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A stretch-activated anion channel is up-regulated by the malaria parasite plasmodium falciparum

机译:疟疾寄生虫恶性疟原虫可上调拉伸激活的阴离子通道

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摘要

A recent study on malaria-infected human red blood cells (RBCs) has shown induced ion channel activity in the host cell membrane, but the questions of whether they are host- or parasite-derived and their molecular nature have not been resolved. Here we report a comparison of a malaria-induced anion channel with an endogenous anion channel in Plasmodium falciparum-infected human RBCs. Ion channel activity was measured using the whole-cell, cell-attached and excised inside-out configurations of the patch-clamp method. Parasitised RBCs were cultured in vitro, using co-cultured uninfected RBCs as controls. Unstimulated uninfected RBCs possessed negligible numbers of active anion channels. However, anion channels could be activated in the presence of protein kinase A (PKA) and ATP in the pipette solution or by membrane deformation. These channels displayed linear conductance (∼15 pS), were blocked by known anion channel inhibitors and showed the permeability sequence I > Br > Cl. In addition, in less than 5 % of excised patches, an outwardly rectifying anion channel (∼80 pS, outward conductance) was spontaneously active. The host membrane of malaria-infected RBCs possessed spontaneously active anion channel activity, with identical conductances, pharmacology and selectivity to the linear conductance channel measured in stimulated uninfected RBCs. Furthermore, the channels measured in malaria-infected RBCs were shown to have a low open-state probability (Po) at positive potentials, which explains the inward rectification of membrane conductance observed when using the whole-cell configuration. The data are consistent with the presence of two endogenous anion channels in human RBCs, of which one (the linear conductance channel) is up-regulated by the malaria parasite P. falciparum.
机译:最近一项关于疟疾感染的人类红细胞(RBC)的研究表明,宿主细胞膜中存在诱导的离子通道活性,但是有关它们是宿主还是寄生虫及其分子性质的问题尚未解决。在这里,我们报告恶性疟原虫感染的人类红细胞中疟疾诱导的阴离子通道与内源性阴离子通道的比较。离子通道活性是使用膜片钳方法的全细胞,细胞附着和切除的内向外构型进行测量的。使用共培养的未感染RBC作为对照,体外培养寄生的RBC。未经刺激的未感染红细胞的活性阴离子通道数量可忽略不计。但是,在移液管中存在蛋白激酶A(PKA)和ATP的情况下或通过膜变形,可以激活阴离子通道。这些通道显示线性电导(〜15 pS),被已知的阴离子通道抑制剂阻滞,并显示通透性序列I ---。此外,在少于5%的切除斑块中,一个向外整流的阴离子通道(〜80 pS,向外传导)是自发激活的。疟疾感染的红细胞的宿主膜具有自发的活性阴离子通道活性,在刺激的未感染红细胞中测得的线性电导通道具有相同的电导,药理学和选择性。此外,在疟疾感染的红细胞中测得的通道在正电势下具有较低的开态概率(Po),这解释了使用全细胞配置时观察到的膜电导的向内整流。数据与人红细胞中存在两个内源性阴离子通道一致,其中一个(线性电导通道)被疟原虫恶性疟原虫上调。

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