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MeCAT peptide labeling for the absolute quantification of proteins by 2D-LC-ICP-MS

机译:MeCAT肽标记可通过2D-LC-ICP-MS对蛋白质进行绝对定量

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摘要

Metal-Coded Affinity Tags (MeCAT) reagents were devised for the absolute quantification of labeled proteins and peptides using inductively coupled plasma mass spectrometry (ICP-MS). After the recent publication of quantification approaches for digested proteins, this work presents a multidimensional strategy for the application of MeCAT to samples which require higher chromatographic resolution. Two-dimensional separations based on strong cation exchange (SCX) and reversed-phase (RP) chromatography, were used for the quantification of lysozyme, bovine serum albumin and transferrin after tryptic digestion. The elution protocols were optimized to improve the resolution of the MeCAT-labeled peptides which led to faster elutions in SCX and longer retention times in RP compared with unlabeled peptides. The optimized method provided enough resolution for the samples analyzed. Peptides losses during the whole procedure were studied. Although recoveries of greater than 90% were found in the RP dimension, important global losses in the two-dimensional offline approach forced us to use specific internal standards, in this case MeCAT-labeled standard peptides. External calibration and label-specific isotope dilution analysis (IDA) were tested and compared as possible quantification techniques. While both techniques showed accurate and precise determinations, the label-specific IDA technique resulted in more straightforward measurements and more affordable external calibrations. Finally, simultaneous quantification of three different samples labeled with different lanthanides was successfully performed demonstrating the potential of MeCAT combined with ICP-MS for multiplexing. Electrospray ionization mass spectrometry techniques provided the structural information needed for the identification of the labeled species.
机译:设计了金属编码的亲和标签(MeCAT)试剂,用于使用电感耦合等离子体质谱(ICP-MS)绝对定量标记的蛋白质和多肽。在最近发表了针对消化蛋白质的定量方法的出版物之后,这项工作提出了将MeCAT应用到需要更高色谱分辨率的样品的多维策略。胰蛋白酶消化后,基于强阳离子交换(SCX)和反相(RP)色谱的二维分离用于定量溶菌酶,牛血清白蛋白和转铁蛋白。优化洗脱方案以提高MeCAT标记的肽的分离度,与未标记的肽相比,可导致SCX的洗脱速度更快,RP的保留时间更长。优化的方法为所分析的样品提供了足够的分辨率。研究了整个过程中的肽损失。尽管在RP方面发现了90%以上的回收率,但是二维离线方法中的重大全球损失迫使我们使用特定的内标,在这种情况下为MeCAT标记的标准肽。测试了外部校准和标记特异性同位素稀释分析(IDA),并比较了可能的定量技术。虽然这两种技术都显示出准确而精确的测定结果,但特定于标签的IDA技术可实现更直接的测量和更实惠的外部校准。最后,成功地同时量化了三个标有不同镧系元素的不同样品,证明了MeCAT与ICP-MS联用的潜力。电喷雾电离质谱技术提供了识别标记物种所需的结构信息。

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