Patent Publication Number: US-2022235314-A1

Title: Recombinant escherichia coli strain for producing succinic acid and construction method thereof

Description:
FIELD OF THE INVENTION 
     The present invention relates to the technical field of biological engineering, and more particularly to a recombinant  Escherichia coli  strain for efficiently producing succinic acid and a construction method thereof 
     DESCRIPTION OF THE RELATED ART 
     Succinic acid is an important C4 platform compound. As a starting material for the synthesis of general chemicals, succinic acid has a wide range of applications in food, chemistry, medicine and other fields. Succinic acid is listed by the US Department of Energy at the top place among the 12 most promising bulk bio-based chemicals. 
     Succinic acid is traditionally produced by chemical synthesis, mainly including paraffin oxidation, cyanidation and hydrolysis of methyl chloroacetate, and catalytic hydrogenation of vanadium pentoxide. However, due to the depletion of petroleum resources and the increasingly serious environmental pollution problems, the disadvantages of chemical synthesis become more and more notorious. The production of succinic acid by fermentation can get rid of the dependence on non-renewable strategic resource petroleum, and using renewable resources to fix carbon dioxide and reduce the greenhouse effect shows a prosperous development prospect. At present, the mostly extensively studied succinic acid-producing bacteria include  Actinobacillus succinogenes, Anaerobiospirillum succiniciproducens , and  E. coli. Actinobacillus succinogenes  is usually screened from nature and directed engineered to tolerate high concentration of succinate. Mutant  Actinobacillus succinogenes  strain FZ53 is used by Guettler M et al. to produce succinic acid with a high yield, where glucose is used as a carbon source, and a maximum production reaches 110 g/L after fermentation for 48 h. There are few studies on the  Actinobacillus succinogenes  strains, and further research on their physiological characteristics, fermentation performance and genetic background is needed.  Anaerobiospirillum succiniciproducens  can make use of a wide range of fermentation substrates, such as glucose, lactose, and glycerol, etc. The research results of Samuelov et al. show that the production of succinic acid by  Anaerobiospirillum succiniciproducens  under optimal conditions can be up to 1.2 mol/1.0 mol glucose, and the highest production is 65.0 g/L. However, the fermentation with this strain requires a strict anaerobic environment, which is difficult to attain in industrial applications. As a type strain,  E. coli  has a clear genetic background and is easy to operate. The strain can be engineered by various molecular biology techniques. Therefore, the use of  E. coli  to produce succinic acid by fermentation has become a hot spot and many progresses have been made in the research. Recombinant  E. coli  strain AFP111 is used by Vemuri et al. in a two-stage method, and after fermentation for 76 h, the final concentration of succinic acid can reach 99.2 g/L, the yield is up to 1.1 g/g glucose, and the space time yield reaches 1.3 g/L/h. A recombinant  E. coli  strain HX024 is constructed by Zhang Xueli et al. by genetic engineering and adaptive evolution strategy, with which one-step anaerobic fermentation is performed for 96 h, to obtain a final succinic acid production up to 95.9 g/L and a yield of 1 g/g glucose. The ppc and pck genes are combinatorially optimized and expressed by Zhu Liwen et al. to enhance the CO 2  fixation pathway, and after fermentation with the recombinant  E. coli  strain AFP111 for 96 h, the succinic acid production reaches 90.7 g/L. The glucose absorption and metabolism pathway is optimized and the encoding gene of the by-product acetic acid is knocked out by Zhang Jianguo et al., and after fermentation for 65 h, the final succinic acid production reaches 98.92 g/L. 
     At present, the production efficiency by fermentation with  E. coli  is low. The fermentation broth usually contains by-products such as lactic acid, formic acid, acetic acid, ethanol, and others. The cofactor metabolism during the fermentation process is unbalanced, and the strain cannot tolerate high concentrations of the product and the substrate glucose, high osmotic pressure, and metabolic imbalance caused by rapid glucose absorption and utilization. The product yield and space time yield are low. To obtain a high-performance production strain, a combination method of traditional breeding, various omics analysis, and molecular biological engineering is generally used. 
     SUMMARY OF THE INVENTION 
     To solve the above problems, the present invention provides a recombinant  E. coli  strain for efficiently producing succinic acid. The pyruvate formate lyase coding gene pflB-focA, the lactate dehydrogenase coding gene ldhA, and the phosphotransacetylase coding gene pta in  E. coli  are knocked out from the host strain FMME-N-5 by the Red homologous recombination technology, and the key enzymes phosphoenolpyruvate carboxykinase pck and phosphite dehydrogenase ptxD involved in the succinate synthesis pathway are overexpressed. 
     A first object of the present invention is to provide a recombinant  E. coli  strain for efficiently producing succinic acid. The recombinant  E. coli  stain is obtained by knocking out one or more of the pyruvate formate lyase coding gene pflB-focA, the lactate dehydrogenase coding gene ldhA, and the phosphotransacetylase coding gene pta and overexpressing the phosphoenolpyruvate carboxykinase Pck and the phosphite dehydrogenase PtxD in  E. coli.    
