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宿主细胞被弓形虫入侵后,弓形虫线粒体膜电位降低。

Reduction in the mitochondrial membrane potential of Toxoplasma gondii after invasion of host cells.

作者信息

Tanabe K, Murakami K

出版信息

J Cell Sci. 1984 Aug;70:73-81. doi: 10.1242/jcs.70.1.73.

Abstract

The membrane potential of Toxoplasma gondii, an obligatory intracellular protozoan parasite, was monitored with the cationic permeant fluorescent dye rhodamine 123 (R123). Fluorescence microscopy revealed R123 to be partitioned predominantly in a restricted part of the parasite, which consisted of twisted or branched tubules, or of granular bodies. These structures were frequently connected to each other. The dye retention by these structures was markedly reduced by treating R123-labelled parasites with the proton ionophore, carbonylcyanide m-chlorophenylhydrazone, the potassium ionophore, valinomycin and the inhibitor of electron transport, antimycin A. Thus, these structures are regarded as the parasite mitochondria. Another cationic fluorescent dye, rhodamine 6G, stained the parasite mitochondria, whereas a negatively charged fluorescent dye, fluorescein, and the neutral compounds, rhodamine 110 and rhodamine B, did not. This fact indicates that R123 monitored the parasite mitochondrial membrane potential. T. gondii-infected 3T3 cells were also stained with R123. In contrast to the mitochondria of extracellular parasites, those of intracellular parasites failed to take up the dye. The absence of fluorescence in intracellular parasites persisted until the infected host cells ruptured and liberated daughter parasites 1 day after infection. Parasites, liberated from the host cells, either spontaneously or artificially by passing the infected cells through a 27G needle, regained the ability to take up the dye. After direct microinjection of R123 into the vacuole in which the parasite grows and multiples, the dye appeared in the host-cell mitochondria but not in the parasite's mitochondria. Thus, we conclude that the mitochondrial membrane potential of T. gondii was reduced after invasion of host cells by the parasite.

摘要

利用阳离子通透荧光染料罗丹明123(R123)监测了细胞内专性寄生原生动物刚地弓形虫的膜电位。荧光显微镜显示,R123主要分布在寄生虫的一个受限区域,该区域由扭曲或分支的小管或颗粒体组成。这些结构常常相互连接。用质子离子载体羰基氰化物间氯苯腙、钾离子载体缬氨霉素和电子传递抑制剂抗霉素A处理R123标记的寄生虫后,这些结构对染料的保留能力明显降低。因此,这些结构被认为是寄生虫的线粒体。另一种阳离子荧光染料罗丹明6G可对寄生虫线粒体进行染色,而带负电荷的荧光染料荧光素以及中性化合物罗丹明110和罗丹明B则不能。这一事实表明,R123监测的是寄生虫线粒体膜电位。用R123对感染了刚地弓形虫的3T3细胞也进行了染色。与细胞外寄生虫的线粒体不同,细胞内寄生虫的线粒体未能摄取该染料。细胞内寄生虫缺乏荧光的情况一直持续到感染后1天被感染的宿主细胞破裂并释放出子代寄生虫。从宿主细胞中自发释放或通过将感染细胞通过27G针头人工释放出的寄生虫恢复了摄取染料的能力。将R123直接显微注射到寄生虫生长和繁殖的液泡中后,染料出现在宿主细胞的线粒体中,而不是寄生虫的线粒体中。因此,我们得出结论,寄生虫侵入宿主细胞后,刚地弓形虫的线粒体膜电位降低。

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