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磷酸和碳饥饿在两个间隔启动子处对ugp操纵子的双重调控。

Dual regulation of the ugp operon by phosphate and carbon starvation at two interspaced promoters.

作者信息

Kasahara M, Makino K, Amemura M, Nakata A, Shinagawa H

机构信息

Department of Experimental Chemotherapy, Osaka University, Japan.

出版信息

J Bacteriol. 1991 Jan;173(2):549-58. doi: 10.1128/jb.173.2.549-558.1991.

Abstract

The ugp operon of Escherichia coli includes genes involved in the uptake of sn-glycerol-3-phosphate and glycerophosphoryl diesters and belongs to the pho regulon which is induced by phosphate limitation. This operon has two transcriptional initiation sites, as determined by S1 nuclease mapping of the in vivo transcripts. The downstream promoter has multiple copies of the pho box, the consensus sequence shared by the pho promoters; the upstream promoter has a consensus sequence for the promoters regulated by cyclic AMP and its receptor protein, CRP. PhoB protein, which is the transcriptional activator for the pho regulon, protected the regulatory region with the pho boxes in DNase I footprinting experiments and activated transcription from the downstream promoter in vitro. Studies with transcriptional fusions between ugp and a promoterless gene for chloramphenicol acetyltransferase show that the upstream promoter is induced by carbon starvation in a manner that required the cya and crp genes. PhoB protein may act as a repressor for this upstream promoter, which also overlaps the upstream third pho box. The downstream promoter was induced by phosphate starvation and requires the PhoB protein for its activation as do the other pho regulon promoters. These results suggest that the two promoters function alternately in responding to phosphate or carbon starvation, thus providing the cell with a means to adapt to these physiological stresses.

摘要

大肠杆菌的ugp操纵子包含参与摄取sn-甘油-3-磷酸和甘油磷酸二酯的基因,属于受磷酸盐限制诱导的pho调节子。如通过体内转录本的S1核酸酶图谱分析所确定的,该操纵子有两个转录起始位点。下游启动子有多个pho框拷贝,pho框是pho启动子共有的共有序列;上游启动子有一个由环腺苷酸及其受体蛋白CRP调节的启动子共有序列。PhoB蛋白是pho调节子的转录激活因子,在DNase I足迹实验中保护了带有pho框的调控区域,并在体外激活了下游启动子的转录。对ugp与氯霉素乙酰转移酶的无启动子基因之间的转录融合研究表明,上游启动子在碳饥饿时被诱导,其诱导方式需要cya和crp基因。PhoB蛋白可能作为该上游启动子的阻遏物,该上游启动子也与上游第三个pho框重叠。下游启动子由磷酸盐饥饿诱导,并像其他pho调节子启动子一样需要PhoB蛋白来激活。这些结果表明,这两个启动子在响应磷酸盐或碳饥饿时交替发挥作用,从而为细胞提供了一种适应这些生理应激的方式。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/95c4/207045/380db2c599f2/jbacter00092-0148-a.jpg

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