CN105200021A - High-activity Bacillus pumilus CotA laccase modified with site-directed mutagenesis - Google Patents

High-activity Bacillus pumilus CotA laccase modified with site-directed mutagenesis Download PDF

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Publication number
CN105200021A
CN105200021A CN201510718946.6A CN201510718946A CN105200021A CN 105200021 A CN105200021 A CN 105200021A CN 201510718946 A CN201510718946 A CN 201510718946A CN 105200021 A CN105200021 A CN 105200021A
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mutant
laccase
cota
bacillus pumilus
cota laccase
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管政兵
陈宇
廖祥儒
罗权
张宁
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Jiangnan University
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Jiangnan University
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    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N9/00Enzymes; Proenzymes; Compositions thereof; Processes for preparing, activating, inhibiting, separating or purifying enzymes
    • C12N9/0004Oxidoreductases (1.)
    • C12N9/0055Oxidoreductases (1.) acting on diphenols and related substances as donors (1.10)
    • C12N9/0057Oxidoreductases (1.) acting on diphenols and related substances as donors (1.10) with oxygen as acceptor (1.10.3)
    • C12N9/0061Laccase (1.10.3.2)
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12YENZYMES
    • C12Y110/00Oxidoreductases acting on diphenols and related substances as donors (1.10)
    • C12Y110/03Oxidoreductases acting on diphenols and related substances as donors (1.10) with an oxygen as acceptor (1.10.3)
    • C12Y110/03002Laccase (1.10.3.2)

Abstract

The invention discloses a Bacillus pumilus CotA laccase mutant with improved catalytic performance and belongs to the field of genetic engineering and enzyme engineering. A composite mutant L386W/G417L CotA laccase gene constructed in the early stage in a laboratory is taken as a template, Asp at the 195th site of the composite mutant is mutated to Trp, Phe, Try and Ile respectively, then a wild type CotA laccase is taken as a control, and the composite mutant L386W/G417L/D195Y is discovered to have higher catalytic activity and specificity on the substrate ABTS (diammonium 2,2'-azino-bis(3-ethylbenzothiazoline-6-sulfonate)), and the industrial application prospect of the Bacillus pumilus CotA laccase is promoted.

