PYRIDOXINE (PYRIDOXAMINE) 5?-PHOSPHATE OXIDASE IN ARABIDOPSIS THALIANA 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. Yuying Sang Certificate of Approval: Robert D. Locy Narendra K. Singh, Chair Professor Professor Biological Sciences Biological Sciences Joe H. Cherry Joanna Wysocka-Diller Emeritus Professor Associate Professor Biological Sciences Biological Sciences Fenny Dane George T. Flowers Professor Dean Horticulture Graduate School PYRIDOXINE (PYRIDOXAMINE) 5?-PHOSPHATE OXIDASE IN ARABIDOPSIS THALIANA Yuying Sang 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 December 19, 2008 iii PYRIDOXINE (PYRIDOXAMINE) 5?-PHOSPHATE OXIDASE IN ARABIDOPSIS THALIANA Yuying Sang Permission is granted to Auburn University to make copies of this dissertation at its discretion, upon request of individuals of institutions and at their expense. The author reserves all publication right. Signature of Author Date of Graduation iv VITA Yuying Sang, daughter of Shiqing Sang and Guilan Wang, was born on January 7, 1975, in Chiping, Shandong, People?s Republic of China. She received the Bachelor of Science degree in Biology in July 1997 from Shandong Normal University and entered the Graduate School of Kunming Institute of Botany, Chinese Academy of Sciences. In the July of 2000, she graduated with a Master of Science degree in Botany and joined East China University of Science and Technology as a lab manager in the Department of Bioengineering. In August 2003, she enrolled in Auburn University to pursue a Doctor of Philosophy Degree in the Department of Biological Sciences. She married Daike Tian in 2000 and had their first child, Olivia Tian, in 2006. v PYRIDOXINE (PYRIDOXAMINE) 5?-PHOSPHATE OXIDASE IN ARABIDOPSIS THALIANA Yuying Sang Doctor of Philosophy, December 19, 2008 (M.S., Kunming Institute of Botany, Chinese Academy of Sciences, China, 2000) (B.S., Shandong Normal University, China, 1997) 106 Typed Pages Directed by Narendra K. Singh Vitamin B 6 is the collective term for a group of three related compounds, pyridoxine (PN), pyridoxal (PL) and pyridoxamine (PM), and their phosphorylated derivatives, pyridoxine 5'-phosphate (PNP), pyridoxal 5'-phosphate (PLP) and pyridoxamine 5'- phosphate (PMP). Many enzymes are involved in the metabolism of vitamin B6, one of which is pyridoxine (pyridoxamine) 5?-phosphate oxidase (PPOX). PPOX has been well studied from bacteria, fungi and animals, but little research about PPOX has been done in plants. In this study, two genes in the genome of Arabidopsis thaliana were found to encode for proteins that demonstrated PPOX activity: one gene is At5g49970 coding for a protein now designated AtPPOX-1, and the other gene is At2g46580 coding for a protein now designated AtPPOX-2. The cDNAs of At5g49970 and At2g46580 were cloned using vi the RT-PCR method, and then subcloned into the E. coli expression vector and subsequentely into yeast shuttle vector. PPOX functionally was demonstrated in two ways, i.e. demonstration of PPOX enzyme assay directly in vitro and by the complementation of a PDX3 (coding for yeast PPOX) knockout of yeast for increased oxidative stress susceptibility. However, the enzyme activity of AtPPOX-1 is almost 300- fold higher than that of AtPPOX-2. The inferred amino acid sequence of AtPPOX-1 is 530 amino acids long and that of AtPPOX-2 is 198 amino acids. Although AtPPOX-1 and AtPPOX-2 are putatively isoenzymes, very little homology was found in their amino acid sequences. In order to understand their evolutionary relationship, phylogenetic analysis of AtPPOX-1 and AtPPOX-2 homologs across the three domains of life suggests that AtPPOX-1 and AtPPOX-2 have independent origins. AtPPOX-1 phylogeny appears congruent with the underlying branching pattern of the overall tree of life, while AtPPOX-2 phylogeny suggests that plant PPOX-2 may have originated from cyanobacteria. Presence of Yjef_N domain in land plants AtPPOX-1 homologs suggests that acquisition of this domain and its fusion with pyridox_oxidase domain began with the endosymbiotic acquisition of the chloroplast. In this study, regulation of the AtPPOX-1 gene and its in vivo physiological functions were investigated. Variable levels of expression of AtPPOX-1 were seen in all tissues of A. thaliana examined. This gene is up-regulated by light, heat shock, ABA, JA and ethylene treatment, and down-regulated by exposure to NaCl. AtPPOX-1 may have two alternative splicing variants. One is expressed in all tissues, but the other is not expressed in root. To determine the biological role of AtPPOX-1, T-DNA insertional vii mutants of A. thaliana in AtPPOX-1 were analyzed. The mutant lines showed sensitivity to NaCl and high light for growth, and sensitivity to high concentrations of sucrose in cotyledon development. These results suggest involvement of AtPPOX-1 in stress tolerance and cotyledon development in A. thalia viii ACKNOWLEDGEMENTS I would like to express my gratitude to Drs. Narendra Singh, Robert Locy, Joe Cherry, Joanna Wysocka-Diller, and Fenny Dane for their guidance and assistance during my graduate studies. My major advisor, Dr. Singh, impressed me in many ways. Not only did he teach me how to do research, but he also taught me how to be a person. He is the nicest person I have ever met. Dr. Locy?s full of knowledge and ideas, always provided me with good suggestions whenever I met problems in the research. I am also grateful for the help from Dr. Leslie Goertzen for his assistance with the phylogenetic analysis. Thanks are due to Dr. Roland Dute who instructed me on how to do immunohistochemistry and allowed me to work in his lab, and also to Dr. Michael Miller who mentored me in immunocytochemisty. As a lab technician and my friend, Ms. Chia- chen Weng gave me much support that assured my experiments moved on smoothly. My labmate, Dr. Nisreen AL-Quareen, also gave me help during my studies. I would like to give many thanks to all other persons in the Biology Department in Auburn University. My parents, Shiqing Sang and Guilan Wang, my sisters, and my husband, Daike Tian, gave me great support throughout my graduate studies. I can not finish my degree without their selfless help. ix Style manual or journal used: Plant Physiology Computer software used: Microsoft Word 2003 Microsoft Excel 2003 Sigma Plot 2000 Adobe Photoshop Paup x TABLE OF CONTENTS LIST OF TABLES..............................................................................................................xi LIST OF FIGURES...........................................................................................................xii I. LITERATURE REVIEW.................................................................................................1 Vitamin B 6 .....................................................................................................................1 Functions of Vitamin B 6 ................................................................................................2 Effects of deficiency and overdose of vitamin B 6 .........................................................7 Biosyntheic pathway of vitamin B 6 ...............................................................................7 Transport of vitamin B 6 ...............................................................................................13 Pyridoxine phosphate oxidase activity.........................................................................14 II. IDENTIFICATION OF ATPPOX-1 FROM ARABIDOPSIS THALIANA ...................20 Abstract ........................................................................................................................20 Introduction..................................................................................................................21 Results and Discussion ................................................................................................23 Materials and Methods.................................................................................................26 III. IDENTIFICATION OF ATPPOX-1 FROM ARABIDOPSIS THALIANA .................33 Abstract ........................................................................................................................33 Introduction..................................................................................................................34 Results..........................................................................................................................35 Discussion....................................................................................................................37 Materials and Methods ................................................................................................38 xi IV. EVOLUTIONARY ANALYSIS OF ATPPOX-1 AND ATPPOX-2 FROM ARABIDOPSIS THALIANA............................................................................................44 Abstract........................................................................................................................44 Introduction..................................................................................................................45 Results..........................................................................................................................46 Discussion....................................................................................................................48 Materials and Methods...............................................................................................50 V. FUNCTIONAL ANALYSIS OF ATPPOX-1 FROM ARABIDOPSIS THALIANA.....58 Abstract ........................................................................................................................58 Introduction..................................................................................................................59 Results..........................................................................................................................61 Discussion ....................................................................................................................62 Materials and Methods.................................................................................................65 REFERENCES ..................................................................................................................81 xii LIST OF TABLES II. 1. PNP/PMP oxidase activities of the purified recombinant proteins........................29 IV. 1. AtPPOX-1 homologs used in the unrooted neighbor joining tree..........................51 2. AtPPOX-1 homologs used in the unrooted neighbor joining tree ..........................53 xiii LIST OF FIGURES II. 1. Amino acid sequence alignment of AtPPOX-1 and yeast PDX3......................30 2. SDS-PAGE of recombinant AtPPOX protein of different lengths separated on a 12.5% gel...........................................................................................................31 3. Complementation of YBR035C under oxidative stress with AtPPOX constructs.........................................................................................................32 III. 1. SDS-PAGE of recombinant AtPPOX-2 protein of different lengths separated on a 12.5% gel.......................................................................................................41 2. PPOX activity of the purified recombinant AtPPOX-1 and AtPPOX-2...............42 3. Complementation of YBR035C under oxidative stress with AtPPOX-2..........43 IV. 1. Amino acid sequence alignment between AtPPOX-1 and AtPPOX-2...........54 2. Conserved regions among all AtPPOX-1 and AtPPOX-2 homologs..............55 3. AtPPOX-1 homolog derived tree .....................................................................56 4. AtPPOX-2 homolog derived tree......................................................................58 V. 1. Determination of optimal amplification cycle duringRT-PCR.........................73 2. Expression of AtPPOX-1 in different tissues of A. thaliana............................73 3. Different forms of AtPPOX-1 and their localization .......................................74 4. Native Basic PAGE in-gel assay for AtPPOX-1 enzyme activity....................75 5. Regulation of AtPPOX-1 by environmental and hormone factors ...................76 6. Phenotype of CS825697 seedlings grown on MS agar with 100mM sucrose..77 7. Sensitivity of CS825697 to NaCl......................................................................78 8. Response of wild type and CS825697 to high light exposure ..........................80 1 I LITERATURE REVIEW VITAMIN B 6 Vitamins are organic compounds required in tiny amounts for essential metabolic reactions in living organisms (Lieberman, 1990). Human need 13 vitamins of which 4 (A, D, E and K) are fat-soluble and 9 (8 B vitamins and vitamin C) are water-soluble. Vitamin B 6 is a collective term used to describe pyridoxal, pyridoxine, pyridoxamine and their respective 5?-phosphorylated forms: pyridoxine 5'-phosphate (PNP), pyridoxal 5'-phosphate (PLP) and pyridoxamine 5'-phosphate (PMP) (http://www.chem.qmul.ac.uk /iupac/misc/B6.html). The chemical entity present at the 4? position of the pyridine ring defines the different vitamers, which can be an aldehyde (pyridoxal), an alcohol (pyridoxine) or an amine (pyridoxamine). Phosphorylation of 5?- position forms their corresponding phosphorylated forms as shown below. A ubiquitous bound form of PN, 5?-O-(-D-glucopyranosyl)-pyridoxine, abbreviated as PN-glucoside is found in many plant tissues. It has been reported that 60-90% 2 of the B 6 vitamers contained in certain foods are in the form of PN-glucoside (Gregory and Nakano, 1997; Gregory and Sartain, 1991). PN-glucoside partially impairs the metabolic utilization of co-ingested non-glycosylated forms of vitamin B 6 (Gilbert and Gregory 1992), because it uses the same transport system as pyridoxine (Zhang and Mccormick, 1992). Upon entry into the cell, PN-glucoside undergoes hydrolysis to release pyridoxine, which is the rate limiting step in metabolism of this ?-glucoside (Zhang and Mccormick, 1993). FUNCTIONS OF VITAMIN B 6 Vitamin B 6 is an essential metabolite for all organisms and plays important role in the regulation of many metabolic activities in the cell. Vitamin B6 is well known for its role as cofactor of many enzymes. PLP-dependent enzymes catalyze over 100 enzymatic reactions, predominantly in amino acid metabolism including transamination, decarboxylation, racemization, C?-C? bond cleavage and ?, ?