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Software for top-down proteomic identification of a plasmid-borne factor (and other proteins) from genomically sequenced pathogenic bacteria using MALDI-TOF-TOF-MS/MS and post-source decay

机译:使用MALDI-TOF-TOF-MS / MS和源极衰减的基因组排序的致病细菌的质粒传播系数(和其他蛋白质)的自上蛋白质组鉴定的软件

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A plasmid-borne factor (hypothetical protein) was identified in three Shiga toxin-producing Escherichia coli O113:H21 strains using antibiotic-induction, MALDI-TOF-TOF tandem mass spectrometry (MS/MS), post-source decay (PSD) and top-down proteomic analysis. The plasmid-encoded factor was identified from three pairs of complementary fragment ions (b/y) which were also used to obtain a more accurate calculation of the mass of the protein than that possible from MS analysis. A software application tool was developed to rapidly search amino acid sequences from whole genome sequencing-derived data to match the observed protein mass and fragment ions on the assumption that the fragment ions are the result of polypeptide backbone cleavage on the C-terminal side of aspartic acid and glutamic acid residues, i.e. aspartic acid effect. Manual inspection and top-down proteomic analysis confirmed the correctness of the identification of this protein using this new application tool. Although the function of the plasmid-borne factor is not known, its antibiotic-induced expression may suggest a role in antimicrobial stress. This approach was also used to identify three highly conserved bacterial cold-shock proteins: CspC, CspE, CsbD from one of the STEC strains. In addition to polypeptide backbone cleavage, metastable CsbD showed multiple small dissociative losses perhaps suggesting ammonia loss from the four arginine residues in its sequence. This phenomenon had been previously observed for metastable ubiquitin which also has four arginine residues. Published by Elsevier B.V.
机译:使用抗生素诱导,MALDI-TOF-TOF串联质谱(MS / MS),源极衰减(PSD)和自上而下的蛋白质组学分析。从三对互补片段(B / Y)鉴定了质粒编码因子,其还用于获得比MS分析的质量更准确地计算蛋白质的质量。开发了一种软件应用工具以从全基因组测序衍生数据中迅速搜索氨基酸序列,以匹配观察到的蛋白质质量和片段离子,假设片段离子是多肽骨干裂解在天冬氨酸的C末端侧的结果酸和谷氨酸残基,即天冬氨酸效应。手动检测和自上而下的蛋白质组学分析证实了使用这种新应用工具鉴定该蛋白质的正确性。虽然质粒归因因子的功能尚不清楚,但其抗生素诱导的表达可能表明在抗微生物应激中的作用。这种方法也用于鉴定三种高度保守的细菌冷冲击蛋白:CSPC,CSPE,来自STEC菌株之一的CSPD。除了多肽骨干裂解外,亚稳态CSBD还显示出多种小的分离损失,也许可能表明在其序列中的四个精氨酸残留物中的氨损失。此前已经观察到这种现象用于亚稳泛素,其还具有四种精氨酸残基。 elsevier b.v出版。

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