Department of Evolution, Systematics & Ecology, The Hebrew University of Jerusalem, 91904 Jerusalem, Israel.
BMC Mol Biol. 2010 May 28;11:41. doi: 10.1186/1471-2199-11-41.
Accurate amino acid insertion during peptide elongation requires tRNAs loaded by cognate amino acids and that anticodons match codons. However, tRNA misloading does not necessarily cause misinsertions: misinsertion is avoided when anticodons mismatch codons coding for misloaded amino acids.
Occasional compensation of misacylation by codon-anticodon mismatch necessarily occurs. Putatively, occasional error compensation may be enhanced beyond the random combination of independent errors in tRNA loading and codon-anticodon interactions: tRNA misacylation might alter potentials for codon-anticodon mismatches, perhaps specifically increasing potentials for mismatching those codons coding for the misacylated non-cognate amino acid. This hypothetical phenomenon is called 'error coordination', in distinction from 'error compensation' that assumes independence between misacylation and mismatch.
Eventually, the hypothesis should be tested for each combination of amino acid misacylation and codon-anticodon mismatch, by comparing stabilities or frequencies of mismatched codon-anticodon duplexes formed by tRNAs loaded by their cognate amino acid with stabilities formed by that tRNA when misloaded with the amino acid coded by the mismatched codon. Competitive mismatching experiments between misloaded and correctly loaded tRNAs could also be useful, yet more sophisticated experiments.
Detecting error coordination implies estimating error compensation, which also promotes protein synthesis accuracy. Hence even in the absence of evidence for error coordination, experiments would yield very useful insights into misacylation and mismatch processes. In case experiments consider post-transcriptional RNA modifications (especially at wobble positions), results on codon-anticodon mismatches would enable significant improvements and sophistications of secondary structure prediction softwares. Positive results would show that protein translation enhances accuracies of products, not of single steps in the production. Ancient translational machineries putatively optimized error coordination, especially before tRNA editing by tRNA synthetases evolved: few primitive, but functionally versatile tRNA species perhaps executed low accuracy translation. Systems artificially designed/selected for low complexity and high efficiency could make use of this property for anticodons with high levels of error compensation and coordination.
在肽延伸过程中准确插入氨基酸需要由相应氨基酸加载的 tRNA,并且反密码子与密码子匹配。然而,tRNA 加载错误不一定会导致错误插入:当反密码子与编码错误加载氨基酸的密码子不匹配时,会避免错误插入。
偶然的反密码子-密码子不匹配补偿必然发生。推测,偶然的错误补偿可能会超出 tRNA 加载和密码子-反密码子相互作用中独立错误的随机组合而增强:tRNA 错酰化可能会改变反密码子不匹配的潜力,也许特别是增加了与错配非同源氨基酸编码的密码子不匹配的潜力。这种假设的现象称为“错误协调”,与假设反密码子-密码子不匹配之间独立性的“错误补偿”不同。
最终,应该通过比较由相应氨基酸加载的 tRNA 形成的错配密码子-反密码子双链体的稳定性或频率与该 tRNA 错误加载由错配密码子编码的氨基酸时形成的稳定性,来检验每种氨基酸错酰化和密码子-反密码子不匹配组合的假说。竞争错配实验,比较错误加载和正确加载的 tRNA 也可能有用,但更复杂的实验。
检测错误协调意味着估计错误补偿,这也促进了蛋白质合成的准确性。因此,即使没有错误协调的证据,实验也会对错酰化和错配过程产生非常有用的见解。如果实验考虑转录后 RNA 修饰(特别是在摆动位置),则关于密码子-反密码子不匹配的结果将能够显著改进和完善二级结构预测软件。阳性结果表明,蛋白质翻译提高了产物的准确性,而不是提高了产物产生过程中的单个步骤的准确性。古老的翻译机制据称优化了错误协调,特别是在 tRNA 合成酶进化之前对 tRNA 进行编辑之后:少数原始但功能多样的 tRNA 可能执行了低精度的翻译。为低复杂度和高效率而人工设计/选择的系统可以利用这种具有高错误补偿和协调水平的反密码子的特性。
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