CN103710364B - Laccase gene Lac7 and expression protein and application thereof - Google Patents
Laccase gene Lac7 and expression protein and application thereof Download PDFInfo
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Abstract
The invention discloses a laccase gene Lac7 and expression protein and application thereof. The DNA sequence of the laccase gene Lac7 is shown in SEQ ID NO.1. According to the laccase gene Lac7 and the expression protein and application thereof, shown by research on the decoloration of recombinant coprinus comatus laccase through 13 kinds of dyes, the decoloration action of recombinant laccase Lac7+10AA mainly occurs in the beginning 1-2 hours of reaction, the decoloration speed is retarded along with time, the decoloration effect of pure laccase is obviously better than that of a crude laccase solution, and the decoloration ratio can be increased after HBT is added into crude laccase or pure laccase; the Lac7+10AA has a relatively good decoloration effect on remazol brilliant blue and malachite green, and the decoloration ratio can reach over 90% after the mediator HBT is added. The laccase gene Lac7 has a very good industrial application prospect and can generate relatively good economic and social effects.
Description
Technical field
Gene engineering technology field of the present invention, particularly a kind of laccase gene Lac7 and expressing protein thereof and application.
Background technology
Laccase is a kind of polyphenoloxidase of cupric, with Vitamin C oxidase and mammalian plasma copper-protein homology, all belong to blue blue multicopper oxidase family, because laccase has special catalytic performance and substrate specificity widely, it is at textile dyestuff decolouring and association with pulp bleaching, Polymer Synthesizing, environment measuring, foodstuffs industry, the aspects such as removing toxic substances and biological restoration have potential using value, therefore, the focus of enzyme technology and the research of environmental science crossing domain is in the world become at present about the heterogenous expression of laccase and the research of expression regulation thereof.
Research about edible fungus laccase gets more and more, such as, occurred the relevant report of honey mushroom, Pleurotus eryngii, Coprinus comatus, flat mushroom, mushroom, needle mushroom etc.Research now about laccase not only relates in its biological characteristics, separation and purification etc., and has been deep into molecular level and enters the genetically engineered stage.But the expression amount of multiple laccase self is very low, to the Cloned culturing of laccase gene, make its high expression restructuring laccase protein on heterologous host, be that to solve its high expression level and applied be important means, therefore someone studies the heterogenous expression of laccase always.
Laccase has multiple isozyme, the fungal laccase of different sources, at molecular weight, have certain difference to the adaptability of temperature and pH and the characteristic aspect such as tolerance, enzymatic reaction kinetics, the enzymatic property of same biogenic different isozyme also there are differences.Therefore also need constantly to further investigate laccase.
Summary of the invention
Goal of the invention: for the deficiencies in the prior art, the object of this invention is to provide a kind of laccase gene Lac7.Another object of the present invention is to provide the expressing protein of a kind of above-mentioned laccase gene Lac7.The present invention also has an object to be to provide the application of a kind of above-mentioned laccase gene Lac7.By the decolorization to 13 kinds of different dyes, for the heterogenous expression of laccase and industrial applications thereof provide theoretical foundation.
Technical scheme: in order to realize foregoing invention object, the technical solution used in the present invention is as follows:
A kind of laccase gene Lac7, its DNA sequence dna is as shown in SEQ ID NO.1.
The expressing protein of described laccase gene, its aminoacid sequence is as shown in SEQ ID NO.2.
An expression method for the expressing protein of described laccase gene, aminoacid sequence shown in described SEQ ID NO.2 is added with the expression label of 10 aminoacid sequence compositions, and described aminoacid sequence is TPFPPFNTNS; Expressed protein sequence is as shown in SEQ ID NO.3.
Described laccase gene Lac7 is to the application in the decolouring of dyestuff.
Beneficial effect: compared with prior art, laccase gene of the present invention and expressing protein thereof and application, the advantage had is: studied restructuring Coprinus comatus decolorization by 13 kinds of dyestuffs, find that the decolorization of restructuring laccase Lac7+10AA mainly occurs in 1 of reaction beginning, in 2 hours, along with the prolongation of time, decolorization rate slows down, the decolorizing effect of pure enzyme is obviously better than crude enzyme liquid, and thick enzyme or pure enzyme all can increase adding HBT rear decoloring rate.The decolorizing effect of Lac7+10AA to thunder agate azoles light blue and malachite green is relatively good, adds amboceptor HBT rear decoloring rate and all can reach more than 90%.There is good prospects for commercial application, can good economic benefit and social effect be produced.
Accompanying drawing explanation
Fig. 1 is Coprinus comatus total serum IgE agarose gel electrophoresis figure; In figure, M is Marker, and 1 is the Coprinus comatus total serum IgE extracted;
Fig. 2 is Coprinus comatus DNA agarose gel electrophoresis figure; In figure, M is Marker, and 1,2 is the Coprinus comatus DNA extracted;
Fig. 3 is the amplification figure of degenerated primers; Left figure is a position and No. two position primer PCR results, and right figure is a position and No. four position primer PCR results;
Fig. 4 is recombinant plasmid PCR Screening and Identification result figure; In figure, M is Marker, 1-8 is positive colony result;
Fig. 5 is recombinant plasmid PCR Screening and Identification result figure; In figure, M is Marker, 1-10 is positive colony result;
Fig. 6 is 5 ' RACE amplification figure; M is Marker, and No. 1 swimming lane is amplified production; D:lac75 ' RACE;
Fig. 7 is laccase 3 '-RACE amplification;
Fig. 8 is that the PCR of lac7+10AA Xba I, sac II restriction enzyme site obtains electrophorogram, and M is Marker, No. 1 result for PCR introducing restriction enzyme site;
Fig. 9 is recombinant plasmid lac7+10AA PCR Screening and Identification result figure, and M is Marker; 1-10 swimming lane is the result that the hickie selected is PCR;
Figure 10 is that recombinant plasmid extracts result electrophorogram; M:mark, 3:lac7+10AA;
Figure 11 is that the dull and stereotyped biological respinse of MM detects laccase lac7 Activity Results figure; B:lac7+10AA;
Figure 12 is the growth curve chart of restructuring laccase;
Figure 13 be copper ion concentration laccase lac7+10AA is expressed affect result figure;
Figure 14 is enzyme liquid SDS-PAGE detected result figure after separation and purification;
Figure 15 is the optimum temperuture result figure of Coprinus comatus restructuring laccase Lac7+10AA;
Figure 16 recombinates the thermal stability results figure of laccase Lac7+10AA;
Figure 17 recombinates the optimal reaction pH result figure of laccase Lac7+10AA;
Figure 18 recombinates the pH stability result figure of laccase Lac7+10AA;
Figure 19 be different time the pure enzyme of Lac7+10AA (without medium) is decoloured affect result figure;
Figure 20 is that different time affects result figure to the impact that the pure enzyme of Lac7+10AA (having medium) decolours;
Figure 21 is that restructuring Coprinus comatus laccase Lac7+10AA is to the decolouring result figure of anthraquinone dyes;
Figure 22 is that restructuring Coprinus comatus laccase Lac7+10AA is to the decolouring result figure of azo dyes;
Figure 23 is that restructuring Coprinus comatus laccase Lac7+10AA is to the decolouring result figure of triphenylmethane dye.
Embodiment
Below in conjunction with specific embodiment, the present invention is further illustrated.
Embodiment 1
(1) acquisition of shaggy mane mycelium
Strain of coprinus comatus is inoculated into PDA flat board from test tube slant, is placed in 25 DEG C of constant incubators and cultivates.It is (Coprinus comatus needs about the ten days) punching on the PDA flat board covering with mycelia of the punch tool of 1cm with sterilized diameter, choose four ferfas and put off in each sterilized 250mL triangular flask (every bottle containing 30mL liquid nutrient medium), be placed in 25 DEG C of constant incubators and cultivate.At the 10th day, add coffic acid (final concentration is 1mM) induction, within the 22nd day, collect mycelia.By mycelia filtered through gauze, then rinse twice with PBS, put into-80 DEG C of Refrigerator stores after liquid nitrogen flash freezer for subsequent use.
(2) extraction of total serum IgE
The TRIZOL reagent of Invitrogen is adopted to extract, detailed process: taken out from-80 DEG C of refrigerators by Coprinus comatus sample, liquid nitrogen grinding powdered; Get appropriate powder and add 1mL TRIZOL reagent, vibrate 6 times, each 15s, room temperature places 5min; Add 0.2mL chloroform, concussion mixes, and room temperature leaves standstill 5min; With the rotating speed 4 DEG C of centrifugal 15min being less than or equal to 12000g; Supernatant liquor is transferred to clean centrifuge tube, adds Virahol 0.25mL, and the NaAc0.25mL for several times room temperature that turns upside down leaves standstill 10min, with the centrifugal 4 DEG C of centrifugal 10min of the rotating speed being no more than 12000g; Abandon supernatant, precipitation uses 75% ethanol purge, softly blows and beats, make precipitation levitating with rifle; With the speed 4 DEG C of centrifugal 5min being less than 7500g; Abandon supernatant, add the rinsing again of 75% ethanol, centrifugation step is the same; Abandon the dry RNA of supernatant, add 20-30 μ LDEPC-H
2o dissolves ,-80 DEG C of preservations.
