Abstract:
The present invention makes use of a chimeric gene that, when incorporated into an appropriate host, results in the overproduction of S-adenosylmethionine without the need to supply the host with a source of untransformed methionine. The need for the methionine source is eliminated because the appropriately chosen host manufactures the amino acid on its own, and when the host is modified by the inclusion of a chimeric gene of the present invention, it transforms the methionine that is produced into S-adenosylmethionine. In addition, the same chimeric gene causes accumulation of methionine and increase in folate content in the same host. One form of the present invention is a fused gene encoding for methylene tetrahydrofolate reductase (MTHFR) made up of an N-terminal domain from a yeast organism and a C-terminal domain from a plant species. An example of a suitable plant species is  Arabidopsis thaliana . An example of a suitable yeast organism is  Saccharomyces cerevisiae.

Description:
FIELD OF THE INVENTION 
     This Application claims the benefit of U.S. Provisional Application No. 60/280,333, filed Mar. 30, 2001. 
    
    
     The U.S. Government may own certain fights in this invention pursuant to the terms of the National Science Foundation grant INB-9813999 and the National Institutes of Health grant RR09276. 
    
    
     BACKGROUND OF THE INVENTION 
     The present invention relates in general to the field of recombinant DNA species, and more particularly to the production of chimeric genes. 
     S-adenosylmethionine is an important metabolic agent that is formed in the body by the reaction of methionine, an essential amino acid, with adenosine triphosphate (ATP). S-adenosylmethionine is active in more than forty biological reactions in vivo. S-adenosylmethionine also operates in association with folic acid and vitamin B-12 as a methylating agent, and is essential for the formation of many sulfur-containing compounds in the body, including glutathione and various components of cartilaginous connective tissue. 
     The body normally generates the required level of S-adenosylmethionine directly from the amino acid methionine; however, a deficiency of methionine, folic acid, or vitamin B-12 can result in decreased levels of S-adenosylmethionine. There is interest in the effects of supplemental dosages of S-adenosylmethionine on various conditions. The interest in supplementation stems, in part, from findings that the elderly and those suffering from osteoarthritis, various liver problems, and depression typically have lowered levels of S-adenosylmethionine. It is also known that merely increasing the dietary intake of methionine does not result in an increase in the concentration of S-adenosylmethionine in the body. S-adenosylmethionine is now widely distributed as an over-the-counter dietary supplement. 
     S-adenosylmethionine is primarily used in the treatment of five conditions: depression, osteoarthritis, fibromyalgia, cirrhosis of the liver and migraine headaches. There have been numerous studies that have supported the efficacy of S-adenosylmethionine for the treatment of these conditions. It has also been recognized that S-adenosylmethionine has an excellent safety record, and is therefore appropriate for long-term use by patients. 
     A major drawback to the use of S-adenosylmethionine as a medicament is the expense. Present methods of production rely on the modification of methionine. Unfortunately, the purified methionine used as a starting material is relatively expensive. There is therefore a need for a method of production of S-adenosylmethionine that eliminates the need to provide a source of methionine. 
     SUMMARY OF THE INVENTION 
     The present invention makes use of a chimeric or “fused” gene that, when incorporated into an appropriate host, results in the overproduction of S-adenosylmethionine without the need to supply the host with a source of untransformed methionine. The need for the methionine source is eliminated by virtue of the fact that the appropriately chosen host manufactures the amino acid on its own, and when the host is modified by the inclusion of a chimeric gene of the present invention, it transforms the methionine that is produced into S-adenosylmethionine. 
     One form of the present invention is a fused gene encoding for methylene tetrahydrofolate reductase (MTHFR) made up of an N-terminal domain from a yeast organism and a C-terminal domain from a plant species. An example of a suitable plant species is  Arabidopsis thaliana . An example of a suitable yeast organism is  Saccharomyces cerevisiae.    
     Other forms of the present invention includes a recombinant DNA vector that includes the fused gene referred to above and host cells, both prokaryotic and eukaryotic, that contain the recombinant DNA vector. The present invention may also take the form of a plasmid containing the fused gene referred to above. 
     Another form of the present invention is a nucleic acid sequence of at least 14 nucleotides from the region where the two domains are joined to form the chimeric gene. Yet another form of the present invention is a purified fusion protein encoded for by the gene referred to above. 
     And yet another form of the present invention includes a recombinant DNA vector that includes the fused gene referred to above and host cells, both prokaryotic and eukaryotic, animal, yeast, or plant, that contain the recombinant DNA vector wherein the fused gene modifies methylneogenesis. The present invention may also take the form of a plasmid containing the fused gene referred to above. 
    
