3 2 2 2 - 2 3 2 2 M a xi mu m 10 0 4 4 1 - 3 3 - 4 3 4 3 2 4 - 2 5 3 4 M i n i mu m 4 0 4 3 1 - 3 2 - 3 2 3 2 2 2 - 2 3 2 2 A v e r age 7. 6 0 4 2. 8 1 - 3 2. 4 - 3. 4 2. 4 3. 6 2. 4 2 2. 8 - 2 3. 8 2. 4 2. 8 I n t ers t i t i a l n e ut r o p h i l s 1 1 0 6 12 - 0 0 - 4 1 0 0 0 2 - 0 0 0 2 l y m p h o c y t e s 0 0 0 3 12 - 1 1 - 2 1 2 1 1 4 - 1 1 1 4 pl a s m a c e l l s 1 1 0 9 16 - 1 2 - 2 1 2 1 1 4 - 1 2 2 6 m a c r o pha ge s 0 0 0 0 0 - 0 0 - 0 0 2 0 0 2 - 0 0 0 2 e o s i n o p h i l s 1 0 0 0 4 - 0 0 - 2 0 0 0 0 4 - 1 0 0 2 e d e m a 4 0 4 2 1 - 3 2 - 3 2 3 2 2 2 - 2 3 2 2 M a xi mu m 5 1 4 11 17 - 4 4 - 7 3 5 3 3 6 - 3 5 4 8 M i n i mu m 4 0 4 2 1 - 3 2 - 3 2 3 2 2 4 - 2 3 2 4 A v e r age 4. 6 0. 4 4 5. 6 9. 8 - 3. 4 2. 6 - 5 2. 6 4. 2 2. 4 2. 4 5. 2 - 2. 6 3. 6 2. 6 5. 2 39 bovine isolate ranged from 0.0 to 7.6 for periglandular inflammation, and 0.4 to 9.8 for interstitial inflammation. In contrast, the overall mean histologic scores for heifers infected with the feline isolates ranged from 2.0 to 3.8 for periglandular inflammation, and 2.4 to 5.2 for interstitial inflammation (Table 3.1). There were no statistically significant differences in mean histologic scores between heifers infected with either isolate with respect to periglandular (P=0.731) and interstitial inflammation (P=0.40). In addition to periglandular and interstitial inflammation, presence or absence of surface epithelium was also noted. Surface columnar epithelium was intact in 7 of 8 heifers infected with the feline isolate of T. foetus (Figs. 3.3A, B), while none of 6 heifers infected with the bovine isolate of T. foetus had intact surface epithelium present (Figs. 3.3C, D) (epithelial scores were not available for 2 heifers). Epithelial scores were statistically significantly different between the 2 groups (P=0.005). Trichomonad infection clearance times were also evaluated between each group. Clearance times were based on positive or negative vaginal and cervical mucus samples. Samples were cultured weekly after the 10 wk study period was complete. Heifers were considered free of infection if 5 consecutive negative vaginal and cervical samples were observed. After 20 wk PI, trichomonads were no longer detectable in heifers infected with the bovine isolate. In contrast, trichomonads were no longer detectable in only 2 of the heifers infected with the feline isolate by 20 wk PI. There is a statistically significant difference in clearance times between each group (P=0.021). Discussion Heifers inoculated with both bovine and feline T. foetus isolates that sustained trichomonad infections had pathologic changes in the reproductive tract consistent with 40 (A) (B) (C) (D) Figure 3.3. Transcervical uterine biopsy samples from three heifers taken six weeks PI. (A) A normal uterine sample, from control heifer ID#6-feline isolate. Note the presence of the epithelial border and glands. (B) A sample from heifer ID#4, infected with the AUTf-1 feline isolate of Tritrichomonas foetus. Note the absence of the epithelial border and the presence of periglandular inflammation and edema. This is the only sample in which the epithelial border was not intact. (C) A normal uterine sample, from control heifer ID#4-bovine isolate. Note the presence of the epithelial border and glands. (D) A sample from heifer ID#5, infected with the D-1 bovine isolate of T. foetus. Note the absence of glands and epithelial border and an infiltrate of mixed inflammatory cells. 30 ?m 41 previous reports of bovine trichomoniasis (Skirrow and BonDurant, 1990a, Anderson, et al., 1996, Felleisen, 1999). Since the experiments were not concurrent, the age of each. heifer was also considered when evaluating infections. The average age of heifers inoculated with the bovine or feline T. foetus isolate was 19.8 and 23 mo, respectively Age did not appear to impact susceptibility to trichomonad infection. Biweekly mucus aspirations revealed vaginitis and cervicitis in infected heifers, and endometritis was evident from uterine washes and uterine biopsy samples. Trichomonads were recovered from vaginal and or cervical samples from heifers in both groups during the first wk of infection, beginning 24 hr PI. Previous studies resulted in similar findings (Skirrow and BonDurant, 1990a). All heifers infected with the bovine T. foetus isolate cleared the infection by wk 20, while 5 heifers infected with the feline T. foetus isolate remained culture positive at wk 20 and 3 heifers remained culture positive at wk 30. Persistence of infection with both isolates in this study remains within range of persistent infection with bovine T. foetus in previous studies (Skirrow and BonDurant, 1990a). In both groups in the present study, 7 of 8 heifers maintained trichomonad infections for the duration of the study and, while not all infected heifers developed uterine infections, there were no statistical differences between the 2 groups. Infertility and abortions due to bovine trichomoniasis can impose economic losses to cattle producers (BonDurant, 1997). Embryonic death may result from endometritis, which can potentially disrupt the implantation of the embryo due to inflammation and loss of surface epithelium. Other protozoan agents, as well as viral or bacterial pathogens may also cause abortion and infertility (Vanroose, et al., 2000). Experimental infection in the present study resulted in endometritis among heifers in both experimental groups. 42 Trichomonads were present in uterine washes and were accompanied by muco-purulent discharge and histologic evidence of inflammation. Biopsy samples of the uterine endometrium contained an influx of mixed inflammatory cells, i.e., plasma cells, macrophages, neutrophils, and eosinophils, as well as edema and loss of surface epithelium. Heifers within the group inoculated with the bovine T. foetus isolate had a significantly higher variability of inflammation than heifers within the group inoculated with the feline isolate. However, mean levels of inflammation between the 2 groups were comparable. This suggests that the trichomonads induce the same pathology, regardless of origin. A significant difference was observed between the 2 isolates regarding the presence or absence of endometrial surface epithelium. All samples from heifers infected with the bovine T. foetus isolate were devoid of an intact surface epithelial border, while only 1 of 7 samples from heifers infected with the feline isolate was without an intact surface epithelial border. Although the feline isolate is capable of inducing trichomoniasis and many of the resulting pathologic effects, the reduced ability to cause the loss of the surface epithelium may suggest different parasite-host interactions. This could represent genetic divergence, and the introduction of a parasite into a host to which it is not readily adapted. This may also suggest that infection with the feline isolate of T. foetus may not cause infertility or abortion, a potential result of endometritis that may cause the loss of surface epithelium and disruption of embryonic implantation. Tritrichomonas foetus may be a multi-host parasite capable of infecting a variety of hosts. Many livestock parasites (as many as 77% by one estimate) are indeed multi- host parasites (Haydon, et al., 2002). All hosts for T. foetus are mammalian and the site 43 of infection is the lumen of either the gastrointestinal or the reproductive tract. Tritrichomonas foetus recovered from cats may have adapted to the new host environment by exploiting the similarities of the cow?s reproductive tract and large intestine. Both are luminal environments, which require the parasite to develop a means of adherence to epithelial cells, a common characteristic of T. foetus in both cows and cats (Felleisen, 1999; Yeager and Gookin, 2005). The mechanism of T. foetus transmission between different host species remains unknown, as does the definitive routes of transmission between feline hosts. Additional cross-transmission studies, particularly attempts to transmit bovine isolates of T. foetus to cats are needed. Additional molecular comparisons are also a necessary component of future research. To date, the internal transcribed spacer region (ITS1 and ITS2) and the 5.8S and 18S rRNA genes are the standards used for genetic comparisons between the bovine and feline isolates of T. foetus (Gookin et al., 2002; Grahn et al., 2005; Levy et al., 2003). Future studies must combine genetic information, biological and structural data, along with host specificity and parasite-host interactions, to conclusively define the taxonomy of T. foetus. 44 CHAPTER IV. EXPERIMENTAL INFECTION OF CATS (FELIS CATUS) WITH TRITRICHOMONAS FOETUS ISOLATED FROM CATTLE Introduction Tritrichomonas foetus is the causative agent of bovine trichomoniasis, a disease of the reproductive tract resulting in infertility and abortions in infected cows (BonDurant, 1985, BonDurant, 1997, Felleisen, 1999). Infected bulls become chronic carriers, while infected cows may clear the infection within 2-6 months (BonDurant, 1997, Stockdale, et al., 2007). In addition, T. foetus has recently been recognized as an agent of feline large bowel disease (Foster et al., 2004; Gookin et al., 1999; Gookin et al., 2001; Levy et al., 2003). Over the past decade, the numbers of reports of T. foetus-induced large bowel diarrhea in cats has increased (Stockdale et al., 2006). Surveys of cats from the United States and other countries have demonstrated that T. foetus is found in both purebred and mixed breed cats that may or may not have been in contact with cattle (Gookin et al., 1999; Gookin et al., 2004). Clinical signs of disease in infected cats include diarrhea with mucus, lethargy, anorexia and weight loss (Gookin et al., 1999; Gookin et al., 2001; Jordan, 1956; Stockdale et al., 2006). Additional signs may include diarrhea with blood, tenesmus, flatulence and malodorous feces. Experimental infection of cats with feline- derived T. foetus has reproduced many of these signs (Gookin et al., 2001). In some reports, the diarrhea associated with trichomonad infection had been attributed to Pentatrichomonas hominis (Romatowski, 1996, 2000). However, it was later shown that 45 T. foetus was the causative agent and not P. hominis (Levy et al., 2003). Previous research has demonstrated that a feline isolate of T. foetus can successfully infect bovines. However, the resulting disease differs from that caused by a bovine isolate of T. foetus (Stockdale et al., 2007). To our knowledge, there exist no published reports of attempts to experimentally infect cats with a bovine isolate of T. foetus. In this study, we report the results of experimental infection of cats with the D-1 bovine isolate of T. foetus. Materials and Methods Protozoal Isolates Two isolates of T. foetus, a feline isolate (AUTf-1) isolated from a naturally infected cat presented to Auburn University College of Veterinary Medicine (Stockdale et al., 2006) and a bovine isolate (D-1) originally collected from a naturally infected, pyometritic cow (Skirrow and BonDurant, 1990a), were obtained and cultured in Trypticase-Yeast-Maltose (TYM) media without agar (Diamond, 1983). These isolates were kept in freezing media in liquid nitrogen until one week before use. Freezing media consisted of fetal calf serum (FCS), dimethyl sulfoxide (DMSO) and TYM media at 3:2:5, respectively. The isolates were then thawed and subcultured in TYM media at 37?C. Cats Eight domestic shorthair cats, 6 females and 2 males, ranging in age from 8-12 months, were obtained from the Scott-Ritchey Research Center, Auburn University College of Veterinary Medicine. Fecal samples were collected from each cat to verify the absence of T. foetus by culture and polymerase chain reaction (PCR) (Grahn et al., 46 2005). Cats were housed in the same room in separate stainless steel cages. Lighting and temperature were automatically controlled and daily care and maintenance was provided by the Division of Laboratory Animal Health, Auburn University College of Veterinary Medicine. The cats were acclimated to the cages and environment for 10 days prior to experimental infection. DNA isolation and PCR Tritrichomonas foetus DNA was isolated from fecal samples by first washing the feces 3 times with Tris-EDTA (TE) buffer (1mM EDTA, 10mM Tris, pH 8.0). After the final wash, the pellet was resuspended in 100?L TE and DNA extraction for PCR analysis was carried out as described in Billeter, et al., 2007. The PCR protocol, with modifications, described in Grahn, et al., 2005 was used to identify T. foetus from culture and fecal samples by amplifying the internal transcribed spacer 1 (ITS1) region. Modifications included 1mM 10X PCR buffer II, 1mM MgCl 2 , 0.2mM dNTP and 0.05 U Taq DNA polymerase (Invitrogen, Carlsbad, CA, USA). Additionally, the annealing temperature was decreased to 56 ?C for 30 s. Inoculation Cats were fasted for twenty-four hours prior to inoculation. For experimental infection, cats were sedated using a mixture of medetomidine hydrochloride (Domitor?, Pfizer Animal Health, Exton, PA, USA) (68mg/ml), butorphanol tartrate (Torbugesic?, Fort Dodge, KS, USA) (1.8mg/ml) and ketamine (Ketaset?, Fort Dodge) (0.14mg/ml) at a rate of 0.075ml/kg. The AUTf-1 and D-1 isolates were washed and resuspended in antibiotic-free, fetal bovine serum-free TYM media without agar approximately one hour prior to inoculation. Six cats received 1.5 X 10 6 trichomonads (D-1 isolate) in 10 ml of 47 antibiotic-free, fetal bovine serum-free TYM media without agar via orogastric intubation. One cat was inoculated with 1.5 X 10 6 trichomonads (AUTf-1 isolate) in similar media. One cat was inoculated with media only. Cats were allowed to recover naturally. Collection of fecal samples and culture Fecal samples were collected from each cat three times a week for five weeks. Samples were obtained per rectum using a plastic loop or from a freshly voided sample in the litter box. Each sample was immediately suspended in 2ml of TYM media and incubated at 37? C. In addition to sample collection, fecal consistency was noted using a scale of 1-4 (1=diarrhea, watery, loose or possibly blood; 2= no form, loose, puddles or piles; 3= formed, soft or wet; 4= formed and hard) (Purina? Fecal Scoring System for Cats, Nestl? Purina PetCare Co., St. Louis, MO, USA). Emesis or other signs were also noted. All samples were examined at 100X magnification after two days in culture. Samples were scored as positive (+) or negative (-) based on the presence of motile T. foetus trophozoites, and were verified using PCR (Grahn et al., 2005). Negative samples were held for 10 days and rechecked every two days. Euthanasia and necropsy At five weeks PI, all cats were sedated as described above. Following sedation, the cats were euthanized by intravenous administration of sodium pentobarbital (Euthasol?, Delmarva Laboratories, Midlothian, VA, USA) at the dose of 17.7mg/kg. At necropsy, the ileum, cecum and colon were removed as one section. The anterior ileum and posterior colon were ligated with cotton twine. Ligatures were also placed at the posterior ileum, base of the cecum and the anterior colon. The colon was then 48 sub-divided into three equal sections using two additional ligatures. This yielded a total of five separate sections of bowel: terminal ileum, cecum, anterior, medial and posterior colon. Approximately 2-5ml of TYM media was injected into each section using a sterile 18-guage needle and 10ml syringe. The sections were then incised and the contents of each section were collected into a separate specimen cup. Approximately 1ml of contents from each section of intestine was resuspended in 5ml of TYM media and incubated at 37? C. Samples were examined as previously described for visible trophozoites and verified using PCR procedures (Grahn et al., 2005). Tissues for histopathologic examination were fixed in 10% buffered formalin. Following fixation, the intestinal segments were trimmed and sections of ileum, cecum, and three sections of colon (proximal, middle and distal) submitted for routine paraffin embedding and tissue sectioning. Five micron sections of tissue from these five locations were cut with a microtome, affixed to glass slides and stained with hematoxylin and eosin stain. Inflammation in the lamina propria of the ileum, cecum and colon was subjectively evaluated, in a blinded fashion, with light microscopic examination of tissue sections stained with hematoxylin and eosin. A grading scale of 0 -3 was followed with 0 being no to few lymphocytes and plasma cells present and 3 being moderate to large numbers of lymphocytes and plasma cells present. The size of Peyer?s patches was also evaluated. Additionally, other histopathologic lesions including crypt abscesses and the amount of mucus present were evaluated and assigned lesion scores. 49 Results Fecal cultures Motile trichomonads were successfully observed in cultures from three fecal samples obtained from the positive control cat (cat no.7), inoculated with the feline (AUTf-1) isolate, beginning day 16 post-inoculation (PI) (Table 4.1). Of the six cats inoculated with the bovine (D-1) isolate, only one cat (cat no.2) was culture positive on day 32 PI (Table 4.1). The remaining five cats inoculated with the bovine (D-1) isolate remained culture negative throughout the study. Neither of the two cats (no.2 bovine [D- 1] isolate and no.7 feline [AUTf-1] isolate) that were culture positive developed diarrhea or demonstrable vomiting, loss of appetite or fever during the study. On day 9 PI, one cat (cat no.5) inoculated with the bovine (D-1) isolate had soft stool with small amounts or blood and mucus, and cat no.4 had episodes of vomiting and a fever of 102.8 F on day 21 PI (Table 4.1), but neither cat was culture positive for T. foetus. Intestinal cultures Motile trichomonads were successfully observed in cultures from the intestinal contents of both fecal culture positive cats (see above) (Table 4.2). Cat no.2, bovine (D- 1) isolate, was culture positive in the cecum. Cat no.7, feline (AUTf-1) isolate, was culture positive in the ileum, cecum, medial colon and posterior colon (Table 4.2). Additionally, cat no.4 bovine (D-1) isolate was culture positive in the cecum. Cat no.8, (media only), was culture positive in the ileum. However this was an erroneous result due to improper labeling of tubes during subculture. That a negative diagnosis was appropriate for this culture is supported by the fact that PCR results in all samples 50 Table 4.1. Results of the fecal sample cultures and health observations of cats over the 5 week study period. Cats were inoculated with either the bovine D-1 isolate (nos. 1-6) or feline AUTf-1 isolate (no. 7) of Tritrichomonas foetus. One cat (no. 8) was not inoculated with trichomonads (media only) and used as a negative control. Over the five week period, 15 samples were taken from each cat, beginning post-inoculation (PI) day 2 (2d). All cats had fecal scores ranging from 3-4 (formed and either soft and wet or hard) unless otherwise noted. Cat ID Isolate No. Positive Fecal Cultures/ Signs of Disease Total No. Samples 1 D-1 0/15 none 2 D-1 PI 32d*; 1/15 none 3 D-1 0/15 none 4 D-1 0/15 PI 21d; fever (102.8 F) vomiting 5 D-1 0/15 PI 9d, blood and mucus in loose stool; fecal score = 1 6 D-1 0/15 none 7 AUTf-1 PI 16d*; 3/15 none 8 Media only 0/15 none * day of first positive culture sample 51 T a bl e 4. 2. Cu l t ur e r e s u l t s o f m a t e r i a l wa s h ed f r o m i n d i v i dua l s e ct i o ns o f i n t e s t i n e f r o m ea c h cat . A ( - ) i n d i cat es an i n t e s t i na l s ect i o n t h at was cul t ur e n e gat i v e f o r t h e pr es en ce o f Tr itr ichomonas f o etus , an d a ( + ) i n d i c a t e s an i n t e s t i n a l s ect i o n t h at was cul t ur e p o s i t i ve f o r t h e pr es en ce o f T. f o e t us . C o nc e n t r a t i o ns o f T. f o e t us r eco v e r e d f r o m cu l t ur e s a m p l e s o f eac h i n t e s t i n a l s e ct i o n a r e lis t e d in p a r e nt he s i s a s t r i c ho m o na d s / m l. C a t I D n o . In t e st i n a l se c t i o n 1 2 3 4 5 6 7 8 i l e u m - - - - - - + (1 .7 3 x 1 0 5 ) + * cecum - + ( 1 . 75x 10 4 ) - + ( 2 . 75x 10 4 ) - - + (3 .1 5 x 1 0 6 ) - a n t e ri o r c o l o n - - - - - - - - m e d i a l c o l o n - - - - - - + (2 .5 x 1 0 3 ) - p o s t e r i o r c o l o n - - - - - - + (5 .0 x 1 0 3 ) - * co n t am i n at i o n due t o m i s l a be l e d t u b e s dur i n g s u b c u l t u r e , n e gat i v e r e s u l t co nf i r m e d by PC R 52 obtained from the original specimen cups at necropsy, and from weekly fecal samples obtained throughout the study, were negative. Histopathologic analysis Tissue samples were obtained and scored as described above from each intestinal section (Table 4.3). All intestinal samples taken from the cat inoculated with the feline (AUTf-1) isolate showed an increase of lymphocytes and plasma cells in the mucosa, which appeared to be migrating from moderately hyperplastic Peyer?s patches (Figure 4.1A). Often grade 3 sections also contained aggregates of lymphocytes and plasma cells in addition to those lymphocytes and plasma cells scattered throughout the proprial tissue. There was also an increase in the presence of crypt abscesses and mucus production. All samples taken from cats inoculated with the bovine (D-1) isolate demonstrated similar lesions (Figure 4.1B). Each cat had some level of lymphocyte and plasma cell infiltration in the sections of intestinal mucosa, although some were more pronounced than others (Table 4.3). Samples collected from the non-infected control cat displayed similar levels of lymphocytes and plasma cells however Peyer?s patches and surrounding mucosa appeared normal (Figure 4.1C). Discussion Results of this study suggest that differences exist in both infectivity and pathogenicity for feline (AUTf-1) and bovine (D-1) isolates in experimentally infected cats. These results are similar to those of our previous study in which heifers infected with the AUTf-1 isolate of T. foetus demonstrated temporal differences in infection and severity of disease when compared to heifers infected with a bovine (D-1) isolate of T. foetus (Stockdale et al., 2007). Of the 6 cats inoculated with the bovine (D-1) isolate, 53 Table 4.3. Histopathological analysis results of intestinal sections recovered from each cat at necropsy. Intestinal sections were stained with hematoxylin and eosin and the presence of lymphocytes and inflammatory cells were scored on a scale of increasing severity (1=minimal, slight, 2=moderate, 3=severe, marked). Individual scores for each intestinal section recovered from each cat are shown along with overall mean scores. bovine D-1 isolate ileum cecum anterior colon medial colon posterior colon mean score 1 2 3+ 2+ 3+ 2+ 2.4 2 1-2 1 1-2+ 2+ 2+ 1.6 3 2 2+ 2+ 1 2+ 1.8 4 2 1+ 1 1 1-2+ 1.3 5 1 2+ 2 2+ 2-3 1.9 6 1-2 1+ 1+ 2-3+ 3+ 1.8 feline AUTf-1 isolate 1 1-2 2+ 2+ 3+ 2-3+ 2.4 media only 1 2 2 2+ 2+ 3+ 2.2 54 (A ) (B ) (C ) F i gur e 4. 