- elimination reactions (Eliot et al., 2004; Drewke et al., 2001; John R, 1995; Fitzpatrick et al., 2007). In its role as a coenzyme, PLP is bound tightly to the apoenzyme by a Schiff base (aldimine) linkage formed through condensation of the 4-carbonyl group with the ?-amino group of specific lysine residues. The resultant Schiff base compound may be subject to nucleophilic attack by a neighboring amino, sulfydryl, or imidazole group to form a substituted aldamine (Ball GF, 2006). All vitamers of vitamin B 6 are reversibly bound and easily dissociate from the apoenzymes. Recent interest in vitamin B 6 study has increased because of its potential antioxidant properties. While studying mechanisms of resistance of Cercospora nicotianae to singlet- 3 oxygen-generating phytotoxins, it was found that the resistance was dependent upon the expression of a gene essential for synthesis of vitamin B 6 (Ehrenshaft et al., 1999). Comparable to vitamin C and E, vitamin B 6 and its derivatives are efficient quenchers of singlet oxygen ( 1 O 2 ), a strong oxidizer that initiates radical oxidation in biological systems (Bilski et al., 2000). Vitamin B 6 and its derivatives are converted to endoperoxide and hydroperoxide intermediates in the reaction of vitamin B 6 with 1 O 2 (Ohta and Foote, 2002). Vitamin B 6 has been linked to oxidative stress in diverse organisms. Antioxidant effect of vitamin B 6 on Schizosaccharomyces pombe cells treated with menadione is due to reduction of glutathione content. This reduction in turn suppressed an increase in peroxide and thiobarbituric acid reactive substances, and increased the viability of the yeast cells under oxidative stress (Chumnantana et al., 2005). Pyridoxine/pyridoxamine 5?-phosphate oxidase knockout mutant in Saccharamyces cerevisiae is sensitive to H 2 O 2 stress (Sang et al, 2007). Involvement of vitamin B6 has been shown in oxidative stress abatement. Mechanisms underlying its function in this complex process require more investigation (Jain and Lim, 2001). Vitamin B 6 may function as a regulator of a number of membrane ion transporters. The enhanced influx of calcium ions into an intracellular compartment of the vascular smooth muscle resulting in hypertension in rat could be blocked by PLP and by dihydropyridine-sensitive calcium channel blockers (DHP), suggesting that PLP could be an endogenous modulator of DHP ? sensitive calcium channels (Dakshinamurti et al., 1998). In addition, vitamin B 6 has been linked to modulation of hormone function because of its ability to bind to steroid receptors (Oka T, 2001), and through modulation 4 of transcription factors by PLP conjugation to transcriptional coregulators (Mostaqul et al., 2007). Because of the essential functions of vitamin B 6 in all organisms, many efforts have been directed into its potential use in curing some diseases in humans. There is growing evidence that vitamin B 6 suppresses colon tumorigenesis by reducing cell proliferation, oxidative stress, NO production and angiogenesis (Komatsu et al., 2003). PLP and PL act as a lipid glycation inhibitors, which presumably contributes to diabetes prevention (Higuchi et al., 2006). Type 2 diabetic patients have an abnormal increase of phosphatidylcholine hydroperoxide (PCOOH) (Nagashima et al., 2002). PCOOH may be related to Amadori-glycated phosphatidylethanolamine (Amadori-PE) which generates reactive oxygen species and thereby triggers lipid peroxidation (Oak et al., 2000). PLP and PL could easily be condensed with PE before the glucose/PE reaction occurred (Higuchi et al., 2006). Advanced glycation end products (AGEs) and advanced lipoxidation end products (ALEs) are implicated in many age-related chronic diseases and in protein aging. PM is not only an inhibitor of AGEs, but also inhibits ALEs by trapping malondialdehyde (MDA) directly under physiological conditions, and provides insight into the mechanism of action of PM in protecting proteins against carbonyl stress (Onorato et al., 2000; Kang et al., 2006). PLP has also been implicated as a precursor of vitamin B 1 (thiamine) biosynthesis in yeast (Zeidler et al., 2002). The pyrimidine unit of thiamin (Vitamin B1) originates from a C5N fragment, derived from C-2',2,N,C-6,5,5' of pyridoxol (Vitamin B 6 ) and an N-C-N fragment derived from L-histidine. Urocanic acid serves as an intermediate in the 5 insertion of the N-C-N fragment of histidine into the thiamin pyrimidine (Zeidler et al., 2003). PLP is synthesized in plants using the DXP-independent biosynthesis pathway in which Pdx1 and Pdx2 proteins are involved (Studart et al., 2005 ). Genes encoding PDX1 have been identified in several plant species, and their functions are extensively studied (Shi et al., 2002; Chen and Xiong, 2005; Studart et al., 2005; Titiz et al., 2006; Wagner et al., 2006; Studart et al., 2007). PDX1 is required for shoot and root development. Arabidopsis pdx1 knockout mutants were impaired in root growth and early seedling development (Chen and Xiong, 2005). In addition to the developmental defects, PDX1 mutants are hypersensitive to salt, osmotic stress and oxidative stress (Chen and Xiong, 2005). These mutant seedlings had increased peroxidation of membrane lipids following UV treatment. These studies establish a critical role of vitamin B6 in plant development and stress tolerance and suggest that vitamin B 6 may represent a new class of antioxidant in plants (Chen and Xiong, 2005; Titiz et al., 2006;Wagner, et al., 2006 ). No homozygous plants could be obtained for pdx2 T-DNA insertion mutants, suggesting that PDX2 is involved in the seed development (Studart et al., 2005). Pdx1 and pdx2 are regulated by stressors, such as high light, chilling, drought, ozone and plant pathogen, which cause oxidative stress indirectly (Denslow et al., 2005; Denslow et al., 2007). These results support a role for vitamin B 6 as an antioxidant and modulator of active oxygen species in vivo. Pyridoxal kinase catalyzes the phosphorylation of the vitamin B 6 vitamers to form the corresponding phosphorylated derivatives (Lum et al., 2002). It is involved in the salvage pathway of the vitamin B 6 biosynthesis. Root growth of A. thaliana SOS4 mutant 6 encoding pyridoxal kinase is slower than that of the wild type, and the mutants do not have root hairs in the maturation zone, suggesting that pyridoxal kinase is required for root hair development in Arabidopsis (Shi and Zhu 2002). But how the pyridoxal kinase affects the root hair development was not explained. Shi et al. (2002) have also demonstrated that pyridoxal kinase is a salt tolerance determinant important for the regulation of Na + and K + homeostasis in plants, and proposed that PLP regulates Na + and K + homeostasis by modulating the activities of ion transporters. Pyridoxamine (pyridoxine) 5?-phosphate oxidase (PPOX), converting PMP and/or PNP to PLP, is another enzyme involved in the salvage pathway. Loss of PPOX activity seriously disrupts cellular metabolism in several ways, with particular effects on amino acid metabolism. In E. coli, excretion of L-glutamate and possibly ?- ketoisovalerate, which triggers L-valine inhibition, were shown (Lam and Winkler, 1992). In Saccharomyces cerevisiae, pleiotropic phenotypes induced by lack of PPOX activity include strong perturbations in amino acid biosynthesis, atypic fatty acid, sterol and cytochrome patterns, and sensitivity to H 2 O 2 stress (Loubbardi et al., 1995). The PPOX mutants of Arabidopsis showed decreased growth in root and shoot under normal conditions, and were incapable of increased growth under high light conditions (Gonzalez et al., 2007). However, physiological functions of PPOX in plant growth and development have not been fully determined. 7 EFFECTS OF DEFICIENCY AND OVERDOSE OF VITAMIN B 6 Humans and animals can not synthesize vitamin B 6 themselves and must obtain it from dietary sources (http://en.wikipedia.org/wiki/vitamin_B6). Either deficiencies or overdoses of vitamin B 6 are known to cause serious problems (Dakshinamurti K., 1990). The classic clinical syndrome for B 6 deficiency is a seborrheic dermatitis-like eruption, atrophic glossitis with ulceration, angular cheilitis, conjunctivitis, intertrigo, and neurologic symptoms of somnolence, confusion, and neuropathy (James et al., 2006; http://en.wikipedia.org/wiki/vitamin_B6). Vitamin B 6 is an important growth factor in rats; a deficiency causes a marked acrodynia type of dertermatitis (Emerson et al., 1938). An overdose of pyridoxine from vitamin B 6 supplements, although never from food source, can cause a temporary deadening of certain nerves such as the proprioceptory nerves, causing a feeling of disembodiment common with the loss of proprioception (http://dietary-supplements.info.nih.gov/factsheets/vitaminb6.asp). This condition is reversible when vitamin B 6 supplementation is stopped. Very high doses of pyridoxine over long periods of time may result in painful neurological symptoms known as sensory neuropathy (Pfeiffer et al., 1995). BIOSYNTHETIC PATHWAY OF VITAMIN B 6 Bacteria, fungi, and plants are able to synthesize the vitamin B6 de novo, but humans and animals must acquire it through their diet. Two distinctive pathways for its de novo synthesis have been identified to date. These are the deoxyxylulose 5-P (DXP)- dependent pathway and the DXP-independent pathway (Franco et al., 2003; Fitzpatrick et 8 al., 2007). DXP-dependent pathway seems to be restricted to the ? subdivision of protobacteria, while DXP-independent pathway appears to be present in fungi, plants, and other bacteria (Salvo et al., 2003). Deoxyxylulose 5-P (DXP)-dependent pathway The vitamin B 6 biosynthesis pathway has been extensively studied in E. coli where PNP is derived from 4-(phosphohydroxy)-L-threonine and 1-deoxy-D-xylulose-5- phosphate (Laber et al., 1999). It was assumed for a long time that vitamin B 6 is synthesized in the same way in all organisms. However, the deoxyxylulose 5-P (DXP)- dependent pathway has now been shown to be generally limited to the gamma-branch of proteobacteria (Flicker et al., 2005; Mittenbuber 2001)), in which two branches with six enzymatic steps are involved (Fitzpatrick et al., 2007) as shown below in Scheme 1. In one branch, Epd, PdxB and SerC catalyze the conversion of D-erythrose 4-phosphate into phospho-hydroxy-threonine (Lam and Winkler, 1990; Yang et al., 1998) which then undergoes oxidation and decarboxylation by PdxA to form 3-hydroxy-1-aminoacetone phosphate (Banks and Cane, 2004; Cane et al., 1998). In the other branch, DXP is derived from glyceraldehyde 3-phosphate and pyruvate by the action of DXP synthase (Sprenger et al., 1997). The products of the two branches, i.e. 3-hydroxy-1-aminoacetone phosphate and DXP, are then condensed in a reaction catalyzed by PdxJ to form PNP (Laber et al., 1999). PNP is oxidized into the cofactor vitamer PLP by PdxH. 9 Deoxyxylulose 5-P (DXP)-independent pathway It has been shown that a large majority of organisms synthesize vitamin B 6 via a completely different pathway from E. coli and the rest of the gama-proteobacteia (shown in Scheme 2). In this pathway, PLP is synthesized directly from either ribose 5- phosphate or ribulose 5-phosphate, in combination with either glyceraldehyde 3- phosphate or dihydroxyacetone phosphate, and glutamine as the nitrogen (N) donor (Burns et al., 2005; Raschle et al., 2005). Pdx1 and Pdx2 are the key enzymes involved in the DXP-independent pathway. Neither of these enzymes show similarity to any of those involved in the DXP-dependent pathway (Ehrenshaft et al,. 1999; Ehrenshaft et al., 2001; Studart et al., 2005). Pdx1 protein was found to be one of the most evolutionarily Scheme 1. Vitamin B 6 biosynthesis by the DXP-dependent pathway. D-erythrose-4phosphate Erythrose 4-phosphate Dehydrogenase ( epd ) erythronate-4-phosphate Erythronate 4-phosphate Dehydrogenase ( pdxB ) 3-hydroxy-4-phospho-hydroxy-?-ketobutyrate Phosphohydroxythreonine transaminase ( serC ) phospho-hydroxy-threonine Dehydrogenase/decarboxylase ( pdxA ) 3-hydroxy-1-amino acetone phosphate 1-deoxy-D-xylulose 5-phosphate D-glyceraldehyde-3-phosphate pyruvate 1-deoxyxylulose-5-phosphate synthase ( dxs ) Pyridoxine-5?-phosphate Pyridoxine 5?-phosphate synthase ( pdxJ ) 10 conserved proteins (Braun et al., 1995). Pdx2 protein is less well conserved but contains several protein motifs that are conserved throughout all Pdx2 proteins (Ehrenshaft et al., 2001). Pdx1 and Pdx2 proteins interact with each other resulting in a functional PLP synthase complex that functions as a glutamine amidotransferase, with the Pdx2 protein as the glutaminase domain and Pdx1 as the acceptor and PLP synthase domain (Belitsky BR, 2004; Dong et al., 2004). Scheme 2. Vitamin B 6 biosynthesis by the DXP-independent pathway. Salvage pathway Most organism possess a vitamin B 6 biosynthesis salvage pathway that interconverts and recycles the various vitamers of pyridoxine. Organisms that do not have the de novo pathway of vitamin B 6 biosynthesis need to acquire vitamin B 6 from their diet, and then interconvert the vitamin B 6 vitamers via this salvage pathway into the active coenzyme (PLP) (Tsuyoshi et al., 2004). Although there is divergence in the de novo synthesis pathway of pyridoxine, the salvage pathway appears to be conserved (as shown in scheme 3). In this pathway, pyridoxine, pyridoxal and pyridoxamine can be reversibly phosphorylated and dephosphorylated through the action of specific kinases (PdxK and glutamine Pdx2 NH3 Pyridoxal 5?-phosphate Ribose 5-phosphate Ribulose 5-phosphate Glyceraldehyde 3-phosphate Dihydroxyacetone phosphate Pdx1 11 PdxY) and apparently unspecific phosphatases respectively (Yang, 1996; Yang, 1998). However, a specific phosphatase has been reported in humans (Fonda, 1992; Jang et al., 2003). Furthermore, PNP or PMP can be converted into PLP by the action of the oxidase PdxH (Zhao and Winkler, 1995), which is included in the de novo pathway of vitamin B 6 biosynthesis by the DXP-dependent route. In addition, a pyridoxal reductase has been identified in yeast (Nakano et al., 1999). It is assumed that the majority of organisms have one or the other of these enzymes. Scheme 3. Vitamin B 6 biosynthesis by the salvage pathway Evolutionary perspectives of the two independent pathways The DXP-dependent pathway is restricted to the ?-division of proteobacteria. It has been suggested that, because the ?-division of proteobacteria is thought to represent the Pyridoxine Phosphate Pyridoxal Phosphate Pyridoxamine Phosphate PdxH PdxK Plr1 Pyridoxine glucosyl transferase Pase* PdxK PdxK PdxH Pyridoxine beta-glucosidase DXP-dependent pathway DXP-independent pathway Pase * Pase * Pyridoxine Pyridoxal Pyridoxamine 5?