CN104342412B - For producing the Ketoreductase mutant of (S) -4- chloro-3-hydroxyl ethyl butyrate - Google Patents
For producing the Ketoreductase mutant of (S) -4- chloro-3-hydroxyl ethyl butyrate Download PDFInfo
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- CN104342412B CN104342412B CN201310345823.3A CN201310345823A CN104342412B CN 104342412 B CN104342412 B CN 104342412B CN 201310345823 A CN201310345823 A CN 201310345823A CN 104342412 B CN104342412 B CN 104342412B
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Abstract
The present invention relates to a kind of Ketoreductase mutants, its wild type ketoreductase for being derived from Kefir grains lactobacillus (Lactobacillus kefir), 4- chloroacetyl acetacetic ester can be converted into (S) -4- chloro-3-hydroxyl ethyl butyrate, with A94S, F147V, one or more mutation in L199P, A202V.Ketoreductase mutant of the invention has apparent high specific enzyme activity, improves 2-20 times than wild type ketoreductase, using the enzyme can biocatalysis 4- chloroacetyl acetacetic ester is converted into (S) -4- chloro-3-hydroxyl ethyl butyrate;Reaction condition is mild, low for equipment requirements, and production process is not necessarily to high temperature or cooling, low energy consumption, since enzymatic has efficiently, single-minded selectivity, therefore production statins key intermediate (S) -4- chloro-3-hydroxyl ethyl butyrate no coupling product generates in this way, purifying is convenient;Furthermore reacting most solvents is water, and three waste discharge is low, environmentally protective.
Description
Technical field
The present invention relates to Ketoreductase mutant and its statins drug midbody production in application, in particular to one
Kind is derived from the Ketoreductase mutant of Kefir grains lactobacillus (Lactobacillus kefir) and its in the chloro- 3- of chirality (S) -4-
Application in hydroxy-butyric acid ethyl ester production.
Background technique
Atorvastatin calcium (trade name LIPITOR is sold by Pfizer), rosuvastatin calcium (trade name CRESTOR
Sold by Astrazeneca AB) and Pitavastatin (trade (brand) name Lipalo is by Nissan Chemical and Kowa company in Japan
Sale), it is important norcholesterol statins.And chirality (S) -4- chloro-3-hydroxyl-ethyl butyrate is these important they
The crucial chiral intermediate of spit of fland class drug.The yield of the domestic intermediate in 2009 is 400 tons, it is contemplated that in the coming years, state
Interior yield is up to 1000 tons or more, and direct economic benefit is in several hundred million members.The many of these chiral intermediates are prepared known
In approach, including chemical method and enzyme process, all tool have disadvantages that.Since chemical method synthesis process condition is harsh, side reaction is more, produces
Product isolate and purify that difficulty is big, and yield is low, at high cost, it is made to be difficult to become the ideal method for commercial scale synthesis.Using enzyme
Method preparation and chirality (S) -4- chloro-3-hydroxyl-ethyl butyrate need to use the ketoreductase with stereoselectivity, but existing
Wild type ketoreductase catalytic activity is very lower, and the ketone substrate of 1g/L can be only converted within 20 hours using the thick enzyme powder of 10g/L, is also made
It is difficult to become the ideal method for commercial scale synthesis.
Summary of the invention
The object of the present invention is to provide a kind of ketoreductases and preparation method thereof that enzymatic activity is high.
Realizing the technical solution of the object of the invention is: naturally depositing in Kefir grains lactobacillus (Lactobacillus kefir)
Wild type ketoreductase, 4- chloroacetyl acetacetic ester (COBE) can be converted to (S) -4- chloro-3-hydroxyl ethyl butyrate (S-
CHBE).The inventor of present disclosure has found ketoreductase and Kefir grains lactobacillus including being mutated in certain position
The wild type ketoreductase (SEQ ID NO:2) that (Lactobacillus kefir) is generated is lived compared to increased catalysis is shown
Property." wild type ketoreductase ", " wild type KRED enzyme " and " wild type KRED ketoreductase " refers to by being originated from Kefir grains lactobacillus
The wild type ketoreductase genes of SEQ ID NO:1 coding of (Lactobacillus kefir), and there is SEQ ID NO:2
Amino acid sequence ketoreductase.4- chloroacetyl acetacetic ester asymmetric reduction can be generated (S) -4- chloro-3-hydroxyl by the enzyme
Ethyl butyrate." wild type " refers to the form of material or substance as found in nature.Such as the protein of wild type
Or nucleic acid sequence be can from nature separation and without artificial modification, the original series present in organism
Form." increased catalytic activity " refers to measured compared with wild type ketoreductase in test in vitro or in vivo, shows
Make substrate (such as 4- chloroacetyl acetacetic ester) to product (such as S-4- chloro-3-hydroxyl ethyl butyrate) the increased ketone of conversion ratio
Reductase.
