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. RNA 聚合酶转录起始和启动子逃避的机制。

Mechanism of transcription initiation and promoter escape by . RNA polymerase.

机构信息

Department of Biochemistry, University of Wisconsin-Madison, Madison, WI 53706.

Department of Chemistry, University of Wisconsin-Madison, Madison, WI 53706.

出版信息

Proc Natl Acad Sci U S A. 2017 Apr 11;114(15):E3032-E3040. doi: 10.1073/pnas.1618675114. Epub 2017 Mar 27.

Abstract

To investigate roles of the discriminator and open complex (OC) lifetime in transcription initiation by RNA polymerase (RNAP; αββ'ωσ), we compare productive and abortive initiation rates, short RNA distributions, and OC lifetime for the λP and T7A1 promoters and variants with exchanged discriminators, all with the same transcribed region. The discriminator determines the OC lifetime of these promoters. Permanganate reactivity of thymines reveals that strand backbones in open regions of long-lived λP-discriminator OCs are much more tightly held than for shorter-lived T7A1-discriminator OCs. Initiation from these OCs exhibits two kinetic phases and at least two subpopulations of ternary complexes. Long RNA synthesis (constrained to be single round) occurs only in the initial phase (<10 s), at similar rates for all promoters. Less than half of OCs synthesize a full-length RNA; the majority stall after synthesizing a short RNA. Most abortive cycling occurs in the slower phase (>10 s), when stalled complexes release their short RNA and make another without escaping. In both kinetic phases, significant amounts of 8-nt and 10-nt transcripts are produced by longer-lived, λP-discriminator OCs, whereas no RNA longer than 7 nt is produced by shorter-lived T7A1-discriminator OCs. These observations and the lack of abortive RNA in initiation from short-lived ribosomal promoter OCs are well described by a quantitative model in which ∼1.0 kcal/mol of scrunching free energy is generated per translocation step of RNA synthesis to overcome OC stability and drive escape. The different length-distributions of abortive RNAs released from OCs with different lifetimes likely play regulatory roles.

摘要

为了研究鉴别器和开放复合物(OC)寿命在 RNA 聚合酶(RNAP;αββ'ωσ)转录起始中的作用,我们比较了 λP 和 T7A1 启动子及其具有交换鉴别器的变体的有产和无产起始速率、短 RNA 分布和 OC 寿命,所有这些启动子都具有相同的转录区域。鉴别器决定了这些启动子的 OC 寿命。高锰酸盐反应性胸腺嘧啶揭示了长寿命 λP-鉴别器 OC 中开放区域的链骨架比短寿命 T7A1-鉴别器 OC 更紧密。从这些 OC 起始的转录表现出两个动力学相,并且至少有两种三元复合物亚群。长 RNA 合成(被限制为单轮)仅发生在初始相(<10 s),所有启动子的速率相似。不到一半的 OC 合成全长 RNA;大多数在合成短 RNA 后停滞。大多数无产循环发生在较慢的相(>10 s),此时停滞的复合物释放其短 RNA 并在没有逃脱的情况下再次形成。在两个动力学相中,寿命较长的 λP-鉴别器 OC 产生大量 8-nt 和 10-nt 转录物,而寿命较短的 T7A1-鉴别器 OC 则不产生长于 7 nt 的 RNA。这些观察结果以及短寿命核糖体启动子 OC 起始时无无产 RNA 的缺乏,都被一个定量模型很好地描述了,该模型认为 RNA 合成的每个转位步骤都会产生约 1.0 千卡/摩尔的紧缩自由能,以克服 OC 的稳定性并驱动逃脱。具有不同寿命的 OC 释放的无产 RNA 的不同长度分布可能具有调节作用。

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