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Spatially-Directed Protein Identification from Tissue Sections by Top-Down LC-MS/MS with Electron Transfer Dissociation

机译:通过自上而下的LC-MS / MS和电子转移解离从组织切片中进行空间定向的蛋白质鉴定

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摘要

MALDI imaging mass spectrometry (MALDI-IMS) has become a powerful tool for localizing both small molecules and intact proteins in a wide variety of tissue samples in both normal and diseased states. Identification of imaged signals in MALDI-IMS remains a bottleneck in the analysis and limits the interpretation of underlying biology of tissue specimens. In this work, spatially directed tissue microextraction of intact proteins followed by LC-MS/MS with electron transfer dissociation (ETD) was used to identify proteins from specific locations in three tissue types; ocular lens, brain, and kidney. Detection limits were such that a 1 μL extraction volume was sufficient to deliver proteins to the LC-MS/MS instrumentation with sufficient sensitivity to detect 50-100 proteins in a single experiment. Additionally, multiple modified proteins were identified; including truncated lens proteins that would be difficult to assign to an imaged mass using a bottom-up approach. Protein separation and identification are expected to improve with advances in intact protein fractionation/chromatography and advances in interpretation algorithms leading to increased depth of proteome coverage from distinct tissue locations.
机译:MALDI成像质谱仪(MALDI-IMS)已成为在正常和患病状态下定位各种组织样本中的小分子和完整蛋白的强大工具。 MALDI-IMS中成像信号的识别仍然是分析的瓶颈,并限制了对组织标本生物学的解释。在这项工作中,完整蛋白质的空间定向组织微提取,然后通过带有电子转移解离(ETD)的LC-MS / MS用于从三种组织类型的特定位置鉴定蛋白质。眼镜,大脑和肾脏。检测限为1μL的提取量足以将蛋白质递送至LC-MS / MS仪器,并具有足够的灵敏度以在单个实验中检测50-100种蛋白质。另外,鉴定了多种修饰的蛋白;包括使用自下而上的方法难以分配给成像质量的截短的晶状体蛋白。随着完整蛋白质分级分离/色谱技术的进步和解释算法的发展,蛋白质的分离和鉴定有望得到改善,从而导致蛋白质组覆盖不同组织位置的深度增加。

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