    
     
       BRIEF DESCRIPTION OF THE DRAWINGS 
       The above and further advantages of the invention may be better understood by referring to the following description in conjunction with the accompanying figures in which: 
         FIG. 1  depicts a map of a chimeric gene in accordance with the present invention; and 
         FIG. 2  depicts the concentration of  13 C-labeled and total S-adenosylmethionine in protein free extracts of host strains DAY4, RRY2, RRY4 and RRY5. 
         FIG. 3  depicts intracellular levels of S-adenosylmethionine (A) and free methionine (B) in yeast strains DAY4, SCY6 and SCY4. 
     
    
    
     DETAILED DESCRIPTION OF THE INVENTION 
     While the making and using of various embodiments of the present invention are discussed herein in terms of recombinant yeasts and a method of producing them, it should be appreciated that the present invention provides many applicable inventive concepts that can be embodied in a wide variety of specific contexts. The specific embodiments discussed herein are merely illustrative of specific ways to make and use the invention and are not meant to limit the scope of the invention in any way. 
     Definitions 
     Terms used herein have meanings as commonly understood by a person of ordinary skill in the areas relevant to the present invention. Terms such as “a,” “an,” and “the” are not intended to refer to only a singular entity, but include the general class of which a specific example may be used for illustration. The terminology herein is used to describe specific embodiments of the invention, but their usage does not limit the invention, except as outlined in the claims. 
     For convenience, certain terms employed in the specification, examples, and appended claims are collected here. 
     As used herein, the term “nucleic acid” refers to polynucleotides such as deoxyribonucleic acid (DNA), and, where appropriate, ribonucleic acid (RNA). The term should also be understood to include, as equivalents, analogs of either RNA or DNA made from nucleotide analogs, and, as applicable to the embodiment being described, single (sense or antisense) and double-stranded polynucleotides. 
     As used herein, the terms “gene”, “recombinant gene” and “gene construct” refer to a nucleic acid having an open reading frame encoding a polypeptide, such as a polypeptide, including both exon and (optionally) intron sequences. In yet another embodiment, the nucleic acid is DNA or RNA. 
     The term “fused gene” and “chimeric gene” are used interchangeably, and refer to a functional gene that has a regulatory domain from one organism and the catalytic domain from another, that have been spliced together using recombinant DNA techniques. The two domains may be attached directly to one another, or they may be connected using intervening nucleic acid sequences. The term “intervening nucleic acid sequences” means any segment of DNA used to connect the two domains that make up the “fused gene.” 
     “Domain” refers to a discreet region of a protein that performs a specific function. “N-terminal domain” and “C-terminal domain” refer to the relative end of the protein that is ultimately produced by the expression of a gene. “C” and “N” refer to the carboxyl and amino terminal ends of the protein, respectively. 
     “Regulatory sequences” of nucleic acids is a generic term used throughout the specification to refer to DNA sequences, such as initiation signals, enhancers, and promoters, as well as polyadenylation sites, which induce or control transcription of protein coding sequences with which they are operably linked. In some embodiments, transcription of a recombinant gene is under the control of a promoter sequence (or other transcriptional regulatory sequence) that controls the expression of the recombinant gene in a cell-type in which expression is intended. It will also be understood that the recombinant gene can be under the control of transcriptional regulatory sequences that are the same or which are different from those sequences and which control transcription of the naturally occurring form of the gene. 
     When referring to proteins, “regulatory domains” are the portion of a protein that controls the activity of the catalytic domain of that protein. In the present invention, the regulatory domain is the sequence that controls the activity of methylene tetrahydrofolate reductase. 
     “Catalytic domain” refers to DNA sequences that ultimately encode for amino acid sequences that form an enzymatically active protein. In the present case, that is the DNA sequence that ultimately encodes methylene tetrahydrofolate reductase. When referring to a protein, a “catalytic domain” is the portion of the protein that produces the enzymatic activity associated with the protein. 
