WO2012036151A1 - 含硫アミノ酸生産菌及び含硫アミノ酸の製造法 - Google Patents
含硫アミノ酸生産菌及び含硫アミノ酸の製造法 Download PDFInfo
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- C07K14/24—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from bacteria from Enterobacteriaceae (F), e.g. Citrobacter, Serratia, Proteus, Providencia, Morganella, Yersinia
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- C07K14/24—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from bacteria from Enterobacteriaceae (F), e.g. Citrobacter, Serratia, Proteus, Providencia, Morganella, Yersinia
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Definitions
- the present invention relates to a process for producing a sulfur-containing amino acid such as L-cysteine or a related substance, and more specifically, a bacterium suitable for producing a sulfur-containing amino acid or a related substance, and a sulfur-containing amino acid or a related substance using the same. It relates to the manufacturing method. Sulfur-containing amino acids and related substances are used in the fields of pharmaceuticals, cosmetics and foods.
- L-cysteine has been obtained by extraction from keratin-containing substances such as hair, horns and feathers, or by microbial enzyme conversion using DL-2-aminothiazoline-4-carboxylic acid as a precursor.
- mass production of L-cysteine by an immobilized enzyme method using a novel enzyme is also planned.
- production of L-cysteine by fermentation using microorganisms has also been attempted.
- Patent Document 1 a coryneform bacterium having an increased intracellular serine acetyltransferase activity (Patent Document 1) is known.
- Patent Document 2 a technique for enhancing L-cysteine production ability by retaining a mutant serine acetyltransferase in which feedback inhibition by L-cysteine is reduced is known (Patent Documents 2 to 4).
- Microorganisms whose L-cysteine production ability is enhanced by suppressing the L-cysteine decomposition system include cystathionine- ⁇ -lyase (Patent Document 2), tryptophanase (Patent Document 5), O-acetylserine sulfate. Coryneform bacteria or Escherichia bacteria in which the activity of hydrhydrase B (Patent Document 6) is reduced or deleted are known.
- Non-patent Document 1 a mar gene locus, emr gene locus, acr gene locus, cmr gene locus, mex gene, bmr gene, or qacA gene, which is a gene encoding a protein suitable for excretion of a substance toxic to cells (Patent Document 7) ), Or emrAB, emrKY, yojIH, acrEF, bcr, or cusA gene (Patent Document 8) to increase the expression of L-cysteine.
- Escherichia coli in which the activity of a positive transcriptional regulator of the cysteine regulon encoded by the cysB gene is known as an L-cysteine-producing bacterium.
- methionine is industrially produced as a DL form mainly by chemical synthesis.
- the L form is required, it can be produced by acetylating the DL form to N-acetyl-DL-methionine and enzymatically deacetylating only the L form.
- production of L-methionine by fermentation using microorganisms has also been attempted.
- the L-methionine-producing bacterium the L-methionine biosynthetic repressor is deleted, the intracellular homoserine transsuccinylase activity is enhanced, and the intracellular S-adenosylmethionine synthetase activity is weakened.
- Patent Document 12 shows L-threonine requirement and has enhanced intracellular cystathionine ⁇ -synthase activity and aspartokinase-homoserine dehydrogenase II activity.
- the yeeE gene is registered in the database EcoCyc (Non-patent Document 2) as a gene encoding a protein (putative transport system permease protein) presumed to be involved in membrane permeation. Moreover, when analyzed using the membrane protein prediction program SOSUI (http://bp.nuap.nagoya-u.ac.jp/sosui/sosui_submit.html), YeeE is predicted to be a 9-transmembrane membrane protein. Is done. Therefore, although it is presumed to be some kind of transporter, the actual function is unknown, and its relation to sulfur-containing amino acid production is not known.
- the yeeE gene is cadmium (Non-patent Document 3), zinc (Non-patent Document 4), and CORM-2, which is a CO-releasing agent (Non-patent Document 5). It has been reported that it is up-regulated by Patent Document 6) and a temperature condition of 37 ° C., which is the human body temperature (Non-Patent Document 7). Further, it is reported that it is down-regulated by acetic acid (Non-patent Document 8), by ursolic acid (Non-patent Document 9), and in the IHF ( ⁇ ) strain (Non-patent Document 10). However, all of them are only listed as one of many genes whose expression has changed in microarray experiments, and no association with sulfur-containing amino acid production has been suggested.
- JP 2002-233384 A Japanese Patent Laid-Open No. 11-155571 US Patent Application Publication No. 20050112731 US Pat. No. 6,218,168 JP 2003-169668 A JP-A-2005-245311 US Pat. No. 5,972,663 JP 2005-287333 A International pamphlet No. 01/27307 US Pat. No. 5,856,148 US Patent Application Publication No. 20050009162 US Patent No. 7611873
- the present invention develops a novel technology for improving the ability of bacteria to produce sulfur-containing amino acids, and provides a method for producing sulfur-containing amino acid-producing bacteria and sulfur-containing amino acids or related substances using the bacteria, or a mixture thereof.
- the issue is to provide.
- the present inventor can improve the ability to produce sulfur-containing amino acids by modifying bacteria so that the activity of the protein encoded by the yeeE gene is increased.
- the present invention has been completed. That is, the present invention is as follows. (1) Bacteria belonging to the family Enterobacteriaceae, which have the ability to produce sulfur-containing amino acids and have been modified so that the activity of the protein encoded by the yeeE gene is increased. (2) The bacterium in which the activity of the protein is increased by increasing the expression amount of the yeeE gene or increasing the translation amount of the yeeE gene.
- the bacterium, wherein the protein is the protein described in (A) or (B) below.
- A) A protein consisting of the amino acid sequence shown in SEQ ID NO: 14.
- B) The amino acid sequence shown in SEQ ID NO: 14 has an amino acid sequence including substitution, deletion, insertion, or addition of one or several amino acids, and contains sulfur when the intracellular activity is increased. A protein that improves amino acid production.
- the bacterium, wherein the yeeE gene is the DNA described in the following (a) or (b).
- (B) hybridizes under stringent conditions with a DNA consisting of the base sequence shown in SEQ ID NO: 13; or (b) a base sequence complementary to the base sequence shown in SEQ ID NO: 13 or a probe which can be prepared from the base sequence. And a DNA encoding a protein whose ability to produce sulfur-containing amino acids is improved when the intracellular activity is increased.
- the bacterium having at least one of the following properties. i) Modified to increase serine acetyltransferase activity. ii) It has been modified to increase the expression of the ydeD gene. iii) modified to increase 3-phosphoglycerate dehydrogenase activity.
- the bacterium as described above, wherein the bacterium is an Escherichia bacterium.
- the bacterium as described above, wherein the bacterium is Escherichia coli.
- the bacterium as described above, wherein the bacterium is a Pantoea bacterium.
- the bacterium as described above, wherein the bacterium is Pantoea ananatis.
- the bacterium is cultured in a medium, and a sulfur-containing amino acid or a related substance thereof, or a mixture thereof is collected from the medium, or a sulfur-containing amino acid or a related substance thereof, or a mixture thereof Manufacturing method.
- the method as described above, wherein the sulfur-containing amino acid is L-cysteine.
- the method as described above, wherein the sulfur-containing amino acid is L-cysteine and the related substance is cystine or a thiazolidine derivative.
- the ability of bacteria to produce sulfur-containing amino acids can be improved.
- a sulfur-containing amino acid or those related substances, or these mixtures can be manufactured efficiently.
- the bacterium of the present invention is a bacterium belonging to the family Enterobacteriaceae which has a sulfur-containing amino acid-producing ability and has been modified so that the activity of a protein encoded by the yeeE gene is increased. .
- sulfur-containing amino acids examples include L-cysteine and L-methionine, with L-cysteine being preferred.
- the bacterium of the present invention may be capable of producing both L-cysteine and L-methionine.
- the sulfur-containing amino acid may be a free sulfur-containing amino acid or a salt thereof, or a mixture thereof.
- the salt include sulfate, hydrochloride, carbonate, ammonium salt, sodium salt, and potassium salt.
- the sulfur-containing amino acid-producing ability means that, when the bacterium of the present invention is cultured in a medium, a sulfur-containing amino acid or a related substance thereof, or a mixture thereof is produced in the medium or in the cells, and the medium or The ability to accumulate to the extent that it can be recovered from the cells.