     Preferably, the nucleotide sequence of the gene encoding the phosphoenolpyruvate carboxykinase is as shown in SEQ ID NO:1, and the nucleotide sequence of the gene encoding the phosphite dehydrogenase is as shown in SEQ ID NO:2. 
     Preferably, the phosphoenolpyruvate carboxykinase pck and the phosphite dehydrogenase ptxD are expressed by the plasmid pTrcHisA. 
     Preferably, the nucleotide sequence of the pyruvate formate lyase coding gene pflB-focA is as shown in SEQ ID NO:3; the nucleotide sequence of the lactate dehydrogenase coding gene ldhA is as shown in SEQ ID NO:4; and the nucleotide sequence of the phosphotransacetylase coding gene pta is as shown in SEQ ID NO:5. 
     Preferably, the host of the recombinant  E. coli  strain is FMME-N-5, which was deposited in the China Center for Type Culture Collection (Address: Wuhan University, Wuhan, China) on Aug. 27, 2020, under CCTCC Accession NO: M 2020454. 
     The second object of the present invention is to provide a method for constructing a recombinant  E. coli  strain, which comprises the following steps: 
     (1) constructing pflB-focA, ldhA, and pta gene knockout frame fragments; sequentially transferring the gene knockout frame fragments into a host cell carrying the pKD46 plasmid, and screening to obtain a strain in which the target genes are knocked out; and 
     (2) obtaining the gene fragments of the phosphoenolpyruvate carboxykinase pck and the phosphite dehydrogenase ptxD, ligating the gene fragments to an expression vector, and then transferring the expression vector ligated with the gene fragments to the strain in Step (1), to obtain the recombinant  E. coli  strain. 
     A third object of the present invention is to provide use of the  E. coli  strain in the production of succinic acid. The aerobic-anaerobic two-stage fermentation is carried out with the recombinant  E. coli  strain in a fermentation medium, to obtain a fermentation broth containing succinic acid. 
     Preferably, the fermentation medium includes: glucose 30-50 g/L, corn steep liquor 15-25 g/L, (NH 4 ) 2 SO 4  2-4 g/L, K 2 HPO 4  1.2-2.0 g/L, KH 2 PO 4  0.5-1.0 g/L, MgSO 4 .7H 2 O 0.2-0.5 g/L, and NaCl 1-2 g/L. 
     Preferably, in the aerobic-anaerobic two-stage fermentation, the aerobic stage is shifted to the anaerobic stage when the bacterial cell suspension has an OD 600  of 52-60. 
     More preferably, the aerobic stage is shifted to the anaerobic stage by introducing CO 2  or adding 10-20 g/L bicarbonate. 
     Preferably, in the anaerobic stage, the glucose concentration is controlled to 5-15 g/L. 
     Preferably, the inoculation amount in the aerobic-anaerobic two-stage fermentation is 6-12 vol %; and the fermentation temperature is 35-38° C. 
     Preferably, the fermentation time of the aerobic-anaerobic two-stage fermentation is 50-96 h. 
     Preferably, in the anaerobic stage, a pH neutralizer is added, and the pH neutralizer is selected from the group consisting of Na 2 CO 3 , K 2 CO 3 , NaOH, KOH, CaCO 3 , and basic magnesium carbonate and any combination thereof. 
     Preferably, after aerobic-anaerobic two-stage fermentation for 48 h, an osmotic protective agent is added, the osmotic protective agent is selected from the group consisting of proline, methionine, cysteine, betaine and any combination thereof. 
     In the present invention, the phosphite dehydrogenase (ptxD) can catalyze the conversion of phosphite into one molecule of phosphate, while consuming one molecule of NAD +  to produce one molecule of NADH. The phosphate produced in this reaction has no inhibition on the cell growth and ptxD activity, and the reaction catalyzed by ptxD will not directly compete with the metabolites in the cell. Therefore, the expression of ptxD will increase the supply of NADH without affecting the main metabolic pathway for succinate production. 
     The present invention has the following beneficial effects. 
     In the present invention, the Red homologous recombination strategy is used to knock out the genes encoding related enzymes that affect succinic acid production, including the pyruvate formate lyase, the lactate dehydrogenase, and the phosphotransacetylase, so as to reduce the accumulation of by-products and facilitate the accumulation of succinic acid while the growth of the bacterial cells is not affected. Moreover, the phosphoenolpyruvate carboxykinase and the phosphite dehydrogenase involved in the succinate synthesis pathway are overexpressed, to effectively increase the production of succinic acid. Finally, an engineered strain  E. coli  FMME-N-5(ΔfocA-pflB-ΔldhA-Δpta)-pck-ptxD is obtained. After fermentation with the strain for 96 h, the production of succinic acid reaches 137 g/L, the yield of succinic acid is up to 1 g/g glucose, and the space time yield is 1.43 g/L/h, while no by-products lactic acid and formic acid are accumulated, and the acetic acid content is less than 10 g/L. The strain constructed in the present invention is beneficial to the industrial production of succinic acid. 
     Deposit of Biological Material 
     The  E. coli  strain FMME-N-5 was deposited in the China Center for Type Culture Collection (Address: Wuhan University, Wuhan, China) on Aug. 27, 2020, under CCTCC Accession NO: M 2020454. 
    
