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RNA 焦磷酸水解酶 RppH 的缺陷增强了大肠杆菌中 L-半胱氨酸的发酵生产。

Defect of RNA pyrophosphohydrolase RppH enhances fermentative production of L-cysteine in Escherichia coli.

机构信息

Graduate School of Life and Environmental Sciences, University of Tsukuba.

Research & Development Center, Carlit Holdings Co., Ltd.

出版信息

J Gen Appl Microbiol. 2021 Feb 26;66(6):307-314. doi: 10.2323/jgam.2019.12.004. Epub 2020 Aug 7.

DOI:10.2323/jgam.2019.12.004
PMID:32779574
Abstract

Fermentative production of L-cysteine has been established using Escherichia coli. In that procedure, thiosulfate is a beneficial sulfur source, whereas repressing sulfate utilization. We first found that thiosulfate decreased transcript levels of genes related to sulfur assimilation, particularly whose expression is controlled by the transcription factor CysB. Therefore, a novel approach, i.e. increment of expression of genes involved in sulfur-assimilation, was attempted for further improvement of L-cysteine overproduction. Disruption of the rppH gene significantly augmented transcript levels of the cysD, cysJ, cysM and yeeE genes (≥1.5-times) in medium containing sulfate as a sole sulfur source, probably because the rppH gene encodes mRNA pyrophosphohydrolase that triggers degradation of certain mRNAs. In addition, the ΔrppH strain appeared to preferentially uptake thiosulfate rather than sulfate, though thiosulfate dramatically reduced expression of the known sulfate/thiosulfate transporter complexes in both ΔrppH and wild-type cells. We also found that both YeeE and YeeD are required for the strain without the transporters to grow in the presence of thiosulfate as a sole sulfur source. Therefore, yeeE and yeeD are assigned as genes responsible for thiosulfate uptake (tsuA and tsuB, respectively). In final, we applied the ΔrppH strain to the fermentative production of L-cysteine. Disruption of the rppH gene enhanced L-cysteine biosynthesis, as a result, a strain producing approximately twice as much L-cysteine as the control strain was obtained.

摘要

利用大肠杆菌成功建立了 L-半胱氨酸的发酵生产方法。在此过程中,硫代硫酸盐是一种有益的硫源,而抑制硫酸盐的利用。我们首先发现硫代硫酸盐降低了与硫同化相关基因的转录水平,特别是那些受转录因子 CysB 控制的基因。因此,我们尝试了一种新方法,即增加参与硫同化的基因的表达,以进一步提高 L-半胱氨酸的过量生产。在含有硫酸盐作为唯一硫源的培养基中,rppH 基因的缺失显著增加了 cysD、cysJ、cysM 和 yeeE 基因的转录水平(≥1.5 倍),这可能是因为 rppH 基因编码的 mRNA 焦磷酸水解酶触发了某些 mRNA 的降解。此外,ΔrppH 菌株似乎优先摄取硫代硫酸盐而不是硫酸盐,尽管硫代硫酸盐显著降低了已知硫酸盐/硫代硫酸盐转运体复合物在 ΔrppH 和野生型细胞中的表达。我们还发现,YeeE 和 YeeD 对于没有转运体的菌株在以硫代硫酸盐作为唯一硫源的情况下生长都是必需的。因此,yeeE 和 yeeD 分别被指定为负责硫代硫酸盐摄取的基因(tsuA 和 tsuB)。最终,我们将 ΔrppH 菌株应用于 L-半胱氨酸的发酵生产。rppH 基因的缺失增强了 L-半胱氨酸的生物合成,结果获得了一株比对照菌株产量增加约两倍的 L-半胱氨酸生产菌株。

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