1. T i s s u e s a m p l e s t a ken at n ecr o p s y f r o m t h e i n t e s t i n e o f cat s i n f ect ed w i t h Tr itr ichomona s f o etus . T h e f e l i ne i s o l at e, A U T f - 1 ( A ) , t h e b o vi ne i s o l at e, D- 1 ( B ) an d t h e n o n - i n f e ct ed c o n t r o l ( C ) . I m age s ar e t a ken at 100 X m a g n i f i cat i o n . 55 only 1 was positive by fecal culture during the 5 week study. This occurred on the last day of sampling. The cat inoculated with the feline (AUTf-1) isolate was positive by fecal culture at 15 days PI. PCR results supported that negative fecal cultures were truly negative and not the result of too few organisms to culture successfully. Positive fecal cultures were also positive by PCR, supporting the sensitivity of the fecal culture method (Gookin et al., 1999; Gookin et al., 2003; Gookin et al., 2004; Grahn et al., 2005). Similar results were obtained from culture samples from intestinal contents of the ileum, cecum and colon of each cat at necropsy. The cat inoculated with the feline (AUTf-1) isolate was again culture positive in the ileum, cecum, medial and distal colon. Of the 6 cats inoculated with the D-1 isolate, a single cat that was fecal culture positive was also positive when cecal contents were collected. One additional cat was culture positive when cecal contents were collected but was negative based on fecal culture. These results were again verified using PCR (Grahn et al., 2005). It is possible that trichomonads are passed in feces intermittently or in low numbers only during episodes of diarrhea. Consequently, in situ sampling techniques would likely be more sensitive than fecal culture techniques. The use of PCR procedures for detection of trichomonads in organ contents or in feces would be expected to be more sensitive than culture, only requiring a minute amount of DNA and able to easily distinguish between different trichomonads easily {Grahn et al., 2005). This is important when trichomonad populations are low or a mixed infection is suspected. Interpretation of histologic changes in the colon can be difficult. Lymphocytes and plasma cells normally respond to antigens within the colonic lumen. Wide variation in numbers of lymphocytes and plasma cells is common place and can even be 56 interpreted as a normal response to the ever changing enteric microenvironment (Wilcock, 1992). Analysis of histopathologic changes in each feline intestinal section revealed aggregates of lymphocytes and plasma cells of approximately equal frequency and intensity in both treatment groups. Based on prior research (Yeager and Gookin, 2005), the experimental infection results suggest that longer infection times may be necessary to show demonstrably different pathogenic events in cats. These cats were not specific pathogen-free animals and the pathologic changes observed in the intestinal mucosa could be in response to any intraluminal antigen such as food antigens or antigens from one or several of the many species of bacteria and other microorganisms living in the colonic contents. The results of this study together with the results of our previous research in bovines suggest that there are differences in biological or pathogenic behavior of the feline and bovine isolates that cannot be ignored. The two studies provide compelling evidence that fundamental differences exist between the different isolates of T. foetus. In the opinion of the authors, these differences exceed what one would expect to observe in normal intra-specific variation. 57 CHAPTER V. FURTHER BIOLOGICAL CHARACTERIZATION OF TRITRICHOMONAS FOETUS OF FELINE ORIGIN Introduction Tritrichomonas foetus was originally described in Europe and is the causative agent of venereal trichomoniasis in cattle. Clinical signs in cows include vaginitis, cervicitis, pyometra, and endometritis. Infertility and early to mid-term abortions can also result from T. foetus infection. In bulls, inflammation of the prepuce and glans penis (balanoposthitis) can occur however infected bulls are often asymptomatic (BonDurant, 1985, BonDurant, 1997, Felleisen, 1999). The first report of trichomoniasis in cats in the early 1900s described nine kittens infected with trichomonads detected in diarrheic stool (Kessel, 1928). Clinical signs included yellow-brown diarrhea with or without blood. Years later, trichomoniasis was reported in a young cat brought to a veterinary clinic displaying similar clinical signs (Jordan, 1956). The reported symptoms of feline trichomoniasis include chronic, malodorous large-bowel diarrhea, that may contain blood or mucus, flatulence, tenesmus, and fecal incontinence leading to soiling outside the litter box (Gookin, et al., 1999, Foster, et al., 2004). Over the past decade, there have been increasing reports of clinical feline trichomoniasis (Gookin, et al., 1999, Gookin, et al., 2004, Stockdale, et al., 2006). 58 Published comparisons of the genomic sequences of two internal transcribed spacer (ITS) regions, ITS-1 and ITS-2, along with highly conserved 18S, 5.8S and 28S rRNA genes has suggested that the causative agent of bovine and feline trichomoniasis is T. foetus (Felleisen, 1997, Felleisen, et al., 1998, Gookin, et al., 2002, Levy, et al., 2003, Grahn, et al., 2005). I believe that host specificity, along with morphological and genetic information should be included in any taxonomic evaluation. Differences were observed in disease and host specificity in heifers infected with T. foetus isolated from a cat and also from cats infected with T. foetus isolated from cows (Stockdale, et al., 2007, Stockdale, et al., 2007). The purpose of this study was to further characterize and compare feline and bovine isolates of T. foetus using information from experimental infections in both cattle and cats in addition to genetic sequencing and phylogenetic analysis and acquired morphological data. Materials and Methods Sources of organisms and maintenance Each of the twelve feline trichomonad isolates used in this study were obtained from naturally infected cats presented to the Auburn University parasitology laboratory. Only one feline isolate, AUTf-1, was observed by electron microscopy and used for morphological comparisons. The bovine isolate, D-1, was obtained from a naturally infected, pyometritic cow, donated by Dr. R. H. BonDurant. Additional bovine isolates (no. 25, 33, 34, 36) were obtained from naturally infected cows culled from a herd in Florida. All organisms were cultured in trypticase-yeast-maltose (TYM) Diamond?s medium (Diamond, 1983) without agar and incubated at 37 ?C during experimental 59 observations. Organisms were stored in liquid nitrogen in freezing medium made under sterile conditions using FCS, DMSO and TYM at 3:2:5, respectively. Light Microscopy Direct smears from cultured solutions of AUTf-1 were prepared using TYM Diamond?s medium. Organisms were examined with an Olympus bifocal microscope (Olympus America Inc., Center Valley, PA) at 100X. Differential interference contrast (DIC) photomicrographs were taken using a Nikon TE-2000 C1 (Nikon Instruments Inc., Melville, NY) at 60X. Prior to viewing, organisms were gently pelleted and the majority of supernatant media was removed. Pelleted organisms were resuspended in a 1:1 solution of paraformaldehyde-cacodylate. A direct smear was made from this mixture and sealed using Paramount? histological mounting medium (Fisher Scientific Co, Fair Lawn, NJ). Scanning Electron Microscopy (SEM) Suspensions of AUTf-1 in TYM Diamond?s medium without agar were concentrated from 15ml to 1ml by gentle centrifugation and removal of excess medium. Round glass slides were cleaned with 1% HCl in 70% EtOH and coated with 0.1% poly-L-lysine for 5 minutes. Slides were dried at 60 o C for 1 hour, washed with distilled water, and coated with the concentrated trichomonad-TYM medium solution. This was allowed to set for 15 minutes and excess media was removed. The slides were then fixed in 2.5% glutaraldehyde, 0.1M cacodylate buffer for 2 hours, washed with 0.2M cacodylate buffer for 2-3 minutes. Slides were then fixed in 1% OsO 4 in distilled water for 5 minutes and washed again in distilled water for 2-3 minutes. After a dehydration series of increasing ethanol concentrations (30%, 50%, 70%, 80%, 90%, 95%, 100%) for 10 minutes each, 60 slides were critical point dried with CO 2 (1150-1200 psi at 33 o C), coated twice with gold and viewed using a Zeiss DSM 940 scanning electron microscope (Carl Zeiss Inc., Oberkochen, Germany). Transmission Electron Microscopy (TEM) Suspensions of AUTf-1 in TYM Diamond?s medium without agar were concentrated from 15ml to 1ml by gentle centrifugation and removal of excess medium. Concentrated organisms were resuspended and fixed in 2.5% glutaraldehyde, 4% paraformaldehyde, and 5mM CaCl 2 in 0.1M cacodylate buffer (pH 7.4) overnight at 4C. The organisms were washed in 0.1 M cacodylate buffer for 5 minutes, embedded in 1% SeaPlaque (FMC Marine Colloids, Rockland, ME), and washed 3 additional times, 5 minutes each. The parasites were then post-fixed in 1% OsO 4, 0.1M cacodylate buffer, pH 7.4 at room temperature for 2 hours, and dehydrated in increasing concentrations of ethanol (50%, 70%, 95%, 100%) 3 changes, for 20 minutes each at 4 o C. Propylene oxide was used as a transient solvent. After embedding in Epon 812 epoxy resin (Ladd Research Industries, Inc., Burlington, VT), thin sections (70nm) were made and stained with uranyl acetate/lead citrate then viewed with a Philips 301 transmission electron microscope (FEI Co., Hillsboro, OR) operated at 60kV. Molecular characterization of Tritrichomonas foetus Trichomonad DNA was extracted from 12 feline trichomonad isolates using a previously described protocol (Billeter, et al., 2007) and identified using PCR with primers targeting the ITS-1 and ITS-2 regions, the 5.8S rRNA gene and partial 18S and 28S rRNA genes using previously described protocols (Felleisen, et al., 1998, Gookin, et al., 2002, Grahn, et al., 2005). The PCR products were directly sequenced using the 61 TFR-3 and TFR-4 primer sets, giving sequences of both strands (Appendix C). Other trichomonad sequences were obtained from GenBank and included trichomonads isolated from feline (AF466750, AF466751 and EF165538) (Levy, et al., 2003, Dahlgren, et al., 2007) and canine hosts (AY758392) (Gookin, et al., 2005), and additional bovine (U85967 and AF339736) (Felleisen, 1997, Walker, et al., 2003), porcine (U85966) (Felleisen, 1997), and reptilian trichomonads (AY886845) (Cepicka, et al., 2006). Random amplification of polymorphic DNA (RAPD) Nine previously described 12 mer oligonucleotide primers (Table 5.1) were used to amplify random DNA markers (Fraga, et al., 2002, Rojas, et al., 2004). Template DNA totaling 15 samples was extracted from 6 feline trichomonad isolates, 5 bovine T. foetus isolates, trichomonads isolated from the peritoneal cavity of a human, T. mobilensis from cotton rats, Trichomonas vaginalis from humans and Giardia sp. from humans as an outgroup. The DNA amplification method was adapted from Rojas et al., 2004 and performed in a final volume of 25?l. The reaction conditions were in 1X Thermopol II PCR buffer (includes 2 mM MgSO 4 , New England Biolabs), 200 ?M dNTPs (US Biochemicals), 25pM 12-mer primer, 2U StandardTaq DNA polymerase (New England Biolabs) and 100ng of template DNA. The PCR amplification conditions were an initial denaturation at 94 o C for 5 min and 40 cycles of 94 o C for 1 min, 35 o C for 1 min and 72 o C for 1 min, followed by a final extension at 72?C for 5 min. The PCR products were analyzed by electrophoresis on in 1.5% agarose gels in TBE buffer and stained with ethidium bromide, and photographed with a digital camera. The RAPD analysis was performed three times on different days by two separate investigators to ensure reproducibility. 