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Nearly 1000 protein identifications from 50 ng of Xenopus laevis zygote homogenate using on-line sample preparation on a strong cation exchange monolith-based microreactor coupled with capillary zone electrophoresis

机译:使用基于阳离子交换整体柱的微型反应器和毛细管区带电泳的在线样品制备方法从50 ng非洲爪蟾合子匀浆中鉴定出近1000种蛋白质

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摘要

A sulfonate-silica hybrid strong cation exchange monolith microreactor was synthesized and coupled to a linear polyacrylamide coated capillary for online sample preparation and capillary zone electrophoresis-tandem mass spectrometry (CZE-MS/MS) bottom-up proteomic analysis. The protein sample was loaded onto the microreactor in an acidic buffer. After online reduction, alkylation, and digestion with trypsin, the digests were eluted with 200 mM ammonium bicarbonate at pH 8.2 for CZE-MS/MS analysis using 1 M acetic acid as the background electrolyte. This combination of basic elution and acidic background electrolytes results in both sample stacking and formation of a dynamic pH junction. 369 protein groups and 1,274 peptides were identified from 50 ng of Xenopus laevis zygote homogenate, which is comparable with an offline sample preparation method, but the time required for sample preparation was decreased from over 24 h to less than 40 min. Dramatically improved performance was produced by coupling the reactor to a longer separation capillary (~100 cm) and a Q Exactive HF mass spectrometer. 975 protein groups and 3,749 peptides were identified from 50 ng Xenopus protein using the online sample preparation method.
机译:合成了磺酸盐-二氧化硅杂化的强阳离子交换整体式微反应器,并与线性聚丙烯酰胺包被的毛细管偶联,用于在线样品制备和毛细管区带电泳-串联质谱(CZE-MS / MS)自下而上的蛋白质组学分析。将蛋白质样品在酸性缓冲液中上样至微反应器。在线还原,烷基化并用胰蛋白酶消化后,将消化液用pH 8.2的200 mM碳酸氢铵洗脱,用于CZE-MS / MS分析,使用1 M乙酸作为背景电解质。碱性洗脱液和酸性背景电解质的这种结合会导致样品堆积和形成动态pH结。从50 ng非洲爪蟾合子匀浆中鉴定出369个蛋白质组和1,274个肽段,与离线样品制备方法相当,但是样品制备所需的时间从24小时以上减少到不到40分钟。通过将反应器连接到更长的分离毛细管(〜100 cm)和Q Exactive HF质谱仪上,可以显着提高性能。使用在线样品制备方法从50 ng非洲爪蟾蛋白中鉴定出975个蛋白质组和3,749个肽。

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