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Improved Molecular Weight-Based Processing of Intact Proteins for Interrogation by Quadrupole-Enhanced FT MS/MS

机译:通过四极杆增强的FT MS / MS改进的基于分子量的完整蛋白处理方法用于询问

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摘要

Complete coverage of protein primary structure is demonstrated for 37 yeast protein forms between 6 and 30 kDa in an improved platform for Top Down mass spectrometry (MS). Tandem mass spectrometry (MS/MS) for protein identification with 100% sequence coverage is achieved in a highly automated fashion with 15–300-fold less sample amounts than an initial report of a proteome fractionation approach employing preparative gel electrophoresis with an acid-labile surfactant to facilitate reversed phase separation in a second dimension. Using a quadrupole-enhanced Fourier Transform Ion Cyclotron Resonance Mass Spectrometer (FTICRMS) improves the dynamic range for protein detection by ~50-fold and MS/MS by ~30-fold. The technology development illustrated here typifies an accelerating effort to detect whole proteins in a more general and higher throughput fashion for improved biomarker identification and detection of diverse post-translational modifications. Capillary RPLC is used in both off-line and on-line modes, with one on-line LC/FTMS sample providing 25 observed protein forms from 11 to 22 kDa.
机译:在改良的Top Down质谱(MS)平台中,证明了6至30 kDa之间的37种酵母蛋白质形式完全覆盖了蛋白质一级结构。串联质谱(MS / MS)以高度自动化的方式实现了100%序列覆盖率的蛋白质鉴定,其样品量比采用制备凝胶电泳和对酸不稳定的蛋白质组分馏方法的最初报告少了15-300倍在第二维中促进反相分离的表面活性剂。使用四极增强型傅立叶变换离子回旋加速器共振质谱仪(FTICRMS)可将蛋白质检测的动态范围提高约50倍,将MS / MS的动态范围提高约30倍。此处说明的技术发展代表了加快工作的步伐,即以更通用和更高通量的方式检测全蛋白,以改善生物标志物的识别和各种翻译后修饰的检测。毛细管RPLC可用于离线和在线两种模式,其中一个在线LC / FTMS样品可提供25种观察到的11至22 kDa的蛋白质形式。

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