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嗜热栖热菌Lrp样蛋白LysM可根据赖氨酸的可利用性调节赖氨酸的生物合成。

The Sulfolobus solfataricus Lrp-like protein LysM regulates lysine biosynthesis in response to lysine availability.

作者信息

Brinkman Arie B, Bell Stephen D, Lebbink Robert Jan, de Vos Willem M, van der Oost John

机构信息

Laboratory of Microbiology, Department of Agrotechnology and Food Sciences, Wageningen University, Hesselink van Suchtelenweg 4, 6703 CT Wageningen, The Netherlands.

出版信息

J Biol Chem. 2002 Aug 16;277(33):29537-49. doi: 10.1074/jbc.M203528200. Epub 2002 May 31.

Abstract

Although the archaeal transcription apparatus resembles the eukaryal RNA polymerase II system, many bacterial-like regulators can be found in archaea. Particularly, all archaeal genomes sequenced to date contain genes encoding homologues of Lrp (leucine-responsive regulatory protein). Whereas Lrp-like proteins in bacteria are involved in regulation of amino acid metabolism, their physiological role in archaea is unknown. Although several archaeal Lrp-like proteins have been characterized recently, no target genes apart from their own coding genes have been discovered yet, and no ligands for these regulators have been identified so far. In this study, we show that the Lrp-like protein LysM from Sulfolobus solfataricus is involved in the regulation of lysine and possibly also arginine biosynthesis, encoded by the lys gene cluster. Exogenous lysine is the regulatory signal for lys gene expression and specifically serves as a ligand for LysM by altering its DNA binding affinity. LysM binds directly upstream of the TFB-responsive element of the intrinsically weak lysW promoter, and DNA binding is favored in the absence of lysine, when lysWXJK transcription is maximal. The combined in vivo and in vitro data are most compatible with a model in which the bacterial-like LysM activates the eukarya-like transcriptional machinery. As with transcriptional activation by Escherichia coli Lrp, activation by LysM is apparently dependent on a co-activator, which remains to be identified.

摘要

尽管古菌转录装置类似于真核生物的RNA聚合酶II系统,但在古菌中可以发现许多类似细菌的调节因子。特别是,迄今为止测序的所有古菌基因组都包含编码Lrp(亮氨酸响应调节蛋白)同源物的基因。虽然细菌中的Lrp样蛋白参与氨基酸代谢的调节,但其在古菌中的生理作用尚不清楚。尽管最近已经对几种古菌Lrp样蛋白进行了表征,但除了它们自己的编码基因外,尚未发现其他靶基因,并且迄今为止尚未鉴定出这些调节因子的配体。在本研究中,我们表明来自嗜热栖热菌的Lrp样蛋白LysM参与赖氨酸以及可能还有精氨酸生物合成的调节,由lys基因簇编码。外源赖氨酸是lys基因表达的调节信号,并且通过改变其DNA结合亲和力特异性地作为LysM的配体。LysM直接结合在固有弱启动子lysW的TFB响应元件上游,并且在赖氨酸不存在时,当lysWXJK转录最大时,DNA结合更有利。体内和体外数据相结合最符合一种模型,即类似细菌的LysM激活类似真核生物的转录机制。与大肠杆菌Lrp的转录激活一样,LysM的激活显然依赖于一种共激活因子,有待确定。

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