62 Table 5.1. Oligonucleotide primers used for amplification of random DNA markers of various trichomonads (adapted from Rojas et al., 2004). Primer Sequence (5?-3?) 1 CGC ACT CGG AGT 2 TCG GCC GCT ATC 3 CCG TGA CAC GCA 4 GGG ACA CTC TGG 5 CCG CTG TAC TCC 6 GGG ACC TAC TGC 7 GAG TCG CAC AGG 8 TCC TCA CCG ACC 9 CCC CAG TAC CAG 63 Phylogenetic analysis Internal transcribed spacer regions and ribosomal RNA genes Nucleotide sequence data was collected using Chromas Lite version 2.01 (Technelyium PTY Ltd, Australia) and sequence alignment was performed using the AlignX? option in Vector NTI? Advance 10 (Invitrogen, Carlsbad, CA) followed by manual manipulation. Sequence comparisons were performed using the Maximum Likelihood method (dnaml) found in the Phylogeny Inference Package (PHYLIP) version 3.67 (Joseph Felsenstein, University of Washington, Seattle, WA). The best of tree from 100 replicates was created for each comparison using Phylodraw ver. 0.8 (Graphics Application Lab, Pusan National University). RAPD analysis The bands visualized in the RAPD gels were scored as present (1) or absent (0) for each isolate, with each compared against the other. The inverse of Jaccard?s similarity coefficient (Sj) was used in the following formula: Sj = 1 ? a / (a + b + c) where a = number of bands present in both isolates, b = number of bands present in isolate 1 and absent in isolate 2, and c = number of bands present in isolate 2 and absent in isolate 1. Results were compiled into a 15x15 matrix and analyzed using three methods, Fitch- Margoliash, Fitch-Margoliash with molecular clock (Kitsch) (this method is shown in the results) and Neighbor-Joining distance matrix programs included in the PHYLIP version 3.67. 64 Results Microscopic analysis Measurements of feline trichomonad trophozoites using SEM and TEM (Figs 5.1- 5.2) photomicrographs resulted in a mean cell body length of 10?m (range 5.7-13?m) and mean cell body width of 4.4?m (range 3.9-5.5?m). The axostyle extended from the posterior end of the cell body approximately 2?m and tapers to a thin tip. There were three anterior flagella each averaging 15?m in length, and a posterior flagellum following along and extending from the undulating membrane for approximately 12?m. The undulating membrane was approximately ? the length of the cell body. Internal organelles and cytoskeletal structures were also observed by transmission electron microscopy. Feline trichomonad trophozoites contained a single nucleus and Golgi apparatus. The axostyle ran the length of the cell body and a densely banded costa extending from the basal bodies followed the undulating membrane. Both structures were closely associated with spherical hydrogenosomes. Molecular comparisons DNA sequences containing the ITS-1 and ITS-2 regions, 5.8S rRNA gene and partial 18S and 28S rRNA genes of 12 feline trichomonad isolates were submitted to GenBank and given accession numbers listed in Table 5.2. When compared to the bovine (AF339736) and feline (AF466750) isolates registered in GenBank, all 12 feline isolates demonstrated differences in DNA sequences, including deletions, insertions and nucleotide changes, and point mutations (Table 5.3). We also compared the feline isolates with DNA sequences of trichomonads isolated from additional feline, canine, bovine, porcine and reptilian hosts found in GenBank (Appendix B). 65 (A ) (B ) Fi gur e 5. 1. Ph oto m i c r o gr aph s t a ken o f t h e f e l i n e A U T f - 1 i s o l at e o f Tr itr ichomonas f o etus . (A ) Th e d i ff e r e n t i a l i n t e r f e r e n c e c o n t r a s t m i c r o gr aph ( D I C ) de t a i l s t h e ax o s t y l e ( A X) , po s t er i o r an d an t e r i o r f l age l l a ( P F an d AF , r e s p ect i v e l y ) , co s t a (C ), a n d hy dr o g en o s o m e s ( H ) . ( B ) T h e s canni ng e l ec t r o n m i c r o gr aph ( S E M ) de t a i l s t h e ax o s t y l e , un du lat i n g m e m b r a n e ( U M ) , p o s t e r i o r a n d a n t e r i o r f l a g e l l a . AF PF PF AF AX AX H C UM 66 (A ) (B ) (C ) F i gur e 5. 2. T r an s m i s s i o n e l ect r o n m i c r o gr aph s ( T E M ) t a ken o f t h e f e l i n e A U T f - 1 i s o l at e o f Tr itr ichomonas f o etus . (A ) Se v e ra l i n t e r n a l o r gan e l l e s ar e vi s i b l e, i n c l ud i ng t h e co s t a ( C ) , n u c l eus ( N ) , ax o s t y l e ( A X) an d hy dr o g en o s o m e s ( H ) . ( B ) T h e an t e r io r en d o f t h e ce l l b o d y det a i l i ng t h e a x o s t y l e , n u c l e u s , hy dr o g en o s o m es a n d Go l g i appar a t u s ( G ) . F l a g e l l a ( F ) ar e a l s o vi s i b l e i n t h e t o p l e f t co r n er . ( C ) T h i s det a i l e d vi e w o f t h e an t e r i o r cel l b o d y s h o w s t h e pe l t a ( P ) . N N C UM H AX AX H H G P F 67 Table 5.2. Accession numbers given to feline (AUTf) trichomonad isolates registered in GenBank. The gene regions used for comparisons and corresponding base pairs are also listed. Accession number AUTf isolate 18S ITS-1 5.8S ITS-2 28S EU569301 1 1-3 4-83 84-243 244-308 >309 EU569302 2 1-4 5-84 85-244 245-309 >310 EU569303 3 1-3 4-83 84-243 244-308 >309 EU569304 4 1-4 5-84 85-244 245-309 >310 EU569305 5 0 1-80 81-240 241-305 >305 EU569306 6 1-3 4-83 84-243 244-308 >309 EU569307 7 1 2-81 82-241 242-301 >302 EU569308 9 1 2-81 82-241 242-301 >302 EU569309 10 1-2 3-82 83-242 243-308 >309 EU569310 11 1-5 6-85 86-245 246-310 >311 EU569311 12 1-5 6-85 86-245 246-310 >311 EU569312 13 1 2-81 83-241 242-301 >302 68 Table 5.3. Genetic sequences differences between 12 feline trichomonad isolates and the bovine (AF339736) isolate of T. foetus found in GenBank. Compared sequences are divided into three regions, ITS-1, ITS-2 and 5.8SrRNA. The number of insertions, deletions and single point mutants are given for each feline isolate. Isolates Gene Regions Changes in Genetic Sequences ITS-1, ITS-2, 5.8SrRNA Insertions Deletions Point mutant changes 1 3 3 4 2 4 3 19 3 2 2 1 4 3 5 2 5 7 34 15 6 2 1 2 7 0 2 6 9 6 2 6 10 2 1 0 11 2 3 1 12 2 4 7 13 3 5 7 ITS-1 Insertions Deletions Point mutant changes 1 1 3 4 2 4 3 19 3 2 2 1 4 2 5 2 5 7 34 15 6 2 1 2 7 0 2 5 9 5 2 6 10 1 1 0 11 2 3 1 12 2 4 6 13 2 4 7 ITS-2 Insertions Deletions Point mutant changes 1 2 0 0 2 0 0 0 3 0 0 0 4 1 0 0 5 0 0 0 6 0 0 0 7 0 0 1 9 1 0 0 10 1 0 0 11 0 0 0 12 0 0 1 13 1 1 0 69 Nucleotide sequence identities between the 12 AUTf isolates and those from GenBank ranged from 96-100% (Table 5.4). A phylogenetic tree constructed using the maximum likelihood method (PHYLIP, dnaml) indicates different results depending on the gene(s) compared. When sequences for the partial 28S, 18S and complete 5.8S rRNA genes, along with the ITS-1 and ITS-2 regions, were analyzed, the resulting tree indicates similarities between feline isolates and the isolates evaluated from GenBank (Fig 5.3). These results were also similar to those comparing the ITS-2 region of each trichomonad sequence (Fig 5.4). However, when DNA sequences from the ITS-1 region were compared between feline isolate sequences and sequences from GenBank, the feline isolate sequences clustered separately from the other either as their own group or with the chosen outlier, P. hominis. This clustering was statistically significant (P<0.005) (Fig 5.5). The RAPD results generated from PCR amplification of trichomonad DNA using 9 random primer sequences further support the data obtained by the ITS-1 DNA sequence analysis. The feline Tritrichomonas sp. isolates were more similar to each other than to the bovine T. foetus isolates. The bovine isolates were more similar to each other than to feline Tritrichomonas isolates (Fig 5.6). As expected, the Trichomonas vaginalis and Giardia lamblia DNA displayed different banding patterns than Tritrichomonas isolates of either feline or bovine origin. Tritrichomonas mobilensis and a trichomonad isolated from the peritoneal cavity of a human displayed banding patterns more similar to feline T. foetus isolates than those of bovine origin. The matrix of band differences is shown in Appendix D. The banding pattern differences in banding patterns are depicted in a 70 Table 5.4. Sequence identities (%) determined by BLASTn analysis between the 12 feline isolates (EU569301-EU569312, respectively) and 5 other trichomonads from GenBank. Isolate AF339736 AF466750 AY349190 AY886845 AY886824 (bovine) (feline) (T. suis) (T. nonconforma) (T. mobilensis) 1 97 98 98 97 97 2 99 100 99 98 98 3 98 99 98 98 98 4 97 97 98 97 97 5 97 97 97 100 100 6 98 99 98 98 98 7 97 97 97 96 96 9 97 97 97 96 96 10 99 99 99 99 99 11 98 99 98 98 98 12 98 98 98 97 97 13 97 98 98 97 97 71 Fi gur e 5. 3. Phy l o g e n et i c t r ee depi ct i n g ge n e t i c s e quen c e co m p ar i s o n s o f t h e 5. 8Sr R NA gen e a n d I T S- 1 an d I T S - 2 r e gi o n s bet w een A U T f s e que n c e s an d pu bl i s hed Ge n B a n k s e que n c e s . A U T f i s o l at es 1- 7; 9- 13 ar e l i s t e d as acces s i o n n u m b er s E U 569301- E U 569312, r e s p ect i v e l y . P e ntatr i chomonas homi n is ( A Y758392) , b o vi n e T. f o e t us i s o l at es ( A F 339 736 an d U85967) , f e li ne T. fo e t u s i s o l at es AF 466750 a n d E F 165538) , T. s u is ( U 85966) an d T. noncon f o r m a ( A Y886845) ar e al s o us ed i n t h e co m p ar i s o n . 72 Fi gur e 5. 4. Phy l o g e n et i c t r ee depi ct i n g ge n e t i c s e quen c e co m p ar i s o n s o f t h e I T S- 2 r e gi o n b e t w ee n A U T f s e que n c e s an d pu bl i s hed GenB a n k s e que n c es . A U T f i s o l at es 1- 7; 9- 13 ar e l i s t e d as acces s i o n n u m b er s E U 569301- E U 569312, r e s p ect i v e ly . P e ntatr i chomona s hominis ( A Y758392) , b o vi n e T. f o e t us i s o l at es ( A F 339736 a n d U85967) , f e li ne T. f o e t us i s o l at es ( A F 466750 an d E F 165538) , T. s u is ( U 85966) an d T. noncon f o r m a ( A Y886845) ar e a l s o us ed i n t h e co m p ar i s o n . 