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Verification of Ribosomal Proteins of Aspergillus fumigatus for Use as Biomarkers in MALDI-TOF MS Identification

机译:验证烟曲霉核糖体蛋白用作MALDI-TOF MS鉴定的生物标志物

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摘要

We have previously proposed a rapid identification method for bacterial strains based on the profiles of their ribosomal subunit proteins (RSPs), observed using matrix-assisted laser desorption/ionization time-of-flight mass spectrometry (MALDI-TOF MS). This method can perform phylogenetic characterization based on the mass of housekeeping RSP biomarkers, ideally calculated from amino acid sequence information registered in public protein databases. With the aim of extending its field of application to medical mycology, this study investigates the actual state of information of RSPs of eukaryotic fungi registered in public protein databases through the characterization of ribosomal protein fractions extracted from genome-sequenced Aspergillus fumigatus strains Af293 and A1163 as a model. In this process, we have found that the public protein databases harbor problems. The RSP names are in confusion, so we have provisionally unified them using the yeast naming system. The most serious problem is that many incorrect sequences are registered in the public protein databases. Surprisingly, more than half of the sequences are incorrect, due chiefly to mis-annotation of exon/intron structures. These errors could be corrected by a combination of in silico inspection by sequence homology analysis and MALDI-TOF MS measurements. We were also able to confirm conserved post-translational modifications in eleven RSPs. After these verifications, the masses of 31 expressed RSPs under 20,000 Da could be accurately confirmed. These RSPs have a potential to be useful biomarkers for identifying clinical isolates of A. fumigatus.
机译:我们先前已经提出了一种基于细菌核糖体亚单位蛋白(RSPs)的特征的细菌菌株的快速鉴定方法,该方法使用基质辅助激光解吸/电离飞行时间质谱(MALDI-TOF MS)进行观察。该方法可以根据看家RSP生物标志物的质量进行系统发育鉴定,理想情况下是根据在公共蛋白质数据库中注册的氨基酸序列信息计算得出的。为了扩展其在医学真菌学中的应用范围,本研究通过对从基因组测序的烟曲霉Af293和A1163菌株中提取的核糖体蛋白级分进行表征,研究了在公共蛋白质数据库中注册的真核真菌RSP的实际信息状态。一个模型。在此过程中,我们发现公共蛋白质数据库存在问题。 RSP名称混乱,因此我们已使用酵母命名系统临时将其统一。最严重的问题是在公共蛋白质数据库中注册了许多不正确的序列。令人惊讶地,主要由于外显子/内含子结构的错误注释,导致一半以上的序列不正确。这些错误可以通过序列同源性分析和MALDI-TOF MS测量进行的计算机检测相结合来纠正。我们还能够确认11个RSP中保守的翻译后修饰。经过这些验证,可以准确确认20,000 Da以下31个表达的RSP的质量。这些RSPs可能是有用的生物标志物,用于鉴定烟曲霉的临床分离株。

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