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In-depth reproducible analysis of human plasma using IgY 14 and SuperMix Immunodepletion

机译:使用IgY 14和SuperMix免疫扩增对人类血浆进行深入可重现的分析

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摘要

Identification of cancer and other disease biomarkers in human plasma has been exceptionally challenging due to the complex nature of plasma, and the presence of a moderate number of high- and medium- abundance proteins which mask low abundance proteins of interest. As a result, immunoaffinity depletion formats combining multiple antibodies to target the most abundant plasma proteins have become the first stage in most plasma proteome discovery schemes. This protocol describes the use of tandem IgY 14 and SuperMix immunoaffinity depletion to reproducibly remove > 99% of total plasma protein. This greatly increases the depth of analysis of human plasma proteomes. Depleted plasma samples can then be analyzed in a single high resolution LC-MS/MS run on a Q-Exactive Plus mass spectrometer, followed by label-free quantitation. If greater depth of analysis is desired the depleted plasma can be further fractionated by separating the sample for a short distance on a 1D SDS gel and cuting the gel into uniform slices prior to trypsin digestion. Alternatively, the depleted plasma can be reduced, alkylated, digested with trypsin followed by high pH reverse phase HPLC separation.
机译:由于血浆的复杂性以及适度数量的掩盖低丰度目标蛋白质的高和中度丰度蛋白质的存在,在人血浆中鉴定癌症和其他疾病生物标记物一直是极具挑战性的。结果,结合多种抗体以靶向最丰富的血浆蛋白的免疫亲和力消耗形式已成为大多数血浆蛋白质组发现方案的第一步。该方案描述了串联IgY 14和SuperMix免疫亲和力消耗法可重复去除> 99%的总血浆蛋白的用途。这极大地增加了人类血浆蛋白质组的分析深度。然后可以在Q-Exactive Plus质谱仪上运行的单个高分辨率LC-MS / MS中分析耗尽的血浆样品,然后进行无标记定量。如果需要更大的分析深度,则可以通过在1D SDS凝胶上将样品分离一小段距离,然后在进行胰蛋白酶消化之前将凝胶切成均匀的切片,来进一步分离消耗的血浆。或者,可以将消耗的血浆还原,烷基化,用胰蛋白酶消化,然后进行高pH反相HPLC分离。

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