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Experimental determination of translational starts using peptide mass mapping and tandem mass spectrometry within the proteome of Mycobacterium tuberculosis

机译:在结核分枝杆菌蛋白质组中使用肽质量测绘和串联质谱法的转化型开始实验测定

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Identification of protein translation start sites is largely a bioinformatics exercise, with relatively few confirmed by N-terminal sequencing. Translation start site determination is critical for defining both the protein sequence and the upstream DNA which may contain regulatory motifs. It is demonstrated here that translation start sites can be determined during routine protein identification, using MALDI-MS and MS/MS data to select the correct N-terminal sequence from a list of alternatives generated in silico. Applying the method to 13 proteins from Mycobacterium tuberculosis, 11 predicted translational start sites were confirmed, and two reassigned. The authors suggest that these data (be they confirmation or reassignments) are important for the annotation of both this genome and those of organisms with related genes. It was also shown that N-acetylation, reported to be rare in prokaryotes, was present in three of the 13 proteins (23?%), suggesting that in the mycobacteria this modification may be common, and an important regulator of protein function, although more proteins need to be analysed. This method can be performed with little or no additional experimental work during proteomics investigations.
机译:蛋白翻译起始位点的鉴定主要是生物信息学锻炼,通过N-末端测序确认相对较少。翻译开始部位测定对于定义可能含有调节基序的蛋白质序列和上游DNA至关重要。这里证明了,可以在常规蛋白质识别期间使用MALDI-MS和MS / MS数据来确定翻译开始站点,以从硅中产生的替代品列表中选择正确的N末端序列。将方法应用于13例蛋白质从结核分枝杆菌中,确认了11个预测的平移起始网站,并进行了两次重新分配。作者认为,这些数据(他们确认或重新分配)对于诠释这两个基因组和具有相关基因的生物体是重要的。还表明,据报道的N-乙酰化是在原核生物中罕见的,存在于13个蛋白质中的三种(23μl)中存在,表明在该修饰中,该修饰可能是常见的,并且蛋白质功能的重要调节因素需要分析更多的蛋白质。该方法可以在蛋白质组学研究期间几乎没有或没有额外的实验工作进行。

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