Description

A kind of Fixedpoint mutation modified high reactivity bacillus pumilus CotA laccase
Technical field
The present invention relates to the bacillus pumilus CotA Laccase mutant that a kind of catalytic efficiency improves, belong to genetically engineered and enzyme engineering field.
Background technology
Laccase (laccase, E.C.1.10.3.2) is a kind of cupric polyphenoloxidase, can the redox reaction of phenol substance catalytic, plays a significant role in the biological degradation of xylogen and precursor analogue thereof.The oxidation substrates of laccase is very extensive, and comprise phenols and derivative, arylamine and derivative thereof, aromatic carboxylic acid and derivative thereof etc., therefore laccase application potential is huge.In wood processing field, laccase can replace chemical glue mixture, not only can improve the quality of products, and can alleviate the injury to HUMAN HEALTH and the pollution to environment; In paper industry, laccase is used for paper bio-bleaching and slurrying, can reduce the pollution of pulp and paper making, contribute to paper-making industry and finally realize cleaner production; At food processing field, laccase can be used for removing the muddiness that in fruit juice, phenolic compound causes, thus improves the quality of fruit juice.In addition, laccase is oxidable chlorophenol and derivative thereof also, reduces its toxicity, and reducing with chlorophenols is the environmental pollution that dyestuff produced by industrial raw material, sanitas, weedicide, agrochemical Chemicals cause.
Laccase by sources difference can be divided into three major types: plant laccase, fungal laccase and bacterial laccase.Bacterial laccase comprises the EpoA albumen etc. of the CotA albumen of Bacillus, the PpoA albumen of extra large Zymomonas mobilis, colibacillary CueO albumen, streptomyces griseus, with fungi and plant laccase protein structural similitude, all has 4 cupric ion binding sites.
This laboratory has in earlier stage been cloned and has been recombinated and have expressed CotA laccase from the bacillus pumilus bacterial strain W3 (BacilluspumilusW3) from row filter, research finds that this CotA laccase possesses following advantage relative to other kind laccase: high, the high temperature resistant and Heat stability is good of enzymic activity under alkaline pH, can tolerate high levels of organic solvents and halide-ions environment etc., and these good characteristics just current laccase carry out in treatment of dyeing wastewater field that industrial applications is badly in need of.But the natural expression amount of wild bacillus pumilus CotA laccase is very low, and Substratspezifitaet is poor, and catalytic activity is on the low side, becomes the bottleneck of industrial applications.Therefore the present invention utilizes genetically engineered and enzyme engineering means, improves the catalytic activity of bacillus pumilus CotA laccase, improves its industrial applications prospect further.
Summary of the invention
The invention provides a kind of bacillus pumilus Laccase mutant, this mutant has transformed the double-mutant L386W/G417L laccase gene of acquisition for template with this laboratory early stage, further by the 195th of double-mutant the aspartic acid (Asp, D) tryptophane (Trp is sported respectively, W), phenylalanine (Phe, F), tyrosine (Tyr, Y), Isoleucine (Ile, I), subsequently with wild-type CotA laccase for contrast, finally select substrate 2, 2-joins nitrogen-two (3-ethyl-benzothiazole-6-sulfonic acid) di-ammonium salts (ABTS) and has higher narrow spectrum mutant.
B.pumilusCotA laccase consensus amino acid sequence (being submitted to by this laboratory, GenBank accession number: KF040050) in the parent amino acid sequence of described B.pumilusCotA laccase and ncbi database.
Described mutant is that the Asp of the 195th in complex mutation body L386W/G417L/G57F laccase gene has been mutated into Trp, Phe, Tyr, Ile respectively, called after L386W/G417L/D195W, L386W/G417L/D195F, L386W/G417L/D195Y, L386W/G417L/D195I respectively.
Accompanying drawing explanation
Fig. 1: wild bacillus pumilus CotA laccase three-dimensional simulation structure
Fig. 2: the molecule manipulation principle schematic building mutant plasmid process
Embodiment
Term used in the present invention, unless otherwise specified, generally has the implication that those of ordinary skill in the art understand usually.
