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大鼠肝脏两性体的分离与鉴定。自噬体与早期和晚期内体融合的证据。

Isolation and characterization of rat liver amphisomes. Evidence for fusion of autophagosomes with both early and late endosomes.

作者信息

Berg T O, Fengsrud M, Strømhaug P E, Berg T, Seglen P O

机构信息

Department of Cell Biology, Institute for Cancer Research, The Norwegian Radium Hospital, Montebello, 0310 Oslo, Norway.

出版信息

J Biol Chem. 1998 Aug 21;273(34):21883-92. doi: 10.1074/jbc.273.34.21883.

Abstract

Amphisomes, the autophagic vacuoles (AVs) formed upon fusion between autophagosomes and endosomes, have so far only been characterized in indirect, functional terms. To enable a physical distinction between autophagosomes and amphisomes, the latter were selectively density-shifted in sucrose gradients following fusion with AOM-gold-loaded endosomes (endosomes made dense by asialoorosomucoid-conjugated gold particles, endocytosed by isolated rat hepatocytes prior to subcellular fractionation). Whereas amphisomes, by this criterion, accounted for only a minor fraction of the AVs in control hepatocytes, treatment of the cells with leupeptin (an inhibitor of lysosomal protein degradation) caused an accumulation of amphisomes to about one-half of the AV population. A quantitative electron microscopic study confirmed that leupeptin induced a severalfold increase in the number of hepatocytic amphisomes (recognized by their gold particle contents; otherwise, their ultrastructure was quite similar to autophagosomes). Leupeptin caused, furthermore, a selective retention of endocytosed AOM-gold in the amphisomes at the expense of the lysosomes, consistent with an inhibition of amphisome-lysosome fusion. The electron micrographs suggested that autophagosomes could undergo multiple independent fusions, with multivesicular (late) endosomes to form amphisomes and with small lysosomes to form large autolysosomes. A biochemical comparison between autophagosomes and amphisomes, purified by a novel procedure, showed that the amphisomes were enriched in early endosome markers (the asialoglycoprotein receptor and the early endosome-associated protein 1) as well as in a late endosome marker (the cation-independent mannose 6-phosphate receptor). Amphisomes would thus seem to be capable of receiving inputs both from early and late endosomes.

摘要

自噬体与内体融合后形成的自噬泡(AVs)——两性分子层小体,迄今为止仅在间接的功能方面得到了表征。为了在物理上区分自噬体和两性分子层小体,在与载有AOM-金的内体(通过去唾液酸糖蛋白偶联金颗粒使其致密的内体,在亚细胞分级分离前由分离的大鼠肝细胞内吞)融合后,两性分子层小体在蔗糖梯度中被选择性地进行密度转移。根据这一标准,在对照肝细胞中,两性分子层小体仅占自噬泡的一小部分,而用亮抑酶肽(一种溶酶体蛋白降解抑制剂)处理细胞会导致两性分子层小体积累至自噬泡群体的约一半。定量电子显微镜研究证实,亮抑酶肽使肝细胞两性分子层小体的数量增加了几倍(通过其金颗粒含量识别;否则,其超微结构与自噬体非常相似)。此外,亮抑酶肽导致内吞的AOM-金选择性地保留在两性分子层小体中,而牺牲了溶酶体,这与两性分子层小体-溶酶体融合的抑制一致。电子显微镜照片表明,自噬体可以经历多次独立融合,与多泡(晚期)内体形成两性分子层小体,与小溶酶体形成大自噬溶酶体。通过一种新方法纯化的自噬体和两性分子层小体之间的生化比较表明,两性分子层小体富含早期内体标记物(去唾液酸糖蛋白受体和早期内体相关蛋白1)以及晚期内体标记物(不依赖阳离子的甘露糖6-磷酸受体)。因此,两性分子层小体似乎能够接收来自早期和晚期内体的输入。

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