CN107805622B - Recombinant bacillus subtilis for synthesizing guanosine diphosphate rock sugar and construction method and application thereof - Google Patents

Recombinant bacillus subtilis for synthesizing guanosine diphosphate rock sugar and construction method and application thereof Download PDF

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CN107805622B
CN107805622B CN201711092675.3A CN201711092675A CN107805622B CN 107805622 B CN107805622 B CN 107805622B CN 201711092675 A CN201711092675 A CN 201711092675A CN 107805622 B CN107805622 B CN 107805622B
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bacillus subtilis
recombinant bacillus
guanosine diphosphate
fucose
recombinant
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CN107805622A (en
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刘龙
陈坚
堵国成
邓洁莹
陈春梅
李江华
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Bright Dairy and Food Co Ltd
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    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K14/00Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
    • C07K14/195Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from bacteria
    • C07K14/32Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from bacteria from Bacillus (G)
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    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N9/00Enzymes; Proenzymes; Compositions thereof; Processes for preparing, activating, inhibiting, separating or purifying enzymes
    • C12N9/10Transferases (2.)
    • C12N9/12Transferases (2.) transferring phosphorus containing groups, e.g. kinases (2.7)
    • C12N9/1205Phosphotransferases with an alcohol group as acceptor (2.7.1), e.g. protein kinases
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    • C12N9/00Enzymes; Proenzymes; Compositions thereof; Processes for preparing, activating, inhibiting, separating or purifying enzymes
    • C12N9/10Transferases (2.)
    • C12N9/12Transferases (2.) transferring phosphorus containing groups, e.g. kinases (2.7)
    • C12N9/1241Nucleotidyltransferases (2.7.7)
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    • C12PFERMENTATION OR ENZYME-USING PROCESSES TO SYNTHESISE A DESIRED CHEMICAL COMPOUND OR COMPOSITION OR TO SEPARATE OPTICAL ISOMERS FROM A RACEMIC MIXTURE
    • C12P19/00Preparation of compounds containing saccharide radicals
    • C12P19/26Preparation of nitrogen-containing carbohydrates
    • C12P19/28N-glycosides
    • C12P19/30Nucleotides
    • C12P19/32Nucleotides having a condensed ring system containing a six-membered ring having two N-atoms in the same ring, e.g. purine nucleotides, nicotineamide-adenine dinucleotide
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    • C12YENZYMES
    • C12Y207/00Transferases transferring phosphorus-containing groups (2.7)
    • C12Y207/01Phosphotransferases with an alcohol group as acceptor (2.7.1)
    • C12Y207/01052Fucokinase (2.7.1.52)
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    • C12Y207/00Transferases transferring phosphorus-containing groups (2.7)
    • C12Y207/07Nucleotidyltransferases (2.7.7)
    • C12Y207/0703Fucose-1-phosphate guanylyltransferase (2.7.7.30)

Abstract

The invention provides a recombinant bacillus subtilis for synthesizing guanosine diphosphate fucose, a construction method and application thereof, wherein the recombinant bacillus subtilis is obtained by enhancing expression of a sugar transporter gene of bacillus subtilis 168 and expressing exogenous fucokinase and phosphoguanyltransferase genes. The invention obtains the strain capable of efficiently synthesizing the guanosine diphosphate fucose by modifying the bacillus subtilis 168, and the intracellular accumulation amount of the strain is up to 156 mg/L. The invention can effectively strengthen the expression of the sugar transport protein by strengthening and expressing the sugar transport protein gene, improves the efficiency of transferring exogenous fucose into cells, increases the concentration of intracellular fucose and promotes the synthesis of guanosine diphosphate rock fucose. The recombinant bacillus subtilis has the advantages of simple construction method, convenient use and good application prospect.

Description

Recombinant bacillus subtilis for synthesizing guanosine diphosphate rock sugar and construction method and application thereof
Technical Field
The invention belongs to the technical field of genetic engineering, and particularly relates to recombinant bacillus subtilis for synthesizing guanosine diphosphate fucose, and a construction method and application thereof.
Background
The breast milk contains important nutrients, bioactive substances and factors for stimulating the growth of intestinal flora. Wherein, the breast milk oligosaccharide(Human Milk Oligosacchrides, hMOs) play key roles in many physiological functions, such as promotion of bifidobacterial growth, inhibition of pathogen infection, and enhancement of immune responses. Among the human milk oligosaccharides, the Fucosylated Oligosaccharides (FOSs) have received great attention for their physiological functions such as their ability to act as receptor analogs for enteropathogenic bacteria, ability to promote immune regulation, and ability to reduce inflammation. Since fucosylated oligosaccharides are produced by fucosylation of saccharides catalyzed by fucosyltransferase, guanosine diphosphate fucose (GDP-L-fucose) is required as a donor of fucosyl. As fucosylated oligosaccharides get hotter, many pharmaceutical companies try to synthesize sufficient GDP-L-fucose by chemical and biological methods. In the chemical synthesis, GDP-L-fucose takes L-fucopyranosyl tetraacetic acid as a starting material and HBr and Ag2CO3And N-tetrabutylammonium ditolyl phosphate and the like. GDP-L-fucose is a precursor of kola acid, which is a major component of cell walls of gram-negative bacteria, and thus, some enteric bacteria such as Escherichia coli and Salmonella can synthesize GDP-L-fucose in vivo. Two metabolic pathways for the synthesis of GDP-L-fucose are found in organisms: the salvage route and the de novo route.
The salvage pathway is found in the human metabolic pathway, exogenous fucose is transferred into the cell, and ATP is consumed by fucose kinase and phosphorylated (EC 2.7.1.52) to form fucose-1-phosphate (Fuc-1-P). The Fuc-1-P bound Guanosine Triphosphate (GTP) is catalyzed by fucose-1-phosphate guanylyltransferase (L-fucose-1-phosphate guanylyltransferase) (EC 2.7.7.30) to produce GDP-L-fucose. The de novo synthetic pathway is ubiquitous in prokaryotes and eukaryotes, where GDP-L-fucose is catalytically synthesized from GDP-mannose by mannose dehydrogenase (GMD, EC 4.2.1.47) and GDP-fucose synthetase (WCAG, EC 1.1.1.271). A representative reaction method is shown in FIG. 2.
