RU2268305C2 - Method for preparing l-amino acids by using microorganisms with optimized level of gene expression - Google Patents

Abstract

FIELD: biotechnology, microbiology, genetic engineering, amino acids.

SUBSTANCE: invention describes a microorganism belonging to genus Escherichia used as a producer of L-amino acids with optimized level of expression of gene that effects in disposition of carbon flow, in particular, gene sucAB. Method involves stages for insertion of DNA fragments set into microorganism chromosome synthesized in vitro and comprising regulatory elements of gene expression instead the natural element of regulatory gene region to obtain population of microorganisms and selection of microorganisms showing the enhanced production of L-amino acids. Also, invention describes a method for preparing such L-amino acids as L-glutamic acid, L-proline, L-arginine, L-glutamine, L-leucine by using microorganisms with optimized level of expression of gene sucAB. Invention provides preparing L-amino acids with the high effectiveness degree.

EFFECT: improved preparing method.

15 cl, 1 dwg, 2 tbl, 5 ex

Description

BACKGROUND OF THE INVENTION

Technical field

The present invention relates to a method for producing bacteria with an optimized level of gene expression useful for the production of amino acids or nucleic acids, and to a method for producing L-amino acids or nucleic acids using said bacterium.

Description of the Related Art

The traditional way to increase the production of L-amino acids or nucleic acids by producer strains is to increase the activity of the products of genes involved in the biosynthesis of these L-amino acids or nucleic acids. This can be done by obtaining mutants that are resistant to the target compound or its analogue, increasing the level of expression of biosynthesis genes, reducing the sensitivity of biosynthesis enzymes to inhibition by feedback products or intermediates, by removing strains of bacteria deficient in genes using the precursors of target compounds in other metabolic pathways or the creation of strains of bacteria deficient in genes involved in the degradation of the target compound.

The above manipulations usually result in strains that are not able to grow or are able to grow at a much lower rate, or strains that require additional nutrients necessary for growth, such as amino acids. For example, an increase in the expression level of certain genes can be excessive and can lead to serious inhibition of bacterial growth and, as a result, a decrease in the ability of bacteria to produce the target compound.

It is known that microorganisms belonging to the genus Escherichia, deficient in the activity of α-ketoglutarate dehydrogenase, or microorganisms in which this activity is reduced, acquire the ability to produce L-glutamic acid (US patents 5573945 and 5908768). But such mutants - producers of glutamic acid do not grow well or are not able to grow at all on minimal medium with glucose under aerobic conditions. To restore growth, it is necessary to add succinic acid or lysine in combination with methionine. Thus, the choice of the optimal level of expression of α-ketoglutarate dehydrogenase in bacteria is necessary to restore the ability to produce glutamic acid and growth in a nutrient medium that does not contain additional additives, such as succinic acid, lysine or methionine.

On the other hand, it is known that genes encoding succinate dehydrogenase (sdhCDAB genes), in combination with genes encoding α-ketoglutarate dehydrogenase (sucAB genes) and succinyl CoA synthase (sucCD genes), form a cluster in the E. coli chromosome containing two promoter: P _sdh - sdhCDAB-P _suc -sucAB-sucCD (Park, Chao & Gunsalus, J. Bact. 179.4138-4142.1997; Cunningham & Guest, Microbiology, 144, 2113-2123.1998). The main promoter of this operon is the regulatory region located in front of the sdhC, P _sdh gene. The presence of the weaker P _suc promoter, recognized by E. coli RNA polymerase in complex with σ ³⁸ , provides an additional low level of constitutive expression of sucABCD genes. An increase in substrate concentration does not affect the activity of the second promoter. The effects of anaerobiosis and mutations of the arcA and fnr genes are also negligible. The ArcA protein is a negative regulator of the genes of aerobic pathways of biosynthesis, and the Fnr protein (fumarate and nitrate reduction - restoration of fumarate and nitrate) is involved in the regulation of transcription of genes responsible for aerobic and anaerobic respiration, as well as for the osmotic balance of the cell. Among the potential regulators that have been tested, only IHF (integration host factor - a product of the himA gene) can play a significant role in the repression of P _suc activity. The ArcA and Fnr proteins interact with the P _sdh promoter, and the IHF protein interacts with the weaker P _suc promoter.

A library of synthetic promoters of various strengths has been described for Lactococus lactis (Jensen PR, and Hammer K., Appl. Environ. MicrobioL, 1998, 64, No. l. 82-87 Biotechnol. Bioeng., 1998, 58, 2-3, 191-5). The library consists of 38 oligonucleotides containing a region with a sequence of nucleotides of arbitrary composition between consensus sequences at positions between -35 to -15. To evaluate the strength of the obtained promoters, the oligonucleotides of their library were cloned into the pAK80 expression vector containing the β-galactosidase gene. It was shown that most of the artificial promoters were very weak (activity below 500 units), and only three of them had a force of about 2000 conventional units. But the practical use of the library of synthetic promoters has not been described.

European patent application EP 1033407 A1 describes a method for producing coryneform bacteria having improved ability to produce amino acids or nucleic acids by introducing mutations in the promoter region. Up to 8 different mutant promoter variants were used for each of the genes selected from the group consisting of the glutamate dehydrogenase gene (gdh), the citrate synthase gene (gltA), the isocitrate synthase gene (icd), the pyruvate dehydrogenase gene (pdhA) and the arginginase gene. The disadvantage of the proposed methodology proposed in European application EP 1033407 A1 is that each of these mutants was obtained separately, one after the other. In addition, an increase in the production of L-amino acids in all the described examples was achieved by increasing the activity of certain enzymes using a limited number of promoters of the gene encoding this enzyme. A similar approach is generally accepted and traditional in works aimed at obtaining bacteria producing L-amino acids or nucleic acids, and is not related to the optimization or “fine tuning” of the activity of gene promoters important for the production of L-amino acids or nucleic acids.

Currently, there are no reports describing the application of the method of optimization of gene expression for the production of any metabolite by fermentation using bacteria modified to optimize the expression of the target gene.

