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从胶体物理化学角度看DNA和染色质系统中的液-液相分离

Liquid-liquid phase separation (LLPS) in DNA and chromatin systems from the perspective of colloid physical chemistry.

作者信息

Nordenskiöld Lars, Shi Xiangyan, Korolev Nikolay, Zhao Lei, Zhai Ziwei, Lindman Björn

机构信息

School of Biological Sciences, Nanyang Technological University, Singapore 637551, Singapore.

Department of Biology, Shenzhen MSU-BIT University, Shenzhen 518172, China.

出版信息

Adv Colloid Interface Sci. 2024 Apr;326:103133. doi: 10.1016/j.cis.2024.103133. Epub 2024 Mar 14.

Abstract

DNA is a highly charged polyelectrolyte and is prone to associative phase separation driven by the presence of multivalent cations, charged surfactants, proteins, polymers and colloids. The process of DNA phase separation induced by positively charged species is often called DNA condensation. Generally, it refers to either intramolecular DNA compaction (coil-globule transition) or intermolecular DNA aggregation with macroscopic phase separation, but the formation of a DNA liquid crystalline system is also displayed. This has traditionally been described by polyelectrolyte theory and qualitative (Flory-Huggins-based) polymer theory approaches. DNA in the cell nucleus is packed into chromatin wound around the histone octamer (a protein complex comprising two copies each of the four histone proteins H2A, H2B, H3 and H4) to form nucleosomes separated by linker DNA. During the last decade, the phenomenon of the formation of biomolecular condensates (dynamic droplets) by liquid-liquid phase separation (LLPS) has emerged as a generally important mechanism for the formation of membraneless organelles from proteins, nucleic acids and their complexes. DNA and chromatin droplet formation through LLPS has recently received much attention by in vitro as well as in vivo studies that established the importance of this for compartmentalisation in the cell nucleus. Here, we review DNA and chromatin LLPS from a general colloid physical chemistry perspective. We start with a general discussion of colloidal phase separation in aqueous solutions and review the original (pre-LLPS era) work on DNA (macroscopic) phase separation for simpler systems with DNA in the presence of multivalent cations and well-defined surfactants and colloids. Following that, we discuss and illustrate the similarities of such macroscopic phase separation with the general behaviour of LLPS droplet formation by associative phase separation for DNA-protein systems, including chromatin; we also note cases of segregative association. The review ends with a discussion of chromatin LLPS in vivo and its physiological significance.

摘要

DNA是一种高度带电的聚电解质,容易在多价阳离子、带电表面活性剂、蛋白质、聚合物和胶体的作用下发生缔合相分离。由带正电物质诱导的DNA相分离过程通常称为DNA凝聚。一般来说,它指的是分子内DNA压缩(卷曲-球状转变)或分子间DNA聚集并伴有宏观相分离,但也会表现出DNA液晶系统的形成。传统上,这是通过聚电解质理论和定性(基于弗洛里-哈金斯)聚合物理论方法来描述的。细胞核中的DNA被包装成缠绕在组蛋白八聚体(一种蛋白质复合物,由四种组蛋白H2A、H2B、H3和H4各两个拷贝组成)周围的染色质,形成由连接DNA隔开的核小体。在过去十年中,液-液相分离(LLPS)形成生物分子凝聚物(动态液滴)的现象已成为一种普遍重要的机制,用于由蛋白质、核酸及其复合物形成无膜细胞器。通过LLPS形成DNA和染色质液滴最近受到了体外和体内研究的广泛关注,这些研究确定了这一过程对细胞核区室化的重要性。在这里,我们从一般胶体物理化学的角度综述DNA和染色质的LLPS。我们首先对水溶液中的胶体相分离进行一般性讨论,并回顾在多价阳离子、定义明确的表面活性剂和胶体存在下,DNA(宏观)相分离的原始(LLPS时代之前)工作,这些工作针对更简单的含DNA系统。在此之后,我们讨论并说明这种宏观相分离与DNA-蛋白质系统(包括染色质)通过缔合相分离形成LLPS液滴的一般行为的相似性;我们还指出了分离缔合的情况。综述最后讨论了体内染色质的LLPS及其生理意义。

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