Bacillus subtilis is a production host widely used as food enzyme preparation and important nutritional chemicals, and the product is certified as "general regulated as safe" (GRAS) level by FDA.
Therefore, how to utilize the bacillus subtilis to synthesize the guanosine diphosphate fucose efficiently by a biological method still remains a problem to be solved in the field.
Disclosure of Invention
In order to solve the technical problems, the invention aims to provide the recombinant bacillus subtilis for synthesizing the guanosine diphosphate fucose, and the construction method and the application thereof.
Specifically, in one aspect, the invention provides a recombinant bacillus subtilis for synthesizing guanosine diphosphate fucose, wherein the recombinant bacillus is obtained by enhancing expression of a sugar transport protein gene of bacillus subtilis 168 and expressing exogenous fucokinase and phosphoguanyltransferase genes.
The sugar transporter gene of the bacillus subtilis 168 is not expressed, and the efficiency of transferring exogenous fucose into cells is improved, the concentration of intracellular fucose is increased and the synthesis of guanosine diphosphate fucose is promoted by enhancing the expression of the sugar transporter gene of the bacillus subtilis 168 and expressing exogenous fucokinase and phosphoguanyltransferase genes.
Wherein the promoter of the sugar transporter gene of Bacillus subtilis 168 is replaced by a strong promoter P43 to enhance expression of the sugar transporter gene of Bacillus subtilis 168. The strong promoter P43 strengthens and expresses the sugar transporter gene of the bacillus subtilis 168, effectively strengthens the expression of the sugar transporter, improves the efficiency of transferring exogenous fucose into cells, and increases the concentration of intracellular fucose.
The sugar transporter Gene is shown as Gene ID:936346 in NCBI.
Preferably, the fucose kinase and guanine phosphate transferase genes are fkp genes of Bacteroides fragilis 9343. The fkp gene of Bacteroides fragilis 9343 is shown in GenBank: AY849806.1 at NCBI.
In a second aspect, the invention also provides a construction method of the recombinant bacillus subtilis for synthesizing the guanosine diphosphate fucose, and the construction method comprises the following steps:
(1) constructing a substitution frame containing an upstream and downstream sequence of a sugar transporter gene, a P43 promoter and a bleomycin resistance gene sequence, transforming the constructed substitution frame into recombinant bacillus subtilis 168, and confirming that the sugar transporter gene is successfully expressed in a strengthened manner through verification to obtain recombinant bacillus subtilis BSG;
(2) constructing a recombinant plasmid containing fucokinase and guanine phosphate transferase genes, transforming the constructed recombinant plasmid into bacillus subtilis BSG, and confirming the successful expression of the fucokinase and the guanine phosphate transferase through verification to obtain the recombinant bacillus subtilis BSGF.
Preferably, in step (1), the sequence of the substitution box is shown as SEQ ID NO. 1.
In the step (2), the sequence of the recombinant plasmid is shown as SEQ ID NO. 2.
In a third aspect, the invention also provides an application of the recombinant bacillus subtilis, and the recombinant bacillus subtilis is used for fermenting to generate guanosine diphosphate fucose.
Preferably, the fermentation is to inoculate the recombinant bacillus seed liquid into the fermentation medium with the OD value of 0.1-0.3, and culture the recombinant bacillus seed liquid for 20-25h under the conditions of 35-40 ℃ and 200-250 rpm.
The invention has the beneficial effects that:
the recombinant bacillus subtilis is obtained by enhancing expression of a sugar transporter gene on the basis of bacillus subtilis 168 and expressing fucokinase and phosphoguanyltransferase genes on the basis, and a strain capable of efficiently synthesizing and synthesizing guanosine diphosphate fucose is obtained by modification, wherein the intracellular accumulation amount of the strain is up to 156 mg/L. The invention effectively strengthens the expression of the sugar transport protein by strengthening and expressing the sugar transport protein gene, improves the efficiency of transferring exogenous fucose into cells, increases the concentration of intracellular fucose and promotes the synthesis of guanosine diphosphate rock sugar. The recombinant bacillus subtilis has a simple construction method, is convenient to use and has a good application prospect.
Drawings
FIG. 1 is a GC-MS chromatogram of guanosine diphosphate fucose obtained in example 3 of the present invention.
FIG. 2 is a prior art scheme for the de novo synthesis of guanosine diphosphate fucose.
Detailed Description
The present invention will be explained in detail below with reference to examples and the accompanying drawings.
Example 1
Enhanced expression of the sugar transporter gene glcP
The substitution cassette having a sequence shown in SEQ ID NO.1 was constructed based on the upstream and downstream sequences of the sugar transporter gene glcP, the P43 promoter, and the bleomycin resistance gene of Bacillus subtilis (Bacillus subtilis 168 available from American type culture Collection, ATCC No.27370) published on NCBI.
Electrically transforming competent cells of the bacillus subtilis 168 by using the constructed replacement frame, wherein the addition amount of the replacement frame is 100-300ng, and the electrical transformation conditions are as follows: the voltage is 2.5kV, the electric shock reagent is 5ms, the mixture is revived at 37 ℃ for 5h and coated with LB plates with the final concentration of 10 mug/mL bleomycin resistance, the mixture is anaerobically cultured at 37 ℃ for 48h, and a plurality of monoclonals are selected.
Since the upstream and downstream sequences of the sugar transporter gene glcP exist in the substitution cassette, which is homologous to the transporter gene of Bacillus subtilis 168, the P43 promoter in the substitution cassette replaces the promoter of the sugar transporter gene glcP of Bacillus subtilis 168 by homologous recombination.
Screening by a bleomycin resistance plate, carrying out colony PCR verification, and sequencing to confirm whether the sugar transporter gene (glcP) is successfully expressed in an enhanced manner, wherein the bacteria with positive bleomycin resistance are Bacillus subtilis successfully transformed by a substitution box, the bacteria with a special band are verified by colony PCR, and the sequencing result is consistent with a theoretical result and is the Bacillus subtilis successfully transformed and recombined by the substitution box, namely the Bacillus subtilis successfully expressed in the sugar transporter gene (glcP) in an enhanced manner.