    
     
       BRIEF DESCRIPTION OF THE DRAWINGS 
         FIG. 1  is a gel electrophoretogram for verifying the knock-out of pyruvate formate lyase coding gene; 
         FIG. 2  is a gel electrophoretogram for verifying the knock-out of lactate dehydrogenase coding gene; 
         FIG. 3  is a gel electrophoretogram for verifying the knock-out of phosphotransacetylase coding gene; 
         FIG. 4  is a map of a recombinant vector expressing phosphoenolpyruvate carboxykinase and phosphite dehydrogenase; and 
         FIG. 5  shows the results of 96-h fed-batch fermentation with the constructed engineered strain  E. coli  FMME-N-5(ΔfocA-pflB-ΔldhA-Δpta)-pck-ptxD in a fermentor. 
     
    
    
     DETAILED DESCRIPTION OF THE PREFERRED EMBODIMENTS 
     The present invention will be further described below in connection with specific examples, so that those skilled in the art can better understand and implement the present invention; however, the present invention is not limited thereto. 
     Unmentioned nucleotide sequence information in the Sequence Listing: 
     (1) SEQ ID NO:1 is the nucleotide sequence of  Actinobacillus succinogenes -derived phosphoenolpyruvate carboxykinase pck coding gene; 
     (2) SEQ ID NO:2 is the nucleotide sequence of  Pseudomonas stutzeri -derived phosphite dehydrogenase ptxD coding gene; 
     (3) SEQ ID NO:3 is the nucleotide sequence of pyruvate formate lyase coding gene pflB-focA; 
     (4) SEQ ID NO:4 is the nucleotide sequence of lactate dehydrogenase coding gene ldhA; and 
     (5) SEQ ID NO:5 is the nucleotide sequence of phosphotransacetylase coding gene pta. 
     Determination of Bacterial Cell Density: 
     An appropriate amount of fermentation broth is neutralized with 2 mol/L hydrochloric acid, and the cell density is expressed by the absorbance measured by a spectrophotometer at a wavelength of 600 nm. 
     Determination of Glucose: 
     Pretreatment of fermentation broth: The fermentation broth is centrifuged at 12000 r/min for 5 min, and the supernatant is collected. After dilution by an appropriate factor, the glucose concentration in the fermentation broth is determined by M-100 biosensor analyzer. 
     Determination of Organic Acids: 
     High performance liquid chromatography: Pretreatment of fermentation broth: The fermentation broth is centrifuged at 12000 r/min for 5 min, and the supernatant is collected. After dilution by an appropriate factor, the production of succinic acid, lactic acid, formic acid, and acetic acid is detected by high performance liquid chromatography (HPLC). The instrument is Waters e2695 reversed-phase high performance liquid chromatograph, the chromatographic column is Bio-Rad HPX 87H; the mobile phase is 5 mmoL/L H 2 SO 4 , the flow rate is set to 0.6 mL/min; the detector is a UV detector; the detection wavelength is 210 nm, and the column temperature is 35° C. 
     Example 1: Knockout of Pyruvate Formate Lyase Coding Gene 
     (1) To knock out the gene encoding pyruvate formate lyase to reduce the amount of the by-product formic acid, a gene editing fragment was constructed by the Red homologous recombination technology. The gene editing fragment includes upstream and downstream homologous arm regions, and a resistance screening cassette. Using the plasmid pKD4 as a template, the resistance screening gene Kan was amplified with designed primer pair pflB-focA-S/pflB-focA-A as shown in SEQ ID NO:6/SEQ ID NO:7, to obtain a pflB-focA knockout frame fragment. 
