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肾上腺嗜铬粒蛋白中一种糖蛋白的分离及免疫学特性分析

Isolation and immunological characterization of a glycoprotein from adrenal chromaffin granules.

作者信息

Fischer-Colbrie R, Zangerle R, Frischenschlager I, Weber A, Winkler H

出版信息

J Neurochem. 1984 Apr;42(4):1008-16. doi: 10.1111/j.1471-4159.1984.tb12704.x.

Abstract

A glycoprotein (s-GP III) was isolated from the soluble lysate of chromaffin granules by chromatography with immunoaffinity and lectin columns. An identical protein (m-GP III) was shown to be present in the granule membranes. The apparent molecular weight of these glycoproteins as determined by the electrophoresis system of Laemmli (1970) was 43,000 under reducing conditions. In the absence of mercaptoethanol they aggregated to dimers. Antisera were raised against both the soluble and the membrane-bound forms of this glycoprotein. With these antisera GP III was further characterized: Immunoreplicas were obtained after two-dimensional electrophoresis of soluble and membrane-bound proteins of chromaffin granules. GP III was identified as a protein with a rather broad pI (4.6-5.3), indicating microheterogeneity. As shown by subcellular fractionation, m-GP III is specifically confined to chromaffin granules. GP III can therefore be used as a marker for the membranes of these organelles. The soluble form is secreted from adrenal medulla during stimulation with carbamylcholine chloride. An immunologically identical antigen was detected in adeno- and neurohypophysis. The physiological function of GP III is still unknown. It does not demonstrate any of the enzymatic activities so far known to occur in chromaffin granules.

摘要

通过免疫亲和柱和凝集素柱色谱法从嗜铬颗粒的可溶性裂解物中分离出一种糖蛋白(s-GP III)。结果表明,在颗粒膜中存在一种相同的蛋白质(m-GP III)。根据Laemmli(1970)的电泳系统测定,在还原条件下,这些糖蛋白的表观分子量为43,000。在没有巯基乙醇的情况下,它们聚合成二聚体。制备了针对这种糖蛋白的可溶性和膜结合形式的抗血清。利用这些抗血清对GP III进行了进一步表征:对嗜铬颗粒的可溶性和膜结合蛋白进行二维电泳后获得了免疫复制品。GP III被鉴定为一种pI相当宽(4.6 - 5.3)的蛋白质,表明存在微异质性。如亚细胞分级分离所示,m-GP III特异性地局限于嗜铬颗粒。因此,GP III可作为这些细胞器膜的标志物。可溶性形式在氯化氨甲酰胆碱刺激期间从肾上腺髓质分泌。在腺垂体和神经垂体中检测到一种免疫相同的抗原。GP III的生理功能仍然未知。它不表现出迄今为止已知在嗜铬颗粒中出现的任何酶活性。

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