Provided by the present invention for the Ketoreductase mutant of production (S) -4- chloro-3-hydroxyl ethyl butyrate, feature exists
In being derived from the wild type ketoreductase of Kefir grains lactobacillus (Lactobacillus kefir), wherein mutation is in parent
It is inserted into the amino acid sequence of this ketoreductase, replaces or lack one or more amino acid, or in parent's ketoreductase
One or two end of amino acid sequence adds or deletes one or more amino acid, and compared with using parent's ketoreductase,
Its 2-20 times of ketoreductase increased activity.
Further, the mutant has the amino acid substitution on following one or more amino acid positions, respectively takes
Alternative triplet indicates: alphabet-numeric playing-letter, wherein the position of digital representation mutating acid, and the letter before number is corresponding prominent
Becoming the amino acid of design, the letter after number indicates the amino acid for replacing amino acid before number: A94S, F147V,
L199P, A202V.
Ketoreductase mutant provided by the invention, derived from Kefir grains lactobacillus (Lactobacillus kefir)
Wild type ketoreductase, performance send as an envoy to substrate (such as 4- chloroacetyl acetacetic ester) to product (such as S-4- chloro-3-hydroxyl fourth
Acetoacetic ester) the increased ketoreductase of conversion ratio.The Ketoreductase mutant, the wild type ketoreductase with SEQ ID NO.2
Compared to showing stronger catalytic activity.Ability can be used in Ketoreductase mutant and the polynucleotides for encoding this mutant
The preparation of field technique personnel's commonly used approach.Mutant can by make to encode the vitro recombination of the enzyme, polynucleotides mutagenesis,
DNA reorganization, fallibility PCR and directed evolution method etc. obtain.
Further, the mutant includes the amino acid sequence of SEQ ID NO.4.
The ketoreductase of overall length mutation is for keeping the catalytic activity of enzyme to be not required in that.Correspondingly, it is considered as ketone also
The truncated analog of protoenzyme mutant and the segment for having catalytic activity.For example, in some embodiments, the number of C-terminal or N-terminal
A amino acid can be left out.Any specific truncated analog or segment can use corresponding test and live to assess catalysis
Property.Likewise, additional amino acid residue can be added to one or two end without influencing catalytic activity.Additional sequences
It can be functional or non-functional.For example, Additional amino acid sequences can be used to assist in purifying, as label, or
Execute some other functions.Therefore, the Ketoreductase mutant of present disclosure can be the form of fusion protein, wherein ketone
Enzyme mutant (or its segment) is restored such as by hydrotropy label (such as SUMO albumen), purification tag (as combined metal
His label) and bacterium positioning signal (such as secretion signal) example rather than limitation mode be fused to other oroteins.
Further, the present invention provides the encoding gene of above-mentioned mutant.
Further, encoding gene provided by the present invention, sequence include DNA molecular described in SEQ ID NO.3.Its
Sequence optimisation is had been subjected to be suitable in expression in escherichia coli.In some embodiments, polynucleotides include being optimized for
The codon expressed in certain types of host cell.The use of codon for various types of microorganism and partially
Good property is known, because it is the codon for the optimization of the specific amino acid of expression in these microorganisms.
The present invention provides a kind of recombinant plasmid, and sequence preferably is selected from SEQ ID NO.5, than pET series and the expression of pQE series
Carrier compared to it there is more rigorous expression to control.In some embodiments, control sequence include promoter, leader sequence,
Polyadenylation sequences, propeptide sequence, signal peptide sequence and transcription terminator etc..For bacterial host cell, code sequence is instructed
The suitable promoter of the transcription of column includes but is not limited to from Phage T5, phage t7, bacteriophage lambda, Escherichia coli
LacUV5 operon, Escherichia coli trp operon, Escherichia coli tac operon etc..