- the bacterium having sulfur-containing amino acid-producing ability means a bacterium that can produce and accumulate in a culture medium a sulfur-containing amino acid or a related substance in a larger amount than a wild strain or a parent strain, or a mixture thereof.
- L-cysteine produced by bacteria may be partially converted to L-cystine by a disulfide bond in the medium.
- S-sulfocysteine may be produced by the reaction of L-cysteine and thiosulfuric acid contained in the medium (Szczepkowski T.W., Nature, vol.182 (1958)).
- L-cysteine produced in bacterial cells may be condensed with ketones or aldehydes present in the cells, such as pyruvic acid, to produce thiazolidine derivatives using hemithioketals as intermediates (see Patent No. 2992010). .
- L-cysteine is used as a starting material for biosynthesis of ⁇ -glutamylcysteine, glutathione, cystathionine, homocysteine and the like. Therefore, these compounds can be produced by using bacteria having the ability to produce these compounds in addition to the ability to produce L-cysteine.
- the ability to produce L-cysteine is not limited to the ability to accumulate only L-cysteine in the medium or in the cells, but includes L-cysteine, L-cystine, derivatives of L-cysteine as described above (for example, S -Sulfocysteine, thiazolidine derivatives, hemithioketals) or other compounds produced via L-cysteine as described above (eg ⁇ -glutamylcysteine, glutathione, cystathionine, homocysteine), or mixtures thereof in the medium Including the ability to accumulate in In the present invention, L-cystine, derivatives of L-cysteine as described above, and other compounds produced via L-cysteine as described above are collectively referred to as L-cysteine related substances.
- L-methionine is a sulfur-containing amino acid that is biosynthesized using L-cysteine as one of the starting materials.
- L-methionine is used as a starting material for biosynthesis such as S-adenosylmethionine. Therefore, when the sulfur-containing amino acid is L-methionine, S-adenosylmethionine and the like are produced by using bacteria having the ability to produce S-adenosylmethionine and the like in addition to the ability to produce L-methionine. can do.
- the ability to produce L-methionine is not limited to the ability to accumulate only L-methionine in the medium or in the cells, but L-methionine or other compounds produced via L-methionine (for example, S-adenosylmethionine), or a mixture thereof, shall be included in the medium.
- L-methionine-related substances other compounds produced via L-methionine as described above are referred to as L-methionine-related substances.
- the ability to produce sulfur-containing amino acids refers to the ability to accumulate L-cysteine, an L-cysteine related substance, L-methionine, an L-methionine related substance, or a mixture thereof in a medium.
- L-cysteine-related substances and L-methionine-related substances are also collectively referred to as sulfur-containing amino acid-related substances.
- Bacteria having sulfur-containing amino acid-producing ability may be inherently those having sulfur-containing amino acid-producing ability. It may be modified so as to have an amino acid-producing ability.
- the bacterium used in the present invention includes Escherichia, Enterobacter, Pantoea, Klebsiella, Serratia, Erwinia, Salmonella
- the parent strain of the family Enterobacteriaceae used for modification it is desirable to use, in particular, Escherichia bacteria, Enterobacter bacteria, Pantoea bacteria, Erwinia bacteria, Enterobacter bacteria, or Klebsiella bacteria.
- the Escherichia bacterium is not particularly limited, but specifically, Neidhardt et al. (Backmann, B. J. 1996. Derivations and Genotypes of some mutant derivatives of Escherichia coli K-12, p. 2460-2488. Table 1 In F. D. Neidhardt (ed.), Escherichia coli and Salmonella Cellular and Molecular Biology / Second Edition, American Society for Microbiology Press, Washington, DC). Among them, for example, Escherichia coli is mentioned. Specific examples of Escherichia coli include Escherichia coli W3110 (ATCC 27325) derived from the prototype wild-type K12 strain, Escherichia coli MG1655 (ATCC 47076), and the like.
- strains can be purchased from, for example, the American Type Culture Collection (address: 12301 Parklawn Drive, Rockville, Maryland 20852 P.O. Box 1549, Manassas, VA 20108, United States States of America). That is, a registration number corresponding to each strain is given, and it is possible to receive a sale using this registration number (see http://www.atcc.org/). The registration number corresponding to each strain is described in the catalog of American Type Culture Collection.
- Enterobacter bacteria examples include Enterobacter agglomerans and Enterobacter aerogenes.
- a representative strain of the genus Enterobacter is Enterobacter agglomerans ATCC 12287. Specifically, the strains exemplified in European Patent Application Publication No. 952221 can be used.
- Pantoea bacteria examples include Pantoea ananatis, Pantoea stewartii, Pantoea agglomerans, and Pantoea citrea.
- Pantoea Ananatis include Pantoea Ananatis AJ13355 and SC17.
- the SC17 strain was selected as a mucus low production mutant from AJ13355 strain (FERM BP-6614), which was isolated as a strain capable of growing on a medium containing L-glutamic acid and a carbon source at low pH from soil in Iwata City, Shizuoka Prefecture. (US Pat. No. 6,596,517).
- Pantoea Ananatis AJ13355 was established at the Institute of Biotechnology, Institute of Industrial Science and Technology, Ministry of International Trade and Industry (current name: National Institute of Advanced Industrial Science and Technology, Patent Biological Deposit Center, zip code 305-8565, East of Tsukuba City, Ibaraki Prefecture. 1-chome, 1-address, 1-center, 6), deposited under the deposit number FERM P-16644, transferred to an international deposit under the Budapest Treaty on January 11, 1999 and given the deposit number FERM BP-6614 .
- Pantoea Ananatis SC17 was deposited on February 4, 2009 at the National Institute of Advanced Industrial Science and Technology Patent Biology Center (address zip code 305-8656, 1st, 1st East, 1st Street, Tsukuba City, Ibaraki). The accession number FERM BP-11091 is assigned.
- the Pantoea ananatis AJ13355 strain was identified as Enterobacter agglomerans at the time of isolation and deposited as the Enterobacter agromerans AJ13355 strain. Has been.
- Examples of bacteria belonging to the genus Erwinia include Erwinia amylovora and Erwinia carotovora, and examples of the genus Klebsiella include Klebsiella plantacola.
- Pantoea bacteria, Erbinia bacteria, Enterobacter bacteria are bacteria classified as ⁇ -proteobacteria, and are taxonomically closely related (J Gen Appl Microbiol 1997 Dec; 43 ( 6) 355-361, International Journal Systematic Bacteriology, Oct. 1997, p1061-1067). Therefore, some bacteria belonging to the genus Enterobacter have been reclassified as Pantoea agglomerans or Pantoea dispersa by DNA-DNA hybridization experiments, etc. (International Journal Systematic Bacteriology, July 1989) ; 39 (3) .p.337-345).
- Enterobacter agglomerans have been reclassified as Pantoea agglomerans, Pantoea ananatis, or Pantoea stealty by 16S rRNA sequence analysis.
- bacteria belonging to the genus Ervinia include those that have been reclassified as Pantoea ananas and Pantoea Stuarti (International Journal Systematic Bacteriology, Jan 1993; 43 (1), p.162- 173).
- it may belong to any of the genus Enterobacter, Pantoea, Erwinia and the like.
- An auxotrophic mutant strain capable of producing a sulfur-containing amino acid, an analog resistant strain of a sulfur-containing amino acid, or a metabolically controlled mutant strain is obtained by subjecting a parent strain or a wild strain to normal mutation treatment, that is, irradiation with X-rays or ultraviolet rays, or N-methyl -N'-nitro-N-nitrosoguanidine (NTG) or treatment with a mutagen such as ethyl methanesulfonate (EMS), etc., among the obtained mutant strains, auxotrophy, analog resistance, or metabolism It can be obtained by selecting those exhibiting a controlled mutation and having the ability to produce sulfur-containing amino acids.
- normal mutation treatment that is, irradiation with X-rays or ultraviolet rays, or N-methyl -N'-nitro-N-nitrosoguanidine (NTG) or treatment with a mutagen such as ethyl methanesulfonate (EMS), etc.