The RNA extracted runs agarose electrophoresis, after electrophoretic separation and ethidium bromide staining, judges the integrity of RNA according to the brightness of abundant 28S and 18S ribosome-RNA(rRNA) (rRNA) band.The RNA of thick extraction detects through the agarose gel electrophoresis of non denatured 1%, and as shown in Figure 1,18S and 28S two RNA feature bright bands appear in sample, and RNA quality is better, can follow-uply use.
(3) extraction of Coprinus comatus genomic dna
The extracting method of fungal DNA is with reference to laboratory manual: get 1g mycelia, abundant by liquid nitrogen grinding; Add 10mL DNA lysis buffer(0.1M Tris-Hcl(pH8.0), 0.05M EDTA, 0.5%SDS, 1% beta-mercaptoethanol, 65 DEG C of insulation 1h; Add equal-volume phenol: chloroform: primary isoamyl alcohol (25:24:1), 10000g, 4 DEG C, 15min; Turn the clean centrifuge tube of supernatant to, add equal-volume chloroform: primary isoamyl alcohol (24:1), 10000g, 4 DEG C, 15min; Turn supernatant liquor, add the 3M NaAc(pH5.2 of 1/3 volume), monoploid amasss Virahol; Place 1 hour for-20 DEG C, 10000g, 4 DEG C, 5min; Add 15mL75% ethanol, rinsing DNA precipitates, and room temperature places dry 30min(extremely without ethanol taste); Add 500 μ L TE buffer to dissolve, transfer to the centrifuge tube of 1.5mL; Add RNase10uL, 37 DEG C of insulation 1h; Phenol imitates extracting: 1. add 1 times of volume phenol, and room temperature places 10min, 13000rmp, 10min, gets supernatant; 2. 1/2 volume phenol+1/2 volume of chloroform, room temperature places 10min, 13000rmp, 10min, gets supernatant; 3. monoploid amasss chloroform, and room temperature places 10min, 13000rmp, 10min, gets supernatant.Alcohol settling: 1. 2 times of volume dehydrated alcohols, 1/10 volume 3M NaAc(pH5.2), place a few hours for-20 DEG C; 2. 4 DEG C, 16000rmp, centrifugal 15min, abandons supernatant; 3. add 75% ethanol rinse and precipitate 2 times, air-dry; 4. 500 μ L TE buffer dissolution precipitations are added ,-20 DEG C of preservations.
The DNA agarose gel electrophoresis extracted is identified, as shown in Figure 2, have clear band as seen at more than 5000bp, this DNA can be used as follow-up test.
(4) acquisition of Coprinus comatus laccase gene group DNA sequence dna
Most fungal laccase is monomeric protein, and generally all contain 4 copper atoms in enzyme molecule, the conserved amino acid sequence according to copper land can design degenerated primers, clone's laccase.
Amplification laccase gene fragment primer: position forward primer: 5 '-CAYTGGCAYGGNTTYTTYCA-3 '; No. two position reverse primer: 5 '-GRCTGTGGTACCAGAANGTNCC-3 '; No. four position reverse primer: 5 '-TGCCARTCDATRTGRCARTG-3 '.
Regular-PCR, adopts 25 μ L PCR system: 2 μ L25 × dNTP Mix, 1.5 μ L Mg
+(MgCl
2), 2.5 μ L10 × Advantage2PCR buffer, 15.375 μ L PCR-H
2o, 2.5 μ L template DNAs, 0.125 μ L RTaq, 0.5 μ L forward primer, 0.5 μ L reverse primer.
PCR condition: 95 DEG C (1min), 95 DEG C (30s), 55 DEG C (30s), 72 DEG C (2min); 28circles.
The recovery of object fragment, step is as follows: (1) first weighs the quality of the centrifuge tube of empty 1.5mL, weighs the weight putting into the centrifuge tube of glue subsequently.To record the weight of glue, the corresponding 1 μ L of 1mg.(2) add buffer GC 6 ~ 8min in 68 DEG C of waters bath with thermostatic control extremely to dissolve completely (period often crosses 2 minutes best shaken several times to guarantee abundant dissolving).(3) solution after dissolving is proceeded in the special centrifuge tube of purifying, 12000g, 1min.(4) solution in pipe abandon, adds 500 Μ LDNA Washing Buffer, 12000g, 1min.(5) solution in pipe abandon, idle running is once to remove alcohol residual in DNA Washing Buffer.(6) get a clean centrifuge tube, strainer is placed in centrifuge tube.(7) about 30 μ L ddH are added
2o fully dissolves, 12000g, centrifugal 1min.(8) for ensureing that object sample dissolves completely, the lysate sucking-off in test tube is also squeezed into strainer, recentrifuge again.(9) get the DNA after 5 μ L purifications, carry out identification of dna quality.
Use a position forward primer and No. two position reverse primers, a position forward primer and No. four position reverse primers, with the DNA extracted for template, PCR primer carries out agarose gel electrophoresis qualification, result as shown in Figure 3, the amplified production size of a position and No. two position primers is at about 200bp, the amplified production size of a position and No. four position primers is at about 1600bp, and this is identical with expected results, and these amplified productions available carry out follow-up test.
The connection of purified product and PCR carrier: purified product adds A(VITAMIN B4) put into PCR instrument, 70 DEG C, 30min after tail.Tailing system is: 1 μ L10 × PCR buffer(Mg
2+free), 1 μ L MgCl
2(25mM), 1 μ L dATP(50 ×), 1 μ L Taq polymerase, 7 μ L purified products.
Be connected on PCR carrier by the fragment of the above-mentioned A of adding tail, 4 DEG C of connections are spent the night.Linked system is: 1 μ L10 × ligation buffer, 2 μ L PCR2.1vector, 6 μ L add the product after A tail, 1 μ L T4DNA ligase.
Prepare competent escherichia coli cell: activation intestinal bacteria, cultivate bacterium, about 2 hours with the triangular flask (adding 250mLLB substratum) of 1L, survey OD value 0.5.Centrifugal in packing 50mL centrifuge tube, 2000g, centrifugal 6mim.Add 10mL calcium chloride (first placing in ice) to suspend, 3 pipes are 1 pipe also, is finally settled to 20mL.1200g, 6min are centrifugal.Add 10mL calcium chloride to suspend gently, in ice, place 30min.1200g, 6min are centrifugal.Add 2mL ~ 3mL calcium chloride to suspend, packing 100ul mono-manages ,-80 DEG C of preservations.
Transformation of E. coli DH5 α competent cell: 1. DH5 α competent cell (200 μ l) is taken out from-80 DEG C of refrigerators, thaw on ice.2. connection product is added in the DH5 α thawed, mix with liquid-transfering gun.3. the ice bath 30min even longer time.4. 42 DEG C of thermal shock 2min(are accurate).5. add 0.5mL LB substratum, 37 DEG C, 200rpm, shaking table cultivates 1 hour.6. because bacterium liquid is denseer, therefore do not carry out centrifugal concentrating, IPTG40 μ L and X-Gal20 μ L mixes, after thalline added to be coated with LBA dull and stereotyped.7. overnight incubation in 37 DEG C of incubators.
Blue hickie and bacterium colony PCR screening positive clone also check order: be template from coating containing picking hickie the LBA flat board of IPTG and X-Gal, with T7, M13reverse for primer program 2.2.4.2 carries out pcr amplification, screen the hickie be of convenient length, get positive strain order-checking.Two groups of PCR primer are connected with PCR carrier, proceed to E. coli competent, the LBA of coating containing IPTG and X-Gal is dull and stereotyped, and 37 DEG C of incubated overnight obtain blue hickie, according to the α-complementary principle of β-glucose Glycosylase, know that the hickie obtained is the positive colony inserting exogenous genetic fragment.Bacterium colony PCR screening is carried out to hickie, to determine the recombinant plasmid inserting exogenous genetic fragment.
Due to the about 180bp of length between M13reverse, T7 primer, so amplification fragment is out larger than Insert Fragment, as shown in Figures 4 and 5, recombinant conversion efficiency is very high for result, the some order-checkings of random each picking.Be that primer PCR filters out and amplifies the suitable thalline of fragment length with general M13reverse, T7, order-checking.Obtain Coprinus comatus genomic dna sequence fragment.
Design of primers is the important factor of RACE success.The Coprinus comatus genomic dna sequence fragment obtained according to checking order devises the gene-specific primer for the Coprinus comatus 5 ' terminal sequence that increases:
Laccase7GSP1:5’-CTCCGGAACCACCATCAGCCCAATTAG-3’;
5 ' RACE reaction system: 2.5 μ L5 ' RACE-ready cDNA, 5 μ L UPM(10 ×), 1 μ L LaccaseGSP1,41.5 μ L Master Mix(34.5 μ L PCR-H
2o, 1 μ L50 × Advantage2polymerase Mix, 5 μ L10 × Advantage2PCR buffer, 1 μ L50 × dNTP Mix).
PCR program: 94 DEG C of denaturation 5min; 94 DEG C of 30s, 65 DEG C of 30s, 72 DEG C of 3min; 34cycles; 72 DEG C of 5min.PCR primer detects through the agarose gel electrophoresis of 1.0%.