The present invention provides a kind of host cell, preferably is selected from Escherichia coli W3110, one of DH1 and JM109.Express ketone
The expression vector of reduction enzyme mutant may include permission, and vector integration is into host cell gene group or carrier is in bacterium
The element independently replicated independently of genome.To be integrated into host cell gene group, carrier can make to carry by recombined engineering
Body is integrated into genome.
The present invention provides a kind of method for preparing Ketoreductase mutant, it is characterised in that the following steps are included: (a) is constructed
The genetic engineering bacterium of Ketoreductase mutant is expressed, the genetic engineering bacterium includes host cell, expression vector and ketone reduction
Enzyme mutant gene;(b) it cultivates and induces the genetic engineering bacterium;(c) it is crushed the genetic engineering bacterium, collects crude enzyme liquid simultaneously
Carry out Enzyme activity assay.
The step (a) be will from Kefir grains lactobacillus (Lactobacillus kefir) encoding wild type ketone also
After the polynucleotides (SEQ ID NO:1) of protoenzyme carry out sequence optimisation according to bacterial strain DH1 codon preference, pass through full genome
The mode of synthesis obtains.The polynucleotides of coding ketoreductase after optimization are cloned into expression vector (SEQ ID NO. 5)
Under the control of promoter, the plasmid that can express wild type ketoreductase is obtained.Gained plasmid is transformed by standard method
In Escherichia coli DH1.Cloning process used is the mode of homologous recombination, used amplimer are as follows:
F:5'ATTAAAGAGGAGAAATTAACATATGACTGATCGTTTAAAAGGCAAAG 3';
R:5'AACAGGAGTCCAAGCTCAGCTTATTATTGAGCAGTGTATCCACCATCG 3'.
The polynucleotides for encoding Ketoreductase mutant (SEQ ID NO:3) are cloned into expression vector with same method
Under the control of the promoter of (SEQ ID NO. 5), the plasmid that can express Ketoreductase mutant is obtained.Gained plasmid is led to
Standard method is crossed to be transformed into Escherichia coli DH1.
The step (b) contains for picking has the Escherichia coli single colonie of purpose expression vector to be inoculated in 10ml high pressure sterilization
In the first culture medium afterwards, 30 DEG C, 250rpm is incubated overnight;Next day takes 1L triangular flask, is linked by the inoculative proportion of 1:100
In the second culture medium after 100ml high pressure sterilization, triangular flask is placed in 25 DEG C at once and shaken by culture to thallus OD 5-6 in 30 DEG C
In bed, 250rpm cultivates 1h, and IPTG to final concentration 0.1mM is added, and in 25 DEG C, 250rpm continues to cultivate 15h.
First culture medium are as follows: 10 g/L of tryptone, 5 g/L of yeast extract, 3.55 g/L of disodium hydrogen phosphate,
3.4 g/L of potassium dihydrogen phosphate, 2.68 g/L of ammonium chloride, 0.71 g/L of sodium sulphate, 0.493 g/L of epsom salt, six water chlorinations
Iron 0.027 g/L, glycerol 5g/L, glucose 0.8g/L add ampicillin to 100mg/L after sterilizing.
Second culture medium are as follows: 10 g/L of tryptone, 5 g/L of yeast extract, 3.55 g/L of disodium hydrogen phosphate,
3.4 g/L of potassium dihydrogen phosphate, 2.68 g/L of ammonium chloride, 0.71 g/L of sodium sulphate, 0.493 g/L of epsom salt, six water chlorinations
Iron 0.027 g/L, glycerol 5g/L, glucose 0.3g/L.
The present invention has the effect of positive: (1) Ketoreductase mutant of the invention has apparent high specific enzyme activity, than open country
Raw type ketoreductase improves 2-20 times, and 4- chloroacetyl acetacetic ester can be converted into (S) -4- chloro-3-hydroxyl using the enzyme
Ethyl butyrate;(2) reaction condition of the present invention is mild, low for equipment requirements, and production process is not necessarily to high temperature or cooling, and low energy consumption,
Since enzymatic has efficiently, single-minded selectivity, therefore the chloro- 3- hydroxyl of statins key intermediate (S) -4- is produced in this way
Base ethyl butyrate no coupling product generates, and purifying is convenient;(3) reacting most solvents is water, and three waste discharge is low, environmentally protective.