Description of the invention

An object of the present invention is to provide a method for producing a bacterium with an optimized expression level of a gene encoding a protein that affects the distribution of carbon and nitrogen fluxes in the metabolism of a given bacterium, and includes the following steps: 1) introducing a set of DNA fragments obtained in vitro into the chromosome of a given bacterium containing regulatory sequences for the expression of the specified gene, instead of the natural regulatory sequences of the specified gene, and 2) selection of bacteria with the desired phenotype.

It is also an object of the present invention to provide an L-amino acid producing bacterium with an optimized gene expression level that affects the production of the L-amino acid, and wherein said bacterium is obtained using the method described in claim 1.

It is also an object of the present invention to provide a method for producing an L-amino acid, which includes the following steps: 1) growing a bacterium, as described above, in a nutrient medium in order to accumulate an L-amino acid in a nutrient medium, and 2) isolating the L-amino acid from the culture liquids.

The present invention provides a simple method for producing an L-amino acid producing bacterium in one step with an optimized gene expression level, which affects the distribution of carbon and nitrogen fluxes in bacteria and, therefore, affects the production of L-amino acid or nucleic acid.

The present invention also provides a bacterium with an optimized level of gene expression, which affects the production of L-amino acids or nucleic acids, increasing the specified production, and provides a method for producing L-amino acids, such as glutamic acid or L-amino acid derived from L-glutamic acid, such as L-arginine, L-proline, L-glutamine, and also L-leucine; a method for producing L-amino acids, such as L-lysine, L-isoleucine, L-valine, L-histidine, L-aspartate, L-alanine, L-tyrosine, L-phenylalanine, for the biosynthesis of which L-glutamic acid is required as amino group donor; and a method for producing nucleic acids.

This goal was achieved by replacing the native promoter of the target gene with a sequence similar to the promoter, with a sequence of arbitrary composition ("randomized" sequence) directly on the bacterial chromosome. A similar idea is based on the well-known fact that in mutants with a modified “-35” region of promoters recognized by the E. coli RNA polymerase complex with σ ⁷⁰ , the efficiency of transcription initiation changed significantly. Thus, on the basis of promoters created using sequences of arbitrary composition, promoters of various strengths can be obtained, and the optimal design can be selected by directly evaluating the productivity (or other physiological characteristics) of the obtained plasmid-free strain.

This general approach was used to “fine tune” the level of sucAB gene expression in the model recombinant E. coli strain to increase the level of L-glutamic acid production. Optimization, as opposed to maximizing gene or operon expression, is an urgent problem in creating various bacterial strains producing biologically active substances, especially in cases where the low level of expression of a target gene or group of genes is insufficient to achieve a specific goal, and, on the other hand, overexpression the corresponding gene or group of genes can give not only a neutral, but even a negative effect. Moreover, the desired level of key gene expression is usually not known. "Fine tuning" is the best suited to achieve optimization and, in addition, makes it possible to test a large number of options. The traditional approach of carrying out such “fine tuning” involves molecular cloning of the target gene into a recombinant plasmid, where the gene is placed under the control of various promoters, after which the properties of the obtained recombinant strains are evaluated. If you want to get improved plasmid-free strains, then after selecting the best options you need to make a lot of additional effort.

1. The method according to the present invention

The method according to the present invention is a method for producing an L-amino acid producing bacterium with an optimized gene expression level that affects the distribution of carbon or nitrogen fluxes in said bacterium and as a result affects the L-amino acid production, which includes the following steps:

1) introducing into the bacterial chromosome a set of DNA fragments synthesized in vitro and containing the regulatory elements of gene expression, instead of the natural element of the regulatory region of the gene to obtain a bacterial population; and 2) breeding bacteria with the desired phenotype.

The term "expression", as used here, means the production of a protein product encoded by a certain gene.

The term “optimized expression level” means an expression level of a target gene or several genes at which the bacterium exhibits the desired phenotype.

The term “desired phenotype” includes one or more characteristics of bacteria that are the object of improvement. In particular, this may be the ability of the bacterium to produce L-amino acids in an amount greater than that of the parent strain, the ability to grow on a minimal medium that does not contain additives commonly used to complement auxotrophy or other factors limiting growth, or a combination of such characteristics.

The term "gene encoding a protein that affects the distribution of carbon or nitrogen flows" means a gene encoding a protein involved in the pathway of carbon or nitrogen metabolism. Such genes are genes involved in glycolysis, nitrogen assimilation, genes of the pentose cycle, tricarboxylic acid cycle, etc. More specifically, the genes encoding glutamate dehydrogenase, glutamine synthetase, glutamate synthase, isocitrate dehydrogenase, aconitate hydratase, citrate synthase, phosphoenolpyruvate carboxylase, pyruvate dehydrogenase, pyruvate kinase, phosphoenolpyruvate synthase, enolase, phosphoglyceromutase, phosphoglycerate kinase, glyceraldehyde-3-phosphate dehydrogenase, triozafosfatizomerazu, fruktozadifosfataldolazu, phosphofructokinase, glyukozafosfatizomerazu, glutamine oksoglutarataminotransferazu , isopropyl malate synthase, etc. Bacterial genes involved in the biosynthesis of L-amino acids, nucleic acids and their precursors also belong to such genes.

The term "set of DNA fragments synthesized in vitro" means a mixture of newly synthesized DNA fragments or a mixture of previously known DNA fragments obtained from natural or mutant microorganisms, DNA libraries, GenBank, etc. A set of DNA fragments can be obtained by directly mixing newly synthesized DNA fragments with a known sequence, DNA fragments obtained from various sources mentioned above, or DNA fragments obtained during chemical synthesis in which a certain position or region is “randomized”, t .e. contains a sequence of nucleotides of arbitrary composition.

The term “randomized” means that, during standard chemical synthesis of a DNA fragment, a nucleotide of arbitrary composition (usually denoted as N, where N is adenine, guanine, cytosine or thymine) is inserted into a specific position of this DNA fragment or in a certain region of it. These DNA fragments contain sequences called regulatory elements.

