Hart P D, Young M R
Laboratory for Leprosy and Mycobacterial Research, National Institute for Medical Research, London, United Kingdom.
J Exp Med. 1991 Oct 1;174(4):881-9. doi: 10.1084/jem.174.4.881.
The weak base ammonium chloride has been previously reported to inhibit lysosomal movements and phagosome-lysosome (Ph-L) fusion in cultured mouse macrophages (M phi), thus reducing delivery, to an intraphagosomal infection, of endocytosed solutes that have concentrated in secondary lysosomes. We have now addressed the question, whether NH4Cl might affect any direct interaction (if it exists) between such infection phagosomes and earlier, nonlysosomal compartments of the endocytic pathway, i.e., solute-containing endosomes. The phagosomes studied were formed after ingestion of the mouse pathogen Mycobacterium microti and the nonpathogenic yeast Saccharomyces cerevisiae; and the endosomes were formed after nonreceptor-mediated endocytosis of electronopaque and fluorescent soluble markers. By electron microscopy, survey of the cell profiles of M phi that had been treated with 10 mM NH4Cl so that Ph-L fusion was prevented, and that displayed many ferritin-labeled endosomes, revealed numerous examples of the fusion of electronlucent endosomes, revealed numerous examples of the fusion of electronlucent vesicles with phagosomes, whether containing M. microti bacilli or S. cerevisiae yeasts. Fusion was recognized by transfer of label and by morphological evidence of fusion in progress. The fusing vesicles were classed as endosomes, not NH4Cl-lysosomes, by their appearance and provenance, and because lysosome participation was excluded by the concurrent, NH4Cl-caused block of Ph-L fusion and associated lysosomal stasis. No evidence of such phagosome-endosome (Ph-E) fusion was observed in profiles from M phi treated with chloroquine, nor in those from normal, untreated M phi. NH4Cl-treated living M phi that had ingested yeasts at 37 degrees C, followed by endocytosis of lucifer yellow at 17 degrees C (to accumulate labeled endosomes and postpone label passing to lysosomes), were then restored to 37 degrees C. Fluorescence microscopy showed that as many as half of the yeast phagosomes (previously unlabeled) rapidly became colored. We inferred that this transfer was from endosomes (by Ph-E fusion) because Ph-L passage was blocked (by the NH4Cl). We conclude that NH4Cl induces Ph-E fusion at the same time as it suppressed Ph-L fusion. We discuss the mechanisms of these concurrent effects and suggest that they are independent; and we consider the implications of NH4Cl opening a direct route for endocytosed molecules to reach an intraphagosomal infection without involving lysosomes.
弱碱氯化铵此前曾被报道可抑制培养的小鼠巨噬细胞(M phi)中的溶酶体运动和吞噬体 - 溶酶体(Ph - L)融合,从而减少内吞溶质向吞噬体内感染的传递,这些溶质已在次级溶酶体中浓缩。我们现在探讨了一个问题,即氯化铵是否可能影响此类感染吞噬体与内吞途径中更早的非溶酶体区室(即含溶质的内体)之间的任何直接相互作用(如果存在的话)。所研究的吞噬体是在摄入小鼠病原体微小分枝杆菌和非致病性酵母酿酒酵母后形成的;而内体是在电子不透明和荧光可溶性标记物的非受体介导的内吞作用后形成的。通过电子显微镜观察,对用10 mM氯化铵处理以阻止Ph - L融合且显示许多铁蛋白标记内体的M phi细胞轮廓进行调查,发现了许多电子透明内体与吞噬体融合的例子,无论吞噬体中含有微小分枝杆菌杆菌还是酿酒酵母酵母。融合通过标记物的转移和正在进行融合的形态学证据得以识别。通过其外观和来源,以及由于氯化铵导致的Ph - L融合同时受阻和相关溶酶体停滞排除了溶酶体的参与,将融合的小泡归类为内体,而非氯化铵诱导的溶酶体。在用氯喹处理的M phi细胞轮廓中,或在正常未处理的M phi细胞轮廓中,均未观察到这种吞噬体 - 内体(Ph - E)融合的证据。在37℃下摄入酵母,然后在17℃下内吞荧光素黄(以积累标记的内体并推迟标记传递至溶酶体),随后恢复至37℃的经氯化铵处理的活M phi细胞。荧光显微镜显示,多达一半的酵母吞噬体(先前未标记)迅速变色。我们推断这种转移是通过内体(通过Ph - E融合)进行的,因为Ph - L传递受阻(由氯化铵所致)。我们得出结论,氯化铵在抑制Ph - L融合的同时诱导Ph - E融合。我们讨论了这些并发效应的机制,并表明它们是相互独立的;并且我们考虑了氯化铵开辟了一条使内吞分子无需通过溶酶体即可到达吞噬体内感染部位的直接途径的意义。