Specific embodiment
Embodiment 1 constructs wild type and Ketoreductase mutant engineering bacteria
It will be from the polynucleotides of the encoding wild type ketoreductase of Kefir grains lactobacillus (Lactobacillus kefir)
(SEQ ID NO:1) sequence optimisation is carried out according to bacterial strain DH1 codon preference after (see Puigb ò P, Guzm á n E,
Romeu A, Garcia-Vallvé S. OPTIMIZER: a web server for optimizing the codon
Usage of DNA sequences. Nucleic Acids Res. 2007), pass through the full genome synthesis mode of based on PCR
(PCR-based gene synthesis method) carries out gene chemical synthesis.By the multicore glycosides of the coding ketoreductase after optimization
Acid is cloned under the control of the promoter of expression vector (SEQ ID NO. 5), obtains the matter that can express wild type ketoreductase
Grain.Gained plasmid is transformed by standard method in Escherichia coli DH1.Cloning process used is the mode of homologous recombination, institute
The amplimer used are as follows:
F:5'ATTAAAGAGGAGAAATTAACATATGACTGATCGTTTAAAAGGCAAAG 3';
R:5'AACAGGAGTCCAAGCTCAGCTTATTATTGAGCAGTGTATCCACCATCG 3'.
Similar, the polynucleotides for encoding Ketoreductase mutant (SEQ ID NO:3) are cloned into expression vector (SEQ
ID NO. 5) promoter control under, obtain the plasmid that can express Ketoreductase mutant.Gained plasmid is passed through into standard
Method is transformed into Escherichia coli DH1.
The preparation of 2 ketoreductase of embodiment
Picking, which contains, has the Escherichia coli DH1 single colonie of purpose expression vector to be inoculated in the culture medium after 10ml high pressure sterilization
In: 10 g/L of tryptone, 5 g/L of yeast extract, 3.55 g/L of disodium hydrogen phosphate, 3.4 g/L of potassium dihydrogen phosphate, chlorination
2.68 g/L of ammonium, 0.71 g/L of sodium sulphate, 0.493 g/L of epsom salt, Iron trichloride hexahydrate 0.027 g/L, glycerol 5g/L, Portugal
Grape sugar 0.8g/L adds ampicillin to 100mg/L after sterilizing.30 DEG C, 250rpm is incubated overnight.Next day takes 1L triangular flask,
In culture medium after being linked into 100ml high pressure sterilization by the inoculative proportion of 1:100: 10 g/L of tryptone, yeast extract 5
G/L, 3.55 g/L of disodium hydrogen phosphate, 3.4 g/L of potassium dihydrogen phosphate, 2.68 g/L of ammonium chloride, 0.71 g/L of sodium sulphate, seven water sulphur
Sour 0.493 g/L of magnesium, Iron trichloride hexahydrate 0.027 g/L, glycerol 5g/L, glucose 0.3g/L.Kanamycins is added extremely after sterilizing
50mg/L.Triangular flask is placed in 25 DEG C of shaking tables, 250rpm cultivates 1h by culture at once to thallus OD 5-6 in 30 DEG C.It is added
IPTG to final concentration 0.1mM, and in 25 DEG C, 250rpm continues to cultivate 15h.
After culture, 20min is centrifuged by culture solution in 4 DEG C, under 6000g and finally obtains wet thallus 3.6g.Then it will sink
Twice, collect thallus wash with distilled water in shallow lake.It is resuspended again with distilled water, clarification is crushed under Ultrasonic Cell Disruptor.After broken
It is centrifuged 30min under 4 DEG C, 12000g, collects supernatant, prepares freeze-dried powder with freeze drier after being cooled to -70 DEG C in advance.It finally obtains
Thick 0. 39g of enzyme freeze-dried powder.
The active measurement of 3 ketoreductase of embodiment
Since NADPH has an absorption peak at 340nm, and NADP at 340nm without absorption peak, therefore can be reacted by detection
The variation of NADPH light absorption value in journey, and calculate the activity of ketoreductase.Ketoreductase vitality test system are as follows: take 100ul appropriate
The enzyme solution of concentration is added to final concentration of 100mM pH7.0 Triethanolamine buffer, 1g/L NADP, 50% isopropanol, 1mM sulphur
It is reacted in sour magnesium reaction system.Before enzyme solution is added, need first to mix well reaction system to be placed in 25 DEG C of water-baths.It will
Implement to take in 100ul addition reaction system after the ketoreductase dry powder for preparing dilute in appropriate proportion in 2, after mixing in
Absorbance change value per minute is detected at 340nm.The enzyme activity of ketoreductase is calculated referring to NADPH standard curve.Unit enzyme activity
(U) it is defined as generating enzyme amount required for 1 μm of ol NADP per minute.With the enzyme activity of same method detection wild type ketoreductase.
