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Red Cells: Cytoplasmic remodeling of erythrocyte raft lipids during infection by the human malaria parasite Plasmodium falciparum

机译:红细胞:人类疟原虫恶性疟原虫感染过程中红细胞筏脂质的细胞质重塑

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摘要

Studies of detergent-resistant membrane (DRM) rafts in mature erythrocytes have facilitated identification of proteins that regulate formation of endovacuolar structures such as the parasitophorous vacuolar membrane (PVM) induced by the malaria parasite Plasmodium falciparum. However, analyses of raft lipids have remained elusive because detergents interfere with lipid detection. Here, we use primaquine to perturb the erythrocyte membrane and induce detergent-free buoyant vesicles, which are enriched in cholesterol and major raft proteins flotillin and stomatin and contain low levels of cytoskeleton, all characteristics of raft microdomains. Lipid mass spectrometry revealed that phosphatidylethanolamine and phosphatidylglycerol are depleted in endovesicles while phosphoinositides are highly enriched, suggesting raft-based endovesiculation can be achieved by simple (non–receptor-mediated) mechanical perturbation of the erythrocyte plasma membrane and results in sorting of inner leaflet phospholipids. Live-cell imaging of lipid-specific protein probes showed that phosphatidylinositol (4,5) bisphosphate (PIP2) is highly concentrated in primaquine-induced vesicles, confirming that it is an erythrocyte raft lipid. However, the malarial PVM lacks PIP2, although another raft lipid, phosphatidylserine, is readily detected. Thus, different remodeling/sorting of cytoplasmic raft phospholipids may occur in distinct endovacuoles. Importantly, erythrocyte raft lipids recruited to the invasion junction by mechanical stimulation may be remodeled by the malaria parasite to establish blood-stage infection.
机译:对成熟的红细胞中耐洗涤剂膜(DRM)筏的研究有助于鉴定调节内腔结构形成的蛋白质,例如由疟原虫恶性疟原虫诱导的寄生虫液泡膜(PVM)。但是,由于去污剂会干扰脂质检测,因此对筏状脂质的分析仍然难以捉摸。在这里,我们使用伯氨喹来扰动红细胞膜并诱导无洗涤剂的漂浮囊泡,这些囊泡富含胆固醇以及主要的筏蛋白flotillin和stomatin,并且含有低水平的细胞骨架,这是筏微域的所有特征。脂质质谱分析显示,内囊泡中的磷脂酰乙醇胺和磷脂酰甘油含量很高,而磷酸肌醇则高度富集,这表明可以通过对红细胞质膜进行简单的(非受体介导的)机械扰动来实现基于筏的内囊泡化,并导致内部小叶磷脂的分选。脂质特异性蛋白质探针的活细胞成像显示磷脂酰肌醇(4,5)二磷酸(PIP2)在伯氨喹诱导的囊泡中高度浓缩,证实它是一种红细胞筏脂质。但是,疟疾PVM缺乏PIP2,尽管很容易检测到另一种筏脂磷脂酰丝氨酸。因此,细胞质筏磷脂的不同重塑/分类可能发生在不同的内腔中。重要的是,通过机械刺激被募集到入侵连接处的红细胞筏脂质可能被疟原虫重塑以建立血液阶段感染。

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