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Optimization of ClpXP activity and protein synthesis in an E. coli extract-based cell-free expression system

机译:基于大肠杆菌提取物的无细胞表达系统中ClpXP活性和蛋白质合成的优化

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摘要

Protein degradation is a fundamental process in all living cells and is essential to remove both damaged proteins and intact proteins that are no longer needed by the cell. We are interested in creating synthetic genetic circuits that function in a cell-free expression system. This will require not only an efficient protein expression platform but also a robust protein degradation system in cell extract. Therefore, we purified and tested the activity of E. coli ClpXP protease in cell-free transcription-translation (TX-TL) systems that used E. coli S30 cell extract. Surprisingly, our studies showed that purified ClpXP added to the TX-TL system has very low proteolytic activity. The low activity of ClpXP was correlated with the rapid consumption of adenosine triphosphate (ATP) in cell extract. We improved the activity of ClpXP in cell extract by adding exogenous ATP and an energy regeneration system. We then established conditions for both protein synthesis, and protein degradation by ClpXP to occur simultaneously in the TX-TL systems. The optimized conditions for ClpXP activity will be useful for creating tunable synthetic genetic circuits and in vitro synthetic biology.
机译:蛋白质降解是所有活细胞的基本过程,对于清除细胞不再需要的受损蛋白质和完整蛋白质至关重要。我们对创建在无细胞表达系统中起作用的合成遗传电路感兴趣。这不仅需要高效的蛋白质表达平台,而且还需要细胞提取物中强大的蛋白质降解系统。因此,我们在使用大肠杆菌S30细胞提取物的无细胞转录翻译(TX-TL)系统中纯化和测试了大肠杆菌ClpXP蛋白酶的活性。令人惊讶地,我们的研究表明,添加到TX-TL系统中的纯化ClpXP具有非常低的蛋白水解活性。 ClpXP的低活性与细胞提取物中三磷酸腺苷(ATP)的快速消耗有关。通过添加外源ATP和能量再生系统,我们提高了ClpXP在细胞提取物中的活性。然后,我们为ClpXP的蛋白质合成和蛋白质降解建立了条件,使其在TX-TL系统中同时发生。 ClpXP活性的优化条件将有助于创建可调的合成遗传电路和体外合成生物学。

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