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Phagosome-lysosome fusion. Characterization of intracellular membrane fusion in mouse macrophages

机译:吞噬体-溶酶体融合。小鼠巨噬细胞内细胞膜融合的表征

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摘要

Several approaches have been used to study the determinants of phagosome-lysosome fusion in intact mouse macrophages. Lysosomes were labeled with the fluorescent vital dye acridine orange and the rate and extent of their fusion with yeast-containing phagosomes was monitored by fluorescence microscopy. Fusion was also assayed by electron microscopy, using horseradish peroxidase or thorium dioxide as a marker for secondary lysosomes. Good agreemen samples with an enzymatic marker, and thorium dioxide-labeled samples evaluated by stereology. The rate of usion as assayed by fluorescence was not affected by the number of particles ingested, serum concentration, or prior uptake of digestible or nondigestible substances. With this assay it was possible to observe the rate of fusion separate from and uninfluenced by the phagocytic rate. Both the rate and extent of fusion were dramatically increased after several days in culture and similar changes were found by use of the EM assays. Fusion was strongly affected by incubation temperature, having a Q10 of 2.5 No detectable fusion occurred below 15 degrees C, and this inhibition was rapidly reversed when cells were returned to 37 degrees C.
机译:已使用几种方法来研究完整小鼠巨噬细胞中吞噬体-溶酶体融合的决定因素。用荧光活性染料a啶橙标记溶酶体,并通过荧光显微镜监测其与含酵母吞噬体融合的速率和程度。还使用辣根过氧化物酶或二氧化th作为次级溶酶体的标记物,通过电子显微镜分析融合。良好的酶标物和酶标仪评估的二氧化th标本。通过荧光测定的腐烂率不受摄入的颗粒数量,血清浓度或可消化或不可消化物质的摄取的影响。利用该测定法,可以观察到吞噬速率与不受吞噬速率影响无关的融合速率。培养几天后,融合速率和融合程度都显着提高,并且通过使用EM分析发现了类似的变化。融合受到孵育温度的强烈影响,Q10为2.5,低于15摄氏度时未检测到融合现象,当细胞恢复至37摄氏度时,这种抑制作用迅速逆转。

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