And (3) after confirming that the sugar transporter gene (glcP) intensified expression is successful, obtaining the recombinant bacillus subtilis BSG.
Example 2
Exogenous expression of Bacteroides fragilis exogenous gene
A recombinant plasmid pP43-Fkp having a sequence shown in SEQ ID NO.2 was constructed by digesting and ligating the gene fkp with the restriction enzyme site of plasmid pP43NMK based on the sequences of fucokinase and guanine phosphate group transferase genes fkp of Bacteroides fragilis (ATCC No.25285) published at NCBI.
Electrically transforming the constructed recombinant plasmid into competent cells of the recombinant bacillus subtilis BSG, wherein the addition amount of the recombinant plasmid is 50-300ng, and the electrical transformation conditions are as follows: the voltage is 2.5kV, the electric shock reagent is 5ms, the mixture is revived at 37 ℃ for 5h and coated with LB plates with 10 mug/mL kanamycin resistance, the mixture is anaerobically cultured at 37 ℃ for 48h, and a plurality of monoclonals are selected.
Screening by a kanamycin-resistant plate, carrying out colony PCR verification, and determining whether genes of the fucokinase and the guanine-phosphate transferase are successfully expressed after sequencing, wherein bacillus subtilis which is successfully transformed is positive in kanamycin resistance, special bands are formed in the colony PCR verification, and the bacillus subtilis which is successfully transformed and recombined is obtained when the sequencing result is consistent with the theoretical result, namely the fucokinase and the guanine-phosphate transferase are successfully expressed.
Confirming the successful expression of the fucokinase and the guanine-phosphate transferase of the bacteroides fragilis to obtain the recombinant bacillus subtilis BSGF.
Example 3
Production of guanosine diphosphate rock algae sugar by fermentation
Preparing the recombinant bacillus subtilis BSGF into seed liquid, wherein the formula of a seed liquid culture medium is as follows: 10g/L of tryptone and 5g/L, NaCl 10g/L of yeast powder; the preparation method of the seed liquid comprises the following steps: picking single colony on a fresh plate, and culturing for 8-10h in a seed culture medium.
Inoculating the seed liquid into a fermentation culture medium by an inoculum size with an OD value of 0.1, wherein the formula of the fermentation culture medium is as follows: 20g/L of initial glycerol, 6g/L of peptone, 12g/L of yeast powder, (NH)4)SO46g/L, K2HPO4·3H2O 12.5g/L、KH2PO42.5g/L、CaCO35g/L and 10ml/L of trace elements; the trace element solution contains in g/L: MnSO4·5H2O 1.0、CoCl2·6H2O 0.4、 NaMoO4·2H2O 0.2、ZnSO4·7H2O 0.2、AlCl3·6H2O 0.1、CuCl2·H2O 0.1、 H3BO40.05, 5mol/LHCl, at 35 ℃ and 200rpm for 20 h.
When the fermentation is finished, determining the content of the guanosine diphosphate fucose in the fermentation supernatant by using a gas chromatograph, wherein a gas chromatograph of the guanosine diphosphate fucose is shown in figure 1, and the determined content of the guanosine diphosphate fucose reaches 156 mg/L.
Example 4
Production of guanosine diphosphate rock algae sugar by fermentation
Preparing the recombinant bacillus subtilis BSGF into seed liquid, wherein the formula of a seed culture medium is as follows: 10g/L of tryptone and 5g/L, NaCl 10g/L of yeast powder; the preparation method of the seed liquid comprises the following steps: selecting single colony on fresh plate, and culturing in seed culture medium for 8-10 hr.
Inoculating the seed liquid into a fermentation culture medium by an inoculum size with an OD value of 0.3, wherein the formula of the fermentation culture medium is as follows: 20g/L of initial glycerol, 6g/L of peptone, 12g/L of yeast powder, (NH)4)SO46g/L, K2HPO4·3H2O 12.5g/L、KH2PO42.5g/L、CaCO35g/L and 10ml/L of trace elements; the trace element solution contains in g/L: MnSO4·5H2O 1.0、CoCl2·6H2O 0.4、 NaMoO4·2H2O 0.2、ZnSO4·7H2O 0.2、AlCl3·6H2O 0.1、CuCl2·H2O 0.1、 H3BO40.05, 5mol/LHCl, at 40 ℃ and 250rpm for 25 h.
When the fermentation is finished, the content of the guanosine diphosphate fucose in the fermentation supernatant reaches 154 mg/L.
Comparative example 1
The substitution cassette having a sequence shown in SEQ ID NO.1 was constructed based on the upstream and downstream sequences of the sugar transporter gene glcP, the P43 promoter, and the bleomycin resistance gene of Bacillus subtilis (Bacillus subtilis 168 available from American type culture Collection, ATCC No.27370) published on NCBI.
Electrically transforming competent cells of bacillus subtilis 168 by using the constructed replacement frame, wherein the addition amount of the replacement frame is 50-300ng, and the electrical transformation conditions are as follows: the voltage is 2.5kV, the electric shock reagent is 5ms, the mixture is revived at 37 ℃ for 5h and coated with LB plates with the final concentration of 10 mug/mL bleomycin resistance, the mixture is anaerobically cultured at 37 ℃ for 48h, and a plurality of monoclonals are selected.
Since the upstream and downstream sequences of the sugar transporter gene glcP exist in the substitution cassette, which is homologous to the transporter gene of Bacillus subtilis 168, the P43 promoter in the substitution cassette replaces the promoter of the sugar transporter gene glcP of Bacillus subtilis 168 by homologous recombination.
