Formate Dehydrogenase Mutant with Improved Enzyme Activity and Stability and Construction Method thereof

Information

  • Patent Application
  • 20190161741
  • Publication Number
    20190161741
  • Date Filed
    November 14, 2016
    8 years ago
  • Date Published
    May 30, 2019
    5 years ago
Abstract
The present invention discloses a formate dehydrogenase mutant with improved enzyme activity and stability and a construction method thereof, which belongs to the technical field of genetic engineering. The mutant of the present invention is obtained by mutating alanine at a 10th site to cysteine based on the amino acid shown in SEQ ID NO. 2. The specific enzyme activity of the mutant enzyme obtained by the present invention is improved by 1.3 times compared with that before the mutation, a half-life period (t1/2) at 60° C. is increased by 6.8 times compared with that in the mutation period, the copper ion tolerance is increased by 30 times compared with that before the mutation, and when pH is 4, the stability is improved by 2.0 times, and the catalytic efficiency is increased by 1.4 times. The present invention shows that an amino acid residue at a 10th site is mutated to the cysteine which forms a correct disulfide bond with a cysteine residue at a 30th site of the natural formate dehydrogenase, so that the stability and the catalytic efficiency of the enzyme are improved, and the industrial application potential of the enzyme is improved.
Description
TECHNICAL FIELD

The disclosure herein relates to the field of genetic engineering, and more particularly relates to a formate dehydrogenase mutant with improved enzyme activity and stability and a construction method thereof.


BACKGROUND

Formate dehydrogenase (FDH, EC 1.2.1.2) catalyzes formic acid to generate carbon dioxide and generates NADH along with the reduction of NAD+. Due to various advantages that the reaction is an irreversible reaction, a substrate is cheap formic acid and a product is CO2 and the like, the formate dehydrogenase is used as a coenzyme cycling system to be usually combined with other oxidordeuctase to be used for the bioconversion production of important optical active compounds such as hydroxy acid, chiral alcohol, amino acid and the like. Wild-type FDH (CboFDH) sourced from Candida boidinii is used for regenerating NADH in the production of L-tertiary leucine, which is an example of a maximum application scale of the formate dehydrogenase in the industrialized production at present. Along with the precise parsing of a CboFDH three-dimensional structure, it is possible to reasonably design the CboFDH three-dimensional structure and precisely modify molecules.


The wild-type CboFDH has the disadvantages of low specific enzyme activity and poor operation stability, so that it is of great significance for the chiral compound biosynthesis industry to modify the CboFDH in a site-specific mutagenesis manner, improve the specific enzyme activity and stability and increase the efficiency for regenerating the coenzyme NADH by the CboFDH.


SUMMARY

In order to solve the above-mentioned problems, the present invention provides a formate dehydrogenase mutant with improved enzyme activity and stability and a preparation method thereof.


A first object of the present invention is to provide a formate dehydrogenase mutant with improved enzyme activity and stability, where an amino acid sequence of the formate dehydrogenase mutant is a sequence shown in SEQ ID NO. 1.


The amino acid sequence of the mutant is obtained by mutating the amino acid at a 10th site to cysteine from alanine based on the amino acid with the amino acid sequence shown in SEQ ID NO. 2.


A second object of the present invention is to provide a nucleotide sequence encoding the mutant.


In an embodiment of the present invention, the nucleotide sequence encoding the mutant is a sequence shown in SEQ ID NO. 3.


In an embodiment of the present invention, the nucleotide sequence is obtained by mutating a codon encoding the alanine at the 10th site into a codon encoding the cysteine on the basis of the nucleotide sequence shown in SEQ ID NO. 4.


A third object of the present invention is to provide a recombinant expression vector comprising the nucleotide sequence encoding the mutant.


A fourth object of the present invention is to provide genetically engineered bacteria expressing the formate dehydrogenase mutant.


In an embodiment of the present invention, the genetically engineered bacteria are obtained by connecting the nucleotide sequence shown in SEQ ID NO. 3 to the expression vector to obtain recombinant plasmids, and then convert the recombinant plasmids to host bacteria.


In an embodiment of the present invention, the genetically engineered bacteria are recombinant Escherichia coli genetically engineered bacteria.


In an embodiment of the present invention, the expression vector is pET28a.


In an embodiment of the present invention, the host bacteria are E. coli BL21.


In an embodiment of the present invention, a preparation method of the genetically engineered bacteria is to mutate a codon encoding alanine at the 10th site into a codon encoding cysteine on the basis of the nucleotide sequence shown in SEQ ID NO. 4 to obtain a recombinant gene, connect the recombinant gene to the expression vector to obtain recombinant plasmids, and convert the recombinant plasmids into Escherichia coli BL21 host bacteria, thus obtaining the recombinant genetically engineered bacteria.


In an embodiment of the present invention, the preparation method is specifically as follows


The nucleotide sequence shown in SEQ ID NO. 4 is adopted as a template, and FIprimer (the sequence is shown in SEQ ID NO. 5) and RIprimer (the sequence is shown in SEQ ID NO. 6) are adopted as primers to perform PCR, thus obtaining the recombinant gene A10C shown in SEQ ID NO. 3.