The term "regulatory element" refers to nucleotide sequences located before, inside and / or after the coding region, controlling the transcription and / or expression of the coding region when interacting with a cellular protein biosynthesis apparatus. This term is usually used to refer to promoters, ribosome binding sites (RBS), operators, and other elements of the genome that affect the level of gene expression.

A mixture of these DNA fragments containing regulatory elements is used to introduce bacteria into the chromosome instead of the natural regulatory element to form a bacterial cell population with different levels of expression of the target gene. Bacteria with the desired phenotype are selected by directly assessing the amount of L-amino acid produced by the bacterium on a standard minimum nutrient medium, or by other methods suitable for assessing the characteristics essential for the bacterium to possess the desired phenotype.

The term “bacterium producing L-amino acids”, as used here, also means a bacterium having the ability to produce and accumulate L-amino acids in a nutrient medium in an amount greater than the parent strain or wild-type strain, and preferably means that the bacterium has the ability to production and accumulation in a nutrient medium of at least 0.5 g / l, more preferably at least 1 g / l of the target L-amino acid.

The term "bacterium belonging to the genus Escherichia" means that the bacterium belongs to the genus Escherichia in accordance with the classification known to the person skilled in the field of microbiology. As an example of a microorganism belonging to the genus Escherichia used in the present invention, the bacterium Escherichia coli (E. coli) may be mentioned.

It is not obvious to a person skilled in the art what level of enzyme activity and what type of regulatory element sequence are optimal for specific conditions. And therefore, the choice of the sequence of the regulatory element, based on scientific assumption or insight, may not lead to an optimal result. Moreover, the preparation of even a limited number of mutants with different levels of enzyme activity is a complex process that requires a significant investment of time, since these mutants are traditionally obtained sequentially, one by one. On the contrary, the method according to the present invention has the advantage of being a simple, one-step process of integrating artificial or natural DNA fragments into the chromosome to obtain a bacterial cell population with a wide range of expression levels of the target gene. For example, the “randomization” of 4 nucleotides in a certain region of a chemically synthesized regulatory element gives 4 ⁴ = 256 theoretically possible variants of this region.

Further, it is common practice to initially evaluate the activity of a target enzyme by introducing a gene encoding this enzyme into a plasmid, which is then inserted into a bacterium. But the expression level of the gene integrated into the bacterial chromosome and the expression level of the same gene introduced into the plasmid inserted into the bacterium are not the same. Thus, another advantage of the method according to the present invention is that this method allows the evaluation and selection of bacteria with the expression level of the target gene that is optimal for these specific conditions, followed by the direct use of the obtained bacteria for the production of L-amino acids without any additional manipulations .

Methods for obtaining plasmid DNA, DNA cleavage and ligation, transformation, selection of oligonucleotides as seeds and the like are traditional methods well known to a person skilled in the art. These methods are described, for example, in Sambrook, J., Fritsch, E.F., and Maniatis, T., "Molecular Cloning A Laboratory Manual, Second Edition", Cold Spring Harbor Laboratory Press (1989).

2. The bacterium according to the present invention

The bacterium of the present invention is an L-amino acid producing bacterium having an optimized level of gene expression that affects the production of L-amino acids. A similar bacterium can be obtained by the method according to the present invention.

More specifically, the bacterium of the present invention is a bacterium producing L-amino acid derived from L-glutamic acid, having an optimized expression level of a gene that affects the production of L-glutamic acid. From L-glutamic acid, L-arginine, L-proline and L-glutamine are formed. Also, the bacterium according to the present invention is a bacterium producing L-glutamic acid, having an optimized level of gene expression that affects the production of L-glutamic acid. In addition, L-glutamic acid plays an important role in the biosynthesis of L-leucine, L-lysine, L-isoleucine, L-valine, L-histidine, L-aspartate, L-alanine, L-tyrosine and L-phenylalanine as a donor amino groups. Also, the bacterium of the present invention is an L-leucine producing bacterium with an optimized gene expression level that affects the production of L-leucine.

Thus, an increase in the number of substrate — nitrogen donors — for the gene encoding aminotransferase positively affects the production of amino acids such as L-leucine, L-lysine, L-isoleucine, L-valine, L-histidine, L-aspartate, L-alanine , L-tyrosine and L-phenylalanine.

A practical embodiment of the present invention is an E. coli strain 702ilvA (VKPM B-8012) (European Patent Application 1772433 A1) containing the recombinant plasmid pAYCTERl-cpg and modified to optimize the expression of sucAB genes. The plasmid pAYCTERl-cpg is a derivative of the RSF1010 replicon containing natural genes encoding citrate synthase (gltA gene), PEP carboxylase (ppc gene), glutamate dehydrogenase (gdhA gene) and proBA operon cloned from E. coli K-12 standard methods. Optimization of sucAB gene expression was carried out in accordance with the method according to the present invention. The indicated recombinant strain 702ilvA (pAYCTERl-cpg) is deficient in threonine deaminase activity, requires the presence of L-isoleucine for growth, and is capable of producing L-proline and glutamic acid during cultivation.