Screening by a bleomycin resistance plate, carrying out colony PCR verification, and sequencing to confirm whether the sugar transporter gene (glcP) is successfully expressed in an enhanced manner, wherein the bacteria with positive bleomycin resistance are Bacillus subtilis successfully transformed by a substitution box, the bacteria with a special band are verified by colony PCR, and the sequencing result is consistent with a theoretical result and is the Bacillus subtilis successfully transformed and recombined by the substitution box, namely the Bacillus subtilis successfully expressed in the sugar transporter gene (glcP) in an enhanced manner.
And (3) after confirming that the sugar transporter gene (glcP) intensified expression is successful, obtaining the recombinant bacillus subtilis BSG.
And (3) fermenting and producing guanosine diphosphate fucose by using the recombinant bacillus subtilis BSG, centrifuging and collecting obtained cells after fermentation is finished, and carrying out ultrasonic disruption to obtain an intracellular soluble mixed solution, wherein guanosine diphosphate fucose is not detected.
Comparative example 2
A recombinant plasmid having a sequence shown in SEQ ID NO.2 was constructed based on the sequences of fucokinase and phosphoguanyltransferase genes fkp of Bacteroides fragilis (ATCC No.25285) published at NCBI.
Electrically transforming competent cells of bacillus subtilis 168 with the constructed recombinant plasmid, wherein the addition amount of the recombinant plasmid is 50-300ng, and the electrical transformation conditions are as follows: the voltage is 2.5kV, the electric shock reagent is 5ms, the mixture is revived at 37 ℃ for 5h and coated with LB plates with 10 mug/mL kanamycin resistance, the mixture is anaerobically cultured at 37 ℃ for 48h, and a plurality of monoclonals are selected.
Screening by a kanamycin resistance plate, verifying by colony PCR, and determining whether genes of the fucokinase and the guanine phosphate transferase are successfully expressed or not after sequencing, wherein the bacillus subtilis which is successfully transformed is positive in kanamycin resistance, the bacillus subtilis which is successfully transformed is verified by colony PCR, and the bacillus subtilis which is successfully recombined in a substitution frame is verified by the sequencing result which is consistent with the theoretical result, namely the bacillus subtilis is successfully expressed by the fucokinase and the guanine phosphate transferase.
Confirming the successful expression of fucokinase and guanine-phosphate transferase of bacteroides fragilis, and obtaining the recombinant bacillus subtilis BSF.
And (3) fermenting and producing guanosine diphosphate fucose by using the recombinant bacillus subtilis BSF, centrifuging and collecting obtained cells after fermentation is finished, and carrying out ultrasonic disruption to obtain an intracellular soluble mixed solution, wherein guanosine diphosphate fucose is not detected.
The above description is only for the purpose of illustrating the preferred embodiments of the present invention and is not to be construed as limiting the invention, and any modifications, equivalents and simplifications made in the spirit of the present invention are intended to be included in the scope of the present invention.
Sequence listing
<110> Guangming Dairy milk industry Co., Ltd
<120> recombinant bacillus subtilis for synthesizing guanosine diphosphate rock sugar and construction method and application thereof
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gaaaacataa gcatgtatta tgtgaaaagc ctatggctat ttctcttgaa gaagcaagca 180
taatgaaaga tactgctgaa aggttgagcg taagagccag tatgggattt aattatagat 240
atttatctta cgtaaatatc ttaaaaagct taattatcaa taatgaacta ggtaacatac 300
tgtccataaa agtacacttc aagaaaaata gtgcacttag acgtaagaag tttacttgga 360
gagatgacgc taatagtaag aagacgagtg gatcattggg ggatctgggt attcacctta 420
ttgacatggt atggtatttg ttcgagagtg atttcatcac agaatcagta agggcaaaga 480
tgaacacaaa tgtaaaaaca aaagaggata aacaggtact tgtagatgac tatgcagaaa 540
tttatggcca gctgaagaac aaggtatttg taaatatcat cacatcaaag tgttctgtac 600
ctgaagactg tggttttagc attgaggtag ttggacacaa aaaagagttt aaataccaca 660
caggtaatcc tcacgtttac aagctcatag atggcttgaa cgtggtagac tgcccagtac 720
cgcaaagcct attaaacgat ccgccaaacg agttttatgg atgggctgat tcttttagaa 780
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gtgatggttt tagatctcag gaagtattag aaatgttctt tgagaaagac agcaactctc 900
