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疟原虫转位通道成分 EXP2 促进肝细胞入侵。

Plasmodium translocon component EXP2 facilitates hepatocyte invasion.

机构信息

Instituto de Medicina Molecular João Lobo Antunes, Faculdade de Medicina, Universidade de Lisboa, 1649-028, Lisboa, Portugal.

School of Medicine, Deakin University, Waurn Ponds, Geelong, Australia.

出版信息

Nat Commun. 2020 Nov 6;11(1):5654. doi: 10.1038/s41467-020-19492-4.

Abstract

Plasmodium parasites possess a translocon that exports parasite proteins into the infected erythrocyte. Although the translocon components are also expressed during the mosquito and liver stage of infection, their function remains unexplored. Here, using a combination of genetic and chemical assays, we show that the translocon component Exported Protein 2 (EXP2) is critical for invasion of hepatocytes. EXP2 is a pore-forming protein that is secreted from the sporozoite upon contact with the host cell milieu. EXP2-deficient sporozoites are impaired in invasion, which can be rescued by the exogenous administration of recombinant EXP2 and alpha-hemolysin (an S. aureus pore-forming protein), as well as by acid sphingomyelinase. The latter, together with the negative impact of chemical and genetic inhibition of acid sphingomyelinase on invasion, reveals that EXP2 pore-forming activity induces hepatocyte membrane repair, which plays a key role in parasite invasion. Overall, our findings establish a novel and critical function for EXP2 that leads to an active participation of the host cell in Plasmodium sporozoite invasion, challenging the current view of the establishment of liver stage infection.

摘要

疟原虫寄生虫拥有一个转位器,可将寄生虫蛋白输出到受感染的红细胞中。尽管转位器组件在蚊子和肝脏感染阶段也有表达,但它们的功能仍未被探索。在这里,我们使用遗传和化学测定的组合,表明转位器组件 Exported Protein 2(EXP2)对于侵入肝细胞至关重要。EXP2 是一种形成孔的蛋白质,在与宿主细胞环境接触时从孢子中分泌出来。缺乏 EXP2 的孢子虫在入侵中受到损害,但可以通过外源性给予重组 EXP2 和α-溶血素(金黄色葡萄球菌形成孔的蛋白质)以及酸性鞘磷脂酶来挽救。后者,以及化学和遗传抑制酸性鞘磷脂酶对入侵的负面影响,表明 EXP2 形成孔的活性诱导肝细胞膜修复,这在寄生虫入侵中起着关键作用。总的来说,我们的发现确立了 EXP2 的一个新的关键功能,导致宿主细胞积极参与疟原虫孢子虫的入侵,这对肝脏感染阶段的当前观点提出了挑战。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7651/7648069/d1484a10ac2e/41467_2020_19492_Fig1_HTML.jpg

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