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杜氏锥虫在非吞噬细胞中的侵入及发育机制。

Mechanism of entry and development of Trypanosoma dionisii in non-phagocytic cells.

作者信息

Glauert A M, Baker J R, Selden L F

出版信息

J Cell Sci. 1982 Aug;56:371-87. doi: 10.1242/jcs.56.1.371.

Abstract

Cultures of 'buffalo' (bison) lung (BL) cells were infected with epimastigotes or trypomastigotes of Trypanosoma (Schizotrypanum) dionisii derived from cultures in vitro, fixed after various periods of incubation at 37 degrees C and examined by light or electron microscopy. Few if any epimastigotes entered the BL cells, but many trypomastigotes did so; they adhered to the cell surface within 2 h and then appeared to sink into furrows on the cell surface until engulfed in parasitophorous vacuoles. Cytochalasin D (5-10 micrograms ml-1) completely, but reversibly, inhibited entry of trypomastigotes without affecting parasite motility. It was concluded that entry depended on the interaction of stage-specific components on the trypomastigote's surface with receptors on the BL cells, and that this interaction induced active uptake of the protozoa by a phagocytic process not involving pseudopod formation. Soon after entry of the trypomastigotes into BL cells, the membranes of the parasitophorous vacuoles disintegrated and the parasites, which were now lying free in the cytoplasm of the host cell, transformed into amastigotes (micromastigotes) during the next 24-48 h. Replication then occurred, followed by transformation, beginning after 3 days, through a transitional promastigote phase to small intracellular trypomastigotes at 7 days. The promastigotes had a characteristic curved protrusion extending from the lip of the flagellar pocket (or reservoir) into the host cell's cytoplasm. Trypomastigotes, released into the supernatant medium by rupture of the plasma membranes of the BL cells after 8 days, could re-invade other cells.

摘要

用源自体外培养物的杜氏锥虫(裂体锥虫属)的上鞭毛体或锥鞭毛体感染“水牛”(美洲野牛)肺(BL)细胞培养物,在37℃孵育不同时间段后固定,然后通过光学显微镜或电子显微镜检查。很少有上鞭毛体进入BL细胞,但许多锥鞭毛体能够进入;它们在2小时内粘附于细胞表面,然后似乎沉入细胞表面的沟中,直至被吞噬泡吞噬。细胞松弛素D(5 - 10微克/毫升)完全但可逆地抑制锥鞭毛体的进入,而不影响寄生虫的运动性。得出的结论是,进入依赖于锥鞭毛体表面阶段特异性成分与BL细胞上受体的相互作用,并且这种相互作用通过不涉及伪足形成的吞噬过程诱导原生动物的主动摄取。锥鞭毛体进入BL细胞后不久,吞噬泡的膜解体,此时寄生虫游离于宿主细胞的细胞质中,在接下来的24 - 48小时内转化为无鞭毛体(微鞭毛体)。然后发生复制,随后在3天后开始转化,经过过渡前鞭毛体阶段,在7天时转变为小的细胞内锥鞭毛体。前鞭毛体具有从鞭毛袋(或贮器)边缘延伸到宿主细胞细胞质中的特征性弯曲突起。8天后,BL细胞的质膜破裂,释放到上清培养基中的锥鞭毛体可重新侵入其他细胞。

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