Below in conjunction with concrete preparation embodiment and Application Example, and comparable data describes the present invention in further detail.Should be understood that these embodiments just in order to demonstrate the invention, but not limit the scope of the invention by any way.
Below in an example, the various process do not described in detail and method are ordinary methods as known in the art.
The expression and purification of embodiment 1 wild bacillus pumilus CotA laccase.
From glycerine pipe preseed stage build recombinant strains CotA/pColdII/BL21 (DE3) in LB liquid nutrient medium (containing 100mg/L penbritin) incubated overnight, by 2% inoculum size, seed is accessed LB liquid fermentation medium (containing 100mg/L).After intestinal bacteria cultivate 2h at 37 DEG C, the IPTG adding 0.3mM final concentration induces, and after 15 DEG C of shaking tables continue fermentation culture 26h, by fermented liquid in 4 DEG C, 8000rpm centrifugal 10min removal supernatant, collects thalline.By resuspended for the thalline phosphate buffered saline buffer collected, bacterial cell disruption is discharged intracellular protein by resuspended rear ultrasonic cell disruption instrument, after fragmentation completes, by the liquid of fragmentation in 4 DEG C, 8000rpm centrifugal 10min collection supernatant.The supernatant collected is used for CotA laccase protein purifying.
Because recombinant expressed CotA laccase protein is with polyhistidine label (His 6.tag), nickel ion affinity chromatograph method separate targets albumen is therefore used.Nickel ion affinity chromatograph purification step: (1) balances: balance HisTrapHP nickel ion post (1mL) with the 20mM damping fluid (imidazoles containing 5mM) of 10 times of column volumes; (2) loading: the sample of anticipating is with the flow velocity loading of 1mL/min; (3) wash-out: carry out gradient elution with high density imidazoles, the pipe number that under collection elution requirement, peak type is corresponding, and do Enzyme activity assay.The wild-type CotA laccase that final acquisition purifying is good.
Embodiment 2CotA Laccase mutant builds and prepares
(1) rite-directed mutagenesis
The B.pumilusCotA laccase gene sequence of the double-mutant L386W/G417L successfully constructed with early stage is for template, by the aspartic acid (Asp of the 195th in laccase, D) tryptophane (Trp is sported respectively, W), phenylalanine (Phe, F), tyrosine (Tyr, Y), Isoleucine (Ile, I), called after L386W/G417L/D195W, L386W/G417L/D195F, L386W/G417L/D195Y, L386W/G417L/D195I.
The rite-directed mutagenesis primer introducing D195W sudden change is:
Forward primer 5 '-CCTTTAATGATCATG tGGcGGACATTCCAG-3 ' (underscore is mutational site)
Reverse primer 5 '- cCAcATGATCATTAAAGGGATATCATATTC-3 ' (underscore is mutational site)
The rite-directed mutagenesis primer introducing D195F sudden change is:
Forward primer 5 '-CCTTTAATGATCATG tTcCGGACATTCCAG-3 ' (underscore is mutational site)
Reverse primer 5 '- aAcATGATCATTAAAGGGATATCATATTCA-3 ' (underscore is mutational site)
The rite-directed mutagenesis primer introducing D195Y sudden change is:
Forward primer 5 '-CCTTTAATGATCATG taCCGGACATTCCAG-3 ' (underscore is mutational site)
Reverse primer 5 '- acATGATCATTAAAGGGATATCATATTCAT-3 ' (underscore is mutational site)
The rite-directed mutagenesis primer introducing D195I sudden change is:
Forward primer 5 '-CCTTTAATGATCATG aTcGGACATTCCAG-3 ' (underscore is mutational site)
Reverse primer 5 '- aTcATGATCATTAAAGGGATATCATATTCA-3 ' (underscore is mutational site)
Utilize above-mentioned primer, with double-mutant plasmid pColdII-CotA (WL) for template, carry out PCR reaction.Reaction is all carried out in 50 μ L systems, and reaction conditions is: 95 DEG C of denaturation 3min, carries out 25 circulations (95 DEG C of 20s, 57 DEG C of 20s, 72 DEG C of 6min) subsequently, circulates latter 72 DEG C and extends 7min, last 4 DEG C of insulations.Get 10 μ LPCR products to detect through 1% agarose gel electrophoresis.Add 1 μ LDMT enzyme after object product having been detected in remaining PCR primer, mixing, hatches 1 hour for 37 DEG C.All be separated hatching the product after process, cut glue through 1% agarose gel electrophoresis, reclaim test kit with gel and reclaim object fragment.The object fragment reclaimed is transformed into DMT competent cell after mutant fragments assembling, the LB that converted product is coated containing 100mg/L penbritin is dull and