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Gene recombined candida utilis capable of degrading and utilizing hemicellulose and applications of gene recombined candida utilis

A technology of Candida utilis and genetic recombination, which is applied in the field of genetic engineering and fermentation engineering, can solve the problems of low economic value and low output of xylose, achieve high added value of products, simplify operation steps, and save production costs Effect

Active Publication Date: 2017-03-22
GUANGDONG QIZHI BIOTECHNOLOGY CO LTD
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  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Problems solved by technology

[0005] After hemicellulose is degraded by hemicellulase such as xylanase, a series of products such as xylooligosaccharides, xylose, and arabinose can be produced. However, there is no economical and convenient method to separate xylose and arabinose. Arabinose, to obtain relatively pure xylose and arabinose products; moreover, due to the low economic value of xylose, the input-output ratio of separating xylose from hemicellulose hydrolyzate is very low

Method used

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  • Gene recombined candida utilis capable of degrading and utilizing hemicellulose and applications of gene recombined candida utilis
  • Gene recombined candida utilis capable of degrading and utilizing hemicellulose and applications of gene recombined candida utilis
  • Gene recombined candida utilis capable of degrading and utilizing hemicellulose and applications of gene recombined candida utilis

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Experimental program
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Effect test

Embodiment 1p

[0036] The construction of embodiment 1 pScIKPr carrier

[0037] S1. Double digest pScIKP with Bsp119I and SacI, the digestion conditions are as follows:

[0038]

[0039] After the above-mentioned components were mixed, the enzyme digestion reaction was carried out at 37° C. for 2 hours, and a fragment of about 5.8 kb was recovered by agarose gel electrophoresis.

[0040] S2. The above-mentioned 5.8kb fragment is subjected to end-smoothing treatment with S1 nuclease, and the conditions are as follows:

[0041]

[0042] After mixing the above-mentioned reaction components, react at 23°C for 10 minutes, then add 10mM EDTA to terminate the reaction; then use the PCR product purification kit (Tiangen Biochemical Technology Co., Ltd.) to purify and set aside;

[0043] S3. Self-circularize the fragment obtained in the above step S2 with T4 DNA ligase to obtain the transformed vector pScIKPr.

Embodiment 2

[0044] Construction of embodiment 2 xylanase gene (xyn2) expression cassette

[0045] S1. Design of target gene primers:

[0046] S11. Primers for the mature peptide coding region of xylanase: According to the sequence of the xylanase gene xyn2 of Trichoderma reesei provided by NCBI, use oligo6 biological software to design primers for specific amplification of xyn2 and mutated enzyme digestion The primers for the site, and the sequence of the corresponding enzyme cutting site are as follows:

[0047] Primers for xyn2 and primers for mutant XhoI and SacI sites:

[0048] Mxyn2-F:

[0049]

[0050] Mxyn2-R: 5'- TCTAGA TTAGTTGCTGACACTCTGTGAGGCAG-3'

[0051] The above are the amplification primers of xyn2, and the 5' ends of the two primers are respectively the restriction sites of XhoI and XbaI; the upstream primer simultaneously mutates the restriction site of XhoI in the coding region of xyn2 (dot added below).

[0052] Mxyn2-SacImut-F:

[0053]

[0054] Mxyn2-SacI...

Embodiment 3

[0086] Embodiment 3 Construction of arabinofuranosidase gene (abf1) expression vector

[0087] S1. Design and amplification of target gene primers: According to the sequence of arabinofuranosidase gene abf1 of Trichoderma reesei provided by NCBI, use oligo6 biological software to design primers and mutated restriction sites for specific amplification of abf1 The primers, and the sequence of the corresponding restriction site is as follows:

[0088] abf1 primers and abf1 mutant SacI site primers:

[0089] TrABF1-F: 5'- GGATCC TGCTCTCCAACGCTCGTATC-3';

[0090] TrABF1-R: 5'- ACTAGT TTAAGCAAAACCGCCACTAACCAC-3';

[0091]The above are the amplification primers of abf1, and the 5' ends of the two primers are the restriction sites of BamHI and SpeI respectively.

[0092]

[0093] Above are the primers for the SacI site in the mutated xyn2 coding region (the dots below).

[0094] S2. PCR amplification of the abf1 coding region fragment: a two-step PCR method was used to ampl...

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Abstract

The invention discloses gene recombined candida utilis capable of decomposing hemicellulose and applications of the gene recombined candida utilis. The gene recombined candida utilis can stably express xylanase coming from trichoderma reesei and Arabinfuranosidease. With the gene recombined yeast, an integrated biotechnology capable of degrading hemicellulose for co-producing xylooligosaccharide, arabinose and newtol is established. According to the process, 20g / l bagasse hemicellulose is taken as a substrate, after culture for 156h, xylose produced in the middle process is consumed up by the yeast, the yield of xylooligosaccharide is 20%, at the time, the highest yields of newtol and arabinose, namely, 3.5% and 2.7% are achieved, and the hydrolysis rate of hemicellulose is 40.4%. The integrated biotechnology belongs to a co-production technology which is environmentally friendly, convenient and rapid, and effective.

Description

technical field [0001] The present invention relates to the field of genetic engineering and fermentation engineering, in particular to a genetically recombinant Candida utilis capable of degrading and utilizing hemicellulose and its application. Integrated biotechnology of xylooligosaccharides, arabinose, and xylitol. Background technique [0002] Xylooligosaccharides, xylitol and arabinose are all prebiotics and have important physiological functions. Existing studies have shown that xylooligosaccharides, xylitol and arabinose have important physiological functions, mainly including: (1) As prebiotics, they cannot be digested and absorbed in the human body, and can effectively promote the production of probiotics such as bifidobacteria. Proliferation, thereby inhibiting the growth of harmful bacteria, thereby improving the intestinal environment; (2) improving and inhibiting diarrhea and relieving constipation; (3) inhibiting the absorption of sucrose, so as to inhibit th...

Claims

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Application Information

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Patent Type & Authority Applications(China)
IPC IPC(8): C12N1/19C12N15/81C12N15/66C12P19/00C12P19/02C12P7/18C12R1/72
Inventor 刘泽寰林蒋海武可婧熊春江姜苏峻肖文娟
Owner GUANGDONG QIZHI BIOTECHNOLOGY CO LTD
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