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Use of shotgun proteomics for the identification confirmation and correction of C. elegans gene annotations

机译:shot弹枪蛋白质组学用于秀丽隐杆线虫基因注释的鉴定确认和校正

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摘要

We describe a general mass spectrometry-based approach for gene annotation of any organism and demonstrate its effectiveness using the nematode Caenorhabditis elegans. We detected 6779 C. elegans proteins (67,047 peptides), including 384 that, although annotated in WormBase WS150, lacked cDNA or other prior experimental support. We also identified 429 new coding sequences that were unannotated in WS150. Nearly half (192/429) of the new coding sequences were confirmed with RT-PCR data. Thirty-three (∼8%) of the new coding sequences had been predicted to be pseudogenes, 151 (∼35%) reveal apparent errors in gene models, and 245 (57%) appear to be novel genes. In addition, we verified 6010 exon–exon splice junctions within existing WormBase gene models. Our work confirms that mass spectrometry is a powerful experimental tool for annotating sequenced genomes. In addition, the collection of identified peptides should facilitate future proteomics experiments targeted at specific proteins of interest.
机译:我们描述了一种基于通用质谱法的任何生物基因注释方法,并证明了使用线虫秀丽隐杆线虫的有效性。我们检测到6779个秀丽隐杆线虫蛋白(67,047个肽段),其中384个虽然在WormBase WS150中进行了注释,但缺少cDNA或其他先前的实验支持。我们还确定了WS150中未注释的429个新编码序列。 RT-PCR数据确认了将近一半(192/429)的新编码序列。已有33(〜8%)个新的编码序列被预测为假基因,其中151个(〜35%)揭示了基因模型中的明显错误,而245个(57%)则是新基因。此外,我们在现有WormBase基因模型中验证了6010个外显子-外显子剪接点。我们的工作证实了质谱法是用于注释测序基因组的强大实验工具。此外,已鉴定肽的收集应有助于将来针对特定目的蛋白质的蛋白质组学实验。

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