- L-cysteine-producing ability is imparted or enhanced, and L-cysteine-producing bacteria
- L-cysteine-producing bacteria L-cysteine producing ability of bacteria is the production of compounds that are substrates of the pathway, such as enzymes of the L-cysteine biosynthetic pathway or L-serine. It can be improved by enhancing the activity of the enzyme involved, such as 3-phosphoglycerate dehydrogenase or serine acetyltransferase. 3-Phosphoglycerate dehydrogenase is subject to feedback inhibition by serine, but by allowing the bacteria to retain a mutant serA gene encoding a mutant 3-phosphoglycerate dehydrogenase in which this feedback inhibition is reduced or eliminated, The activity can be enhanced.
- Serine acetyltransferase is also subject to feedback inhibition by L-cysteine. Therefore, the enzyme activity can be enhanced by allowing a bacterium to retain a mutant cysE gene encoding serine acetyltransferase in which this feedback inhibition is reduced or eliminated.
- ydeD gene encodes a ydeD gene encoding YdeD protein (Dabler et al., Mol. Microbiol.
- the ability to produce L-cysteine can also be increased by enhancing the expression of the yeastS gene (European Patent Application Publication No. 1016710).
- the L-cysteine-producing bacterium preferably has at least one of the following properties. i) Modified to increase serine acetyltransferase activity. ii) It has been modified to increase the expression of the ydeD gene. iii) modified to increase 3-phosphoglycerate dehydrogenase activity.
- L-cysteine production ability can be improved by enhancing the activity of the sulfate / thiosulfate transport system.
- the sulfate / thiosulfate transport system protein group is encoded by the cysPTWAM gene cluster (Japanese Patent Laid-Open No. 2005-137369, EP1528108).
- Escherichia coli JM15 strain (US Pat. No. 6,218,168) transformed with a plurality of cysE alleles encoding a feedback inhibition resistant serine acetyltransferase (SAT). No.
- Escherichia coli W3110 strain (US Pat. No.
- pACYC-DES is a plasmid obtained by inserting the three genes into pACYC184, and each gene is controlled by the PompA promoter.
- cystathionine- ⁇ -lyase (metC product, JP-A-11-155571, Chandra55et. Al., Biochemistry, 21 (1982) 3064-3069)
- Tryptophanase (tnaA product, Japanese Patent Application Laid-Open No. 2003-169668, (Austin Newton et. Al., J. Biol. Chem. 240 (1965) 1211-1218)
- O-acetylserine sulfhydrylase B (cysM gene product) JP, 2005-245311), and malY gene product (JP 2005-245311) are known.
- cystathionine- ⁇ -lyase (metC product, JP-A-11-155571, Chandra55et. Al., Biochemistry, 21 (1982) 3064-3069)
- Tryptophanase (tnaA product, Japanese Patent Application Laid-Open No. 2003-169668, (Austin Newton et. Al., J. Bio
- the L-cysteine-producing bacterium preferably retains a mutant SAT that is resistant to feedback inhibition.
- a mutant SAT having resistance to feedback inhibition derived from Escherichia coli a mutant SAT in which the methionine residue at position 256 is substituted with a glutamic acid residue (Japanese Patent Laid-Open No. 11-155571), the methionine residue at position 256 Mutant SAT (Denk, D. and Boeck, A., J.
- the SAT gene is not limited to the Escherichia coli gene, and any gene that encodes a protein having SAT activity can be used.
- an SAT isozyme derived from Arabidopsis that is not subject to feedback inhibition by L-cysteine is known, and a gene encoding this can also be used (FEMS Microbiol. Lett., 179 (1999) 453-459).
- the ability to produce L-cysteine can be imparted or enhanced by introducing and expressing a gene encoding SAT, particularly a gene encoding a mutant SAT resistant to feedback inhibition.
- the activity of these proteins can be increased by increasing the copy number of genes encoding proteins such as SAT.
- the ability to produce compounds such as ⁇ -glutamylcysteine, glutathione, cystathionine, and homocysteine biosynthesized using L-cysteine as a starting material also enhances the enzyme activity in the biosynthetic pathway of the target compound or its biosynthesis It can be imparted or enhanced by reducing the activity of the enzyme of the pathway branched from the pathway or the enzyme that degrades the target compound.
- the ability to produce ⁇ -glutamylcysteine can be enhanced by enhancing ⁇ -glutamylcysteine synthetase activity and / or decreasing glutathione synthetase activity.
- the ability to produce glutathione can be imparted or enhanced by enhancing ⁇ -glutamylcysteine synthetase activity and / or glutathione synthetase activity.
- the ability to produce ⁇ -glutamylcysteine or glutathione can also be enhanced by using a mutant ⁇ -glutamylcysteine synthetase that is resistant to feedback inhibition by glutathione.
- the production of glutathione is described in detail in a review by Li et al. (Yin Li, Gongyuan Wei, Jian Chen. Appl Microbiol Biotechnol (2004) 66: 233-242).
- cystathionine and homocysteine are intermediates in the L-methionine biosynthetic pathway, in order to enhance the production ability of these substances, it is effective to use a part of the method for enhancing the production ability of L-methionine described later. It is.
- Specific methods for enhancing cystathionine-producing ability include a method using a methionine-requiring mutant (Japanese Patent Application No. 2003-010654), cysteine (or a biosynthetic raw material thereof) and / or homoserine (or a biosynthetic raw material) in a fermentation medium. Is known (Japanese Patent Laid-Open No. 2005-168422). Since homocysteine uses cystathionine as a precursor, the above method for enhancing cystathionine production ability is also effective for enhancing homocysteine production ability.
- L-methionine-producing ability can be imparted or enhanced by imparting L-threonine requirement or norleucine resistance to bacteria (Japanese Patent Laid-Open No. 2000). -139471).
- the gene for an enzyme involved in the biosynthesis of L-threonine exists as the threonine operon (thrABC).
- thrABC threonine operon
- the ability to biosynthesize after L-homoserine has been lost by deleting the thrBC moiety.
- L-threonine-requiring strains can be obtained.
- S-adenosylmethionine synthetase activity is weakened and L-methionine producing ability is imparted or enhanced.
- S-adenosylmethionine synthetase is encoded by the metK gene.
- L-methionine production ability is enhanced by the activities of enzymes involved in L-methionine biosynthesis such as methionine repressor deficiency, homoserine transsuccinylase, cystathionine ⁇ -synthase, and aspartokinase-homoserine dehydrogenase II.
- the methionine repressor is encoded by the metJ gene
- the homoserine transsuccinylase is encoded by the metA gene
- the cystathionine ⁇ -synthase is encoded by the metB gene
- the aspartokinase-homoserine dehydrogenase II is encoded by the metL gene.
- the ability to produce L-methionine can also be imparted or enhanced by using a mutant homoserine transsuccinylase resistant to feedback inhibition by methionine (Japanese Patent Laid-Open No. 2000-139471, US20090029424).
- L-methionine is biosynthesized using L-cysteine as an intermediate, L-methionine production ability is improved by improving L-cysteine production ability (Japanese Patent Laid-Open No. 2000-139471, US20080311632). Therefore, in order to impart or enhance L-methionine production ability, the above method for imparting or enhancing L-cysteine production ability is also effective.
- L-methionine-producing bacteria and parent strains used to construct them include AJ11539 (NRRL B-12399), AJ11540 (NRRL B-12400), AJ11541 (NRRL B-12401), AJ11542 (NRRL B-12402) (British Patent No. 2075055), L-methionine analog 218 strains (VKPM B-8125) (Russian Patent No. 2209248) having resistance to norleucine and 73 strains (VKPM (B-8126) (( Russian) Patent No. 2215782), etc.
- L-methionine-producing bacteria and parent strains used to construct them include AJ13425 (FERM P-16808) derived from E. coli W3110 (special No.
- AJ13425 lacks a methionine repressor, weakens intracellular S-adenosylmethionine synthetase activity, and intracellular homoserine transsuccinylase activity, Cystathionine ⁇ -synthase activity and aspar L-threonine-requiring strain with enhanced tokinase-homoserine dehydrogenase II activity AJ13425 was launched on May 14, 1998 from the Institute of Biotechnology, Institute of Industrial Science and Technology, Ministry of International Trade and Industry. The depository number is FERM P-16808, which is deposited at the Institute for Patent Biological Depository, Address Postal Code 305-8566 (1st, 1st, 1st East, Tsukuba City, Ibaraki Prefecture).