Use the SMARTTM RACE cDNA Amplification test kit of CLONTECH company, take total serum IgE as 5 '-RACE ready cDNA of Material synthesis be masterplate (method is with 3 '-RACE ready cDNA), carry primer UPM and laccase Auele Specific Primer Laccase7GSP1 with test kit to increase, electrophoresis detection result as shown in Figure 6, a specificity bright band is there is at 500bp right position in laccase gene 5 '-RACE after increasing, expanding effect is obvious ,-20 DEG C of preservations after the Universal DNA Purification Kit purifying of amplified production use TIANGEN.
The connection of the recovery purifying of object fragment, purified product and PCR carrier, recombinant plasmid transformed competent escherichia coli cell, blue hickie screening positive clone, order-checking, method is all the same.
Fragment after laccase 5 '-RACE amplification, purifying is connected with PCR2.1Vector, transform DH5 α, the LBA of coating containing IPTG and X-Gal is dull and stereotyped, and according to the α-complementary principle of β-glucose Glycosylase, the hickie obtained is probably the positive colony inserting exogenous genetic fragment.Therefore often organize random picking 10 white colonies and carry out colony PCR amplification, then identified by agarose gel electrophoresis, select the company that send of band correct position to check order.Obtain 5 '-RACE sequence fragment sequence as follows:
CTAATACGACTCACTATAGGGCAAGCAGTGGTATCAACGCAGAGTACGCGGGGGATGCCGGATTAGGTATATTTTCGTTTGTCAATGCCCGCCCAAACTTGTTGAACTCAATTACTCACCCCCAAAATTATTGCATGTCTGAATTTCACATCATCTATCTTGGCATATAAGAGCTTCTAGCCTCAAATGTGATCCTGATGTTTCATGTCTGGACGCCGTTAGTGCGTCCCTGGGGTTAATTGCGGGTTTTGGTTTGGTATTCTTTGCAGTTCCAGTTTAAAAGATCTCACTTTTCCTTTTGAATGAACACGAACACGTACCCCCCCCCCCCCAGTACCTTTCCTGTGA
CTCCATTTGCTTTCTTTTGCCTTTATAGGCGCCAATGCTTTTGCGCTTTCTGTCGGTCCACGAGCAACTCTTACATTGACGAATGACGTAGTTGCGCCTGATGGTTTTGAACGATCTGCCATTGTTGTCAACGGAGGACATCCTGGGCCACTGATTCAAGCGAACAAGGGTAATGCCTACACGATTAATGTTGTTAATCGGCTCACGGACTCCACCATGCAGAGAGTTTCTTCTATTCATTGGCATGGTCTCTCTCAGAGAGGTA
Wavy line line part is the base sequence of gene-specific primer GSP1 complementation, and dashed part is 5 '-RACE template, 5 ' Long UP+Smart II oligo held, and the ATG of dash area is laccase lac7 initiator codon.Short fragment sequence is translated into protein, uses SignalP4.0server to carry out the analysis of signal peptide, as shown in Figure 7,5 '-RACE amplified reaction arrive 5 ' to be held analytical results, and include the signal peptide of gene self, front 16 amino acid are signal peptide sequence.
(5) acquisition of laccase cDNA total length
The synthesis of 3 '-RACE Ready cDNA, operation steps: 1. add in centrifuge tube: the Coprinus comatus total serum IgE 1 μ l of extraction, 3 '-CDS primer1 μ l, Smart II oligo1 μ l, H
2o2 μ l, mixes solution, and micro-centrifugal solution aggregation that makes is bottom centrifuge tube.2. 70 DEG C of water-bath 2min.3. cooled on ice 2min, to be micro-ly centrifugally sunken to solution bottom centrifuge tube.4. following material is added in this centrifuge tube: 5 × Frist strand buffer2 μ l, DTT(20mM) 1 μ l, dNTP Mix(10mM) 1 μ l, PowerScript Reverse Transcriptase1 μ l.5. mixed by solution with rifle, micro-centrifugal solution that makes sinks to bottom centrifuge tube.6. the non-water-bath of 42 DEG C of insulation 1.5h().7. the Tricine-EDTA buffer of 100 μ l is added.8. heat 72 DEG C of 7min, sample retention is at-20 DEG C.
The design of 3 '-RACE gene-specific primer (GSP2): according to acquired 5 ' end sequence, use primer-design software Primer Premier5.0, have devised the gene-specific primer GSP2 that holds near 5 ' to obtain cDNA total length according to the annealing temperature of required primer and primer length.
Laccase7GSP2:5’-GGCGCCAATGCTTTTGCGCTTTCTGTCGG-3’;
3 '-RACE reaction system: 2.5 μ L3 ' RACE-ready cDNA, 5 μ L UPM(10 ×), 1 μ L LaccaseGSP2,41.5 μ L Master Mix(34.5 μ L PCR-H
2o, 1 μ L50 × Advantage2polymerase Mix, 5 μ L10 × Advantage2PCR buffer, 1 μ L50 × dNTP Mix).
PCR program: 94 DEG C of denaturation 5min; 94 DEG C of 30s, 65 DEG C of 30s, 72 DEG C of 3min; 34cycles; 72 DEG C of 5min.PCR primer detects through the agarose gel electrophoresis of 1.0%.
Use the SMARTTM RACE cDNA Amplification test kit of CLONTECH company, take total serum IgE as 3 '-RACE ready cDNA of Material synthesis be masterplate, after carrying primer UPM and laccase Auele Specific Primer GSP2 amplification with test kit, electrophoresis detection result, as shown in Figure 7, a specificity bright band is there is at 1500bp right position in laccase gene 3 '-RACE after increasing, expanding effect is obvious ,-20 DEG C of preservations after the Universal DNA Purification Kit purifying of amplified production use TIANGEN.
Fragment after laccase 3 '-RACE amplification, purifying is connected with PCR2.1Vector, transform DH5 α, the LBA of coating containing IPTG and X-Gal is dull and stereotyped, and according to the α-complementary principle of β-glucose Glycosylase, the hickie obtained is probably the positive colony inserting exogenous genetic fragment.Therefore often organize random picking 10 white colonies and carry out colony PCR amplification, then identified by agarose gel electrophoresis, select the company that send of band correct position to check order.
The rubber tapping Purification Kit PCR primer of TIANGEN is adopted to obtain cDNA total length, be connected on PCR carrier, transformation of E. coli competent cell DH5 α, hickie is chosen with T7 after blue hickie screening, M13Reverse is that primer is tested, choose and expand the suitable bacterium colony of fragment length, check order after enlarged culturing, obtain full length sequence 2048bp, as shown in SEQ ID NO.1, online at NCBI, through blast, above sequence is determined that they are that laccase gene fragment is errorless successively, called after laccase gene lac7, the aminoacid sequence of its expressing protein is as shown in SEQ ID NO.2.
Embodiment 2
The bacterial classification that the present embodiment uses, reagent, substratum are as follows:
Yeast KM71H(Mut
s, Arg
+) and expression vector pPicz α B(Invitrogen).PGEM-T Easy Vector system I(Promega), Plasmid Miniprep Kit(BIOMIGA), AxyPrep PCR CleanupKit(AXYGEN), EasySelectTM Pichia Expression Kit(Invitrogen), rTaqDNA Ploymerase(TakaRa), Pfu DNA Ploymerase(Promega), T4DNA Ligase(Promega, Invitrogen), Xba I(promega), sacII(Takara), Sac I(Fermentas), Amp(penbritin SIGMA), EtBr(ethidium bromide AMERSCO), dNTP(TakaRa, Promega), Seakem LE agarose(BMA), all the other reagent are conventional use reagent.
LBA solid medium: often liter of substratum adds 25g agar except same LB substratum equally adds peptone, yeast decoction, NaCl, autoclave sterilization 20min at 121 DEG C, Amp is added when substratum is cooled to 55 DEG C, make ultimate density reach 100 μ g/mL, then pour culture dish into and make flat board.
LBZ(1L): 10g Tryptone, 5g Yeast Extract, 5g NaCl, be cooled to about 60 DEG C, add 1mL ZeocinTM after autoclave sterilization.To make flat board, then add 15g Agar before sterilization.
YPD(1L): 10g Yeast Extract, 20g peptone, be dissolved in 900mL water, autoclave sterilization, adds the glucose of 10 sterilized × D(20% of 100mL), to make flat board, then 15g Agar is added before sterilization.
YPDS+ZeocinTM is dull and stereotyped: 10g Yeast Extract, 20g peptone, 182.2g Sorbitol, 20g Agar is dissolved in 900mL water, autoclave sterilization, adds the glucose of 10 sterilized × D(20% of 100mL), be cooled to about 60 DEG C, add 1mL100mg/mL ZeocinTM, be down flat plate flat board and solidify rear 4 DEG C of preservations.
BMGY:10g Yeast Extract, 20g peptone is dissolved in 700mL water, autoclave sterilization, the potassium phosphate buffer (warm autoclaving) of the 1M of 100mL pH=6 is added after cool to room temperature, the sterilizing of 100mL10 × YNB(filter membrane), 2mL500 × B(20mg biotin is dissolved in the water of 100mL, filter membrane sterilizing), 100mL10 × GY(100mL glycerine is dissolved in 900mL water autoclave sterilization), mix rear 4 DEG C of preservations.
