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吸附性内吞作用和液相内吞作用中的内体与高尔基体囊泡。

Endosomes and Golgi vesicles in adsorptive and fluid phase endocytosis.

作者信息

Gonatas N K, Stieber A, Hickey W F, Herbert S H, Gonatas J O

出版信息

J Cell Biol. 1984 Oct;99(4 Pt 1):1379-90. doi: 10.1083/jcb.99.4.1379.

Abstract

We studied with morphometric methods the endocytosis by pheochromocytoma cells of a conjugate of wheat germ agglutinin with ferritin (WGA-Ft) and of horseradish peroxidase (HRP). Quantitative studies indicated that WGA-Ft was cleared slowly from cell surfaces and that it was not recycled to the surface. Cells labeled with WGA-Ft for 15 min at room temperature were washed and incubated in medium containing HRP for 15 or 30 min at 37 degrees C. The greatest proportion of labeled vesicles and tubules contained only WGA-Ft (83.4% at 15 min and 85.3% at 30 min). A very small fraction of labeled vesicles and tubules contained only HRP (0.2% at 15 min and 0.9% at 30 min). Vesicles and tubules at the Golgi apparatus were labeled almost exclusively with WGA-Ft (97% at 15 min and 30 min); the rest had both labels. Most labeled lysosomes contained both labels (80.1% at 15 min and 80.8% at 30 min). Of the remainder more contained WGA-Ft alone (20% at 15 min and 10.9% at 30 min), then HRP alone (none at 15 min and 8.2% at 30 min). In contrast to the various and varying patterns of labeling with WGA-Ft and HRP of the other organelles studied, the vast majority of endosomes contained both markers (94.1% at 15 min and 100% at 30 min); the rest contained WGA-Ft only. These results demonstrate that endosomes are recipients of both fluid phase and adsorptive endocytosis markers; these findings are consistent with the hypothesis that endosomes mediate the sorting out and subsequent intracellular traffic of membrane bound and fluid phase markers. Cisterns of the Golgi apparatus did not contain WGA-Ft; in sharp contrast, when WGA-HRP was used, the cisterns of the Golgi apparatus consistently contained HRP.

摘要

我们用形态测量学方法研究了嗜铬细胞瘤细胞对小麦胚凝集素与铁蛋白的结合物(WGA-Ft)和辣根过氧化物酶(HRP)的内吞作用。定量研究表明,WGA-Ft从细胞表面清除缓慢,且不会再循环到表面。在室温下用WGA-Ft标记细胞15分钟,然后洗涤,并在含有HRP的培养基中于37℃孵育15或30分钟。标记的囊泡和小管中最大比例仅含有WGA-Ft(15分钟时为83.4%,30分钟时为85.3%)。标记的囊泡和小管中极小一部分仅含有HRP(15分钟时为0.2%,30分钟时为0.9%)。高尔基体处的囊泡和小管几乎完全被WGA-Ft标记(15分钟和30分钟时均为97%);其余的同时含有两种标记。大多数标记的溶酶体同时含有两种标记(15分钟时为80.1%,30分钟时为80.8%)。其余的溶酶体中,更多的仅含有WGA-Ft(15分钟时为20%,30分钟时为10.9%),其次是仅含有HRP(15分钟时没有,30分钟时为8.2%)。与所研究的其他细胞器用WGA-Ft和HRP标记的各种不同模式形成对比的是,绝大多数内体同时含有两种标记(15分钟时为94.1%,30分钟时为100%);其余的仅含有WGA-Ft。这些结果表明,内体是液相和吸附性内吞作用标记物的接收者;这些发现与内体介导膜结合和液相标记物的分选及随后细胞内运输的假说一致。高尔基体的扁平囊不含有WGA-Ft;与之形成鲜明对比的是,当使用WGA-HRP时,高尔基体的扁平囊始终含有HRP。

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