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群体感应转录因子TraR通过与DNA碱基的直接接触以及对DNA柔韧性的检测来解读其DNA结合位点。

The quorum-sensing transcription factor TraR decodes its DNA binding site by direct contacts with DNA bases and by detection of DNA flexibility.

作者信息

White Catharine E, Winans Stephen C

机构信息

Department of Microbiology, Cornell University, Ithaca, NY 14853, USA.

出版信息

Mol Microbiol. 2007 Apr;64(1):245-56. doi: 10.1111/j.1365-2958.2007.05647.x.

Abstract

TraR of Agrobacterium tumefaciens is a member of the LuxR family of transcriptional regulators, and binds to specific DNA sequences (tra boxes) at target promoters of the tumour-inducing (Ti) plasmid. Each tra box has a pronounced dyad symmetry, and each subunit of a TraR dimer binds to one half of a tra box via a helix-turn-helix (HTH) DNA binding motif. Structural analysis has suggested that TraR makes extensive sequence-specific contacts with tra box DNA. In this study, we tested these predictions using synthetic self-complementary oligonucleotides containing variant tra box sequences. Some predictions made from structural analysis were confirmed, while others were shown to be incorrect. Unexpectedly, these experiments also showed that six nucleotides at the centre of the tra box that make no direct contact with TraR are nevertheless critical for high-affinity binding and probably act by facilitating a previously described DNA bend. Variant tra boxes were also tested for transcription activity in vivo. Most transcription assays reflected in vitro binding assays. However, alterations of the outermost nucleotides had little effect on TraR binding but blocked transcription, probably by altering an overlapping -35 promoter motif.

摘要

根癌土壤杆菌的TraR是转录调节因子LuxR家族的成员,它与致瘤(Ti)质粒靶启动子处的特定DNA序列(tra框)结合。每个tra框都有明显的二重对称,TraR二聚体的每个亚基通过螺旋-转角-螺旋(HTH)DNA结合基序与tra框的一半结合。结构分析表明,TraR与tra框DNA进行广泛的序列特异性接触。在本研究中,我们使用含有变异tra框序列的合成自互补寡核苷酸测试了这些预测。结构分析做出的一些预测得到了证实,而其他一些预测则被证明是错误的。出乎意料的是,这些实验还表明,tra框中心不与TraR直接接触的六个核苷酸对于高亲和力结合至关重要,可能通过促进先前描述的DNA弯曲而起作用。还在体内测试了变异tra框的转录活性。大多数转录测定反映了体外结合测定。然而,最外层核苷酸的改变对TraR结合影响很小,但可能通过改变重叠的-35启动子基序而阻断转录。

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