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Molecular cloning and expression ofBacillus subtilis bglS gene inSaccharomyces cerevisiae
Authors:Dr Yongqing Chen  Xinqi Huang  Daxin Song  Fan Yang  Weijun Zheng
Institution:(1) Department of Microbiology and Microbial Technology, Fudan University, 200433 Shanghai, P.R.C.;(2) Present address: Genetic Engineering Institution of Yunnan, Academy of Agriculture Science, Kunming, P.R.C.
Abstract:A 2.7-kb EcoRI DNA fragment carrying aBacillus subtilis endo-beta-1,3-1,4-glucanase gene (bglS) from theE. coli plasmid pFG1 was cloned into anEscherichia coli/yeast shuttle vector to construct a hybrid plasmid YCSH. The hybrid plasmid was used to transformSaccharomyces cerevisiae, and thebglS gene was expressed. Variation between levels ofbglS gene expression inS. cerevisiae was about 2.3-fold, depending on the orientation of the 2.7-kb DNA fragment. Assay of substrate specificity and optimal pH of the enzyme demonstrated that the enzyme encoded by YCSH (bglS) was identical with that found inB. subtilis, but the expression level ofbglS gene inS. cerevisiae (YCSH) was much lower than that inE. coli (YCSH).
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