     “Cells” or “cell cultures” or “recombinant host cells” or “host cells” are often used interchangeably as will be clear from the context. These terms include the immediate subject cell which expresses, e.g., the methylene tetrahydrofolate reductase encoded for by the fused gene of the present invention. It is understood that not all progeny are exactly identical to the parental cell, due to chance mutations or difference in environment. Such altered progeny are included in these terms, so long as the progeny retain the characteristics relevant to those conferred on the originally transformed cell. 
     As used herein, the term “vector” refers to a nucleic acid molecule capable of transporting another nucleic acid to which it has been linked. The term “expression vector” includes DNA expression constructs, e.g., nucleic acid segments, plasmids, cosmids, phages, viruses or virus particles capable of synthesizing the subject proteins encoded by their respective recombinant genes carried by the vector. Alternatively, nucleic acid segments may also be used to create transgenic cells using non-directional or even homologous recombination. Vectors for use with the invention are those capable of autonomous replication and/or expression of nucleic acids to which they are linked. In the present specification, “plasmid” and “vector” are used interchangeably as the plasmid is the most commonly used form of a vector. Moreover, the invention is intended to include such other forms of expression vectors that serve equivalent functions and which become known in the art subsequently hereto. 
     “Homology” and “identity” each refer to sequence similarity between two polypeptide sequences, with identity being a more strict comparison. Homology and identity can each be determined by comparing a position in each sequence that may be aligned for purposes of comparison. When a position in the compared sequence is occupied by the same amino acid residue, then the polypeptides can be referred to as identical at that position; when the equivalent site is occupied by the same amino acid (e.g., identical) or a similar amino acid (e.g., similar in steric and/or electronic nature), then the molecules can be referred to as homologous at that position. 
     A percentage of homology or identity between sequences is a function of the number of matching or homologous positions shared by the sequences. An “unrelated” or “non-homologous” sequence shares less than 40 percent identity, though it may be less than 25 percent identity, with a reference sequence. An “unrelated” or “non-homologous” sequence can also be referred to as not being “substantially homologous” to the reference sequence. The terms “homology” and “similarity” are used interchangeably herein. 
     By “purified”, it is meant, when referring to the component proteins preparations used to generate the reconstituted protein mixture, that the indicated molecule is present in the substantial absence of other biological macromolecules, such as other proteins (particularly other proteins that may substantially mask, diminish, confuse or alter the characteristics of the component proteins either as purified preparations or in their function in the subject reconstituted mixture). 
     The term “purified” as used herein preferably means at least 80% by dry weight, 95-99% by weight or even 99.8% by weight, of biological macromolecules of the same type present (but water, buffers, and other small molecules, especially molecules having a molecular weight of less than 5000, may be present). The term “pure” as used herein preferably has the same numerical limits as “purified” immediately above. “Isolated” and “purified” do not encompass either protein in its native state (e.g., as a part of a cell), or as part of a cell lysate, or that have been separated into components (e.g., in an acrylamide gel) but not obtained either as pure (e.g., lacking contaminating proteins) substances or solutions. 
     The term “isolated” as used herein may also refer to a component protein that is substantially free of cellular material or culture medium when produced by recombinant DNA techniques, or chemical precursors or other chemicals when chemically synthesized. 
     The term “recombinant protein” refers to a protein that is produced by recombinant DNA techniques, wherein generally DNA encoding the protein is inserted into a suitable expression vector that is in turn used to transform a host cell to produce the heterologous protein. Moreover, the phrase “derived from”, with respect to a recombinant gene, is meant to include within the meaning of “recombinant protein” those proteins having an amino acid sequence corresponding to a naturally occurring protein or an amino acid sequence similar thereto that is generated by mutations including substitutions and deletions. 
     All technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art to which this invention belongs, unless defined otherwise. Methods and materials similar or equivalent to those described herein may be used in the practice or testing of the present invention, the generally used methods and materials are now described. 
