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C型凝集素牛胶固素的生化与超微结构研究。

Biochemical and ultrastructural studies of the C-type lectin bovine conglutinin.

作者信息

Andersen O, Nielsen E H, Storgaard P, Højrup P, Friis P, Leslie G, Svehag S E

机构信息

Department of Medical Microbiology, Odense University, Denmark.

出版信息

J Struct Biol. 1992 Nov-Dec;109(3):201-7. doi: 10.1016/1047-8477(92)90032-6.

Abstract

The aim of this study was to correlate the supramolecular organization of conglutinin (BK) with its primary and tertiary structure and to gain more knowledge of functionally important regions of the molecule. BK analyzed by SDS-PAGE under standard reducing conditions (40 mM DTT) showed a major band at 43 kDa and weaker bands at 86 and 180 kDa. In contrast, reduction with 6-50 mM L-cysteine resulted in 37-kDa subunits indicating the presence of intrachain disulfide bonds within this subunit. Hydroxylamine treatment indicated presence of ester bonds in the 86- and 180-kDa subunits. Collagenase digestion and SDS-PAGE under reducing and nonreducing conditions resulted in bands of 20 and 15 kDa, respectively, indicating the presence of intrachain, rather than interchain, disulfide bonds in the carboxy terminus. Deglycosylation and glycan differentiation analysis of BK revealed the presence of O-linked glycans of GalNAc and alpha (2-3) linked sialic acid type, whereas no N-linked glycans were demonstrated. Binding experiments with GlcNAc-gold suggested that multivalency is required for carbohydrate binding to BK. Electron microscopy showed mostly tetramers, 96 nm in diameter, but also mono-, di-, and trimers were seen. The tetramers consisted of 40-nm strands, each with a peripheral globular head composed of subunits and connected to a common central lobe built from four ring-formed structures. The strands occasionally showed two bends, one close to the central lobe and another 25 nm from the lobe. These bends most likely correspond to the interrupted Gly-Xaa-Yaa repeats at residues 38 and 123.

摘要

本研究的目的是将凝集素(BK)的超分子结构与其一级和三级结构相关联,并更多地了解该分子功能重要区域的情况。在标准还原条件(40 mM二硫苏糖醇)下通过SDS-PAGE分析的BK在43 kDa处显示出一条主要条带,在86和180 kDa处显示出较弱条带。相比之下,用6 - 50 mM L-半胱氨酸还原会产生37 kDa的亚基,表明该亚基内存在链内二硫键。羟胺处理表明86 kDa和180 kDa亚基中存在酯键。胶原酶消化以及在还原和非还原条件下的SDS-PAGE分别产生了20 kDa和15 kDa的条带,表明羧基末端存在链内而非链间二硫键。BK的去糖基化和聚糖分化分析显示存在GalNAc型的O-连接聚糖和α(2-3)连接的唾液酸型聚糖,而未检测到N-连接聚糖。用GlcNAc-金进行的结合实验表明碳水化合物与BK结合需要多价性。电子显微镜观察到大多是直径为96 nm的四聚体,但也可见单体、二聚体和三聚体。四聚体由40 nm的链组成,每条链都有一个由亚基组成的外周球状头部,并连接到一个由四个环形结构构成的共同中央叶。这些链偶尔会出现两个弯曲,一个靠近中央叶,另一个距离叶25 nm。这些弯曲很可能对应于第38和123位残基处中断的Gly-Xaa-Yaa重复序列。

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