For the albumen of phase homogenous quantities, improved Ketoreductase mutant improves 18 times than wild type ketoreductase enzyme activity.
Particular embodiments described above has carried out further in detail the purpose of the present invention, technical scheme and beneficial effects
It describes in detail bright, it should be understood that the above is only a specific embodiment of the present invention, is not intended to restrict the invention, it is all
Within the spirit and principles in the present invention, any modification, equivalent substitution, improvement and etc. done should be included in guarantor of the invention
Within the scope of shield.
SEQUENCE LISTING
<110>Nanjing Lang En Biotechnology Co., Ltd
<120>for producing the Ketoreductase mutant of (S) -4- chloro-3-hydroxyl ethyl butyrate
<130> 2013
<160> 5
<170> PatentIn version 3.3
<210> 1
<211> 759
<212> DNA
<213>Kefir grains lactobacillus (Lactobacillus kefir)
<400> 1
atgactgatc gtttaaaagg caaagtagca attgtaactg gcggtacctt gggaattggc 60
ttggcaatcg ctgataagtt tgttgaagaa ggcgcaaagg ttgttattac cggccgtcac 120
gctgatgtag gtgaaaaagc tgccaaatca atcggcggca cagacgttat ccgttttgtc 180
caacacgatg cttctgatga agccggctgg actaagttgt ttgatacgac tgaagaagca 240
tttggcccag ttaccacggt tgtcaacaat gccggaattg cggtcagcaa gagtgttgaa 300
gataccacaa ctgaagaatg gcgcaagctg ctctcagtta acttggatgg tgtcttcttc 360
ggtacccgtc ttggaatcca acgtatgaag aataaaggac tcggagcatc aatcatcaat 420
atgtcatcta tcgaaggttt tgttggtgat ccaactctgg gtgcatacaa cgcttcaaaa 480
ggtgctgtca gaattatgtc taaatcagct gccttggatt gcgctttgaa ggactacgat 540
gttcgggtta acactgttca tccaggttat atcaagacac cattggttga cgatcttgaa 600
ggggcagaag aaatgatgtc acagcggacc aagacaccaa tgggtcatat cggtgaacct 660
aacgatatcg cttggatctg tgtttacctg gcatctgacg aatctaaatt tgccactggt 720
gcagaattcg ttgtcgatgg tggatacact gctcaataa 759
<210> 2
<211> 252
<212> PRT
<213>Kefir grains lactobacillus (Lactobacillus kefir)
<400> 2
Met Thr Asp Arg Leu Lys Gly Lys Val Ala Ile Val Thr Gly Gly Thr
1 5 10 15
Leu Gly Ile Gly Leu Ala Ile Ala Asp Lys Phe Val Glu Glu Gly Ala
20 25 30
Lys Val Val Ile Thr Gly Arg His Ala Asp Val Gly Glu Lys Ala Ala
35 40 45
Lys Ser Ile Gly Gly Thr Asp Val Ile Arg Phe Val Gln His Asp Ala
50 55 60
Ser Asp Glu Ala Gly Trp Thr Lys Leu Phe Asp Thr Thr Glu Glu Ala
65 70 75 80
Phe Gly Pro Val Thr Thr Val Val Asn Asn Ala Gly Ile Ala Val Ser
85 90 95
Lys Ser Val Glu Asp Thr Thr Thr Glu Glu Trp Arg Lys Leu Leu Ser
100 105 110
Val Asn Leu Asp Gly Val Phe Phe Gly Thr Arg Leu Gly Ile Gln Arg
115 120 125
Met Lys Asn Lys Gly Leu Gly Ala Ser Ile Ile Asn Met Ser Ser Ile
130 135 140
Glu Gly Phe Val Gly Asp Pro Thr Leu Gly Ala Tyr Asn Ala Ser Lys
145 150 155 160
Gly Ala Val Arg Ile Met Ser Lys Ser Ala Ala Leu Asp Cys Ala Leu
165 170 175
Lys Asp Tyr Asp Val Arg Val Asn Thr Val His Pro Gly Tyr Ile Lys
180 185 190
Thr Pro Leu Val Asp Asp Leu Glu Gly Ala Glu Glu Met Met Ser Gln