Examples of bacteria belonging to the genus Escherichia that are capable of producing L-glutamic acid and can be used to optimize gene expression are the following E. coli strains: strains that are resistant to aspartic acid antimetabolites and are deficient in α-ketoglutarate dehydrogenase activity, such as AF13199 (FERM BP-5807) (US patent 5908768), or strain FERM P-12379, further characterized by reduced decomposition ability of L-glutamic acid (US patent 5393671); E. coli strain AJ13138 (FERM BP-5565) (US Pat. No. 6,110,714) and the like. The ability to produce L-glutamic acid can be imparted, for example, by introducing DNA encoding any of such enzymes as glutamate dehydrogenase (Japanese Patent Application Laid-Open (Kokai) No. 61-268185 / 1986), Glutamine Synthetase, Glutamate Synthase, Japan Isocitrate Dehydrogenase (Patent Application (Kokai) No. 62-166890 / 1987 and No. 63-214189 / 1988), aconitate hydratase (Japanese Patent Application Laid-Open (Kokai) No. 62-294086 / 1987), citrate synthase (Japanese Patent Laid-open Application (Kokai) No. 62-201585 / 1987 and No. 63-119688 / 1988), phosphoenolpyruvate carboxylase (laid out latent application Yapo Research Institute (Kokai) No. 60-87788 / 1985 and No. 62-55089 / 1987), pyruvate dehydrogenase, pyruvate kinase, phosphoenolpyruvate synthase, enolase, phosphoglyceromutase, phosphoglycerate kinase, glyceraldehyde phosphate phosphate dehydrogenase (3-phosphate dehydrogenase) No. 63-102692 / 1988), glucose phosphatisomerase, glutaminoxoglutarate aminotransferase (WO 99/07853) and so on. Moreover, the bacterium according to the present invention can be modified to reduce the activity of enzymes that catalyze the formation of compounds other than L-glutamic acid, which branch off from the main biosynthesis pathway of L-glutamic acid. Enzymes that catalyze the formation of compounds other than L-glutamic acid branching from the main biosynthesis pathway of L-glutamic acid include α-ketoglutarate dehydrogenase, isocitrate lyase, phosphate acetyltransferase, acetate acetate kinase, acetyl dehydrogenacetase azinase dehydrogen acetate etc.

It is also possible to use bacteria producing L-leucine belonging to the genus Escherichia, such as strains of E. coli H9068 (ATCC 21530), H-9070 (FERM BP-4704) and H-9072 (FERM BP-4706), resistant to 4 -azaleucine or to 5,5,5-trifluoroleucine (US patent 5744331), strains of E. coli, in which there is no inhibition of feedback of isopropyl malate synthase by L-leucine (European patent EP 1067191), E. coli strain AJ11478, resistant to ( 3-2-thienylalanine and β-hydroxyleucine (US patent 5763231), strain E. coli 57 (VKPM B-7386, Russian patent No. 2140450) and the like.

A similar strategy described above for L-glutamic acid can be used to obtain other known L-amino acids.

2. The method of obtaining L-amino acids

The method according to the present invention is a method for producing L-amino acids, comprising the steps of growing a bacterium according to the present invention in a nutrient medium in order to produce and accumulate an L-amino acid in a nutrient medium and isolate the L-amino acid from the culture fluid. In particular, the method according to the present invention is a method for producing L-glutamic acid, comprising the steps of growing a bacterium according to the present invention in a culture medium in order to produce and accumulate L-glutamic acid in a culture medium, and isolate L-glutamic acid from the culture fluid. Also, a method for producing L-amino acids includes a method for producing L-leucine, comprising the steps of growing a bacterium according to the present invention in a culture medium (for the purpose of production and accumulation of L-leucine in a culture medium) and isolating L-leucine from the culture fluid.

In the present invention, the cultivation, isolation and purification of an L-amino acid from a culture or similar liquid may be carried out in a manner similar to traditional fermentation methods in which the amino acid is produced using a bacterium.

The nutrient medium used for growing can be either synthetic or natural, provided that the medium contains sources of carbon, nitrogen, mineral additives and, if necessary, the appropriate amount of nutrient additives necessary for the growth of bacteria. Carbon sources include various carbohydrates such as glucose and sucrose, as well as various organic acids. Depending on the nature of the assimilation of the microorganism used, alcohols such as ethanol and glycerin may be used. Various inorganic ammonium salts, such as ammonia and ammonium sulfate, other nitrogen compounds, such as amines, natural nitrogen sources, such as peptone, soybean hydrolyzate, microorganism fermentolizate, can be used as a nitrogen source. As mineral additives, potassium phosphate, magnesium sulfate, sodium chloride, iron sulfate, manganese sulfate, calcium chloride and the like can be used. Thiamine and yeast extract can be used as vitamins.

The cultivation is preferably carried out under aerobic conditions, such as mixing the culture fluid on a rocking chair, shaking with aeration, at a temperature in the range from 20 to 40 ° C, preferably in the range from 30 to 38 ° C. The pH of the medium is maintained in the range from 5 to 9, preferably from 6.5 to 7.2. The pH of the medium can be adjusted by ammonia, calcium carbonate, various acids, bases and buffer solutions. Typically, growing for 1 to 5 days leads to the accumulation of the target L-amino acid in the culture fluid.

After growth, solid residues, such as cells, can be removed from the culture fluid by centrifugation or filtration through a membrane, and then the L-amino acid can be isolated and purified by ion exchange chromatography, concentration and crystallization.

BEST MODE FOR CARRYING OUT THE INVENTION

The present invention will be described in more detail below with reference to Examples.

Example 1. Replacement of the natural region located in the chromosome of the E. coli bacterium before sucAB genes, a hybrid regulatory element containing the synthetic promoter P _tac * and SD _lacZ .

The modified P _tac * promoter, attached to the Shine-Dalgarno sequence (SD sequence) of the E. coli lacZ gene, was integrated upstream of the coding portion of sucAB genes in the chromosome of E. coli strain 702ilvA (pAYCTERl-cpg) instead of the native region using the technique described Datsenko KA and Wanner BL (Proc.Natl.Acad.Sci.USA, 97, 6640-6645, 2000), also called “recombination using the Red system”. The modified P _tac * promoter contained only the first 11 base pairs from 21 pairs of the lactose operator (O _lac ) and therefore was not able to interact with the lactose repressor due to the lack of nucleotides essential for such a specific DNA-protein contact. In addition, an artificial DNA fragment containing the chloramphenicol resistance gene (Cm ^R ) necessary for the selective integration of the obtained fragments into the corresponding region of the bacterial chromosome was attached to the 5'-part of the modified P _tac * promoter.