- the ability to produce compounds such as S-adenosylmethionine biosynthesized using L-methionine as a starting material also enhances the enzyme activity of the biosynthetic pathway of the target compound or branches off from the biosynthetic pathway. It can be imparted or enhanced by reducing the activity of the enzyme of the pathway or the enzyme that degrades the target compound.
- the ability to produce S-adenosylmethionine can be imparted or enhanced by enhancing methionine adenosyltransferase (EP0647712, EP1457569) or enhancing excretion factor MdfA (US7410789).
- the bacterium of the present invention is a protein belonging to the family Enterobacteriaceae having the ability to produce sulfur-containing amino acids as described above (hereinafter referred to as “YeeE”). Or may be described as “YeeE protein”) to increase activity.
- YeeE sulfur-containing amino acids as described above
- the sulfur-containing amino acid-producing ability may be imparted or enhanced after modification so that the activity of the YeeE protein is increased.
- the activity of the protein encoded by the yeeE gene is increased means that the activity of the YeeE protein encoded by the yeeE gene is increased relative to an unmodified strain such as a wild strain or a parent strain.
- the activity of the protein is not particularly limited as long as it is increased compared to the non-modified strain, but is preferably 1.5 times or more, more preferably 2 times or more, more preferably 3 times or more compared to the non-modified strain. To increase.
- the activity of the protein encoded by the yeeE gene is increased means not only an increase in the activity of the YeeE protein in a strain that originally has the activity of the YeeE protein, but also a strain that originally does not have the activity of the YeeE protein. Conferring the activity of the YeeE protein. That is, for example, Pantoea ananatis does not have the yeeE gene, but includes imparting the activity of the YeeE protein to Pantoea ananatis.
- Modifications that increase the activity of the YeeE protein are achieved, for example, by enhancing the expression of the yeeE gene.
- the modification for enhancing the expression of the yeeE gene can be performed, for example, by increasing the copy number of the gene in the cell using a gene recombination technique.
- a DNA fragment containing the yeeE gene may be ligated with a vector that functions in a host bacterium, preferably a multicopy vector, to produce a recombinant DNA, which is introduced into the bacterium and transformed.
- the vector include a vector capable of autonomous replication in a host bacterial cell.
- DNA-receptive cells such as those known for Bacillus subtilis, actinomycetes, and yeast, are introduced into the DNA-receptor cells in a protoplast or spheroplast state that readily incorporates recombinant DNA.
- DNA-receptive cells such as those known for Bacillus subtilis, actinomycetes, and yeast.
- increasing the number of copies of the yeeE gene can also be achieved by making multiple copies of the above-described yeeE gene on the bacterial genomic DNA.
- homologous recombination is performed using a sequence present in multiple copies on the genomic DNA as a target.
- a sequence present in multiple copies on genomic DNA a repetitive DNA sequence (inverted repeat) present at the end of a transposable element can be used. Further, it may be linked in tandem beside the yeeE gene present on the genome, or may be redundantly incorporated on an unnecessary gene on the genome.
- the expression of the yeeE gene is regulated by the method described in International Publication No. 00/18935 pamphlet and the expression regulation of each promoter of the yeeE gene on genomic DNA or plasmid Replace the sequence with a strong one, bring the -35 and -10 regions of each gene closer to the consensus sequence, amplify a regulator that increases the expression of the yeeE gene, or decrease the expression of the yeeE gene It can also be achieved by deleting or weakening such regulators.
- a strong promoter for example, lac promoter, trp promoter, trc promoter, tac promoter, araBA promoter, lambda phage PR promoter, PL promoter, tet promoter, T7 promoter, ⁇ 10 promoter and the like are known.
- the promoter of the threonine operon of Escherichia coli can also be used. It is also possible to introduce a base substitution or the like into the promoter region or SD region of the yeeE gene and modify it to a stronger one.
- the SD region sequence can be directly replaced with the SD region sequence downstream of the ⁇ 10 promoter.
- the expression regulatory region such as the promoter of the yeeE gene can also be determined using a promoter search vector or gene analysis software such as GENETYX. These promoter substitutions or modifications enhance the expression of the yeeE gene. For example, a method using a temperature sensitive plasmid or a Red driven integration method (WO2005 / 010175) can be used for the replacement of the expression regulatory sequence.
- Modifications that increase the expression level of the yeeE gene can be achieved, for example, by modulating a regulator that positively regulates the expression of the yeeE gene or a regulator that negatively regulates the expression of the yeeE gene.
- a regulator that positively regulates the expression of the yeeE gene or a regulator that negatively regulates the expression of the yeeE gene.
- those belonging to the LysR family and the like are listed as control factors, and can be found using a database EcoCyc (http://ecocyc.org/) or the like.
- An increase in the transcription amount of the yeeE gene or an increase in the amount of YeeE protein may be observed by modulating the regulatory factor.
- the increase in expression of the yeeE gene can be confirmed by confirming that the amount of transcription of the yeeE gene has increased, or by confirming that the amount of YeeE protein has increased.
- Confirmation that the transcription amount of the yeeE gene has increased can be performed by comparing the amount of mRNA transcribed from the same gene with a wild strain or an unmodified strain.
- methods for evaluating the amount of mRNA include Northern hybridization, RT-PCR, and the like (Molecular cloning (Cold spring Laboratory Press, Cold spring Harbor (USA), 2001)). It is preferable that the amount of mRNA increases, for example, 1.5 times or more, 2 times or more, or 3 times or more as compared with the unmodified strain.
- the amount of the protein is preferably increased by 1.5 times or more, 2 times or more, or 3 times or more, for example, compared to the unmodified strain.
- recombinant DNA can be introduced into bacteria by the same method, and the copy number of the gene can be increased.
- the yeeE gene of Escherichia coli K12 MG1655 strain corresponds to the complementary sequence of sequences 2082491 to 2083549 in the genome sequence registered as GenBank accession NC_000913 (VERSION NC_000913.2 GI: 49175990) in the NCBI database.
- the yeeE gene of Escherichia coli K12 MG1655 strain is synonymous with ECK2007 and JW1995.
- the nucleotide sequence of the EE1 gene of the MG1655 strain and the amino acid sequence encoded by the gene are shown in SEQ ID NOs: 13 and 14, respectively.
- the yeeE gene that has been modified to increase the activity of the YeeE protein has the base sequence shown in SEQ ID NO: 13. It may be a variant.
- a variant of the yeeE gene can be searched by BLAST or the like with reference to the nucleotide sequence of SEQ ID NO: 13 (http://blast.genome.jp/).
- the variant of a yeeE gene contains the homologue of the same gene.
- the homologue of the gene can be amplified by PCR using, for example, a synthetic oligonucleotide prepared based on the nucleotide sequence of SEQ ID NO: 13, using a chromosome of a microorganism such as Enterobacteriaceae or coryneform bacteria as a template. Gene.
- Examples of yeeE gene homologues of bacteria other than Escherichia coli include the following bacterial yeeE genes (Table 1).
- identity indicates the identity by BLAST of the YeeE protein (SEQ ID NO: 14) of Escherichia coli K12 strain and the homologue of each bacterium.
- accession number indicates the accession number of the NCBI database.
- the yeeE gene encodes a protein that enhances the ability to produce sulfur-containing amino acids when the intracellular activity is increased, 1 is present at one or several positions in the amino acid sequence of the YeeE protein as described above.
- it may be a gene encoding a protein having a sequence including substitution, deletion, insertion or addition of several amino acids.
- the “one or several” differs depending on the position of the amino acid residue in the three-dimensional structure of the protein and the type of amino acid residue, but specifically preferably 1 to 20, more preferably 1 to 10, More preferably, it means 1 to 5.
- One or several amino acid substitutions, deletions, insertions or additions described above are conservative mutations in which the function of the protein is maintained normally.
- a typical conservative mutation is a conservative substitution.
- Conservative substitution is, for example, when the substitution site is an aromatic amino acid, between Phe, Trp, and Tyr, and when the substitution site is a hydrophobic amino acid, between Leu, Ile, and Val, a polar amino acid Is an amino acid having a hydroxyl group between Lys, Arg and His when it is a basic amino acid, and between Asp and Glu when it is an acidic amino acid.
- it is a mutation that substitutes between Ser and Thr.
