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Compilation and analysis of Bacillus subtilis sigma A-dependent promoter sequences: evidence for extended contact between RNA polymerase and upstream promoter DNA.

机译:枯草芽孢杆菌西格玛A依赖启动子序列的编辑和分析:RNA聚合酶和上游启动子DNA延长接触的证据。

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摘要

Sequence analysis of 236 promoters recognized by the Bacillus subtilis sigma A-RNA polymerase reveals an extended promoter structure. The most highly conserved bases include the -35 and -10 hexanucleotide core elements and a TG dinucleotide at position -15, -14. In addition, several weakly conserved A and T residues are present upstream of the -35 region. Analysis of dinucleotide composition reveals A2- and T2-rich sequences in the upstream promoter region (-36 to -70) which are phased with the DNA helix: An tracts are common near -43, -54 and -65; Tn tracts predominate at the intervening positions. When compared with larger regions of the genome, upstream promoter regions have an excess of An and Tn sequences for n > 4. These data indicate that an RNA polymerase binding site affects DNA sequence as far upstream as -70. This sequence conservation is discussed in light of recent evidence that the alpha subunits of the polymerase core bind DNA and that the promoter may wrap around RNA polymerase.
机译:枯草芽孢杆菌西格玛A-RNA聚合酶识别的236个启动子的序列分析揭示了扩展的启动子结构。高度保守的碱基包括-35和-10六核苷酸核心元素,以及-15,-14位的TG二核苷酸。另外,在-35区的上游存在几个弱保守的A和T残基。对二核苷酸组成的分析揭示了上游启动子区域(-36至-70)中富含A2-和T2的序列,这些序列与DNA螺旋相定:一个片段在-43,-54和-65附近很常见; Tn道在中间位置占主导。当与基因组的较大区域比较时,上游启动子区域的n和n>序列具有过量的An和Tn序列。这些数据表明,RNA聚合酶结合位点会影响直至-70上游的DNA序列。根据最近的证据讨论了该序列保守性,即聚合酶核心的α亚基结合DNA,并且启动子可以包裹RNA聚合酶。

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