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《南京师大学报（自然科学版）》[ISSN:1001-4616/CN:32-1239/N]

Issue:

2014年03期

Page:

95-

Research Field:

生命科学

Publishing date:

Info

Title:

Chromosome-based TEV Protease Overexpression

Author(s):

Li Ling; Ling Wen; Shi Mudan; Shang Guangdong

School of Life Sciences,Nanjing Normal University,Jiangsu Engineering and Technology Research Center for Microbiology,Jiangsu Key Laboratory for Microbes and Functional Genomics,Nanjing 210023,China

Keywords:

chromosome-based; recombineering; TEV; protein expression

PACS:

Q819

DOI:

-

Abstract:

Due to its high proteinase cleavage activity,specificity and effective in a wide range of conditions,Tobacco etch virus protease(TEV)has many applications,ranging from protein isolation to proteomics study.Currently,TEV is produced by plasmid-based overexpression in Escherichia coli BL21(DE3).Yet,the method has inherent disadvantages,for example,it needs antibiotic to maintain the plasmid which may bring impurities during the protein purification; and non-homogeneity of the strain population which may reduce the yield.Herein,we report the recombineering mediated integration of MBP fused TEV gene under the strong T7 promoter into E.coli BL21(DE3)chromosome.Intracellular digestion of chromosomal based overexpression of MBP-TEV released TEV which was subsequently isolated though Ni-NTA affinity purification,the yield of TEV was up to 4.2 mg/L.Purified TEV shows fine protease activity.The engineered strain has the potential to be used for large scale TEV purification,the established recombineering method can be a platform for the genome engineering and heterologus gene expression in E.coli BL21(DE3).

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Last Update: 2014-09-30