     (2) The pKD46 plasmid was transformed into the expression host  E. coli  FMME-N-5 competent cells, and a recombinant strain  E. coli  FMME-N-5-pKD46 was screened out by colony PCR. The obtained pflB-focA knockout frame fragment was transferred into competent cells of the recombinant strain  E. coli  FMME-N-5-pKD46 by electroporation, and a positive transformant was obtained by screening in a plate containing 50 μg/mL Kan. Finally, the temperature-sensitive plasmid pCP20 was used to thermally induce the expression of FLP recombinase to remove the Kan resistance gene, and the cells were subcultured three times at 42° C., to remove the temperature-sensitive plasmids pKD46 and pCP20. In this way,  E. coli  FMME-N-5 (ΔfocA-pflB) in which pyruvate formate lyase coding gene was knocked out was successfully obtained. 
     
       
         
           
               
               
            
               
                   
                 Primer sequence information: 5′→3′ direction 
               
               
                   
                 pflB-focA-S: 
               
               
                   
                 TTACTCCGTATTTGCATAAAAACCATGCGAGTTACGGGCC 
               
               
                   
                   
               
               
                   
                 TATAAGTGTAGGCTGGAGCTGCTTC 
               
               
                   
                   
               
               
                   
                 pflB-focA-A: 
               
               
                   
                 ATAGATTGAGTGAAGGTACGAGTAATAACGTCCTGCTGCT 
               
               
                   
                   
               
               
                   
                 GTTCTCATATGAATATCCTCCTTAG 
               
            
           
         
       
     
     Example 2: Knockout of Lactate Dehydrogenase Expressing Gene 
     (1) The construction of  E. coli  FMME-N-5 (ΔfocA-pflB) was the same as in Example 1. 
     To knock out the gene encoding lactate dehydrogenase to further reduce the amount of the by-product lactic acid, a gene editing fragment was constructed by the Red homologous recombination technology. The gene editing fragment includes upstream and downstream homologous arm regions, and a resistance screening cassette. Using the plasmid pKD4 as a template, the resistance screening gene Kan was amplified with designed primer pair ldhA-S/ldhA-A as shown in SEQ ID NO:8/SEQ ID NO:9, to obtain a ldhA knockout frame fragment. 
     (3) The pKD46 plasmid was transformed into the expression host  E. coli  FMME-N-5-ΔfocA-pflB competent cells, and a recombinant strain  E. coli  FMME-N-5-ΔfocA-pflB-pKD46 was screened out by colony PCR. The obtained ldhA knockout frame fragment was transferred into competent cells of the recombinant strain  E. coli  FMME-N-5-ΔfocA-pflB-pKD46 by electroporation, and a positive transformant was obtained by screening in a plate containing 50 μg/mL Kan. Finally, the temperature-sensitive plasmid pCP20 was used to thermally induce the expression of FLP recombinase to remove the Kan resistance gene, and the cells were subcultured three times at 42° C., to remove the temperature-sensitive plasmids pKD46 and pCP20. In this way,  E. coli  FMME-N-5 (ΔfocA-pflB-ΔldhA) in which lactate dehydrogenase coding gene was knocked out was successfully obtained. 
     