The recombinant gene sequence obtained in the previous step is connected into the pET28a expression vector to obtain recombinant plasmids pET28a-A10C, and the recombinant plasmids were converted into the E. coli BL21 to obtain a recombinant engineering strain named as pET28a-A10C/E. coli BL21.


A fifth object of the present invention is to provide a mutant, a nucleotide sequence encoding the mutant, a vector comprising the nucleotide sequence encoding the mutant, and an application of genetically engineered bacteria expressing the mutant.


In an embodiment of the present invention, the application comprises a step of constructing a coenzyme NADH cycling system by combining corresponding dehydrogenase.


In an embodiment of the present invention, the application can be used for regenerating NADH in the bioconversion production of important optical active compounds such as hydroxy acid, chiral alcohol, amino acid and the like.


On the basis of the natural formate dehydrogenase, the molecular structure of the formate dehydrogenase is modified through a site-specific mutagenesis biological technology, the specific enzyme activity of the pure enzyme of the mutant enzyme is improved by 1.3 times compared with that before the mutation, a half-life period (t½) at 60° C. is increased by 6.8 times compared with that in the mutation period, and the copper ion tolerance is improved by 30 times compared with that before the mutation; and meanwhile, the acid resistance of the mutant is also improved, and when the pH is 4, the stability is improved by 2.0 times. Furthermore, the affinity Km of the mutant enzyme A10C to the substrate NAD+is decreased by 1.4 times compared with that before the mutation, while the affinity Km of the mutant enzyme A10C to the formic acid is not significantly decreased compared with that before the mutation, and the catalytic efficiency (kcat/Km)NAD+ is increased by 1.4 times. The present invention shows that the cysteine obtained by mutating the amino acid residue at 10th site can form a correct disulfide bond with the original cysteine residue at 30th site of the natural formate dehydrogenase, so that the oxidation of the free cysteine is prevented from improving the resistance of the mutant enzyme to copperions (the copper ions are well-known transitional metal ions for promoting the sulfydryl oxidation), and the stability, the specific enzyme activity and the catalytic efficiency are improved. The mutant enzyme obtained by the present invention can be combined with corresponding dehydrogenase to construct the NADH coenzyme cycling system applied to the bioconversion production of optical active compounds and exquisite chemicals.







DETAILED DESCRIPTION

TV fermentation medium: 8 g·L−1 of yeast powder, 12 g·L−1 of peptone, 4.02 g·L−1 of K3PO4, 3 g·L−1 of NaCl, 2 g·L−1 of citric acid, 0.3 g·L−1 of ammonium ferric citrate, 10 g·L−1 of glycerinum, 2.5 g·L−1 of (NH)4SO4, and MgSO4.7H2O2. The pH was adjusted to 7.2.


Definition of enzyme activity: an enzyme amount required by reducing 1 μmol of NAD+ to NADH in every one minute was defined as one enzyme activity unit U. The specific enzyme activity was defined as the enzyme activity U·mg−1 of per unit protein.


Method for determining enzyme activity of formate dehydrogenase: a reaction system was 10 mmol·L−1 of potassium phosphate buffer solution with the pH being 7.5 which contains 1.67 mmol·L−1 of NAD and 167 mmol·L−1 of sodium formate. An appropriate amount of enzyme liquid was added to initiate the reaction, the reaction was performed for 1.5 minutes at 30° C., an absorbance value at 340 nm was measured every 30 s, and the data was recorded. The concentration of NADH was calculated according to the increment of the absorbance value at 340 nm of the reaction solution, the enzyme activity was calculated, and a reaction formula was as follows: NaCOOH+NAD+=CO2+NADH+Na+.


EXAMPLE 1: CONSTRUCTION OF A RECOMBINANT VECTOR COMPRISING THE FORMATE DEHYDROGENASE MUTANT

(1) Acquisition of mutant A10C: the nucleotide sequence shown in SEQ ID NO. 4 was adopted as a template, and F primer (the sequence was shown in SEQ ID NO. 5) and R primer (the sequence was shown in SEQ ID NO. 6) were adopted as primers to perform PCR, thus obtaining the recombinant gene shown in SEQ ID NO. 3.


(2) The recombinant gene and pET28a were bi-digested by utilizing EcoRI and XhoI and were ligated overnight at 16° C. by utilizing T4 DNA ligase after being purified. A ligation product was converted into E. coli BL21 competent cells in a chemical method. A conversion solution was smeared on an LB flat panel containing kanamycin (50 mg·L−1), plasmids were extracted, and the constructed recombinant plasmids were verified by virtue of double-restriction enzyme digestion and were named as pET28a-A10C. Sequencing work was carried out by Shanghai Sangon Biotech.