     Inserting Chimeric Genes into Plant Cells 
     A variety of methods may be used to insert foreign DNA, e.g., the chimeric genes of the present invention into plant cells. One such method, involves inserting a chimeric gene into Ti plasmids carried by  A. tumefaciens , and co-cultivating the  A. tumefaciens  cells with plants. In this process, a segment of T-DNA carrying the chimeric gene is transferred into the plant genome, causing transformation. 
     A variety of other methods are listed below. These methods are capable of inserting the chimeric genes of this invention into plant cells, although the reported transformation efficiencies achieved to date by such methods have been low. The chimeric genes of this invention (especially those chimeric genes such as neomycin phosphotransferase I and II, NPTI and NPTII, respectively, which may be used as selectable markers because the gene codes for the aminoglycoside 3′-phosphotransferase enzyme that inactivates by phosphorylation a range of aminoglycoside antibiotics) are likely to facilitate research on methods of inserting DNA into plants or plant cells. 
     While only relatively small DNA molecules have been transferred into plant cells by means of liposomes, and none have yet been expressed, future, liposome-delivery technology may be developed, to transfer plasmids containing the chimeric genes of this invention into plant cells by means involving liposomes. Another technique involves contacting plant cells with vector DNA that is complexed with either (a) polycationic substances, such as poly-L-ornithine, or (b) calcium phosphate. Although efficiencies of transformation achieved to date have been low, these methods may be used as selection of the transformants is possible. 
     Another method involves fusing bacteria that contain desired plasmids with the plant cells. Such methods involve converting the bacteria into spheroplasts and converting the plant cells into protoplasts. Both of these methods remove the cell wall barrier from the bacterial and plant cells, using enzymatic digestion. The two cell types can then be fused together by exposure to chemical agents, such as polyethylene glycol. Although the transformation efficiencies achieved to date by this method are low, similar experiments using fusions of bacterial and animal cells have produced good results. 
     Other methods that may be used to genetically transform animal cells involve (a) direct microinjection of DNA into animal cells, using very thin glass needles, and (b) electric-current-induced uptake of DNA by animal cells, or electroporation. These techniques may also be used to transform other eukaryotic cells. 
     S-adenosylmethionine, herein interchangeably referred to as AdoMet, is active in more than forty biological reactions in vivo. It operates in association with folic acid and vitamin B-12 as a methylating agent, and is also essential for the formation of many sulfur-containing compounds in the body, including glutathione and various components of cartilaginous connective tissue. S-adenosylmethionine has been known to be a substance having a therapeutic effect on jecur adipsum, lipema and arteriosclerosis. 
     This invention describes a DNA sequence of recombinant plant-yeast hybrid methylene tetrahydrofolate reductase (E.C. #1.5.1.20) that consists of the cDNA sequence encoding for the catalytic aminoterminal domain of yeast MTHFR (MET13), joined to the cDNA sequence encoding the regulatory carboxyterminal domain of MTHFR from the plant  Arabidopsis thaliana  (AtMTHFR-1). 
     The DNA sequences of MET13 and AtMTHFR-1 are SEQ ID NO.: 1 and SEQ ID NO.3, respectively. The protein sequences of MET13 and ATMTHFR-1 are SEQ ID NO.: 2 and SEQ ID NO.: 4, respectively. The hybrid is coded for by a fusion gene made from a DNA fragment composed of base 826 to base 1824 of SEQ ID NO.: 1 that is fused to another DNA fragment composed of base 1107 to base 1838 of SEQ ID NO.: 3. A 42-base DNA sequence that codes for the 14 amino acid sequence where the two fragments that make up the hybrid are joined is given in SEQ ID NO.: 13. The DNA sequence of SEQ ID NO.: 13 codes for seven amino acids from each fragment that makes up the hybrid. 
     MET13 encodes an S-adenosylmethionine-sensitive, NADPH dependent enzyme. AtMTHFR-1 encodes an S-adenosylmethionine-insensitive, NADH-dependent enzyme. The hybrid encodes an S-adenosylmethionine-insensitive enzyme that can use both NADPH and NADH, and has novel combined catalytic and regulatory properties of both its parents. When the two yeast genomic MTHFR DNA sequences (genes MET12 and MET13) encoding S-adenosylmethionine-sensitive, NADPH-dependent proteins, are replaced with DNA encoding the hybrid MTHFR, yeast cells accumulate a high level of S-adenosylmethionine. 
