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傅里叶变换质谱法监测透明质酸与蛋白质的相互作用:氢/氘酰胺交换的应用

Fourier transform mass spectrometry to monitor hyaluronan-protein interactions: use of hydrogen/deuterium amide exchange.

作者信息

Seyfried Nicholas T, Atwood James A, Yongye Austin, Almond Andrew, Day Anthony J, Orlando Ron, Woods Robert J

机构信息

Complex Carbohydrate Research Center, University of Georgia, 315 Riverbend Road, Athens, GA 30602, USA.

出版信息

Rapid Commun Mass Spectrom. 2007;21(2):121-31. doi: 10.1002/rcm.2817.

Abstract

The use of Fourier transform mass spectrometry (FTMS) to monitor noncovalent complex formation in the gas phase under native conditions between the Link module from human tumor necrosis factor stimulated gene-6 (Link_TSG6) and hyaluronan (HA) oligosaccharides is reported. In particular, a titration experiment with increasing concentrations of octasaccharide (HA(8)) to protein produced a noncovalent complex with 1:1 stoichiometry when the oligosaccharide was in molar excess. However, in the presence of a molar excess of tetrasaccharide (HA(4)) nearly all proteins and oligosaccharides were observed in their unbound charge states. These results are consistent with solution-phase properties for this interaction in which HA(8), but not HA(4), supports high affinity Link_TSG6 binding. Hydrogen/deuterium amide exchange mass spectrometry (H/D-EX MS) was also utilized to investigate the level of global deuterium incorporation, over time, for Link_TSG6 in both the absence and presence of HA(8). After dilution into quenching conditions, deuterium incorporation reached limiting asymptotic values of 37 and 26 deuterons for the free and bound protein at 240 and 480 min, respectively, indicating that the oligosaccharide interferes with amide exchange on binding. To detect sequence-specific deuterium incorporation, pepsin digestion of Link_TSG6 in both the absence and presence of HA(8) was performed. A level of deuterium incorporation of 10-30% was observed for peptides analyzed in free Link_TSG6. Interestingly, HA(8) blocked some sites of proteolysis in Link_TSG6 compared to the free protein. Molecular modeling indicated that amino acids proximal to the ligand correlated with regions of the protein that were resistant to enzymatic digestion. Of the peptides that could be analyzed by H/D-EX MS in the presence of the ligand, a 30-60% reduction in deuterium incorporation, relative to the free protein, was observed, even for those sequences not directly involved in HA binding. These results support the utility of FTMS as a method for the characterization of protein-carbohydrate interactions.

摘要

本文报道了利用傅里叶变换质谱(FTMS)监测人肿瘤坏死因子刺激基因-6的连接模块(Link_TSG6)与透明质酸(HA)寡糖在天然条件下于气相中形成非共价复合物的情况。具体而言,用浓度递增的八糖(HA(8))对蛋白质进行滴定实验,当寡糖摩尔过量时,生成了化学计量比为1:1的非共价复合物。然而,在四糖(HA(4))摩尔过量的情况下,几乎所有蛋白质和寡糖都以未结合的电荷状态被观察到。这些结果与该相互作用在溶液相中的性质一致,即HA(8)而非HA(4)支持Link_TSG6的高亲和力结合。氢/氘酰胺交换质谱(H/D-EX MS)也被用于研究在不存在和存在HA(8)的情况下,Link_TSG6随时间的整体氘掺入水平。在稀释到淬灭条件后,游离和结合蛋白的氘掺入在240分钟和480分钟时分别达到37和26个氘核的极限渐近值,这表明寡糖在结合时会干扰酰胺交换。为了检测序列特异性氘掺入,对不存在和存在HA(8)的Link_TSG6进行了胃蛋白酶消化。在游离Link_TSG6中分析的肽段观察到10 - 30%的氘掺入水平。有趣的是,与游离蛋白相比,HA(8)阻断了Link_TSG6中的一些蛋白水解位点。分子建模表明,配体附近的氨基酸与蛋白质中对酶消化有抗性的区域相关。在配体存在的情况下,可通过H/D-EX MS分析的肽段,相对于游离蛋白,即使是那些不直接参与HA结合的序列,氘掺入也减少了30 - 60%。这些结果支持了FTMS作为一种表征蛋白质 - 碳水化合物相互作用方法的实用性。

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