195 200 205
Arg Thr Lys Thr Pro Met Gly His Ile Gly Glu Pro Asn Asp Ile Ala
210 215 220
Trp Ile Cys Val Tyr Leu Ala Ser Asp Glu Ser Lys Phe Ala Thr Gly
225 230 235 240
Ala Glu Phe Val Val Asp Gly Gly Tyr Thr Ala Gln
245 250
<210> 3
<211> 759
<212> DNA
<213>artificial sequence
<400> 3
atgaccgacc gtctgaaagg taaagttgct atcgttaccg gtggtaccct gggtatcggt 60
ctggctatcg ctgacaaatt cgttgaagaa ggtgctaaag ttgttatcac cggtcgtcac 120
gctgacgttg gtgaaaaagc tgctaaatct atcggtggta ccgacgttat ccgtttcgtt 180
cagcacgacg cttctgacga agctggttgg accaaactgt tcgacaccac cgaagaagct 240
ttcggtccgg ttaccaccgt tgttaacaac gctggtatct ctgtttctaa atctgttgaa 300
gacaccacca ccgaagaatg gcgtaaactg ctgtctgtta acctggacgg tgttttcttc 360
ggtacccgtc tgggtatcca gcgtatgaaa aacaaaggtc tgggtgcttc tatcatcaac 420
atgtcttcta tcgaaggtgt tgttggtgac ccgaccctgg gtgcttacaa cgcttctaaa 480
ggtgctgttc gtatcatgtc taaatctgct gctctggact gcgctctgaa agactacgac 540
gttcgtgtta acaccgttca cccgggttac atcaaaaccc cgctggttga cgacccggaa 600
ggtgttgaag aaatgatgtc tcagcgtacc aaaaccccga tgggtcacat cggtgaaccg 660
aacgacatcg cttggatctg cgtttacctg gcttctgacg aatctaaatt cgctaccggt 720
gctgaattcg ttgttgacgg tggttacacc gctcagtaa 759
<210> 4
<211> 252
<212> PRT
<213>artificial sequence
<400> 4
Met Thr Asp Arg Leu Lys Gly Lys Val Ala Ile Val Thr Gly Gly Thr
1 5 10 15
Leu Gly Ile Gly Leu Ala Ile Ala Asp Lys Phe Val Glu Glu Gly Ala
20 25 30
Lys Val Val Ile Thr Gly Arg His Ala Asp Val Gly Glu Lys Ala Ala
35 40 45
Lys Ser Ile Gly Gly Thr Asp Val Ile Arg Phe Val Gln His Asp Ala
50 55 60
Ser Asp Glu Ala Gly Trp Thr Lys Leu Phe Asp Thr Thr Glu Glu Ala
65 70 75 80
Phe Gly Pro Val Thr Thr Val Val Asn Asn Ala Gly Ile Ser Val Ser
85 90 95
Lys Ser Val Glu Asp Thr Thr Thr Glu Glu Trp Arg Lys Leu Leu Ser
100 105 110
Val Asn Leu Asp Gly Val Phe Phe Gly Thr Arg Leu Gly Ile Gln Arg
115 120 125
Met Lys Asn Lys Gly Leu Gly Ala Ser Ile Ile Asn Met Ser Ser Ile
130 135 140
Glu Gly Val Val Gly Asp Pro Thr Leu Gly Ala Tyr Asn Ala Ser Lys
145 150 155 160
Gly Ala Val Arg Ile Met Ser Lys Ser Ala Ala Leu Asp Cys Ala Leu
165 170 175
Lys Asp Tyr Asp Val Arg Val Asn Thr Val His Pro Gly Tyr Ile Lys
180 185 190
Thr Pro Leu Val Asp Asp Pro Glu Gly Val Glu Glu Met Met Ser Gln
195 200 205
Arg Thr Lys Thr Pro Met Gly His Ile Gly Glu Pro Asn Asp Ile Ala
210 215 220
Trp Ile Cys Val Tyr Leu Ala Ser Asp Glu Ser Lys Phe Ala Thr Gly
225 230 235 240
Ala Glu Phe Val Val Asp Gly Gly Tyr Thr Ala Gln
245 250
<210> 5
<211> 3390
<212> DNA
<213>artificial sequence
<400> 5
ctcgagaaat cataaaaaat ttatttgctt tgtgagcgga taacaattat aatatgtgga 60
attgtgagcg ctcacaattc cacagaattc attaaagagg agaaattaac atatgaagct 120
taattagctg agcttggact cctgttgata gatccagtaa tgacctcaga actccatctg 180
gatttgttca gaacgctcgg ttgccgccgg gcgtttttta ttggtgagaa tccaagctag 240
cttggcgaga ttttcaggag ctaaggaagc taaaatggag aaaaaaatca ctggatatac 300
