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Quantitation and intracellular localization of the 85K heat shock protein by using monoclonal and polyclonal antibodies.

机译:通过使用单克隆和多克隆抗体对85K热激蛋白进行定量和细胞内定位。

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摘要

Two monoclonal antibodies have been produced against the human 85,000-molecular-weight heat shock protein (hsp85). One of these, 16F1, cross-reacts with the murine homolog and is shown by peptide map immunoblots to be directed against an epitope different from that recognized by the other monoclonal antibody, 9D2. Both monoclonal antibodies recognize only a single Mr-85,000 species in two-dimensional immunoblots. Immunoprecipitation did not reveal an association of this heat shock protein with any other protein in HeLa cells. Immunoperoxidase staining showed a purely cytosolic distribution at both light and electron microscopic levels and no association with membranes, mitochondria, or other organelles. The 9D2 monoclonal and a polyclonal antimurine hsp85 antibody were used to identify the antigens and to quantitate their levels in a variety of normal tissues by immunoautoradiography. Relative abundance in the various tissues as determined by Coomassie blue staining correlates reasonably well with the immunoreactivity. Testis and brain, for example, have high hsp85 levels, whereas heart and skeletal muscle have little or none. The Mr-85,000 sodium dodecyl sulfate-polyacrylamide gel band in testis and brain lysates was further confirmed to be hsp85 by one-dimensional partial proteolytic peptide mapping. Based on these data and our previous observations showing that synthesis and levels of the protein are altered by depriving cultured cells of glucose, we speculate that intracellular hsp85 levels depend on differences in the intermediary metabolism of glucose in the various tissues. Furthermore, it appears that high basal levels of this heat shock protein may not necessarily protect cells against heat shock, since testis is one of the most heat-sensitive tissues and has the highest hsp85 level.
机译:已经针对人类85,000分子量的热休克蛋白(hsp85)产生了两种单克隆抗体。其中的16F1与鼠类同系物发生交叉反应,并通过肽图免疫印迹显示其针对的抗原决定簇与另一种单克隆抗体9D2识别的抗原决定簇不同。两种单克隆抗体在二维免疫印迹中仅识别单个Mr-85,000物种。免疫沉淀未显示该热激蛋白与HeLa细胞中的任何其他蛋白有关联。免疫过氧化物酶染色在光镜和电子镜下均显示纯胞质分布,与膜,线粒体或其他细胞器无关联。使用9D2单克隆抗体和多克隆抗鼠hsp85抗体通过免疫放射自显影技术来鉴定抗原并定量在各种正常组织中的抗原水平。通过考马斯亮蓝染色确定的各种组织中的相对丰度与免疫反应性具有相当好的相关性。例如,睾丸和大脑的hsp85水平很高,而心脏和骨骼肌则很少或根本没有。通过一维部分蛋白水解肽作图进一步证实了睾丸和脑裂解物中的Mr-85,000十二烷基硫酸钠-聚丙烯酰胺凝胶带是hsp85。基于这些数据和我们以前的观察结果,结果表明蛋白质的合成和水平因剥夺培养细胞的葡萄糖而改变,我们推测细胞内hsp85的水平取决于各种组织中葡萄糖的中间代谢差异。此外,由于睾丸是对热最敏感的组织之一,并且具有最高的hsp85水平,因此高基础水平的热休克蛋白似乎不一定保护细胞免受热激。

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