Alcohol dehydrogenase mutant and application thereof in cofactor regeneration

Abstract

Disclosed is an alcohol dehydrogenase mutant and application thereof in cofactor regeneration, and belongs to the technical fields of enzyme engineering and bioengineering. The alcohol dehydrogenase mutant is obtained by mutating valine at position 84 and/or tyrosine at position 127 in alcohol dehydrogenase having an original amino acid sequence as set forth in SEQ ID No. 1. The alcohol dehydrogenase mutant has high activity for a variety of alcohol co-substrates, and can catalyze these enzyme co-substrates for the regeneration of cofactor NADPH. Compared with the wild-type alcohol dehydrogenase KpADH, the alcohol dehydrogenase mutant has higher activity and catalytic efficiency, and for co-substrate 1,4-butanediol, its k.sub.cat value can be up to 75.9 min.sup.−1, its k.sub.cat/K.sub.m value can be up to 2009 min.sup.−1.Math.M.sup.−1, and its K.sub.m value can be as low as 11.3 mM. Therefore, the alcohol dehydrogenase mutant has a higher value in industrial application.

Claims

1. An alcohol dehydrogenase mutant, wherein the alcohol dehydrogenase mutant comprises the amino acid sequence of SEQ ID NO: 1 except for substitutions) selected from the group consisting of: a substitution of valine at position 84 of SEQ ID NO: 1 with isoleucine, a substitution of tyrosine at position 127 of SEQ ID NO: 1 with cysteine, a substitution of tyrosine at position 127 of SEQ ID NO: 1 with methionine, a substitution of valine at position 84 of SEQ ID NO: 1 with isoleucine and a substitution of tyrosine at position 127 of SEQ ID NO: 1 with cysteine, and a substitution of valine at position 84 of SEQ ID NO: 1 with isoleucine and a substitution of tyrosine at position 127 of SEQ ID NO: 1 with methionine, and wherein the alcohol dehydrogenase mutant possesses alcohol dehydrogenase activity.

2. An alcohol dehydrogenase mutant, wherein the amino acid sequence of the alcohol dehydrogenase mutant is SEQ ID NO: 2, SEQ ID NO: 3, SEQ ID NO: 4, SEQ ID NO: 5, or SEQ ID NO: 6.

3. A method for producing sodium D-phenylalanine, comprising combining the alcohol dehydrogenase mutant of claim 1, sodium phenylpyruvate, amino acid dehydrogenase DAADH.sub.D94A, NADP+, one of (NH.sub.4).sub.2SO.sub.4, NH.sub.4Cl or CH.sub.3COONH.sub.4, and one of 1,4-butanediol, 1,5-pentanediol, 1,6-hexanediol, isopropanol or 2,3-butanediol in a buffer to conduct an asymmetric reduction reaction at 30-35° C. and a pH value of 7-9 for 1-24 h to obtain sodium D-phenylalanine.

4. The method of claim 3, wherein the amount of the sodium phenylpyruvate is 10-200 mmol/L.

5. The method of claim 3, wherein the amount of the amino acid dehydrogenase DAADH.sub.D94A is 0.5-5 kU/L.

6. The method of claim 3, wherein the amount of the NADP+ is 0.1-1.0 mmol/L.

7. The method of claim 3, wherein the amount of the (NH.sub.4).sub.2SO.sub.4 is 20-200 mmol/L.

8. The method of claim 3, wherein the amount of the 1,4-butanediol is 5-100 mmol/L.

9. The method of claim 3, wherein the amount of the alcohol dehydrogenase mutant is 0.3-3 kU/L.

Description

BRIEF DESCRIPTION OF FIGURES

(1) FIG. 1: Electrophoresis of whole plasmid PCR of wild-type alcohol dehydrogenase KpADH and its mutants M1-M5.

(2) FIG. 2: Electrophoresis of gradient elution of alcohol dehydrogenase mutants M1-M3.

(3) FIG. 3: Electrophoresis of gradient elution of alcohol dehydrogenase mutant M4-M5.