       
         
           
               
               
            
               
                   
                 Primer sequence information: 5′→3′ direction 
               
               
                   
                 ldhA-S: 
               
               
                   
                 ATGAACTCGCCGTTTTATAGCACAAAACAGTACGACAAGAA 
               
               
                   
                   
               
               
                   
                 GTACGTGTAGGCTGGAGCTGCTTC 
               
               
                   
                   
               
               
                   
                 ldhA-A: 
               
               
                   
                 TTAAACCAGTTCGTTCGGGCAGGTTTCGCCTTTTTCCAGAT 
               
               
                   
                   
               
               
                   
                 TGCTCATATGAATATCCTCCTTAG 
               
            
           
         
       
     
     Example 3: Knockout of Phosphotransacetylase Expressing Gene 
     (1) The construction of  E. coli  FMME-N-5 (ΔfocA-pflB-ΔldhA) was the same as in Example 2. 
     (2) To knock out the gene encoding phosphotransacetylase to further reduce the amount of the by-product acetic acid while the growth of cells is ensured, a gene editing fragment was constructed by the Red homologous recombination technology. The gene editing fragment includes upstream and downstream homologous arm regions, and a resistance screening cassette. Using the plasmid pKD4 as a template, the resistance screening gene Kan was amplified with designed primer pair pta-S/pta-A as shown in SEQ ID NO:10/SEQ ID NO:11, to obtain a pta knockout frame fragment. 
     The pKD46 plasmid was transformed into the expression host  E. coli  FMME-N-5-ΔfocA-pflB-ΔldhA competent cells, and a recombinant strain  E. coli  FMME-N-5-ΔfocA-pflB-ΔldhA-pKD46 was screened out by colony PCR. The obtained pta knockout frame fragment was transferred into competent cells of the recombinant strain  E. coli  FMME-N-5-ΔfocA-pflB-ΔldhA-pKD46 by electroporation, and a positive transformant was obtained by screening in a plate containing 50 μg/mL Kan. Finally, the temperature-sensitive plasmid pCP20 was used to thermally induce the expression of FLP recombinase to remove the Kan resistance gene, and the cells were subcultured three times at 42° C., to remove the temperature-sensitive plasmids pKD46 and pCP20. In this way,  E. coli  FMME-N-5 (ΔfocA-pflB-ΔldhA-Δpta) in which phosphotransacetylase coding gene was knocked out was successfully obtained. 
     
       
         
           
               
               
            
               
                   
                 Primer sequence information: 5′→3′ direction 
               
               
                   
                 pta-S: 
               
               
                   
                 GTGTCCCGTATTATTATGCTGATCCCTACCGGAACCAGCGT 
               
               
                   
                   
               
               
                   
                 CGGTCGTGTAGGCTGGAGCTGCTTC 
               
               
                   
                   
               
               
                   
                 pta-A: 
               
               
                   
                 TACACCATCGCGCTGACTGCGATTCAGTCTGCACAGCAGCA 
               
               
                   
                   
               
               
                   
                 GCAGTAACATATGAATATCCTCCTTAG 
               
            
           
         
       