-O-(beta-D-glucopyranosyl) pyridoxine Tase * 12 most recent lineage of prokaryotic evolution, the genes of the ancestral Pdx1/Pdx2 pathway were lost during evolution of the proteobacteria and PdxA/PdxJ pathway evolved in this lineage (Mittenbuber, 2001). The reason for the loss of the Pdx1 and Pdx2 genes is unknown. However, there is the hypothesis that there may have been a time during the evolution of the ?-division of proteobacteria where uptake of the vitamin from the environment was selected for and the Pdx1 and Pdx2 genes became dispensable. Then the Pdx1/Pdx2 genes might have been lost without deleterious consequences. Later, it became necessary to produce the vitamin de novo leading to ?reinvention? of the synthesis of the pyridoxine ring (Fitzpatrick et al., 2007). Fitzpatrick et al. (2007) also did comparison between the two independent routes to the biosynthesis of vitamin B6. Supprisingly, it was found that the key biosynthetic enzymes of both pathways are, in fact, very similar both structurally and mechanistically. TRANSPORT OF VITAMIN B 6 Transport of vitamin B6 has been mostly studied in mammals, yeast and bacteria. However, there is no information available about the transport of vitamin B 6 in plants. Mammals are auxotrophic for vitamin B 6 and must acquire it from their diet. Liver and intestine are very active in the metabolism of B 6 vitamers. In the intestinal lumen, the dietary phosphorylated vitamin B 6 is hydrolyzed into dephosphorylated forms. PL, PM and PN are then absorbed by passive diffusion (Hamm et al. 1979). However, PL is the only form transported in the blood (Sakurai et al., 1991). The absorbed PM and PN are rapidly acted on by PL kinase and then converted to PLP by pyridoxine (pyridoxamine) 13 5?-phosphate oxidase (PPOX) (Ink SL, 1984). These two enzymes plus phosphohydrolase provide a means of converting dietary PN and PM to circulating PL which is then taken up and phosphorylated into PLP by other organs that contain pyridoxal kinase (Sakurai et al., 1987; Sakurai et al., 1991). Unlike mammals, yeast is prototrophic for vitamin B 6 , but in vitamin B 6 auxotrophic mutants, uptake of PN, PL, or PM from the extracellular space is required to generate intracellular PLP via a salvage pathway. Vitamin B 6 transport has been intensively studied in S. carlsbergensis, in which two distinct uptake systems that differ in structural specificity and ionic requirements are present. System 1 has affinity for PL and PN and a pH optimum of 3.5, whereas system 2 is specific for PM and PN and has a pH optimum of 6.0 (Shane and Snell, 1976). For S. cerevisiae, Tpn1p was found to be the only functional transport protein for vitamin B6 encoded in the genome. This protein was also shown to mediate the uptake of PL, and to a lesser extent, PM. The activity of Tpn1p is very similar to that of system 1 and the protein that corresponds to system 2 of S. carlsbergensis is not known. Moreover, S. carlsbergensis contains a protein that is almost identical to Tpn1p and thus is very likely to function in PN uptake (Stolz and Vielreicher, 2003). No transport protein for vitamin B 6 has ever been found in bacteria. Salmonella typhimurium can transport PN and PL with the K m values of 2.0 x 10 -7 M and 1.2 x 10 -7 M, respectively, but this bacteria can not transport pyridoxamine (Mulligan and Snell, 1976). However, a vitamin B 6 auxotroph derived from E. coli K12, utilized the three unphosphorylated forms of vitamin B 6 , more or less effectively, for growth (Yamada et al., 1977; Mulligan and Snell, 1977). 14 PYRIDOXINE/PYRIDOXAMINE 5?-PHOSPHATE OXIDASE ACTIVITY PPOX catalyzes the oxidation of either PNP or PMP into PLP, with FMN as its cofactor and oxygen as the final electron acceptor. During the oxidation, a hydrogen atom is removed from the C4? alcohol group of PNP or amino group of PMP, and a pair of electrons is transferred to tightly bound FMN, forming PLP and FMNH 2 . PLP contains a very reactive aldehyde group that reacts with virtually all nucleophiles in the cell. How is PLP protected in the cell from adventitious reactions with non-productive nucleophiles? PPOX is a kinetically sluggish but moderately abundant enzyme in E. coli. It contains a non-catalytic PLP binding site and a catalytic PLP binding site (Zhao and Winkler, 1995; Yang and Schirch, 2000). PLP dissociates very slowly from the non-catalytic PLP binding site, and this slowly dissociating PLP can be readily transferred to the PLP requiring apoenzyme to form the active holoenzyme. Safo et al. (2001) proposed that a possible tunnel exists between the two sites so that PLP formed at the active sites may transfer to the non-catalytic site without passing through the solvent. However, there is no report about how the non-catalytic binding PLP is transferred to the PLP requiring apoenzymes. PPOX from different organisms PPOX was first isolated and purified from rabbit liver (Kazarinoff et. al., 1975). Subsequently, the enzyme was purified from sheep and pig brain (Choi and Churchich, 1987). Wheat seedlings were reported to have at least three PPOX enzymes, but only two 15 of them were partially purified (Tsuge et. al., 1982). PPOX from E. coli, and A. thaliana was overexpressed and purified from E. coli (Salvo et al., 1998; Sang et al., 2007). Both the prokaryotic and eukaryotic Pyridoxine 5?-phosphate oxidases are homodimers. The two identical monomers are held together via disulfide bonds as well as salt-bridge interactions. Each subunit tightly binds one molecule of PLP and one molecule of FMN as a cofactor (Kazarinoff et al., 1975; Choi et al., 1983; Zhao et al., 1995; Salvo et al., 1998). Most extensive biochemical studies have been carried out with the PPOX from rabbit liver and E. coli., and their kinetic constants for the oxidation reaction catalyzed by PPOX have been determined . PPOX of E. coli has the K m of 2 ?M for PNP at 37 ?C and pH 8.5 and the K cat of 0.76 s -1 . Whereas K m for PMP is higher around 105 ?M and K cat value is 1.72 s -1 (Zhao and Winkler, 1995; Salvo, et al., 1998). For the enzyme from rabbit liver, kinetic constants are quite similar for the two substrates (K m = 8 ?M, K cat = 0.7 s -1 for PNP; K m = 6?M, K cat = 0.1 s -1 for PMP (Choi et al., 1983). The PMP oxidase activity of the PPOX from E. coli showed a sharp pH profile. The PMP oxidase enzyme activity was absent at pH 6, rose sharply as the pH increased from 6 to 8.5, and then remained nearly constant at pH values between 8.5 and 10. In contrast, the PNP oxidase activity showed a very broad pH profile. PNP is by far the better substrate for the PPOX from E. coli at pH?s above 8.0, whereas PPOX from rabbit liver oxidizes both substrates to almost the same extent. Below pH 8.0, PNP is by far the better substrate for both E. coli and rabbit liver PPOX. Because the aminomethyl group of PMP is largely protonated 16 below pH 9.0, the unprotonated group is attacked preferentially by the enzyme (Wada and Snell, 1961). The PPOX is relatively thermal stable at high pH, and easily loses its activity at lower pH (Zhao and Winkler, 1995; Wada and Snell, 1961). Mechanistic pathway of the PPOX The mechanistic pathway of PPOX on a molecular level is: from the resting enzyme with no substrate bound, to the initial binding of PNP at the active site (pre-reaction state), to the catalytic stage and finally to the transfer of the catalytic product PLP from the active site to the PLP binding site for subsequent transfer to vitamin B 6 apoenzyme (Safo et al, 2005). In the absence of PLP, the active site of the enzyme is in an ?open? conformation. Once substrate binds and is converted to PLP, the active site of the enzyme is in a partially ?closed? conformation. Specific amino acid residues can form hydrogen bonds with the PLP, thus forming a lid that physically covers the active site, giving rise to the ?closed? conformation (Yang and Schirch, 2000; Safo et al, 2001). Once the PLP is transferred to the binding site, the active site is open and ready for the next substrate. Regulation of PPOX Substrate inhibition was observed using PNP as substrate, with a K i of 50 ?M, and was partially relieved by increasing O 2 concentration (Choi et al., 1983). Substrate inhibition seemed to occur by binding of PNP to the reduced form of the enzyme, forming an abortive complex. On the other hand, no substrate inhibition was observed for PMP oxidase activity (Zhao and Winkler, 1995). PLP is a very strong competitive inhibitor of the oxidase in both E. coli and mammals. PLP and PLP analogs were shown 17 to inactivate PPOX by binding to a specific lysine residue in the active site of the dimeric form of the protein (Choi et al., 1987). Sheep brain PPOX is activated by tryptophan metabolites 3-hydroxyanthranilate and 3-hydroxykynurenine which bind to a regulatory domain distinct from the catalytic site. The structural domain with full catalytic activity composes approximately one-half of the molecular mass of PPOX, whereas the remaining portion contains the regulatory binding site (Kwon et al., 1991). Low concentrations of urea yield a rapidly formed ?activated? species of the oxidase that is changed primarily at the active site in a manner that allows increased dissociation of substrate and product (Horiike et al., 1979). Characteristics of PPOX in Arabidopsis thaliana Only one PPOX protein has been reported in bacteria, yeast or animals (Salvo et al, 1998; Choi et al., 1983; Kazarinoff et al., 1975; Zhao and Winkler, 1995). However, wheat seedlings have at least three PPOX proteins, and two of these show PPOX activity (Tsuge et al., 1982). One isozyme was relatively more specific for PNP than PMP (9.22:1) and the other one was somewhat less specific (1.58:1) (Tsuge et al., 1982). One PPOX activity and the gene encoding this activity was identified in Arabidopsis thaliana (Sang et al., 2007). This PPOX can use both PNP and PMP as substrates, but with higher Km value for PNP than for PMP (Sang et al., 2007). The subunit of PPOX from bacteria, yeast and animals has 200-300 amino acids, which contains only a pyridox_oxidase domain. However PPOX from Arabidopsis thaliana is 530 amino acids long and has both a pyridox_oxidase domain and Yjef_N domain (Sang et al., 2007). Yjef_N domain exists widely in organisms. It is very well conserved, but its function is still not known. 18 The Yjef_N domain is fairly conserved across the three principal superkingdoms of life. It exists either as a single protein, or fused with other domains. A single copy of the Yjef_N domain is traceable to the last universal common ancestor of all life forms. Proteins with both Yjef_N domain and other domains can be found in archea, bacteria, fungi, plant, animals, and human. In bacteria the Yjef_N domain is often found fused to a C-terminal kinase domain of the ribokinase superfamily, which suggests that the ancestral form of the Yjef_N domain may have functioned in the metabolism of a critical low molecular weight compound. Given that kinase domains are often fused to different phosphoesterase (phosphatase) domains, it is possible that the Yjef_N-type Rossman fold domains may also catalyze this reaction. The conservation of the acidic residues in the predicted active site of the Yjef_N domains is reminiscent of such residues in the active sites of diverse hydrolases. Thus, in the context of the decapping pathway, it is possible that the Yjef_N domains of Dcp3p and FLJ21128 catalyze hydrolytic RNA-processing reactions, such as, phosphoester hydrolysis, dephosphorylation, demethylation or glycosyl bond hydrolysis ( Anantharaman and Aravind, 2004). The screening for additional human YjeF_N domain containing proteins beside the apolipoprotein A-I interacting protein (AI-BP), identified two other genes designated hYjeF_N2-15q23 (formerly human homologue of yeast edc3) and hYjeF_N3-19p13.11 comprising the human YjeF_N family. Immunohistochemistry of human testes and ovaries showed an expression of hYjeF_N3-19p13.11 only in Leydig cells and theca cells, respectively, indicating a role in steroid hormone metabolism. Interestingly, the protein was also strongly expressed in Leydig cell tumors and in thecofibromas. The 19 identification of hYjeF_N2-15q23 in theca cells and granulosa cells in ovaries, in human spermatids of meiotic division part II and the apical membrane of Sertoli cells in testes suggest similar functions in oogenesis and sperm maturation which is strengthened by the identification of the spermatogenesis regulator HMGA1 as a conserved transcription factor. However, in contrast to AI-BP, both homologous proteins are unable to bind apoA-I. These results relate the human YjeF_N domain containing protein family to cholesterol processing and steroid hormone metabolism in spermiogenesis and oogenesis, and AI-BP may link this function to the HDL pathway (Rudolph et al., 2007). Question mark for PPOX All PPOX identified thus far need oxygen as the final electron acceptor. The question is how PNP oxidization to PLP occurs in anaerobically growing cells in which the PPOX presumably does not work. Two possibilities have been suggested (Salvo, et al., 2003). One possibility is that there is a single form of PdxH oxidase in wild-type E. coli, which uses oxygen aerobically and another electron acceptor anaerobically. A second possibility is that there is a second PPOX that functions under anaerobic conditions, but PdxH protein is required for expression or activation of this second anaerobic form of PPOX. 20 II IDENTIFICATION OF ATPPOX-1 FROM ARABIDOPSIS THALIANA ABSTRACT Pyridoxine (Pyridoxamine) 5?-phosphate oxidase (PPOX) catalyzes the oxidative conversion of pyridoxamine 5?-phosphate (PMP) or pyridoxine 5?-phosphate (PNP) to pyridoxal 5?-phosphate (PLP). The At5g49970 gene of Arabidopsis thaliana shows homology to PPOX?s from a number of organisms including the Saccharomyces cervisiae PDX3 gene. A cDNA corresponding to putative A. thaliana PPOX (AtPPOX) was obtained using RT-PCR and primers landing at the start and stop codons of At5g49970. The putative AtPPOX is 530 amino acid long and predicted to contain three distinct parts: a 64 amino acid long N-terminal putative chloroplast transit peptide, followed by a long Yjef_N domain of unknown function and a C-terminal Pyridox_oxidase domain. Recombinant proteins representing the C-terminal domain of AtPPOX and AtPPOX without transit peptide were expressed in E. coli and showed PPOX enzyme activity. The PDX3 knockout yeast strain deficient in PPOX activity exhibited sensitivity to oxidative stress. Constructs of AtPPOX cDNA of different lengths complemented PDX3 knockout yeast for oxidative stress. The role of the Yjef_N domain of AtPPOX was not determined, but it shows homology with a number of conserved hypothetical proteins of unknown function. 