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[ AmtB、GlnK和谷氨酰胺合成酶在枯草芽孢杆菌转录因子TnrA调控中的作用 ]

[The role of AmtB, GlnK and glutamine synthetase in regulation of transcription factor TnrA in Bacillus subtilis].

作者信息

Fedorova K P, Tarasov N V, Halitova D V, Il'inskaia O N, Barabanshchikov B I, Kaiumov A R

出版信息

Tsitologiia. 2012;54(12):898-901.

Abstract

The nitrogen is a macroelement for all alive cells, from bacteria to animals. Although NH3/NH4+ are highly toxic to animal, they are the preferred source of nitrogen for the most microorganisms and are assimilated by glutamine synthetase in the GOGAT cycle. The nitrogen limitation triggers a number of regulatory processes and activates many genes, providing the utilizing of alternative nitrogen sources. In Bacillus subtilis the genes of nitrogen metabolism are regulated by the transcription factor TnrA. In a cells it is bound to AmtB-GlnK proteins, the interaction with Glutamine synthetase (GS) represses its DNA-binding activity. Here we show the lack of AmtB leads to the nitrogen deficiency in a cell and, consequently, the increased expression of TnrA-dependent genes. In the lack of GlnK the transcription factor TnrA is constitutive bound to GS, the TnrA activity is repressed even under nitrogen limit conditions. Apparently, the TnrA activity is subjected to permanent repression by GS. In the absence of GS, the TnrA activity is strongly higher in compare to control, even under nitrogen limitation, when GS is active. These data allow to suggest that TnrA activity is regulated by the competitive binding to GlnK and GS.

摘要

氮是从细菌到动物等所有活细胞的一种大量元素。尽管氨/铵离子对动物具有高毒性,但它们是大多数微生物首选的氮源,并在谷氨酰胺合成酶的谷氨酰胺合成酶-谷氨酸合酶循环中被同化。氮限制会引发许多调节过程并激活许多基因,以实现对替代氮源的利用。在枯草芽孢杆菌中,氮代谢基因由转录因子TnrA调控。在细胞中,它与AmtB-GlnK蛋白结合,与谷氨酰胺合成酶(GS)的相互作用会抑制其DNA结合活性。在此我们表明,AmtB的缺失会导致细胞中的氮缺乏,从而导致TnrA依赖性基因的表达增加。在缺乏GlnK的情况下,转录因子TnrA与GS组成型结合,即使在氮限制条件下,TnrA的活性也受到抑制。显然,TnrA的活性受到GS的持续抑制。在没有GS的情况下,即使在氮限制且GS有活性时,与对照相比,TnrA的活性也强烈更高。这些数据表明,TnrA的活性受与GlnK和GS的竞争性结合调控。

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