A design diagram of the indicated artificial DNA fragment is shown in the drawing. The nucleotide sequence of the replaced natural region upstream of the sucAB genes is shown in Sequence Listing No. 1 (SEQ ID NO: 1).

The in vitro construction of the aforementioned artificial DNA fragment, in addition to containing the chloramphenicol resistance gene (Cm ^R ), was carried out in several stages. In the first stage, the P _tac * promoter was amplified by PCR so that the resulting fragment in the 5'-region contained the BglII recognition site (for the convenience of obtaining the subsequent genetic engineering construct, see below) and the SD sequence and ATG start codon of the lacZ gene from E. coli, attached directly to the N-terminal part of the coding region of the sucA gene, in the 3'-region of the obtained fragment containing the promoter. A commercially available recombinant plasmid pDR540 (GenBank / EMBL U13847, Pharmacia, USA) was used as a template for PCR. Chemically modified oligonucleotides PI (SEQ ID NO: 2) and P2 (SEQID NO: 3) were used as primers for PCR.

In all cases, PCR was performed using a Perkin-Elmer 2400 GeneAmp PCR System thermal cycler. The reaction mixture with a total volume of 50 μl contained 5 μl of 10x PCR buffer (Fermentas, Lithuania) supplemented with MgCl ₂ to a final concentration of 1.5 mM, 200 μM of each dNTP triphosphate in the reaction mixture, 400 nM of each seed used and 2 units of Taq- polymerases (Fermentas, Lithuania). The amount of DNA used as a template for PCR was added at the rate of 0.2 ng of the target DNA fragment. The PCR temperature profile was as follows: denaturation step for 5 min at 95 ° С followed by 20 denaturation cycles at 95 ° С for 30 seconds, annealing at 55 ° С for 30 seconds, chain growth at 72 ° С; the final stage of polymerization at 72 ° C for 2 minutes. The chain growth time was chosen in accordance with the recommendations of the Taq polymerase manufacturer depending on the length of the amplified DNA fragment. In particular, for this particular case, the chain growth time was 1.5 minutes.

In parallel, the second stage of the construction of the hybrid DNA fragment was carried out. The Cm ^R gene was amplified using the commercially available plasmid pACYC184 (accession number X06403 at GenBank, Fermentas, Lithuania) as a template and chemically synthesized oligonucleotides P3 (SEQ ID NO: 4) and P4 (SEQ ID NO: 5) as seeds . Oligonucleotide P3 contained the BglII recognition site used to attach to the previously obtained DNA fragment with the P _tac * promoter. P4 oligonucleotide contained 36 nucleotides located in front of the regulatory region of sucAB genes in the E. coli chromosome, which are necessary for subsequent recombination of the target fragment into the bacterial chromosome using the Red system.

The two DNA fragments obtained were treated with BglII restriction endonuclease and then ligated with T4 DNA ligase (Maniatis T., Fritsch EF, Sambrook, J .: Molecular Cloning: A Laboratory Manual. 2 ^nd edn. Cold Spring Harbor, NY: Cold Spring Harbor Laboratory Press, 1989). In the last step, the ligation product was amplified using P1 and P4 seeds. The resulting DNA fragment was purified by precipitation in ethanol and used for electroporation and recombination using the Red system into the chromosome of E. coli strain 702ilvA (pAYCTERl-cpg). The strain E. coli 702ilvA (pAYCTERl-cpg) is a derivative of the strain E. coli 702ilvA - producer of L-glutamic acid (VKPM B-8012) (European patent application 1772433 A1), additionally carrying the recombinant plasmid pAYCTERl-cpg. The plasmid pAYCTERl-cpg is a derivative of the vector pAYCTER3 carrying the natural genes encoding citrate synthase (gltA gene), PEP carboxylase (ten ppc), glutamate dehydrogenase (gdhA gene) and proBA operon cloned from E. coli K-12 using standard methods as PCR using the chromosomal DNA of E. coli K-12 strain as a template and seed with restriction enzyme recognition sites suitable for further cloning and assembly of PCR products. The vector pAYCTER3 is a derivative of the mid-copy and very stable vector pAYC32 constructed on the basis of the plasmid RSF1010 (Christoserdov AY, Tsygankov YD, Plasmid, 1986, v.16, pp. 161-167), which carries a marker of resistance to streptomycin. The pAYCTER3 vector was obtained by introducing a polylinker from plasmid pUC19 and the strong terminator rrnB into plasmid pAYC32 instead of its promoter as follows. First, using the PCR and primers shown in the List of sequences under numbers 6 (SEQ ID NO: 6) and 7 (SEQ ID NO: 7), the polylinker of plasmid pUC19 was obtained. The resulting PCR product was treated with restriction enzymes EcoRI and BglII. The rrnB terminator was also obtained using PCR and primers shown in the Sequence Listing numbers 8 (SEQ ID NO: 8) and 9 (SEQ ID NO: 9). The resulting PCR product was treated with restriction enzymes BglII and BclI. These two DNA fragments were then ligated into the pAYC32 plasmid pretreated with restriction enzymes EcoRI and BclI. So the plasmid pAYCTER3 was obtained.