21 INTRODUCTION Vitamin B 6 is the collective term for a group of three related compounds, pyridoxine (PN), pyridoxal (PL) and pyridoxamine (PM), and their phosphorylated derivatives, pyridoxine 5'-phosphate (PNP), pyridoxal 5'-phosphate (PLP) and pyridoxamine 5'-phosphate (PMP). All organisms require PLP and must either produce it or acquire it through their diet. PLP is an important cofactor in a wide range of biochemical reactions, including amino acid metabolism and antibiotic biosynthesis (Studart et al., 2005). Additionally, PLP or its derivatives may function as regulatory molecules in signal transduction regulating a number of membrane ion transporters (Hamasaki and Okubo, 1996; Palmieri et al., 2001; Salhany and Schopfer, 1993). Vitamin B 6 is also an efficient singlet oxygen quencher and potential antioxidant (Bilski et al, 2000). PLP is required for post-embryonic root development, and protects plant from high-salt, ultraviolet rays, osmotic and oxidative stresses (Shi et al, 2002; Chen and Xiong, 2005). Most bacteria, fungi, and plants possess vitamin B 6 biosynthesis pathways, but mammals must be supplied with the vitamin in their diet (Tsuyoshi et al., 2004). Different vitamin B 6 biosynthetic pathways, referred to as the de novo pathway and the salvage pathway, are known. In E. coli, PNP is synthesized from the condensation of deoxyxylulose 5-phosphate and 4-hydroxythreonine-4-phosphate, catalyzed by PdxA and PdxJ (Laber et al., 1999), while plants, fungi and some other bacteria utilize ribose 5- phosphate or ribulose 5-phosphate and dihydroxyacetone phosphate or glyceraldehyde 3- phosphate to synthesize PLP (Studart et al., 2005; Raschle et al., 2005). 22 The vitamin B 6 salvage pathway is involved in interconvertions between different vitameric forms of vitamin B 6 . In vitamin B 6 auxotrophic organisms, uptake of PN, PL, or PM from the extracellular space is required to generate intracellular PLP via the salvage pathway. Pyridoxine (Pyridoxamine) 5?-phosphate oxidase (PPOX), pyridoxal kinase, pyridoxal reductase, and vitamin B 6 phosphatase are all involved in the salvage pathway of plants (Tsuyoshi et al., 2004). However, only pyridoxal kinase in this pathway has been studied in detail (Shi and Xiong, 2002; Lum et al., 2002). This enzyme catalyzes the transfer of a phosphate from ATP to vitamin B 6 vitamers resulting in corresponding phosphorylated derivatives (Kerry et al., 1986). PPOX plays an important role in the salvage pathway because it converts PMP or PNP to PLP, the active form of vitamin B 6 (Salvo et al., 1998). PPOX has been identified in S. cerevisiae, human, mammalian cells, E. coli and several other bacteria (Lam and Winkler, 1992; Loubbardi et al., 1995; Kang et al., 2004; Bahn et al., 2002), but little information is available about PPOX in plants. Two isozymes of PPOX from wheat seedlings were partially purified. One isozyme used only pyridoxine 5?-phosphate as substrate, while the other one used both PNP and PMP with approximately equal efficiency (Tsuge et al., 1982). Here we present isolation and characterization of an A. thaliana cDNA encoding a putative pyridoxine (pyridoxamine) 5?-phosphate oxidase, and the functional characterization of various parts of a recombinant protein made from this cDNA. The plant protein also is functionally sufficient to complement the abatement of oxidative stress in yeast cells lacking a functional PPOX gene. 23 RESULTS AND DISCUSSION Isolation of A. thaliana pyridoxine (pyridoxamine) 5?- phosphate oxidase cDNA and its homology to S. cerevisiae PDX3 PDX3 showed PPOX activity in S. cerevisiae (Loubbardi et al., 1995). BLASTP analysis using PDX3 demonstrated a putative PPOX protein in A. thaliana. PDX3 shows homology with the C-terminal half of AtPPOX encoded by At5g49970. The C-terminal half of AtPPOX shares 44% amino acid sequence identity and 61% similarity with S. cerevisiae PDX3 (Fig. 1A). Additionally, the AtPPOX amino acid sequence shows roughly the same level of homology with a number of PPOX genes from a wide range of bacteria, fungi, and lower and higher animals. The cDNA corresponding to the AT5G49970 gene was amplified using RT-PCR with primers that include the putative start and stop codons. The 1593 bp cDNA sequence is in full length and encodes a 530 amino acid polypeptide that contains three significant features. The N-terminal 64 amino acids are identifiable as a putative chloroplast transit peptide (http://www.cbs.dtu.dk/services/ChloroP/). A Yjef_N domain of unknown function can be identified at amino acid position 100 to 281. And the C- terminal region contains a Pyridox_oxidase domain starting at amino acid position 364 and ending at position 454 (Fig. 1B). Amino acid sequence of AtPPOX has unique Yjef_N domain. Both the rice and Giardia lamblia PPOXes have amino acid sequence similar to AtPPOX that contain a Yjef_N domain (www.ncbi.nlm.nih.gov/BLAST/Blast.cgi). The human Yjef_N domain shows homology to apolipoprotein A-I binding protein and may be involved in the 24 regulation of vesicle fusion in the endosomal/lysosomal route (Schmitz and Rudolph, 2004). The Yjef_N domain also shows homology to human TGR-CL10C thyroidal receptor for N-acetylglucosamine (www.ncbi.nlm.nih.gov/BLAST/Blast.cgi). YNL200C in S. cerevisiae carrying Yjef_N domain homologue is a hypothetical protein and shows similarity to E. coli hydroxyethylthiazole kinase at the C-terminus and to enzymes involved in thiamine biosynthesis, and it may be involved in interactions with other Pfam family proteins (http://www.sanger.ac.uk/cgi-bin/Pfam/getacc?PF03853). The function of Yjef_N domain in AtPPOX remains to be elucidated. Expression of the recombinant AtPPOX in E. coli and assay of PPOX activity To determine the PNP/PMP oxidase activity of putative AtPPOX, constructs of different length were expressed in E. coli. The recombinant proteins were derived from the full coding sequence (AtPPOX-1593), the AtPPOX without the putative chloroplast transit peptide sequence (AtPPOX-1401), and the C-terminal pyridox_oxidase domain sequence (AtPPOX-681). AtPPOX-1401 and AtPPOX-681 were highly expressed (Fig. 2), but recombinant protein from the full length AtPPOX-1593 was not detected. The expressed recombinant proteins were purified using the Probond TM purification system, and both the total protein extracts and purified recombinant proteins were analyzed utilizing SDS-PAGE (Fig. 2). Recombinant protein from AtPPOX-1401 and from AtPPOX-681 tagged with 6?His and Xpress TM epitope had a theoretical molecular weight of 56 kDa and 30 kDa, respectively. The molecular determined from the SDS-PAGE were consistent with this inferred theoretically. 25 The purified recombinant proteins encoded by AtPPOX-1401 and AtPPOX-681 used both PNP and PMP as substrates, but the relative rate of catalytic activity for PNP was about 3.4 times higher than for PMP (Table 1). When the molecular size of each protein is taken into account, the specific activity of the AtPPOX-681 derived protein is approximately 17% higher than that of the AtPPOX-1401 derived protein. These results suggest that the C-terminal pyridox_oxidase domain has PPOX activity with PNP and PMP, and that the activity is independent of the N-terminal Yjef_N domain regardless of the substrate utilized. Complementation of YBR035C for oxidative stress tolerance by AtPPOX Since pyridoxine vitamers act as singlet oxygen scavengers [5], the PDX3 deletion strain (YBR035C) was grown in different concentrations of hydrogen peroxide. In YPD liquid medium containing 2mM H 2 O 2 , YBR035C showed a distinct growth defect compared to the wild type BY4743 strain (Fig. 3). Yeast shuttle plasmids, p426GPD/AtPPOX-1593, p426GPD /AtPPOX-1401 and p426GPD / AtPPOX-681 were introduced into YBR035C strain of yeast. As a control, the p426GPD empty vector was also introduced. In YPD liquid media without H 2 O 2, no differences in the growth of control strain (BY4743), PDX3 deletion strain (YBR035C) and four different transformants were demonstrated. While in YPD medium with 2mM H 2 O 2, YBR035C and those transformed with p426GPD empty vector did not grow, whereas YBR035C transformed with p426GPD/AtPPOX-1593, p426GPD /AtPPOX-1401 and p426GPD /AtPPOX-681 constructs showed significant growth (Fig. 3). Complementation efficiency was calculated from the growth of control strain BY4743 under identical growth 26 conditions. The efficiency of complementation was 89% for AtPPOX-681 followed by AtPPOX-1401 and AtPPOX-1593 showing 86% and 60% complementation, respectively. The complementation result reaffirmed measurement of PPOX enzyme activity of the recombinant proteins and provided support for the independent function of C-terminal pyridox_oxidase domain of AtPPOX in the catalytic activity. MATERIAL AND METHODS RNA extraction and cDNA cloning Two-week-old A. thaliana seedlings were ground to a powder in liquid nitrogen. RNA was extracted using RNAeasy plant mini kit (Qiagen), as described in the instruction manual. Total RNA (0.5?g) was reverse-transcribed using the one-step RT- PCR kit (Qiagen) in a 50 ?l RT-PCR reaction mixture. PCR primers used were 5?- ATGAGGAATGTGATACGCAGAGTC-3? and 5?-TCATGGGGCCAATCTATGAA-3?. Amplification was performed in a thermal-cycler as follows: 30 min at 50?C; 15 min at 95?C; then 1 min at 94?C; 1 min at 55?C; 1 and a half min at 72?C for 30 cycles, followed by 10 min at 72?C. The single RT-PCR product of 1593 bp was observed in agarose gel electrophoresis and cloned into the PGEM-T Easy vector (Promega). The sequence of both strands of the amplified DNA was verified. Expression of recombinant protein and purification of the AtPPOX-1 A set of primers, 5?-ATGCAAGATTCAGGATCACCAC-3? and 5?- TCATGGGGCCAACTATGAA-3? was used to amplify the AtPPOX-1 without putative 27 transit peptide sequence, and the resulting PCR product was 1401 bp long. Another pair of primers, 5?-ATGCAAGATTCAGGATCACCAC-3? and 5?-GTCGACTTAAATTC TAACACAC-3? was used to amplify the C-terminal pyridox-domain of the AtPPOX-1 resulting in a PCR product of 681 bp. The 1593 bp, 1401 bp, and 681 bp fragments were TA cloned into the pTrcHis-TOPO expression vector (Invitrogen) for expression of the recombinant proteins fused to the C-terminus of XpressTM epitope and hexa-histidine tag. These three plasmids were designated as pTrcHis-TOPO/AtPPOX-1593, pTrcHis- TOPO/AtPPOX-1401 and pTrcHis-TOPO/ AtPPOX-681, respectively. The expression of recombinant proteins from these constructs were induced by the addition of 1 mM isopropyl-1-?-thio-D-galactopyranoside (IPTG) when the culture reached an OD 600 = 0.5, followed by growth for 5h at 37?C. The recombinant proteins were purified using the ProBond TM purification System (Invitrogen) under nondenaturing conditions as described by the manufacturer. Assay of AtPPOX enzyme activity PMP was obtained from Sigma Chemical Co. PNP was synthesized by reducing PLP with sodium borohydride (Musayev et al., 2003). PNP and PMP oxidase activities were measured by monitoring PLP formation in Tris-phosphate buffer as described by Zhao et al (Zhao and Winkler, 1995). At 414 nm, the Schiff base formed between Tris and PLP has an extinction coefficient of 5900 M -1 cm -1 . Reaction mixtures (1.0 ml) contained 0.2 M Tris-HCl, 0.2 M KPO 4 (pH 8.5), 0.1 mg BSA, 2.0 ?M FMN, 0.5 mM PMP or PNP, and 20 to 30 ?g purified recombinant proteins. The enriched 6?His Xpress TM epitope was used as control for the enzyme assay, and the assay blanks 28 contained the same as reaction mixture except that no enzyme was added. Initial velocities were measured by monitoring the constant increase in A 414 for 5min at 37?C. No more than 3% of the substrate was used during this incubation. One unit of specific activity was defined as the formation of 1?mol of PLP per min at 37?C. Protein concentrations were determined using Bradford microassay method with BSA (1 ?g/ml- 20 ?g/ml) as the standard (Bradford MM, 1976). Yeast complementation The S. cerevisiae wild type control strain BY4743 and PDX3 deletion strain YBR035C were obtained from American Type Culture Collection (Manassas, VA, USA). Amplified PCR products of 1593 bp, 1401 bp and 681 bp fragments cloned in PGEM-T Easy vector (Promega) were isolated by EcoR1 digestion, and subcloned into the EcoR1 site of p426GPD yeast shuttle vector. Three resulting plasmids were designated as p426GPD/AtPPOX-1593, p426GPD /AtPPOX-1401 and p426GPD /AtPPOX-681, respectively. These three plasmids were transferred into YBR035C respectively by the heat shock method (Gietz and Woods, 1994). Complementation for sensitivity to oxidative stress was carried out in YPD liquid medium with 2mM H 2 O 2 . The complementation efficiency was calculated by dividing the OD 600nm of the complemented yeast strain by that of the control strain BY4743 during logarithmic phase. 29 Table 1. PNP/PMP oxidase activities of the purified recombinant proteins, AtPPOX- 1401 and AtPPOX-681, for PMP and PNP* Specific Enzyme Activity PNP PMP Purified Recombinant Protein units/mg units/pmole units/mg units/pmole Activity Ratio (PNP/PMP) AtPPOX-1401 154.6 8.7 45.8 2.6 3.4 AtPPOX-681 338.1 10.1 101.2 3.1 3.3 * Details about enzyme expression and purification, enzyme assay, and unit definition are in Materials and Methods. 