stereotyped, through 37 DEG C of incubated overnight, choose 10 single bacterium colonies from flat board and carry out bacterium colony PCR checking, 3 single bacterium colony access LB liquid nutrient mediums are chosen from the bacterium colony be proved to be successful, be saved in two glycerine pipes by each bacterium liquid after 10h, a-20 DEG C of preservations, a being used for checks order.The correct mutant of order-checking is inoculated into incubated overnight LB liquid nutrient medium from glycerine pipe, after spending the night, first preserves glycerine pipe, then will remain bacterium liquid extracting plasmid and transform access BL21 (DE3) competent cell.
(2) expression and purification of mutant enzyme
Mutant Expression and purification process as described in Example 1.
Embodiment 3CotA Laccase mutant enzyme is lived and is analyzed.
(1) enzyme unit definition alive
When adopting ABTS method to measure laccase activity, enzyme amount required when definition per minute transforms 1 μm of ol substrate is as a unit of activity.
(2) enzyme activity determination step
Preheating: get the citrate buffer solution of 2.4mLpH4.0 in test tube, adds 0.5mLABTS solution (final concentration of ABTS is 0.5mM) and is placed in 37 DEG C of water-bath preheating 2min in test tube.
Reaction: add 0.1mL sample enzyme liquid, concussion evenly.
Measure: uniform for concussion sample spectrophotometer is carried out kinetic measurement, under 420nm wavelength, measure the variable quantity (speed of reaction is at the uniform velocity reaction) of OD value p.s. in 30s and calculate enzyme activity.
Embodiment 4 laccase Determination of Kinetic Parameters
The kinetic parameter of pure enzyme is measured using the ABTS of different concns as substrate.In the reaction system of 3mL, the final concentration scope of ABTS is 5-500 μM.The reaction system of 3mL comprises 2mL citrate buffer solution (0.1M; PH4.0), the ABTS solution (being diluted to 0.9mL with deionized water get the ABTS mother liquor of respective volume according to final concentration after) of the pure enzyme liquid of 0.1mL, 0.9mL.Reaction system is placed in 37 DEG C of water-baths reaction a moment, under 420nm wavelength, measures the variable quantity (speed of reaction is at the uniform velocity reaction) of OD value p.s. in 30s.Live according to enzyme activity formulae discovery enzyme.With mapping, draws a straight line.The slope of straight line is with the intersection point of the longitudinal axis with the intersection point of transverse axis kinetic parameter V can be obtained like this maxand K m, after measuring protein content, just can obtain k cat.
Enzyme activity formula: enzyme activity
In formula: the changing value V of Δ OD-absorbancy OD alwaysthe volume of-reaction system
The n-enzyme liquid extension rate Δ t-reaction times
V 0the molar absorptivity of the volume ε-substrate of-enzyme liquid
The catalytic activity analysis of embodiment 5 Laccase mutant
Take ABTS as the kinetic parameter V that substrate determines wild-type and mutant laccase max, K m, k cat, k cat/ K m.
The kinetic parameter of table 1 wild-type (WT) and mutant laccase
K mvalue can judge specificity and the natural substrate of enzyme, the maximum K of avidity of enzyme during suitable substrate mminimum.
In certain enzyme concn, enzyme is to the V of specific substrates maxalso be a constant.
K catrepresent the molecule number of each enzyme molecule conversion p.s. substrate when enzyme is saturated by substrate, this constant is commonly referred to as catalytic constant, and the catalytic efficiency of its value larger expression enzyme is higher.
K cat/ K mthe apparent secondary rate constant that enzyme and substrate reactions are formed, sometimes also referred to as specificity constant.
Can calculate from table 1, mutant is compared with wild-type laccase, and the catalytic efficiency of L386W/G417L/D195Y and specificity have maximum raising.The catalytic efficiency of mutant L386W/G417L/D195Y is 2.3 times of wild-type, and ABTS Substratspezifitaet is 3.7 times of wild-type.
Although the present invention with preferred embodiment openly as above; but it is also not used to limit the present invention, any person skilled in the art, without departing from the spirit and scope of the present invention; all can do various changes and modification, what therefore protection scope of the present invention should define with claims is as the criterion.

