Sir William Dunn School of Pathology, University of Oxford, Oxford OX1 3RE, UK.
Nucleic Acids Res. 2013 Feb 1;41(4):2216-27. doi: 10.1093/nar/gks1441. Epub 2013 Jan 8.
An RNA polymerase has been thought to transcribe by seeking out a promoter, initiating and then tracking down the template. We add tumor necrosis factor α to primary human cells, switch on transcription of a 221-kb gene and monitor promoter position during the ensuing transcription cycle (using RNA fluorescence in situ hybridization coupled to super-resolution localization, chromosome conformation capture and Monte Carlo simulations). Results are consistent with a polymerase immobilized in a 'factory' capturing a promoter and reeling in the template, as the transcript and promoter are extruded. Initially, the extruded promoter is tethered close to the factory and so likely to re-initiate; later, the tether becomes long enough to allow re-initiation in another factory. We suggest close tethering underlies enhancer function and transcriptional 'bursting'.
人们一直认为 RNA 聚合酶通过寻找启动子、起始并追踪模板来进行转录。我们向原代人细胞中添加肿瘤坏死因子 α,启动一个 221kb 基因的转录,并在随后的转录循环中监测启动子位置(使用 RNA 荧光原位杂交与超分辨率定位、染色体构象捕获和蒙特卡罗模拟相结合)。结果与聚合酶固定在“工厂”中捕获启动子并将模板卷取出来的情况一致,因为转录本和启动子被挤出。最初,挤出的启动子与工厂紧密连接,因此很可能重新起始;后来,连接变得足够长,允许在另一个工厂中重新起始。我们认为紧密连接是增强子功能和转录“爆发”的基础。
Zotero 插件