(4) FIG. 4: Schematic diagram of the enzyme-coupled cofactor regeneration reaction system.

(5) FIG. 5: Chiral chromatogram of product D-phenylalanine produced from sodium phenylpyruvate catalyzed by the enzyme-coupled cofactor regeneration reaction.

(6) FIG. 6: Gas chromatogram of coproduct γ-butyrolactone in the enzyme-coupled cofactor regeneration reaction.

DETAILED DESCRIPTION

(7) The present disclosure is further described below in conjunction with specific examples. The primers, vectors, and host cells involved in the following examples are only used for the purpose of illustrating the present disclosure without any limitations thereto.

(8) Detection methods involved in the following embodiment s are as follows:

(9) Method for Detecting Alcohol Dehydrogenase Activity:

(10) The total reaction system is 200 μL, comprising: 1.0 mM NADP.sup.+, 200 mM 1,4-butanediol as the substrate, and glycine sodium hydroxide buffer (Gly-NaOH, 100 mM, pH 9.5), which are thoroughly mixed, incubated at 30° C. for 2 min, and then an appropriate amount of an enzyme solution is added thereto. Changes in absorbance at 340 nm are measured.

(11) The enzyme activity is calculated using the following formula:
Enzyme activity (U)=EW×V×10.sup.3/(6220×I);

(12) In the formula, EW is the change in absorbance at 340 nm in 1 min; V is the volume of the reaction solution in mL; 6220 is the molar extinction coefficient of NAD(P)H in L/(mol.Math.cm); I is optical distance in cm.

(13) One unit of activity (U) corresponds to the amount of enzyme required for the catalytic oxidation of 1 μmol NADP.sup.+ per minute under the above conditions.

(14) Method for Determination of k.sub.cat, K.sub.m and k.sub.cat/K.sub.m Values:

(15) Kinetic measurement is conducted according to the enzyme activity assay, with 10 μL of alcohol substrates of different concentrations, 1 mM NADP.sup.+, 10 μL of enzymes of appropriate concentrations, 170 μL of glycine-sodium hydroxide buffer at pH 9.5, with each sample in triplicate. The change in OD.sub.340 at 30° C. is measured to calculate the specific activity at different concentrations, and further calculate the Michaelis constant (K.sub.m), the maximum reaction velocity (V.sub.max) and the catalytic rate (k.sub.cat). The calculation formulas are as follows:

(16) $\frac{1}{V} = \frac{K_{m}}{V_{\max}} \times \frac{1}{[S]} + \frac{1}{V_{\max}};$

(17) The V.sub.max and K.sub.m values can be calculated from the intercepts of the double reciprocal plot on the X and Y axes;

(18) $k_{cat} = \frac{V_{\max}}{[E]};$

(19) The k.sub.cat value can be further calculated according to the formula.

(20) Method for Detecting the Yield of Product D-Sodium Phenylalanine:

(21) The reacted sample is passed through a membrane and then tested by liquid chromatography where an Astec CHIROBIOTIC™ T chiral column (150 mm×4.6 mm×5 μm, Sigma Technologies Co. Ltd) is used, the mobile phase is methanol:ultrapure water=70:30, the flow rate is 0.5 mL.Math.min.sup.−1, the column oven is set at a temperature of 30° C., the UV absorption wavelength is 210 nm, and the retention time of the product sodium D-phenylalanine is 8.49 min. The liquid chromatogram is shown in FIG. 5.

(22) Method for Detecting Optical Purity of Product D-Phenylalanine:

(23) Method for detecting optical purity ee:

(24) $e e = \frac{A_{S} - A_{R}}{A_{S} + A_{R}} \times 100 %;$

(25) In the formula, A.sub.S is the molar concentration of sodium D-phenylalanine obtained by liquid chromatography; A.sub.R is the molar concentration of sodium L-phenylalanine obtained by liquid chromatography.

