Extraction of recombinant protein from Escherichia coli by using a novel cell autolysis activity of VanX |
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| Authors: | Tetsuya Kamioka Shihori Sohya Nan Wu Tei Maki Tomoki Matsuda Takahisa Ikegami Haruki Nakamura Yutaka Kuroda |
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| Affiliation: | 1. Department of Biotechnology and Life Science, Graduate School of Engineering, Tokyo University of Agriculture and Technology, Tokyo 184-8588, Japan;2. EM Application Group, EM Business Unit, JEOL, Tokyo 196-8558, Japan;3. Institute of Scientific and Industrial Research, Osaka University, Osaka 567-0047 , Japan;4. Institute for Protein Research, Osaka University, Osaka 565-0871, Japan |
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| Abstract: | ![]()
Escherichia coli is a versatile, low-cost, and popular host for expressing recombinant proteins. However, extracting recombinant proteins from E. coli requires cell wall breakage, which is both time- and effort-consuming. Here we report a novel cell breakage method based on our recent finding that VanX, which is a d-Ala-d-Ala dipeptidase encoded in a vancomycin-resistant VanA gene cluster, exhibits a strong cell lysis activity when expressed in isolation in E. coli. In our strategy, we coexpress VanX with the target protein, causing cell autolysis and release of the cellular content into the culture medium. We demonstrated this strategy for two model proteins, a green fluorescent protein variant (GFPuv) and Gaussia luciferase, and optimized the autolysis conditions and coexpression vectors. The fluorescence activity of GFPuv collected from the medium was identical to that of GFPuv purified by conventional methods. Cell breakage by VanX-mediated autolysis is very simple to implement and will efficiently complement traditional methods. |
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| Keywords: | Cell lysis Bacterial cell wall VanX GFP Protein purification Coexpression |
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