73 Fi gur e 5. 5. Phy l o g e n et i c t r ee depi ct i n g ge n e t i c s e quen c e co m p ar i s o n s o f t h e I T S- 1 r e gi o n b e t w ee n A U T f s e que n c e s an d pu bl i s hed GenB a n k s e que n c es . A U T f i s o l at es 1- 7; 9- 13 ar e l i s t e d as acces s i o n n u m b er s E U 569301- E U 569312, r e s p ect i v e ly . P e ntatr i chomona s hominis ( A Y758392) , b o vi n e T. f o e t us i s o l at es ( A F 339736 a n d U85967) , f e li ne T. f o e t us i s o l at es ( A F 466750 an d E F 165538) , T. s u is ( U 85966) an d T. noncon f o r m a ( A Y886845) ar e a l s o us ed i n t h e co m p ar i s o n . 74 Fi gur e 5. 6. R A PD PC R r e s u l t s us i n g 9 o l i g o n u c l e o t i d e 12- m e r pr i m e r s to c o m p ar e ge n e t i c s e que n c e ban d i ng pat t e r n s b e t w ee n A U T f f e li ne t r i c h o m o n a d i s o l at es an d ot h e r tr i c h o m o n a d i s o l at es . F a r l e f t : 1kb l a dder , L a n e s 1- 5: b ovi ne i s o l at e ( D - 1 ) , F l o r i d a b o vi ne i s o l at es n o . 25, 33, 34 an d 36, r e s p ect i v e l y . L a n e s 6- 10, 12: A U T f i s o l at es 1 ( E U569301) , 7 ( E U569307) , 9 ( E U569308) , 10 ( E U569309) , 4 ( E U569304 ) an d 12 ( E U569311) , r e s p ect i v e l y . L a n e 11: Tr ichomonas vaginalis , L a nes 13- 16: Tr itr ichomonas mobile ns is , t r i c ho m o n a d f r o m hu ma n p e r i t o ne a l c a v i t y , Giar dia s pp. , an d n e g a t i ve co n t r o l , r e s p ect i v e 75 dendrogram created using Phylodraw after using the Kitsch (PHYLIP) matrix analysis method (Fig. 5.7). Discussion The morphological characteristics of T. foetus recovered from the reproductive tract of cattle have been extensively described (Wenrich and Emmerson, 1933, Honigberg, et al., 1971, Mehlhorn, et al., 1988, Mattos, et al., 1997, Benchimol, 2004, 2005). The mean length of T. foetus isolated from cattle can range from 10-25?m and the width may be one-third the length, or an average of 6?m (Wenrich and Emmerson, 1933, Mattos, et al., 1997). There were no morphological differences between feline trichomonad isolates and T. foetus recovered from cattle. A PCR protocol has been described that identifies trichomonads recovered from cattle using amplification of the ITS-1 region and differentiates between the trichomonads T. foetus, P. hominis and Tetratrichomonas sp. (Grahn, et al., 2005). The amplified sequence includes only 157 base pairs; however there is enough diversity in the ITS-1 region to differentiate between three separate genera of morphologically similar trichomonads. DNA sequence analysis of PCR products amplifying the ITS-1, 5.8SrRNA and ITS-2 genes (Felleisen, 1997, Gookin, et al., 2002, Grahn, et al., 2005) indicated a 97-100% sequence identity for feline (AF466750) and a 97-99% sequence identity for bovine (AF339736) isolates published in GenBank when compared against the 12 feline trichomonad isolate sequences (Table 5.4). Additionally, these feline sequences had a 97-99% sequence identity with T. suis (AY349190), 96-100% sequence identity with T. nonconforma (AY886845) and 96-100% sequence identity to T. mobilensis (AY886842). 76 F i gur e 5. 7. P h y l o g e n et i c t r ee depi ct i n g ge n e t i c s e quen c e co m p ar i s o n s o f t h e RA P D P CR r e s u l t s b e t w een A U T f s e que n c e s an d publi s h e d Ge nB a n k s e que n c e s . A U T f i s o l at es 1, 4, 7, 9- 10 , 12 ar e l i s t e d as acces s i o n n u m b er s E U 569301, - 304 , - 307, - 308 , - 309 , an d - 311, r e s p ect i v e l y . B o vi ne T. f o e t us i s o l at es i n c l uded ( D - 1 ) an d t h o s e i s o l at ed f r o m n a t u r a l l y i n f e ct ed c o ws i n F l o r i d a ( 25- , 33 - , 34- , an d 36- b o vi n e ) . A d d i t i o n a l s e que n c es f r o m T. mobile ns is , Giar dia s pp. , Tr ichomonas vaginalis an d t r i c h o m o n a d s i s o l at ed f r o m a h u m a n per i t o n e a l c a v i t y ( p er i t o n ea l ) wer e al s o us ed f o r c o m p ar i s o n . 77 DNA sequence analysis at the ITS-1 and ITS-2 regions along with rRNA genes of feline trichomonad isolates are similar to those of T. foetus species recovered from naturally infected cats and cows. However, this is only true when the DNA sequences including both ITS regions and rRNA gene are compared. When looking at this region as a whole, the feline trichomonad isolates grouped with T. foetus isolates of both bovine and feline origin (Fig 5.3). This was also true when the ITS-2 region was used for comparison (Fig 5.4). These results are to be expected since the rRNA genes are highly conserved between species. When the nucleotide sequences are evaluated more closely, there are clear sequence differences at the ITS-1 region, demonstrated in both the phylogenetic tree (Fig. 5.5) and DNA sequences (Table 5.3). If only the ITS-1 gene region is used for comparison between the 12 feline trichomonad isolates and the feline (AF466750) and bovine (AF339736) isolates published in GenBank, the number of nucleotide insertions range from 0-7, nucleotide deletions range from 1-34 and nucleotide point mutations range from 1-19 (Table 5.3). The feline trichomonad isolates grouped separately or closer to P. hominis in a statistically significant manner (Fig 5.5). This shift between two genera may suggest a species in transition with more than intra- specific genetic differences. Additionally, T. suis (U85966) grouped closely with T. foetus of bovine origin (AF339736, U85967) in each separate ITS sequence analysis (Figs. 5.3-5.5) supporting the proposed synonymy between T. suis and T. foetus (Tachezy, et al., 2002). The RAPD results further support the differences between the feline and bovine trichomonad isolates at the ITS-1 region (Figs 5.6-5.7). Five of six feline trichomonad isolates grouped together, along with T. mobilensis and trichomonads isolated from the 78 human peritoneal cavity. Additionally, four of the five bovine isolates grouped together, branching separately from the feline isolates. The phylogenetic trees depicted the differences visualized in the banding patterns on the gel (Fig 5.6). Although there were differences among members of the bovine and feline isolates within each group, there were similarities between banding patterns of isolates within each group and between the two groups. The banding patterns of T. mobilensis and the additional trichomonad found in the human peritoneal cavity are more similar to those of the feline rather than bovine isolates. This difference is displayed in the phylogenetic tree (Fig 5.7). These differences observed at the molecular level are further supported by the cross-infection studies that demonstrated significant differences in the host specificity of a trichomonad isolated from the feces a cat and the reproductive tract of a cow. Tritrichomonas sp. isolated from felines did not induce the same level pathogenesis in infected heifers when compared heifers infected with the bovine T. foetus isolate (Stockdale, et al., 2007). Of 8 sampled heifers infected with a feline trichomonad isolate, only 1 had lost the surface epithelial layer of the uterus, while all 6 sampled heifers infected with a bovine isolate of T. foetus has lost the surface epithelial layer. Additionally, of six cats infected with the bovine D-1 T. foetus isolate fecal culture samples from only one cat was culture positive for trichomonads and at PI day 32, the last day of sampling. The cat infected with the feline Tritrichomonas sp. was fecal culture positive by PI day 16 (Stockdale, et al., 2008). DNA sequence analysis using highly conserved genes should not be the sole basis of species differentiation. There are numerous examples of parasite species within the same genus that can be differentiated based on host specificity and/or pathogenicity that 79 possess similar gene sequences. The Plasmodium gene PgSES contains 3 highly conserved regions within various protein homologs (LaCrue, et al., 2006). These conserved regions are found within 7 Plasmodium species and are expressed in multiple parasite stages. The ITS and rRNA genetic sequence data of the feline trichomonad isolates and published sequences of T. foetus of bovine and feline origin were nearly identical (98-99%) to T. nonconforma and T. mobilensis, two established and valid species (data not shown). I feel that there are inconsistencies in host specificity and differences in pathogenicity of the feline and bovine trichomonad isolates, along with the DNA sequence analysis that exceed what would be expected as intra-specific variation. When ITS-1 gene regions are isolated for comparison between feline and bovine isolates of T. foetus there are clear sequence differences that may account for species differences in addition to genera differentiation as previously described (Grahn, et al., 2005). Results from the RAPD PCR analysis suggest additional genetic differences between bovine and feline trichomonad isolates and suggest species differences and that the causative agent of feline trichomoniasis is not Tritrichomonas foetus, in light of past molecular and morphological data. 80 CHAPTER VI OVERALL CONCLUSIONS Results of my research indicate that Tritrichomonas foetus is prevalent in the pet population and that its presence appears to correlate with the presence of diarrhea. Of the 173 cats surveyed, 17 were fecal culture positive for T. foetus and all suffered from chronic diarrhea. Our survey offers limited insight into the prevalence of T. foetus in the pet cat population and produces additional questions. One question that remains is whether T. foetus is the only cause of large-bowel disease in cats or if it is an opportunist working in conjunction with other pathogens to exacerbate the symptoms of enteritis. Many reported cases of feline trichomoniasis also report concurrent infections with Giardia spp., Cryptosporidium spp., coccidia or the cat also suffered from FIP. Another question is whether pure bred cats are at a greater risk of T. foetus infection than domestic mixed breeds or if likelihood of infection can be attributed more to living environments. Many of the infected cats in this survey live in multi-cat households or catteries where cats are densely populated. There have also been no reports linking T. foetus infection in the feline intestine to T. foetus infection in the bovine reproductive tract. The possibility of cross-transmission of T. foetus between the two species seems unlikely. The combined results of the experimental infections in bovines and felines indicate that the diseases caused by the feline and bovine isolates of T. foetus in cattle are not identical and the susceptibility of cats to the feline and bovine isolates of T. foetus 81 also appears demonstrably different. Biopsy samples taken from the 8 heifers experimentally infected with T. foetus collected from a naturally infected cat demonstrated that a single heifer lost the surface epithelial layer of the uterus. When the same