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Decoding with the A:I wobble pair is inefficient.

机译:使用A:I摆动对进行解码效率低下。

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摘要

tRNAs with inosine (I) in the first position read three codons ending in U, C and A. However, A-ending codons read with I are rarely used. In Escherichia coli, CGA/U/C are all read solely by tRNAICGArg. CGU and CGC are very common codons, but CGA is very rare. Three independent in vivo assays show that translation of CGA is relatively inefficient. In the first, nine tandem CGA cause a strong rho-mediated polar effect on expression of a lacZ reporter gene. The inhibition is made more extreme by a mutation in ribosomal protein S12 (rpsL), which indicates that ribosomal binding by tRNAICGArg is slow and/or unstable in the CGA cluster. The second assay, in which codons are substituted for the regulatory UGA of the RF2 frameshift, confirms that aa-tRNA selection is slow and/or unstable at CGA. In the third assay, CGA is found to be a poor 5' context for amber suppression, which suggests that an A:I base pair in the P site can interfere with translation of a codon in the A site. Two possible errors, frameshifting and premature termination by RF2, are not significant causes for inefficiency at CGA. It is concluded that the A:I pair destabilizes codon:anticodon complexes during two successive ribosomal cycles, and it is suggested that these properties contribute to the rare usage of codons read with the A:I base pair.
机译:肌苷(I)位于第一个位置的tRNA读取三个以U,C和A结尾的密码子。但是,很少使用以I读取的A末端密码子。在大肠杆菌中,CGA / U / C只能由tRNAICGArg读取。 CGU和CGC是非常常见的密码子,但CGA非常罕见。三种独立的体内试验表明,CGA的翻译效率相对较低。首先,九个串联的CGA对lacZ报告基因的表达产生强烈的rho介导的极性作用。核糖体蛋白S12(rpsL)突变使抑制作用更加极端,这表明tRNAICGArg结合核糖体在CGA簇中缓慢和/或不稳定。第二个试验用密码子代替了RF2移码的调节UGA,证实了在CGA处,aa-tRNA的选择缓慢和/或不稳定。在第三种测定法中,发现CGA在琥珀抑制方面的5'情况较差,这表明P位点的A:I碱基对可干扰A位点的密码子翻译。两个可能的错误,即移码和RF2提前终止,并不是导致CGA效率低下的重要原因。结论是,在两个连续的核糖体循环中,A:I对使密码子:反密码子复合物不稳定,并且表明这些性质有助于罕见地使用A:I碱基对读取的密码子。

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