Brief Funct Genomics. 2018 Mar 1;17(2):96-103. doi: 10.1093/bfgp/elx038.
The growing appreciation of the importance of long noncoding RNAs (lncRNAs), together with the awareness that some of these RNAs are associated with chromatin, has inspired the development of methods to detect their sites of interaction on a genome-wide scale at high resolution. Hybridization capture methods combine antisense oligonucleotide hybridization with enrichment of RNA from cross-linked chromatin extracts. These techniques have provided insight into lncRNA localization and the interactions of lncRNAs with protein to better understand biological roles of lncRNAs. Here, we review the core principles of hybridization capture methods, focusing on the three most commonly used protocols: capture hybridization analysis of RNA targets (CHART), chromatin isolation by RNA purification (ChIRP) and RNA affinity purification (RAP). We highlight the general principles of these techniques and discuss how differences in experimental procedures present distinct challenges to help researchers using these protocols or, more generally, interpreting the results of hybridization capture experiments.
越来越多的人认识到长非编码 RNA(lncRNAs)的重要性,并且意识到其中一些 RNA 与染色质有关,这激发了开发方法的灵感,以便在全基因组范围内以高分辨率检测它们在基因组上的相互作用位点。杂交捕获方法将反义寡核苷酸杂交与交联染色质提取物中 RNA 的富集相结合。这些技术深入了解了 lncRNA 的定位以及 lncRNA 与蛋白质的相互作用,从而更好地理解了 lncRNA 的生物学功能。在这里,我们回顾了杂交捕获方法的核心原则,重点介绍了三种最常用的方案:RNA 靶标杂交捕获分析(CHART)、RNA 纯化的染色质分离(ChIRP)和 RNA 亲和纯化(RAP)。我们强调了这些技术的一般原理,并讨论了实验程序的差异如何带来不同的挑战,以帮助使用这些方案的研究人员,或者更一般地说,解释杂交捕获实验的结果。