BMMY:10g Yeast Extract, 20g peptone is dissolved in 700mL water, autoclave sterilization, add after cool to room temperature, the potassium phosphate buffer (warm autoclaving) of the 1M of 100mL pH=6, the sterilizing of 100mL10 × YNB(filter membrane), 2mL500 × B(20mg biotin is dissolved in the water of 100mL, filter membrane sterilizing), the methyl alcohol of 100mL10 × M(5%), mix rear 4 DEG C of preservations
MM flat board (1L) is (containing 0.2mM Cu
2+, 0.1mM ABTS): 0.05gABTS, 0.032gCuSO4,15g Agar is dissolved in 800mL water autoclave sterilization, adds the sterilizing of 100mL10 × YNB(filter membrane after cool to room temperature), 2mL500 × B(20mg biotin is dissolved in the water of 100mL, filter membrane sterilizing), the methyl alcohol of 100mL10 × M(5%)
Separation and purification solution: A liquid (20mM Tris-HCl, pH8.0): take Tris2.4228g, adding distil water, to 800mL, is settled to 1L, 4 DEG C storages after regulating pH to 8.0 with HCl.B liquid (containing the Tris-HCl damping fluid of 1M NaCl, pH8.0): take Tris2.4228g, NaCl58.44g, adding distil water, to 800mL, is settled to 1L, 4 DEG C storages after regulating pH to 8.0 with HCl.
Sieve chromatography buffer: NaH
2pO
4-Na
2hPO
4buffer:20mM NaH
2pO
4, 20mM NaH
2pO
4, adjust pH to 7.0.
SDS-PAGE reagent: polyacrylamide list binary: (30:0.8) takes 30g Arc, 0.8g Bis adds after 50mL distilled water fully dissolves and is settled to 100mL, 4 DEG C of storages.
5 × seperating buffer(pH8.8): 22.69g Tris base0.125mL TEMED, 0.5g SDS adjusts pH to 8.8, is settled to 100mL.
5 × stacking buffer(pH6.8): 9.85g Tris base, 0.125mL TEMED, 0.5g SDS adjust pH to 6.8, are settled to 100mL.
5 × sample buffer:0.98g Tris base, 2.0g SDS, 7.5mL glycerine, 5mL beta-mercaptoethanol adjusts pH to 6.8, is settled to 100mL.
1 × Running buffer(pH8.3Tris-Gly): 3.027g Tris base, 14.41g glycine, 1.0g SDS adjust pH to 8.3, are settled to 1L.
5% ammonium persulphate: take 0.5g AP and add water and be settled to 10mL, point is filled in 1.5mL centrifuge tube ,-20 DEG C of storages.
Destainer (Destaining solution): methyl alcohol 400mL, distilled water 500mL, Glacial acetic acid 100mL.
One, the structure of expression vector
(1) design of laccase two ends restriction enzyme site
That select is pPICZ α B, if make the laccase gene reading frame of insertion correct, must introduce the restriction enzyme site of correct restriction enzyme on laccase gene.By analysis, the restriction enzyme site of these two restriction enzymes of Xba I and sac II be introduced, design primer:
Introducing 10 aminoacid sequences is: TPFPPFNTNS;
Corresponding nucleotides sequence is classified as: ACGCCATTCCCCCCTTTCAACACCAACTCT;
Restriction enzyme site XbaI:TCTAGA, sacII:CCGCGG;
Lac7gcDNAF:5’-GCTCTAGATGACGCCATTCCCCCCTTTCAACACCAACTCTCTTTCTGTCGGTCCACGAGCA-3’;
Lac7gcDNAR:5’-GTCCCCGCGGATGTTTCACCATAGGCACAAT-3’。
The aminoacid sequence of the lac7+10AA built is as shown in SEQ ID NO.3.
(2) acquisition of the gene containing Xba I and sac II restriction enzyme site
Take recombinant plasmid as template, with Lac7gcDNAF, Lac7gcDNAF for upstream and downstream primer, use the pfu enzyme (reaction system: 5 μ L10 × pfu buffer with high-fidelity performance, 4 μ L dNTP(2.5mM), 1 μ L contains the recombinant plasmid of laccase gene, 1 μ L Primer lacgcDNAF, 1 μ L Primer lacgcDNAR, 0.5 μ L pfu DNA polymerase, 37.5 μ L PCR-H
2o), with program D553(94 DEG C of denaturation 5min, 94 DEG C of 30s, 55 DEG C of 30s, 72 DEG C of 3min, 30cycles, 72 DEG C of 10min) amplification introducing restriction enzyme site, amplified production agarose gel electrophoresis detects, and result as shown in Figure 8, all meets the requirements with the primer amplified lac7+10AA band out containing restriction enzyme site designed.
(3) double digestion laccase gene and plasmid pPICZ α B
Laccase lac7+10AA gene PCR being introduced Xba I and sac II double enzyme site uses the product purification of TIANGEN to reclaim test kit by after PCR primer purifying, Xba I and sac II double digestion (double digestion reaction system: 4 μ L10 × buffer C is used respectively with plasmid pPICZ α B, 0.4 μ L0.1%BSA, 2 μ L Xba I, 1 μ L sac II, 15 μ L goal gene, 17.6 μ L PCR-H
2o, 37 DEG C of enzymes are cut 3h and are continued follow-up test).Use the PCR clean up Kit purifying of TIANGEN to reclaim enzyme the lac7+10AA gene fragment after double digestion and expression vector pPICZ α B and cut after product, 1% agarose gel electrophoresis detects enzyme and cuts front and back, and result is correct.
(4) connection of laccase gene and pPICZ α B
Laccase lac7+10AA gene after double digestion is connected (linked system: the laccase gene fragment after 6 μ L double digestions respectively with expression vector pPICZ α B fragment, pPICZ α B after 2 μ L double digestions, 1 μ L10 × ligation buffer, 1 μ L T4DNA ligase) after, 4 DEG C are spent the night.
(5) conversion of product, screening and order-checking is connected
LBZ flat board is coated with by after the laccase recombinant plasmid pPICZ alpha B-10AA-lac7 transformation of E. coli competent cell DH5 α connected, after 37 DEG C of incubators spend the night, from plate, picking 1-10 single bacterium colony is with 3 ' AOX, and 5 ' AOX is primer (5 ' AOX:5'-GACTGGTTCCAATTGACAAGC-3'; 3 ' AOX:5'-GGCAAATGGCATTCTGACAT-3'), D553PCR increases, and the bacterium colony line conservation that screening amplified production is of convenient length, chooses 1-2 order-checking simultaneously.As shown in Figure 9, recombinant plasmid sequencing result translates into the aminoacid sequence of corresponding protein through expasy to electrophoresis result, and 5 ' part adds ten amino acid, 3 ' part has myc to mark, sequence is finally 6 Histidines, and translates smoothness completely, shows construction of recombinant plasmid success.
Two, recombinant plasmid electricity is transformed into Pichia pastoris
(1) alkaline process upgrading grain
The preparation of solution: Solution I:25mM Tris HCl(pH8.0), 10mM EDTA, 50mM Glucose.Solution II:0.2N NaOH, 1%SDS, mix 0.4NNaOH and 2%SDS before the use.Solution III(3M K+, 5M acetate): 29.4g potassium acetate+, 11.5mL glacial acetic acid, constant volume, can not heat sterilization to 100mL, room temperature preservation.Lysozyme(10mg/mL)
Operation steps: 1) inoculation is containing the DH5 α of laccase lac7+10AA gene in LBZ liquid nutrient medium, and the product getting 0.5-1mL overnight incubation is in the fresh substratum of 100mL, and 37 DEG C, 200rpm shaking table is cultivated until thalline saturated (cultivating about 20h); 2) with 50mL centrifuge tube 5000rpm, the centrifugal thalline of 10min; 3) 2mL Solution I and 100ul Lysozyme(10mg/mL is added) mix, room temperature places 5min; 4) add 4mL Solution II, vibration is until solution becomes clarification gently, places 5min on ice; 5) add 3mL Solution III, vibrate gently, room temperature places 5min; 6) the centrifugal 10min of 10000rpm; 7) supernatant liquor is transferred in a clean 50mL centrifuge tube; 8) add equal-volume Virahol to mix, place 10min or longer for-20 DEG C; 9) the centrifugal 30min of 12000rpm, removes supernatant, air-dry precipitation; 10) the TE buffer(pH8.0 of 1mL is added) dissolution precipitation, solution is proceeded in the centrifuge tube of 1.5mL; 11) RNase10ul is added, 37 DEG C of water-bath 30min; 12) phenol imitates extracting plasmid: add 1/2 volume of phenol, 1/2 volume of chloroform puts 10min, and 13000rpm is centrifugal, and 10min gets supernatant; 13) add equal-volume chloroform and put 10min, the centrifugal 10min of 13000rpm, gets supernatant; 14) add the sodium-acetate of 1/10 volume 3M, 2 times of volumes 100% ethanol place 5min on ice; 15) 4 DEG C of centrifugal 10min of 12000rpm, abandon supernatant, and the ethanol precipitated with 75% is washed; 16) 70 μ l PCR-H are added after centrifugal airing
2o, takes out 2 μ l leakage of electricity swimming, and surveys A260 calculating DNA concentration.
