The maturation and quality control of mRNA in eukaryotes is a tightly regulated, multistep process that begins on nascent transcripts. A 7-methyl guanosine (~7MeG) cap structure is added to the 5' end of pre-mRNA as it emerges from the exit channel of RNA Polymerase II. The multifunctional nuclear cap-binding complex (CBC), consisting of two protein subunits (CBP80 and CBP20), assembles at the pre-mRNA cap early during transcript formation and helps recruit the splicesome machinery to the cap-proximal intron (1, 2). Termination of transcription involves cleavage and polyadenylation at the 3' end, and the mature mRNA is retained in the nucleus or exported to the cytoplasm. In either case, the mRNA undergoes a pioneer round of translation and surveillance by the nonsense-mediated mRNA decay (NMD) pathway to eliminate defective or misspliced transcripts. Although the CBC localizes primarily to the nucleus, it remains associated with mRNAs during export to the cytoplasm and during the pioneer round of translation and mRNA surveillance. After the first round of translation, the CBC is replaced by the eukaryotic initiation complex eIF4F, and the mRNA steady-state translation initiation complex is formed (3). But not all RNA Pol II transcripts are predestined for translation.
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机译:真核生物中mRNA的成熟和质量控制是一个严格的,多步骤的过程,始于新生的转录本。当7-甲基鸟苷(〜7MeG)帽结构从RNA聚合酶II的出口通道出来时,被添加到pre-mRNA的5'末端。多功能核帽结合复合物(CBC)由两个蛋白亚基(CBP80和CBP20)组成,在转录本形成的早期就组装在mRNA前帽上,并有助于将剪接体机制募集到帽近端内含子上(1,2) 。转录终止涉及3'端的切割和聚腺苷酸化,成熟的mRNA保留在细胞核中或输出到细胞质中。无论哪种情况,mRNA都会通过无意义介导的mRNA衰减(NMD)途径进行先驱的翻译和监视,以消除缺陷或错接的转录本。尽管CBC主要定位于细胞核,但在输出到细胞质以及翻译和mRNA监测的先驱阶段,它仍然与mRNA相关。第一轮翻译后,CBC被真核起始复合物eIF4F取代,并形成了mRNA稳态翻译起始复合物(3)。但并非所有RNA Pol II转录本都注定要翻译。
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