30 Figure 1. (A ) Amino acid sequence alignment of AtPPOX and yeast PDX3. Amino acids identical in these two proteins are highlighted in black, and conservative substitutions are highlighted in gray. Putative transit peptide is shown in bold and the Yjef_N domain is underlined. The CLUSTALW program (Thompson et al., 1994) was used for sequence alignment. (B) Schematic diagram of predicted domains of AtPPOX. AtPPOX contains a putative chloroplast transit peptide, N- terminal YjeF_N domain and C-terminal Pyridox_oxidase domain. A AtPPOX 1 MRNVIRRVTTMTFTFLLQSPPLPISPSPPQFSLSSSPLSKTQRFITPSQGSRLRTLCTKV yeastPDX3 1 ------------------------------------------------------------ AtPPOX 61 IIPNMQDSGSPPLSYLTQREAAEIDETLMGPLGFSIDQLMELAGLSVAASIAEVYKPEEY yeastPDX3 1 ------------------------------------------------------------ AtPPOX 121 SRVLAICGPGNNGGDGLVAARHLHHFGYKPFICYPKRTAKPLYTGLVTQLDSLSVPFVSV yeastPDX3 1 ------------------------------------------------------------ AtPPOX 181 EDLPDDLSKDFDVIVDAMFGFSFHGAPRPPFDDLIRRLVSLQNYEQTLQKHPVIVSVDIP yeastPDX3 1 ------------------------------------------------------------ AtPPOX 241 SGWHVEEGDHEDGGIKPDMLVSLTAPKLCAKRFRGPHHFLGGRFVPPSVAEKYKLELPSY yeastPDX3 1 ------------------------------------------------------------ AtPPOX 301 PGTSMCVRIGKPPKVDISAMRVNYVSPELLEEQVETDPTVQFRKWFDEAVAAGLRETN-- yeastPDX3 1 -MTKQAEETQKP--IIFAPETYQYDKFTLNEKQLTDDPIDLFTKWFNEAKED-PRETLPE AtPPOX 359 AMALSTANKDK-KPSSRMVLLKGFDENGFVWFTNY-ESKKGSDLSENPSAALLFYWEILN yeastPDX3 57 AITFSSAELPSGRVSSRILLFKELDHRGFTIYSNWGTSRKAHDIATNPNAAIVFFWKDLQ AtPPOX 417 RQVRIEGPVERIPESESENYFHSRPRGSQIGAIVSKQSSVVPGRHVLYDEYEELTKQYSD yeastPDX3 117 RQVRVEGITEHVNRETSERYFKTRPRGSKIGAWASRQSDVIKNREELDELTQKNTERFKD AtPPOX 477 GSVIPKPKNWGGFRLKPNLFEFWQGQPSRLHDRLQYSLQDVNGNPAWKIHRLAP yeastPDX3 177 AEDIPCPDYWGGLRIVPLEIEFWQGRPSRLHDRFVYRRKTEND--PWKVVRLAP B 31 Figure 2. SDS-PAGE of recombinant AtPPOX protein of different lengths separated on a 12.5% gel. Lanes: 1, crude cell lysate of E. coli transformed with pTrcHis- TOPO/AtPPOX-1401; 2, purified AtPPOX-1401 recombinant protein; 3, crude cell lysate of E. coli transformed with pTrcHis-TOPO/AtPPOX-681; 4, purified AtPPOX-681 recombinant protein; 5, crude extract of E. coli transformed with pTrcHis-TOPO vector. kDa 1 2 3 4 5 181.8 115.5 82.2 64.2 48.8 37.1 25.9 19.4 14.8 6.0 32 Figure 3. Complementation of YBR035C under oxidative stress with AtPPOX constructs. BY4743, YBR035C and YBR035C transformed with vector p426GPD, p426GPD /AtPPOX-1593, p426GPD /AtPPOX-1401 and p426GPD /AtPPOX-681, respectively were grown in liquid YPD medium without H 2 O 2 (top) or with 2mM H 2 O 2 (bottom). YPD - H 2 O 2 YPD + 2mM H 2 O 2 Time (hrs) 024681012 OD 60 0nm 0 1 2 BY4743 YBR035C AtPPOX-1593 AtPPOX-1401 AtPPOX-681 p426 GPD Time (hrs) 024681012 OD 6 00nm 0 1 2 BY4743 YBR035C AtPPOX-1593 AtPPOX-1401 AtPPOX-681 p426 GPD 33 III IDENTIFICATION OF ATPPOX-2 FROM ARABIDOPSIS THALIANA ABSTRACT Pyridoxine (Pyridoxamine) 5?-phosphate oxidase (PPOX) is an important enzyme involved in the salvage pathway of vitamin B 6 biosynthesis. This enzyme converts pyridoxine 5?-phosphate (PNP) or pyridoxamine 5?-phosphate (PMP) into pyridoxal 5?- phosphate (PLP), a cofactor for numerous enzymes. Using RT-PCR, we cloned the cDNA of AtPPOX-2, a second putative PPOX gene at the locus of At2g46580 in Arabidopsis thaliana. The RT-PCR amplified cDNA was cloned into an E. coli expression vector and a yeast shuttle vector. Both PPOX enzyme assay and the complementation of PDX3 knockout yeast for oxidative stress showed that the gene at locus At2g46580 encodes for a PPOX (AtPPOX-2) with low PPOX specific activity. The catalytic efficiency of AtPPOX-1 is almost 300-fold higher than that of AtPPOX-2. Based on bioinformatic analysis, there is a putative transit peptide at the N-terminus. The truncated AtPPOX-2 without 18 amino acids at the N-terminal end lost PPOX activity suggesting that the N-terminal amino acids are necessary for the enzyme activity of AtPPOX-2. 34 INTRODUCTION Pyridoxine (Pyridoxamine) 5?-phosphate oxidase (PPOX) catalyzes the oxidation of pyridoxine 5?-phosphate (PNP) and pyridoxamine 5?-phosphate (PMP) into pyridoxal 5?- phosphate (PLP) (Wada and Snell, 1961; Yang and Schirch, 2000). PLP is the active form of vitamin B6, acting as a ubiquitous, essential cofactor for numerous enzymes involved in amino acid metabolism and several other metabolic pathways. Plants and fungi can synthesize PLP directly via PLP synthase complex (Studart et al., 2005). In mammalian cells where vitamin B 6 is a nutritional requirement and acquired from their nutrients, PPOX is especially important for the biosynthesis of PLP through the PLP salvage pathway. PPOX exists in almost all organisms. Wheat seedlings have at least two PPOX enzymes (Tsuge et. al., 1982) while bacteria, fungi and animals appear to have only one PPOX enzyme (Zhao and Winkler, 1995; Kazarinoff et. al., 1975; Choi and Churchich, 1987). Two isozymes of PPOX from wheat seedlings were partially purified. One isozyme used only pyridoxine 5?-phosphate as substrate, while the other one used both PNP and PMP with approximately equal efficiency. PNP is by far the better substrate for the PPOX from E. coli, whereas PPOX from rabbit liver oxidizes both substrates to almost the same extent (Zhao and Winkler, 1995; Choi et al., 1983). AtPPOX-1 encoded by At5g49970 in Arabidopsis thaliana oxidizes both PNP and PMP, with higher efficiency towards PNP (Sang et al., 2007). Bioinformatic analysis of A. thaliana genome suggested the presence of an additional gene at the At2g46580 locus which also contains a pyridox_oxidase superfamily domain, but there is no biochemical evidence to support its function as PPOX enzyme. In this 35 study, we report that At2g46580 encodes for a second PPOX in A. thaliana (AtPPOX-2). The catalytic efficiency of AtPPOX-2 is about 300-fold lower than that of AtPPOX-1. RESULTS Cloning of cDNA at the At2g46580 locus in A. thaliana Bioinformatically, the protein encoded by At2g46580 locus in A. thaliana showed homology to the Pyridox_oxidase domain found in pyridoxine 5'-phosphate oxidase- related proteins in the NCBI data base. In order to determine the function of protein encoded by the At2g46580 locus, the corresponding cDNA was amplified by a one-step RT-PCR using the total RNA as template. The primers included the first 22 nucleotides of the ORF, including the ATG start codon, and the last 23 nucleotides, including the stop codon. Amplified PCR products were cloned into the PGEM-T Easy vector and both strands were sequenced. The full length cDNA is 597 base pairs long and encodes for a 198 amino acid polypeptide. Expression and purification of the recombinant protein AtPPOX-2 To express AtPPOX-2, its cDNA sequence without a stop codon was first cloned into the PGEM-T Easy vector, and then subcloned into the pET-20b expression vector. The resulting pET-20b/AtPPOX-2 plasmid was transformed into C41 pLys host cells. When induced by IPTG at room temperature, the recombinant protein was highly expressed. Since the recombinant protein has a C-terminal His tag, it was purified using the Probond TM purification system. The purified recombinant proteins and the total protein extracts were analyzed utilizing SDS-PAGE (Fig. 1). Recombinant AtPPOX-2 36 protein tagged with 6?His had a molecular weight of 28 kDa. The molecular weight inferred from the SDS-PAGE was consistent with that obtained theoretically. PPOX activity of the recombinant AtPPOX-2 To determine if the purified protein has PPOX activity, the Schiff base method described by Zhao et al. (1995) was used. But PPOX activity was not detected in the recombinant protein. However, we were able to measure the PPOX activity using a method described by Tsuge et al. (1982). This result demonstrated that the recombinant putative AtPPOX-2 protein had low PPOX activity. Controls for each enzyme assay did not show any activity. We previously had found and characterized a PPOX in Arabidopsis thaliana (Sang et al., 2007) encoded by the A5g49970 gene which we named as AtPPOX-1. Similar to AtPPOX-1, AtPPOX-2 can accept both PNP and PMP as substrate and the catalytic activity for PNP was higher than for PMP. However, the catalytic efficiency of AtPPOX-1 is almost 300-fold higher than that of AtPPOX-2. PPOX activity of AtPPOX-1 and AtPPOX-2 measured using the method developed by Tsuge et al. is shown in Figure 2. The truncated AtPPOX-2 without the N-terminal 18 amino acids was also expressed and purified, but it has no enzyme activity (data not shown). This result demonstrated that the N-terminal 18 amino acids are necessary for PPOX activity of AtPPOX-2. Complementation of yeast YBR035C for oxidative stress tolerance by AtPPOX-2 PDX3 is a yeast gene coding for yeast PPOX protein. The yeast PDX3 deletion strain, YBR035C, showed a distinct growth defect compared to the wild type BY4743 37 strain when grown in YPD liquid medium containing 2mM H 2 O 2 (Sang et al., 2007). To confirm if AtPPOX-2 encoded protein has PPOX activity, full length cDNA was cloned into the p426GPD yeast shuttle vector, and the resulting construct p426GPD/AtPPOX-2 was used to transform YBR035C yeast strain. As a control, the p426GPD empty vector was transformed into the YBR035C yeast strain. On SCM media without 2mM H 2 O 2, BY4743, YBR035C and the transformants with p426GPD/AtPPOX-2 plasmid or empty p426GPD grew almost the same. On SCM media supplemented with 2mM H 2 O 2, YBR035C control and the YBR035C transformed with empty p426GPD vector did not show appreciable growth, whereas the YBR035C transformed with p426GPD/AtPPOX-2 construct showed some growth (Figure 3). This result demonstrated a weak complementation of PDX3 by AtPPOX-2. This result is consistent with the enzyme assay. DISCUSSION Pyridoxine (Pyridoxamine) 5?-phosphate oxidase (PPOX) has been widely found in bacteria, fungi, animals and plants. Except for wheat seedlings, no other organisms have been reported to have more than one PPOX isozyme. Wheat seedlings were reported to have three PPOX isozymes (Tsuge et al., 1982). We reported the first PPOX encoded by At5g49970 in A. thaliana (Sang et al., 2007). Herein, a second PPOX isozyme encoded by At2g46580 in A. thaliana is identified. PPOX from different organisms catalyze PMP and PNP oxidation at different catalytic efficiency. PNP is by far the better substrate for the PPOX from E. coli (Zhao and Winkler, 1995; Salvo et. al. 1998). PPOX from rabbit liver oxidizes both substrates to almost the same extent (Choi et al., 1983). Wheat seedlings were reported to have at 38 least three PPOX isozymes, two of which were partially purified. One of the PPOX isozymes oxidized both PNP and PMP at approximately equal rates, whereas the other used only PNP as substrate (Tsuge et al., 1982). However, in Arabidopsis thaliana, both AtPPOX-1 and AtPPOX-2 can accept PNP and PMP as substrate, and have higher catalytic efficiency toward PNP. All PPOX studied thus far need oxygen as the final electron acceptor. The question is how PNP oxidization to PLP occurs in anaerobically growing cells in which the PPOX presumably does not work. Two possibilities have been suggested (Salvo et al., 2003). One possibility is that there is a single form of PdxH oxidase in wild-type E. coli, which uses oxygen aerobically and another electron acceptor anaerobically. A second possibility is that there is a second PPOX that functions anaerobically. Compared to AtPPOX-1, AtPPOX-2 has a much lower PPOX activity in vitro. It is possible that AtPPOX-2 needs the specific final electron acceptor or other factors that do not exist in vitro conditions. It is also likely that the recombinant AtPPOX-2 expressed in E. coli does not have the correct modifications which may occur in plants. MATERIAL AND METHODS cDNA cloning of AtPPOX-2 RNAeasy plant mini kit (Qiagen) was used to extract the total RNA from the two- week-old A. thaliana seedlings, as described in the instruction manual. Total RNA (0.5?g) was reverse-transcribed using the one-step RT-PCR kit (Qiagen) in a 50 ?l RT-PCR reaction mixture. PCR primers used were 5?-ATGGGAACACATGTAGCACCAT-3? and 5?-TTATGGGTTAACCTTTTCTGAAGTC-3?. Amplification was performed in a 39 thermal-cycler as follows: 30 min at 50?C; 15 min at 95?C; then 1 min at 94?C; 1 min at 52?C; 1 min at 72?C for 30 cycles, followed by 10 min at 72?C. The single RT-PCR product of 597 bp was observed in agarose gel electrophoresis. This fragment was cloned into the PGEM-T Easy vector (Promega). The sequence of the amplified DNA was verified. Expression and purification of the recombinant AtPPOX-2 A set of primers, 5?-GGATCCATGGGAACACATGTAGCACCAT-3? and 5?- GAATCCTGGGTTAACCTTTTCTGAAGTC-3? was used to amplify the cDNA of At2g46580. The 606 bp fragments were TA cloned into the PGEM-T Easy vector. The fragments were cut out with BamH1 and EcoR1 and cloned into the pET-20b expression vector (Novagen) for expression of the recombinant proteins fused to the C-terminus hexa-histidine tag. The resulting plasmid was designated as pET-20b/AtPPOX-2 and was used to transform E. coli strain, C41 pLys. The transformed E. coli culture was induced by the addition of 1 mM isopropyl-1-?-thio-D-galactopyranoside (IPTG) when the culture reached an OD 600 = 0.5, followed by growth for 5 hrs at 26?C. Cell lysate was used to purify the recombinant proteins using the ProBond TM purification System (Invitrogen) under nondenaturing conditions as described by the manufacturer. Enzyme Assay of the recombinant AtPPOX-2 The activity of PPOX was measured with a colorimetric procedure (Gonz?lez et al., 2007). Enzyme activity of purified recombinant protein was determined in 0.5-mL reaction mixtures containing 200 mM Tris-HCl, 200 mM KPO 4 , pH 8.5, and 0.2 mM 40 PMP/PNP. After 1 h of incubation at 37?C, reactions were stopped by addition of 50 ?L of chilled 50% (w/v) TCA. The reaction mixture was centrifuged at 4?C and 1,500 rcf for 10 min, and supernatant was transferred to a clean tube. PLP formation was measured at OD 410 following addition of 2% (w/v) phenylhydrazine in 10 N H 2 SO 4 and incubation on ice for 30 min. Protein concentration was determined with the Bradford protein assay kit (Bio-Rad Laboratories) with bovine serum albumin as the standard. Complementation of PDX3 deletion strain for oxidative tress The S. cerevisiae wild type control strain BY4743 and PDX3 deletion strain YBR035C were obtained from American Type Culture Collection (Manassas, VA, USA). Amplified PCR products of 597 bp fragments cloned in PGEM-T Easy vector (Promega) were isolated by EcoR1 digestion, and subcloned into the EcoR1 site of p426GPD yeast shuttle vector. The resulting p426GPD/AtPPOX-2 plasmid was transferred into YBR035C by the heat shock method (Gietz et al., 1994). Complementation for sensitivity to oxidative stress was carried out on SCM medium plate supplemented with 2mM H 2 O 2 as described by Sang et al. (2007). 41 Figure 1. SDS-PAGE of the recombinant AtPPOX-2 separated on a 12.5% SDS- Polyacrylamide gel. Lanes: 1, purified recombinant AtPPOX-2; 2, crude extract of C41 pLys host cells transformed with Empty pET-20b vector; 3, crude cell lysate of C41 pLys host cells transformed with pET-20b/AtPPOX-2. 42 Figure 2. PPOX activity of the purified recombinant AtPPOX-1 and AtPPOX-2 with PMP and PNP as substrates. The enzyme activity was measured by determining the amount of PLP formed with a colorimetric assay after 1 hour incubation of enzyme reactions containing increasing amounts of total protein. 