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体内枯草芽孢杆菌碳通量调节剂 Crh 的磷酸化状态的碳源控制。

Carbon source control of the phosphorylation state of the Bacillus subtilis carbon-flux regulator Crh in vivo.

机构信息

Department of General Microbiology, Institute of Microbiology and Genetics, Georg-August-University, Göttingen, Germany.

出版信息

FEMS Microbiol Lett. 2012 Feb;327(1):47-53. doi: 10.1111/j.1574-6968.2011.02456.x. Epub 2011 Nov 28.

DOI:10.1111/j.1574-6968.2011.02456.x
PMID:22092971
Abstract

Bacillus subtilis possesses carbon-flux regulating histidine protein (Crh), a paralog of the histidine protein (HPr) of the phosphotransferase system (PTS). Like HPr, Crh becomes (de)phosphorylated in vitro at residue Ser46 by the metabolite-controlled HPr kinase/phosphorylase HPrK/P. Depending on its phosphorylation state, Crh exerts regulatory functions in connection with carbohydrate metabolism. So far, knowledge on phosphorylation of Crh in vivo has been limited and derived from indirect evidence. Here, we studied the dynamics of Crh phosphorylation directly by non-denaturing gel electrophoresis followed by Western analysis. The results confirm that HPrK/P is the single kinase catalyzing phosphorylation of Crh in vivo. Accordingly, phosphorylation of Crh is triggered by the carbon source as observed previously for HPr, but with some differences. Phosphorylation of both proteins occurred during exponential growth and disappeared upon exhaustion of the carbon source. During exponential growth, 80% of the Crh molecules were phosphorylated when cells utilized a preferred carbon source. The reverse distribution, i.e. around 20% of Crh molecules phosphorylated, was obtained upon utilization of less favorable substrates. This clear-cut classification of the substrates into two groups has not previously been observed for HPr(Ser)P formation. The likely reason for this difference is the additional PTS-dependent phosphorylation of HPr at His15, which limits accumulation of HPr(Ser)~P.

摘要

枯草芽孢杆菌拥有碳通量调节组氨酸蛋白(Crh),这是磷酸转移酶系统(PTS)中组氨酸蛋白(HPr)的同源物。与 HPr 一样,Crh 在体外通过代谢物控制的 HPr 激酶/磷酸化酶 HPrK/P 在残基 Ser46 处(去)磷酸化。根据其磷酸化状态,Crh 在与碳水化合物代谢有关的调节功能。到目前为止,关于 Crh 的体内磷酸化的知识是有限的,并且是从间接证据中得出的。在这里,我们通过非变性凝胶电泳后进行 Western 分析直接研究了 Crh 磷酸化的动力学。结果证实 HPrK/P 是催化 Crh 体内磷酸化的单一激酶。因此,Crh 的磷酸化如先前观察到的 HPr 一样,由碳源触发,但存在一些差异。当细胞利用首选碳源时,两种蛋白质都在指数生长期发生磷酸化,并且当碳源耗尽时磷酸化消失。在指数生长期,当细胞利用优选的碳源时,约 80%的 Crh 分子被磷酸化。当利用不太有利的底物时,得到相反的分布,即约 20%的 Crh 分子被磷酸化。这种对底物的明确分类成两类,以前在 HPr(Ser)P 形成中没有观察到。造成这种差异的可能原因是 HPr 在 His15 处的 PTS 依赖性磷酸化,这限制了 HPr(Ser)P 的积累。

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