Cell-free synthesis of GFP under high temperature conditions

T. Kanai, T. Endoh, T. Imanaka
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Abstract

Previously, we have developed a system for cell-free protein synthesis that can be operated at high temperatures using a lysate of Thermococcus kodakaraensis. Here, we tested cell-free synthesis of green fluorescent protein (GFP) using the T. kodakaraensis system. A thermostable GFP derivative (tGFP) was used as a reporter protein. By changing the codon usage of tGFP gene for T. kodakaraensis, production of tGFP was detectable in a temperature range of 50degC to 65degC, with an optimum at 60degC. In this condition, active tGFP constitute only 34-62 % of the total protein synthesized. The ratio of active tGFP synthesized markedly increased to 77-84 % by the addition of T. kodakaraensis chaperonin (CpkB) oligomers at 60degC. As tGFP, once folded properly, showed a high stability under these conditions, the results here clearly indicate the presence of a heat-labile state(s) in the folding process of tGFP.
高温条件下无细胞合成绿色荧光蛋白
之前,我们已经开发了一种无细胞蛋白质合成系统,可以在高温下使用柯达卡拉热球菌的裂解物进行操作。在这里,我们使用T. kodakaraensis系统测试了绿色荧光蛋白(GFP)的无细胞合成。使用耐热GFP衍生物(tGFP)作为报告蛋白。通过改变T. kodakaraensis tGFP基因密码子的使用,tGFP的产生在50 ~ 65℃的温度范围内检测到,在60℃时达到最佳。在这种情况下,活性tGFP仅占总合成蛋白的34- 62%。在60℃条件下,添加CpkB寡聚物可显著提高活性tGFP的合成率,达到77 ~ 84%。由于tGFP一旦被正确折叠,在这些条件下表现出很高的稳定性,因此这里的结果清楚地表明在tGFP的折叠过程中存在热不稳定状态。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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