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通过羟基自由基足迹法探究分解代谢物激活蛋白(CAP)与大肠杆菌半乳糖和乳糖启动子的相互作用。结合在gal位点的第二个CAP分子以及结合在lac位点的一个CAP分子可能以相同方式刺激转录。

Interactions of the catabolite activator protein (CAP) at the galactose and lactose promoters of Escherichia coli probed by hydroxyl radical footprinting. The second CAP molecule which binds at gal and the one CAP at lac may act to stimulate transcription in the same way.

作者信息

Shanblatt S H, Revzin A

出版信息

J Biol Chem. 1987 Aug 25;262(24):11422-7.

PMID:3040701
Abstract

The catabolite activator protein (CAP) binding sites of the Escherichia coli galactose and lactose operons were probed by hydroxyl radical footprinting. This method reveals each base that is protected by the bound protein. The patterns of protection seen for the primary CAP sites at gal and lac were virtually identical. In the presence of RNA polymerase the footprint of the second CAP molecule at gal was found to be very similar to those at the other two sites. This upstream site in gal align's perfectly with the lac CAP site with respect to the start of P1 transcription. Replacing most of the gal second CAP site DNA with heterologous sequences did not abolish binding although it became noticeably weaker. In vitro transcription studies of this hybrid gal promoter DNA further demonstrated the reduced affinity of the second CAP. These results are consistent with molecular models proposed for specific CAP binding and suggest that the second CAP at gal may be responsible for overall stimulation of transcription at this operon. Thus, in spite of differences in stoichiometry, the mechanisms of activation by CAP at gal and lac may be quite similar.

摘要

通过羟自由基足迹法探测了大肠杆菌半乳糖操纵子和乳糖操纵子的分解代谢物激活蛋白(CAP)结合位点。该方法可揭示被结合蛋白保护的每个碱基。在半乳糖(gal)和乳糖(lac)操纵子中,主要CAP位点的保护模式几乎相同。在存在RNA聚合酶的情况下,发现半乳糖操纵子中第二个CAP分子的足迹与其他两个位点的足迹非常相似。就P1转录起始而言,半乳糖操纵子中的这个上游位点与乳糖操纵子的CAP位点完美对齐。用异源序列取代半乳糖操纵子第二个CAP位点的大部分DNA,虽然结合明显变弱,但并未消除结合。对这种杂合半乳糖启动子DNA的体外转录研究进一步证明了第二个CAP的亲和力降低。这些结果与针对特定CAP结合提出的分子模型一致,并表明半乳糖操纵子中的第二个CAP可能负责该操纵子转录的整体刺激。因此,尽管化学计量存在差异,但CAP在半乳糖操纵子和乳糖操纵子中的激活机制可能非常相似。

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