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公猪唾液脂联素的克隆、翻译后修饰、异源表达及配体结合

Cloning, post-translational modifications, heterologous expression and ligand-binding of boar salivary lipocalin.

作者信息

Loebel D, Scaloni A, Paolini S, Fini C, Ferrara L, Breer H, Pelosi P

机构信息

Institut fur Physiologie, University of Hohenheim, Garbenstrasse 30, 70599 Stuttgart, Germany.

出版信息

Biochem J. 2000 Sep 1;350 Pt 2(Pt 2):369-79.

PMID:10947950
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1221263/
Abstract

Boar submaxillary glands produce the sex-specific salivary lipocalin (SAL), which binds steroidal sex pheromones as endogenous ligands. The cDNA encoding SAL was cloned and sequenced. From a single individual, two protein isoforms, differing in three amino acid residues, were purified and structurally characterized by a combined Edman degradation/MS approach. These experiments ascertained that the mature polypeptide is composed of 168 amino acid residues, that one of the three putative glycosylation sites is post-translationally modified and the structure of the bound glycosidic moieties. Two of the cysteine residues are paired together in a disulphide bridge, whereas the remaining two occur as free thiols. SAL bears sequence similarity to other lipocalins; on this basis, a three-dimensional model of the protein has been built. A SAL isoform was expressed in Escherichia coli in good yields. Protein chemistry and CD experiments verified that the recombinant product shows the same redox state at the cysteine residues and that the same conformation is observed as in the natural protein, thus suggesting similar folding. Binding experiments on natural and recombinant SAL were performed with the fluorescent probe 1-aminoanthracene, which was efficiently displaced by the steroidal sex pheromone, as well as by several odorants.

摘要

公猪的颌下腺分泌性别特异性唾液脂蛋白(SAL),它能结合甾体类性信息素作为内源性配体。编码SAL的cDNA被克隆并测序。从单个个体中纯化出两种在三个氨基酸残基上存在差异的蛋白质异构体,并通过Edman降解/MS联用方法对其进行结构表征。这些实验确定成熟多肽由168个氨基酸残基组成,三个假定的糖基化位点之一发生了翻译后修饰以及所结合糖苷部分的结构。其中两个半胱氨酸残基通过二硫键配对在一起,而其余两个则以游离硫醇形式存在。SAL与其他脂蛋白存在序列相似性;在此基础上构建了该蛋白质的三维模型。一种SAL异构体在大肠杆菌中高效表达。蛋白质化学和圆二色性实验证实重组产物在半胱氨酸残基处具有相同的氧化还原状态,并且观察到与天然蛋白质相同的构象,从而表明具有相似的折叠方式。用荧光探针1-氨基蒽对天然和重组SAL进行结合实验,甾体类性信息素以及几种气味剂能有效取代该探针。

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