(26) Method for Detecting Yield of Co-Product γ-Butyrolactone:

(27) The co-product γ-butyrolactone is detected by gas chromatography with a CP-Chirasil-Dex CB column (25 m×0.25 mm×0.25 μm, Agilent Technologies Co. Ltd). The column temperature is maintained at 70° C. for 5 min and then increased at a rate of 20° C./min to 200° C. which is maintained for 5 min. The temperature of both the vaporization chamber and the detector is set to 250° C. The retention time of γ-butyrolactone is 7.92 min. The gas chromatogram is shown in FIG. 6.

Embodiment 1: Construction of Recombinant Vectors and Recombinant Bacteria Containing Genes Encoding Alcohol Dehydrogenase Mutants M1 to M5

(28) Specifically, the steps are as follows:

(29) Using the recombinant plasmid pET28a-KpADH deposited in the laboratory as a template (described in the patent application with publication number CN105936909A), the amino acid residues at position 84 and position 127 of ADH having an amino acid sequence set forth in SEQ ID NO.1 underwent site-saturation mutagenesis by using the full-plasmid PCR method to obtain recombinant vectors comprising M1, M2, and M3. Then, using the M1 recombinant plasmid as a template, the residue at position 127 of M1 underwent site-saturation mutation by using the full-plasmid PCR method to obtain recombinant vectors comprising M4 and M5;

(30) The primers involved are as follows (all described in the 5′-3′ direction, and the underline represents the mutation site):

(31) TABLE-US-00001 M1: V84-F having an amino acid sequence set forth in SEQ. ID No. 7: GCTTCACCAnnkAACTTCGGC; V84-R having an amino acid sequence set forth in SEQ. ID No. 8: GCCGAAGTTmnnTGGTGAAGC; M2, M3: Y127-F having an amino acid sequence set forth in SEQ. ID No. 9: ACTGCTTCTnnkGCTTCAATT; Y127-R having an amino acid sequence set forth in SEQ. ID No. 10: AATTGAAGCmnnAGAAGCAGT; M4: V84I/Y127C-F having an amino acid sequence set forth in SEQ. ID No. 11: ACTGCTTCTtgtGCTTCAATT; V84I/Y127C-R having an amino acid sequence set forth in SEQ. ID No. 12: AATTGAAGCacaAGAAGCAGT; M5: V84I/Y127M-F having an amino acid sequence set forth in SEQ. ID No. 13: ACTGCTTCTatgGCTTCAATT; V84I/Y127M-R having an amino acid sequence set forth in SEQ. ID No. 14: AATTGAAGCcatAGAAGCAGT;

(32) Among others, the PCR reaction system (50 μL) consists of: 1.0 μL of KOD enzyme (2.5 U/mL), 1.0 μL of template (5-50 ng), 4.0 μL of dNTP, 5.0 μL of 10× reaction buffer, upstream and downstream primers, 1.0 μL each, and ddH.sub.2O making up to 50 μL;

(33) The PCR amplification procedure consists of: (1) denaturation at 94° C. for 3 min, (2) denaturation at 94° C. for 30 sec, (3) annealing at 54° C. for 30 sec, (4) extension at 72° C. for 150 sec, repeating steps (2) to (4) for 10-15 cycles, and finally extension at 72° C. for 10 min; the PCR amplification product is stored at 4° C.

(34) After the PCR was completed, Dpnl restriction endonuclease was added to the reaction mixture and incubated at 37° C. for 1 h. Ten μL of the digested PCR reaction solution was transferred into 50 μL of E. coli BL21 (DE3) competent cells by the CaCl.sub.2 thermal transformation method, and spread onto an LB agar plate containing 50 μg/ml kanamycin sulfate and cultivated at 37° C. for 12 h to obtain recombinant bacteria harboring the recombinant plasmids.

