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嗜热四膜虫中的三类溶酶体酶

Three pools of lysosomal enzymes in Tetrahymena thermophila.

作者信息

Kiy T, Vosskühler C, Rasmussen L, Tiedtke A

机构信息

Institute for General Zoology and Genetics, Münster, Germany.

出版信息

Exp Cell Res. 1993 Apr;205(2):286-92. doi: 10.1006/excr.1993.1088.

DOI:10.1006/excr.1993.1088
PMID:8482338
Abstract

Secretion of lysosomal enzymes into the extracellular surroundings has been observed in many eukaryotic cells. We studied the activity of lysosomal enzymes in different subcellular fractions of Tetrahymena thermophila to get more insight into this general phenomenon. By density gradient centrifugation a light and a dense fraction of lysosomal particles were found. Electron microscopy revealed that the light fraction mainly consists of cell surface membranes. By immunostaining a lysosomal enzyme (beta-hexosaminidase) was detected on the plasma membrane. The Triton X-114 assay showed that the light fraction as well as purified cilia (an enriched source of plasma membrane) contain lysosomal enzymes predominantly covalently bound to the membrane. The dense fraction contains both membrane-bound and soluble forms of lysosomal enzymes. By labeling phagosomes/phagolysosomes with magnetic particles the dense fraction can be subdivided into two lysosomal vesicle populations: phagolysosomes and a further population of lysosomal vesicles which can not be labeled. The relationship between membrane-bound and soluble enzyme forms in phagolysosomes and this unlabeled vesicle population is different: In phagolysosomes 80% of the acid phosphatase and 20% of the beta-hexosaminidase are membrane-bound, whereas in the unlabeled vesicles 42% of the acid phosphatase and 8% of the beta-hexosaminidase are bound to the membrane. Furthermore, we present results suggesting that the unlabeled vesicle population of the dense fraction is the source of secreted lysosomal enzymes. A working model summarizing our present knowledge about the connection of the three pools of lysosomal enzymes in Tetrahymena is presented.

摘要

在许多真核细胞中都观察到溶酶体酶分泌到细胞外环境中。我们研究了嗜热四膜虫不同亚细胞组分中溶酶体酶的活性,以更深入地了解这一普遍现象。通过密度梯度离心,发现了轻、重两个溶酶体颗粒组分。电子显微镜显示,轻组分主要由细胞表面膜组成。通过免疫染色,在质膜上检测到一种溶酶体酶(β-己糖胺酶)。Triton X-114分析表明,轻组分以及纯化的纤毛(质膜的丰富来源)含有主要与膜共价结合的溶酶体酶。重组分包含膜结合形式和可溶性形式的溶酶体酶。通过用磁性颗粒标记吞噬体/吞噬溶酶体,重组分可细分为两个溶酶体囊泡群体:吞噬溶酶体和另一个无法标记的溶酶体囊泡群体。吞噬溶酶体和这个未标记的囊泡群体中膜结合和可溶性酶形式之间的关系不同:在吞噬溶酶体中,80%的酸性磷酸酶和20%的β-己糖胺酶是膜结合的,而在未标记的囊泡中,42%的酸性磷酸酶和8%的β-己糖胺酶与膜结合。此外,我们给出的结果表明,重组分中未标记的囊泡群体是分泌的溶酶体酶的来源。本文提出了一个工作模型,总结了我们目前关于嗜热四膜虫中溶酶体酶三个池之间联系的知识。

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