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多阴离子在溶酶体内的积累。I. 胞饮泡和吞噬泡与次级溶酶体的融合。

Intralysosomal accumulation of polyanions. I. Fusion of pinocytic and phagocytic vacuoles with secondary lysosomes.

作者信息

Kielian M C, Steinman R M, Cohn Z A

出版信息

J Cell Biol. 1982 Jun;93(3):866-74. doi: 10.1083/jcb.93.3.866.

Abstract

The long-term exposure of macrophages to low concentrations of a number of polyanions leads to their accumulation in high concentration within secondary lysosomes. This was associated with enlargement of the lysosomes, the presence of membranous whorls, and intense toluidine blue staining of the organelles at pH 1.0. After the ingestion of a particulate load by these cells, newly formed phagocytic vacuoles failed to fuse with polyanion-laden lysosomes. The lack of fusion was evident in both fluorescence and electron micrographic studies which followed the transfer of acridine orange or Thorotrast from 2 degrees lysosomes to phagosomes. Agents that inhibited phagosome-lysosome (P-L) fusion included molecules containing high densities of sulfate, sulfonate, or carboxylate residues. Dextran sulfate (DS) in microgram/ml quantities was an excellent inhibitor, whereas nonsulfated dextran (D) was without effect at 1,000-fold higher concentrations. In contrast to their effects on P-L fusion, polyanions failed to influence the fusion of pinocytic vesicles with 2 degrees lysosomes. The uptake, intravacuolar distribution, and intralysosomal digestion of fluid-phase pinocytic markers were unaltered in lysosomes containing either D or DS. Furthermore, subcellular fractionation studies showed that the fluid-phase pinocytic marker HRP was efficiently transferred from pinosomes to large, dense 2 degrees lysosomes containing DS.

摘要

巨噬细胞长期暴露于低浓度的多种聚阴离子会导致它们在次级溶酶体内高浓度积累。这与溶酶体增大、出现膜性涡旋以及在pH 1.0时细胞器的甲苯胺蓝强烈染色有关。这些细胞摄取颗粒负荷后,新形成的吞噬泡无法与富含聚阴离子的溶酶体融合。在吖啶橙或钍造影剂从次级溶酶体转移到吞噬体后的荧光和电子显微镜研究中,融合缺乏现象很明显。抑制吞噬体-溶酶体(P-L)融合的物质包括含有高密度硫酸根、磺酸根或羧酸根残基的分子。微克/毫升量的硫酸葡聚糖(DS)是一种极好的抑制剂,而未硫酸化的葡聚糖(D)在浓度高1000倍时则无作用。与它们对P-L融合的影响相反,聚阴离子不会影响胞饮小泡与次级溶酶体的融合。在含有D或DS的溶酶体中,液相胞饮标记物的摄取、泡内分布和溶酶体内消化均未改变。此外,亚细胞分级分离研究表明,液相胞饮标记物辣根过氧化物酶(HRP)能有效地从胞饮体转移到含有DS的大的、致密的次级溶酶体中。

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