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通过 NMR、交联和质谱研究糖胺聚糖-蛋白复合物中的赖氨酸和精氨酸侧链:以因子 H-肝素相互作用为例。

Lysine and arginine side chains in glycosaminoglycan-protein complexes investigated by NMR, cross-linking, and mass spectrometry: a case study of the factor H-heparin interaction.

机构信息

Edinburgh Biomolecular NMR Unit, School of Chemistry and School of Biological Sciences, University of Edinburgh, West Mains Road, Edinburgh EH9 3JJ, Scotland, United Kingdom.

出版信息

J Am Chem Soc. 2010 May 12;132(18):6374-81. doi: 10.1021/ja1000517.

DOI:10.1021/ja1000517
PMID:20394361
Abstract

We have used the interaction between module 7 of complement factor H (CFH approximately 7) and a fully sulfated heparin tetrasaccharide to exemplify a new approach for studying contributions of basic side chains to the formation of glycosaminoglycan (GAG)-protein complexes. We first employed HISQC and H(2)CN NMR experiments to monitor the side-chain resonances of lysines and arginines in (15)N, (13)C-labeled protein during titrations with a fully sulfated heparin tetrasaccharide under physiological conditions. Under identical conditions and using (15)N-labeled protein, we then cross-linked tetrasaccharide to CFH approximately 7 and confirmed the 1:1 stoichiometry by FT-ICR-MS. We subsequently characterized this covalent protein-GAG conjugate by NMR and further MS techniques. MALDI-TOF MS identified protein fragments obtained via trypsin digestion or chemical fragmentation, yielding information concerning the site of GAG attachment. Combining MS and NMR data allowed us to identify the side chain of K405 as the point of attachment of the cross-linked heparin oligosaccharide to CFH approximately 7. On the basis of the analysis of NMR and MS data of the noncovalent and cross-linked CFH approximately 7-tetrasaccharide complexes, we conclude that the K446 side chain is not essential for binding the tetrasaccharide, despite the large chemical shift perturbations of its backbone amide (15)N and (1)H resonances during titrations. We show that R444 provides the most important charge-charge interaction within a C-terminal heparin-binding subsite of CFH approximately 7 whereas side chains of R404, K405, and K388 are the predominant contributors to an N-terminal binding subsite located in the immediate vicinity of residue 402, which is implicated in age-related macular degeneration (AMD).

摘要

我们利用补体因子 H(CFH 约 7)模块 7 与完全硫酸化肝素四糖之间的相互作用,举例说明了一种研究碱性侧链在糖胺聚糖(GAG)-蛋白复合物形成中的作用的新方法。我们首先采用 HISQC 和 H(2)CN NMR 实验,在生理条件下监测赖氨酸和精氨酸的侧链共振,这些赖氨酸和精氨酸在(15)N、(13)C 标记的蛋白中,与完全硫酸化的肝素四糖进行滴定。在相同条件下,使用(15)N 标记的蛋白,我们将四糖交联到 CFH 约 7 上,并通过 FT-ICR-MS 证实了 1:1 的化学计量比。随后,我们通过 NMR 和进一步的 MS 技术对这种共价蛋白-GAG 缀合物进行了表征。MALDI-TOF MS 鉴定了通过胰蛋白酶消化或化学断裂获得的蛋白片段,提供了有关 GAG 附着部位的信息。将 MS 和 NMR 数据相结合,使我们能够确定通过交联肝素低聚糖与 CFH 约 7 结合的 K405 侧链。基于非共价和交联 CFH 约 7-四糖复合物的 NMR 和 MS 数据分析,我们得出结论,尽管在滴定过程中其骨架酰胺(15)N 和(1)H 共振的化学位移扰动很大,但 K446 侧链对于结合四糖并非必不可少。我们表明,R444 在 CFH 约 7 的 C 末端肝素结合亚基内提供最重要的电荷-电荷相互作用,而 R404、K405 和 K388 的侧链是位于紧邻残基 402 的 N 末端结合亚基的主要贡献者,该亚基与年龄相关性黄斑变性(AMD)有关。

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