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首页> 外文期刊>Molecular and Biochemical Parasitology >The Plasmodium falciparum MESA erythrocyte cytoskeleton-binding (MEC) motif binds to erythrocyte ankyrin
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The Plasmodium falciparum MESA erythrocyte cytoskeleton-binding (MEC) motif binds to erythrocyte ankyrin

机译:疟原虫Mesa红细胞细胞骨架结合(MEC)基序与红细胞ankyrin结合

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摘要

The MESA erythrocyte cytoskeleton binding (MEC) motif is a 13-amino acid sequence found in 14 exported Plasmodium falciparum proteins. First identified in the P. falciparum Mature-parasite-infected Erythrocyte Surface Antigen (MESA), the MEC motif is sufficient to target proteins to the infected red blood cell cytoskeleton. To identify host cell targets, purified MESA MEC motif was incubated with a soluble extract from uninfected erythrocytes, precipitated and subjected to mass spectrometry. The most abundant co-purifying protein was erythrocyte ankyrin (ANK1). A direct interaction between the MEC motif and ANK1 was independently verified using co-purification experiments, the split-luciferase assay, and the yeast two-hybrid assay. A systematic mutational analysis of the core MEC motif demonstrated a critical role for the conserved aspartic acid residue at the C-terminus of the MEC motif for binding to both erythrocyte inside-out vesicles and to ANK1. Using a panel of ANK1 constructs, the MEC motif binding site was localized to the ZU5(C) domain, which has no known function. The MEC motif had no impact on erythrocyte deformability when introduced into uninfected erythrocyte ghosts, suggesting the MEC motif's primary function is to target exported proteins to the cytoskeleton. Finally, we show that PF3D7_0402100 (PFD0095c) binds to ANK1 and band 4.1, likely through its MEC and PHIST motifs, respectively. In conclusion, we have provided multiple lines of evidence that the MEC motif binds to erythrocyte ANK1.
机译:MESA红细胞细胞骨架结合(MEC)基序是14种出口的疟原虫蛋白质中发现的13-氨基酸序列。首先在P.Malciparum成熟 - 寄生虫感染的红细胞表面抗原(MESA)中鉴定,MEC基序足以靶向受感染的红细胞细胞骨架。为了鉴定宿主细胞靶标,将纯化的MESA MEC基序与来自未感染的红细胞的可溶性提取物一起孵育,沉淀并进行质谱法。最丰富的共净化蛋白质是红细胞Ankyrin(ANK1)。使用共纯化实验,分裂 - 荧光素酶测定和酵母双杂交测定,独立地验证了MEC基序和ANK1之间的直接相互作用。核心MEC基质的系统突变分析证明了MEC基序的C-末端的保守天冬氨酸残基的关键作用,用于与红细胞内部囊泡和ANK1结合。使用ANK1构建体的面板,MEC基序结合位点被定位于ZU5(C)域,其没有已知功能。当引入未感染的红细胞鬼魂时,MEC MOTIF对红细胞变形性没有影响,表明MEC MOTIF的主要功能是将出口的蛋白质靶向细胞骨架。最后,我们显示PF3D7_0402100(PFD0095C)分别通过其MEC和Phist图案绑定到ANK1和频段4.1。总之,我们提供了多条证据表明MEC基序与红细胞ANK1结合。

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