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ggaatttact ttcctgcttt ttcatatagg ggtgtaatga gattgggatc ctctagagat 1020
tctaccgttc gtatagcata cattatacga agttatcttg atatggcttt ttatatgtgt 1080
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ctcaccgcgc gcgacgtcgc cggagcggtc gagttctgga ccgaccggct cgggttctcc 1200
cgggacttcg tggaggacga cttcgccggt gtggtccggg acgacgtgac cctgttcatc 1260
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ctggacgagc tgtacgccga gtggtcggag gtcgtgtcca cgaacttccg ggacgcctcc 1380
gggccggcca tgaccgagat cggcgagcag ccgtgggggc gggagttcgc cctgcgcgac 1440
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ggaaacctgt cgtgccagct gcattaatga atcggccaac gcgcggggag aggcggtttg 1860
cgtattgggc gccagggtgg tttttctttt caccagtgag acgggcaaca gctgattgcc 1920
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cattgcgccc agcgccatct gatcgttggc aaccagcatc gcagtgggaa cgatgccctc 2160
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cgctatcggc tgaatttgat tgcgagtgag atatttatgc cagccagcca gacgcagacg 2280
cgccgagaca gaacttaatg ggcccgctaa cagcgcgatt tgctggtgac ccaatgcgac 2340
cagatgctcc acgcccagtc gcgtaccgtc ttcatgggag aaaataatac tgttgatggg 2400
tgtctggtca gagacatcaa gaaataacgc cggaacatta gtgcaggcag cttccacagc 2460
aatggcatcc tggtcatcca gcggatagtt aatgatcagc ccactgacgc gttgcgcgag 2520
aagattgtgc accgccgttt tacaggcttc gacgccgctt cgttctacca tcgacaccac 2580
cacgctggca cccagttgat cggcgcgaga tttaatcgcc gcgacaattt gcgacggcgc 2640
gtgcagggcc agactggagg tggcaacgcc aatcagcaac gactgtttgc ccgccagttg 2700
ttgtgccacg cggttgggaa tgtaattcag ctccgccatc gccgcttcca ctttttcccg 2760
cgttttcgca gaaacgtggc tggcctggtt caccacgcgg gaaacggtct gataagagac 2820
accggcatac tctgcgacat cgtataacgt tactggtttc atcaaaatcg tctccctccg 2880
tttgaatatt tgattgatcg taaccagatg aagcactctt tccactatcc ctacagtgtt 2940
atggcttgaa caatcacgaa acaataattg gtacgtacga tctttcagcc gactcaaaca 3000
tcaaatctta caaatgtagt ctttgaaagt attacatatg taagatttaa atgcaaccgt 3060
tttttcggaa ggaaatgatg acctcgtttc caccggaatt agcttggtac caaaggaggt 3120
gaaatgtaca catgttaaga gggacatatt tatttggata tgctttcttt tttacagtag 3180
gtattatcca tatatcaaca gggagtttga caccattttt attagaggct tttaacaaga 3240
caacagatga tatttcggtc ataatcttct tccagtttac cggatttcta agcggagtat 3300
taatcgcacc tttaatgatt aagaaataca gtcattttag gacacttact ttagctttga 3360
caataatgct tgtagcgtta agtatctttt ttctaaccaa ggattggtat tatattattg 3420
taatggcttt tctcttagga tatggagcag gcacattaga aacgacagtt ggttcatttg 3480
ttattgctaa tttcgaaagt aatgcagaaa aaatgagtaa gctggaagtt ctctttggat 3540
taggcgcttt atctttccca ttattaatta attccttcat agatatcaat aactggtttt 3600
taccatatta ctgtatattc acctttttat tcgtcctatt cgtagggtgg ttaattttct 3660
tgtctaagaa ccgagagtac gctaagaatg ctaaccaaca agtgaccttt ccagatggag 3720
gagcatttca atactttata ggagatagaa aaaaatcaaa gcaattaggc ttttttgtat 3780
ttttcgcttt cctatatgct ggaattgaaa caaattttgc caacttttta ccttcaatca 3840
tgataaacca agacaatgaa caaattagtc ttataagtgt ctcctttttc tgggtaggga 3900
tcatcatagg aagaatattg attggtttcg taagtagaag gcttgatttt tccaaatacc 3960
ttctttttag ctgtagttgt ttaattgttt tgttgattgc cttctcttat ataagtaacc 4020
caatacttca attgagtggt acatttttga ttggcctaag tatagcgggg atatttccca 4080
ttgctttaac actagcatca atcattattc agaagtacgt tgacgaagtt acaagtttat 4140
ttattgcctc ggcaagtttc ggaggagcga tcatctcttt cttaattgga tggagtttaa 4200
accaggatac gatcttatta accatgggaa tatttacaac tatggcggtc attctagtag 4260
gtatttctgt aaagattagg agaactaaaa cagaagaccc tatttcactt gaaaacaaag 4320
catcaaaaac acagtag 4337
<210> 2
<211> 9577
<212> DNA
<213> Artificial sequence (unknown)
<400> 2
tcgcgcgttt cggtgatgac ggtgaaaacc tctgacacat gcagctcccg gagacggtca 60
cagcttgtct gtaagcggat gccgggagca gacaagcccg tcagggcgcg tcagcgggtg 120
ttggcgggtg tcggggctgg cttaactatg cggcatcaga gcagattgta ctgagagtgc 180
accatatgcg gtgtgaaata ccgcacagat gcgtaaggag aaaataccgc atcaggcgcc 240
attcgccatt caggctgcgc aactgttggg aagggcgatc ggtgcgggcc tcttcgctat 300
tacgccagct ggcgaaaggg ggatgtgctg caaggcgatt aagttgggta acgccagggt 360
tttcccagtc acgacgttgt aaaacgacgg ccagtgaatt ccttaaggaa cgtacagacg 420
gcttaaaagc ctttaaaaac gtttttaagg ggtttgtaga caaggtaaag gataaaacag 480
cacaattcca agaaaaacac gatttagaac ctaaaaagaa cgaatttgaa ctaactcata 540
accgagaggt aaaaaaagaa cgaagtcgag atcagggaat gagtttataa aataaaaaaa 600
gcacctgaaa aggtgtcttt ttttgatggt tttgaacttg ttctttctta tcttgataca 660
tatagaaata acgtcatttt tattttagtt gctgaaaggt gcgttgaagt gttggtatgt 720
atgtgtttta aagtattgaa aacccttaaa attggttgca cagaaaaacc ccatctgtta 780
aagttataag tgactaaaca aataactaaa tagatggggg tttcttttaa tattatgtgt 840
cctaatagta gcatttattc agatgaaaaa tcaagggttt tagtggacaa gacaaaaagt 900
