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首页> 外文期刊>Journal of proteome research >Moving away from the reference genome: Evaluating a peptide sequencing tagging approach for single amino acid polymorphism identifications in the genus populus
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Moving away from the reference genome: Evaluating a peptide sequencing tagging approach for single amino acid polymorphism identifications in the genus populus

机译:远离参考基因组:评估一种用于杨属中单个氨基酸多态性鉴定的肽序列标记方法

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摘要

The genetic diversity across natural populations of the model organism, Populus, is extensive, containing a single nucleotide polymorphism roughly every 200 base pairs. When deviations from the reference genome occur in coding regions, they can impact protein sequences. Rather than relying on a static reference database to profile protein expression, we employed a peptide sequence tagging (PST) approach capable of decoding the plasticity of the Populus proteome. Using shotgun proteomics data from two genotypes of P. trichocarpa, a tag-based approach enabled the detection of 6653 unexpected sequence variants. Through manual validation, our study investigated how the most abundant chemical modification (methionine oxidation) could masquerade as a sequence variant (Ala→Ser) when few site-determining ions existed. In fact, precise localization of an oxidation site for peptides with more than one potential placement was indeterminate for 70% of the MS/MS spectra. We demonstrate that additional fragment ions made available by high energy collisional dissociation enhances the robustness of the peptide sequence tagging approach (81% of oxidation events could be exclusively localized to a methionine). We are confident that augmenting fragmentation processes for a PST approach will further improve the identification of single amino acid polymorphism in Populus and potentially other species as well.
机译:模式生物自然种群胡杨的遗传多样性是广泛的,大约每200个碱基对包含一个核苷酸多态性。当在编码区发生与参考基因组的偏离时,它们会影响蛋白质序列。我们不是依靠静态参考数据库来分析蛋白质表达,而是采用了能够解码Populus蛋白质组可塑性的肽序列标签(PST)方法。利用来自两个毛果单胞菌基因型的shot弹枪蛋白质组学数据,基于标签的方法能够检测到6653个意想不到的序列变体。通过手动验证,我们的研究调查了在很少存在定点离子的情况下,如何将最丰富的化学修饰(蛋氨酸氧化)伪装成序列变体(Ala→Ser)。实际上,对于70%的MS / MS光谱来说,具有多个潜在位置的多肽的氧化位点的精确定位是不确定的。我们证明了通过高能碰撞解离可获得的其他碎片离子增强了肽序列标记方法的鲁棒性(81%的氧化事件可以专门定位于蛋氨酸)。我们相信,为PST方法增加片段化过程将进一步改善对胡杨和其他潜在物种中单个氨基酸多态性的鉴定。

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