     EXAMPLE 
     The present invention makes use of a chimeric gene that when incorporated into an appropriate host results in the over production of S-adenosylmethionine, without the need to supply the host with a source of untransformed methionine. The hyperaccumulation of S-adenosylmethionine is accompanied by an increased accumulation of methionine and more than twice the total folate content (as compared to a host expressing a wild-type gene). The overaccumulation of methionine and S-adenosylmethionine in yeast strains engineered with ChimeraI demonstrates that allosteric inhibition of MTHFR by S-adenosylmethionine controls or modifies methylneogenesis, and hence, the commitment of Carbon-1 units to methylneogenesis. Chemicals Used 
     [ 14 C]Formaldehyde (53 mCi mmol −1 ) was purchased from NEN Life Science Products, and (6R, 6S)-[methyl- 14 C]CH 3 -tetrahydrofolic acid (“CH 3 -THF”) (56 mCI mmol 1 ) from Amersham Pharmacia Biotech; specific radioactivities were adjusted to the desired values with unlabeled compound. (6R, 6S)-THF and (6R, 6S)-CH 3 -THF were obtained from Schircks Laboratories (Jona, Switzerland). The purity of THF was 86%, estimated by letting the NADH—CH 2 -THF oxidoreductase reaction go to completion. CH 3 -THF and  14 CH 3 -THF were dissolved in 8 mM sodium ascorbate and stored at −80 degrees Centigrade. THF was dissolved just before use in N 2 -gassed 0.25 M triethanolamine-HCl, pH 7, containing 40 mM 2-mercaptoethanol. Glucose-6-phophate dehydrogenase (recombinant  Leuconostoc mesenteroides  enzyme) and all other biochemicals were from Sigma. Enzyme Isolation 
     All operations were at about 0–10 degrees Centigrade. Yeast cultures were grown to an A 600  of at least about 1–2, washed, and broken by agitation with glass beads in 100 mM potassium phosphate buffer, pH 6.8 or 7.2, containing 1 mM EDTA, 12–25 micromolar FAD, and 10% (v/v) glycerol (Buffer A) plus 1 mM PMSF. Extracts were cleared by centrifugation (25,000×g, 30 minutes), desalted on PD-10 columns (Amersham Pharmacia Biotech) equilibrated in buffer A, and concentrated if necessary in Centricon-30 units (Amicon). Extracts were stored at −80 degrees Centigrade after freezing in liquid N 2 ; this did not affect MTHFR activity. Protein was estimated by Bradford&#39;s method using bovine serum albumin as the standard. 
     Assays for MTHFR Activity 
     Assays were made under conditions in which substrates were saturating and product formation was proportional to enzyme concentration and time. NAD(P)H-CH 2 -THF oxidoreductase activity was measured in reaction mixtures (final volume 20 microliters, in 2-mL screw-cap microcentrifuge tubes) containing 100 mM potassium phosphate buffer, pH 7.2, 0.3 mM EDTA, 4 mM 2-mercaptoethanol, 42 nmol (0.1 μCi) of [ 14 C]formaldehyde, 20 nmol of THF, 0.5 nmol of FAD, 4 nmol of NAD(P)H, 20 nmol of glucose 6-phosphate, 0.06 units of glucose-6-phosphate dehydrogenase (1 unit=1 micromole of NADC reduced min −1  at pH 7.2, 24 degrees Centigrade), and enzyme preparation. 
     Blank assays contained no NAD(P)H. The buffer, EDTA, [ 14 C]formaldehyde, THF, and 2-mercaptoethanol were mixed and held for 5 minutes at 24 degrees Centigrade in hypoxic conditions (to allow  14 CH 2 -THF to form) before adding other components. Reactions were incubated at 30 degrees Centigrade for 20 minutes, and stopped by adding 1 mL of 100 mM formaldehyde. 
     After standing for 20 minutes at 24 degrees Centigrade (to allow  14 C to exchange out of CH 2 -THF), 0.2 mL of a slurry of AG-50(H + ) resin (1:1 with water) was added to bind  14 CH 3 -THF. The resin was washed with 3×1.5 mL of 100 mM formaldehyde, mixed with 1 mL of scintillation fluid, and counted. The counting efficiency was 40%, determined using assays spiked with  14 CH 3 -THF. 
     Construction of Chimeric Enzyme 
     ChimeraI was constructed by a PCR-based approach. Alternative construction methods such as selective restriction fragment cloning using sticky ends, or even blunt end ligations may also be used. A map of ChimeraI is depicted in  FIG. 1 . The DNA fragments encoding the N-terminal domain of Met13 (5′-met13 fragment) and the C-terminal domain of AtMTHFR-1 (3′-AtMTHFR-1 fragment) were amplified separately by PCR and joined using a short overlap sequence. The following primer pairs were used: 
     A. For the amplification of the DNA fragment encoding the N-terminal domain of Met13 (5′-met13 fragment):
         &gt;MET13-5PRIME (SEQ ID NO.: 5)   5′-CATGAAGATCACAGAAAAATTAGAGC-3′   &gt;MET13-1-SOER (SEQ ID NO.: 6)   5′- GGTTTGCCCAGAAGATAGG TCTGACTTCC-3′   B. For the amplification of the DNA fragment encoding the C-terminal domain of AtMTHFR-1 (3′-AtMTHFR-1 fragment):   &gt;W43486-1-SOEF (SEQ ID NO.: 7)   5- CCTATCTTCTGGGCAAACC GTCCAAAGAGC-3′   W43486-3PRIME (SEQ ID NO.: 8)   5′TGCACTGCAGTCAAGCAAAGACAGAGAAG-3′       