ggaaaagtga gaccatggag agaaaagaaa atcgctaatg ttgattactt tgaacttctg 960
catattcttg aatttaaaaa ggctgaaaga gtaaaagatt gtgctgaaat attagagtat 1020
aaacaaaatc gtgaaacagg cgaaagaaag ttgtatcgag tgtggttttg taaatccagg 1080
ctttgtccaa tgtgcaactg gaggagagca atgaaacatg gcattcagtc acaaaaggtt 1140
gttgctgaag ttattaaaca aaagccaaca gttcgttggt tgtttctcac attaacagtt 1200
aaaaatgttt atgatggcga agaattaaat aagagtttgt cagatatggc tcaaggattt 1260
cgccgaatga tgcaatataa aaaaattaat aaaaatcttg ttggttttat gcgtgcaacg 1320
gaagtgacaa taaataataa agataattct tataatcagc acatgcatgt attggtatgt 1380
gtggaaccaa cttattttaa gaatacagaa aactacgtga atcaaaaaca atggattcaa 1440
ttttggaaaa aggcaatgaa attagactat gatccaaatg taaaagttca aatgattcga 1500
ccgaaaaata aatataaatc ggatatacaa tcggcaattg acgaaactgc aaaatatcct 1560
gtaaaggata cggattttat gaccgatgat gaagaaaaga atttgaaacg tttgtctgat 1620
ttggaggaag gtttacaccg taaaaggtta atctcctatg gtggtttgtt aaaagaaata 1680
cataaaaaat taaaccttga tgacacagaa gaaggcgatt tgattcatac agatgatgac 1740
gaaaaagccg atgaagatgg attttctatt attgcaatgt ggaattggga acggaaaaat 1800
tattttatta aagagtagtt caacaaacgg gccagtttgt tgaagattag atgctataat 1860
tgttattaaa aggattgaag gatgcttagg aagacgagtt attaatagct gaataagaac 1920
ggtgctctcc aaatattctt atttagaaaa gcaaatctaa aattatctga aaagggaatg 1980
agaatagtga atggaccaat aataatgact agagaagaaa gaatgaagat tgttcatgaa 2040
attaaggaac gaatattgga taaatatggg gatgatgtta aggctattgg tgtttatggc 2100
tctcttggtc gtcagactga tgggccctat tcggatattg agatgatgtg tgtcatgtca 2160
acagaggaag cagagttcag ccatgaatgg acaaccggtg agtggaaggt ggaagtgaat 2220
tttgatagcg aagagattct actagattat gcatctcagg tggaatcaga ttggccgctt 2280
acacatggtc aatttttctc tattttgccg atttatgatt caggtggata cttagagaaa 2340
gtgtatcaaa ctgctaaatc ggtagaagcc caaacgttcc acgatgcgat ttgtgccctt 2400
atcgtagaag agctgtttga atatgcaggc aaatggcgta atattcgtgt gcaaggaccg 2460
acaacatttc taccatcctt gactgtacag gtagcaatgg caggtgccat gttgattggt 2520
ctgcatcatc gcatctgtta tacgacgagc gcttcggtct taactgaagc agttaagcaa 2580
tcagatcttc cttcaggtta tgaccatctg tgccagttcg taatgtctgg tcaactttcc 2640
gactctgaga aacttctgga atcgctagag aatttctgga atgggattca ggagtggaca 2700
gaacgacacg gatatatagt ggatgtgtca aaacgcatac cattttgaac gatgacctct 2760
aataattgtt aatcatgttg gttacgtatt tattaacttc tcctagtatt agtaattatc 2820
atggctgtca tggcgcatta acggaataaa gggtgtgctt aaatcgggcc attttgcgta 2880
ataagaaaaa ggattaatta tgagcgaatt gaattaataa taaggtaata gatttacatt 2940
agaaaatgaa aggggatttt atgcgtgaga atgttacagt ctatcccggc attgccagtc 3000
ggggatatta aaaagagtat aggtttttat tgggataaag taggtttcac tttggttcac 3060
catgaagatg gattcgcagt tctaatgtgt aatgaggttc ggattcatct atgggaggca 3120
agtgatgaag gctggcgcct cgtagtaatg attcaccggt ttgtacaggt gcggagtcgt 3180
ttattgctgg tactgctagt tgccgcattg aagtagaggg aattgatgaa ttatatcaac 3240
atattaagcc tttgggcatt ttgcacccca atacatcatt aaaagatcag tggtgggatg 3300
aacgagactt tgcagtaatt gatcccgaca acaatttgat tagctttttt caacaaataa 3360
aaagctaaaa tctattatta atctgttcag caatcgggcg cgattgctga ataaaagata 3420
cgagagacct ctcttgtatc ttttttattt tgagtggttt tgtccgttac actagaaaac 3480
cgaaagacaa taaaaatttt attcttgctg agtctggctt tcggtaagct agacaaaacg 3540
gacaaaataa aaattggcaa gggtttaaag gtggagattt tttgagtgat cttctcaaaa 3600
aatactacct gtcccttgct gatttttaaa cgagcacgag agcaaaaccc ccctttgctg 3660
aggtggcaga gggcaggttt ttttgtttct tttttctcgt aaaaaaaaga aaggtcttaa 3720
aggttttatg gttttggtcg gcactgccgc gcctcgcaga gcacacactt tatgaatata 3780
aagtatagtg tgttatactt tacttggaag tggttgccgg aaagagcgaa aatgcctcac 3840
atttgtgcca cctaaaaagg agcgatttac atatgagtta tgcagtttgt agaatgcaaa 3900
aagtgaaatc agctggacta aaaggcatgc aatttcataa tcaaagagag cgaaaaagta 3960
gaacgaatga tgatattgac catgagcgaa cacgtgaaaa ttatgatttg aaaaatgata 4020
aaaatattga ttacaacgaa cgtgtcaaag aaattattga atcacaaaaa acaggtacaa 4080
gaaaaacgag gaaagatgct gttcttgtaa atgagttgct agtaacatct gaccgagatt 4140
tttttgagca actggatcct gataggtggt atgttttcgc ttgaactttt aaatacagcc 4200
attgaacata cggttgattt aataactgac aaacatcacc ctcttgctaa agcggccaag 4260
gacgctgccg ccggggctgt ttgcgttttt gccgtgattt cgtgtatcat tggtttactt 4320
atttttttgc caaagctgta atggctgaaa attcttacat ttattttaca tttttagaaa 4380
tgggcgtgaa aaaaagcgcg cgattatgta aaatataaag tgatagcggt accgagctca 4440
aaggaggtga aatgtacaca tgcaaaagtt actgtctctc ccatctaact tagtccagag 4500
ctttcatgaa ttagaaagag taaatcggac tgactggttt tgcacatccg acccggtcgg 4560
aaaaaagctt ggcagtggcg gtggcacatc atggctgctc gaggaatgct ataatgaata 4620
ctctgacggc gcaactttcg gagagtggct cgaaaaagag aaaagaatac tgctccacgc 4680
cggtgggcag tcccgccgtt tgccgggtta cgctcctagt ggtaagatcc ttacgccggt 4740