The recombinant plasmid pKD46 (Datsenko, KA, Wanner, BL, Proc.Natl.Acad.Sci. USA, 97, 6640-6645, 2000) with a heat-sensitive replicon was used as a donor of phage λ genes necessary for the Red recombination system. Cells of strain 702ilvA (pAYCTERl-cpg) were transformed with plasmid pKD46 according to the standard Ca transformation protocol (Maniatis T., Fritsch EF, Sambrook, J .: Molecular Cloning: A Laboratory Manual. 2 ^nd edn. Cold Spring Harbor, NY: Cold Spring Harbor Laboratory Press, 1989) followed by selection of transformants on L-agar plates (Tryptone, 10 g / L; yeast extract, 5 g / L; NaCl, 10 g / L; agar 1.5%) containing ampicillin ( 100 μg / ml). The plates were incubated overnight at 30 ° C and the resulting clones were used to prepare an electrocompetent culture. For this, cells were grown overnight at 30 ° C in LB liquid medium containing ampicillin (100 μg / ml) and streptomycin (25 μg / ml), then diluted in a ratio of 1: 100 with SOB medium (yeast extract, 5 g / l ; NaCl, 0.5 g / L; Trypton, 20 g / L, KCl, 2.5 mm; MgCl ₂ , 10 mm) containing ampicillin (100 μg / ml), streptomycin (25 μg / ml) and arabinose (10 mm ) (arabinose was used to induce a plasmid encoding the genes of the phage X homologous recombination system) and grown at 30 ° C until the optical density of the bacterial culture was OD ₆₀₀ = 0.8-1.0. Cells from 10 ml of the obtained bacterial culture were washed 3 times with deionized water, cooled in ice, then 200 ml of glycerol (10%) and resuspended in 40 μl of glycerol (10%). 0.5 μg of the amplified DNA fragment described above was dissolved in 5 μl of deionized water and added to the bacterial culture immediately prior to electroporation. Electroporation was carried out using the Bio-Rad device for electro-transformation of bacteria (USA) (No. 165-2098, version 2-89) in accordance with the manufacturer's recommendations for E. coli cells (pulse time - 4-5 milliseconds, electric field intensity - 12.5 kV / cm).

Immediately after electroporation, 1 ml of SOC medium was added to the cell suspension (yeast extract, 5 g / L; NaCl, 0.5 g / L; Tryptone, 20 g / L, KCl, 2.5 mm; MgCl ₂ , 10 mm; glucose, 20 mm). Then, the obtained cells were grown with stirring for 2 hours at 37 ° C and the integrands were selected on L-agar plates containing chloramphenicol (25 μg / ml) and streptomycin (25 μg / ml), growing them overnight at 37 ° FROM.

The obtained Cm ^R , Sm ^R clones were replicated onto L-agar plates and grown overnight at 42 ° C in order to eliminate the heat-sensitive auxiliary plasmid pKD46. The replacement of the natural regulatory region of sucAB genes with an artificial in vitro hybrid DNA fragment in Ap ^S Cm ^R Sm ^R clones obtained from strain 702ilvA (pAYCTERl-cpg) was confirmed by PCR.

Example 2. The effect of the promoter P _tac * on the activity of α-ketoglutarate dehydrogenase and the production of L-glutamic acid and L-proline.

One loop of each of the strains 702ilvA (pAYCTERl-cpg) and 702ilvA tac * (pAYCTERl-cpg) grown on L-agar plates inoculated Erlenmeyer flasks containing 75 ml of culture medium containing Tryptone 10 g / l; yeast extract 5 g / l; NaCl 4 g / l and streptomycin (25 μg / ml) to stabilize the recombinant plasmid pAYCTER1-cpg, and were grown for 6 hours at 37 ° C with stirring (140 rpm). Then, 50 ml of the grown culture was inoculated with a Jar fermenter (Marubishi, Japan). The composition of the nutrient medium for fermentation (total volume 500 ml) is as follows: glucose 100 g / l; (NH ₄ ) ₂ SO ₄ 2 g / l; KH ₂ PO ₄ 1 g / l; MgSO ₄ * 7H ₂ O 0.4 g / l; FeSO ₄ * 7H ₂ O 0.01 g / l; MnSO ₄ * 5H ₂ O 0.01 g / l; L-isoleucine, 0.2 g / l; Mameno 0.2 g / l (total nitrogen); thiamine ^* HCl 0.0004 g / l; pH 6.7. During fermentation with aeration and stirring (900 rpm) at 35 ° C, the pH of the medium was maintained by adding a solution of NH ₄ OH.

The amount of L-glutamic acid and L-proline was determined by high performance liquid chromatography (HPLC). Conditions for HPLC: Luna C ₁₈ (2) column, 150 × 3 mm, 5U, temperature 17 ° C. Eluent: CH ₃ CN - 0.8% (v / v), H ₃ PO ₄ 0.1% (v / v), KH ₂ PO ₄ - 10 mM, nC ₈ H ₁₇ SO ₃ Na - 3 mM. The flow rate of 0.4 ml / min, the application volume of 10 μl. Detection at 200 nm. Retention times: glutamic acid 9.3; proline 12.1.

The level of activity of α-ketoglutarate dehydrogenase in the obtained strains was determined in accordance with the standard method (Amarasingham & Davis // J. Biol. Chem. 1965. 240, 3664-3668) after cell growth under conditions in which the level of accumulation of L-glutamic acid and L-proline. The data are shown in Table 1.

As can be seen from the data shown in Table 1, the replacement of the natural promoter P _suc * with the stronger promoter P _tac * leads to an increase of up to 3 times the specific activity of α-ketoglutarate dehydrogenase in the cells of the new strain compared to its predecessor.

At the same time, the cells of the new strain partially lost the ability to superproduce L-glutamic acid. Although the level of accumulation of L-proline by the new strain slightly increased compared to the unmodified strain, the total conversion of carbon from glucose to amino acids of the L-glutamic acid family (in this case, L-glutamic acid and L-proline) decreased significantly.

The results clearly indicate that the use of the strong constitutive promoter P _tac * containing the consensus regions “-10” and “-35” leads to a 3-fold increase in the activity of α-ketoglutarate dehydrogenase and, accordingly, to a decrease in the ability to produce L-glutamine acids. There was a slight increase in the growth rate of the obtained strain compared with the strain containing the natural promoter P _suc (table 1). This is probably due to an increase in the carbon flux through the tricarboxylic acid cycle and, consequently, to a higher level of ATP synthesis in this strain.

On the other hand, as mentioned in the description of the prior art, mutants belonging to the genus Escherichia are producers of glutamic acid, which lack or reduce the activity of α-ketoglutarate dehydrogenase, are not able to grow or are able to grow at a low rate in a minimal environment with glucose under aerobic conditions. To restore the ability to grow, suppression of succinic acid or lysine in combination with methionine is necessary. Thus, it is necessary to select the optimal level of expression of α-ketoglutarate dehydrogenase in bacteria in order for such a bacterium to be able to produce glutamic acid and grow in a nutrient medium that does not contain additional nutritional supplements, such as succinic acid, lysine or methionine.