Utilize the alkaline process of plasmid to extract recombinant plasmid in a large number, the results are shown in Figure 10.
(2) plasmid linearization: with SacI single endonuclease digestion plasmid, make plasmid linearization.The endonuclease reaction system of SacI: 10 μ L contain the pPICZ α B of laccase lac+10AA gene, 5 μ L10 × buffer SacI, 3.5 μ L SacI restriction enzymes, 31.5 μ L PCR-H
2o.After 37 DEG C of enzymes cut 1h, detection enzyme is cut quality and is met service requirements.
(3) plasmid electricity transformed yeast competent cell, step: 1) get competent cell that 80 μ L prepare and the linearizing plasmid DNA of 5-10ug (is dissolved in 5-10 μ L PCR-H
2o), mix, the electricity they being proceeded to ice-cold 0.2cm transforms in cup; 2) electricity conversion cup and linearizing plasmid DNA place 5min on ice; 3) pulsed cell; 4) rapidly 1M sorbyl alcohol ice-cold for 1mL is added electricity and transform cup, after the thalline transformed by electricity in cup mixes, proceed in the centrifuge tube of 1.5mL; 5) centrifuge tube is incubated 1-2h at 30 DEG C, does not vibrate; 6) coated plate YPDS+ZeocinTM; 7) cultivate 2-3 days for 30 DEG C, formed to single bacterium colony; 8) choose 10-30 single bacterium colony, rule at fresh YPDS+ZeocinTM.
Three, there is the screening of the positive colony of laccase activity
Flat band method screening has bioactive bacterial strain: with toothpick picking positive colony list bacterium colony from YPDSZ flat board, point sample with containing Cu
2+with on the MM flat board of ABTS after be positioned in 28 DEG C of incubators and cultivate, the methyl alcohol adding 100 μ L100% every day induces it to produce expression of enzymes on the lid of culture dish, observes its colour-change every day.If seen at the distinctive blackish green haloing of single periphery of bacterial colonies appearance, prove express and have activity.As shown in figure 11, lac7+10AA has expression to dull and stereotyped detected result.
Whether shaking culture qualification recombinant bacterial strain expresses: 1. recombination yeast 28 DEG C of shaking tables in 3mL YPD+3 μ l Zeocin test tube are cultivated; 2. press 1% inoculum size by bacterium liquid in test tube, be inoculated in and be equipped with in the 250mL triangular flask of 50mLBMGY substratum, 28 DEG C of 250rpm shaking tables are cultured to OD
600=30; 3. the centrifugal 5min of 1500-3000g room temperature collects thalline, abandons supernatant; 4. use the resuspended thalline of BMMY, be concentrated to the 2/5(20mL of original volume); 5. resuspended thalline is put into the triangular flask of 250mL, every bottle adds Cu
2+be 500 μMs of 250rpm to final concentration, 25 DEG C of cultivations; 6. within every 24 hours, adding the methyl alcohol of one time 100%, is 1% to final concentration; 7. every 24 hours sampling 0.2mL, 5000rpm centrifuging and taking supernatants.Sample 15 days altogether; 8. detect supernatant liquor enzyme according to ABTS method to live, make growth curve chart.
As shown in figure 12, use the result of shaking culture and the MM dull and stereotyped result that develops the color consistent, lac7+10AA has expression to result.
Four, different concns cupric ion is on the impact of restructuring laccase induction
Impact restructuring laccase expression level a lot of because have in pichia spp, because cupric ion is the structure element of laccase, the impact that research different concns cupric ion is induced restructuring laccase.Cultivate restructuring laccase lac7+10AA respectively, when transferring in BMMY using do not add cupric ion as blank, establish 100 μMs, 200 μMs, 300 μMs, 400 μMs, 500 μMs, 600 μMs 6 concentration gradients respectively, each concentration 3 bottles of Duplicate Samples, starting cell concentration OD600 is 30,25 DEG C of 250rpm shaking tables are cultivated, and every 24h samples and adds methyl alcohol to final concentration is 1%, and centrifuging and taking supernatant is surveyed enzyme and lived.
Different Cu ionic concn affects result as shown in figure 13 to lac7+10AA induction product enzyme, adds different concns Cu
2+with do not add Cu
2+substratum compare, enzyme live all is greatly increased, different Cu
2+the impact that concentration produces enzyme to laccase is also different.The present embodiment lac7+10AA culture effect is it is preferred that add 500 μMs of Cu when abduction delivering
2+, induce enzyme work after 11 days to reach 1.288IU/mL.
Five, the separation and purification of restructuring laccase
The process of crude enzyme liquid: cultivate the enzyme liquid after 7d through BMMY abduction delivering, 4 DEG C of centrifugal 10min of 5000rpm get clear enzyme solution, through suction filtration, ultrafiltration and concentration 20mM Tris-HCl(pH8.0) dialysis after prepared anion column, often walk all detects enzyme work and protein content.
The separation and purification process of DEAE-SepharoseTMCL-6B: the crude enzyme liquid after process carries out DEAE-SephroseTMCL-6B ion-exchange chromatography, adopts balance liquid A phase: 20mM Tris-HCl buffer(pH8.0); Elution buffer B phase: containing the 20mmol/L Tris-HCl damping fluid (pH8.0) of 1M NaCl.Loading flow velocity: 0.5mL/min, elution speed: 0.5mL/min.Type of elution: B phase 0-1.0M NaCl linear elution; Be in charge of collection elutriant, every 10min collects a pipe, detects laccase activity, obtains the collection liquid of laccase activity.
Sephadex G-75 sieve chromatography: the collection liquid of laccase activity that has collected after DEAE ion-exchange chromatography is loaded in dialysis tubing, 4 DEG C of gentle agitation dialysis 24h(dialyzates: 20mmol/L NaH
2pO
4-Na
2hPO
4buffer, pH7.0), change 3-4 damping fluid therebetween.Salt ionic concentration through the enzyme liquid of dialysis is adjusted.Enzyme liquid after process carries out Sephadex G-75 sieve chromatography, elution buffer (20mmol/L NaH
2pO
4-Na
2hPO
4buffer, pH7.0).Loading flow velocity: 0.5mL/min, elution speed: 0.5mL/min.Every 4min collects a pipe, detects laccase activity, obtains the collection liquid of laccase activity.Enzyme liquid again chromatography 4 DEG C of gentle agitation dialysis 24h(dialyzates: pH7.0, phosphate buffered saline buffer), put into-20 DEG C of preservations.
The mensuration of protein content: the protein content measuring enzyme liquid adopts BCA Protein Assay Kit.First react production standard curve with the bovine serum albumin of different concns and working fluid.Allow enzyme liquid and working fluid react according to the making method of typical curve, record absorbance, typical curve is found out the protein concn corresponding to this absorbance.
The making of BCA protein assay kit standard curve: the bovine serum albumin standardized solution preparing a series of concentration, 0 μ g/mL, 25 μ g/mL, 125 μ g/mL, 250 μ g/mL, 500 μ g/mL, 750 μ g/mL, 1000 μ g/mL, 1500 μ g/mL, 2000 μ g/mL, get 25 μ l and often plant standard protein, add the working fluid that in test kit, A reagent and B reagent are made into, after mixing rear 37 DEG C of insulation 30min, be cooled to the absorbance that room temperature surveys 562nm.With the absorbance recorded for ordinate zou, protein concentration is X-coordinate production standard curve: y=0.0012x.
The detection of six, separation and purification effect
SDS-PAGE electrophoresis detection purification effect, step is as follows:
1) preparation (amounts of two pieces of glue) of separation gel: 4.0mL Acer-Bis(30:0.8), 2.4mL5 × Separatingbuffer, 5.4mL Distilled water, 4 μ L TEMED, 120 μ L AP.After separation gel solution is mixed successively (finally adding AP), rapidly glue is injected gel mold, after reaching desired height, glue face is injected the distilled water of one deck 1-5mm gently, then leave standstill 20-60 minute and wait for gel polymerisation.
2) preparation (amounts of two pieces of glue) of concentrated glue: 1.25mL Acer-Bis(30:0.8), 2.0mL5 × Stacking buffer, 6.6mL Distilled water, 4 μ L TEMED, 120 μ L AP.After glue polymerization to be separated, first remove the water layer on separation gel, then will concentrate on sol solution immediate stability ground injection separation gel until top.Careful tilts to insert comb on top, and in time arriving sheet glass top at the bottom of its tooth, flatten comb, attention should avoid increment to leave bubble, leaves standstill 30 minutes and waits for gel polymerisation, then carefully take out comb, do not tear well.
3) process of sample: the ratio of sample and sample buffer is 4:1,40 μ l samples are got in this experiment and 10 μ l5 sample buffer (containing SDS) doubly mixes.100 DEG C are boiled 10min.Of short durationly centrifugal water of condensation on tube wall is deposited at the bottom of pipe.