cccagtattt cgctgggaaa gaggacagca cctgggccag aaccttttga gtttacagct 4800
tccactttat gagaaaataa tgagcttagc tcctgacaag cttcataccc ttatcgccag 4860
cggagatgtc tatatacgct ctgaaaaacc gttgcagtcc atacctgagg ccgacgttgt 4920
ttgttacggg ctgtgggtcg acccttcctt ggcgacgcac catggggtat tcgccagtga 4980
ccgcaaacat ccggagcagc tcgacttcat gctccagaag ccttctttgg cagaacttga 5040
aagtctctct aagactcatc ttttcctgat ggacataggg atttggttat tgtccgatcg 5100
cgcggtagag attttgatga agcggtccca taaggagtcc tctgaagaat tgaaatacta 5160
tgatctttac agcgactttg ggcttgccct gggcacccac ccacggatag aagatgagga 5220
agtgaatact ctctcagttg caattctgcc tctcccgggc ggggagtttt atcattacgg 5280
tactagcaaa gagctgattt cctccaccct gtcagtccag aataaggttt atgaccaacg 5340
ccggatcatg catagaaagg tcaaaccgaa ccctgccatg tttgtccaaa atgcggtagt 5400
acgtatccca ctgtgcgctg agaacgcaga cctctggatt gaaaactcac atataggtcc 5460
gaagtggaag atagcgagcc ggcatattat tactggggtg ccggagaacg actggagttt 5520
agcagtgcca gcaggggtat gtgtcgacgt tgtcccgatg ggtgataaag gttttgtggc 5580
acggccttac gggctggacg atgtatttaa aggagacctg agagattcaa aaaccacttt 5640
gaccggaatc ccattcggtg aatggatgtc caaacgggga ctctcctaca ctgatctgaa 5700
aggtcggact gacgaccttc aagccgtgag cgtgtttccg atggtcaatt ccgttgagga 5760
attgggcctc gtactccgct ggatgctttc agaacctgag ttggaagagg gtaagaacat 5820
ctggcttcgc tccgagcact tctctgcgga tgaaataagc gctggagcga acctgaagcg 5880
cctctatgct caacgggaag aattccggaa ggggaactgg aaagcattag ccgttaacca 5940
tgagaagtcc gtattttacc aactcgattt ggccgatgcg gcggaggatt tcgtacggtt 6000
gggactcgac atgcctgaat tactccctga ggacgccctg cagatgagtc gcatccataa 6060
tagaatgctt cgcgctcgca tcctcaagct cgacggcaaa gattaccggc ctgaggaaca 6120
ggcagcgttc gatctgctgc gcgacggttt gctcgatgga atctctaacc gtaaaagcac 6180
accaaagctg gacgtttatt ctgaccaaat agtgtggggc cggagcccag tacggattga 6240
tatggccggc ggctggaccg acaccccacc ttatagctta tattccggag gcaatgttgt 6300
gaaccttgcg attgaattaa atggtcaacc tccattgcag gtatacgtta agccgtgtaa 6360
ggacttccat atcgtcctgc ggtccattga catgggggct atggagatag tctcaacttt 6420
tgacgagctg caagactaca aaaagatcgg ttccccgttt tccataccaa aagccgctct 6480
ctctcttgct ggattcgccc cggcatttag cgctgtgtca tatgcatcat tggaggaaca 6540
gttgaaagat tttggagctg gtattgaggt tacgttatta gccgccattc cggctggttc 6600
tggtcttggt acatcatcaa tactggcttc cacagtgctc ggggcaatta atgatttttg 6660
tggactcgca tgggacaaaa atgaaatttg tcagagaaca ttagttttag agcaactgct 6720
gactacggga ggaggctggc aggaccagta cggcggggtc ttgcaaggtg ttaagcttct 6780
gcagaccgag gccgggttcg cgcaatcccc attagttaga tggctgccag accacctctt 6840
tacgcaccct gaatacaagg actgccattt gttatattac acaggaatta cgcgtacggc 6900
aaagggaata ctggcggaga tcgtctctag catgtttctc aatagtagcc tgcacctgaa 6960
tttactctca gaaatgaaag cgcatgccct cgacatgaac gaggctatac agcgcggctc 7020
ctttgttgag ttcggtcgcc ttgtcggaaa gacatgggag caaaacaagg cactcgacag 7080
tggtaccaac ccaccagcag tcgaagccat aatcgactta attaaggatt atacattagg 7140
gtataaactc ccaggggctg gaggaggcgg gtacctctac atggttgcta aagatccgca 7200
ggcagcagtg cgcatccgca aaattttaac agagaacgcg ccaaaccctc gtgcccggtt 7260
tgtggaaatg actctgtccg acaaaggctt tcaagtaagt cggtcctaaa ctagtgattg 7320
ctagctctag actgcagaag cttggcgtaa tcatggtcat agctgtttcc tgtgtgaaat 7380
tgttatccgc tcacaattcc acacaacata cgagccggaa gcataaagtg taaagcctgg 7440
ggtgcctaat gagtgagcta actcacatta attgcgttgc gctcactgcc cgctttccag 7500
tcgggaaacc tgtcgtgcca gctgcattaa tgaatcggcc aacgcgcggg gagaggcggt 7560
ttgcgtattg ggcgctcttc cgcttcctcg ctcactgact cgctgcgctc ggtcgttcgg 7620
ctgcggcgag cggtatcagc tcactcaaag gcggtaatac ggttatccac agaatcaggg 7680
gataacgcag gaaagaacat gtgagcaaaa ggccagcaaa aggccaggaa ccgtaaaaag 7740
gccgcgttgc tggcgttttt ccataggctc cgcccccctg acgagcatca caaaaatcga 7800
cgctcaagtc agaggtggcg aaacccgaca ggactataaa gataccaggc gtttccccct 7860
ggaagctccc tcgtgcgctc tcctgttccg accctgccgc ttaccggata cctgtccgcc 7920
tttctccctt cgggaagcgt ggcgctttct catagctcac gctgtaggta tctcagttcg 7980
gtgtaggtcg ttcgctccaa gctgggctgt gtgcacgaac cccccgttca gcccgaccgc 8040
tgcgccttat ccggtaacta tcgtcttgag tccaacccgg taagacacga cttatcgcca 8100
ctggcagcag ccactggtaa caggattagc agagcgaggt atgtaggcgg tgctacagag 8160
ttcttgaagt ggtggcctaa ctacggctac actagaagaa cagtatttgg tatctgcgct 8220
ctgctgaagc cagttacctt cggaaaaaga gttggtagct cttgatccgg caaacaaacc 8280
accgctggta gcggtggttt ttttgtttgc aagcagcaga ttacgcgcag aaaaaaagga 8340
tctcaagaag atcctttgat cttttctacg gggtctgacg ctcagtggaa cgaaaactca 8400
cgttaaggga ttttggtcat gagattatca aaaaggatct tcacctagat ccttttaaat 8460
taaaaatgaa gttttaaatc aatctaaagt atatatgagt aaacttggtc tgacagttac 8520
caatgcttaa tcagtgaggc acctatctca gcgatctgtc tatttcgttc atccatagtt 8580