procedure was performed using heifers infected with T. foetus collected from a naturally infected, pyometritic cow all 6 available samples showed a loss of surface epithelium. Lesions scores between two groups were significantly different (P = 0.005). Additionally, there was a significant difference in the time required to clear the trichomonad infection between the two groups. Those heifers infected with the bovine isolate cleared the infection by post-inoculation (PI) week 19, while 2 heifers infected with the feline isolate were still culture positive by PI week 30. In the second experimental infection study, the cat infected with a feline isolate of T. foetus became fecal culture positive by PI day 16, while only 1 of 6 cats infected with the bovine isolate was fecal culture positive by PI day 32. Additionally, when intestinal contents of each cat were analyzed it was found that the cat infected with the feline isolate was culture positive in the ileum, cecum, middle and distal colon. Of the 6 cats infected with the bovine isolate of T. foetus, 2 were culture positive in the cecum only. These results suggest that feline and bovine trichomonad isolates are different species with different host specificities. These data also suggest that direct transmission from bovines to felines is not the primary means of trichomonad infection in cats. Further biological characterization of 12 feline isolates of T. foetus presented to the parasitology laboratory at Auburn University demonstrated similar morphological characteristics when using published descriptions of both bovine and feline T. foetus isolates. Differences were found primarily in the internal transcribed spacer (ITS) 1 82 region rather than the ITS-2 or highly conserved 5.8SrRNA regions commonly used for comparisons of trichomonads. In some feline isolates, there were as many as 34 nucleotide changes that were either insertions, deletions or point mutations, when compared with bovine and some feline isolates published in GenBank. Phylogenetic analysis suggests variable sequence differences between the isolates depending on the genetic region analyzed (i.e. ITS-1, ITS-2, rRNA). Feline isolates tended to group with themselves or in many instances closer to Pentatrichomonas hominis. This could suggest a species in transition implying there are more than intra-specific differences between the isolates. Differences between feline and bovine isolates are also supported in data produced by random amplified polymorphic DNA (RAPD) analysis where banding patterns of feline isolates were more similar to each other than to bovine isolates. This was also depicted by the phylogenetic tree. Additionally, all T. foetus isolates used for DNA sequence comparisons were nearly identical (97-100%) to T. nonconforma and T. mobilensis, two established and valid species originating from an Anolis lizard and tree shrew, respectively. These studies provide compelling evidence that fundamental differences exist between the different isolates of T. foetus exceeding what one would expect to observe in normal intra-specific variation. 83 CUMULATIVE BIBLIOGRAPHY Adl, S. M., A. G. B. Simpson, M. A. Farmer, R. A. Andersen, O. R. Anderson, J. R. Barta, S. S. Bowser, G. Brugerolle, R. A. Fensome, S. Fredericq, T. Y. James, S. Karpov, P. Kugrens, J. Krug, C. E. Lane, L. A. Lewis, J. Lodge, D. H. Lynn, D. G. Mann, R. M. McCourt, L. Mendoza, ?. Moestrup, S. E. Mozley-Standridge, T. A. Nerad, C. A. Shearer, A. V. Smirnov, F. W. Spiegel and M. F. R. Taylor. 2005. The new higher level classification of eukaryotes with emphasis on the taxonomy of protists. Journal of Eukaryotic Microbiology 52: 399-451 Anderson, M. L., R. H. BonDurant, R. R. Corbeil and L. B. Corbeil. 1996. Immune and inflammatory responses to reproductive tract infection with Tritrichomonas foetus in immunized and control heifers. Journal of Parasitology 82: 594-600 [APPMA] American Pet Products Manufacturers Association. 2008. 2007-2008 National Pet Owners Survey. www.appma.org/. Accessed Jan 7 2008. Benchimol, M. 2004. Trichomonads under microscopy. Microscopy and Microanalysis 10: 528-550 ---. 2005. New ultrastructural observations on the skeletal matrix of Tritrichomonas foetus. Parasitology Research 97: 408-416 Benchimol, M., R. da Silva Fontes and ?. Jos? Buria Dias. 2007. Tritrichomonas foetus damages bovine oocytes in vitro. Veterinary Research 38: 399-408 Bielanski, A., D. F. Ghazi and B. Phipps-Toodd. 2004. Observations on the fertilization and development of preimplantation bovine embryos in vitro in the presence of Tritrichomonas foetus. Theriogenology 61: 821-829 Billeter, S. A., J. A. Spencer, B. Griffin, C. C. Dykstra and B. L. Blagburn. 2007. Prevalence of Anaplasma phagocytophilum in domestic felines in the United States. Veterinary Parasitology 147: 194-198 BonDurant, R. H. 1985. Diagnosis, treatment and control of bovine trichomoniasis. Compendium of Continuing Education for the Practicing Veterinarian 7: S179-S188 ---. 1997. Pathogenesis, diagnosis and management of trichomoniasis in cattle. Veterinary Clinics of North America Food Animal Practice 13: 345-361 84 BonDurant, R. H., M. L. Anderson, P. Blanchard, D. Hird, C. Danaye-Elmi, C. Palmer, W. M. Sischo, D. Suther, W. Utterback and B. J. Weigler. 1990. Prevalence of trichomoniasis among California beef herds. Journal of the American Veterinary Medical Association 196: 1590-1593 BonDurant, R. H. and B. M. Honigberg. 1994. Trichomonads of veterinary importance. In: Parasitic Protozoa, J. P. Kreier (ed.). Academic Press, San Diego, CA, p. 111-188. Brugerolle, G. and J. Lee. 2000. Phylum Parabasalia. In: The Illustrated Guide to the Protozoa, J. Lee, G. Leedale and P. Bradbury (ed.). Society of Protozoologists, Lawrence, KS, p. 1196-1210. Campero, C. M., R. G. Hirst, P. W. Ladds, J. A. Vaughan, D. L. Emery and D. L. Watson. 1990. Measurement of antibody in serum and genital fluids of bulls by ELISA after vaccination and challenge with Tritrichomonas foetus. Australian Veterinary Journal 67: 175-178 Cepicka, I., V. Hampl, J. Kulda and J. Flegr. 2006. New evolutionary lineages, unexpected diversity, and host specificity in the parabasalid genus Tetratrichomonas. Molecular Phylogenetics and Evolution 39: 542-551 Corbeil, L. B., J. L. Hodgson, D. W. Jones, R. R. Corbeil, P. R. Widders and L. R. Stephens. 1989. Adherence of Tritrichomonas foetus to bovine vaginal epithelial cells. Infection and Immunity 57: 2158-2165 Dahlgren, S. S., B. Gjerde and H. Y. Pettersen. 2007. First record of natural Tritrichomonas foetus infection of the feline uterus. Journal of Small Animal Practice 48: 654-657 Diamond, L. S. 1983. Lumen dwelling protozoa: Entamoeba, Trichomonads and Giardia. In: In vitro cultivation of protozoan parasites, J. B. Jensen (ed.). CRC Press, Boca Raton, Florida, p. 65-111. Felleisen, R. S. J. 1997. Comparative sequence analysis of 5.8S rRNA genes and internal transcribed spacer (ITS) regions of trichomonadid protozoa. Parasitology 115: 111-119 ---. 1999. Host-parasite interaction in bovine infection with Tritrichomonas foetus. Microbes and Infection 1: 807-816 Felleisen, R. S. J., N. Lambelet, P. Bachmann, J. Nicolet, N. M?ller and B. Gottstein. 1998. Detection of Tritrichomonas foetus by PCR and DNA enzyme immunoassay based on rRNA gene unit sequences. Journal of Clinical Microbiology 36: 513-519 Fitzgerald, P. R., A. E. Johnson, J. Thorne, L. H. Davis and D. M. Hammond. 1958. Trichomoniasis in range cattle. Veterinary Medicine 53: 249-252 85 Foster, D. M., J. L. Gookin, M. F. Poore, M. E. Stebbins and M. G. Levy. 2004. Outcome of cats with diarrhea and Tritrichomonas foetus infection. Journal of the American Veterinary Medical Association 225: 888-892 Fraga, J., L. Rojas, I. Sariego and C. Sarr?a. 2002. Optimization of random amplified polymorphic DNA techniques for its use in genetic studies of Trichomonas vaginalis isolates. Infection, Genetics and Evolution 2: 73-75 Gookin, J. L., A. J. Birkenheuer, E. B. Breitschwerdt and M. G. Levy. 2002. Single-tube nested PCR for detection of Tritrichomonas foetus in feline feces. Journal of Clinical Microbiology 40: 4126-4130 Gookin, J. L., A. J. Birkenheuer, V. St.John, M. Spector and M. G. Levy. 2005. Molecular characterization of trichomonads from feces of dogs with diarrhea. Journal of Parasitology 91: 939-943 Gookin, J. L., E. B. Breitschwerdt, M. G. Levy, R. B. Gager and J. G. Benrud. 1999. Diarrhea associated with trichomonosis in cats. Journal of the American Veterinary Medical Association 215: 1450-1454 Gookin, J. L., C. N. Copple, M. G. Papich, M. Poore, S. H. Stauffer, A. J. Birkenheuer, D. C. Twedt and M. G. Levy. 2006. Efficacy of ronidazole for treatment of feline Tritrichomonas foetus infection. Journal of Veterinary Internal Medicine 20: 536-543 Gookin, J. L., D. M. Foster, M. Poore, M. E. Stebbins and M. G. Levy. 2003. Use of a commercially available culture system for diagnosis of Tritrichomonas foetus infection in cats. Journal of the American Veterinary Medical Association 222: 1376-1379 Gookin, J. L., M. G. Levy, J. M. Law, M. G. Papich, M. F. Poore and E. B. Breitschwerdt. 2001. Experimental infection of cats with Tritrichomonas foetus. American Journal of Veterinary Research 62: 1690-1697 Gookin, J. L., S. H. Stauffer, M. R. Coccaro, M. Poore, M. G. Levy and M. G. Papich. 2007. Efficacy of tinidazole for treatment of cats experimentally infected with Tritrichomonas foetus. American Journal of Veterinary Research 68: 1085-1088 Gookin, J. L., M. E. Stebbins, E. Hunt, K. Burlone, M. Fulton, R. Hochel, M. Talaat, M. Poore and M. G. Levy. 2004. Prevalence of and risk factors for feline Tritrichomonas foetus and Giardia infection. Journal of Clinical Microbiology 42: 2707-2710 Grahn, R. A., R. H. BonDurant, K. A. v. Hoosear, R. L. Walker and L. A. Lyons. 2005. An improved molecular assay for Tritrichomonas foetus. Veterinary Parasitology 127: 33-41 Gunn-Moore, D. A., T. M. McCann, N. Reed, K. E. Simpson and B. Tennant. 2007. Prevalence of Tritrichomonas foetus infection in cats with diarrhoea in the UK. Journal of Feline Medicine and Surgery 9: 214-218 86 Haydon, D. T., S. Cleaveland, L. H. Taylor and M. K. Laurenson. 2002. Identifying reservoirs of infection: a conceptual and practical challenge. Emerging Infectious Diseases 8: 1468-1473 Honigberg, B. M. 1963. Evolutionary and systematic relationships in the flagellate order Trichomonadida Kirby. Journal of Protozoology 10: 20-63 Honigberg, B. M. and D. E. Burgess. 1994. Trichomonads of importance in human medicine including Dientamoeba fragilis. In: Parasitic Protozoa, J. P. Kreier (ed.). Academic Press, San Diego, CA, p. 1-57. Honigberg, B. M., C. F. T. Mattern and W. A. Daniel. 1971. Fine structure of the mastigont system in Tritrichomonas foetus (Riedm?ller). Journal of Protozoology 18: 183-198 Hook, R. R., M. C. St.Claire, L. K. Riley, C. L. Franklin and C. L. Besch-Williford. 1995. Tritrichomonas foetus: Comparison of isolate virulence in an estrogenized mouse model. Experimental Parasitology 81: 202-207 [HSUS] The Humane Society of the United States. 