4) application of sample: gel is put into electrophoresis chamber, adds electrophoretic buffer, makes gel two ends be immersed in damping fluid, connects electrode, loading.Draw 40 μ l enzyme liquid with microsyringe, carefully stretch into bottom well, stable by sample addition one arrowband.Sample buffer should be added, to prevent fringing effect in emptying aperture.
5) electrophoresis: after application of sample, adds voltage at electrophoresis chamber the two poles of the earth, and before sample enters separation gel, voltage is 100V, after entering separation gel, voltage is increased to 200V, when going to bottom separation gel to blue forward position, stops electrophoresis.
6) dyeing and decolouring: take out gel, preparation coomassie brilliant blue staining about 4 hours, then decolour once for every 5 hours with destainer.Glue there will be obviously and clearly blue bands, photographic recording.
Enzyme liquid SDS-PAGE after separation and purification detects, and the results are shown in Figure 14: the Lac7+10AA molecular weight after purifying is 70kDa, after the process of pure enzyme deglycosylating enzyme, molecular weight is about 52kDa.
Seven, the mensuration of laccase activity
1) ABTS method: in 1mL reaction mixture, containing 100 μ L1mmol/L(final concentrations) ABTS, 800 μ L0.1mol/L NaAc-HAc damping fluid (pH4.5), 100 μ L enzyme liquid are 1 Ge Meihuo unit (IU) at 40 DEG C with the enzyme amount of the 1 μm of olABTS of catalyzed oxidation in 1min.The OD changing value in 1min is measured at 420nm place.The molar extinction coefficient of known 420nm place ABTS is ε 420=3.6 × 104M
-1.cm
-1.
Enzyme (IU/mL)=OD alive
420/ (3.6 × 104 × V/106) (V is that enzyme liquid amasss)
2) guaiacol method: by enzyme liquid at 4 DEG C, supernatant liquor 0.1mL is got after the centrifugal 20min of 10000r/min, add 0.3mL distilled water and 2mL50mmol/mL(containing 1mmol/L methyl catechol) succinate buffer (pH5.0), mix and be placed on 37 DEG C of water-bath 30min, ice bath termination reaction, surveys its light absorption value at 465nm place.Enzyme unit definition of living be the enzyme amount that per minute is oxidized 1 μm of ol methyl catechol is a Ge Meihuo unit.
Enzyme (IU/mL)=2.4 × OD alive
465/ (12100 × 30 × V/106) (V is that enzyme liquid amasss)
3) syringaldazine method: in 1mL reaction mixture, containing 100 μ L1mmol/L(final concentrations) syringaldazine, 800 μ L0.1mol/L NaAc-HAc damping fluid (pH4.5), 100 μ L enzyme liquid are 1 Ge Meihuo unit (IU) at 40 DEG C with the enzyme amount of the 1 μm of ol syringaldazine of catalyzed oxidation in 1min.The OD changing value in 1min is measured at 525nm place.The molar extinction coefficient of known 525nm place syringaldazine is ε 525=6.5 × 105M
-1.cm
-1.
Enzyme (IU/mL)=OD alive
525/ (6.5 × 105 × V/106) (V is that enzyme liquid amasss)
4) 2,6-xylenol method: in 1mL reaction mixture, containing 100 μ L1mmol/L(final concentrations) 2,6-xylenol, 800 μ L0.1mol/L NaAc-HAc damping fluid (pH4.5), 100 μ L enzyme liquid are 1 Ge Meihuo unit (IU) at 40 DEG C with the enzyme amount of 1 μm of ol2, the 6-xylenol of catalyzed oxidation in 1min.The OD changing value in 1min is measured at 421nm place.The molar extinction coefficient of known 421nm place 2,6-xylenol is ε 421=5.78 × 104M
-1.cm
-1.
Enzyme (IU/mL)=OD alive
421/ (5.78 × 104 × V/106) (V is that enzyme liquid amasss)
Eight, the analysis of restructuring Coprinus comatus laccase enzymatic property
1) optimum temperuture of restructuring Coprinus comatus laccase: be the reaction vigor of restructuring Coprinus comatus laccase under different amboceptor and differing temps after investigating purifying, obtain optimal reaction temperature, devise different temperature of reaction, it is 20 DEG C-90 DEG C, gradient is 5 DEG C, amboceptor is respectively ABTS, methyl catechol, syringaldazine and 2,6-syringol.Laccase activity is detected according to the method described above under differing temps.Live soprano for 100% with enzyme.As shown in figure 15, Lac7+10AA corresponding A BTS, methyl catechol, syringaldazine, the optimum temperuture of each substrate of 2,6-syringol is 60 DEG C to result respectively, 60 DEG C, 65 DEG C, 65 DEG C.
Laccase Lac7+10AA after purifying, after 30 DEG C-70 DEG C scope inside holding 15min, 30min, 45min, 60min, take ABTS as the laccase activity under substrate detects differing temps insulation different time.Preserve uninsulated enzymes with 4 DEG C to live as 100%, the results are shown in Figure 16, after the laccase Lac7+10AA after purifying is incubated 15min, 30 DEG C, 40 DEG C, 50 DEG C residual enzyme work more than 80%, 60 DEG C drop to 47.9%, and at 70 DEG C only surplus 1.8%; After 30min, 30 DEG C, 40 DEG C, 50 DEG C residual enzymes are lived and are still maintained about 80%, but the enzyme that substantially do not have at only remaining 26%, 70 DEG C at 60 DEG C is lived; After insulation 60min, 30 DEG C, 40 DEG C, 50 DEG C still have the enzyme of more than 60% to live, and the enzyme of 60 DEG C is lived and dropped to 8.7%.Result shows, and laccase Lac7+10AA has good thermostability between 30 DEG C-50 DEG C.
2) optimal pH of restructuring Coprinus comatus laccase: be the reaction vigor of restructuring Coprinus comatus laccase under different amboceptor and different pH after investigating purifying, obtain optimum response pH, configuration pH is the extensive damping fluid of 1.0-12.0, gradient is 0.5, amboceptor is respectively ABTS, methyl catechol, syringaldazine and 2,6-syringol.Laccase activity is measured according to the method described above under different pH damping fluid.Live soprano for 100% with enzyme.The results are shown in Figure 17, Lac7+10AA corresponding A BTS, methyl catechol, syringaldazine, the optimal pH of each substrate of 2,6-syringol is 3,5,6,5 respectively.
Laccase Lac7+10AA after purifying 4 DEG C of placements under the condition of pH1-12 are surveyed enzyme and are lived after 24 hours, live as 100% with the highest enzyme.Result is as Figure 18, and display Lac7+10AA has good stability between pH5-7, and residual enzyme work reaches more than 80%.
With reference to aforesaid method, the laccase gene of clone is directly connected with pPICZ α B carrier by the present embodiment, but lac7 does not express.
Embodiment 3 is recombinated the decolouring of Coprinus comatus laccase to dyestuff
The preparation of enzyme liquid: triangular flask cultivates the restructuring laccase Lac7+10AA of clone, at 25 DEG C, 500MCu
2+every 24h adds 1% methanol induction to express, and cultivate and collect enzyme liquid afterwards in 10 days, after suction filtration, ultrafiltration and concentration ,-80 DEG C save backup.
(1) to recombinate under different time the decolouring of Coprinus comatus laccase to dyestuff
In 2mL decolouring system, dye concentrations 50mg/L, 0.1mol/L NaAc-HAc damping fluid, to enzyme amount 0.5IU/mL, the final concentration 0 of HBT or 0.1g/L, pH4.5, temperature 40 DEG C, respectively the time be 1,2,3,4,12h time, measure the light absorption value (A of each reaction solution in corresponding dyestuff maximum absorption wave strong point
1), in contrast with inactivator liquid, same method records its light absorption value A simultaneously
0, percent of decolourization is R=(A
0-A
1)/A
0× 100%.
As shown in Figures 19 and 20, restructuring laccase Lac7+10AA has good decolorizing effect to each dyestuff, and when 1-2h, percent of decolourization increase is the fastest, and subsequently along with the prolongation of time, decolorization rate slows down, and substantially completes to during 12h the decolouring of dyestuff.It is fast that enzyme process decolouring has degradation speed, the advantage that the reaction times is short, Yang Bo
[64]study carefully laccase to find the decolouring of reactive brilliant blue K-GR, reacting that one hour percent of decolourization just can reach is 74.2% and 78.6%, reacts two hours percent of decolourizations and reaches 78% and 79.5%.The decolorization great majority of laccase to dyestuff occur in initial one or two hour as can be seen here.
(2) pure enzyme and thick enzyme are to the contrast of the dye decolored effect of three classes
In 2mL decolouring system, dye concentrations 50mg/L, 0.1mol/L NaAc-HAc damping fluid, to enzyme amount (0.5IU/mL), have medium (0.1g/L) with without in the reaction conditions of medium, pH4.5, temperature 40 DEG C, the time is 12h, measures the light absorption value (A of each reaction solution in corresponding dyestuff maximum absorption wave strong point
1), in contrast with inactivator liquid, same method records its light absorption value A simultaneously
0, percent of decolourization is R=(A
0-A
1)/A
0× 100%.