43 Figure 3. Complementation of the YBR035C under oxidative stress by AtPPOX-2. BY4743, YBR035C, YBR035C transformed with p426GPD/AtPPOX-2, and YBR035C transformed with empty vector p426GPD control were grown on SCM - H 2 O 2 (left) or +2mM H 2 O 2 (right). Each row represents a serial 10-fold dilution from a starter culture with an OD of 0.01at 600 nm. Stationary phase cultures (12 hrs) were diluted to an optical density (OD 600 ) of 0.01. - H2O2 + 2mM H2O2 BY 4743 YBR035C YBR035C/p426GPD YBR035C/AtPPOX-2 44 IV EVOLUTIONARY ANALYSIS OF ATPPOX-1 AND ATPPOX-2 FROM ARABIDOPSIS THALIANA ABSTRACT Pyridoxine (Pyridoxamine) 5?-phosphate oxidase (PPOX) is an important enzyme involved in the salvage pathway of vitamin B6 biosynthesis. It converts pyridoxine 5?- phosphate (PNP) or pyridoxamine 5?-phosphate (PMP) into pyridoxal 5?-phosphate (PLP), a cofactor for numerous enzymes. Two PPOX proteins have been identified in Arabidopsis thaliana, which show considerable difference in size of the mature protein and amino acid sequence. Phylogenetic analysis of AtPPOX-1 and AtPPOX-2 homologs across all domains of life suggests that AtPPOX-1 and AtPPOX-2 have independent origins. AtPPOX-1 phylogeny appears congruent with the underlying branching pattern of the overall tree of life, while AtPPOX-2 phylogeny suggest that plant PPOX-2 may have originated from cyanobacteria. AtPPOX-1 homologs from over 30 plant species have an additional Yjef_N domain preceding Pyridox_Oxidase domain at the C-terminal end. AtPPOX-1 homologs from bacteria, fungi and animals have only the Pyridox_Oxidase domain. Presence of Yjef_N domain in land plants in AtPPOX-1 homologs suggest that acquisition of this domain and its fusion with pyridox_oxidase domain began with the endosymbiotic acquisition of the chloroplast. 45 INTRODUCTION Pyridoxine (Pyridoxamine) 5?-phosphate oxidase (PPOX) converts pyridoxine 5?- phosphate (PNP) or pyridoxamine 5?-phosphate (PMP) into pyridoxal 5?-phosphate (PLP), a cofactor for numerous enzymes, and is found in all organisms. Both the prokaryotic and eukaryotic enzymes are homodimers with one molecule of FMN tightly binding to each subunit (Kazarinoff et al., 1975; Choi et al., 1983; Zhao et al., 1995; Salvo et al., 1998). It was thought that the subunit size of both the prokaryotic and eukaryotic PPOX is 25-28 kDa (Salvo et al., 1998). However, AtPPOX-1 from A. thaliana is 530 amino acids long and has a molecular weight of 62 kDa (Sang et al., 2007). Besides the pyridox_oxidase domain present in all PPOX, AtPPOX-1 has an extra Yjef_N domain. Truncated recombinant AtPPOX-1 without a Yjef_N domain has full enzyme activity, suggesting that PPOX activity of AtPPOX-1 is independent of the Yjef_N domain. AtPPOX-2 is a considerably smaller protein with 24 kDa size. AtPPOX- 2 has pyridox_oxidase domain and does not have Yjef_N domain at its N-terminal. In order to determine the evolutionary relationship of two very dissimilar proteins, i.e. AtPPOX-1 and AtPPOX-2 in A. thaliana, and to determine the stage when the yjef_N domain began to fuse with pyridox_oxidase domain in AtPPOX-1 homologs, various genomic databases were searched for AtPPOX-1 and AtPPOX-2 homolog from various organisms. Using the retrieved protein sequences, phylogenetic analysis was carried out to analyze the evolutionary history of AtPPOX-1 and AtPPOX-2. 46 RESULTS AtPPOX-1 and AtPPOX-2 have low similarity Since AtPPOX-1 and AtPPOX-2 both have PPOX activity, amino acid sequence alignment was performed to determine similarities between these two proteins (Figure 1). The amino acid sequences of these two PPOX show 37% similarities only in the ppox_domain of the protein. AtPPOX-1 and AtPPOX-2 homologs retrieved from various databases All available homologs of AtPPOX-1 and AtPPOX-2 were retrieved from protein, EST, and genome databases across all domains of life. Most sequences used here are available from the NCBI protein database, but some were reconstructed from EST and genomic sequence. Complete coding sequences were retrieved for most proteins, while for some only partial sequences were obtained. Overall, 144 AtPPOX-1 homologs (Table 1) and 56 AtPPOX-2 homologs (Table 2) were retrieved. Some organisms have both AtPPOX-1 and AtPPOX-2 homologs, but only one of them was found in many organisms. Animals have only the AtPPOX-1 homolog. Prasinophyte algae, such as Ostreococcus tauri and Ostreococcus lucimarinus possess only AtPPOX-2 homolog. However, no AtPPOX-1 or AtPPOX-2 homolog was found in Archea. Conserved regions among all AtPPOX-1 and AtPPOX-2 homologs To determine the conserved regions among all PPOX proteins, one amino acid sequence of AtPPOX-1 and AtPPOX-2 homologs from each domain of life was aligned. It was found that there are three conserved regions among all PPOX (Figure 2). In terms 47 of AtPPOX-2, R 42 , V 44 , V 45 , P 88 , P 90 , P 93 , P 191 and P 198 are conserved among all PPOX proteins. AtPPOX-1 homologs from plants have both yjef_N and pyridox_oxidase domain Similar to AtPPOX-1, AtPPOX-1 homologs from Vitis vinifera, Oryza sativa, Picea sitchensis and Physcomitrella patens found in NCBI protein database are also much longer than PPOX found in bacteria, fungi, and animals. These proteins from plants not only have pyridox_oxidase domain but also have an extra Yjef_N domain, whereas AtPPOX-1 homologs from other domains of life have only pyridox_oxidase domain. In order to determine if all plant AtPPOX-1 homologs have both domains, AtPPOX-1 homologs retrieved from database searches were analyzed. Interestingly, AtPPOX-1 homologs from all land plants, Chlorophyte algae, Charaphyte algae and red algae have both yjef_N domains and pyridox_oxidase domains. In Prasinophyte algae, only Ostreococcus tauri and Ostreococcus lucimarinus sequences are available, and no AtPPOX-1 homolog was found. The AtPPOX-1 homolog derived tree Figure 3 shows an unrooted neighbor-joining tree of AtPPOX-1 homologs. Clustering of the organisms into fungi, green plants and animals can be observed. However, three clusters were formed for bacteria. AtPPOX-1 homologs of the bacteroidetes form a tight cluster and the other two clusters have bacteria from different families. AtPPOX-1 homologs from plants and animals have much closer relationship than that from fungi. The fungal enzymes are most closely related to AtPPOX-1 48 homologs found in the genomes of the bacteroidetes. Cyanidioschyzon merolae and Galdieria sulphuraria are unicellular algae, but they were not in the same cluster. AtPPOX-1 homologs from Cyanidioschyzon merolae fall in the same cluster with bacteria, whereas AtPPOX-1 homologs from Galdieria sulphuraria fall in the same cluster with green plants. Interestingly, AtPPOX-1 homologs from Volvox cateri, the best-known chlorophytes was grouped with animal PPOX. The AtPPOX-2 homolog derived tree Figure 4 shows an unrooted phylogenetic tree of AtPPOX-2 homologs. Since animals do not have AtPPOX-2 homolog, only bacteria, fungi and plants are included in this tree. Clustering of the organisms into fungi and land plants can be observed. AtPPOX-2 homologs from cyanobacteria and marine algae such as Chlamydomonas reinhardtii and Ostreococcus sp., form a tight cluster, and this cluster is positioned closely to the AtPPOX-2 homologs from land plants. AtPPOX-2 homologs from other bacteria form a different cluster. AtPPOX-1 homologs from fungi show close relation to other bacteria. DISCUSSION The subunit of AtPPOX-1 is much longer than that of PPOX found in bacteria, fungi and animals. Besides the C-terminal pyridox_oxidase domain, AtPPOX-1 has an extra N-terminal Yjef_N domain, whereas PPOX in bacteria, fungi and animals have only pyridox_oxidase domain. AtPPOX-1 homologs found in over 30 plant organisms including red algae, land plants, charaphyte algae and chlorophyte algae have both Yjef_N domain and pyridox_oxidase 49 domain. Yjef_N domain is conserved across all domains of life, but its function is unknown. It exists either as a single protein, or is fused with other domains (Anantharaman and Aravind, 2004). In archea and bacteria, the Yjef_N domain is often found fused to a C-terminal kinase domain of the ribokinase superfamily. In fungi, Yjef_N domain is not only found in a conserved hypothetic protein, but also found in the fungal Dcp3p-like protein. The animal FLJ22/28-like protein contains FDF domain, Sm domain, and Yjef_N domain. The apolipoprotein A-I binding protein that is involved in the regulation of vesicle fusion in the endosomal/lysomomal route in mammals shows a high similarity to the Yjef_N domain family (Schmitz et al., 2004). In the AtPPOX-1 homolog derived tree, bacteria form three clusters rather than one tight cluster. This demonstrates that AtPPOX-1 homologs from bacteria evolved very rapidly. Fungal AtPPOX-1 homologs are more closely related to bacteroidetes than they are to plants or animals. So the fungal enzyme may have the same origin as bacteroidetes, while enzymes from plants and animals originated from other bacteria. Cyanidioschyzon merolae form the same cluster with bacteria, whereas Galdieria sulphuraria form the same cluster with green plants. Interestingly, AtPPOX-1 homologs from Volvox cateri, the best-known chlorophytes grouped within the animals. In the AtPPOX-2 homolog derived tree, cyanobacteria and green algae, such as Chlamydomonas reinhardtii and Ostreococcus sp., form a tight cluster, and this cluster is closely related to that formed by land plants. Since cyanobacteria are the origin of chloroplast, it is possible that AtPPOX-2 in Arabidopsis thaliana was originally present in the endosymbiotic ancestor of the chloroplast, and may target back into the chloroplast after translation. 50 MATERIAL AND METHODS Database searches for PPOX and Yjef_N domain family The non-redundant database of protein sequences was searched using a BLASTP program at NCBI (Altschul et al., 1997), with the Blosum62 matrix and default parameters. We performed PSI-BLAST throughout all organisms using Arabidopsis thaliana PPOX (NP_568717 or NP_566081) as the query sequence. Each search resulted in a list of similar sequences, which was added to the next round of PSI-BLAST iteration searches, and each search continued until no new sequences with an alignment score above the default threshold was retrieved. The sequences returned by these queries were combined and all redundant sequences were discarded. Sequences were also retrieved using a tBLASTN search in the EST databases. The returned overlapped EST sequences in the same organism were conjugated into one full EST sequence using the Bioedit program, and then translated into the amino acid sequence. Plant Genomes Central in NCBI was also used to search for EST sequences encoding for PPOX enzymes in plants. PPOX homologs and EST sequences that are not available in NCBI were also retrieved from the DOE Joint Genome Institute. PPOX in Cyanidioschyzon merolae was found in http://merolae.biol.s.u-tokyo.ac.jp/blast/blast.html, and EST sequences encoding PPOX in Galdieria sulphuraria was found in http://genomics.msu.edu/galdieria/index.html. Sequence alignments and phylogenetic analysis of PPOX All protein sequences retrieved using the above methods were examined individually and aligned using Clustal X program (Thompson et al., 1997). Manual adjustments were made where necessary. Cluster analyses were perfomed in Paup * v. 4.0 (Swofford, 2002). 51 Table 1. AtPPOX-1 homologs. Members of this family are listed in alphabetial order (144 sequences) Acaryochloris_YP_001518889 Lodderomyces_XP_001525388 Acidiphilium_YP_001233967 Human_NP_060599 Acidovorax_YP_971145 Lottia Acidovorax_YP_986310 Magnetospirillum_YP_420249 Algoriphagus_ZP_01717977 Mannheimia_EDN74621 Anabaena_YP_321076 Marinobacter_YP_957449 Aquilegia Medicago Arabidopsis_NP_568717_5G Methylibium_A2SJZ5 Ashbya_NP_982729 Methylibium_YP_001022119 Arcobacter_YP_001490460 Methylobacterium_ZP_02118090 Azorhizobium_YP_001524113 Microcystis_CAO90251 Azotobacter_ZP_00418533 Microscilla_ZP_01693022 Bacteroides_NP_810490 Monodelphis_XP_001372689 Bacteroides_YP_098738 Monosiga Bradyrhizobium_NP_729624 Mouse_NP_598782 Bdellovibrio_NP_969371 Myxococcus_YP_629552 Bordetella_NP_881799 Nectria Bordetella_Q2KVR0 Neurospora_XP_961897 Botryotinia_XP_001551181 Nodularia_ZP_01632435 Bovine_NP_001014907 Nostoc_NP_485291 Brassica Nostoc_ZP_00111879 Burkholderia_ZP_01499380 Oceanobacter_ZP_01307236 Caenorhabditis_NP_498518 Opitutaceae_ZP_02013944 Candidatus_YP_266037 Oryza_NP_001064477 Candida_XP_447454 Pedobacter_ZP_01882425 Capitella Phaeosphaeria_EAT83869 Castor_m006117 Physcomitrella_EDQ52531 Cellulophaga_ZP_01049128 Pichia_XP_001386486 Chaetomium_XP_001223947 Picea Chloroflexus_ZP_01517186 Picea_ABK24840 Citrus Pinus Colwellia_YP_267797 Polaribacter_ZP_01117843 Comamonas_ZP_01518565 Polaromonas_YP_550365 Coxiella_NP_819941 Populus Croceibacter_ZP_00951035 Porphyromonas_NP_905824 Crocosphaera_ZP_00516266 Prochlorococcus_NP_896023 Cyanidiochyzon_CMM155C Pseudomonas_ZP_01716544 Cyanothece_ZP_01730885 Psychromonas_ZP_01216352 Cytophaga_YP_678384 Psychroflexus_ZP_01252609 Daphnia Radish Danio_XP_688664 Ralstonia Debaryomyces_XP_461102 Reinekea_ZP_01114160 Deinococcus_YP_603915 Rhodopirellula_NP_869187 Delftia_YP_001564960 Rhodopseudomonas_YP_484826 Dictyostelium_XP_642126 Robiginitalea_ZP_01120734 Dichelobacter_YP_001209911 Roseiflexus_YP_001431186 52 Drosophila_AAM50875 Rubrobacter_YP_645112 Escherichia_ZP_00712973 Sacchramyces_P38075 Flavobacterium_YP_001296578 Saccharum Flavobacterium_ZP_01061540 Salinibacter_83815282 Frankia_YP_710403 Salinispora_YP_001157287 Fugu Selaginella Galdieria_Gs00430 Schizophyllum_AAC28862 Gibberella_XP_389815 Schizosaccharomyces_NP_594650 Gluconacetobacter Sclerotinia_XP_001585171 Gluconobacter_YP_192380 Sorangium_YP_001615726 Gossypium_ES822756 Sphingopyxis_YP_615708 Gramella_YP_861872 Stigmatella_ZP_01466924 Haemophilus_ZP_01793932 Synechocystis_NP441623 Hahella_YP_435655 Tenacibaculum_ZP_01052536 Halorhodospira_YP_001003348 Thermosynechococcus_NP_681121 Helobdella Thiomicrospira_YP_392256 Herminiimonas_YP_001100841 Triticum Horse_XP_001501967 Vanderwaltozyma_XP_001644128 Hyphomonas_YP_759551 Verminephrobacter_YP_997327 Kluyveromyces_XP_451844 Vibrio_ZP_01866118 Kordia_ZP_02163182 Vitis_CAO61642 Laccaria_EDR13720 Volvox lentisphaera_ZP_01874593 Xanthobacter_YP_001417377 Leptospira_NP_711347 Xenopus_NP_001086328 Leptospira_YP_798481 Yarrowia_XP_502816 Limnobacter_ZP_01915478 Zea 53 Table 2. AtPPOX-2 homologs. Members of this family are listed in alphabetial order (56 sequences) Acaryochloris_YP_001516769 Medicago_AW574109 Alteromonas_ZP_01112037 Methylobacterium_ZP_01850257 Anabaena_YP_322187 Nodularia_ZP_01632312 Ananas_CO731833 Nostoc_NP_488078 Arabidopsis_NP_566081 Oceanobacter_ZP_01306347 Burkholderia_ZP_00983542 Oryza_NP_001048753 Candida_XP_716959 Ostreococcus_CAL56347 Carthamus_EL404654 Ostreococcus_XP_001420885 