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转录因子 TFIIF 和 TFIIS 通过协同和独立的机制促进 RNA 聚合酶 II 的转录延伸。

Transcription factors TFIIF and TFIIS promote transcript elongation by RNA polymerase II by synergistic and independent mechanisms.

机构信息

Departments of Biology, Chemistry, Structural Biology, and Applied Physics, Stanford University, Stanford, CA 94305.

出版信息

Proc Natl Acad Sci U S A. 2014 May 6;111(18):6642-7. doi: 10.1073/pnas.1405181111. Epub 2014 Apr 14.

Abstract

Recent evidence suggests that transcript elongation by RNA polymerase II (RNAPII) is regulated by mechanical cues affecting the entry into, and exit from, transcriptionally inactive states, including pausing and arrest. We present a single-molecule optical-trapping study of the interactions of RNAPII with transcription elongation factors TFIIS and TFIIF, which affect these processes. By monitoring the response of elongation complexes containing RNAPII and combinations of TFIIF and TFIIS to controlled mechanical loads, we find that both transcription factors are independently capable of restoring arrested RNAPII to productive elongation. TFIIS, in addition to its established role in promoting transcript cleavage, is found to relieve arrest by a second, cleavage-independent mechanism. TFIIF synergistically enhances some, but not all, of the activities of TFIIS. These studies also uncovered unexpected insights into the mechanisms underlying transient pauses. The direct visualization of pauses at near-base-pair resolution, together with the load dependence of the pause-entry phase, suggests that two distinct mechanisms may be at play: backtracking under forces that hinder transcription and a backtrack-independent activity under assisting loads. The measured pause lifetime distributions are inconsistent with prevailing views of backtracking as a purely diffusive process, suggesting instead that the extent of backtracking may be modulated by mechanisms intrinsic to RNAPII. Pauses triggered by inosine triphosphate misincorporation led to backtracking, even under assisting loads, and their lifetimes were reduced by TFIIS, particularly when aided by TFIIF. Overall, these experiments provide additional insights into how obstacles to transcription may be overcome by the concerted actions of multiple accessory factors.

摘要

最近的证据表明,RNA 聚合酶 II(RNAPII)的转录延伸受影响进入和退出转录非活跃状态(包括暂停和停滞)的机械线索调节。我们进行了一项单分子光学捕获研究,研究了 RNAPII 与转录延伸因子 TFIIS 和 TFIIF 的相互作用,这些因子会影响这些过程。通过监测包含 RNAPII 以及 TFIIF 和 TFIIS 组合的延伸复合物对受控机械负载的反应,我们发现这两种转录因子都能够独立地将停滞的 RNAPII 恢复到有生产力的延伸状态。TFIIS 除了在促进转录物切割方面的既定作用外,还被发现通过第二种与切割无关的机制来缓解停滞。TFIIF 协同增强了 TFIIS 的一些(但不是全部)活性。这些研究还揭示了对短暂暂停机制的意外见解。在接近碱基对分辨率下对暂停进行直接可视化,以及暂停进入阶段对负载的依赖性,表明可能存在两种不同的机制:在阻碍转录的力下发生回溯,以及在辅助负载下发生回溯独立的活动。测量的暂停寿命分布与回溯作为纯粹扩散过程的流行观点不一致,这表明回溯的程度可能受到 RNAPII 固有机制的调节。由于肌苷三磷酸错误掺入而引发的暂停会导致回溯,即使在辅助负载下也是如此,并且 TFIIS 会缩短其寿命,尤其是在 TFIIF 辅助时。总的来说,这些实验提供了更多的见解,了解多个辅助因子的协同作用如何克服转录的障碍。

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