Embodiment 2: Screening of Recombinant Bacteria Harboring Recombinant Vectors

(35) Specifically, the steps are as follows:

(36) Recombinant bacteria with alcohol dehydrogenase mutants M1 to M3 were obtained according to Embodiment 1, and were cultured to obtain bacterial colonies;

(37) 300 μL of an LB liquid medium containing kanamycin (Kan) was added to each well of a 96-deep-well plate, and then the single colonies on the plate in Embodiment 1 were picked out one by one with toothpicks and placed into the deep-well plate, leaving two wells with the wild type KpADH as controls and two wells without inoculation as blank controls. The plate was placed on a shaker to culture overnight at 37° C. and 120 r.Math.min.sup.−1;

(38) The next day, the cultured recombinant bacteria were transferred to another 96-deep-well plate with 600 μL of a liquid medium supplemented with kan. 70 μL of 30% glycerol was added to each well of the original plate which was placed at −80° C. for preserving the bacteria. The other deep-well plate was placed in a shaker to culture at 37° C. with shaking at 120 r.Math.min.sup.−1 for 2 h. Thereafter, the inducer IPTG was added (to a final concentration of 0.2 mmol.Math.L.sup.−1). The plate was cultured at a temperature of 30° C. with shaking for 5 h, and then centrifuged at 4° C. and 4000 r.Math.min.sup.−1 for 10 min. The supernatant was discarded, and the plate was frozen at −80° C. for more than 1 h, and then 200 μL of a lysis buffer (pH 7.5, 10 mmol.Math.L.sup.−1 Tris-HCl, 750 mg.Math.L.sup.−1 lysozyme, and 10 mg.Math.L.sup.−1 DNase) was added to each well. The plate was cultured at 37° C. with shaking at 120 r.Math.min.sup.−1 for 1 h.

(39) The plate was centrifuged and the supernatant was taken to determine the specific activity of the KpADH mutants for 1,4-butanediol. The alcohol dehydrogenase mutants with improved specific activity were selected and verified by sequencing, thereby obtaining recombinant bacteria containing recombinant plasmids that successfully overexpressed alcohol dehydrogenase mutants M1-M3 (the results of full plasmid PCR nucleic acid electrophoresis of M1-M3 are shown in FIG. 1).

(40) M4 and M5 can be directly obtained by site-directed mutagenesis of the 127th position of M1 by using the full-plasmid PCR method using the recombinant plasmid comprising M1 as a template (see FIG. 1).

Embodiment 3: Expression and Purification of Alcohol Dehydrogenase Mutants M1 to M5

(41) 1. Expression

(42) Specifically, the steps are as follows:

(43) The recombinant bacteria harboring the recombinant plasmids obtained in Embodiment 1 were inoculated into a LB medium containing kanamycin sulfate (50 μg/mL) at a inoculation amount of 2% to culture with shaking at 37° C. and 200 r.Math.min.sup.−1. When the absorbance OD.sub.600 of the culture solution reached 0.8, 0.2 mM isopropyl-β-D-thiogalactopyranoside (IPTG) was added for induction at 25° C. for 8 h, which was followed by centrifugation at 8000 r.Math.min.sup.−1 for 10 min, thereby obtaining recombinant bacterial strains expressing alcohol dehydrogenase mutants M1-M5. The collected bacterial strains were suspended in a potassium phosphate buffer solution (100 mM, pH 7.0) and ultrasonicated to obtain alcohol dehydrogenase mutants M1-M5.

(44) 2. Purification

(45) The purification was conducted using a nickel affinity column HisTrap FF crude by affinity chromatography using the histidine tag on the recombinant protein. The specific steps are as follows:

(46) First, the nickel column was equilibrated with solution A, and loaded with the crude enzyme solution. Further, solution A was used to elute the breakthrough peak. After equilibration, gradient elution was performed using solution B (20 mM sodium phosphate, 500 mM NaCl, 500 mM imidazole, pH 7.4) to elute the recombinant protein bound to the nickel column to obtain purified alcohol dehydrogenase mutants M1 to M5. After purification, the alcohol dehydrogenase protein was concentrated and displaced using a 10 kDa ultrafiltration tube into PBS (100 mM, pH 7.0) buffer for later use.