Centaurea_EH748604 Parvibaculum_YP_001412025 Centaurea_EH787638 Physcomitrella_EDQ64399 Chlamydomonas_XP_001700070 Picea_EX433496 Cichorium_EH680966 Pichia_XP_001484478 Coprinopsis_EAU92424 Polaribacter_ZP_01118414 Crocosphaera_ZP_00516567 Populus_ABK94044 Cucumis_CK085633 Prochlorococcus_YP_001484786 Cyanothece_ZP_01732408 Prochlorococcus_NP_893475 Debaryomyces_XP_458405 Prunus_DY642627 Flavobacteriales_ZP_01108137 Psychroflexus_ZP_01252931 Fragaria_EX662000 Raphanus_EX746271 Fulvimarina_ZP_01439324 Rhizobium_YP_766790 Gossypium_CM028803 Robiginitalea_ZP_01121883 Helianthus_EE645774 Saccharomyces_EDN61616 Laccaria_EDR15974 Synechococcus_YP_475391 Lettuce_DW169932 Trichodesmium_YP_722646 Lodderomyces_XP_001523793 Triticum_CK207357 Lycopersicon_S5289081 Ustilago_XP_759066 Lyngbya_ZP_01621013 Vanderwaltozyma_XP_001644619 Magnetospirillum_ZP_00052487 Vitis_CAO14403 54 Figure 1. Amino acid sequence alignment between AtPPOX-1 and AtPPOX-2. Amino acids identical in these two proteins are highlighted in black, and conservative substitutions are highlighted in gray. The CLUSTALW program was used for sequence alignment (Thompson et al., 1994). AtPPOX-1 1 MRNVIRRVTTMTFTFLLQSPPLPISPSPPQFSLSSSPLSKTQRFITPSQGSTLTTLCTKVIIPNMQDSGS AtPPOX-2 1 ---------------------------------------------------------------------- AtPPOX-1 71 PPLSYLTQREAAEIDETLMGPLGFLIDQLMELAGLSVAASIAEVYKPEEYSRVLAICGPGNNGGDGLVAA AtPPOX-2 1 ---------------------------------------------------------------------- AtPPOX-1 141 RHLHHFGYKPFICYPKRTAKPLYTGLVTQLDSLSVPFVSVEDLPDDLSKDFDVIVDAMFGFSFHGAPRPP AtPPOX-2 1 ---------------------------------------------------------------------- AtPPOX-1 211 FDDLIRRLVSLQNYEQTLQKHPVIVSVDIPSGWHVEEGDHEDGGIKPDMLVSLTAPKLCAKRFRGPHHFL AtPPOX-2 1 ---------------------------------------------------------------------M AtPPOX-1 281 GGRFVPPSVAEKYKLELPSYPGTSMCVRIGKPPKVDISAMRVNYVSPELLEEQVETDPTVQFTKWFDEAV AtPPOX-2 2 GTHVAP---------------------------------------WKQLLFGAIEAN------------- AtPPOX-1 351 AAGLRETNAMALSTANKDKKPSSRMVLLKGFDENG--FVWFTNYESKKGSDLSENPSAALLFYWEILNRQ AtPPOX-2 20 -SHLSHSSYVQLATIGLNGRPSNRTVVFRGFEENSDRIQINTDLRSRKIEELKHCPFSEMCWYFSDTWEQ AtPPOX-1 419 VRIEGPVERIPESESE-NYFHSRPRGSQIGAIVSKQSSVVPGRHVLYDEYEELTKQYSDGSVIPKPKNWG AtPPOX-2 89 FRINGRIEVIDASNPDQTKLQQREKAWFANSLRSRLIYVCPTPGSPCNSEQSSQQVKLDPSSGPVP-EYC AtPPOX-1 488 GFRLKPNLFEFWQGQPSRLHDRLQYS-LQDVNGNPAWKIHRLAP AtPPOX-2 158 LLLLEPEKVDYLN---LKTNQRLFFSSMATGTGEKCWTSEKVNP 55 Figure 2. Conserved regions among all AtPPOX-1 and AtPPOX-2 homologs Conserved region I Region II Region III Arabidopsis-AtPPOX-1 KKPSSRMVLLKGFDE NRQVRIEGP WKIHRLAP Nostoc-AtPPOX-1 GQPSARMVLLKDFDE ERQVRISGR WEIHRLSP Human-AtPPOX-1 GKPSARMLLLKGFGK NRQVRVEGP WLYERLAP Sacharamyces-AtPPOX-1 GRVSSRILLFKELDH QRQVRVEGI WKVVRLAP Nostoc-AtPPOX-2 GHPANRTIVFRGFLA REQFRITGQ WTIQGVNP Ostreococcus-AtPPOX-2 GAPSVRTVVFRGFLD REQFRVRGT WVSTRVNP Arabidopsis-AtPPOX-2 GRPSNRTVVFRGFEE WEQFRINGR WTSEKVNP Sacharamyces-AtPPOX-2 NKPRCRTVVFRDFLF WEQYRFSGQ WEEQEVCP 56 Figure 3. AtPPOX-1 homolog derived tree 57 Figure 4. AtPPOX-2 homolog derived tree 58 V EXPRESSIONAL ANALYSIS AND FUNCTIONAL ROLE OF PYRIDOXINE/ PYRIDOXAMINE PHOSPHATE OXIDASE-1 IN ARABIDOPSIS THALIANA ABSTRACT Pyridoxal phosphate (PLP), a vitamin B 6 vitamer, is an essential cofactor for numerous enzymes. Pyridoxine/pyridoxamine phosphate oxidase (PPOX) catalyzes the synthesis of pyridoxal phosphate from pyridoxine or pyrodoxamine. AtPPOX-1 is one of the PPOX enzymes in Arabidopsis thaliana that is involved in the salvage pathway of vitamin B 6 metabolism, and it is responsible for synthesis of PLP. In this study, regulation of the AtPPOX-1 gene expression and in vivo physiological function of AtPPOX-1 were investigated. A variable level of expression of AtPPOX-1 was seen in all tissues of A. thaliana examined. This gene is up-regualted by light, heat shock, ABA, JA and ethylene treatment, and down-regulated by exposure to NaCl. Monoclonal antibodies against different domains of ATPPOX-1 recognized different sizes of protein in root and shoot tissues suggesting expression of alternate splice variants of AtPPOX-1 in root and shoot. To determine the biological role of AtPPOX-1, T-DNA insertional mutants of A. thaliana in AtPPOX-1 were analyzed. The mutant lines showed sensitivity to NaCl and high light for growth, and sensitivity to high concentrations of sucrose relative to cotyledon development. These results suggest involvement of AtPPOX-1 in stress tolerance and cotyledon development in A. thaliana. 59 INTRODUCTION Vitamin B 6 is known for its function as an essential cofactor for numerous enzyme reactions (John, 1995). The B 6 vitamers are also excellent antioxidants comparable to vitamin E and C, and are particularly active in quenching singlet oxygen and superoxide anion (Ehrenshaft et al., 1999; Osmani et al., 1999; Jain and Lim, 2001). In plants, vitamin B 6 is involved in stress tolerance, growth and development (Shi et al., 2002; Chen and Xiong, 2005; Studart et al., 2005; Titiz et al., 2006; Wagner et al., 2006; Studart et al., 2007) . Vitamin B 6 is synthesized in plants using the DXP-independent biosynthesis pathway in which PDX1 and PDX2 proteins are involved (Studart et al., 2005). PDX1 is required for shoot and root development (Chen and Xiong, 2005). In addition to the developmental defects, PDX1 mutants are hypersensitive to salt, osmotic stress and oxidative stress (Chen and Xiong, 2005). PDX2 is involved in the seed development (Studart et al., 2005; Studart et al., 2007). SOS4 catalyzes the phosphorylation of the vitamin B6 vitamers to form the corresponding phosphorylated derivatives (Lum et al., 2002). An SOS4 mutant had very short root when treated with high salt (Shi and Zhu, 2002), and SOS4 mutants do not have root hairs in the maturation zone, suggesting that pyridoxal kinase is required for root hair development in Arabidopsis thaliana (Shi and Zhu, 2002). Pyridoxine/pyridoxamine phosphate oxidase (PPOX) is involved in the salvage pathway responsible for synthesis of PLP from PMP or PNP. A PPOX mutant of Arabidopsis showed a decrease in root and shoot growth under normal conditions, and was sensitive to high light (Gonzalez et al., 2007). 60 Regulation of PDX1 and PDX2 genes in plants has been extensively studied. PDX2 and three PDX1 genes were responsive to abiotic stressors including high light, chilling, drought, and ozone (Denslow et al., 2007). However, the response of PDX1.2 was different from that of the other PDX genes and showed lower sensitivity to high light, chilling, and drought, but an increased sensitivity to ozone (Denslow et al., 2007). PDX1and PDX2 transcript levels in Nicotiana tabacum decrease following inoculation with the incompatible pathogen Pseudomonas syringae pv. phaseolicola and transiently increased in response to salicylic acid and methyl jasmonate (Denslow et al., 2005). However, expression of PDX1 in Phaseolus vulgaris did not change with MeJA treatment. Expression of pvPDX1 was slightly up-regulated within two hourse of wounding. Treatment with ACC and GA 3 caused the greatest increase in pvPDX1 expression, while hydrogen peroxide or rose Bengal did not affect pvPDX1 expression (Graham et al., 2004). SOS4 expression was modulated by NaCl, abscisic acid, and cold treatment, but not by drought (Shi et al., 2002). In this study, we describe the expression of the AtPPOX-1 gene and its regulation by tissue specificity, abiotic stresses and hormones. Results indicat that AtPPOX-1 gene has two alternative splice variants expressed in different tissues. T-DNA insertional mutants of AtPPOX-1 in A. thaliana were analyzed for their phenotypic properties under different treatments to determine the role of AtPPOX-1 in plant growth and development. 61 RESULTS Expression of the AtPPOX-1 in different tissues of A. thaliana To determine the linear range of amplification during quantitative RT-PCR, different cycle numbers were used (Figure 1). Based on this observation 25 cycles of amplification appeared to be optimal for quantitative RT-PCR. The expression of the AtPPOX-1 in different tissues of A. thaliana was determined, and results are shown in Figure 2. AtPPOX-1 is highly expressed in leaf and stem at similar levels, but its expression is considerably less in flower. The expression of AtPPOX-1 in root is higher than that in flower, but lower than that in leaf and stem. Expression of the AtPPOX-1 protein in different tissues of A. thaliana Expression of AtPPOX-1 was determined by Western blot using anti-PPOXCT monoclonal antibody. Protein from leaf, stem, flower and root tissues demonstrated the presence of PPOX in all tissues in Western blot except in root (figure 2). However, AtPPOX-1 gene is transcribed in root which also shows PPOX activity. Two sets of SDS- PAGE for shoot and root proteins were independently probed with anti-PPOXCT and anti-PPOXNT monoclonal antibodies in a Western blot analysis. The anti-PPOXNT detected AtPPOX-1 from both shoot and root, while anti-PPOXCT detected only the AtPPOX-1 from shoot. AtPPOX-1 expressed in both shoot and root has a molecular weight of 51 kDa, while the shoot AtPPOX-1 has a molecular weight of 49 kDa (Figure 3A). 62 AtPPOX-1 protein is not localized in chloroplast On the basis of bioinformatic analysis, AtPPOX-1 protein was predicted to be localized in the chloroplast according to TargetP (http://www.cbs.dtu.dk/services/ TargetP/) and ChloroplastP (http://www.cbs.dtu.dk/services/ChloroP/) servers. To determine if the prediction is correct, intact chloroplast were isolated. Proteins from the intact chloroplast and from the supernatant of chloroplast isolation were blotted using both anti-PPOXCT and anti-PPOXNT. The AtPPOX-1 protein appears not to be present inside chloroplast (Figure 3B). Immunohistochemical analysis of AtPPOX-1 using monoclonal antibodies failed to detect the protein in any compartment of cell (results not shown). Native PAGE in-gel assay for AtPPOX-1 enzyme activity In order to determine the number of PPOX proteins in A. thaliana, native PAGE in- gel assay was performed. In native basic PAGE in-gel assay, one activity band was observed in leaf, stem and flower tissues, and root (weaker) tissue, and no PPOX activity bands were observed in silique tissue (Figure 4). Western blot using anti-PPOXCT demonstrated that the activity band in the in-gel assay was AtPPOX-1, and no activity band was detected in native acidic PAGE in-gel assays (data not shown). Regulation of the AtPPOX-1 gene The expression of AtPPOX-1 was regulated by light-dark cycles. Plants grown in dark for 72 hr have a very low expression of AtPPOX-1, but expression returned to normal once plants held in the dark were returned to light (Figure 5A). Expression of 63 AtPPOX-1 was up-regulated by high light, but down-regulated by exposure to 150mM NaCl. No substantial change in expression was noted by exposure to UV and drought treatments (Figure 5B). Heat treatment greatly increased the expression of AtPPOX-1. Ethlylene had no effect on the expression of AtPPOX-1 during an 8 hr exposure. Both ABA and JA treatments resulted in increased expression of AtPPOX-1 at 4 hr treatment, while expression levels returned to normal after 8 hr treatment (Figure 5C). Analysis of an A. thaliana mutant Six different T-DNA insertional mutant lines were obtained from ABRC stock center. These lines were self-pollinated for three generations to produce homozygous lines. All of the mutants had significant expression of AtPPOX-1 protein and RNA, and did not show any appreciable phenotypic difference, except that CS825697 with a T- DNA insertion in the promoter region of the gene showed a reduced level of AtPPOX-1 mRNA. One-week old seedlings were transferred to MS medium and MS medium supplemented with 100mM sucrose. The phenotype was observed one week after transfer. The CS825697 homozygous mutant showed a difference in growth from wild type (Figure 6). On MS medium with 100mM sucrose, CS825697 had very short cotyledonary petiole. Cotyledon of CS825697 lost function earlier than wild type cotyledon, while CS825697 has stronger true leaves and purple color of shoot which disappeared gradually over time. One-week old seedlings grown on MS medium and MS medium supplemented with 50mM, 75mM or 100mM NaCl did not show a big influence on the fresh weight of wild 64 type after two weeks growth, but the fresh weight of CS825697 was significantly increased when grown on MS medium with 50mM and 75mM NaCl, and showed a substantial reduction in fresh weight at 100mM NaCl (Figure 7A). The leaves of CS825697 mutant showed abnormal leaf development and turned yellow (Figure 7B) and had impaired primary root growth, but stronger secondary roots than of the wild type (Figure 7C) on 75mM or higher NaCl plate. One-week old seedlings were exposed to continuous light in a growth chamber with high light intensity (1000 ?mol S -1 m -2 ) for one week. Wild type seedlings continued to grow under high light intensity and fresh weight almost doubled in one week, while the CS825697 mutant stopped growing and fresh weight even decreased after one week exposure to high light intensity (Figure 8). DISCUSSION The level of AtPPOX-1 expression varied in different tissues of A. thaliana with the highest levels of mRNA found in leaf and stem tissues followed by root and flower tissues. Protein levels were consistent with the RNA levels except in the root tissues. Tissue specific expression of other genes/proteins in the vitamin B 6 pathway involving pyridoxal kinase (Lum et at., 2002), PDX1 and PDX2 (Wagner et al., 2006; Studart et al., 2007; Titiz et al., 2006) have been shown. During initial analysis of AtPPOX-1 protein in root and shoot tissues the inconsistency between RNA and protein expression was further analysed. AtPPOX-1 protein in root and shoot tissues showed variation in the size of protein and their differential recognition by ant-PPOXCT and anti-PPOXNT antibodies. SOS4 catalyzes 65 the pyridoxal kinase reaction in the vitamin B 6 pathway and is regulated by alternative splicing. Two splice variants of SOS4 are modulated by development and various environmental stresses (Shi et al., 2002). Immunochemical analysis using two different lines of monoclonal antibody against AtPPOX-1 also identified two different AtPPOX-1 proteins: one with a molecular weight of 51 kDa and the other of 49 kDa. Both of them were expressed in shoot, but only the longer transcript was expressed in root. The predicted full length amino acid sequence of AtPPOX-1 has a molecular weight of 59.4 kDa, but the mature protein is 51 kDa in size (Sang et al., 2007). There are two possible