gcctgactcc ccgtcgtgta gataactacg atacgggagg gcttaccatc tggccccagt 8640
gctgcaatga taccgcgaga cccacgctca ccggctccag atttatcagc aataaaccag 8700
ccagccggaa gggccgagcg cagaagtggt cctgcaactt tatccgcctc catccagtct 8760
attaattgtt gccgggaagc tagagtaagt agttcgccag ttaatagttt gcgcaacgtt 8820
gttgccattg ctacaggcat cgtggtgtca cgctcgtcgt ttggtatggc ttcattcagc 8880
tccggttccc aacgatcaag gcgagttaca tgatccccca tgttgtgcaa aaaagcggtt 8940
agctccttcg gtcctccgat cgttgtcaga agtaagttgg ccgcagtgtt atcactcatg 9000
gttatggcag cactgcataa ttctcttact gtcatgccat ccgtaagatg cttttctgtg 9060
actggtgagt actcaaccaa gtcattctga gaatagtgta tgcggcgacc gagttgctct 9120
tgcccggcgt caatacggga taataccgcg ccacatagca gaactttaaa agtgctcatc 9180
attggaaaac gttcttcggg gcgaaaactc tcaaggatct taccgctgtt gagatccagt 9240
tcgatgtaac ccactcgtgc acccaactga tcttcagcat cttttacttt caccagcgtt 9300
tctgggtgag caaaaacagg aaggcaaaat gccgcaaaaa agggaataag ggcgacacgg 9360
aaatgttgaa tactcatact cttccttttt caatattatt gaagcattta tcagggttat 9420
tgtctcatga gcggatacat atttgaatgt atttagaaaa ataaacaaat aggggttccg 9480
cgcacatttc cccgaaaagt gccacctgac gtctaagaaa ccattattat catgacatta 9540
acctataaaa ataggcgtat cacgaggccc tttcgtc 9577

Claims (6)

1. A recombinant bacillus subtilis for synthesizing guanosine diphosphate fucose is characterized in that the recombinant bacillus subtilis is obtained by enhancing and expressing a sugar transporter gene of bacillus subtilis 168 and expressing exogenous fucokinase and phosphoguanine transferase genes; and the promoter of the sugar transporter gene of the bacillus subtilis 168 is replaced by a strong promoter P43 to enhance the expression of the sugar transporter gene of the bacillus subtilis 168; the sugar transporter Gene is shown as Gene ID:936346 in NCBI; the genes of the fucokinase and the guanine-phosphotransferase are fkp genes derived from Bacteroides fragilis 9343, and the fkp gene of the Bacteroides fragilis 9343 is shown as GenBank: AY849806.1 on NCBI.
2. The method for constructing recombinant Bacillus subtilis for synthesizing guanosine diphosphate fucose according to claim 1, wherein the method for constructing recombinant Bacillus subtilis comprises the following steps:
(1) constructing a substitution frame containing an upstream and downstream sequence of a sugar transporter gene, a P43 promoter and a bleomycin resistance gene sequence, transforming the constructed substitution frame into recombinant bacillus subtilis 168, and confirming that the sugar transporter gene is successfully expressed in a strengthened manner through verification to obtain recombinant bacillus subtilis BSG;
(2) constructing a recombinant plasmid containing fucokinase and guanine phosphate transferase genes, transforming the constructed recombinant plasmid into bacillus subtilis BSG, and confirming the successful expression of the fucokinase and the guanine phosphate transferase through verification to obtain the recombinant bacillus subtilis BSGF.
3. The method for constructing recombinant Bacillus subtilis for synthesizing guanosine diphosphate fucose according to claim 2, wherein the sequence of the substitution box in the step (1) is shown in SEQ ID No. 1.
4. The method for constructing recombinant Bacillus subtilis for synthesizing guanosine diphosphate fucose according to claim 2, wherein in the step (2), the sequence of the recombinant plasmid is shown as SEQ ID No. 2.
5. The use of recombinant Bacillus subtilis for the synthesis of guanosine diphosphate fucose as claimed in claim 1, wherein the guanosine diphosphate fucose is produced by fermentation using said recombinant Bacillus subtilis.
6. The use of the recombinant Bacillus subtilis for the synthesis of guanosine diphosphate fucose as claimed in claim 5, wherein the fermentation is carried out by inoculating the recombinant Bacillus subtilis seed solution into a fermentation medium at an OD value of 0.1-0.3, and culturing at 35-40 ℃ and 200-250rpm for 20-25 h.
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Engineering the Substrate Transport and Cofactor Regeneration Systems for Enhancing 2"-Fucosyllactose Synthesis in Bacillus subtilis;Jieying Deng等;《ACS Synth Biol》;20191018;第8卷(第10期);第2418-2427页 *
GenBank:AY849806.1;GenBank;《GenBank》;20050321;第1-2页 *
Metabolic Engineering of Escherichia Coli to Produce 2"-fucosyllactose via Salvage Pathway of Guanosine 5"-diphosphate (GDP)-l-fucose;Young-Wook Chin等;《Biotechnol Bioeng》;20161130;第113卷(第11期);第2443-2452页 *

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