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大肠杆菌DNA依赖性RNA聚合酶的一维扩散:一种促进启动子定位的机制。

One-dimensional diffusion of Escherichia coli DNA-dependent RNA polymerase: a mechanism to facilitate promoter location.

作者信息

Ricchetti M, Metzger W, Heumann H

机构信息

Max-Planck-Institut für Biochemie, Martinsried, Federal Republic of Germany.

出版信息

Proc Natl Acad Sci U S A. 1988 Jul;85(13):4610-4. doi: 10.1073/pnas.85.13.4610.

Abstract

The mechanism of promoter location by DNA-dependent RNA polymerase of Escherichia coli was investigated. The occupancies of DNA fragments carrying the A1 promoter of bacteriophage T7 were analyzed as a function of the length of flanking sequences adjacent to the promoter. Competition between the promoters on different fragments showed qualitatively that DNA sequences downstream of the promoter enhanced promoter occupancy, whereas upstream flanking sequences had little or no influence on occupancy. This was studied quantitatively by using a set of DNA fragments with four identical A1 promoters (I-IV) equidistant from each other, but with different lengths of flanking sequences upstream from promoter I and downstream from promoter IV. The relative occupancies of these promoters showed that downstream DNA sequences of up to 250 base pairs increased the occupancy of the adjacent promoter, whereas upstream sequences longer than 70 base pairs had little or no effect on occupancy. Promoter occupancies measured as a function of the length of the downstream flanking DNA sequences were fit by a published theory that takes into account an enhancement of signal-sequence location by linear diffusion.

摘要

对大肠杆菌依赖DNA的RNA聚合酶确定启动子位置的机制进行了研究。分析了携带噬菌体T7 A1启动子的DNA片段的占有率,作为启动子相邻侧翼序列长度的函数。不同片段上启动子之间的竞争定性地表明,启动子下游的DNA序列增强了启动子占有率,而上游侧翼序列对占有率几乎没有影响或没有影响。通过使用一组具有四个彼此等距的相同A1启动子(I-IV)但在启动子I上游和启动子IV下游具有不同长度侧翼序列的DNA片段进行了定量研究。这些启动子的相对占有率表明,长达250个碱基对的下游DNA序列增加了相邻启动子的占有率,而长度超过70个碱基对的上游序列对占有率几乎没有影响或没有影响。作为下游侧翼DNA序列长度的函数测量的启动子占有率通过一种已发表的理论进行拟合,该理论考虑了线性扩散对信号序列定位的增强作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/fa71/280484/95d6a1443459/pnas00265-0042-a.jpg

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