- substitutions considered as conservative substitutions include substitution from Ala to Ser or Thr, substitution from Arg to Gln, His or Lys, substitution from Asn to Glu, Gln, Lys, His or Asp, Asp to Asn, Glu or Gln substitution, Cys to Ser or Ala substitution, Gln to Asn, Glu, Lys, His, Asp or Arg substitution, Glu to Gly, Asn, Gln, Lys or Asp Substitution, Gly to Pro substitution, His to Asn, Lys, Gln, Arg or Tyr substitution, Ile to Leu, Met, Val or Phe substitution, Leu to Ile, Met, Val or Phe substitution, Substitution from Lys to Asn, Glu, Gln, His or Arg, Met to Ile, L u, Val or Phe substitution, Phe to Trp, Tyr, Met, Ile or Leu substitution, Ser to Thr or Ala substitution, Thr to Ser or Ala substitution, Trp to Phe or Tyr substitution , Sub
- amino acid substitutions, deletions, insertions, additions, or inversions as described above include naturally occurring mutations (mutants or variants) such as cases based on individual differences or species differences of microorganisms from which genes are derived. Also included by mutations (mutants or variants) such as cases based on individual differences or species differences of microorganisms from which genes are derived. Also included by mutations (mutants or variants) such as cases based on individual differences or species differences of microorganisms from which genes are derived. Also included by
- the gene having a conservative mutation as described above is 80% or more, preferably 90% or more, more preferably 95% or more, more preferably 97%, based on the entire amino acid sequence of the YeeE protein as described above. As described above, it may be a gene encoding a protein having a homology of 99% or more and improving the ability to produce sulfur-containing amino acids when the intracellular activity is increased.
- “homology” may refer to “identity”.
- the yeeE gene hybridizes under stringent conditions with a probe that can be prepared from a known gene sequence, for example, the complementary sequence of the nucleotide sequence shown in SEQ ID NO: 13, and encodes a protein having a function equivalent to that of the YeeE protein. It may be DNA.
- stringent conditions refers to conditions under which so-called specific hybrids are formed and non-specific hybrids are not formed. For example, highly homologous DNAs, for example, 80% or more, preferably 90% or more, more preferably 95% or more, more preferably 97% or more, particularly preferably 99% or more DNAs having homology.
- the probe may be a part of a gene complementary sequence.
- a probe can be prepared by PCR using an oligonucleotide prepared on the basis of a known gene sequence as a primer and a DNA fragment containing these base sequences as a template.
- hybridization washing conditions include 50 ° C., 2 ⁇ SSC, and 0.1% SDS.
- gene and protein variants can be applied mutatis mutandis to enzymes such as serine acetyltransferase and 3-phosphoglycerate dehydrogenase, or YdeD proteins, and genes encoding them.
- the yeeD gene exists downstream of the yeeE gene, and both genes are considered to form an operon (database “EcoCys”; http://ecocyc.org/, database “ RegulonDB "; http://regulondb.ccg.unam.mx/).
- the gene group forming the operon often has a common function or a related function. Therefore, when a modification that increases the activity of the YeeE protein exerts some effect, the modification that increases the activity of the YeeD protein may exhibit the same effect.
- a modification that increases the activity of the YeeD protein may be performed together with a modification that increases the activity of the YeeE protein.
- bacterium of the present invention obtained as described above is cultured in a medium, and the sulfur-containing amino acid or the compounds thereof are cultured from the medium. These compounds can be produced by collecting the related substances or a mixture thereof.
- the sulfur-containing amino acid is L-cysteine
- examples of L-cysteine-related substances include S-sulfocysteine, thiazolidine derivatives, hemithioketals corresponding to the thiazolidine derivatives described above.
- sulfur-containing amino acid is L-methionine
- examples of the related substance of L-methionine include the aforementioned S-adenosylmethionine.
- Examples of the medium to be used include a normal medium containing a carbon source, a nitrogen source, a sulfur source, inorganic ions, and other organic components as required.
- Examples of the carbon source include sugars such as glucose, fructose, sucrose, molasses and starch hydrolysate, and organic acids such as fumaric acid, citric acid, and succinic acid.
- the nitrogen source examples include inorganic ammonium salts such as ammonium sulfate, ammonium chloride, and ammonium phosphate, organic nitrogen such as soybean hydrolysate, ammonia gas, and aqueous ammonia.
- inorganic ammonium salts such as ammonium sulfate, ammonium chloride, and ammonium phosphate
- organic nitrogen such as soybean hydrolysate, ammonia gas, and aqueous ammonia.
- sulfur source examples include inorganic sulfur compounds such as sulfate, sulfite, sulfide, hyposulfite, and thiosulfate.
- an organic trace nutrient source it is desirable to contain an appropriate amount of a required substance such as vitamin B1 or a yeast extract.
- a required substance such as vitamin B1 or a yeast extract.
- potassium phosphate, magnesium sulfate, iron ions, manganese ions and the like are added in small amounts as necessary.
- Cultivation is preferably carried out under aerobic conditions for 30 to 90 hours, and the culture temperature is preferably controlled at 25 ° C. to 37 ° C. and the pH during culture is preferably controlled at 5 to 8.
- an inorganic or organic acidic or alkaline substance, ammonia gas or the like can be used for pH adjustment.
- the collection of sulfur-containing amino acids from the culture can be carried out by combining ordinary ion exchange resin methods, precipitation methods and other known methods.
- L-cysteine obtained as described above can be used for the production of L-cysteine derivatives.
- L-cysteine derivatives include methylcysteine, ethylcysteine, carbocysteine, sulfocysteine, acetylcysteine and the like.
- the thiazolidine derivative of L-cysteine when the thiazolidine derivative of L-cysteine accumulates in the medium, the thiazolidine derivative is collected from the medium, and the reaction equilibrium between the thiazolidine derivative and L-cysteine is shifted to the L-cysteine side. Can be manufactured. Further, when S-sulfocysteine accumulates in the medium, it can be converted to L-cysteine by reduction using a reducing agent such as dithiothreitol.
- L-cysteine producing bacteria Mutant cysE (US20050112731 (A1)) encoding mutant serine acetyltransferase with reduced feedback inhibition by L-cysteine, ydeD gene (US5972663A) encoding L-cysteine excretion factor ), And pACYC-DES having a mutant serA gene (US6180373) encoding 3-phosphoglycerate dehydrogenase with reduced feedback inhibition by L-serine on one plasmid, Escherichia coli MG1655 strain and Pantoea ananatis It was introduced into the SC17 strain, and L-cysteine producing bacteria MG1655 / pACYC-DES and SC17 / pACYC-DES were constructed.
- the threonine residue at position 167 is substituted with an alanine residue.
- the 3-phosphoglycerate dehydrogenase lacks the tyrosine residue at position 410.
- the construction of pACYC-DES is described in Japanese Patent Application Laid-Open No. 2005-137369 (US20050124049 (A1), EP1528108 (A1)).
- the PCR cycle is as follows. 95 ° C 3 minutes, 95 ° C 60 seconds, 50 ° C 30 seconds, 72 ° C 40 seconds 2 cycles, 94 ° C 20 seconds, 55 ° C 20 seconds, 72 ° C 15 seconds 25 cycles, finally 72 ° C 5 minutes.
- the obtained fragment was digested with SalI and PaeI and inserted into the SalI-PaeI site of pMIV-5JS (JP 2008-99668) to obtain plasmid pMIV-Pnlp0.
- the base sequence of the PaeI-SalI fragment of the Pnlp0 promoter inserted into this pMIV-Pnlp0 plasmid is as shown in SEQ ID NO: 3.
- a DNA fragment containing about 300 bp of the terminator region of the rrnB gene is obtained by PCR using primer P3 (agctgatctagaaaacagaatttgcctggcggc: SEQ ID NO: 4) and primer P4 (agctgaggatccaggaagagtttgtagaaacgc: SEQ ID NO: 5). did. Restriction enzymes XbaI and BamHI sites are designed at the 5 ′ ends of these primers, respectively.
- the PCR cycle is as follows.
- the obtained fragment was digested with XbaI and BamHI and inserted into the XbaI-BamHI site of pMIV-Pnlp0 to obtain plasmid pMIV-Pnlp0-ter.
- a DNA fragment of about 700 bp containing the yeastS gene was obtained by PCR using primer P5 (agctgagtcgacgtgttcgctgaatacggggt: SEQ ID NO: 6) and primer P6 (agctgatctagagaaagcatcaggattgcagc: SEQ ID NO: 7). Restriction enzymes SalI and XbaI sites are designed at the 5 ′ ends of these primers, respectively.