As shown in figures 21-23, when without amboceptor, the thick enzyme of Lac7+10AA, to triphenylmethane dye decolorization best results, is secondly anthraquinone dyes, relatively poor to the dye decolored effect of azo.Thick enzyme is after adding HBT, and the percent of decolourization of all dyestuffs all increases, and to increase maximum be azo dyes, and be secondly triphenylmethane dye, the percent of decolourization increase of anthraquinone dyes is less.Thunder agate azoles light blue, Reactive Brilliant Blue X-BR, reactive brilliant bule K-GR and reactive brilliant bule K-3R(anthraquinone dyes) percent of decolourization be increased to 39.56%, 19.37%, 34.07%, 38.25% by 32.31%, 7.18%, 26.39%, 37.5% respectively.Reactive orange, reaction brilliant red X-3B, percent of decolourization that is Congo red and reactive deep blue K-R (azo dyes) are increased to 5.2%, 30.65%, 22.35%, 73.06% by 1.48%, 1.08%, 15.79%, 69.64% respectively.The percent of decolourization of malachite green, Coomassie brilliant G-250, methyl violet, tetrabromophenol sulfonphthalein and victoria blue B (triphenylmethane dye) is added to 78.6%, 14.53%, 41.63%, 40.09%, 25.8% by 66.7%, 10.85%, 17.43%, 24.09%, 17.72% respectively.
The pure enzyme of Lac7+10AA is best to anthraquinone dyes decolouring, is secondly triphenylmethane dye, relatively poor to the dye decolored effect of azo.After adding amboceptor HBT, decolorizing effect also obviously increases.The pure enzyme of Lac7+10AA, after adding HBT, all increases the percent of decolourization of all dyestuffs, and wherein increasing maximum is azo dyes, and be secondly triphenylmethane dye, anthraquinone dyes increase is relatively little.Thunder agate azoles light blue, Reactive Brilliant Blue X-BR, reactive brilliant bule K-GR and reactive brilliant bule K-3R(anthraquinone dyes) percent of decolourization be increased to 95.66%, 68.52%, 75.9%, 85.52% by 75.38%, 38.12%, 65.83%, 73.65% respectively.Reactive orange, reaction brilliant red X-3B, percent of decolourization that is Congo red and reactive deep blue K-R (azo dyes) are increased to 55.06%, 70.56%, 58.34%, 89.12% by 4.4%, 3.15%, 28.26%, 80.52% respectively.The percent of decolourization of malachite green, Coomassie brilliant G-250, methyl violet, tetrabromophenol sulfonphthalein and victoria blue B (triphenylmethane dye) is added to 93.96%, 58.02%, 76.17%, 79.12%, 57.22% by 83.73%, 26.72%, 45.28%, 62.67%, 30.42% respectively.
SEQUENCE LISTING
<110> Nanjing Forestry University
<120> laccase gene Lac7 and expressing protein thereof and application
<130> 100
<160> 15
<170> PatentIn version 3.3
<210> 1
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<213> Copyinds comatus Gray
<400> 2
Met Leu His Leu Leu Ser Phe Ala Phe Ile Gly Ala Asn Ala Phe Ala
1 5 10 15
Leu Ser Val Gly Pro Arg Ala Thr Leu Thr Leu Thr Asn Asp Val Val
20 25 30
Ala Pro Asp Gly Phe Glu Arg Ser Ala Ile Val Val Asn Gly Gly His
35 40 45
Pro Gly Pro Leu Ile Gln Ala Asn Lys Gly Asp Ala Tyr Thr Ile Asn
50 55 60
Val Val Asn Arg Leu Thr Asp Ser Thr Met Gln Arg Val Ser Ser Ile
65 70 75 80
His Trp His Gly Leu Ser Gln Arg Gly Thr Asn Trp Ala Asp Gly Gly
85 90 95
Ser Gly Val Asn Gln Cys Pro Ile Ser Pro Asn His Ser Phe Glu Tyr
100 105 110
Gln Phe Ser Gly Arg Lys Asp Gln Ala Gly Thr Phe Trp Tyr His Ser
115 120 125
His Tyr Ser Ile Gln Tyr Cys Asp Gly Leu Arg Gly Pro Leu Val Ile
130 135 140
Tyr Asp Pro Asn Asp Pro Phe Lys Asn Leu Tyr Asp Val Asp Asp Glu
145 150 155 160
Ser Thr Val Ile Thr Leu Thr Asp Trp Tyr His Thr Pro Phe Pro Ser
165 170 175
Val Thr Gly Pro Pro Thr Ser Asp Ser Thr Leu Ile Asn Gly Lys Gly
180 185 190
Arg Tyr Pro Gly Gly Pro Asn Val Asp Leu Ser Val Ile Asn Val Glu
195 200 205
Arg Gly Lys Arg Tyr Arg Phe Arg Leu Val Ala Leu Thr Cys Glu Asn
210 215 220
Ser His Leu Phe Gly Ile Asp Gly His Gln Leu Leu Val Ile Glu Thr
225 230 235 240
Gly Gly Glu Ser Thr Val Pro Thr Leu Val Asp Lys Ile Thr Leu Leu
245 250 255
Ala Gly Gln Arg Tyr Ser Phe Val Leu Asp Ala Asn Gln Ala Val Asp
260 265 270
Asn Tyr Trp Ile Arg Gly Leu Pro Arg Ser Gly Val Pro Ser Leu Lys
275 280 285
Ala Gly Tyr Glu Gly Gly Leu Asn Ser Ala Ile Leu Arg Tyr Gln Gly
290 295 300
Ala Pro Ile Thr Glu Pro Gln Thr Thr Asp Asn Glu Asn Ala Ala Leu
305 310 315 320
Leu Asp Glu Ala Gln Leu Val Pro Thr Arg Asn Pro Phe Ala Pro Gly
325 330 335
Arg Pro Thr Ser Gly Gly Ala Asp Phe Asn Val Thr Val Asn Phe Glu
340 345 350
Leu Asp Leu Thr Thr Gly Ser Pro His Phe Lys Leu Asn Gly Lys Ile
355 360 365
Tyr Gln Pro Pro Thr Val Pro Ile Leu Leu Gln Ile Ile Ser Gly Ala
370 375 380
Arg Lys Ala Glu Glu Leu Leu Pro Glu Gly Asn Ile Tyr Phe Val Pro
385 390 395 400
Arg Asn Lys Val Val Glu Val Thr Val Pro Gly Gly Ile Pro Gly Ala
405 410 415
Pro His Pro Met His Leu His Gly His His Phe Ser Val Val Lys Ser
420 425 430
Ala Gly Lys His Asn Gln Val Asn Tyr Leu Thr Pro Val Arg Arg Asp
435 440 445
Thr Thr Ala Ser Pro Val Glu Val Asp Asp Asn Thr Thr Ile Arg Phe
450 455 460
Thr Thr Asp Ser Pro Gly Pro Trp Ile Phe His Cys His Phe Asn Lys
465 470 475 480
His Gln Ser Ile Gly Met Ala Val Val Phe Val Ala Asp Ile Asp Glu
485 490 495
Val Ala Glu Lys Asn Pro Thr Pro Asp Ala Trp Asn Asp Leu Cys Pro
500 505 510
Ile Tyr Gln Ser Leu Ser Glu Ser Glu Thr Val Val Glu Ile Val Pro
515 520 525
Met Val Lys His
530
<210> 3
<211> 551
<212> PRT
<213> Artificial
<220>
The aminoacid sequence of <223> Lac7+10AA
<400> 3
Thr Pro Phe Pro Pro Phe Asn Thr Asn Ser Ser Arg Leu Ser Val Gly
1 5 10 15
Pro Arg Ala Thr Leu Thr Leu Thr Asn Asp Val Val Ala Pro Asp Gly
20 25 30
Phe Glu Arg Ser Ala Ile Val Val Asn Gly Gly His Pro Gly Pro Leu
35 40 45
Ile Gln Ala Asn Lys Gly Asp Ala Tyr Thr Ile Asn Val Val Asn Arg
50 55 60
Leu Thr Asp Ser Thr Met Gln Arg Val Ser Ser Ile His Trp His Gly
65 70 75 80
Leu Ser Gln Arg Gly Thr Asn Trp Ala Asp Gly Gly Ser Gly Val Asn
85 90 95
Gln Cys Pro Ile Ser Pro Asn His Ser Phe Glu Tyr Gln Phe Ser Gly
100 105 110
Arg Lys Asp Gln Ala Gly Thr Phe Trp Tyr His Ser His Tyr Ser Ile
115 120 125
Gln Tyr Cys Asp Gly Leu Arg Gly Pro Leu Val Ile Tyr Asp Pro Asn
130 135 140
Asp Pro Phe Lys Asn Leu Tyr Asp Val Asp Asp Glu Ser Thr Val Ile
145 150 155 160
Thr Leu Thr Asp Trp Tyr His Thr Pro Phe Pro Ser Val Thr Gly Pro
165 170 175
Pro Thr Ser Asp Ser Thr Leu Ile Asn Gly Lys Gly Arg Tyr Pro Gly
180 185 190
Gly Pro Asn Val Asp Leu Ser Val Ile Asn Val Glu Arg Gly Lys Arg
195 200 205
Tyr Arg Phe Arg Leu Val Ala Leu Thr Cys Glu Asn Ser His Leu Phe
210 215 220
