Expression, production, and characterization of full-length vitronectin in Escherichia coli

维生素连接蛋白 大肠杆菌 包涵体 重组DNA 紫胶操纵子 化学 融合蛋白 生物化学 尿素 分子生物学 细菌 生物 细胞 整合素 遗传学 基因
作者
Katherine Wojciechowski,Chien‐Hsing Chang,Denise C. Hocking
出处
期刊:Protein Expression and Purification [Elsevier BV]
卷期号:36 (1): 131-138 被引量:16
标识
DOI:10.1016/j.pep.2004.04.004
摘要

Vitronectin (VN) is one of the primary adhesive proteins in serum and serves to promote the attachment and spreading of a wide variety of cell types to tissue culture plastic. In this study, the pGEX2t expression vector was used to express full-length human VN as a GST-tagged fusion protein in Escherichia coli. GST/VN production was induced with IPTG and the protein was found to localize to inclusion bodies. The inclusion bodies were isolated from cell lysates, washed once with 2 M urea and Triton X-100, and then solubilized with 8 M urea in the presence of a reducing compound. Solubilized GST/VN was purified by heparin affinity chromatography and refolded by dialysis against phosphate buffered saline. Approximately 40 mg of GST/VN was recovered from 1L of bacterial culture. Purified GST/VN migrated at the predicted molecular mass on SDS-PAGE and was recognized by both anti-GST and anti-VN antibodies. GST/VN bound to heparin and promoted cell adhesion, spreading, and growth to a similar extent as that observed with plasma-derived VN. As such, the production of recombinant VN in bacteria represents a rapid and convenient method to produce large quantities of VN for cellular studies.

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