首页> 外文期刊>Molecular and Biochemical Parasitology >Evidence for vesicle-mediated trafficking of parasite proteins to the host cell cytosol and erythrocyte surface membrane in Plasmodium falciparum infected erythrocytes.
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Evidence for vesicle-mediated trafficking of parasite proteins to the host cell cytosol and erythrocyte surface membrane in Plasmodium falciparum infected erythrocytes.

机译:恶性疟原虫感染的红细胞中囊泡介导的寄生虫蛋白向宿主细胞胞浆和红细胞表面膜运输的证据。

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摘要

Plasmodium falciparum malaria parasites actively remodel the host cell cytosol and plasma membrane during the erythrocytic cycle. The focus of this investigation was to characterize intra-parasitic and -erythrocytic secretory pathways. Electron-dense vesicles, similar in appearance to mammalian secretory vesicles were detected in proximity to smooth tubo-vesicular elements at the periphery of the parasite cytoplasm in mature parasites by transmission electron microscopy. Vesicles (60-100 nm diameter), which appeared to be coated, were visualized on the erythrocytic side of the parasite vacuolar membrane and in the erythrocyte cytosol. The vesicles seemed to bind to and fuse with the erythrocyte membrane, giving rise to cup-shaped electron-dense structures, which might be intermediates in knob structure formation. Treatment of mature parasites with aluminum tetrafluoride, an activator of GTP-binding proteins, resulted in the accumulation of the vesicles with an electron-dense limiting membrane in the erythrocyte cytosol into multiple vesicle strings. These vesicle complexes were often associated with and closely abutted the erythrocyte membrane, but were apparently prevented from fusing by the aluminum fluoride treatment. The parasite proteins PfEMP1 and PfEMP3 were found by immunoelectron microscopy to be associated with these vesicles, suggesting they are responsible for transporting these proteins to the erythrocyte membrane.
机译:恶性疟原虫疟疾寄生虫在红细胞周期中主动重塑宿主细胞的细胞质和质膜。这项研究的重点是表征内寄生和-红细胞分泌途径。电子致密囊泡的外观类似于哺乳动物的分泌囊泡,通过透射电子显微镜在成熟寄生虫的寄生虫细胞质外围的光滑微管泡囊元件附近被检测到。在寄生虫液泡膜的红细胞侧和红细胞胞浆中可见囊泡(直径为60-100 nm)。囊泡似乎与红细胞膜结合并融合,产生了杯状的电子致密结构,这可能是纽结结构形成的中间产物。用四氟化铝(一种GTP结合蛋白的活化剂)处理成熟的寄生虫,导致带有电子致密限制膜的囊泡在红细胞胞质溶胶中积聚成多个囊泡串。这些囊复合物通常与红细胞膜结合并紧密邻接,但是显然通过氟化铝处理阻止了融合。通过免疫电子显微镜发现寄生虫蛋白PfEMP1和PfEMP3与这些囊泡有关,表明它们负责将这些蛋白转运至红细胞膜。

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