Gly Ile Asp Gly His Gln Leu Leu Val Ile Glu Thr Gly Gly Glu Ser
225 230 235 240
Thr Val Pro Thr Leu Val Asp Lys Ile Thr Leu Leu Ala Gly Gln Arg
245 250 255
Tyr Ser Phe Val Leu Asp Ala Asn Gln Ala Val Asp Asn Tyr Trp Ile
260 265 270
Arg Gly Leu Pro Arg Ser Gly Val Pro Ser Leu Lys Ala Gly Tyr Glu
275 280 285
Gly Gly Leu Asn Ser Ala Ile Leu Arg Tyr Gln Gly Ala Pro Ile Thr
290 295 300
Glu Pro Gln Thr Thr Asp Asn Glu Asn Ala Ala Leu Leu Asp Glu Ala
305 310 315 320
Gln Leu Val Pro Thr Arg Asn Pro Phe Ala Pro Gly Arg Pro Thr Ser
325 330 335
Gly Gly Ala Asp Phe Asn Val Thr Val Asn Phe Glu Leu Asp Leu Thr
340 345 350
Thr Gly Ser Pro His Phe Lys Leu Asn Gly Lys Ile Tyr Gln Pro Pro
355 360 365
Thr Val Pro Ile Leu Leu Gln Ile Ile Ser Gly Ala Arg Lys Ala Glu
370 375 380
Glu Leu Leu Pro Glu Gly Asn Ile Tyr Phe Val Pro Arg Asn Lys Val
385 390 395 400
Val Glu Val Thr Val Pro Gly Gly Ile Pro Gly Ala Pro His Pro Met
405 410 415
His Leu His Gly His His Phe Ser Val Val Lys Ser Ala Gly Lys His
420 425 430
Asn Gln Val Asn Tyr Leu Thr Pro Val Arg Arg Asp Thr Thr Ala Ser
435 440 445
Pro Val Glu Val Asp Asp Asn Thr Thr Ile Arg Phe Thr Thr Asp Ser
450 455 460
Pro Gly Pro Trp Ile Phe His Cys His Phe Asn Lys His Gln Ser Ile
465 470 475 480
Gly Met Ala Val Val Phe Val Ala Asp Ile Asp Glu Val Ala Glu Lys
485 490 495
Asn Pro Thr Pro Asp Ala Trp Asn Asp Leu Cys Pro Ile Tyr Gln Ser
500 505 510
Leu Ser Glu Ser Glu Thr Val Val Glu Ile Val Pro Met Val Lys His
515 520 525
Pro Arg Glu Gln Lys Leu Ile Ser Glu Glu Asp Leu Asn Ser Ala Val
530 535 540
Asp His His His His His His
545 550
<210> 4
<211> 20
<212> DNA
<213> Artificial
<220>
<223> position forward primer
<220>
<221> misc_feature
<222> (12)..(12)
<223> n is a, c, g, or t
<400> 4
caytggcayg gnttyttyca 20
<210> 5
<211> 22
<212> DNA
<213> Artificial
<220>
<223> No. bis-position reverse primers
<220>
<221> misc_feature
<222> (17)..(17)
<223> n is a, c, g, or t
<220>
<221> misc_feature
<222> (20)..(20)
<223> n is a, c, g, or t
<400> 5
grctgtggta ccagaangtn cc 22
<210> 6
<211> 20
<212> DNA
<213> Artificial
<220>
<223> No. tetra-position reverse primers
<400> 6
tgccartcda trtgrcartg 20
<210> 7
<211> 27
<212> DNA
<213> Artificial
<220>
<223> Laccase7 GSP1
<400> 7
ctccggaacc accatcagcc caattag 27
<210> 8
<211> 643
<212> DNA
<213> Artificial
<220>
<223> 5'-RACE sequence fragment sequence
<400> 8
ctaatacgac tcactatagg gcaagcagtg gtatcaacgc agagtacgcg ggggatgccg 60
gattaggtat attttcgttt gtcaatgccc gcccaaactt gttgaactca attactcacc 120
cccaaaatta ttgcatgtct gaatttcaca tcatctatct tggcatataa gagcttctag 180
cctcaaatgt gatcctgatg tttcatgtct ggacgccgtt agtgcgtccc tggggttaat 240
tgcgggtttt ggtttggtat tctttgcagt tccagtttaa aagatctcac ttttcctttt 300
gaatgaacac gaacacgtac cccccccccc ccagtacctt tcctgtgaat gctccatttg 360
ctttcttttg cctttatagg cgccaatgct tttgcgcttt ctgtcggtcc acgagcaact 420
cttacattga cgaatgacgt agttgcgcct gatggttttg aacgatctgc cattgttgtc 480
aacggaggac atcctgggcc actgattcaa gcgaacaagg gtaatgccta cacgattaat 540
gttgttaatc ggctcacgga ctccaccatg cagagagttt cttctattca ttggcatggt 600
ctctctcaga gaggtactaa ttgggctgat ggtggttccg gag 643
<210> 9
<211> 29
<212> DNA
<213> Artificial
<220>
<223> Laccase7GSP2
<400> 9
ggcgccaatg cttttgcgct ttctgtcgg 29
<210> 10
<211> 30
<212> DNA
<213> Artificial
<220>
<223> introduces nucleotide sequence corresponding to 10 aminoacid sequences
<400> 10
acgccattcc cccctttcaa caccaactct 30
<210> 11
<211> 10
<212> PRT
<213> Artificial
<220>
<223> introduces 10 aminoacid sequences
<400> 11
Thr Pro Phe Pro Pro Phe Asn Thr Asn Ser
1 5 10
<210> 12
<211> 61
<212> DNA
<213> Artificial
<220>
<223> Lac7gcDNAF
<400> 12
gctctagatg acgccattcc cccctttcaa caccaactct ctttctgtcg gtccacgagc 60
a 61
<210> 13
<211> 31
<212> DNA
<213> Artificial
<220>
<223> Lac7gcDNAR
<400> 13
gtccccgcgg atgtttcacc ataggcacaa t 31
<210> 14
<211> 21
<212> DNA
<213> Artificial
<220>
<223> 5'AOX sequence
<400> 14
gactggttcc aattgacaag c 21
<210> 15
<211> 20
<212> DNA
<213> Artificial
<220>
<223> 3'AOX sequence
<400> 15
ggcaaatggc attctgacat 20
Claims (4)
1. a laccase gene Lac7, its DNA sequence dna is sequence as shown in the 349-1947 position Nucleotide of SEQ ID NO.1.
2. the expressing protein of laccase gene described in claim 1, its aminoacid sequence is as shown in SEQ ID NO.2.
3. an expression method for the expressing protein of laccase gene described in claim 2, is characterized in that: the expression label being added with 10 aminoacid sequence compositions on aminoacid sequence shown in described SEQ IDNO.2, and described aminoacid sequence is TPFPPFNTNS; Expressed protein sequence is as shown in SEQ ID NO.3.
4. laccase gene Lac7 according to claim 1 is to the application in dye decolored.
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| CN110295182A (en) * | 2019-07-04 | 2019-10-01 | 山东省农业科学院生物技术研究中心 | A kind of laccase gene slr1573 derived from cytoalgae and the application in dye decolored |
Citations (2)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN101845420A (en) * | 2010-03-31 | 2010-09-29 | 中国科学院南京土壤研究所 | Method of extracting crude enzyme preparation for degrading polycyclic aromatic hydrocarbons |
| CN102268414A (en) * | 2011-06-16 | 2011-12-07 | 北京市农林科学院 | Coprinus comatus laccase with activity of inhibiting tumor cell proliferation and preparation method thereof |
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Patent Citations (2)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN101845420A (en) * | 2010-03-31 | 2010-09-29 | 中国科学院南京土壤研究所 | Method of extracting crude enzyme preparation for degrading polycyclic aromatic hydrocarbons |
| CN102268414A (en) * | 2011-06-16 | 2011-12-07 | 北京市农林科学院 | Coprinus comatus laccase with activity of inhibiting tumor cell proliferation and preparation method thereof |
Non-Patent Citations (4)
| Title |
|---|
| Engineering the expression and characterization of two novel laccase isoenzymes from Coprinus comatus in Pichia pastoris by fusing an additional ten amino acids tag at N-terminus;Chunjuan Gu et al;《PlosONE》;20140407;摘要、图2、材料与方法部分 * |
| Heterologous expression and characterization of a novel laccase isoenzyme with dyes decolorization potential from Coprinus comatus;Songyuan Bao et al;《Mol Biol Rep 》;20121018;第40卷;摘要、第1928页左栏第3段至1929页左栏第1段、1930页左栏第5段至1930页右栏第1段、图1、表3 * |
| 栓菌漆酶在毕赤酵母中高效表达及重组酶的性质;周宏敏 等;《生物工程学报》;20071130;第23卷(第6期);摘要、1.1-1.4节 * |
| 鸡腿菇漆酶诱导、对染料脱色及基因克隆研究;姜曼;《中国优秀硕士论文全文数据库》;20120515;摘要、第4.2、4.3节 * |
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