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大肠杆菌壳二糖操纵子的表达受三种转录因子调控:NagC、ChbR和CAP。

Expression of the chitobiose operon of Escherichia coli is regulated by three transcription factors: NagC, ChbR and CAP.

作者信息

Plumbridge Jacqueline, Pellegrini Olivier

机构信息

Institut de Biologie Physico-Chimique (CNRS UPR9073), 13, rue Pierre et Marie Curie, 75005 Paris, France.

出版信息

Mol Microbiol. 2004 Apr;52(2):437-49. doi: 10.1111/j.1365-2958.2004.03986.x.

Abstract

The chitobiose operon, chbBCARFG, encodes genes for the transport and degradation of the N-acetylglucosamine disaccharide, chitobiose. Chitobiose is transported by the phosphotransferase system (PTS) producing chitobiose-6P which is hydrolysed to GlcNAc-6P by the chbF gene product and then further degraded by the nagBA gene products. Expression of the chb operon is repressed by NagC, which regulates genes involved in amino sugar metabolism. The inducer for NagC is GlcNAc-6P. NagC binds to two sites separated by 115 bp and the transcription start point of the chb operon lies within the downstream NagC operator. In addition the chb operon encodes its own specific regulator, ChbR, an AraC-type dual repressor-activator, which binds to two direct repeats of 19 bp located between the two NagC sites. ChbR is necessary for transcription activation in the presence of chitobiose in vivo. Induction of the operon also requires CAP, which binds to a site upstream of the ChbR repeats. In the absence of chitobiose both NagC and ChbR act as repressors. Together these three factors cooperate in switching chb expression from the repressed to the activated state. The need for two specific inducing signals, one for ChbR to activate the expression of the operon and a second for NagC to relieve its repression, ensure that the chb operon is only induced when there is sufficient flux through the combined chb-nag metabolic pathway to activate expression of both the chb and nag operons.

摘要

壳二糖操纵子chbBCARFG编码参与N - 乙酰葡糖胺二糖(壳二糖)运输和降解的基因。壳二糖通过磷酸转移酶系统(PTS)进行转运,产生壳二糖 - 6P,壳二糖 - 6P由chbF基因产物水解为GlcNAc - 6P,然后由nagBA基因产物进一步降解。chb操纵子的表达受NagC抑制,NagC调控参与氨基糖代谢的基因。NagC的诱导物是GlcNAc - 6P。NagC结合到两个相隔115 bp的位点,chb操纵子的转录起始点位于下游的NagC操纵子内。此外,chb操纵子编码其自身的特异性调节因子ChbR,一种AraC型双阻遏物 - 激活物,它结合到位于两个NagC位点之间的19 bp的两个直接重复序列上。ChbR在体内壳二糖存在时对转录激活是必需的。操纵子的诱导还需要CAP,它结合到ChbR重复序列上游的一个位点。在没有壳二糖的情况下,NagC和ChbR都作为阻遏物起作用。这三个因子共同协作将chb的表达从抑制状态转变为激活状态。需要两个特异性诱导信号,一个用于ChbR激活操纵子的表达,另一个用于NagC解除其抑制,以确保只有当通过chb - nag联合代谢途径有足够通量来激活chb和nag操纵子的表达时,chb操纵子才会被诱导。

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