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[3H]哇巴因从HeLa细胞表面摄取到溶酶体区室的过程。

Uptake of [3H]ouabain from the cell surface into the lysosomal compartment of HeLa cells.

作者信息

Cook J S, Tate E H, Shaffer C

出版信息

J Cell Physiol. 1982 Jan;110(1):84-92. doi: 10.1002/jcp.1041100114.

DOI:10.1002/jcp.1041100114
PMID:6279680
Abstract

[3H]Ouabain specifically bound at sublethal concentrations to Na,K-ATPase on the surface of HeLa cells is taken up (internalized) by the cells at a rate of three membrane equivalents of labeled sites per generation. Immediately following a pulse label with the glycoside, codistribution of radioactivity with the surface marker 5'-nucleotidase is found in both conventional sucrose-gradient fractionation and in fractionation following a digitonin treatment. At appropriate concentrations digitonin increases the buoyant density of the HeLa surface membrane and solubilizes the lysosomal marker beta-hexosaminidase (Tulkens et al., 1974). After internalization, [3H]ouabain is also solubilized by digitonin. A shear analysis is described which shows internalized ouabain and beta-hexosaminidase to be codistributed in a particulate fraction that is homogeneous with respect to shear; extrapolation to zero-shear shows that little or none of either marker is found in the soluble fraction of the cytosol. Both markers are coreleased from the particulate fraction by osmotic shock. Although internalized ouabain is subsequently released from these cells with a half-time of about 70 hr, apparently by exocytosis, the shear sensitivity of the remaining cell-associated ouabain does not change for up to 72 hr. Thus ouabain (together with Na,K-ATPase?) appears to be taken up from the surface into a lysosomal compartment and, by at least one criterion, this compartment does not change its physical properties with time, i.e., does not "age."

摘要

[3H]哇巴因在亚致死浓度下特异性结合于HeLa细胞表面的钠钾ATP酶,并以每代三个标记位点膜当量的速率被细胞摄取(内化)。在用糖苷进行脉冲标记后,立即在传统的蔗糖梯度分级分离以及洋地黄皂苷处理后的分级分离中发现放射性与表面标记物5'-核苷酸酶共分布。在适当浓度下,洋地黄皂苷增加HeLa表面膜的浮力密度并溶解溶酶体标记物β-己糖胺酶(图尔肯斯等人,1974年)。内化后,[3H]哇巴因也被洋地黄皂苷溶解。描述了一种剪切分析,结果表明内化的哇巴因和β-己糖胺酶在一个颗粒部分中共分布,该颗粒部分在剪切方面是均匀的;外推至零剪切表明,在细胞质的可溶部分中几乎找不到或找不到任何一种标记物。两种标记物都通过渗透压休克从颗粒部分中共同释放出来。尽管内化的哇巴因随后以约70小时的半衰期从这些细胞中释放出来,显然是通过胞吐作用,但剩余的细胞相关哇巴因的剪切敏感性在长达72小时内没有变化。因此,哇巴因(可能与钠钾ATP酶一起)似乎从表面被摄取到溶酶体区室中,并且根据至少一个标准,这个区室的物理性质不会随时间变化,即不会“老化”。

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