Medical Research Council Laboratory of Molecular Biology, Cambridge CB2 0QH, United Kingdom.
Genes Dev. 2022 Feb 1;36(3-4):210-224. doi: 10.1101/gad.349223.121. Epub 2022 Feb 17.
3' end processing of most human mRNAs is carried out by the cleavage and polyadenylation specificity factor (CPSF; CPF in yeast). Endonucleolytic cleavage of the nascent pre-mRNA defines the 3' end of the mature transcript, which is important for mRNA localization, translation, and stability. Cleavage must therefore be tightly regulated. Here, we reconstituted specific and efficient 3' endonuclease activity of human CPSF with purified proteins. This required the seven-subunit CPSF as well as three additional protein factors: cleavage stimulatory factor (CStF), cleavage factor IIm (CFIIm), and, importantly, the multidomain protein RBBP6. Unlike its yeast homolog Mpe1, which is a stable subunit of CPF, RBBP6 does not copurify with CPSF and is recruited in an RNA-dependent manner. Sequence and mutational analyses suggest that RBBP6 interacts with the WDR33 and CPSF73 subunits of CPSF. Thus, it is likely that the role of RBBP6 is conserved from yeast to humans. Overall, our data are consistent with CPSF endonuclease activation and site-specific pre-mRNA cleavage being highly controlled to maintain fidelity in mRNA processing.
大多数人类 mRNA 的 3' 末端加工是由切割和多聚腺苷酸化特异性因子(CPSF;酵母中的 CPF)完成的。新生前体 mRNA 的内切核酸酶切割定义了成熟转录本的 3' 末端,这对于 mRNA 的定位、翻译和稳定性很重要。因此,切割必须受到严格的调控。在这里,我们使用纯化的蛋白重新构建了人 CPSF 的特异性和高效的 3' 内切酶活性。这需要七个亚基的 CPSF 以及另外三个蛋白质因子:切割刺激因子(CStF)、切割因子 II m(CFIIm),以及重要的多结构域蛋白 RBBP6。与作为 CPF 稳定亚基的酵母同源物 Mpe1 不同,RBBP6 不会与 CPSF 共纯化,而是以 RNA 依赖性方式被募集。序列和突变分析表明,RBBP6 与 CPSF 的 WDR33 和 CPSF73 亚基相互作用。因此,RBBP6 的作用很可能在从酵母到人中是保守的。总的来说,我们的数据与 CPSF 内切酶的激活和特定的前体 mRNA 切割相一致,这高度控制着 mRNA 加工的保真度。
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