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Development of a vector system for the expression of bioengineered proteins.

作者信息

Snouwaert J N, Jambou R C, Skonier J E, Earnhardt K, Stebbins J R, Fowlkes D M

机构信息

Department of Pathology, University of North Carolina, Chapel Hill 27599.

出版信息

Clin Chem. 1989 Jul;35(7 Suppl):B7-12.

PMID:2663236
Abstract

The low natural abundance of many proteins is a major factor in preventing their development as therapeutic or diagnostic tools. To circumvent this barrier, we have used synthetic oligonucleotide technology to construct a gene based on the sequence of a cDNA for human interleukin 6 (IL-6). The synthetic gene encodes a cysteine-free, bioengineered rIL-6 protein, which is expressed at high concentrations in Escherichia coli as a tripartite fusion protein. Cleavage of the fusion protein with collagenase (EC 3.4.24.8) releases a 23-kDa rIL-6 protein that can be easily purified to homogeneity. This rIL-6 protein displays a range of biological activities similar to those of natural human IL-6, as demonstrated by its ability to (a) protect cells from viral infection and (b) stimulate the synthesis of fibrinogen in rat FAZA cells.

摘要

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