- the PCR cycle is as follows.
- the obtained fragment was digested with SalI and XbaI and inserted into the SalI-XbaI site of pMIV-Pnlp0-ter to obtain plasmid pMIV-Pnlp0-YeaS3.
- an expression unit of yeastS was constructed in which the nlpD promoter, the yeastS gene, and the rrnB terminator were connected in this order on the pMIV-5JS vector.
- the nlpD promoter region (FIG. 1) has two regions that are presumed to function as promoters.
- the -10 region and the -35 region are represented by P1 (-10) and P1 (-35), and P2 ( ⁇ 10) and P2 ( ⁇ 35).
- the -10 region (P1 (-10)) contained in the 3 'end of the nlpD promoter is randomized by PCR using the primer P1 and the primer P7 (atcgtgaagatcttttccagtgttnannagggtgccttgcacggtnatnangtcactgg: SEQ ID NO: 8).
- the obtained DNA fragment was obtained.
- the PCR cycle is as follows. 95 ° C 3 minutes, 95 ° C 60 seconds, 50 ° C 30 seconds, 72 ° C 40 seconds 2 cycles, 94 ° C 20 seconds, 60 ° C 20 seconds, 72 ° C 15 seconds 25 cycles, finally 72 ° C 5 minutes.
- the PCR cycle is as follows. 95 ° C 3 minutes, 95 ° C 60 seconds, 50 ° C 30 seconds, 72 ° C 40 seconds 2 cycles, 94 ° C 20 seconds, 60 ° C 20 seconds, 72 ° C 15 seconds 25 cycles, and finally 72 ° C 5 minutes.
- the obtained 3′-end and 5′-end fragments can be joined together by the BglII sites designed for the primers P7 and P8 to construct a full length nlpD promoter in which two ⁇ 10 regions are randomized. be able to.
- a DNA fragment of the modified nlpD promoter full length was obtained by PCR using P1 and P2 as primers.
- the PCR cycle is as follows. 95 ° C 3 minutes, 95 ° C 60 seconds, 50 ° C 30 seconds, 72 ° C 40 seconds 2 cycles, 94 ° C 20 seconds, 60 ° C 20 seconds, 72 ° C 15 seconds 12 cycles, and finally 72 ° C 5 minutes.
- the amplified fragment is digested with the restriction enzymes SalI and PaeI designed at the 5 ′ end of the primer, and inserted into the plasmid pMIV-Pnlp0-YeaS3, which is also digested with SalI and PaeI, so that the wild-type nlpD promoter site on the plasmid (Pnlp0) was replaced with mutant Pnlp.
- the one having the promoter sequence (Pnlp8) shown in SEQ ID NO: 10 was selected and named pMIV-Pnlp8-YeaS7.
- the base sequence of the PaeI-SalI fragment of the Pnlp8 promoter inserted into this plasmid is shown in SEQ ID NO: 10.
- the Pnlp8 promoter is a stronger promoter than the Pnlp0 promoter.
- Amplification of the Escherichia coli yeeE gene was carried out using the MG1655 strain genomic DNA as a template, yeeE (Ec) SalI-F (acgcgtcgacatgttttcaatgatattaagcgggc: SEQ ID NO: 11), yeeE (Ec) XbaI-R (ctagtctagattaatttgccgcagt
- the PCR cycle (94 ° C., 5 minutes, 98 ° C., 5 seconds, 55 ° C., 5 seconds, 72 ° C., 90 seconds, 30 cycles, finally 4 ° C. incubation) was used. SalI and XbaI sites are designed at both ends of the primer.
- the amplified fragment was digested with SalI and XbaI and inserted into pMIV-Pnlp8-YeaS7, which was also digested with SalI and XbaI, to prepare pMIV-Pnlp8-eeE (Ec). Also, pMIV-5JS (Japanese Patent Laid-Open No. 2008-99668) was used as the corresponding empty vector (for control).
- the DNA sequence of the yeeE gene is shown in SEQ ID NO: 13, and the predicted amino acid sequence of the yeeE gene product is shown in SEQ ID NO: 14.
- L-cysteine production culture Escherichia coli
- Escherichia coli MG1655 / pACYC-DES was transformed into the yE overexpression plasmid pMIV-Pnlp8-yeE.
- Ec and the strain introduced with the empty vector pMIV-5JS for control were subjected to fermentation production culture, and the production amounts of L-cysteine and L-cysteine related compounds were compared.
- an L-cysteine production medium having the following composition was used.
- Sterilization was performed by autoclaving at 110 ° C. for 30 minutes (components 1 and 2), dry heat sterilization (component 5) at 180 ° C. for 5 hours or more, and filter sterilization (components 3 and 4).
- L-cysteine production culture was performed according to the following procedure. Each L-cysteine-producing bacterium is spread on LB agar medium, pre-cultured overnight at 37 ° C., and then about 7 cm of cells on a plate with a 10 microliter inoculation loop (NUNC Blue Loop) 3 times (3 loops), inoculated into the above L-cysteine production medium with 2 ml in a large test tube (inner diameter 23 mm, length 20 cm), and the amount of cells at the start of culture is almost the same. It was prepared so that it might become. Shaking culture was performed at 32 ° C., and the culture was terminated after 30 hours.
- NUNC Blue Loop 10 microliter inoculation loop
- L-cysteine including some L-cysteine-related substances such as cystine
- the quantification of L-cysteine (including some L-cysteine-related substances such as cystine) produced in the medium was determined by Gaiton, M. et al. K. (Biochem J. 1967 Aug; 104 (2): 627-33.). Each strain was tested in quadruplicate, and L-cysteine yield (average value), standard deviation, and L-cysteine yield relative to glucose consumed are shown in Table 2. Overexpression of the yeeE gene increased the accumulated concentration of L-cysteine. Thus, it was revealed that L-cysteine production can be improved by increasing the activity of the YeeE protein.
- L-cysteine production culture (Panteoanaanatis)
- the above-described L-cysteine producing bacterium Pantoea ananatis SC17 / pACYC-DES was transformed into the yE overexpression plasmid pMIV-Pnlp8-yeE ( Ec) and a strain introduced with the control empty vector pMIV-5JS were subjected to fermentation production culture, and the production amounts of L-cysteine and L-cysteine related compounds were compared.
- L-cysteine production culture and the L-cysteine quantification method are almost the same as those in the above-mentioned Example of Escherichia coli. However, the amount of inoculation was 1 loop and the culture time was 22 hours. Each strain was tested in quadruplicate, and L-cysteine yield (average value), standard deviation, and L-cysteine yield relative to glucose consumed are shown in Table 3. Overexpression of the yeeE gene increased the accumulated concentration of L-cysteine. Thus, it was revealed that L-cysteine production can be improved by increasing the activity of the YeeE protein.
- the ability of bacteria to produce sulfur-containing amino acids can be improved, and sulfur-containing amino acids or their related substances, or mixtures thereof can be efficiently produced.
