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核蛋白复合物对大肠杆菌acsP2启动子处CRP依赖性转录的调控:类核蛋白FIS和IHF的抗激活作用

Modulation of CRP-dependent transcription at the Escherichia coli acsP2 promoter by nucleoprotein complexes: anti-activation by the nucleoid proteins FIS and IHF.

作者信息

Browning Douglas F, Beatty Christine M, Sanstad Erik A, Gunn Kathryn E, Busby Stephen J W, Wolfe Alan J

机构信息

Department of Microbiology and Immunology, Stritch School of Medicine, Loyola University Chicago, Maywood, IL 60153, USA.

出版信息

Mol Microbiol. 2004 Jan;51(1):241-54. doi: 10.1046/j.1365-2958.2003.03824.x.

Abstract

acs encodes acetyl-coenzyme A synthetase, a high-affinity enzyme that allows cells to scavenge for acetate during carbon starvation. CRP activates acs transcription by binding tandem DNA sites located upstream of the major promoter, acsP2. Here, we used electrophoretic mobility shift assays and DNase I footprint analyses to demonstrate that the nucleoid proteins FIS and IHF each bind multiple sites within the acs regulatory region, that FIS competes successfully with CRP for binding to their overlapping and neighbouring sites and that IHF binds independently of either FIS or CRP. Using in vitro transcription assays, we demonstrated that FIS and IHF independently reduce CRP-dependent acs transcription. Using in vivo reporter assays, we showed that disruption of DNA sites for FIS or deletion of DNA sites for IHF increases acs transcription. We propose that FIS and IHF each function directly as anti-activators of CRP, each working independently at different times during growth to set the levels of CRP-dependent acs transcription.

摘要

acs编码乙酰辅酶A合成酶,这是一种高亲和力的酶,可使细胞在碳饥饿期间清除乙酸盐。CRP通过结合位于主要启动子acsP2上游的串联DNA位点来激活acs转录。在这里,我们使用电泳迁移率变动分析和DNase I足迹分析来证明类核蛋白FIS和IHF各自结合acs调控区域内的多个位点,FIS与CRP成功竞争结合其重叠和相邻位点,并且IHF独立于FIS或CRP进行结合。使用体外转录分析,我们证明FIS和IHF独立降低CRP依赖性acs转录。使用体内报告基因分析,我们表明破坏FIS的DNA位点或删除IHF的DNA位点会增加acs转录。我们提出FIS和IHF各自直接作为CRP的抗激活剂发挥作用,在生长过程中的不同时间各自独立发挥作用,以设定CRP依赖性acs转录的水平。

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