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通过含有肽键模型的两亲物胶束中的化学捕获,同时测定酰胺键、羧酸盐基团和水的界面摩尔浓度。

Simultaneous determination of interfacial molarities of amide bonds, carboxylate groups, and water by chemical trapping in micelles of amphiphiles containing peptide bond models.

机构信息

Department of Chemistry and Chemical Biology, Wright-Rieman Laboratories, Rutgers, The State University of New Jersey, New Brunswick, New Jersey 08903, United States.

出版信息

Langmuir. 2013 Jan 15;29(2):534-44. doi: 10.1021/la3040819. Epub 2012 Dec 31.

DOI:10.1021/la3040819
PMID:23237147
Abstract

Chemical trapping is a powerful approach for obtaining experimental estimates of interfacial molarities of weakly basic nucleophiles in the interfacial regions of amphiphile aggregates. Here, we demonstrate that the chemical probe 4-hexadecyl-2,6-dimethylbenzenediazonium ion (16-ArN(2)(+)) reacts competitively with interfacial water, with the amide carbonyl followed by cleavage of the headgroups from the tail at the amide oxygen, and with the terminal carboxylate groups in micelles of two N-acyl amino-acid amphiphiles, sodium N-lauroylsarcosinate (SLS) and sodium N-lauroylglycinate (SLG), simple peptide bond model amphiphiles. Interfacial molarities (in moles per liter of interfacial volume) of these three groups were obtained from product yields, assuming that selectivity toward a particular nucleophile compared to water is the same in an aqueous reference solution and in the interfacial region. Interfacial carboxylate group molarities are 1.5 M in both SLS and SLG micelles, but the concentration of the amide carbonyl for SLS micelles is ~4.6-5 times less (ca. 0.7 M) than that of SLG micelles (3 M). The proton on the secondary N of SLG helps solubilize the amide bond in the aqueous region, but the methyl on the tertiary N of SLS helps solubilize the amide bond in the micellar core, reducing its reaction with 16-ArN(2)(+). Application of chemical trapping to proteins in membrane mimetic interfaces should provide insight into the topology of the protein within the interface because trapping of the amide carbonyl and cleavage at the C-N bond occurs only within the interface, and fragment characterization marks those peptide bonds located within the interface.

摘要

化学捕获是一种获取两亲分子聚集界面区域中弱碱性亲核试剂界面摩尔浓度实验估计值的有效方法。在这里,我们证明了化学探针 4-十六烷基-2,6-二甲基苯重氮离子(16-ArN(2)(+))与界面水竞争反应,酰胺羰基随后在酰胺氧处断裂头基,与两种 N-酰基氨基酸两亲物,即月桂酰基肌氨酸钠(SLS)和月桂酰基甘氨酸钠(SLG)胶束中的末端羧酸盐基团反应,这是简单肽键模型两亲物。从产物产率中获得了这三个基团的界面摩尔浓度(界面体积每升摩尔数),假设与水相比对特定亲核试剂的选择性在水参考溶液中和界面区域中是相同的。在 SLS 和 SLG 胶束中,界面羧酸盐基团的摩尔浓度约为 1.5 M,但 SLS 胶束中酰胺羰基的浓度(约 0.7 M)比 SLG 胶束(约 3 M)低约 4.6-5 倍。SLG 中仲氮上的质子有助于酰胺键在水相区域中的溶解,但 SLS 中叔氮上的甲基有助于酰胺键在胶束核中的溶解,从而减少其与 16-ArN(2)(+)的反应。将化学捕获应用于膜模拟界面中的蛋白质应该可以深入了解蛋白质在界面中的拓扑结构,因为只有在界面内才能捕获酰胺羰基并在 C-N 键处断裂,并且片段特征标记那些位于界面内的肽键。

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