caccgttgat atatcccaat ggcatcgtaa agaacatttt gaggcatttc agtcagttgc 360
tcaatgtacc tataaccaga ccgttcagct ggatattacg gcctttttaa agaccgtaaa 420
gaaaaataag cacaagtttt atccggcctt tattcacatt cttgcccgcc tgatgaatgc 480
tcatccggaa tttcgtatgg caatgaaaga cggtgagctg gtgatatggg atagtgttca 540
cccttgttac accgttttcc atgagcaaac tgaaacgttt tcatcgctct ggagtgaata 600
ccacgacgat ttccggcagt ttctacacat atattcgcaa gatgtggcgt gttacggtga 660
aaacctggcc tatttcccta aagggtttat tgagaatatg tttttcgtct cagccaatcc 720
ctgggtgagt ttcaccagtt ttgatttaaa cgtggccaat atggacaact tcttcgcccc 780
cgttttcacc atgggcaaat attatacgca aggcgacaag gtgctgatgc cgctggcgat 840
tcaggttcat catgccgttt gtgatggctt ccatgtcggc agaatgctta atgaattaca 900
acagtactgc gatgagtggc agggcggggc gtaatttttt taaggcagtt attggtgccc 960
ttaaacgcct ggggtaatga ctctctagct tgaggcatca aataaaacga aaggctcagt 1020
cgaaagactg ggcctttcgt tttatctgtt gtttgtcggt gaacgctctc ctgagtagga 1080
caaatccgcc ctctagagct gcctcgcgcg tttcggtgat gacggtgaaa acctctgaca 1140
catgcagctc ccggagacgg tcacagcttg tctgtaagcg gatgccggga gcagacaagc 1200
ccgtcagggc gcgtcagcgg gtgttggcgg gtgtcggggc gcagccatga cccagtcacg 1260
tagcgatagc ggagtgtata ctggcttaac tatgcggcat cagagcagat tgtactgaga 1320
gtgcaccata tgcggtgtga aataccgcac agatgcgtaa ggagaaaata ccgcatcagg 1380
cgctcttccg cttcctcgct cactgactcg ctgcgctcgg tcgttcggct gcggcgagcg 1440
gtatcagctc actcaaaggc ggtaatacgg ttatccacag aatcagggga taacgcagga 1500
aagaacatgt gagcaaaagg ccagcaaaag gccaggaacc gtaaaaaggc cgcgttgctg 1560
gcgtttttcc ataggctccg cccccctgac gagcatcaca aaaatcgacg ctcaagtcag 1620
aggtggcgaa acccgacagg actataaaga taccaggcgt ttccccctgg aagctccctc 1680
gtgcgctctc ctgttccgac cctgccgctt accggatacc tgtccgcctt tctcccttcg 1740
ggaagcgtgg cgctttctca tagctcacgc tgtaggtatc tcagttcggt gtaggtcgtt 1800
cgctccaagc tgggctgtgt gcacgaaccc cccgttcagc ccgaccgctg cgccttatcc 1860
ggtaactatc gtcttgagtc caacccggta agacacgact tatcgccact ggcagcagcc 1920
actggtaaca ggattagcag agcgaggtat gtaggcggtg ctacagagtt cttgaagtgg 1980
tggcctaact acggctacac tagaaggaca gtatttggta tctgcgctct gctgaagcca 2040
gttaccttcg gaaaaagagt tggtagctct tgatccggca aacaaaccac cgctggtagc 2100
ggtggttttt ttgtttgcaa gcagcagatt acgcgcagaa aaaaaggatc tcaagaagat 2160
cctttgatct tttctacggg gtctgacgct cagtggaacg aaaactcacg ttaagggatt 2220
ttggtcatga gattatcaaa aaggatcttc acctagatcc ttttaaatta aaaatgaagt 2280
tttaaatcaa tctaaagtat atatgagtaa acttggtctg acagttacca atgcttaatc 2340
agtgaggcac ctatctcagc gatctgtcta tttcgttcat ccatagttgc ctgactcccc 2400
gtcgtgtaga taactacgat acgggagggc ttaccatctg gccccagtgc tgcaatgata 2460
ccgcgagacc cacgctcacc ggctccagat ttatcagcaa taaaccagcc agccggaagg 2520
gccgagcgca gaagtggtcc tgcaacttta tccgcctcca tccagtctat taattgttgc 2580
cgggaagcta gagtaagtag ttcgccagtt aatagtttgc gcaacgttgt tgccattgct 2640
acaggcatcg tggtgtcacg ctcgtcgttt ggtatggctt cattcagctc cggttcccaa 2700
cgatcaaggc gagttacatg atcccccatg ttgtgcaaaa aagcggttag ctccttcggt 2760
