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超螺旋影响参与基因调控的环的形成。

Supercoiling biases the formation of loops involved in gene regulation.

作者信息

Finzi Laura, Dunlap David

机构信息

Department of Physics, Emory University, 400 Dowman Dr. N.E., Atlanta, GA, 30322, USA.

出版信息

Biophys Rev. 2016 Nov;8(Suppl 1):65-74. doi: 10.1007/s12551-016-0211-0. Epub 2016 Jul 5.

Abstract

The function of DNA as a repository of genetic information is well-known. The post-genomic effort is to understand how this information-containing filament is chaperoned to manage its compaction and topological states. Indeed, the activities of enzymes that transcribe, replicate, or repair DNA are regulated to a large degree by access. Proteins that act at a distance along the filament by binding at one site and contacting another site, perhaps as part of a bigger complex, create loops that constitute topological domains and influence regulation. DNA loops and plectonemes are not necessarily spontaneous, especially large loops under tension for which high energy is required to bring their ends together, or small loops that require accessory proteins to facilitate DNA bending. However, the torsion in stiff filaments such as DNA dramatically modulates the topology, driving it from extended and genetically accessible to more looped and compact, genetically secured forms. Furthermore, there are accessory factors that bias the response of the DNA filament to supercoiling. For example, small molecules like polyamines, which neutralize the negative charge repulsions along the phosphate backbone, enhance flexibility and promote writhe over twist in response to torsion. Such increased flexibility likely pushes the topological equilibrium from twist toward writhe at tensions thought to exist in vivo. A predictable corollary is that stiffening DNA antagonizes looping and bending. Certain sequences are known to be more or less flexible or to exhibit curvature, and this may affect interactions with binding proteins. In vivo all of these factors operate simultaneously on DNA that is generally negatively supercoiled to some degree. Therefore, in order to better understand gene regulation that involves protein-mediated DNA loops, it is critical to understand the thermodynamics and kinetics of looping in DNA that is under tension, negatively supercoiled, and perhaps exposed to molecules that alter elasticity. Recent experiments quantitatively reveal how much negatively supercoiling DNA lowers the free energy of looping, possibly biasing the operation of genetic switches.

摘要

DNA作为遗传信息储存库的功能是众所周知的。后基因组研究的目标是了解这条包含信息的细丝是如何被伴侣蛋白管理以控制其压缩和拓扑状态的。事实上,转录、复制或修复DNA的酶的活性在很大程度上受到可及性的调节。通过在一个位点结合并与另一个位点接触(可能作为更大复合物的一部分)沿着细丝远距离起作用的蛋白质会形成构成拓扑结构域并影响调节的环。DNA环和超螺旋结构不一定是自发形成的,特别是处于张力下的大环,需要高能量才能将其末端聚集在一起,或者小环需要辅助蛋白来促进DNA弯曲。然而,像DNA这样的刚性细丝中的扭转会显著调节拓扑结构,使其从伸展且基因可及的形式转变为更多环化和紧凑、基因安全的形式。此外,还有一些辅助因子会使DNA细丝对超螺旋的反应产生偏差。例如,多胺等小分子会中和磷酸主链上的负电荷排斥,增强柔韧性,并在受到扭转时促进扭曲转变为缠绕。这种增加的柔韧性可能会在体内认为存在的张力下将拓扑平衡从扭曲推向缠绕。一个可预测的推论是,使DNA变硬会对抗环化和弯曲。已知某些序列或多或少具有柔韧性或呈现曲率,这可能会影响与结合蛋白的相互作用。在体内,所有这些因素同时作用于通常在某种程度上呈负超螺旋的DNA。因此,为了更好地理解涉及蛋白质介导的DNA环的基因调控,了解处于张力下、负超螺旋且可能暴露于改变弹性的分子的DNA中环化的热力学和动力学至关重要。最近的实验定量揭示了负超螺旋DNA降低环化自由能的程度,这可能会影响遗传开关的运作。

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