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首页> 外文期刊>ACS Synthetic Biology >Preventing T7 RNA Polymerase Read-through Transcription-A Synthetic Termination Signal Capable of Improving Bioprocess Stability
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Preventing T7 RNA Polymerase Read-through Transcription-A Synthetic Termination Signal Capable of Improving Bioprocess Stability

机译:防止T7 RNA聚合酶通读转录-A能够改善生物过程稳定性的合成终止信号

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摘要

The phage-derived T7 RNA polymerase is the most prominent orthogonal transcriptions system used in the field of synthetic biology. However, gene expression driven by T7 RNA polymerase is prone to read-through transcription 11 due to contextuality of the T7 terminator.. The native T7 emulator has a termination efficiency of approximately 80% and therefore provides insufficient insulation of the expression unit. By using a combination of a synthetic T7 termination signal with two well-known transcriptional terminators (rrnBT1 and T7), we have been able to increase the termination efficiency to 99%. To characterize putative effects of an enhanced termination signal on product yield and I process stability, industrial-relevant fed batch cultivations have been performed. Fermentation of a E. coli HMS174(DE3) strain carrying a pET30a derivative containing the improved termination signal showed a significant decrease of plasmid copy number (PCN) and an increase in total protein yield under standard conditions.
机译:噬菌体来源的T7 RNA聚合酶是合成生物学领域中最著名的正交转录系统。但是,由于T7终止子的上下文关系,由T7 RNA聚合酶驱动的基因表达易于通读转录11。天然T7仿真器的终止效率约为80%,因此无法充分隔离表达单元。通过将合成的T7终止信号与两个众所周知的转录终止子(rrnBT1和T7)结合使用,我们已经能够将终止效率提高到99%。为了表征增强的终止信号对产品收率和工艺稳定性的推定效果,已进行了与工业相关的分批培养。带有包含改良终止信号的pET30a衍生物的大肠杆菌HMS174(DE3)菌株的发酵显示,在标准条件下,质粒拷贝数(PCN)显着降低,总蛋白产量提高。

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