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在小鼠子宫腔液中对源自24p3基因的一种糖蛋白的证明。

Demonstration of a glycoprotein derived from the 24p3 gene in mouse uterine luminal fluid.

作者信息

Chu S T, Huang H L, Chen J M, Chen Y H

机构信息

Institute of Biological Chemistry, Academia Sinica, Taipel, Taiwan, Republic of China.

出版信息

Biochem J. 1996 Jun 1;316 ( Pt 2)(Pt 2):545-50. doi: 10.1042/bj3160545.

Abstract

A glycoprotein in mouse uterine luminal fluid was purified to homogeneity via a series of purification steps involving Sephadex G-100 chromatography, Sephadex G-50 chromatography and HPLC on a reverse-phase C18 column, in that order. Automated Edman degradation was unable to determine the N-terminal residue of the glycoprotein and the partial sequences determined from its trypsin digests were found to be identical with the protein sequence deduced from 24p3 cDNA. The core protein and the total amount of carbohydrate together gave a molecular mass of 25.8 kDa. Results from the characterization of the glycopeptide bond indicated the presence of N-linked carbohydrate but no O-linked carbohydrate in the protein, which has two potential sites for N-linked carbohydrate at Asn81 and Asn85, as deduced from analysis of the primary structure. The core protein was shown to have a molecular mass equal to that of the putative protein deduced from cDNA, suggesting that this protein may contain no signal peptide. Results of Northern-blot analysis for various tissues of adult mice revealed that the 24p3 gene was expressed in lung, spleen, uterus, vagina and epididymis.

摘要

通过一系列纯化步骤,包括依次进行的Sephadex G - 100柱层析、Sephadex G - 50柱层析和反相C18柱高效液相色谱,将小鼠子宫腔液中的一种糖蛋白纯化至同质。自动Edman降解法无法确定该糖蛋白的N端残基,并且发现从其胰蛋白酶消化产物中确定的部分序列与从24p3 cDNA推导的蛋白质序列相同。核心蛋白和碳水化合物总量给出的分子量为25.8 kDa。糖肽键的表征结果表明该蛋白质中存在N - 连接的碳水化合物,但不存在O - 连接的碳水化合物,从一级结构分析推断,该蛋白质在Asn81和Asn85处有两个潜在的N - 连接碳水化合物位点。核心蛋白的分子量显示与从cDNA推导的假定蛋白质的分子量相等,表明该蛋白质可能不包含信号肽。对成年小鼠各种组织进行的Northern杂交分析结果显示,24p3基因在肺、脾、子宫、阴道和附睾中表达。

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