[Construction of recombinant Bacillus subtilis by co-expression of heterologous D-hydantoinase and N-carbamoylase].

微生物学报 Pub Date : 2017-01-04
Yameng Wang, Rui Ban, Lu Liu, Yu Shen
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Abstract

Objective: We aimed at co-expressing heterologous D-hydantoinase and N-carbamoylase in Bacillus subtilis, and evaluating the feasibility of producing D-p-hydroxyphenylglycine by the recombinant B. subtilis whole-cell catalysis.

Methods: The Paco expression cassette was combined with the coding sequence of hyd or sd1 gene as an artificial gene to express D-hydantoinase. The PAE expression cassette was combined with the coding sequence of adc gene as an artificial gene to express N-carbamoylase. The D-hydantoinase and N-carbamoylase co-expression plasmids pHCS(sd1+adc) and pHCY(hyd+adc) were constructed, using plasmid pHP13 as carrier; the co-expression plasmids pUCS(sd1+adc) was constructed, using plasmid pUB110 as carrier. The additional copy of acoR and sigL gene was integrated at chromosome. The skf and sdp gene were knocked out in B. subtilis. All recombinant strains bearing co-expression plasmid were characterized by analyzing whole-cell catalysis activity.

Results: In the recombinant strains with plasmid pHCY and with pHCS, the whole-cell catalytic activity reached 0.21 U/mL and 0.31 U/mL, respectively. After the over-expression of acoR, sigL, and high-copy-number pUCS, the whole-cell catalytic activity reached 1.0 U/mL.

Conclusion: Overexpression of acoR, sigL and the deletion of skf, sdp genes had significant effects on the catalysis activity of recombinant whole-cell.

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[异种d -羟脲酶和n -氨基淀粉酶共表达构建重组枯草芽孢杆菌]。
目的:在枯草芽孢杆菌中共表达外源d -羟化酶和n -氨基甲酰化酶,评价重组枯草芽孢杆菌全细胞催化生产d -对羟基苯基甘氨酸的可行性。方法:将Paco表达盒与hyd或sd1基因编码序列结合,作为人工基因表达d -羟化酶。将PAE表达盒与adc基因编码序列结合,作为人工基因表达n -氨基甲酰酶。以质粒pHP13为载体,构建d -羟脲酶和n -氨基甲酰酶共表达质粒pHCS(sd1+adc)和pHCY(hyd+adc);以质粒pUB110为载体构建共表达质粒pUCS(sd1+adc)。acoR和sigL基因的附加拷贝整合在染色体上。skf和sdp基因在枯草芽孢杆菌中被敲除。所有携带共表达质粒的重组菌株通过全细胞催化活性分析进行了表征。结果:以pHCY和pHCS为质粒的重组菌株的全细胞催化活性分别达到0.21 U/mL和0.31 U/mL。过表达acoR、sigL和高拷贝数pUCS后,全细胞催化活性达到1.0 U/mL。结论:acoR、sigL的过表达和skf、sdp基因的缺失对重组全细胞的催化活性有显著影响。
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期刊介绍: Acta Microbiologica Sinica(AMS) is a peer-reviewed monthly (one volume per year)international journal,founded in 1953.It covers a wide range of topics in the areas of general and applied microbiology.The journal publishes original papers,reviews in microbiological science,and short communications describing unusual observations. Acta Microbiologica Sinica has been indexed in Index Copernicus (IC),Chemical Abstract (CA),Excerpt Medica Database (EMBASE),AJ of Viniti (Russia),Biological Abstracts (BA),Chinese Science Citation Database (CSCD),China National Knowledge Infrastructure(CNKI),Institute of Scientific and Technical Information of China(ISTIC),Chinese Journal Citation Report(CJCR),Chinese Biological Abstracts,Chinese Pharmaceutical Abstracts,Chinese Medical Abstracts and Chinese Science Abstracts.
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