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Abstract
Description
すなわち本発明は以下のとおりである。
(1)含硫アミノ酸生産能を有し、かつ、yeeE遺伝子によりコードされるタンパク質の活性が増大するように改変された腸内細菌科に属する細菌。
(2)yeeE遺伝子の発現量を増大させること、又は、yeeE遺伝子の翻訳量を増大させることにより、前記タンパク質の活性が増大した、前記細菌。
(3)yeeE遺伝子のコピー数を高めること、又は同遺伝子の発現調節配列を改変することにより、yeeE遺伝子の発現量が増大した、前記細菌。
(4)前記タンパク質が、下記(A)または(B)に記載のタンパク質である前記細菌。
(A)配列番号14に示すアミノ酸配列からなるタンパク質。
(B)配列番号14に示すアミノ酸配列において、1若しくは数個のアミノ酸の置換、欠失、挿入、または付加を含むアミノ酸配列を有し、かつ、細胞内の活性を増大させたときに含硫アミノ酸生産能が向上するタンパク質。
(5)前記yeeE遺伝子が、下記(a)または(b)に記載のDNAである、前記細菌。
(a)配列番号13に示す塩基配列からなるDNA、または
(b)配列番号13に示す塩基配列と相補的な塩基配列又は同塩基配列から調製され得るプローブとストリンジェントな条件下でハイブリダイズし、かつ、細胞内の活性を増大させたときに含硫アミノ酸生産能が向上するタンパク質をコードするDNA。
(6)さらに、下記の性質の少なくともいずれかを有する前記細菌。
i)セリンアセチルトランスフェラーゼ活性が上昇するように改変されている。
ii)ydeD遺伝子の発現が上昇するように改変されている。
iii)3-ホスホグリセレートデヒドロゲナーゼ活性が上昇するように改変されている。
(7)前記細菌がエシェリヒア属細菌である、前記細菌。
(8)前記細菌がエシェリヒア・コリである、前記細菌。
(9)前記細菌がパントエア属細菌である、前記細菌。
(10)前記細菌がパントエア・アナナティスである、前記細菌。
(11)前記細菌を培地中で培養し、該培地から含硫アミノ酸もしくはそれらの関連物質、又はこれらの混合物を採取することを特徴とする、含硫アミノ酸もしくはそれらの関連物質、又はこれらの混合物の製造法。
(12)前記含硫アミノ酸がL-システインである、前記方法。
(13)前記含硫アミノ酸がL-システインであり、前記関連物質がシスチン又はチアゾリジン誘導体である、前記方法。
本発明の細菌は、含硫アミノ酸生産能を有し、かつ、yeeE遺伝子によりコードされるタンパク質の活性が増大するように改変された腸内細菌科に属する細菌である。
細菌のL-システイン生産能は、L-システイン生合成経路の酵素、又はL-セリン等、同経路の基質となる化合物の生成に関与する酵素、例えば、3-ホスホグリセレートデヒドロゲナーゼ、又はセリンアセチルトランスフェラーゼ等の活性を増強することにより、向上させることができる。3-ホスホグリセレートデヒドロゲナーゼは、セリンによるフィードバック阻害を受けるが、このフィードバック阻害が低減又は解除された変異型3-ホスホグリセレートデヒドロゲナーゼをコードする変異型serA遺伝子を細菌に保持させることによって、同酵素活性を増強することができる。また、セリンアセチルトランスフェラーゼは、L-システインによるフィードバック阻害を受ける。したがって、このフィードバック阻害が低減又は解除されたセリンアセチルトランスフェラーゼをコードする変異型cysE遺伝子を細菌に保持させることによって、同酵素活性を増強することができる。
i)セリンアセチルトランスフェラーゼ活性が上昇するように改変されている。
ii)ydeD遺伝子の発現が上昇するように改変されている。
iii)3-ホスホグリセレートデヒドロゲナーゼ活性が上昇するように改変されている。
L-メチオニン生産能は、L-スレオニン要求性あるいはノルロイシン耐性を細菌に付与することによって、付与又は増強することができる(特開2000-139471号)。E. coliにおいては、L-スレオニンの生合成に関与する酵素の遺伝子は、スレオニンオペロン(thrABC)として存在し、例えば、thrBC部分を欠失させることによってL-ホモセリン以降の生合成能を失ったL-スレオニン要求株を取得することができる。ノルロイシン耐性株では、S-アデノシルメチオニンシンセターゼ活性が弱化され、L-メチオニン生産能が付与又は増強される。E. coliにおいては、S-アデノシルメチオニンシンセターゼはmetK遺伝子にコードされている。また、L-メチオニン生産能は、メチオニンリプレッサーの欠損、ホモセリントランスサクシニラーゼ、及びシスタチオニンγ-シンテース、及びアスパルトキナーゼ-ホモセリンデヒドロゲナーゼII等のL-メチオニン生合成に関与する酵素の活性の増強によっても、付与又は増強することができる(特開2000-139471号)。E. coliにおいては、メチオニンリプレッサーはmetJ遺伝子に、ホモセリントランスサクシニラーゼはmetA遺伝子に、シスタチオニンγ-シンテースはmetB遺伝子に、アスパルトキナーゼ-ホモセリンデヒドロゲナーゼIIはmetL遺伝子にそれぞれコードされている。また、メチオニンによるフィードバック阻害に対して耐性をもつ変異型ホモセリントランスサクシニラーゼを用いることでもL-メチオニンの生産能を付与又は増強することができる(特開2000-139471号、US20090029424)。なお、L-メチオニンはL-システインを中間体として生合成されるため、L-システインの生産能の向上によりL-メチオニンの生産能も向上する(特開2000-139471号、US20080311632)。よって、L-メチオニン生産能を付与又は増強するためには、L-システイン生産能を付与又は増強させる上記方法も有効である。
本発明の細菌は、上述したような含硫アミノ酸生産能を有する腸内細菌科に属する細菌を、yeeE遺伝子によりコードされるタンパク質(以下、「YeeE」又は「YeeEタンパク質」と記載することがある)の活性が増大するように改変することによって得ることができる。ただし、YeeEタンパク質の活性が増大するように改変を行った後に、含硫アミノ酸生産能を付与又は増強してもよい。
上記のようにして得られる本発明の細菌を培地中で培養し、該培地から含硫アミノ酸、もしくはそれらの関連物質、又はこれらの混合物を採取することにより、これらの化合物を製造することができる。含硫アミノ酸がL-システインである場合は、L-システインの関連物質としては、先述したS-スルホシステイン、チアゾリジン誘導体、同チアゾリジン誘導体に対応するヘミチオケタール等が挙げられる。含硫アミノ酸がL-メチオニンである場合は、L-メチオニンの関連物質としては、先述したS-アデノシルメチオニン等が挙げられる。
L-システインによるフィードバック阻害が低減された変異型セリンアセチルトランスフェラーゼをコードする変異型cysE(US20050112731(A1))、L-システイン排出因子をコードするydeD遺伝子(US5972663A)、及びL-セリンによるフィードバック阻害が低減された3-ホスホグリセレートデヒドロゲナーゼをコードする変異型serA遺伝子(US6180373)が1つのプラスミドに載ったpACYC-DESを、エシェリヒア・コリ MG1655株及びパントエア・アナナティス SC17株に導入し、L-システイン生産菌MG1655/pACYC-DES、及びSC17/pACYC-DESを構築した。前記変異型セリンアセチルトランスフェラーゼは、167位のスレオニン残基がアラニン残基に置換されている。また、前記3-ホスホグリセレートデヒドロゲナーゼは、410位のチロシン残基を欠失している。pACYC-DESの構築は、特開2005-137369(US20050124049(A1)、EP1528108(A1))に記載されている。
YeeEタンパク質の活性を増強するために用いられる、yeeE遺伝子の過剰発現用プラスミドpMIV-Pnlp8-yeeE(Ec)を以下の手順で構築した。
エシェリヒア・コリ MG1655(ATCC 47076)の染色体DNAをテンプレートとして、プライマーP1(agctgagtcgacccccaggaaaaattggttaataac:配列番号1)、及びプライマーP2(agctgagcatgcttccaactgcgctaatgacgc:配列番号2)をプライマーとして用いたPCRによってnlpD遺伝子のプロモーター領域(Pnlp0)約300bpを含むDNA断片を取得した。これらのプライマーの5'末端には制限酵素SalI及びPaeIのサイトがそれぞれデザインされている。PCRサイクルは次のとおりである。95℃ 3分の後、95℃ 60秒、50℃ 30秒、72℃ 40秒を2サイクル、94℃ 20秒、55℃ 20秒、72℃ 15秒を25サイクル、最後に72℃ 5分。得られた断片をSalI及びPaeIで消化し、pMIV-5JS(特開2008-99668)のSalI-PaeIサイトに挿入しプラスミドpMIV-Pnlp0を取得した。このpMIV-Pnlp0プラスミドに挿入されたPnlp0プロモーターのPaeI-SalI断片の塩基配列は配列番号3に示したとおりである。
