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在大肠杆菌中,alaE基因的表达受全局调控因子Lrp的正向调控,以响应L-丙氨酸在细胞内的积累。

Expression of the alaE gene is positively regulated by the global regulator Lrp in response to intracellular accumulation of l-alanine in Escherichia coli.

作者信息

Ihara Kohei, Sato Kazuki, Hori Hatsuhiro, Makino Yumiko, Shigenobu Shuji, Ando Tasuke, Isogai Emiko, Yoneyama Hiroshi

机构信息

Laboratory of Animal Microbiology, Department of Microbial Biotechnology, Graduate School of Agricultural Science, Tohoku University, 468-1 Aramaki Aza Aoba, Aoba-ku, Sendai 980-0845, Japan.

NIBB Core Research Facilities, National Institute for Basic Biology, Nishigonaka 38, Myodaiji, Okazaki 444-8585, Aichi, Japan.

出版信息

J Biosci Bioeng. 2017 Apr;123(4):444-450. doi: 10.1016/j.jbiosc.2016.11.015. Epub 2017 Jan 3.

DOI:10.1016/j.jbiosc.2016.11.015
PMID:28057466
Abstract

The alaE gene in Escherichia coli encodes an l-alanine exporter that catalyzes the active export of l-alanine using proton electrochemical potential. In our previous study, alaE expression was shown to increase in the presence of l-alanyl-l-alanine (Ala-Ala). In this study, the global regulator leucine-responsive regulatory protein (Lrp) was identified as an activator of the alaE gene. A promoter less β-galactosidase gene was fused to an alaE upstream region (240 nucleotides). Cells that were lacZ-deficient and harbored this reporter plasmid showed significant induction of β-galactosidase activity (approximately 17-fold) in the presence of 6 mM l-alanine, l-leucine, and Ala-Ala. However, a reporter plasmid possessing a smaller alaE upstream region (180 nucleotides) yielded transformants with strikingly low enzyme activity under the same conditions. In contrast, lrp-deficient cells showed almost no β-galactosidase induction, indicating that Lrp positively regulates alaE expression. We next performed an electrophoretic mobility shift assay (EMSA) and a DNase I footprinting assay using purified hexahistidine-tagged Lrp (Lrp-His). Consequently, we found that Lrp-His binds to the alaE upstream region spanning nucleotide -161 to -83 with a physiologically relevant affinity (apparent K, 288.7 ± 83.8 nM). Furthermore, the binding affinity of Lrp-His toward its cis-element was increased by l-alanine and l-leucine, but not by Ala-Ala and d-alanine. Based on these results, we concluded that the gene expression of the alaE is regulated by Lrp in response to intracellular levels of l-alanine, which eventually leads to intracellular homeostasis of l-alanine concentrations.

摘要

大肠杆菌中的alaE基因编码一种L-丙氨酸输出蛋白,该蛋白利用质子电化学势催化L-丙氨酸的主动输出。在我们之前的研究中,已表明在L-丙氨酰-L-丙氨酸(Ala-Ala)存在的情况下alaE表达会增加。在本研究中,全局调节因子亮氨酸应答调节蛋白(Lrp)被鉴定为alaE基因的激活因子。一个不含启动子的β-半乳糖苷酶基因与alaE上游区域(240个核苷酸)融合。携带此报告质粒的lacZ缺陷型细胞在存在6 mM L-丙氨酸、L-亮氨酸和Ala-Ala的情况下显示出β-半乳糖苷酶活性的显著诱导(约17倍)。然而,具有较小alaE上游区域(180个核苷酸)的报告质粒在相同条件下产生的转化体酶活性极低。相比之下,lrp缺陷型细胞几乎没有β-半乳糖苷酶诱导,表明Lrp正向调节alaE表达。接下来,我们使用纯化的六聚组氨酸标记的Lrp(Lrp-His)进行了电泳迁移率变动分析(EMSA)和DNase I足迹分析。结果,我们发现Lrp-His以生理相关亲和力(表观K,288.7±83.8 nM)结合到alaE上游区域核苷酸-161至-83。此外,Lrp-His对其顺式元件的结合亲和力被L-丙氨酸和L-亮氨酸增强,但不被Ala-Ala和D-丙氨酸增强。基于这些结果,我们得出结论,alaE的基因表达受Lrp调节以响应细胞内L-丙氨酸水平,这最终导致L-丙氨酸浓度的细胞内稳态。

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