     Pst I 
     The reaction mixtures for PCR amplification contained:
         5 μL each primer (5 μM stock)   1 μL dNTP mixture (10 mM stock of each dATP, dGTP, dTTP, and dCTP)   2 μL (5 units) Pfu turbo polymerase (Stratagene)   5 μL 10× buffer for Pfu polymerase   2 μL (100 ng) met 13 cDNA or AtMTHFR-1 cDNA   30 μL water       

     The PCR products were run on 1% low-melting agarose gel, the amplified DNA bands were cut out and purified over the Wizard DNA purification minicolumn (Promega). Final volume of each sample was 50 μL. 
     The two fragments (5′-met13 and 3′-AtMTHFR-1) were then joined by a second round of PCR as follows: 
     PCR reaction mix contained:
         5 μL MET13-5PRIME primer (5 μM stock)   5 μL W43486-3PRIME primer (5 μM stock)   1 μL dNTP mixture (10 mM stock of each dATP, dGTP, dTTP, and dCTP)   2 μL (5 units) Pfu turbo polymerase (Stratagene)   5 μL 10× buffer for Pfu polymerase   2 μL (out of 50 1L) of the 5′-met13 fragment amplified in the first step of PCR   2 μL (out of 50 μL) of the 3′-AtMTHFR-1 fragment amplified in the first step of PCR   28 μL water       