To obtain a prototrophic strain with a high level of L-glutamic acid production and good growth rate, it was decided to optimize the expression of sucAB genes by “randomizing” the consensus region “-35” of the P _tac * promoter in order to decrease the efficiency of transcription initiation (in comparison with the P promoter _tac *) and, as a result, a decrease in the activity of α-ketoglutarate dehydrogenase and an increase in the yield of L-glutamic acid.

Example 3. Obtaining an artificial regulatory element containing a region with a sequence of nucleotides of random composition ("randomized" region), and replacing the natural site in front of sucAB genes in the E. coli chromosome with such an artificial element.

A set of artificial regulatory elements containing a “-35” randomized region was obtained by PCR using synthetic oligonucleotides PI (SEQ ID NO: 2) and PS (SEQ ID NO: 10) as seeds and plasmid pDR540 as a template. The PS seed (SEQ ID NO: 10) consists of 51 nucleotides and contains a region with 4 nucleotides of random composition, designated in the sequence SEQ ID NO: 10 by the letter "n". Thus, the artificial DNA fragment contained a hybrid regulatory element with a "randomized" region and a chloramphenicol resistance gene (Cm ^R ), and the subsequent integration of this fragment into the chromosome was carried out as described in Example 1.

The colonies of the obtained integrants grown on L-agar had different sizes and had different growth rates. Selection was carried out by the productivity of L-glutamic acid. Two of the best clones, No. 2 and No. 21, with the highest L-glutamic acid production, were selected. At the same time, these clones had a high overall conversion of glucose carbon to amino acids of the L-glutamic acid family (in this case, L-glutamic acid and L-proline). Genomic DNA from these clones was isolated using the "Genomic DNA isolation kit" (Sigma, USA) in accordance with the manufacturer's recommendations. To amplify an artificial regulatory element containing a "randomized" region, PCR was performed using isolated DNA as a template and oligonucleotides PI (SEQ ID NO: 2) and P4 (SEQ ID NO: 5) as seeds. The sequences of both amplification products were determined by the Senger method. Artificial promoters from clones 2 and 21 were designated P _tac-2 and P _tac21, respectively. The sequences of tetramers obtained by "randomization" are shown in the List of sequences under the numbers 11 (SEQ ID NO: 11) and 12 (SEQ ID NO: 12), respectively.

Example 4. The effect of an artificial regulatory element on the activity of α-ketoglutarate dehydrogenase and the production of L-glutamic acid and L-proline.

The fermentation of clones 2 and 21, the measurement of the amount of L-glutamic acid and L-proline, as well as the determination of the activity of α-ketoglutarate dehydrogenase was carried out as described in Example 2.

As can be seen from Table 1, we can assume that the introduction of a constitutive promoter, such as P _tac , with an optimized strength lower than that of P _tac , instead of the natural promoter P _suc, allows _one to choose strain variants with improved production of L-glutamic acid and higher carbon conversion from glucose to amino acids of the L-glutamic acid family (in this case, -L-glutamic acid and L-proline). Moreover, strain variants exhibit the ability to grow well on minimal medium that does not contain additional additives, such as succinic acid, lysine or methionine, with glucose as a carbon source. As can be seen from Table 1, the optical density of the cultures under standard fermentation conditions for strains containing the P _tac-2 and P _{tac21 promoters} was not much lower than that of the strain with the natural P _suc promoter.

Table 1 Strain Promoter SucAB activity, rel. OD ₅₄₀ Growing time, h amount The total yield of glutamic acid from glucose *,% L-proline, g / l L-glutamic acid, g / l 702ilvA [pAYCTER1-cpg] P _suc 90 37.8 25.5 18.0 8.1 37.3 702ilvA tac * [pAYCTER1-cpg] P _tac * 300 41.4 27.1 21.1 0 33.8 2 P _tac-2 80 33.0 26.3 14.0 20.5 44.1 21 P _tac-21 55 33.0 27.0 12.5 25.2 46.5 * The yield was calculated by L-glutamic acid, taking into account the molecular weights (MW) of L-glutamic acid and L-proline, according to the following formula: Total yield = amount of L-glutamic acid ^* 100 / amount of glucose + (amount of L-proline * MW L-glutamic acid * 100) / (amount of glucose * MW L-proline)

Example 5. The effect of the artificial promoter P _tac-21 on the activity of α-ketoglutarate dehydrogenase and the production of L-leucine.

As can be seen from Table 1, the artificial promoter P _tac-21 provides the lowest level of α-ketoglutarate dehydrogenase activity, resulting in a maximum yield of L-glutamic acid. The reduced activity of the SucAB protein involved in the tricarboxylic acid (TCA) cycle leads to a decrease in acetyl CoA consumption in the TCA cycle. Acetyl-CoA is a precursor of L-leucine, therefore, an increased pool of acetyl-CoA can be used for biosynthesis of L-leucine, and, ultimately, can positively affect the production of L-leucine.