Claims (4)

1. a mutant for bacillus pumilus CotA laccase, is characterized in that, is for its Asp of the 195th is sported Trp, Phe, Try, Ile by template respectively with the bacillus pumilus CotA laccase gene of the two sudden change of L386W/G417L.
2. the preparation method of mutant according to claim 1, comprises the steps:
(1) with early stage build double-mutant plasmid pColdII-CotA (WL) for template, adopt the method for rolling ring PCR, in introducing mutational site, overlapping region during design primer, pcr amplification plasmid pColdII-CotA (WL) is utilized to obtain the open loop recombinant vectors of the gene order containing coding CotA Laccase mutant;
(2) in PCR primer, add DMT enzymic digestion PCR primer, then carry out 1% agarose gel electrophoresis and reclaim fragment;
(3) utilize special recombinase and homologous recombination principle, by seamless spliced for open loop recombinant vectors, form ring texture;
(4) be transformed into by cyclic plasmid in DMT competent cell, slat chain conveyor picking list bacterium colony checks order, in order that extract correct mutant plasmid;
(5) by correct recombinant plasmid transformed e. coli bl21 (DE3), abduction delivering.
3. the method according to right 2, is characterized in that, also comprises further and uses AVANT protein purification instrument and HisTrapHP1mL nickel post, desalting column, anion-exchange column to carry out purifying to laccase.
4. the method according to right 2, is characterized in that, recombinant bacterium step (5) obtained 37 DEG C of liquid culture in the LB substratum containing penbritin are spent the night, and the LB fermentation broth 37 DEG C that rear access contains penbritin is cultured to OD 600≈ 0.5, be cooled to rapidly 15 DEG C and leave standstill at least 30min, the inductor IPTG adding ultimate density 0.3mM induces, and during 26h, centrifugal acquisition precipitation, resuspended with damping fluid, is crude enzyme liquid.Complex mutation body L386W/G417L/D195Y joins nitrogen-two (3-ethyl-benzothiazole-6-sulfonic acid) di-ammonium salts (ABTS) to substrate 2,2-and has higher catalytic activity, be 2.3 times of wild-type, and specificity is 3.7 times of wild-type.
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Cited By (5)

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Publication number Priority date Publication date Assignee Title
CN107034199A (en) * 2017-06-12 2017-08-11 江南大学 The bacillus pumilus CotA Laccase mutants that a kind of Fixedpoint mutation modified stability and activity are improved
CN107034200A (en) * 2017-06-12 2017-08-11 江南大学 The bacillus pumilus CotA laccase complex mutation bodies that a kind of amount of soluble expression is improved
CN107227302A (en) * 2017-06-12 2017-10-03 江南大学 The bacillus pumilus CotA Laccase mutants that a kind of amount of soluble expression is improved
CN109294936A (en) * 2018-10-29 2019-02-01 江南大学 A kind of heterologous recombination Pichia yeast engineering GS115-pPIC9K-LacGWLF and its application
CN112921043A (en) * 2021-03-16 2021-06-08 安徽大学 Mutant nucleic acid, expression vector, laccase mutant with high specific activity and preparation method thereof

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CN104087560A (en) * 2013-12-05 2014-10-08 安徽大学 Bacterial laccase mutant protein, recombinant expression plasmid, transformed engineered strain and fermentation preparation method thereof
CN104726436A (en) * 2015-03-18 2015-06-24 江南大学 Higher-substrate-specificity keratinase mutant and preparation method thereof

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Cited By (6)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN107034199A (en) * 2017-06-12 2017-08-11 江南大学 The bacillus pumilus CotA Laccase mutants that a kind of Fixedpoint mutation modified stability and activity are improved
CN107034200A (en) * 2017-06-12 2017-08-11 江南大学 The bacillus pumilus CotA laccase complex mutation bodies that a kind of amount of soluble expression is improved
CN107227302A (en) * 2017-06-12 2017-10-03 江南大学 The bacillus pumilus CotA Laccase mutants that a kind of amount of soluble expression is improved
CN109294936A (en) * 2018-10-29 2019-02-01 江南大学 A kind of heterologous recombination Pichia yeast engineering GS115-pPIC9K-LacGWLF and its application
CN112921043A (en) * 2021-03-16 2021-06-08 安徽大学 Mutant nucleic acid, expression vector, laccase mutant with high specific activity and preparation method thereof
CN112921043B (en) * 2021-03-16 2022-06-14 安徽大学 Mutant nucleic acid, expression vector, laccase mutant with high specific activity and preparation method thereof

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