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延伸因子G可稳定70S核糖体的杂合态构象。

Elongation factor G stabilizes the hybrid-state conformation of the 70S ribosome.

作者信息

Spiegel P Clint, Ermolenko Dmitri N, Noller Harry F

机构信息

Center for Molecular Biology of RNA, Department of Molecular, Cell and Developmental Biology, University of California-Santa Cruz 95064, USA.

出版信息

RNA. 2007 Sep;13(9):1473-82. doi: 10.1261/rna.601507. Epub 2007 Jul 13.

Abstract

Following peptide bond formation, transfer RNAs (tRNAs) and messenger RNA (mRNA) are translocated through the ribosome, a process catalyzed by elongation factor EF-G. Here, we have used a combination of chemical footprinting, peptidyl transferase activity assays, and mRNA toeprinting to monitor the effects of EF-G on the positions of tRNA and mRNA relative to the A, P, and E sites of the ribosome in the presence of GTP, GDP, GDPNP, and fusidic acid. Chemical footprinting experiments show that binding of EF-G in the presence of the non-hydrolyzable GTP analog GDPNP or GDP.fusidic acid induces movement of a deacylated tRNA from the classical P/P state to the hybrid P/E state. Furthermore, stabilization of the hybrid P/E state by EF-G compromises P-site codon-anticodon interaction, causing frame-shifting. A deacylated tRNA bound to the P site and a peptidyl-tRNA in the A site are completely translocated to the E and P sites, respectively, in the presence of EF-G with GTP or GDPNP but not with EF-G.GDP. Unexpectedly, translocation with EF-G.GTP leads to dissociation of deacylated tRNA from the E site, while tRNA remains bound in the presence of EF-G.GDPNP, suggesting that dissociation of tRNA from the E site is promoted by GTP hydrolysis and/or EF-G release. Our results show that binding of EF-G in the presence of GDPNP or GDP.fusidic acid stabilizes the ribosomal intermediate hybrid state, but that complete translocation is supported only by EF-G.GTP or EF-G.GDPNP.

摘要

肽键形成后,转运RNA(tRNA)和信使RNA(mRNA)会通过核糖体进行易位,这一过程由延伸因子EF-G催化。在此,我们结合化学足迹法、肽基转移酶活性测定和mRNA足迹法,以监测在存在鸟苷三磷酸(GTP)、鸟苷二磷酸(GDP)、鸟苷二磷酸核糖(GDPNP)和夫西地酸的情况下,EF-G对tRNA和mRNA相对于核糖体A、P和E位点位置的影响。化学足迹实验表明,在不可水解的GTP类似物GDPNP或GDP-夫西地酸存在的情况下,EF-G的结合会诱导脱酰基tRNA从经典的P/P状态移动到杂交的P/E状态。此外,EF-G对杂交P/E状态的稳定作用会损害P位点密码子-反密码子的相互作用,导致移码。在存在EF-G与GTP或GDPNP但不存在EF-G-GDP的情况下,结合在P位点的脱酰基tRNA和A位点的肽基-tRNA会分别完全易位到E位点和P位点。出乎意料的是,与EF-G-GTP的易位会导致脱酰基tRNA从E位点解离,而在EF-G-GDPNP存在的情况下tRNA仍保持结合状态,这表明tRNA从E位点的解离是由GTP水解和/或EF-G释放所促进的。我们的结果表明,在GDPNP或GDP-夫西地酸存在的情况下,EF-G的结合会稳定核糖体中间杂交状态,但只有EF-G-GTP或EF-G-GDPNP才能支持完全易位。

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