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近端小管细胞内吞过程中顶端胰岛素结合位点的分选与再循环效率

Sorting and recycling efficiency of apical insulin binding sites during endocytosis in proximal tubule cells.

作者信息

Nielsen S

机构信息

Department of Cell Biology, University of Aarhus, Denmark.

出版信息

Am J Physiol. 1993 Apr;264(4 Pt 1):C810-22. doi: 10.1152/ajpcell.1993.264.4.C810.

DOI:10.1152/ajpcell.1993.264.4.C810
PMID:8476016
Abstract

Intracellular traffic and recycling of apical insulin binding sites are examined in isolated, perfused proximal tubules. The endocytic binding sites were specific as revealed by 90% reduction in 125I-labeled insulin binding by 10(-5) M insulin. The traffic was followed by developing a chemical cross-linking method to covalently label the binding sites. Only 3% of cross-linked insulin-gold was transported to the lysosomes, reflecting high sorting and recycling efficiency. Correspondingly, only 4% of cross-linked 125I-insulin was degraded, and only 5% of the electron microscopy-autoradiographic grains was associated with lysosomes. No label was transferred to the Golgi apparatus; thus neither lysosomes nor Golgi apparatus is involved in the recycling. In contrast, approximately 40% of non-cross-linked ligand was transferred to the lysosomes. Tubules first pretreated with cross-linker and then perfused with insulin-gold or 125I-labeled insulin-like growth factor I revealed lysosomal accumulation and degradation at control levels. Thus the cross-linker does not interfere with membrane or protein processing. The study also provides evidence for a vesicular transtubular transport because insulin-gold was transcytosed to the basolateral part of the cells and to the intracellular spaces (0.5%). In contrast cross-linked label was never observed in intercellular spaces, suggesting sorting of apical binding sites, a mechanism contributing to maintenance of cell polarity. In conclusion, traffic, sorting, and recycling of binding sites take place with high efficiency.

摘要

在分离的灌注近端小管中研究了顶端胰岛素结合位点的细胞内运输和再循环。如10(-5)M胰岛素使125I标记的胰岛素结合减少90%所示,内吞结合位点具有特异性。通过开发一种化学交联方法来共价标记结合位点,追踪运输过程。只有3%的交联胰岛素-金被转运到溶酶体,这反映了高效的分选和再循环效率。相应地,只有4%的交联125I胰岛素被降解,只有5%的电子显微镜放射自显影片颗粒与溶酶体相关。没有标记转移到高尔基体;因此,溶酶体和高尔基体都不参与再循环。相比之下,约40%的非交联配体被转移到溶酶体。先用交联剂预处理小管,然后用胰岛素-金或125I标记的胰岛素样生长因子I灌注,显示溶酶体在对照水平上积累和降解。因此,交联剂不干扰膜或蛋白质加工。该研究还为囊泡跨小管运输提供了证据,因为胰岛素-金被转胞吞到细胞的基底外侧部分和细胞内空间(0.5%)。相比之下,在细胞间隙中从未观察到交联标记,这表明顶端结合位点的分选是维持细胞极性的一种机制。总之,结合位点的运输、分选和再循环高效进行。

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