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Structural analysis of the genetic switch that regulates the expression of restriction-modification genes

机译:调控限制性修饰基因表达的遗传开关的结构分析

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Controller (C) proteins regulate the timing of the expression of restriction and modification (R-M) genes through a combination of positive and negative feedback circuits. A single dimer bound to the operator switches on transcription of the C-gene and the endonuclease gene; at higher concentrations, a second dimer bound adjacently switches off these genes. Here we report the first structure of a C protein-DNA operator complex, consisting of two C protein dimers bound to the native 35 bp operator sequence of the R-M system Esp1396I. The structure reveals a role for both direct and indirect DNA sequence recognition. The structure of the DNA in the complex is highly distorted, with severe compression of the minor groove resulting in a 50 degrees bend within each operator site, together with a large expansion of the major groove in the centre of the DNA sequence. Cooperative binding between dimers governs the concentration-dependent activation-repression switch and arises, in part, from the interaction of Glu25 and Arg35 side chains at the dimer-dimer interface. Competition between Arg35 and an equivalent residue of the sigma(70) subunit of RNA polymerase for the Glu25 site underpins the switch from activation to repression of the endonuclease gene.
机译:控制器(C)蛋白通过正反馈电路和负反馈电路的组合来调节限制性和修饰(R-M)基因表达的时间。绑定到操纵基因的单个二聚体打开C基因和核酸内切酶基因的转录。在较高浓度下,结合的第二个二聚体会关闭这些基因。在这里,我们报告一个C蛋白-DNA操纵子复合体的第一个结构,该复合物由两个与R-M系统Esp1396I的天然35 bp操纵子序列结合的C蛋白二聚体组成。该结构揭示了直接和间接DNA序列识别的作用。复合物中DNA的结构高度变形,严重挤压小沟,导致每个操作位点内弯曲50度,同时大沟在DNA序列中心大膨胀。二聚体之间的合作结合决定了浓度依赖性的激活-抑制开关,部分源于二聚体-二聚体界面上的Glu25和Arg35侧链的相互作用。 Arg35和RNA聚合酶sigma(70)亚基的等价残基之间竞争Glu25的位点将支持从激活到内切核酸酶基因抑制的转换。

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