EXAMPLE 2: CONSTRUCTION OF RECOMBINANT Escherichia coli ENGINEERED BACTERIA PRODUCING THE FORMATE DEHYDROGENASE MUTANT

A strain comprising correct recombinant plasmids pET28a-A10C obtained in the embodiment 1 was the recombinant gene engineered bacteria pET28a-A10C/E. coli BL21 of the present invention.


EXAMPLE 3: EXPRESS FORMATE DEHYDROGENASE WITH RECOMBINANT BACTERIA pET28A-A10C/E. Coli BL21 AND ENZYME ACTIVITY DETERMINATION

The recombinant bacteria pET28a-A10C/E. coli BL21 constructed in the embodiment 2 and a reference strain pET28a-FDH/E. coli BL21 expressing non-mutated wild enzyme CboFDH (amino acid sequence was shown in SEQ ID NO.2) were separately inoculated into 10 mL of LB culture medium containing kanamycin, were oscillated at 37° C. and cultured overnight to be transferred into a TY fermentation medium at a subsequent day in an amount of 4% of the inoculation amount, and were induced for 16 hours at 24° C. with the addition of 0.5 mM of IPTG after being cultured at 37° C. for 4 h. Cells were collected by centrifuge and disrupted, and the cell supernatant (crude enzyme liquid) was used for determining the enzyme activity.


The obtained crude enzyme liquid was purified to obtain the formate dehydrogenase mutant A10C, kinetic parameters of the purified recombinant formate dehydrogenase mutant A1OC were analyzed, as shown in table 1, the affinity Km of the mutant enzyme A10C to the substrate NAD+ was decreased by 1.4 times compared with that before the mutation, while the affinity Km of the mutant enzyme A10C to the substrate formic acid was not significantly decreased compared with that before the mutation, the catalytic efficiency (kcat/Km)NAD+ was increased by 1.4 times, and the specific enzyme activity was improved by 1.3 times co pared with that before the mutation.









TABLE 1







A10C reaction kinetic parameters

















Specific




Km

(kcat/Km)
enzyme



Km NAD
formate
kcat
NAD
activity


Enzyme
(μM)
(mM)
(s−1)
(μM−1 s−1)
(U mg−1)





CboFDH
53.6 ± 3.4
7.3 ± 0.6
3.3 ± 0.3
0.06
5.6 ± 0.4


A10C
74.2 ± 2.6
8.2 ± 0.4
6.2 ± 0.5
0.08
7.4 ± 0.5









The copper ion tolerance of the obtained pure enzyme was analyzed, the enzyme activities of the wild-type CboFDH and the mutant enzyme A10C under the condition of different concentrations of copperions were detected, where the required concentration of the copper ions was 15 mM when the residual enzyme activity of the mutant enzyme was 50%, and the required concentration of the copper ions was smaller than 0.5 mM when the residual enzyme activity of the wild-type enzyme CboFDH was 50%. This showed that the tolerance of the mutant enzyme A10C to the copper ions was increased by more than 30 times.


Thermal stability analysis was carried out on the obtained pure enzyme, and the pure enzyme was hatched for different times at the temperature of 60° C., the half-life period of the mutant enzyme was 21.6 min and was increased by 6.8 times compared with the wild-type CboFDH (3.2 min).


PH stability analysis was carried out on the obtained pure enzyme, and the obtained pure enzyme was hatched for 1 h under the condition of different pH, it was discovered that the residual enzyme activity of the mutant enzyme A10C under the acid addition was higher than the wild-type enzyme CboFDH, where when the pH was 4, the residual enzyme activity of the mutant enzyme A10C was 89.2%, while the residual enzyme activity of the wild-type enzyme CboFDH was only 45.3%.

Claims
  • 1. A formate dehydrogenase mutant, wherein an amino acid sequence of the mutant is set forth in SEQ ID NO. 1.
  • 2. A nucleotide sequence encoding the mutant of claim 1.
  • 3. The nucleotide sequence according to claim 2, wherein the nucleotide sequence is set forth in SEQ ID NO. 3.
  • 4. A recombinant expression vector comprising the nucleotide sequence according to claim 2.
  • 5. A genetically engineered bacterium expressing the formate dehydrogenase mutant of claim 1.
  • 6. The genetically engineered bacterium according to claim 5, wherein the genetically engineered bacterium comprises a recombinant plasmid having the nucleotide sequence set forth in SEQ ID NO. 3 connected to an expression vector.
  • 7. The genetically engineered bacterium according to claim 5, wherein the genetically engineered bacterium is a recombinant Escherichia coli genetically engineered bacterium.
  • 8. (canceled)
  • 9. A method, wherein the method comprises expressing a formate dehydrogenase mutant with an amino acid sequence set forth in SEQ ID NO. 1, and constructing a coenzyme NADH cycling system by comprising the mutant.
  • 10. The method of claim 9, comprising using the system for NADH regeneration in a bioconversion production.
Priority Claims (1)
Number Date Country Kind
201610978442.2 Nov 2016 CN national
PCT Information
Filing Document Filing Date Country Kind
PCT/CN2016/105699 11/14/2016 WO 00