High‐level expression of enzymatically active bovine leukemia virus proteinase in  E. coli | Zendy

Andreánsky Martin | Zendy; Hrušková-Heidingsfeldová Olga | Zendy; Sedláčeka Juraj | Zendy; Konvalinka Jan | Zendy; Bláha Ivo | Zendy; Ječmen Petr | Zendy; Hořejši Magda | Zendy; Štrop Petr | Zendy; Fábry Milan | Zendy

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High‐level expression of enzymatically active bovine leukemia virus proteinase in E. coli

Author(s) -

Andreánsky Martin,

Hrušková-Heidingsfeldová Olga,

Sedláčeka Juraj,

Konvalinka Jan,

Bláha Ivo,

Ječmen Petr,

Hořejši Magda,

Štrop Petr,

Fábry Milan

Publication year - 1991

Publication title -

febs letters

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 1.593

H-Index - 257

eISSN - 1873-3468

pISSN - 0014-5793

DOI - 10.1016/0014-5793(91)80032-x

Subject(s) - bovine leukemia virus , chemistry , biochemistry , escherichia coli , enzyme , yield (engineering) , microbiology and biotechnology , plasmid , proteinase k , peptide , cytoplasm , biology , virus , gene , virology , materials science , metallurgy

An E. coli plasmid expressing efficiently an artificial precursor of bovine leukemia virus (BLV) proteinase under transcriptional control of the phage T7 promoter was constructed. The expression product accumulates in the induced E. coli cells in the form of insoluble cytoplasmic inclusions. Solubilization of the inclusions and a refolding step yield almost pure and completely self‐processed proteinase. Purification to homogeneity was achieved by ion‐exchange chromatography and reverse‐phase HPLC. On a preparative scale, a high yield of enzymatically active proteinase was obtained. An initial study using a series of synthetic peptide substrates shows a distinct substrate specificity of BLV proteinase.

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