     
     Example 4: Knockout of Phosphotransacetylase-Acetokinase Expressing Gene 
     (1) The construction of  E. coli  FMME-N-5 (ΔfocA-pflB-ΔldhA-Δpta) was the same as in Example 3. 
     To further reduce the amount of the by-product lactic acid, a gene editing fragment was constructed by the Red homologous recombination technology. The gene editing fragment includes upstream and downstream homologous arm regions, and a resistance screening cassette. Using the plasmid pKD4 as a template, the resistance screening gene Kan was amplified with designed primer pair pta-ackA-S/pta-ackA-A as shown in SEQ ID NO:12/SEQ ID NO:13, to obtain a pta-ackA knockout frame fragment. 
     The pKD46 plasmid was transformed into the expression host  E. coli  FMME-N-5-ΔfocA-pflB-ΔldhA-Δpta competent cells, and a recombinant strain  E. coli  FMME-N-5-ΔfocA-pflB-ΔldhA-pKD46 was screened out by colony PCR. The obtained pta-ackA knockout frame fragment was transferred into competent cells of the recombinant strain  E. coli  FMME-N-5-ΔfocA-pflB-ΔldhA-pKD46 by electroporation, and a positive transformant was obtained by screening in a plate containing 50 μg/mL Kan. Finally, the temperature-sensitive plasmid pCP20 was used to thermally induce the expression of FLP recombinase to remove the Kan resistance gene, and the cells were subcultured three times at 42° C., to remove the temperature-sensitive plasmids pKD46 and pCP20. In this way,  E. coli  FMME-N-5 (ΔfocA-pflB-ΔldhA-Δpta-ackA) in which phosphotransacetylase-acetokinase expressing gene was knocked out was successfully obtained. 
     
       
         
           
               
               
            
               
                   
                 Primer sequence information: 5′→3′ direction 
               
               
                   
                 pta-ackA-S: 
               
               
                   
                 ATGTCGAGTAAGTTAGTACTGGTTCTGAACTGCGGTAGTTC 
               
               
                   
                   
               
               
                   
                 TTCAGTGTAGGCTGGAGCTGCTTC 
               
               
                   
                   
               
               
                   
                 pta-ackA-A: 
               
               
                   
                 TCAGGCAGTCAGGCGGCTCGCGTCTTGCGCGATAACCAGTT 
               
               
                   
                   
               
               
                   
                 CTTCCATATGAATATCCTCCTTAG 
               
            
           
         
       
     
     Example 5: Construction of Expression Vector pTrcHisA-Pck 
     The phosphoenolpyruvate carboxykinase pck used in the present invention was derived from  Actinobacillus succinogenes . The genomic DNA of  Actinobacillus succinogenes  was extracted. 
     According to the published genome sequence information, primer pair pck-S/pck-A with a sequence as shown in SEQ ID NO:14/SEQ ID NO:15 was designed. Using the genomic DNA extracted from  Actinobacillus succinogenes  as a template, the pck gene was obtained by amplification using a standard PCR amplification system and procedure. 
     
       
         
           
               
               
            
               
                   
                 pck-S : 
               
               
                   
                    ATGACTGACTTAAACAAACTCGTT 
               
               
                   
                   
               
               
                   
                 pck-A: 
               
               
                   
                    AATACGAAAACCTGGCCGCGGTT 
               
            
           
         
       
     
     The pck obtained by PCR amplification was extracted and recovered by agarose gel nucleic acid electrophoresis. The recovered product and the expression vector pTrcHisA were digested with restriction endonuclease BamH I and XhoI for 3 hrs, and the digested product was recovered by agarose gel nucleic acid electrophoresis. The DNA and linearized plasmid were 1617 and 4405 bp, respectively, which were then ligated overnight at 16° C. with T4 DNA ligase and transformed into JM109 competent cells. Single colonies were picked up for verification by PCR, and the positive transformant was sequenced to be correct, which indicates that the expression vector was constructed successfully. The plasmid was designated as pTrcHisA-pck. 
     Example 6: Construction of Expression Vector pTrcHisA-Pck-ptxD 
     The phosphite dehydrogenase ptxD used in the present invention was derived from  Pseudomonas stutzeri . The genomic DNA of  Pseudomonas stutzeri  was extracted. 
     According to the published genome sequence information, primer pair ptxD-S/ptxD-A with a sequence as shown in SEQ ID NO:16/SEQ ID NO:17 was designed. Using the genomic DNA extracted from  Pseudomonas stutzeri  as a template, the ptxD gene was obtained by amplification using a standard PCR amplification system and procedure. 
     
