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18O掺入的蛋白水解标记优化及回交换抑制的考量

Considerations for proteolytic labeling-optimization of 18O incorporation and prohibition of back-exchange.

作者信息

Storms Henricus F, van der Heijden Robert, Tjaden Ubbo R, van der Greef Jan

机构信息

Division of Analytical Biosciences, Leiden/Amsterdam Center for Drug Research, P.O. Box 9502, 2300 RA Leiden, The Netherlands.

出版信息

Rapid Commun Mass Spectrom. 2006;20(23):3491-7. doi: 10.1002/rcm.2738.

Abstract

Proteolytic (18)O labeling is a very powerful tool for differential analysis applied to proteome studies. However, it is a relatively new technique and the optimization of the labeling process still needs some attention. We found that the two-step post-proteolytic labeling should be favored over the conventional digestion of proteins in H(2) (18)O, since the former allows for higher sample concentrations and thus more favorable kinetics. It was demonstrated that the inhibitory effect of urea on (18)O incorporation could be compensated by the use of higher sample concentrations. Furthermore, it was shown that heat-deactivation of trypsin prevents (18)O/(16)O back-exchange. In addition, no non-specific hydrolysis of the peptides could be observed as a result of the heating. Heat inactivation of trypsin opens the way for the use of capillary electrophoresis as a separation technique in proteolytic labeling studies, as it abolishes the need for use of detrimental additives. Analysis of a labeled protein digest by capillary isoelectric focusing/mass spectrometry showed the applicability of the method. No back-exchange was observed across the entire electropherogram.

摘要

蛋白水解(18)O标记是蛋白质组研究中用于差异分析的一种非常强大的工具。然而,这是一项相对较新的技术,标记过程的优化仍需关注。我们发现,两步蛋白水解后标记应优于在H(2)(18)O中对蛋白质进行常规消化,因为前者允许更高的样品浓度,从而具有更有利的动力学。结果表明,使用更高的样品浓度可以补偿尿素对(18)O掺入的抑制作用。此外,研究表明胰蛋白酶的热失活可防止(18)O/(16)O反向交换。另外,加热未观察到肽的非特异性水解。胰蛋白酶的热失活为在蛋白水解标记研究中使用毛细管电泳作为分离技术开辟了道路,因为它消除了使用有害添加剂的必要性。通过毛细管等电聚焦/质谱对标记蛋白消化物进行分析表明了该方法的适用性。在整个电泳图中均未观察到反向交换。

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