(47) The purified alcohol dehydrogenase mutants M1-M5 were tested for activity and analyzed by SDS-PAGE.

(48) Detection results: as shown in FIGS. 2 and 3 and as analyzed by SDS-PAGE, after purification on a nickel column, the alcohol dehydrogenase mutants M1 to M5 showed a single band at about 40 kDa, and there were fewer other proteins, indicating good purification effects.

Embodiment 4: Kinetic Analysis of Alcohol Dehydrogenase Mutants M1-M5 for the Smart Co-Substrate 1,4-Butanediol

(49) The activity of KpADH under different substrate concentrations and cofactor concentrations was measured, and a double reciprocal plot was made according to the reciprocals of the activity and substrate concentration. The kinetic parameters were calculated. The results are shown in Table 1.

(50) As can be seen from Table 1, the mutant M1 plays an important role in the oxidation of 1,4-butanediol. Its k.sub.cat value was 75.9 min.sup.−1, which was 7.3 times that of wild-type KpADH, and its k.sub.cat/K.sub.m value was 620 min.sup.−1.Math.M.sup.−1, which was 4.53 times that of wild-type KpADH; the K.sub.m values of M2 and M3 for 1,4-butanediol were 38.1 mM and 12.1 mM, respectively, and their catalytic rates k.sub.cat were 27.8 mM and 16.8 mM, respectively. As can be seen, the Y127 site significantly reduced the K.sub.m value, which plays a positive role in binding of the substrate 1,4-butanediol; the mutant M5 had the highest k.sub.cat/K.sub.m value of 2009 min.sup.−1.Math.M.sup.−1, which was 14.7 times of that of the wild-type KpADH.

(51) TABLE-US-00002 TABLE 1 Kinetic parameters of KpADH mutants toward 1,4-butanediol embedded image Variant K.sub.M[mM] k.sub.cat[min.sup.−1] k.sub.cat/K.sub.M[min.sup.−1•M.sup.−1] KpADH 75.6 ± 0.4 10.4 ± 0.4 137 M1 122 ± 2.1 75.9 ± 1.3 620 M2 38.1 ± 1.9 27.8 ± 0.5 729 M3 12.1 ± 0.9 16.8 ± 1.1 1390 M4 30.4 ± 1.3 39.1 ± 0.4 1286 M5 11.3 ± 0.8 22.7 ± 1.1 2009

Embodiment 5: Kinetic Analysis of the KpADH Mutants M1-M5 Towards Alcohol Co-Substrates 1,5-Pentanediol and 1,6-Hexanediol

(52) The activity of KpADH under different substrate concentrations and cofactor concentrations was measured, and a double reciprocal plots were made according to the reciprocals of the activity and substrate concentration. The kinetic parameters were calculated. The results are shown in Table 2.

(53) It can be seen from Table 2 that better catalytic efficiency was achieved for these two diol substrates with longer carbon chains as compared with 1,4-butanediol. Among others, the K.sub.m values of the mutant M1 for 1,5-pentanediol and 1,6-hexanediol were 42.5 mM and 12.3 mM, respectively, and their k.sub.cat values were 51.1 min.sup.−1 and 64.7 min.sup.−1, respectively, indicating that both the binding capacity and catalytic rate of M1 for these two diol substrates are improved;

(54) The K.sub.m value of mutant M3 for 1,5-pentanediol was as low as 14.3 mM, compared to 74.4 mM in the case of wild-type KpADH, and its K.sub.m value for 1,6-hexanediol was as low as 6.48 mM, compared to 18.5 mM in the case of wild-type KpADH. This is mainly due to the improvement in substrate affinity;

(55) The catalytic efficiency k.sub.cat/K.sub.m of M3 for 1,5-pentanediol and 1,6-hexanediol was 4.36 and 2.69 times that of wild-type KpADH, respectively;

(56) The K.sub.m values of double mutant M5 for 1,5-pentanediol and 1,6-hexanediol were 8.21 mM and 6.52 mM respectively, which were far lower than those of wild-type KpADH (74.4 mM and 18.5 mM), and their catalytic efficiency k.sub.cat/K.sub.m was 2353 min.sup.−1.Math.M.sup.−1 and 12032 min.sup.−1.Math.M.sup.−1, which is 3.14 and 5.3 times the wild-type KpADH respectively. This indicates that the double mutant M5 is a promising mutant for catalytic oxidation of diol substrates to regenerate NADPH.