explanations for this unexpected result. Either the root or shoot tissues have different splice variants of AtPPOX-1 RNA that are preferentially translated in respective tissues or the domain of AtPPOX-1 that is recognized by these monoclonal antibodies has undergone post translational modifications. These two alternative possibilities are being examined. Alternative splicing is an important mechanism for regulating gene expression at the post-transcriptional level and contributes to proteome complexity (Lareau et al., 2004; Reddy, 2007; Stamm et al. 2005). This widespread process comprises various mechanisms such as exon skipping, mutually exclusive exons, intron retention, or the usage of alternative 5' or 3' splice sites (Cartegni et al., 2002). Alternative splicing has been extensively studied in mammals. Recent evidence indicates more than 60% of the genes in the human genome are alternatively spliced (Kim et al., 2006) compared to about 20?30% of plant genes (Campbell et al., 2006; Wang and Brendel, 2006). Although proteins from one gene have the same or similar functions, they can have different 66 characteristics, such as their binding properties, intracellular localization, enzymatic activity, regulation and stability (Stamm, 2002). Bioinformatic analysis of AtPPOX-1 suggested that the protein has three domains consisting of Pyridox_oxidase domain at the C terminal, followed by a Yjef_N domain and a putative transit peptide for localization of AtPPOX-1 to chloroplast. Our result using isolated chloroplasts did not support the information produced by bioinformatic analysis. The protein appears to be present in soluble fraction outside the chloroplast. Hence, the function of the N-terminal domain of AtPPOX-1 remains to be determined. Our effort to use immunohistochemical localization of the protein was not successful because the monoclonal antibodies did not recognize the native protein in tissue sections. Expression of AtPPOX-1 is reduced in dark and its expression returns to normal when grown under normal light. Expression of AtPPOX-1 is up-regulated by high light which may induce photoxidative stress. Under high light, wild type grew better than under normal light conditions. However, the growth of AtPPOX-1 insertional mutant line, CS825697 was inhibited. These results suggests a working hypothesis that vitamin B 6 functions as an ROS quenchers. Both PDX1 and PDX2 are regulated by light (Titiz et al., 2006; Studart et al., 2007). When exposed to NaCl, leaves of the CS825697 insertional mutant showed reduced accumulation of chlorophyll. Salt stress inhibits chlorophyll accumulation partly by reducing the rate of porphyrin formation but also by a possible reduction in the formation of chlorophyll-binding proteins (Abdelkader et al., 2007). The high salt-induced reduction of chlorophyll content is mediated by decreased synthesis of 5-aminolaevulinic acid, a 67 precursor of chlorophyll, rather than the chlorophyllase mediated degradation of chlorophyll (Conceicao, 2004). The T-DNA insertional mutant of AtPPOX-1, CS825697, shows altered development of cotyledons when grown on MS media containing high concentrations of sucrose, but not in low concentrations of sucrose or in other treatments. The result indicated that the alteration of petiole development is mediated by sucrose sensing, which suggests that AtPPOX-1 or PLP may be a component of the sucrose-signaling pathway or a sucrose sensing pathways. All of the insertional mutants of A. thaliana had substantial AtPPOX-1 protein. Our effort to obtain a highly reduced level of AtPPOX-1 by RNAi silencing did not yield any transgenic lines with substantial reduction in AtPPOX-1. Transgenic lines overexpressing AtPPOX-1 under the control of a strong promoter produced slightly higher levels of mRNA but there was no significant difference in the level of AtPPOX-1 protein (data not shown). All these results suggest that a minimal level of expression of AtPPOX-1 is required for survival of A. thaliana, and that the level of this protein expression is highly regulated. MATERIALS AND METHODS Plant materials and growth conditions Arabidopsis seeds were first placed at 4?C for at least 2 days to break the dormancy of the seeds, and then were sown by sprinkling them onto the damp soil covered with a transparent plastic cover. The cover was removed after seeds germinated. Two-week-old seedlings in the growth chamber at 22?C with continuous light were then transferred into 68 individual pots for stress treatment. When using solid media, seeds were surface sterilized, rinsed with sterile water and placed in rows onto Murashige and Skoog (MS) nutrients agar media (MP Biomedicals, Ohio). After exposure of 4?C for 2 days, the plates were placed vertically in the growth chamber at 22?C with continuous light. One-week old seedlings were then transferred to MS plates with or without treatment. Stress treatments for quantitative RT-PCR For dark treatment, four-week old Arabidopsis seedlings grown on soil were moved to a dark chamber for different length of time. Some of the plants were moved back to the light after dark treatments. For high light treatment, four-weeks old seedlings were moved to an 8 hr photoperiod at 1000 ?mol S -1 m -2 light. For UV light treatment, seedlings were moved to a UV box for 1 hr treatment at 30uJ/m?S UV light. For drought stress treatments, seedlings growing in the soil were not watered until they became wady. For NaCl treatment, seedlings were irrigated with 150mM NaCl for one week. For heat treatment, seedlings were transferred to 42?C for different times as indicated in text, table and figure legends. For ABA and JA treatment, seedlings were sprayed with 100?M ABA or 200 ?M JA and grown as indicated n text table and figure legends. For ethylene treatment, the seedlings were placed in a chamber with 100ppm ethylene. Isolation of RNA and quantitative RT-PCR A. thaliana seedlings were ground to a powder in liquid nitrogen. RNA was extracted using RNAeasy plant mini kit (Qiagen), as described in the instruction manual. Total RNA (0.4 ?g) was reverse-transcribed using the one-step RT-PCR kit (Qiagen) in a 69 50 ?l RT-PCR reaction mixture. Amplification was performed in a thermal-cycler as follows: 30 min at 50?C; 15 min at 95?C; then 1 min at 94?C; 1 min at 55?C; 1 and a half min at 72?C for 25 cycles, followed by 10 min at 72?C. CBP20 primers were added together with AtPPOX-1 primers into the reaction mixture as internal control. Primers for AtPPOX-1 were 5?- ATGAGGAATGTGATACGCAGAGTC-3? and 5?- TCATGGGGCCAATCTATGAA -3?. Primers for CBP20 were 5?-ATGGCTTCT TTGTT CAAGGAGC-3? and 5? ?TTAAGATCTTCTCTTCCGATCATC -3?. Chloroplast isolation Chloroplasts were isolated with some modification described by Locy et al., 1996. Fresh leaf tissues of A. thaliana were suspended in chilled grinding buffer (50 mM Hepes-KOH, pH 8.3, 350 mM Sorbitol, 1 mM MgCl 2 , 1 mM MnCl 2 , 2 mM EDTA, 2 mM EGTA, 0.5% BSA, 4.4 mM ascorbate), and were homogenized in a Waring Blendor equipped with razor blades at the top speed three times for 5 seconds each. The homogenate was filtered through two layers of Miracloth (Calbiochem) between two layers of cheesecloth. The filtrate was centrifuged for 5 min at 3000 rpm in a Sorvall HB- 4 rotor to pellet the crude chloroplast fraction. The pellets were gently resuspended in grinding buffer using a soft brush. The suspension was layered onto a percoll step gradient consisting of 40 and 80% (v/v) percoll. The gradients were centrifuged at 9000 rpm for 4 min at 4?C in a Sorvall HB-4 rotor with the brake turned off. The upper band containing broken membranes was separated from the middle band containing intact chloroplasts. The middle band was diluted with three times the volume of grinding buffer, and repelletted by centrifuge. The pellet was resuspended in the grinding buffer, and then 70 reloaded onto a second percoll step gradient. Resuspension buffer (50 mM Hepes-KOH, pH 8.3, 375 mM Sorbitol, 10 mM Na 2 HPO 4 , 0.96 mM DTT) was added to the material from the middle band, and after gentle mixing, the mixture was centrifuged at 4000 rpm for 4 min to wash of the percoll. The pellet was dissolved in the SDS-PAGE loading buffer or saved at -80?C for future use. Native PAGE in-gel enzyme assay for Pyridoxine/Pyridoxamine 5?-Phosphate Oxidase Basic native PAGE gel was carried out using 7.5% acrylamide separating gel (pH 8.8), 3% acrylamide stacking gel 6.8%, and Tris-glycine (pH8.3) as the running buffer. After loading samples, the electrophoresis was carried out at 4?C, and 10 mA current was applied. PPOX enzyme activity was visualized by incubating the gels in 0.2M Tris-HCl (pH 8), 1.9mM PNP, 0.1 mg/ml of nitroblue tetrazolium, 0.05mg/ml of phenazine methosulfate, and 1 ?M FMN at room temperature for 5 hours until maroon bands appeared (Kazarinoff and McCormick, 1975). Preparation of monoclonal antibody against PPOXCT and PPOXNT The recombinant proteins derived from Yjef_N domain of AtPPOX-1 (PPOXNT) and the Pyridox_oxidase domain of AtPPOX-1 (PPOXCT) were expressed and purified using the method described by Sang et al (2007). The purified recombinant proteins were treated with enterokinaseMax (Invitrogen) to remove the C-terminal 6?His and Xpress TM tag following the manufacturer?s instructions, and separated on the SDS-PAGE. The respective proteins were eluted from gel after electrophoresis using a Bio-Rad Hercules 71 whole-gel elutor (Bio-Rad). The eluted proteins were dialyzed against double-distilled water at 4?C and quantified with the Bradford microassay with BSA as the standard (Bradford, 1976). The monoclonal antibodies against PPOXNT and PPOXCT were generated in mice at Hybridoma Facility at Auburn University, AL. Immunochemical analysis For Western Blot analysis, proteins were extracted from fresh plant tissue by homogenization in liquid nitrogen and 1 volume of 50 mM Tris-HCl, pH7.5, containing 100 mM NaCl and 0.5% NP-40. Debris was removed by centrifugation at 10,000 g for 15 min at 4?C. Total protein was quantified using Bradford method, and was separated on 12.5% SDS-PAGE. For immunodetection, the protein was blotted onto a nitrocellulose membrane and blocked by incubation with Tris buffered saline (TBS; 10mM Tris-HCl, pH7.5, 0.9% NaCl) containing 0.05% Tween-20 and 5% milk powder. AtPPOX-1 was detected by incubating the blots for 1 hr with monoclonal anti-PPOXCT and anti- PPOXNT. This was followed by incubation of 30 min with a 1:5000 dilution of a donkey anti-mouse alkaline phosphatase conjugated secondary antibody. NBT and BCIP substrates were used for the detection of the blot. T-DNA insertional mutants Five lines of T-DNA insertional mutants were obtained from ABRC stock Center, Ohio State University. The mutant lines were self-pollinated for three generations to obtain homozygous lines that did not show further segregation. Total RNA was extracted from the mutant seedlings, and quantitative RT-PCR was used to determine the level of 72 AtPPOX-1 expression in each of the mutant lines. Level of AtPPOX-1 protein in these mutants was determined by Western blot using anti-PPOXCT. Seeds from the mutant lines and wild type were surface sterilized as above and plated on MS medium with 1.2% agar and pH 5.7. Plates were placed at 4 ?C for 48 hr to synchronize germination and then incubated vertically at 22 ?C under continuous light. One-week old seedlings were transferred to MS medium alone or supplemented with 100mM NaCl, 100mM Mannitol, 100mM Sucrose. Response of the mutant lines and wild type to high light was carried out at continous1000 ?mol S -1 m -2 light. Seedlings were monitored for phenotypic changes for 2 weeks, after which all plants were harvested and fresh weighs were determined. 73 Figure 1. Determination of the optimal amplification cycle during RT-PCR. Three RT-PCR reactions were retrieved from the thermocycler at the indicated cycles and analyzed on 1% agarose gel electrophoresis. Figure 2. Expression of AtPPOX-1 in different tissues of A. thaliana. The level of AtPPOX-1 RNA in different tissues was determined by quantitative RT-PCR and the result were normalized using internal, CBP20 RNA level in each reaction. Anti- PPOXCT antibody was used for determination of AtPPOX-1 protein in different tissues. 74 Figure 3. Different forms of AtPPOX-1 in root and shoot tissues (A) and localization of AtPPOX-1 protein (B). Total protein from shoot and root were separated on a 12.5% SDS-PAGE, transferred onto a nitrocellulose membrane, and then probed with anti-PPOXCT and anti-PPOXNT respectively. Total RNA from shoot and root amplified using RT-PCR and were separated on a 2% agarose gel. B) Proteins from the intact chloroplast and soluble supernatant outside intact chloroplast were analyzed by Western blot using mixture of anti-PPOXCT and anti- PPOXNT monoclonal antibodies. A) B) 75 Figure 4. Native basic PAGE in-gel assay for AtPPOX-1 enzyme activity. 144, 115, 204, 15, 44 ?g protein was loaded for leaf, stem, flower, silique, and root tissue respectively. 76 Figure 5. Regulation of AtPPOX-1 by environmental and hormone factors. A) Analysis of AtPPOX-1 expression in light-dark cycles. Control is the plants growing at 25 ?C with continuous light. B) Analysis of AtPPOX-1 expression with high light, UV light, drought and NaCl treatment. C) Analysis of AtPPOX-1 expression with heat, ABA, JA and ethylene treatment. A) B) C) 77 Figure 6. Two-week old wild type and CS825697 seedlings grown on MS agar plate with or without 100 mM sucrose. Phenotypic differences were recorded two weeks after transfer. 78 Figure 7. Sensitivity of CS825697 to NaCl. Morphology of wild type and CS825697 mutants grown on vertically placed MS agar plates supplemented with different concentrations of NaCl. Seedlings were first grown on vertical MS agar plates for seven days before being transferred to vertical agar plates without or with NaCl. The plates were placed upside down for root bending. Fresh weight and the photographs were taken 2 weeks after the transfer. Fresh weight of WT and CS825697 plants grown on MS plate supplemented with different concentrations of NaCl (A); Response of the leaves of CS825697 mutants to NaCl (B); Root growth of WT and CS825697 plants grown on MS plate supplemented with 50mM NaCl (C). A) 0 50 100 150 200 250 0mM NaCl 50mMNaCl 75mMNaCl 100mM NaCl To t a l F r e s h W e i g ht ( m g) WT CS 825697 79 B) C) 80 Figure 8. Response of wild type and CS825697 to high light exposure. One-week old seedlings were transferred to MS medium plate and placed in a chamber with high light. 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