     The obtained full-length PCR fragment, ChimeraI, was run on 1% low-melting agarose gel, the amplified DNA band was cut out and purified over the Wizard DNA purification minicolumn (Promega). 
     For the enzyme kinetics studies, the PCR product obtained was inserted into the yeast expression vector pVT103-U as follows: The ChimeraI PCR fragment was digested with PstI restriction enzyme. The digested fragment was run on 1% low-melting agarose gel, cut out, and purified over the Wizard DNA purification minicolumn (Promega). 
     The yeast expression vector pVT103U was prepared for ligation of the insert as follows: The vector was linearized with BamHI, ethanol precipitated, resuspended in water, and treated with T4 polymerase. Reaction was stopped by heating at 70 degrees Centigrade for 15 minutes, followed by chloroform extraction and ethanol precipitation. The fragment was then resuspended in water and digested with Pst I, run on 1% low-melting agarose gel and purified over the Wizard column as before. 
     The purified vector (pVT103U) fragment and the purified ChimeraI fragment were mixed, ligated overnight, and introduced by electroporation into competent  E. coli DH 10B cells. The identity of the construct was verified by restriction digests and by DNA sequencing. 
     The resulting construct (pChimeraI) was then introduced into RRY3 (Δmet12Δmet13) yeast strain for expression and enzyme kinetics studies. 
     Strain Construction 
     The pVT-Chimeral plasmid containing the yeast MET13 gene with its putative regulatory carboxyl terminal domain replaced by the corresponding domain of the AtMTHFR-1 gene from  Arabidopsis thaliana  was used as template for construction of strains RRY4 and RRY5. The Chimeral gene (CHIMERAL) was amplified with primers 5′-CAACAGGTTCATGCCACTGG-3′ (MTR2.1, SEQ ID NO.: 9) and 5′-ACAATGGAAAAGGAAGGAGCAAAATCTGGT-AAAAATTCTCGGAGATCAAGCA-3′, (Chimera-R1, SEQ ID NO.: 10); sequence homologus to yeast MET13 gene in bold). 
     The 1.4 Kbp CHIMERAI fragment was gel purified using the QIAquick gel extraction kit (Qiagen) and used to transform the methionine requiring strains RRY1 (MET12 Δmet13) and RRY3 (Δmet12 Δmet13). Transformants were selected by methionine prototrophy indicating successful integration of the CHIMERAI fragment at the disrupted met13 locus. Integration was confirmed by PCR on genomic DNA from RRY4 (MET12 CHIMERAI) and RRY5 (Δmet12 CHIMERAI) using primers 5′-AAGGTGATATTTCGCTCGTGG-3′(M13-USF, SEQ ID NO.: 11) and 5′-ATGGATCCGGGTGTTAACCAA-3′(M13-DSR, SEQ ID NO.: 12). 
     Preparation of Extracts for NMR Analysis 
     Yeast were grown in 500 mL cultures supplemented with  13 C-labeled glycine or formate as indicated. Cells were harvested at an OD 600  of approximately 3-5 and washed with sterile water. Extracts used for measurement of labeled choline and purines were prepared by resuspending the cell pellets in 30 mL of 0.3 N HCl and heating over a steam bath for 1.5 hours. Samples were centrifuged for 10 minutes at 10,000× g to pellet the cellular debris. The supernatant was evaporated in a Rotavapor-R evaporator, dissolved in 1 mL D 2 O, and submitted for NMR analysis. 
     Extracts used for measurement of  13 C-labeled S-adenosylmethionine were prepared by resuspending the cell pellet in 500 mL sterile water and lysing the cells with glass beads by vortexing continuously at 4 degrees Centigrade for 20-30 minutes. Lysates were clarifed by centrifugation at 13,000× g for 15 minutes. Proteins were precipitated by adding 95% ethanol to a final concentration of approximately 60-70% to the crude extract. The samples were incubated on ice for 20 minutes and precipitated proteins were collected by centrifugation at 13,000× g for 15 minutes. The supernatant was evaporated down, dissolved in D 2 O and used to measure the  13 C labeling of S-adenosylmethionine via NMR. 
     NMR Analysis 
     NMR spectra were obtained on a Varian Unity-Inova Spectrometer with an  1 H frequency of 500 MHz and a  13 C frequency of 125 MHz.  13 C data were collected with an acquisition time of 1.3-sec with a 3-sec delay and 90 degree pulse angle. Two level composite pulse was used for proton decoupling with a power level of 48 dB during acquisition and 40 dB during delay. A total of 200-2000 scans of 64K data points were acquired over a sweep width of 25 kHz. Data processing included exponential line broadening of 1 Hz. 
     Metabolites were identified based on the value of the chemical shifts observed from the natural abundance spectra of standard samples. The extent of the labeling of choline and purines was determined by dividing the peak integral values of the various labeled positions (C1 and C4 for choline; C2 and C8 for purines) by the peak integral value at the position derived directly from glycine (C2 for choline and C5 for purines). The ratios were normalized by dividing the sample ratio by the same ratio derived from the natural abundance spectra of a standard sample. The amount of  13 C-labeled S-adenosylmethionine was calculated by comparing the NMR peak heights to a standard sample of known concentration.  FIG. 2  depicts a comparison of the concentration of  13 C labeled and total S-adenosylmethionine in protein free extracts of hosts strains DAY4, RRY2, RRY4 and RRY5. 
     HPLC Analysis 
     The method of Wise, et al. was used to measure the concentration of S-adenosylmethionine in protein-free extracts using HPLC. Twenty μl of sample was injected into a Waters HPLC attached to a Waters Spherisorb ODS2, 250×4.6 mm (5 μm particle size) column with a guard column. A Waters Lambda-Max Model 481 LC Spectrophotometer was used for detection at 254 nm. The mobile phase consisted of 50 mM NaH 2 PO 4 , 10 mM heptanesulfonic acid (Sigma) and 20% methanol adjusted to a pH of 4.38 with phosphoric acid. Samples were run at a rate of 0.8 mL/min. Standard samples of S-adenosylmethionine (Sigma) ranging from 2.3 to 210 μg/mL in deionized H 2 O were run before the experimental samples. 
     Determination of Methionine 
     To determine methionine, 200-mg samples of wet cells were suspended in 180 μL of water and heated at 100 degrees Centigrade for 5 minutes. After cooling on ice, cells were extracted essentially as above except that protein was precipitated with 5-sulfosalicylic acid (final concentration 3.5%). The deproteinized samples were submitted to Biosynthesis Inc. (Lewisville, Tex.) for amino acid analysis using a Beckman 7300 analyzer. 
     Intracellular levels of S-adenosylmethionine (A) and free methionine (B) in yeast strains DAY4, SCY6 and SCY4 are shown in  FIG. 3 . Cells were grown in synthetic minimal medium supplemented with glycine, formate, leucine, histidine, trytophan, and uracil and harvested at an absorbance reading of 2.6–2.9 (at 600 nm) (Roje S, et al., Metabolic Engineering in Yeast Demonstrates That S-Adenosylmethionine Controls Flux Through the Methylenetetrahydrofolate Reductase Reaction in Vivo, 2002 277:4056-61, relevant portions incorporated herein by reference). S-adenosylmethionine data are means of duplicate determinations on the same samples with standard error values less than or equal to 1% of the means. Strain SCY4 expressing the chimeric MTHFR hyperaccumulated S-adenosylmethionine compared to strain DAY4. The hyperaccumulation was observed in cultures harvested at a range of cell densitites; its magnitude varied from 75-fold to 254-fold above wild-type in four independent experiments. In addition, this strain accumulated 7-fold more methionine than DAY4. 
     Folate Determination 
     Yeast strains were grown, harvested, and washed as described above for S-adenosylmethionine and methionine determination. Pelleted cells were suspended in twice their wet weight of extraction buffer (50 mM HEPES, 50 mM 2-(cyclohexylamino)ethanesulfonic acid, 0.2 M 2-mercaptoethanol, and 2% (w/v) sodium ascorbate, pH 7.9). Glass beads were added at 1.5 times the wet weight of the pellet. The samples were heated at 100 degrees Centrigrade for 10 minutes and lysed by votexing for 4 minutes. After centrifugation at 20,000× g for 30 minutes, supernatants were decanted, their volumes were measured, and they were stored at −70 degrees Centigrade until analysis. Folate species were separated by HPLC and quantitated using the  Lactobacillus casei  microbiologic assay. 
     Yeast were grown in minimal medium supplemented with glycine, formate, leucine, histidine, tryptophan, and uracil. Folate species as determined by HPLC are shown in the TABLE where data are means of duplicates. 
     