(57) TABLE-US-00003 TABLE 2 Kinetic parameters of alcohol dehydrogenase mutants toward 1,5-pentanediol and 1,6- hexanediol embedded image k.sub.cat/K.sub.M k.sub.cat/K.sub.M Variant K.sub.M[mM] k.sub.cat[min.sup.−1] [min.sup.−1•M.sup.−1] K.sub.M[mM] k.sub.cat[min.sup.−1] [min.sup.−1•M.sup.−1] KpADH 74.4 ± 2.2 55.7 ± 1.0 749 18.5 ± 1.5 41.9 ± 0.9 2269 M1 42.5 ± 1.5 51.1 ± 0.8 1202 12.3 ± 0.7 64.7 ± 1.7 5252 M2 63.5 ± 0.1 25.1 ± 0.9 396 31.8 ± 1.7 36.2 ± 2.2 1138 M3 14.3 ± 0.9 46.6 ± 1.7 3269 6.48 ± 0.45 39.5 ± 1.9 6093 M4 16.3 ± 0.8 24.8 ± 1.1 1521 12.9 ± 1.3 98.3 ± 2.5 7630 M5 8.21 ± 0.22 19.3 ± 0.9 2353 6.52 ± 1.0 75.2 ± 2.1 12032

Embodiment 6: Production of Sodium D-Phenylalanine from Sodium Phenylpyruvate as Catalyzed by Alcohol Dehydrogenase Mutants M1, M2, M5 Coupled to Amino Acid Dehydrogenase DAADH.SUB.D94A

(58) The amino acid dehydrogenase DAADH.sub.D94A derived from Ureibacillus thermosphaericus can catalyze the production of D-phenylalanine, which is an important chiral component of drug nateglinide for the treatment of type 2 diabetes, from the substrate sodium phenylpyruvate. However, the catalytic reaction requires the addition of expensive cofactor NADPH.

(59) The alcohol dehydrogenase mutants M1, M2, and M5 obtained in Embodiment 3 were used to regenerate NADPH to construct an enzyme-coupled cofactor regeneration reaction to produce sodium D-phenylalanine below. The specific steps are as follows:

(60) Establishment of a 50 mM biocatalytic system of substrate sodium phenylpyruvate: alcohol dehydrogenase mutant M1, M2, M5 or wild-type KpADH pure enzyme (protein concentration 1.5 kU/L) or glucose dehydrogenase GDH (1.5 kU/L), DAADH.sub.D94A (5 kU/L), substrate sodium phenylpyruvate (50 mM), co-substrate 1,4-butanediol (50 mM), and (NH.sub.4).sub.2SO.sub.4 (100 mM);

(61) The biocatalytic system reacted at 30° C. and 180 r.Math.min.sup.−1, and was sampled over time to detect the yield of sodium D-phenylalanine in the reaction. The results are shown in Table 3.

(62) It can be seen from Table 3 that 4 h after the reaction began, for wild-type KpADH, the yield of the product was only 46.4%, while the yields of sodium D-phenylalanine in NADPH regeneration reaction of mutants M1 and M2 were increased to 88.0% and 89.0%, respectively, and for mutant M5, the yield of sodium D-phenylalanine was 99.9% in 4 h, with an e.e. value of >99.9%.