To test this hypothesis, the artificial P _tac-21 promoter before sucAB genes was transferred by standard P1 transduction (Sambrook et al, Molecular Cloning A Laboratory Manual, Second Edition, Cold Spring Harbor Laboratory Press (1989)) to the L-leucine producer strain E. coli and selected for resistance to Cm, while E. coli strain 21 was used as a donor. Since the effect of increasing the production of L-leucine is noticeable only in the producer strain with a high yield of L-leucine, the ability to produce L-leucine in the strain producing L-leucine E. coli 57 (VKPM B-7386, Russian patent No. 2140450) was additionally reinforced. Strain 57 produces 1.5-1.7 g / L of L-leucine by fermentation in vitro. For this purpose, leucine auxotrophy was transferred from strain E. coli C600 (leu ^- ) (Appleyard RK, Genetics, 39, 440-452 (1954)) to the chromosome of strain 57 by transduction of phage PI, as described above. Further, the obtained leucine auxotrophy in strain 57leu ^was complementarily replaced by the leuA ^* BCD genes from the E. coli 55 donor strain by analogous P1 transduction. Strain 55 contains the leuA ^* gene encoding mutant alphaisopropylmalate synthase resistant to leucine inhibition by the feedback principle (Russian patent No. 2201454). After gene ilνE, encoding a protein with the activity of transaminase branched amino acids was inactivated in the resulting strain 57leuA ^* and the activity of transaminase aromatic amino acids encoded by the genome of tyrB, was enhanced in the strain 57leuA ^* ilvE ^- transforming the recombinant plasmid pACYC-tyrB (patent Russian Application 2002116773). The resulting strain 57leuA ^* ilvE ^- / pACYC-tyrB produced about 9 g / L L-leucine in vitro fermentation.

The promoter P _tac-21 was introduced into the chromosome of the obtained strain 57leuA ^* ilvE ^- / pACYC-tyrB using standard P1 transduction. The production of L-leucine obtained as a result of strain 57sucleuA ^* ilvE ^- / pACYC-tyrB increased to 11.4 g / l of L-leucine by fermentation in vitro.

One complete microbiological loop of each of the 57leuA ^* ilvE ^- / pACYC-tyrB and 57suc leuA * ilvE ^- / pACYC-tyrB strains grown on L-agar plates was added to 20 × 200 mm fermentation tubes containing 2 ml of medium of the following composition : glucose - 60 g / l, (NH ₄ ) ₂ SO ₄ - 15 g / l, KH ₄ PO ₄ - 1.5 g / l, MgSO ₄ * 7H ₂ O - 1 g / l, thiamine * HCl - 0.1 g / l, CaCO ₃ - 2 g / l, and incubated for 72 hours at a temperature of + 34 ° C on a rotary shaker (250 rpm).

The amount of L-leucine was determined using high performance liquid chromatography (HPLC). The following HPLC conditions were used: Separon SGX C ₁₈ , 150 × 3.3 mm, 5 μm, temp: 22 ° C. Eluent: СН ₃ СМ-15% (v / v), Cu (СН ₃ СОО) ₂ - 0.1 M. Flow rate - 0.3 ml / mm, sample volume - 0.5 μl. The wavelength is 232 nm.

As can be seen from Table 2, the replacement of the natural promoter with the artificial promoter P _tac-21 in the chromosome of strain 57suc leuA * ilvE ^- / pACYC-tyrB is expressed in a decrease in the activity of ketoglutarate dehydrogenase and in an increase in the production of L-leucine.

table 2 Strain Promoter SucAB activity, relative units The concentration of L-leucine, g / l 57leuA * ilvE ^- / pACYC-tyrB Natural P _suc 90 9.1 57leuA * ilvE ^- suc / pACYC-tyrB P _tac-21 36 11.4

Claims (17)

1. A method of producing a bacterium belonging to the genus Escherichia, with an optimized expression level of a gene encoding a protein, affecting the distribution of carbon and nitrogen fluxes in said bacterium, comprising the steps of: but. introducing into the chromosome of the bacterium a set of DNA fragments synthesized in vitro and containing elements that regulate the expression of the specified gene, instead of the natural element of the regulatory region of the specified gene to obtain a population of bacteria and b. breeding bacteria with the desired phenotype. 2. The method according to claim 1, characterized in that said bacterium is a bacterium producing L-amino acids. 3. The method according to claim 2, characterized in that the L-amino acid is selected from the group consisting of L-glutamic acid, L-glutamine, L-proline, L-arginine and L-leucine. 4. The method according to claim 1, characterized in that said bacterium is a bacterium producing a nucleic acid. 5. The method according to claim 4, characterized in that the nucleic acid is selected from the group consisting of inosine, guanosine and adenosine. 6. The method according to claim 1, characterized in that the DNA fragment contains one or more regulatory elements selected from the group consisting of a promoter, a ribosome binding site (RBS) and an operator. 7. The method according to claim 6, characterized in that the set of DNA fragments contains regulatory elements with a sequence of nucleotides of arbitrary composition. 8. The method according to claim 7, characterized in that the set of DNA fragments is composed of regulatory elements with a known sequence and known strength. 9. A bacterium belonging to the genus Escherichia is a producer of an L-amino acid belonging to the L-glutamic acid family with an optimized expression level of a gene encoding a protein that affects the production of the L-amino acid, and such a bacterium is obtained by the method according to any one of claims. 1-8. 10. The bacterium according to claim 9, characterized in that the sequence of the “-35” region of the sucAB gene promoter contains the sequence shown in the List of sequences numbered 11 or 12. 11. The bacterium according to claim 9, characterized in that the L-amino acid belonging to the L-glutamic acid family is selected from the group consisting of L-glutamic acid, L-glutamine, L-proline and L-arginine 12. A bacterium belonging to the genus Escherichia is a producer of an L-amino acid, preferably L-leucine, with an optimized expression level of a gene encoding a protein that affects the production of an L-amino acid, which bacterium is obtained by the method according to any one of claims 1 to 8 . 13. A method for producing an L-amino acid belonging to the L-glutamic acid family, comprising the steps of growing the bacterium of claim 9 in a nutrient medium, causing production and accumulation of the L-amino acid in the nutrient medium, and isolating the L-amino acid from the culture fluid. 14. The method according to item 13, wherein the L-amino acid belonging to the L-glutamic acid family is selected from the group consisting of L-glutamic acid, L-glutamine, L-proline and L-arginine. 15. A method for producing an L-amino acid, preferably L-leucine, comprising the steps of growing the bacterium of claim 12 in a culture medium, causing production and accumulation of the L-amino acid in the culture medium, and isolating the L-amino acid from the culture fluid. Priority on points: 03/12/2003 according to claims 1-11, 13, 14; 12/18/2003 according to paragraphs 12, 15.