       
         
               
             
               
               
               
               
               
             
           
               
                 TABLE 
               
             
             
               
                   
               
               
                 Folate Levels in DAY4 and SCY4 Yeast Strains 
               
             
          
           
               
                   
                 10-CHO- 
                   
                 5-CHO- 
                 5-CH 3 - 
               
               
                 Strain 
                 THF 
                 THF 
                 THF 
                 THF 
               
               
                   
               
               
                 DAY4 (MET13) 
                  6.5 
                  4.3 
                  6.2 
                  49.2 
               
               
                 SCY4 (Δmet13 CHIMERA-1) 
                 19.9 
                 14.1 
                 13.5 
                 108.4 
               
               
                   
               
               
                 All units in nmol/g (wet weight) 
               
             
          
         
       
     
     The TABLE illustrates that the most abundant folate in all strains was 5-CH 3 -THF, constituting at least or more than 68% of the total folate pool. The most striking difference between strains was that SCY4 expressing ChimeraI had more than twice the total folate content of the wild-type strain DAY4, although the relative amounts of the individual folates were essentially unchanged. 
     Although the invention has been described in connection with specific embodiments, it should be understood that the invention as claimed should not be unduly limited to such specific embodiments. Modifications and variations of the described compositions and methods of the invention will be apparent to those skilled in the art without departing from the scope and spirit of the invention. Indeed, various modifications of the described compositions and modes of carrying out the invention that are obvious to those skilled in molecular biology or related arts are intended to be within the scope of the following claims.