       
         
           
               
               
            
               
                   
                 Primer sequence information: 5′→3′ direction: 
               
               
                   
                 ptxD-S: 
               
               
                   
                    ATGCTGCCGAAACTGGTGATCACG 
               
               
                   
                   
               
               
                   
                 ptxD-A: 
               
               
                   
                    AATCGTGCGGCGACCAAGCCGAAA 
               
            
           
         
       
     
     The ptxD obtained by PCR amplification was extracted and recovered by agarose gel nucleic acid electrophoresis. The recovered product and the expression vector pTrcHisA-pck were digested with restriction endonuclease XhoI and Hind III for 3 h, and the digested product was recovered by agarose gel nucleic acid electrophoresis. The DNA and linearized plasmid were 1011 and 4370 bp, respectively, which were then ligated overnight at 16° C. with T4 DNA ligase and transformed into JM109 competent cells. Single colonies were picked up for verification by PCR, and the positive transformant was sequenced to be correct, which indicates that the expression vector was constructed successfully. The plasmid was designated as pTrcHisA-pck-ptxD. The recombinant plasmid was electroporated into the expression host  E. coli  FMME-N-5 (ΔfocA-pflB-ΔldhA-Δpta-ackA), to obtain the recombinant strain  E. coli  FMME-N-5 (ΔfocA-pflB-ΔldhA-Δpta-ackA)-pck-ptxD. 
     Example 7: Fed-Batch Fermentation with Recombinant  E. coli  Strain FMME-N-5 (ΔfocA-pflB-ΔldhA-ΔPta-ackA)-Pck-ptxD in a Fermentor 
     The fermentation medium in the fermentor includes glucose 35 g/L, corn steep liquor 20 g/L, (NH 4 ) 2 SO 4  3 g/L, K 2 HPO 4  1.4 g/L, KH 2 PO 4  0.6 g/L, MgSO 4 .7H 2 O 0.5 g/L, and NaCl 2 g/L; and the fed-batch medium comprises glucose 800 g/L. 
     The recombinant  E. coli  strain FMME-N-5-ΔfocA-pflB-ΔldhA-Δpta-pck-ptxD was picked up for two-stage fermentation in a 7.5 L fermentor. The single colonies were inoculated in 25 mL LB medium (in 50 mL shake flask) and used as the primary seed culture, and then cultured at 38° C. and 200 rpm for 8.5 h. 200 μl of the primary seed culture was inoculated into a seed medium in an amount of 50 mL/500 mL, and cultured at 38° C. and 200 rpm for 7.5 h to obtain a secondary seed culture. The initial liquid volume in the fermentor was 4 L, and the inoculation amount of the seed culture was 10%. The fermentation conditions in the aerobic stage were as follows. The culture temperature was 38° C., the air flow rate for aeration was 1 vvm, the initial stirring speed was 600 r/min, the pH was controlled to 7.0 with ammonia, and the dissolved oxygen in the whole aerobic stage was controlled at a level of 20%. The process was shifted to the anaerobic fermentation stage when the bacterial cell density was grown to an OD 600  of 55-60. In the anaerobic stage, aeration was stopped, the stirring speed was 200 r/min, 800 g/L glucose was fed and the feed rate was controlled to control the pH of the fermentation broth to be less than 10 g/L. Basic magnesium carbonate was used to control the pH to 6.5 in the anaerobic stage. The fermentation period was 96 h in total. 
     The test result of the production of succinic acid is shown in  FIG. 5 . After 96 h of fermentation, the production of succinic acid by the recombinant  E. coli  strain FMME-N-5-ΔfocA-pflB-ΔldhA-Δpta-pck-ptxD is up to 137 g/L, the yield of succinic acid is 1 g/g glucose, and the space time yield is 1.43 g/L/h, while no by-products lactic acid and formic acid are accumulated, and the acetic acid content is only 1-2 g/L. 
     The above results indicate that in the present invention, related by-product coding genes including pyruvate formate lyase coding gene focA-pflB, lactate dehydrogenase coding gene ldhA, and phosphotransacetylase coding gene pta are knocked out, and the phosphoenolpyruvate carboxykinase pck and the phosphite dehydrogenase ptxD involved in the succinate synthesis pathway are overexpressed by genetic engineering technologies to balance the cofactor metabolism, thereby effectively improving the production of succinic acid. 
     The above-described embodiments are merely preferred embodiments for the purpose of fully illustrating the present invention, and the scope of the present invention is not limited thereto. Equivalent substitutions or modifications can be made by those skilled in the art based on the present invention, which are within the scope of the present invention as defined by the claims.