2008. US Pet Ownership Statistics. www.hsus.org. Accessed Jan 7 2008. Jordan, H. E. 1956. Trichomonas spp. in feline: A case report. Veterinary Medicine 51: 23-24 Kessel, J. F. 1928. Trichomoniasis in kittens. Transactions of the Royal Society of Tropical Medicine and Hygiene 22: 61-80 Kleina, P., J. Bettim-Bandinelli, S. L. Bonatto, M. Benchimol and M. R. Bogo. 2004. Molecular phylogeny of Trichomonadidae family inferred from ITS-1, 5.8S rRNA and ITS-2 sequences. International Journal for Parasitology 34: 963-970 Kofoid, C. A. 1920. A critical review of the nomenclature of human intestinal flagellates, Cercomonas, Chilomastix, Trichomonas, Tetratrichomonas, and Giardia. University of California Publications in Zoology 20: 145-168 Kvasnicka, W., M. Hall and D. Hanks. 1999. Bovine Trichomoniasis. In: Current veterinary therapy 4: food animal practice, J. Howard (ed.). WB Saunders Co, Philadelphia, PA, p. 420-425. LaCrue, A. N., M. Sivaguru, M. F. Walter, D. A. Fidock, A. A. James and B. T. Beerntsen. 2006. A ubiquitous Plasmodium protein displays a unique surface labeling pattern in sporozoites. Molecular & Biochemical Parasitology 148: 199-209 Laing, J. A. 1956. Trichomonas foetus infection of cattle. FAO of the United Nations. 33: 39. 87 Lappin, M. 2000. Protozoal and miscellaneous infections. In: Textbook of Veterinary Internal Medicine: Diseases of the Dog and Cat, S. Ettinger and E. Feldman (ed.). WB Saunders, Philadelphia, PA, p. 408-417. Levy, M. G., J. L. Gookin, M. Poore, A. J. Birkenheuer, M. J. Dykstra and R. W. Litaker. 2003. Tritrichomonas foetus and not Pentatrichomonas hominis is the etiologic agent of feline trichomonal diarrhea. Journal of Parasitology 89: 99-104 Mattos, A., A. M. Sol?-Cava and G. DeCarli. 1997. Fine structure and isozymic characterization of trichomonadid protozoa. Parasitology Research 83: 290-295 Mehlhorn, H., J. F. Dubremetz, M. Franz, M. Gustafsson, W. Peters, H. Taraschewski, V. Walldorf and W. P. Voigt. 1988. Morphology. In: Parasitology in Focus: Facts and Trends, H. Mehlhorn (ed.). Springer-Verlag, Berlin, p. 161-312. Morgan, B. B. 1944. Bovine Trichomoniasis, Burgess Publishing, Minneapolis, Minnesota, 165 p. ---. 1947. A summary of research of Trichomonas foetus. Journal of Parasitology 33: 201-206 Okamoto, S., M. Wakui, H. Kobayashi, N. Sato, A. Ishida, M. Tanabe, T. Takeuchi, S. Fukushima, T. Yamada and Y. Ikeda. 1998. Tritrichomonas foetus meningoencephalitis after allogenic peripheral blood stem cell transplantation. Bone Marrow Transplantation 21: 89-91 Parsonson, I. M., B. L. Clark and J. H. Dufty. 1976. Early pathogenesis and pathology of Tritrichomonas foetus infection in virgin heifers. Journal of Comparative Pathology 86: 59-66 Rae, D. 1989. Impact of trichomoniasis on the cow-calf producer's profitability. Journal of the American Veterinary Medical Association 194: 771-775 Rae, D., P. Chenoweth, P. Genho, A. McIntosh, C. Crosby and S. Moore. 1999. Prevalence of Tritrichomonas fetus in a bull population and effect on production in a large cow-calf enterprise. Journal of the American Veterinary Medical Association 214: 1051-1055 Rhyan, J. C., L. L. Stackhouse and W. J. Quinn. 1988. Fetal and placental lesions in bovine abortion due to Tritrichomonas foetus. Veterinary Pathology 25: 350-355 Rhyan, J. C., K. L. Wilson, B. Wagner, M. L. Anderson, R. H. BonDurant, D. E. Burgess, G. K. Mutwiri and L. B. Corbeil. 1999. Demonstration of Tritrichomonas foetus in the external genitalia and of specific antibodies in prepucial secretions of naturally infected bulls. Veterinary Pathology 36: 406-411 88 Riedm?ller, L. 1928. Ueber die Morphologie, Uebertragungsversuche und klinische Bedeutung der beim sporadischen Abortus des Rindes vorkommenden Trichomonaden. Zentralblatt fur Bakteriologie, Parasitenkunde, Infektionskrankheiten und Hygiene. 1. Abt., 108: 103-118 Roberts, L. and J. Janovy. 2000. Parasitic protozoa: Form, function and classification. In: Foundations of Parasitology, G. Schmidt and L. Roberts (ed.). McGraw-Hill, Boston, MA, p. 37-54. Rojas, L., J. Fraga and I. Sariego. 2004. Genetic variability between Trichomonas vaginalis isolates and correlation with clinical presentation. Infection, Genetics and Evolution 4: 53-58 Romatowski, J. 1996. An uncommon protozoan parasite (Pentatrichomonas hominis) associated with colitis in three cats. Feline Practice 24: 10-14 ---. 2000. Pentatrichomonas hominis infection in four kittens. Journal of the American Veterinary Medical Association 216: 1270-1272 Skirrow, S. Z. and R. H. BonDurant. 1990a. Induced Tritrichomonas foetus infection in beef heifers. Journal of the American Veterinary Medical Association 196: 885-889 ---. 1990b. Immunoglobulin isotype of specific antibodies in reproductive tract secretions and sera in Tritrichomonas foetus-infected heifers. American Journal of Veterinary Research 51: 645-653 Stockdale, H. D., A. R. Dillon, J. Newton, R. C. Bird, R. H. BonDurant, P. Deinnocentes, S. Barney, J. Butler, T. Land, J. A. Spencer, D. S. Lindsay and B. L. Blagburn. 2007. Experimental infection of cats (Felis catus) with Tritrichomonas foetus isolated from cattle. Veterinary Parasitology ---. 2008. Experimental infection of cats (Felis catus) with Tritrichomonas foetus isolated from cattle. doi: 10/1016/j.vetpar.2008.02.024 Stockdale, H. D., S. P. Rodning, M. D. Givens, D. M. Carpenter, S. D. Lenz, J. A. Spencer, C. C. Dykstra, D. S. Lindsay and B. L. Blagburn. 2007. Experimental infection of cattle with a feline isolate of Tritrichomonas foetus. Journal of Parasitology 93: 1429- 1434 Stockdale, H. D., J. A. Spencer, C. C. Dykstra, G. S. West, T. Hankes, K. L. McMillan, M. Whitley and B. L. Blagburn. 2006. Feline Trichomoniasis: An Emerging Disease. Compendium of Continuing Education for the Practicing Veterinarian 28: 463-471 Tachezy, J., R. Tachezy, V. Hampl, M. Sedinova, S. Vanacova, M. Vrlik, M. vanRanst, J. Flegr and J. Kulda. 2002. Cattle pathogen Tritrichomonas foetus (Riedmuller, 1928) and pig commensal Tritrichomonas suis (Gruby & Delafond, 1843) belong to the same species. Journal of Eukaryotic Microbiology 49: 154-163 89 Vanroose, G., A. d. Kruif and A. V. Soom. 2000. Embryonic mortality and embryo- pathogen interactions. Animal Reproduction Science 60-61: 131-143 Walker, R. L., D. C. Hayes, S. J. Sawyer, R. W. Nordhausen, K. A. Van Hoosear and R. H. BonDurant. 2003. Comparison of the 5.8S rRNA gene and internal transcribed space regions of trichomonadid protozoa recovered from the bovine prepucial cavity. Journal of Veterinary Diagnostic Investigation 15: 14-20 Wenrich, D. H. and M. A. Emmerson. 1933. Studies on the morphology of Tritrichomonas foetus (Riedm?ller) (Protozoa, Flagellata) from American cows. Journal of Morphology 55: 193-205 Wilcock, B. 1992. Endoscopic biopsy interpretation in canine or feline enterocolitis. Seminars in Veterinary Medicine and Surgery (Small Animal) 7: 162-171 Wilson, S. K., A. A. Kocan, E. T. Gaudy and D. Goodwin. 1979. The prevalence of trichomoniasis in Oklahoma beef bulls. Bovine Practitioner 14: 109-110 Yeager, M. J. and J. L. Gookin. 2005. Histologic features associated with Tritrichomonas foetus-induced colitis in domestic cats. Veterinary Pathology 42: 797-804 90 APPENDIX A COMPLETE DATA RESULTS OBTAINED FROM VETERINARIANS PARTICIPATING IN THE SURVEY OF THE PET CAT POPULATION 91 92 93 94 95 96 97 APPENDIX B ALIGNED SEQUENCES FOR ALL ISOLATES USED IN GENETIC COMPARISONS OF THE ITS-1, ITS-2 AND 5.8S rRNA GENES 98 20 samples (GenBank Accession numbers) 350 base pairs AF339736 TCAGTTTCGTTAATAATTAC----AAACATAT-TTTTTTAATGTCTATAA AF466750 TCAGTTTCGTTAATAATTAC----AAACATAT-TTTTTTAATGTCTATAA DQ233455 -------------AAAATAC----AAACATTAATTTTTTTAAAATTTTAA EU569301 -CAGTTTCGTTAATAATTAC-----AACATAT-TTTTTTAATGTCTATAT EU569302 TCAGTTTCGTTAACTATGCC---GTTGTATCT-GTTCTCATAGCCCGGGC EU569303 -CAGTTTCGTTAATAATTAC----AA-CATAT-TTTTTTAATGTCTATAC EU569304 TCAGTTTCGTTAATTACAA-------ACATAT-TTTTTT-ATGTCTATAT EU569305 -------------CCCTGCCC--GTTGGATCT-TTTCGT-TAACC--GGC EU569306 -CAGTTTCGTTAATAATTAC---AAAACATAT-TTTTTTATTGTCTATAT EU569307 ---GTTTCGTTAATA-TTAC---AAA-CATAT-TTTTTT-TTGTCTATAA EU569308 ---GTTTCGTTAACTGAGTGT--ACAACATATATTTTTTATTGTCTATAA EU569309 --AGTTTCGTTAATAATTAC----AAACATAT-TTTTTTAATGTCTATAA EU569310 TCAGTTTCGTTAATAGTTAC-----AACATAT-TTTTTTATTGTCTATAA EU569311 TCAGTTTCGTTAATAATTAC-----AACATAT-TTTTTT-ATGTCTATCT EU569312 ---GTTTCGTTAACTATTAC-----AACATAT-TTTTTT-ATGTCTATCA AY758392 TAACGGTAGGTGAACCTGCCGTTGGATCAGTTCTAGTTTAATACCAAATT U85967 TCAGTTTCGTTAATAATTAC----AAACATAT-TTTTTTAATGTCTATAA EF165538 TCAGTTTCGTTAATAATTAC----AAACATAT-TTTTTTAATGTCTATAA AY886845 TCAGTTTCGTTAATAATTAC----AAACATAT-TTTTTTAATGTCTATAA U85966 TCAGTTTCGTTAATAATTAC----AAACATAT-TTTTTTAATGTCTATAA CTATTTATAC--AAAATTAAA-CACATAATCTAAA---AAATTTAGACCT CTATTTATAC--AAAATTAAA-CACATAATCTAAA---AAATTTAGACCT AAACATATACATAAAATTAAA--TTTTTTTTTAAAA--AATTTTAGACCT CTATTTATAC--AAAATTA-A-CACATAATCTAAC---AAATTTAGACCT CTCTTTATAC--AAAATTAAA-CACATAATCTAAA---AAATTTAGACCT CTATTTATACC-AAAATTAAA-CACATAATCTAAA---AAATTTAGACCT CTATTTATAC--AAAATTAAA-CACATAATCTAAA---AAATTTAGACCT CTCATGTATC--GATTTTATA-CACTGAATCTCAC---AA-TTTAGACCT CTATTTATAC--AAAATTAAA-CACATAATCTAAA---AAATTTAGACCT CTATTTATAC--AAAATTAAA-CACATAATCTATTC--AAATTTAGACCT CTATTTATAC--AAAATTAAA-CACATAATCTAAA---AAATTTAGACCT CTATTTATAC--AAAATTAAA-CACATAATCTAAA---AAATTTAGACCT CTATTTATAC--AAAATTAAA-CACATAATCTAAA---AAATTTAGACCT CTATTTATAC--AAAATTAAA-CACATAATCTAAA---AAATTTAGACCT CTATTTATAC--AAAATTAAA-CACATAATCTAAA---AAATTTAGACCT CTTTTTTGATA-AAACCAATACAATATAAACCTAACTTAATGTAAGGTCT CTATTTATAC--AAAATTAAA-CACATAATCTAAA---AAATTTAGACCT CTATTTATAC--AAAATTAAA-CACATAATCTAAA---AAATTTAGACCT CTATTTATACA-AAAATTAAAACATATAATCTAAA---AAATTTAGACCT CTATTTATAC--AAAATTAAA-CACATAATCTAAA---AAATTTAGACCT -TAGGCAATGGATGTCTTGGCTTCTTACACGATGAAGAACGTTGCATAAT -TAGGCAATGGATGTCTTGGCTTCTTACACGATGAAGAACGTTGCATAAT -TAGACAACGGATGTCTTGGCTCTTTACACGATGAAGAACGTTGCATAAT -TAGGCAATGGATGTCTTGGCTTCTTACACGATGAAGAACGTTGCATAAT -TAGGCAATGGATGTCTTGGCTTCTTACACGATGAAGAACGTTGCATAAT -TAGGCAATGGATGTCTTGGCTTCTTACACGATGAAGAACGTTGCATAAT -TAGGCAATGGATGTCTTGGCTTCTTACACGATGAAGAACGTTGCATAAT -TAGGCAATGGATGTCTTGGCTTCTTACACGATGAAGAACGTTGCATAAT -TAGGCAATGGATGTCTTGGCTTCTTACACGATGAAGAACGTTGCATAAT -TAGGCAATGGATGTCTTGGCTTCTTACACGATGAAGAACGTTGCATAAT -TAGGCAATGGATGTCTTGGCTTCTTACACGATGAAGAACGTTGCATAAT -TAGGCAATGGATGTCTTGGCTTCTTACACGATGAAGAACGTTGCATAAT 99 -TAGGCAATGGATGTCTTGGCTTCTTACACGATGAAGAACGTTGCATAAT -TAGGCAATGGATGTCTTGGCTTCTTACACGATGAAGAACGTTGCATAAT -TAGGCAATGGATGTCTTGGCTTCTTACACGATGAAGAACGTTGCATAAT CTAAACAATGGATGTCTTGGCTCCTCACACGATGAAGAACGTTGCATAAT -TAGGCAATGGATGTCTTGGCTTCTTACACGATGAAGAACGTTGCATAAT -TAGGCAATGGATGTCTTGGCTTCTTACACGATGAAGAACGTTGCATAAT -TAGGCAATGGATGTCTTGGCTTCTTACACGATGAAGAACGTTGCATAAT -TAGGCAATGGATGTCTTGGCTTCTTACACGATGAAGAACGTTGCATAAT GCGATAAGCGGCTGGATTAGCTTTCTTTGCGACAAGTTCGATCTTTGAAT GCGATAAGCGGCTGGATTAGCTTTCTTTGCGACAAGTTCGATCTTTGAAT GTGATAAGCGGCTAGAATTGCTTAATTTGTGATAAGTTCGATCTTTGAAT GCGATAAGCGGCTGGATTAGCTTTCTTTGCGACAAGTTCGATCTTTGAAT GCGATAAGCGGCTGGATTAGCTTTCTTTGCGACAAGTTCGATCTTTGAAT GCGATAAGCGGCTGGATTAGCTTTCTTTGCGACAAGTTCGATCTTTGAAT GCGATAAGCGGCTGGATTAGCTTTCTTTGCGACAAGTTCGATCTTTGAAT GCGATAAGCGGCTGGATTAGCTTTCTTTGCGACAAGTTCGATCTTTGAAT GCGATAAGCGGCTGGATTAGCTTTCTTTGCGACAAGTTCGATCTTTGAAT GCGATAAGCGGCTGGATTAGCTTTCTTTGCGACAAGTTCGATCTTTGAAT