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基于固定在氧化石墨烯修饰聚合物微球上的胰蛋白酶的酶反应器,实现蛋白质组的自动定量分析。

Enzymatic Reactor with Trypsin Immobilized on Graphene Oxide Modified Polymer Microspheres To Achieve Automated Proteome Quantification.

机构信息

CAS Key Laboratory of Separation Sciences for Analytical Chemistry, National Chromatographic R & A Center, Dalian Institute of Chemical Physics, Chinese Academy of Sciences , Dalian 116023, China.

University of Chinese Academy of Sciences , Beijing 100049, China.

出版信息

Anal Chem. 2017 Jun 20;89(12):6324-6329. doi: 10.1021/acs.analchem.7b00682. Epub 2017 Jun 1.

Abstract

Protein digestion and isotope labeling are two critical steps in proteome quantification. However, the conventional in-solution protocol unavoidably suffers from disadvantages such as time-consuming, low labeling efficiency, and tedious off-line manual operation, which might affect the quantification accuracy, reproducibility, and throughput. To address these problems, we developed a fully automated proteome quantification platform, in which an ultraperformance immobilized microreactor (upIMER) with graphene-oxide-modified polymer microspheres as the matrix was developed, to achieve not only the simultaneous protein digestion and O labeling, but also the online integration with nano-high-pressure liquid chromatography-electrospray ionization-tandem mass spectrometry (nanoHPLC-ESI-MS/MS). Compared to the conventional off-line protocols, such a platform exhibits obviously improved digestion and O labeling efficiency (only 8% peptides with missed cleavage sites, 99% labeling efficiency, and 2.5 min reaction time), leading to the increased quantification coverage, accuracy, precision and throughput. All the results demonstrated that our developed fully automated platform should provide new opportunities to improve the accuracy, reproducibility, and throughput for proteome quantification.

摘要

蛋白质消化和同位素标记是蛋白质组定量的两个关键步骤。然而,传统的溶液内方案不可避免地存在耗时、标记效率低和繁琐的离线手动操作等缺点,这可能会影响定量的准确性、重现性和通量。为了解决这些问题,我们开发了一种全自动蛋白质组定量平台,其中开发了一种超高性能的固定化微反应器(upIMER),其基质为氧化石墨烯修饰的聚合物微球,不仅可以实现蛋白质的同步消化和 O 标记,还可以与纳升高效液相色谱-电喷雾串联质谱(nanoHPLC-ESI-MS/MS)在线集成。与传统的离线方案相比,该平台显示出明显提高的消化和 O 标记效率(仅 8%的肽有未切割位点,99%的标记效率和 2.5 分钟的反应时间),从而提高了定量的覆盖度、准确性、精密度和通量。所有结果表明,我们开发的全自动平台应为提高蛋白质组定量的准确性、重现性和通量提供新的机会。

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