nlpDプロモーターの-10領域を改変することでより強力なプロモーターとするため、以下の手法で-10領域のランダム化を行った。nlpDプロモーター領域(図1)には、プロモーターとして機能すると推定される領域が2箇所存在し、それぞれの-10領域及び-35領域を、P1(-10)及びP1(-35)、並びにP2(-10)及びP2(-35)と示す。プラスミドpMIV-Pnlp0をテンプレートとして、プライマーP1及びプライマーP7(atcgtgaagatcttttccagtgttnannagggtgccttgcacggtnatnangtcactgg:配列番号8)をプライマーとして用いたPCRによってnlpDプロモーターの3'末端側に含まれる-10領域(P1(-10))をランダム化したDNA断片を取得した。PCRサイクルは次のとおりである。95℃ 3分の後、95℃ 60秒、50℃ 30秒、72℃ 40秒を2サイクル、94℃ 20秒、60℃ 20秒、72℃ 15秒を25サイクル、最後に72℃ 5分。
先述の発現プラスミドpMIV-Pnlp8-YeaS7に組み込まれているyeaS遺伝子をyeeE遺伝子に置き換えることで、pMIV-5JSベクター上にPnlp8プロモーター、yeeE遺伝子、及びrrnBターミネーターの順に繋がったyeeEの発現ユニットが搭載されたプラスミドを構築した。yeeE遺伝子の過剰発現用プラスミドpMIV-Pnlp8-yeeE(Ec)の構築方法を以下に示す。
yeeE遺伝子の過剰発現がL-システイン及びL-システイン関連化合物の発酵生産に及ぼす効果を調べるため、先述のL-システイン生産菌 エシェリヒア・コリ MG1655/pACYC-DESにyeeE過剰発現プラスミドpMIV-Pnlp8-yeeE(Ec)及びその対照用の空ベクターpMIV-5JSを導入した株の発酵生産培養を行い、L-システイン及びL-システイン関連化合物の生産量を比較した。培養には下記組成のL-システイン生産培地を使用した。
〔L-システイン生産培地〕(各成分の濃度は最終濃度)
成分1:
(NH4)2SO4 15g/L
KH2PO4 1.5g/L
MgSO4・7H2O 1g/L
トリプトン 10g/L
イーストエクストラクト 5g/L
NaCl 10g/L
L-ヒスチジン塩酸塩一水和物 135mg/L
L-メチオニン 300mg/L
成分2:
グルコース 40g/L
成分3:
チオ硫酸ナトリウム 7g/L
成分4:
ピリドキシン塩酸塩 2mg/L
成分5:
炭酸カルシウム 20g/L
各成分について、各々100/47.5倍(成分1)、100/47.5倍(成分2)、50倍(成分3)、1000倍(成分4)のストック溶液を作製しておき、使用時に混合し滅菌水で規定の量までメスアップして最終濃度となるように調製した。殺菌は、110℃、30分のオートクレーブ(成分1、2)、180℃、5時間以上の乾熱滅菌(成分5)、フィルター滅菌(成分3、4)により行った。
yeeE遺伝子過剰発現がL-システイン及びL-システイン関連化合物の発酵生産に及ぼす効果を調べるため、先述のL-システイン生産菌 パントエア・アナナティス SC17/pACYC-DESにyeeE過剰発現プラスミドpMIV-Pnlp8-yeeE(Ec)及びその対照用の空ベクターpMIV-5JSを導入した株の発酵生産培養を行い、L-システイン及びL-システイン関連化合物の生産量を比較した。L-システイン生産培養及びL-システインの定量方法は先述のエシェリヒア・コリでの実施例と概ね同じである。ただし、植菌量を1ループ、培養時間を22時間とした。各株とも4連で実験を行い、そのときのL-システイン生産量(平均値)と標準偏差、消費グルコースに対するL-システイン収率を表3に示した。yeeE遺伝子の過剰発現によりL-システインの蓄積濃度が増大した。よって、YeeEタンパク質の活性を増大させることにより、L-システインの生産を向上させることができると明らかになった。
配列番号1:Pnlp0増幅用プライマー
配列番号2:Pnlp0増幅用プライマー
配列番号3:Pnlp0の塩基配列
配列番号4:rrnB遺伝子のターミネーター領域増幅用プライマー
配列番号5:rrnB遺伝子のターミネーター領域増幅用プライマー
配列番号6:yeaS遺伝子増幅用プライマー
配列番号7:yeaS遺伝子増幅用プライマー
配列番号8:Pnlp0の-10領域(3’側)ランダム化プライマー
配列番号9:Pnlp0の-10領域(5’側)ランダム化プライマー
配列番号10:Pnlp8の塩基配列
配列番号11:yeeE遺伝子増幅用プライマー
配列番号12:yeeE遺伝子増幅用プライマー
配列番号13:エシェリヒア・コリ野生型yeeE遺伝子の塩基配列
配列番号14:エシェリヒア・コリ野生型YeeEタンパク質のアミノ酸配列
配列番号15:yeaS遺伝子との連結部位を含むPnlp0の塩基配列
配列番号16:yeaS遺伝子との連結部位を含むPnlp8の塩基配列
Claims (13)
- 含硫アミノ酸生産能を有し、かつ、yeeE遺伝子によりコードされるタンパク質の活性が増大するように改変された腸内細菌科に属する細菌。
- yeeE遺伝子の発現量を増大させること、又は、yeeE遺伝子の翻訳量を増大させることにより、前記タンパク質の活性が増大した、請求項1に記載の細菌。
- yeeE遺伝子のコピー数を高めること、又は同遺伝子の発現調節配列を改変することにより、yeeE遺伝子の発現量が増大した、請求項2に記載の細菌。
- 前記タンパク質が、下記(A)または(B)に記載のタンパク質である、請求項1~3のいずれか1項に記載の細菌。
(A)配列番号14に示すアミノ酸配列からなるタンパク質。
(B)配列番号14に示すアミノ酸配列において、1若しくは数個のアミノ酸の置換、欠失、挿入、又は付加を含むアミノ酸配列からなり、かつ、細胞内の活性を増大させたときに含硫アミノ酸生産能が向上するタンパク質。 - 前記yeeE遺伝子が、下記(a)または(b)に記載のDNAである、請求項1~4のいずれか1項に記載の細菌。
(a)配列番号13に示す塩基配列からなるDNA。
(b)配列番号13に示す塩基配列と相補的な塩基配列又は該塩基配列から調製され得るプローブとストリンジェントな条件下でハイブリダイズし、かつ、細胞内の活性を増大させたときに含硫アミノ酸生産能が向上するタンパク質をコードするDNA。 - さらに、下記の性質の少なくともいずれかを有する請求項1~5のいずれか1項に記載の細菌。
i)セリンアセチルトランスフェラーゼ活性が上昇するように改変されている。
ii)ydeD遺伝子の発現が上昇するように改変されている。
iii)3-ホスホグリセレートデヒドロゲナーゼ活性が上昇するように改変されている。 - 前記細菌がエシェリヒア属細菌である、請求項1~6のいずれか1項に記載の細菌。
- 前記細菌がエシェリヒア・コリである、請求項7に記載の細菌。
- 前記細菌がパントエア属細菌である、請求項1~6のいずれか1項に記載の細菌。
- 前記細菌がパントエア・アナナティスである、請求項9記載の細菌。
- 請求項1~10のいずれか1項に記載の細菌を培地中で培養し、該培地から含硫アミノ酸もしくはそれらの関連物質、又はこれらの混合物を採取することを特徴とする、含硫アミノ酸もしくはそれらの関連物質、又はこれらの混合物の製造法。
- 前記含硫アミノ酸がL-システインである、請求項11に記載の方法。
- 前記含硫アミノ酸がL-システインであり、前記関連物質がシスチン又はチアゾリジン誘導体である、請求項11に記載の方法。
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US8962284B2 (en) | 2010-09-14 | 2015-02-24 | Ajinomoto Co., Inc. | Sulfur-containing amino acid-producing bacterium and method for producing sulfur-containing amino acid |
WO2015033849A1 (ja) * | 2013-09-04 | 2015-03-12 | 国立大学法人奈良先端科学技術大学院大学 | L―システインの製造方法 |
JP2015528301A (ja) * | 2012-09-17 | 2015-09-28 | ワッカー ケミー アクチエンゲゼルシャフトWacker Chemie AG | L−システインおよび該アミノ酸の誘導体の発酵生産方法 |
WO2020204179A1 (en) | 2019-04-05 | 2020-10-08 | Ajinomoto Co., Inc. | Method of producing l-amino acids |
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EP2617808B1 (en) | 2016-06-15 |
JPWO2012036151A1 (ja) | 2014-02-03 |
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CN103119154B (zh) | 2015-11-25 |
US20130164793A1 (en) | 2013-06-27 |
EP2617808A1 (en) | 2013-07-24 |
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US8962284B2 (en) | 2015-02-24 |
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