(63) TABLE-US-00004 TABLE 3 Preparation of sodium D-phenylalanine by enzyme-coupled cofactor regeneration reaction Reaction Conversion rate (%) time (h) WT GDH M1 M2 M5 0.5 5.1 67.0 36.4 43.5 88.3 1 11.5 72.1 71.6 77.6 96.1 1.5 17.9 72.4 80.8 78.4 97.9 2 24.8 74.3 85.4 82.4 98.2 3 39.3 74.4 87.0 88.3 99.7 4 46.4 74.4 88.0 89.0 99.9

Embodiment 7: Production of Sodium D-Phenylalanine from Sodium Phenylpyruvate as Catalyzed by Alcohol Dehydrogenase Mutant M5-Coupled to Amino Acid Dehydrogenase DAADH.SUB.D94A

(64) The optimal alcohol dehydrogenase mutant M5 as determined in Embodiment 6 was used to regenerate NADPH to construct an enzyme-coupled cofactor regeneration system, and the amount of co-substrate 1,4-butanediol was reduced to 0.5 equivalent. Specifically, the steps are as follows (the reaction of the regeneration system is shown in FIG. 4):

(65) Establishment of a 100 mM biocatalytic system A of substrate sodium phenylpyruvate: alcohol dehydrogenase mutant M5 (1.5 kU/L), DAADH.sub.D94A (5 kU/L), substrate sodium phenylpyruvate (100 mM), co-substrate 1,4-butanediol (50 mM), and (NH.sub.4).sub.2SO.sub.4 (200 mM);

(66) Establishment of a 200 mM biocatalytic system B of substrate sodium phenylpyruvate: alcohol dehydrogenase mutant M5 (protein concentration 10 mg/mL), DAADH.sub.D94A (5 kU/L), substrate sodium phenylpyruvate (200 mM), co-substrate 1,4-butanediol (100 mM), and (NH.sub.4).sub.2SO.sub.4 (200 mM);

(67) Both the biocatalytic systems A and B reacted at 30° C. and 180 r.Math.min.sup.−1, and were sampled over time to determine the yield of sodium D-phenylalanine and co-product γ-butyrolactone. The results are shown in Table 4.

(68) It can be seen from Table 4 that in the reaction of 100 mM substrate, the yield of sodium D-phenylalanine reached 99.8% in 2 h, and the yield of γ-butyrolactone reached 90.6% in 1 h; when the addition amount of substrate sodium phenylpyruvate was further increased to 200 mM and the addition amount of co-substrate 1,4-butanediol was increased to 100 mM accordingly, the yield of the product D-phenylalanine sodium reached 99.2% in 6 h, and the yield of the co-product γ-butyrolactone reached 90.3% (see FIG. 5 for the chiral chromatogram of the product sodium D-phenylalanine and FIG. 6 for the gas chromatogram of the co-product γ-butyrolactone).

(69) TABLE-US-00005 TABLE 4 Detection of D-phenylalanine in coupling reaction using M5 for regeneration of NADPH Reaction D-phenylalanine yield (%) time (h) 100 mM 200 mM 0 0 0 0.5 67.6 26.1 1 98.5 41.1 1.5 98.8 60.6 2 99.8 77.6 3 99.9 95.0 4 99.9 98.5 6 99.9 99.2

(70) TABLE-US-00006 TABLE 5 Detection of γ-butyrolactone in coupling reaction using M5 for regeneration of NADPH Reaction γ-butyrolactone yield (%) time (h) 100 mM 200 mM 0 0 0 0.5 62.6 26.8 1 90.6 45.6 1.5 88.7 65.9 2 85.9 80.0 3 84.9 85.6 4 85.7 87.1 6 84.6 90.3

Alcohol dehydrogenase mutant and application thereof in cofactor regeneration

Assignee

Inventors

Cpc classification

Classification Explorer

C12N9/0006

CHEMISTRY; METALLURGY

Classification Explorer

C12Y101/01001

CHEMISTRY; METALLURGY

Classification Explorer

C12P13/222

CHEMISTRY; METALLURGY

International classification

Classification Explorer

C12N9/04

CHEMISTRY; METALLURGY

Classification Explorer

C12P13/22

CHEMISTRY; METALLURGY

Abstract

Claims

Description