GCGATAAGCGGCTGGATTAGCTTTCTTTGCGACAAGTTCGATCTTTGAAT GCGATAAGCGGCTGGATTAGCTTTCTTTGCGACAAGTTCGATCTTTGAAT GCGATAAGCGGCTGGATTAGCTTTCTTTGCGACAAGTTCGATCTTTGAAT GCGATAAGCGGCTGGATTAGCTTTCTTTGCGACAAGTTCGATCTTTGAAT GCGATAAGCGGCTGGATTAGCTTTCTTTGCGACAAGTTCGATCTTTGAAT GTGATAAGTAACTGGAGTTGCGAACATTGTGACAAGTTA-ATCTTTGAAT GCGATAAGCGGCTGGATTAGCTTTCTTTGCGACAAGTTCGATCTTTGAAT GCGATAAGCGGCTGGATTAGCTTTCTTTGCGACAAGTTCGATCTTTGAAT GCGATAAGCGGCTGGATTAGCTTTCTTTGCGACAAGTTCGATCTTTGAAT GCGATAAGCGGCTGGATTAGCTTTCTTTGCGACAAGTTCGATCTTTGAAT GCACATTGCGCGCCGTTTTAGCTTGC--TAGAACACGCATATATGTTACA GCACATTGCGCGCCGTTTTAGCTTGC--TAGAACACGCATATATGTTACA GCACATTGCGTATTTAATGATTTTTAATTATTAAATACATATATTTATAA GCACATTGCGCGCCGTTTTAGCTTGC--TAGAACACGCATATATGTTACA GCACATTGCGCGCCGTTTTAGCTTGC--TAGAACACGCATATATGTTACA GCACATTGCGCGCCGTTTTAGCTTGC--TAGAACACGCATATATGTTACA GCACATTGCGCGCCGTTTTAGCTTGC--TAGAACACGCATATATGTTACA GCACATTGCGCGCCGTTTTAGCTTGC--TAGAACACGCATATATGTTACA GCACATTGCGCGCCGTTTTAGCTTGC--TAGAACACGCATATATGTTACA GCACATTGCGCGCCGTTTTAGCTTGC--TAGAACACGCATATATGTTACA GCACATTGCGCGCCGTTTTAGCTTGC--TAGAACACGCATATATGTTACA GCACATTGCGCGCCGTTTTAGCTTGC--TAGAACACGCATATATGTTACA GCACATTGCGCGCCGTTTTAGCTTGC--TAGAACACGCATATATGTTACA GCACATTGCGCGCCGTTTTAGCTTGC--TAGAACACGCATATATGTTACA GCACATTGCGCGCCGTTTTAGCTTGC--TAGAACACGCATATATGTTACA GCAAATTGCGCATACCTGAATTTATT-----CAGATGCATATATATTCTA GCACATTGCGCGCCGTTTTAGCTTGC--TAGAACACGCATATATGTTACA GCACATTGCGCGCCGTTTTAGCTTGC--TAGAACACGCATATATGTTACA GCACATTGCGCGCCGTTTTAGCTTGC--TAGAACACGCATATATGTTACA GCACATTGCGCGCCGTTTTAGCTTGC--TAGAACACGCATATATGTTACA GTAACCCATATTAATTTAATACCAAATTCTCTTTTTAAGCAAAAGAGCGA GTAACCCATATTAATTTAATACCAAATTCTCTTTTTAAGCAAAAGAGCGA GTAACCTATTTTAATTTATTAATCATTTTTTTTTTTTAAAAAATGTGAAA GTAACCCATATTAATTTAATACCAAATTCTCTTTTTAAGCAAAAGAGCGA 100 GTAACCCATATTAATTTAATACCAAATTCTCTTTTTAAGCAAAAGAGCGA GTAACCCATATTAATTTAATACCAAATTCTCTTTTTAAGCAAAAGAGCGA GTAACCCATATTAATTTAATACCAAATTCTCTTTTTAAGCAAAAGAGCGA GTAACCCATATTAATTTAATACCAAATTCTCTTTTTAAGCAAAAGAGCGA GTAACCCATATTAATTTAATACCAAATTCTCTTTTTAAGCAAAAGAGCGA GTAACCCATATTAATTTAATACCAAATTCTCTTTTTAAGCAAAAGAGCGA GTAACCCATATTAATTTAATACCAAATTCTCTTTTTAAGCAAAAGAGCGA GTAACCCATATTAATTTAATACCAAATTCTCTTTTTAAGCAAAAGAGCGA GTAACCCATATTAATTTAATACCAAATTCTCTTTTTAAGCAAAAGAGCGA GTAACCCATATTAATTTAATACCAAATTCTCTTTTTAAGCAAAAGAGCGA GTAACCCATATTAATTTAATACCAAATTCTCTTTTTAAGCAAAAGAGCGA GTACTACATCTT---TTAAT----AATTCTTCTTATAA---AAGAAGCAA GTAACCCATATTAATTTAATACCAAATTCTCTTTTTAAGCAAAAGAGCGA GTAACCCATATTAATTTAATACCAAATTCTCTTTTTAAGCAAAAGAGCGA GTAACCCATATTAATTTAATACCAAATTCTCTTTTTAAGCAAAAGAGCGA GTAACCCATATTAATTTAATACCAAATTCTCTTTTTAAGCAAAAGAGCGA AAAACA-AATATGTATTAACAAAAGGGTTCTGTCTCATATAGG--AAGAC AAAATA-AATATGTATTAACAAAAGGGTTCTGTCTCATATAGG--AAGAC AAAATTTAAAATATTTTTTTTAAAGG-TTCTTGTTTATATAGG--AAGAC AAAATA-AATATGTATTAACAAAAGGGTTCTGTCTCATATAGGGGAAGAC AAAATA-AATATGTATTAACAAAAGGGTTCTGTCTCATATAGG--AAGAC AAAATA-AATATGTATTAACAAAAGGGTTCTGTCTCATATAGG--AAGAC AAAATA-AATATGTATTAACAAAAGGGTTCTGTCTCATATAGGG-AAGAC AAAATA-AATATGTATTAACAAAAGGGTTCTGTCTCATATAGG--AAGAC AAAATA-AATATGTATTAACAAAAGGGTTCTGTCTCATATAGG--AAGAC AAAATA-AATATGTATTAACAAAAGGGTTCTGGCTCATATAGG--AAGAC AAAATA-AATATGTATTAACAAAAGGGTTCTGTCTCATATAGGG-AAGAC AAAATA-AATATGTATTAACAAAAGGGTTCTGTCTCATATAGGG-AAGAC AAAATA-AATATGTATTAACAAAAGGGTTCTGTCTCATATAGG--AAGAC AAAATA-AATATGTATTAACAAAAGGGTTCTGGCTCATATAGG--AAGAC AAAATA-AATATGTATTAACAAAAGGGTTCTGTCTCATATAGGG-AAGAC ATAACT--AAAAGCA--AACACGTAG--TCTGGGATATGTAGG--AGAAC AAAACA-AATATGTATTAACAAAAGGGTTCTGTCTCATATAGG--AAGAC AAAATA-AATATGTATTAACAAAAGGGTTCTGTCTCATATAG-------- AAAATA-AATATGTATTAACAAAAGGGTTCTGTCTCATATA--------- AAAACA-AATATGTATTAACAAAAGGGTTCTGTCTCATATAGG--AAGAC 101 APPENDIX C SEQUENCES OF FELINE ISOLATES REGISTERED IN GENBANK WITH CORRESPONDING ACCESSION NUMBERS 102 EU569301 1 CAGTTTCGTT AATAATTACA ACATATTTTT TTAATGTCTA TATCTATTTA TACAAAATTA ACACATAATC TAACAAATTT AGACCTTAGG CAATGGATGT CTTGGCTTCT TACACGATGA AGAACGTTGC ATAATGCGAT AAGCGGCTGG ATTAGCTTTC TTTGCGACAA GTTCGATCTT TGAATGCACA TTGCGCGCCG TTTTAGCTTG CTAGAACACG CATATATGTT ACAGTAACCC ATATTAATTT AATACCAAAT TCTCTTTTTA AGCAAAAGAG CGAAAAATAA ATATGTATTA ACAAAAGGGT TCTGTCTCAT ATAGGGGAAG ACCCGTACTT GCAGAAGAAG TAGCATCGTC CACCTGTGTT TCAGGGGGGG GCCACCCCCC AGGAAAGG EU569302 1 TCAGTTTCGT TAACTATGCC GTTGTATCTG TTCTCATAGC CCGGGCCTCT TTATACAAAA TTAAACACAT AATCTAAAAA ATTTAGACCT TAGGCAATGG ATGTCTTGGC TTCTTACACG ATGAAGAACG TTGCATAATG CGATAAGCGG CTGGATTAGC TTTCTTTGCG ACAAGTTCGA TCTTTGAATG CACATTGCGC GCCGTTTTAG CTTGCTAGAA CACGCATATA TGTTACAGTA ACCCATATTA ATTTAATACC AAATTCTCTT TTTAAGCAAA AGAGCGAAAA ATAAATATGT ATTAACAAAA GGGTTCTGTC TCATATAGGA AGACCCGACT TCCTGCTGAT GAAGCAGGAC CAGCCGTCTT TTGTTTAAGG GGGGGGGGCC CCCCA EU569303 1 CAGTTTCGTT AATAATTACA ACATATTTTT TTAATGTCTA TACCTATTTA TACCAAAATT AAACACATAA TCTAAAAAAT TTAGACCTTA GGCAATGGAT GTCTTGGCTT CTTACACGAT GAAGAACGTT GCATAATGCG ATAAGCGGCT GGATTAGCTT TCTTTGCGAC AAGTTCGATC TTTGAATGCA CATTGCGCGC CGTTTTAGCT TGCTAGAACA CGCATATATG TTACAGTAAC CCATATTAAT TTAATACCAA ATTCTCTTTT TAAGCAAAAG AGCGAAAAAT AAATATGTAT TAACAAAAGG GTTCTGTCTC ATATAGGAAG ACCCGTAGTT CCAGTCAAGG ACCCGCGTTC TTCTTTCTAA TGGGGGTCGC GTGTAGGCCC CTTGTTGAGT TAG EU569304 1 TCAGTTTCGT TAATTACAAA CATATTTTTT TATGTCTATA TCTATTTATA CAAAATTAAA CACATAATCT AAAAAATTTA GACCTTAGGC AATGGATGTC TTGGCTTCTT ACACGATGAA GAACGTTGCA TAATGCGATA AGCGGCTGGA TTAGCTTTCT TTGCGACAAG TTCGATCTTT GAATGCACAT TGCGCGCCGT TTTAGCTTGC TAGAACACGC ATATATGTTA CAGTAACCCA TATTAATTTA ATACCAAATT CTCTTTTTAA GCAAAAGAGC GAAAAATAAA TATGTATTAA CAAAAGGGTT CTGTCTCATA TAGGGAAGAC CCGTGTTCTG AAGCATCACT TGCTGCGGAG GCCATTTTTA CTACCTAGGA TACTCGGAGG AAGTGCCACC AAAGAAAGTA GAGTTCGTCG ACCTAATCCC CCGAGAAATG TGGTTGAGAG GCTTTTTGCC TTACGAAACT GTTCAACCGG C EU569305 1 CCCTGCCCGT TGGATCTTTT CGTTAACCGG CCTCATGTAT CGATTTTATA CACTGAATCT CACAATTTAG ACCTTAGGCA ATGGATGTCT TGGCTTCTTA CACGATGAAG AACGTTGCAT AATGCGATAA GCGGCTGGAT TAGCTTTCTT TGCGACAAGT TCGATCTTTG AATGCACATT GCGCGCCGTT TTAGCTTGCT AGAACACGCA TATATGTTAC AGTAACCCAT ATTAATTTAA TACCAAATTC TCTTTTTAAG CAAAAGAGCG AAAAATAAAT ATGTATTAAC AAAAGGGTTC TGTCTCATAT AGGAAGACCC GACCTGCTGT TGTTTCAGTT TCATCAATCA GCAGCTGTTT CAATTCGATT AGAAGAGCGC TGCTCTATTT CTGTAACATA ATGGCTATTA AAGTTTTAAA GAAGAAAGTG GGATTAGAAC AAATAAAATT TTTGGACGAG TAAGATAAGT AAAATAAGAA AGATTAGGTT TGAGTATTAA TTAAAAA 103 EU569306 1 CAGTTTCGTT AATAATTACA AAACATATTT TTTTATTGTC TATATCTATT TATACAAAAT TAAACACATA ATCTAAAAAA TTTAGACCTT AGGCAATGGA TGTCTTGGCT TCTTACACGA TGAAGAACGT TGCATAATGC GATAAGCGGC TGGATTAGCT TTCTTTGCGA CAAGTTCGAT CTTTGAATGC ACATTGCGCG CCGTTTTAGC TTGCTAGAAC ACGCATATAT GTTACAGTAA CCCATATTAA TTTAATACCA AATTCTCTTT TTAAGCAAAA GAGCGAAAAA TAAATATGTA TTAACAAAAG GGTTCTGTCT CATATAGGAA GACCCGATCT TCTGTTGTAG CAGCAGCTTC ATTAGGCTGT TGGTGATTTT TGGGAGAGGG CGCCCCCCCA GCGACG EU569307 1 GTTTCGTTAA TATTACAAAC ATATTTTTTT TTGTCTATAA CTATTTATAC AAAATTAAAC ACATAATCTA TTCAAATTTA GACCTTAGGC AATGGATGTC TTGGCTTCTT ACACGATGAA GAACGTTGCA TAATGCGATA AGCGGCTGGA TTAGCTTTCT TTGCGACAAG TTCGATCTTT GAATGCACAT TGCGCGCCGT TTTAGCTTGC TAGAACACGC ATATATGTTA CAGTAACCCA TATTAATTTA ATACCAAATT CTCTTTTTAA GCAAAAGAGC GAAAAATAAA TATGTATTAA CAAAAGGGTT CTGGCTCATA TAGGAAGACC CGA EU569308 1 GTTTCGTTAA CTGAGTGTAC AACATATATT TTTTATTGTC TATAACTATT TATACAAAAT TAAACACATA ATCTAAAAAA TTTAGACCTT AGGCAATGGA TGTCTTGGCT TCTTACACGA TGAAGAACGT TGCATAATGC GATAAGCGGC TGGATTAGCT TTCTTTGCGA CAAGTTCGAT CTTTGAATGC ACATTGCGCG CCGTTTTAGC TTGCTAGAAC ACGCATATAT GTTACAGTAA CCCATATTAA TTTAATACCA AATTCTCTTT TTAAGCAAAA GAGCGAAAAA TAAATATGTA TTAACAAAAG GGTTCTGTCT CATATAGGGA AGACCCGACC TGCTGCTGGA GCAGCTTCTT CATTACTGCT GCCGTTAATC AGGGGGGGGG GGGCCCCCAA GAG EU569309 1 AGTTTCGTTA ATAATTACAA ACATATTTTT TTAATGTCTA TAACTATTTA TACAAAATTA AACACATAAT CTAAAAAATT TAGACCTTAG GCAATGGATG TCTTGGCTTC TTACACGATG AAGAACGTTG CATAATGCGA TAAGCGGCTG GATTAGCTTT CTTTGCGACA AGTTCGATCT TTGAATGCAC ATTGCGCGCC GTTTTAGCTT GCTAGAACAC GCATATATGT TACAGTAACC CATATTAATT TAATACCAAA TTCTCTTTTT AAGCAAAAGA GCGAAAAATA AATATGTATT AACAAAAGGG TTCTGTCTCA TATAGGGAAG ACCCGTATTT ATAAGAAGGG GGGAAAAAAA AAAAATATAA AAAAAAGAGG GGGGGGGGGG CGCGCGCCCA CCATAAAATA AATTTTTATT AATTTGAAAA GTAAAAAAAA A EU569310 1 ATCAGTTTCG TTAATAGTTA CAACATATTT TTTTATTGTC TATAACTATT TATACAAAAT TAAACACATA ATCTAAAAAA TTTAGACCTT AGGCAATGGA TGTCTTGGCT TCTTACACGA TGAAGAACGT TGCATAATGC GATAAGCGGC TGGATTAGCT TTCTTTGCGA CAAGTTCGAT CTTTGAATGC ACATTGCGCG CCGTTTTAGC TTGCTAGAAC ACGCATATAT GTTACAGTAA CCCATATTAA TTTAATACCA AATTCTCTTT TTAAGCAAAA GAGCGAAAAA TAAATATGTA TTAACAAAAG GGTTCTGTCT CATATAGGAA GACCCGA 104 EU569311 1 ATCAGTTTCG TTAATAATTA CAACATATTT TTTTATGTCT ATCTCTATTT ATACAAAATT AAACACATAA TCTAAAAAAT TTAGACCTTA GGCAATGGAT GTCTTGGCTT CTTACACGAT GAAGAACGTT GCATAATGCG ATAAGCGGCT GGATTAGCTT TCTTTGCGAC AAGTTCGATC TTTGAATGCA CATTGCGCGC CGTTTTAGCT TGCTAGAACA CGCATATATG TTACAGTAAC CCATATTAAT TTAATACCAA ATTCTCTTTT TAAGCAAAAG AGCGAAAAAT AAATATGTAT TAACAAAAGG GTTCTGGCTC ATATAGGAAG ACCCGA EU569312 1 GTTTCGTTAA CTATTACAAC ATATTTTTTT ATGTCTATCA CTATTTATAC AAAATTAAAC ACATAATCTA AAAAATTTAG ACCTTAGGCA ATGGATGTCT TGGCTTCTTA CACGATGAAG AACGTTGCAT AATGCGATAA GCGGCTGGAT TAGCTTTCTT TGCGACAAGT TCGATCTTTG AATGCACATT GCGCGCCGTT TTAGCTTGCT AGAACACGCA TATATGTTAC AGTAACCCAT ATTAATTTAA TACCAAATTC TCTTTTTAAG CAAAAGAGCG AAAAATAAAT ATGTATTAAC AAAAGGGTTC TGTCTCATAT AGGGAAGACC C 105 APPENDIX D MATRIX RESULTING FROM RAPD PCR BANDING PATTERN ANALYSIS 106 1 5 sa m p l e s D1- b o v i n e 0. 0000 0. 2307 0. 6875 0. 6875 0. 800 0 0. 8000 0. 7500 0. 8125 0. 9230 0. 7500 0. 9375 1. 0 000 0. 9444 0. 8666 0. 9411 25- b o vi ne 0. 2307 0. 0000 0. 5625 0. 5625 0. 888 8 0. 8947 0. 8000 0. 8888 0. 8461 0. 8947 0. 9411 0. 8 823 0. 8888 0. 7142 0. 6428 33- b o vi ne 0. 6875 0. 5625 0. 0000 0. 0000 0. 875 0 0. 8125 0. 6363 0. 8750 1. 0000 1. 0000 0. 7692 0. 9 375 0. 9411 0. 8571 0. 6923 34- b o vi ne 0. 6875 0. 5625 0. 0000 0. 0000 0. 875 0 0. 8125 0. 6363 0. 8750 1. 0000 1. 0000 0. 7692 0. 9 375 0. 9411 0. 8571 0. 6923 36- b o vi ne 0. 8000 0. 8888 0. 8750 0. 8750 0. 000 0 0. 7857 0. 9166 0. 9333 0. 7777 0. 7857 0. 9230 0. 6 923 0. 7692 0. 8333 0. 9285 E U 569301 0. 8000 0. 8947 0. 8125 0. 8125 0. 785 7 0. 0000 0. 7272 0. 1111 0. 6666 0. 2000 0. 8461 0. 5 454 0. 4545 0. 6363 0. 9333 E U 569307 0 . 7500 0 . 8000 0 . 6363 0 . 6363 0 . 9166 0 . 7272 0 . 0000 0 . 9166 0 . 8571 0 . 9230 0 . 9000 0. 9090 0. 9166 0. 9000 0. 0000 E U 569308 0. 8125 0. 8888 0. 8750 0. 8750 0. 933 3 0. 1111 0. 9166 0. 0000 0. 7777 0. 3000 0. 8333 0. 5 000 0. 4000 0. 6000 0. 8461 E U 569309 0. 9230 0. 8461 1. 0000 1. 0000 0. 777 7 0. 6666 0. 8571 0. 7777 0. 0000 0. 6666 1. 0000 0. 5 714 0. 9000 0. 8750 0. 8888 E U 569304 0. 7500 0. 8947 1. 0000 1. 0000 0. 785 7 0. 2000 0. 9230 0. 3000 0. 6666 0. 0000 1. 0000 0. 2 222 0. 3000 0. 5000 0. 9333 T. vaginalis 0 . 9375 0 . 9411 0 . 7692 0 . 7692 0. 92 30 0. 8461 0. 9000 0. 8333 1. 0000 1. 0000 0. 0000 1. 0000 0. 9230 1. 0000 1. 0000 E U 569311 1. 0000 0. 8823 0. 9375 0. 9375 0. 692 3 0. 5454 0. 9090 0. 5000 0. 5714 0. 2222 1. 0000 0. 0 000 0. 6363 0. 7000 0. 9230 T. mobile ns is 0 . 9444 0 . 8888 0 . 9411 0 . 9411 0 . 7 692 0. 4545 0. 9166 0. 4000 0. 9000 0. 3000 0. 9230 0 . 6363 0 . 0000 0 . 6000 1 . 0000 Per i to n e a l 0. 8666 0. 7142 0. 8571 0. 8571 0. 833 3 0. 6363 0. 9000 0. 6000 0. 8750 0. 5000 1. 0000 0. 7 000 0. 6000 0. 0000 0. 9166 Giar dia 0 . 9411 0 . 6428 0 . 6923 0 . 6923 0 . 9285 0 . 9333 1 . 0000 0 . 8461 0 . 8888 0 . 9333 1 . 0000 0 . 9230 1. 0000 0. 9166 0. 0000