cctccgatcg ttgtcagaag taagttggcc gcagtgttat cactcatggt tatggcagca 2820
ctgcataatt ctcttactgt catgccatcc gtaagatgct tttctgtgac tggtgagtac 2880
tcaaccaagt cattctgaga atagtgtatg cggcgaccga gttgctcttg cccggcgtca 2940
atacgggata ataccgcgcc acatagcaga actttaaaag tgctcatcat tggaaaacgt 3000
tcttcggggc gaaaactctc aaggatctta ccgctgttga gatccagttc gatgtaaccc 3060
actcgtgcac ccaactgatc ttcagcatct tttactttca ccagcgtttc tgggtgagca 3120
aaaacaggaa ggcaaaatgc cgcaaaaaag ggaataaggg cgacacggaa atgttgaata 3180
ctcatactct tcctttttca atattattga agcatttatc agggttattg tctcatgagc 3240
ggatacatat ttgaatgtat ttagaaaaat aaacaaatag gggttccgcg cacatttccc 3300
cgaaaagtgc cacctgacgt ctaagaaacc attattatca tgacattaac ctataaaaat 3360
aggcgtatca cgaggccctt tcgtcttcac 3390
Claims (7)
1. the Ketoreductase mutant for producing (S) -4- chloro-3-hydroxyl ethyl butyrate, which is characterized in that the mutant
Amino acid sequence be SEQ ID NO.4.
2. described in claim 1 for producing the coding base of the Ketoreductase mutant of (S) -4- chloro-3-hydroxyl ethyl butyrate
Cause.
3. encoding gene according to claim 2, which is characterized in that the sequence of the gene is SEQ ID NO.3.
4. containing the recombinant plasmid of encoding gene as claimed in claim 2.
5. the host cell containing recombinant plasmid described in claim 4.
6. the Ketoreductase mutant described in claim 1 for producing (S) -4- chloro-3-hydroxyl ethyl butyrate is producing
(S) application in -4- chloro-3-hydroxyl-ethyl butyrate.
7. a kind of production (S) -4- chloro-3-hydroxyl-ethyl butyrate method, which is characterized in that the method is with 4- chloracetyl
Ethyl acetate is substrate, under the catalytic action of the mutant described in claim 1, obtains (S) -4- chloro-3-hydroxyl-butyric acid second
Ester.
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| CN109055324B (en) * | 2018-07-10 | 2021-05-04 | 天津迪沙医药技术开发有限公司 | Improved ketoreductase and application thereof |
| CN109943542B (en) * | 2018-12-29 | 2022-07-12 | 南京诺云生物科技有限公司 | Alcohol dehydrogenase for producing atazanavir intermediate |
| CN110093302B (en) * | 2019-06-13 | 2020-08-28 | 浙江华睿生物技术有限公司 | Lactobacillus mutant strain and application thereof |
| KR20220066952A (en) * | 2019-09-26 | 2022-05-24 | 코덱시스, 인코포레이티드 | Ketoductase Polypeptides and Polynucleotides |
| CN110923277B (en) * | 2019-12-27 | 2021-05-11 | 南京朗恩生物科技有限公司 | Method for preparing S-3-dimethylamino-1- (2-thienyl) -1-propanol by biocatalysis |
| CN111593077B (en) * | 2019-12-30 | 2021-10-01 | 南京朗恩生物科技有限公司 | Method for preparing (R) -4-chloro-3-hydroxy ethyl butyrate through biocatalysis |
| CN112522334A (en) * | 2020-11-30 | 2021-03-19 | 江苏阿尔法药业有限公司 | Synthesis method of (R) -4-cyano-3-hydroxy ethyl butyrate |
| CN112941115A (en) * | 2021-03-30 | 2021-06-11 | 宿迁盛基医药科技有限公司 | Preparation method of ticagrelor chiral intermediate |
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