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Proteomics-based Refinement of Deinococcus deserti Genome Annotation Reveals an Unwonted Use of Non-canonical Translation Initiation Codons

机译:基于蛋白质组学的Deinococcus deserti基因组注释的精炼揭示了非经典翻译起始密码子的未经授权的使用

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摘要

Deinococcaceae are a family of extremely radiation-tolerant bacteria that are currently subjected to numerous studies aimed at understanding the molecular mechanisms for such radiotolerance. To achieve a comprehensive and accurate annotation of the Deinococcus deserti genome, we performed an N terminus-oriented characterization of its proteome. For this, we used a labeling reagent, N-tris(2,4,6-trimethoxyphenyl)phosphonium acetyl succinimide, to selectively derivatize protein N termini. The large scale identification of N-tris(2,4,6-trimethoxyphenyl)phosphonium acetyl succinimide-modified N-terminal-most peptides by shotgun liquid chromatography-tandem mass spectrometry analysis led to the validation of 278 and the correction of 73 translation initiation codons in the D. deserti genome. In addition, four new genes were detected, three located on the main chromosome and one on plasmid P3. We also analyzed signal peptide cleavages on a genome-wide scale. Based on comparative proteogenomics analysis, we propose a set of 137 corrections to improve Deinococcus radiodurans and Deinococcus geothermalis gene annotations. Some of these corrections affect important genes involved in DNA repair mechanisms such as polA, ligA, and ddrB. Surprisingly, experimental evidences were obtained indicating that DnaA (the protein involved in the DNA replication initiation process) and RpsL (the S12 ribosomal conserved protein) translation is initiated in Deinococcaceae from non-canonical codons (ATC and CTG, respectively). Such use may be the basis of specific regulation mechanisms affecting replication and translation. We also report the use of non-conventional translation initiation codons for two other genes: Deide_03051 and infC. Whether such use of non-canonical translation initiation codons is much more frequent than for other previously reported bacterial phyla or restricted to Deinococcaceae remains to be investigated. Our results demonstrate that predicting translation initiation codons is still difficult for some bacteria and that proteomics-based refinement of genome annotations may be helpful in such cases.
机译:狄氏球菌科是一类极耐辐射的细菌,目前正进行大量旨在了解这种耐辐射性分子机制的研究。为了获得沙漠迪诺球菌基因组的全面而准确的注释,我们对其蛋白质组进行了面向N末端的表征。为此,我们使用了标记试剂,N-三(2,4,6-三甲氧基苯基)phosph乙酰琥珀酰亚胺,选择性地衍生蛋白质N末端。 shot弹枪液相色谱-串联质谱分析法大规模鉴定N-三(2,4,6-三甲氧基苯基)乙酰琥珀酰亚胺修饰的N-末端最末端的肽导致278的验证和73翻译起始的校正D. deserti基因组中的密码子。此外,检测到四个新基因,三个位于主染色体上,一个位于质粒P3上。我们还在全基因组范围内分析了信号肽的裂解。在比较蛋白质组学分析的基础上,我们提出了一组137个更正,以改善Radiodurans球菌和Geothermalis球菌的基因注释。其中一些校正会影响涉及DNA修复机制的重要基因,例如polA,ligA和ddrB。令人惊讶的是,获得的实验证据表明,在Dinococcaceae中从非规范密码子(分别为ATC和CTG)启动了DnaA(参与DNA复制起始过程的蛋白质)和RpsL(S12核糖体保守蛋白质)的翻译。这种使用可能是影响复制和翻译的特定调控机制的基础。我们还报告了使用非常规翻译起始密码子用于另外两个基因:Deide_03051和infC。这种非规范翻译起始密码子的使用是否比其他先前报道的细菌门更为频繁或仅限于迪诺球菌科尚待研究。我们的结果表明,对于某些细菌而言,预测翻译起始密码子仍然很困难,并且在这种情况下,基于蛋白质组学的基因组注释改进可能会有所帮助。

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