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Dimerization of ABCG2 Analysed by Bimolecular Fluorescence Complementation

机译:双分子荧光互补分析ABCG2的二聚化

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摘要

ABCG2 is one of three human ATP binding cassette transporters that are functionally capable of exporting a diverse range of substrates from cells. The physiological consequence of ABCG2 multidrug transport activity in leukaemia, and some solid tumours is the acquisition of cancer multidrug resistance. ABCG2 has a primary structure that infers that a minimal functional transporting unit would be a homodimer. Here we investigated the ability of a bimolecular fluorescence complementation approach to examine ABCG2 dimers, and to probe the role of individual amino acid substitutions in dimer formation. ABCG2 was tagged with fragments of venus fluorescent protein (vYFP), and this tagging did not perturb trafficking or function. Co-expression of two proteins bearing N-terminal and C-terminal fragments of YFP resulted in their association and detection of dimerization by fluorescence microscopy and flow cytometry. Point mutations in ABCG2 which may affect dimer formation were examined for alterations in the magnitude of fluorescence complementation signal. Bimolecular fluorescence complementation (BiFC) demonstrated specific ABCG2 dimer formation, but no changes in dimer formation, resulting from single amino acid substitutions, were detected by BiFC analysis.
机译:ABCG2是三种人ATP结合盒转运蛋白之一,在功能上能够从细胞中输出多种底物。 ABCG2多药转运活性在白血病和某些实体瘤中的生理后果是获得对癌症的多药耐药性。 ABCG2具有一级结构,可以推断最小的功能性转运单位是同源二聚体。在这里,我们研究了双分子荧光互补方法检查ABCG2二聚体,并探究单个氨基酸取代在二聚体形成中的作用的能力。 ABCG2标记有金星荧光蛋白(vYFP)的片段,这种标记不会干扰运输或功能。共表达两种带有YFP N端和C端片段的蛋白质,通过荧光显微镜和流式细胞术检测它们的缔合和二聚化检测。检查了可能影响二聚体形成的ABCG2中的点突变,以检测荧光互补信号强度的变化。双分子荧光互补(BiFC)显示特定的ABCG2二聚体形成,但通过BiFC分析未检测到由于单个氨基酸取代导致的二聚体形成变化。

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