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利用 Lac 和 λ 阻遏物在体内和体外进行长距离 DNA 环化的 DNA 系链效应的定量。

Quantitation of the DNA tethering effect in long-range DNA looping in vivo and in vitro using the Lac and λ repressors.

机构信息

Discipline of Biochemistry, School of Molecular and Biomedical Science, University of Adelaide, Adelaide, SA 5005, Australia.

出版信息

Proc Natl Acad Sci U S A. 2014 Jan 7;111(1):349-54. doi: 10.1073/pnas.1317817111. Epub 2013 Dec 16.

Abstract

Efficient and specific interactions between proteins bound to the same DNA molecule can be dependent on the length of the DNA tether that connects them. Measurement of the strength of this DNA tethering effect has been largely confined to short separations between sites, and it is not clear how it contributes to long-range DNA looping interactions, such as occur over separations of tens to hundreds of kilobase pairs in vivo. Here, gene regulation experiments using the LacI and λ CI repressors, combined with mathematical modeling, were used to quantitate DNA tethering inside Escherichia coli cells over the 250- to 10,000-bp range. Although LacI and CI loop DNA in distinct ways, measurements of the tethering effect were very similar for both proteins. Tethering strength decreased with increasing separation, but even at 5- to 10-kb distances, was able to increase contact probability 10- to 20-fold and drive efficient looping. Tethering in vitro with the Lac repressor was measured for the same 600-to 3,200-bp DNAs using tethered particle motion, a single molecule technique, and was 5- to 45-fold weaker than in vivo over this range. Thus, the enhancement of looping seen previously in vivo at separations below 500 bp extends to large separations, underlining the need to understand how in vivo factors aid DNA looping. Our analysis also suggests how efficient and specific looping could be achieved over very long DNA separations, such as what occurs between enhancers and promoters in eukaryotic cells.

摘要

蛋白质与同一 DNA 分子结合的有效且特异的相互作用可能依赖于连接它们的 DNA 连接物的长度。这种 DNA 连接效应的强度的测量主要局限于两个位点之间的短距离,而且尚不清楚它如何促进长距离 DNA 环化相互作用,如在体内发生的数十至数百千碱基对的分离。在这里,使用 LacI 和 λ CI 阻遏物的基因调控实验,结合数学建模,用于定量测量大肠杆菌细胞内 250-10000bp 范围内的 DNA 连接。尽管 LacI 和 CI 以不同的方式环化 DNA,但两种蛋白质的连接效应测量非常相似。连接强度随分离的增加而降低,但即使在 5-10kb 的距离,仍能够增加接触概率 10-20 倍,并驱动有效的环化。使用束缚粒子运动的体外 Lac 阻遏物测量了相同的 600-3200bp DNA 的连接,该技术是一种单分子技术,在该范围内,体外的连接强度比体内弱 5-45 倍。因此,先前在体内观察到的在 500bp 以下分离的环化增强延伸到较大的分离,强调需要了解体内因素如何辅助 DNA 环化。我们的分析还表明,在非常长的 DNA 分离中,如何实现有效且特异的环化,如在真核细胞中增强子和启动子之间发生的情况。

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