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Use of O-18 labels to monitor deamidation during protein and peptide sample processing

机译:使用O-18标签监测蛋白质和多肽样品处理过程中的脱酰胺作用

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Nonenzymatic deamidation of asparagine residues in proteins generates aspartyl (Asp) and isoaspartyl (isoAsp) residues via a succinimide intermediate in a neutral or basic environment. Electron capture dissociation (ECD) can differentiate and quantify the relative abundance of these isomeric products in the deamidated proteins. This method requires the proteins to be digested, usually by trypsin, into peptides that are amenable to ECD. ECD of these peptides can produce diagnostic ions for each isomer; the c. + 58 and z - 57 fragment ions for the isoAsp residue and the fragment ion ((M + nH) ((n-l)+.) - 60) corresponding to the side-chain loss from the Asp residue. However, deamidation can also occur as an artifact during sample preparation, particularly when using typical tryptic digestion protocols. With O-18 labeling, it is possible to differentiate deamidation occurring during trypsin digestion which causes a +3 Da (O-18(1)+ 1D) mass shift from the pre-existing deamidation, which leads to a +1-Da mass shift. This paper demonstrates the use of O-18 labeling to monitor three rapidly deamidating peptides released from proteins (calmodulin, ribonuclease A, and lysozyme) during the time course of trypsin digestion processes, and shows that the fast ((similar to)4 h) trypsin digestion process generates no additional detectable peptide deamidations.
机译:蛋白质中天冬酰胺残基的非酶脱酰胺作用会在中性或碱性环境中通过琥珀酰亚胺中间体产生天冬氨酰(Asp)和异天冬氨酰(isoAsp)残基。电子捕获解离(ECD)可以区分和量化脱酰胺化蛋白质中这些异构产物的相对丰度。该方法要求通常通过胰蛋白酶将蛋白质消化成适合ECD的肽。这些肽的ECD可以为每种异构体产生诊断离子。 c。 isoAsp残基的+ 58和z-57片段离子和对应于Asp残基侧链损失的片段离子((M + nH)((n-1)+。)-60)。但是,脱酰胺作用也可能在样品制备过程中作为伪影发生,特别是在使用典型的胰蛋白酶消化方案时。使用O-18标记,可以区分在胰蛋白酶消化过程中发生的脱酰胺作用,该过程导致质量+3 Da(O-18(1)+ 1D)与先前的脱酰胺作用产生质量偏移,从而导致+ 1-Da的质量转移。本文证明了在胰蛋白酶消化过程中使用O-18标记监测从蛋白质释放的三种快速脱酰胺肽(钙调蛋白,核糖核酸酶A和溶菌酶)的过程,并显示了快速((相似)4 h)胰蛋白酶消化过程不会产生其他可检测的肽脱酰胺作用。

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