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Mutations of charged amino acids at the cytoplasmic end of transmembrane helix 2 affect transport activity of the budding yeast multidrug resistance protein Pdr5p

机译:跨膜螺旋2胞质末端带电氨基酸的突变影响发芽酵母多药耐药蛋白Pdr5p的转运活性

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摘要

Pdr5p is a major ATP-binding cassette (ABC) transporter in Saccharomyces cerevisiae. It displays a sequence and functional homology to the pathogenic Candida albicans multidrug resistance protein Cdr1p. The transmembrane helices of Pdr5p act in substrate recognition, binding, translocation and eventual removal of toxic substances out of the plasma membrane via the formation of a binding pocket. In this study, we identify two novel Pdr5 mutants (E574K and E580K), which exhibit impaired substrate efflux functions. Both mutants remained hypersensitive to all tested Pdr5p substrates without affecting their protein expression levels, localization or ATPase activities. As E574 and E580 are both located adjacent to the predicted cytoplasmic end of transmembrane helix 2, this implies that such charged residues are functionally essential for Pdr5p. Molecular docking studies suggest the possibility that oppositely charged substitution at residue E574 may disturb the interaction between the substrates and Pdr5p, resulting in impaired transport activity. Our results present new evidence, suggesting that transmembrane helix 2 plays an important role for the efflux function of Pdr5p.
机译:Pdr5p是酿酒酵母中的主要ATP结合盒(ABC)转运蛋白。它显示出与致病性白色念珠菌多药耐药蛋白Cdr1p的序列和功能同源性。 Pdr5p的跨膜螺旋通过结合袋的形成,在底物识别,结合,易位以及最终从质膜中去除有毒物质方面发挥作用。在这项研究中,我们确定了两个新的Pdr5突变体(E574K和E580K),它们表现出受损的底物外排功能。两种突变体均对所有测试的Pdr5p底物保持超敏性,而不会影响其蛋白表达水平,定位或ATPase活性。由于E574和E580都位于跨膜螺旋2的预计胞质末端附近,这意味着这些带电荷的残基对Pdr5p具有功能上的必要性。分子对接研究表明,残基E574上带相反电荷的取代可能会干扰底物与Pdr5p之间的相互作用,从而导致转运活性受损的可能性。我们的结果提供了新的证据,表明跨膜螺旋2在Pdr5p的外排功能中起着重要作用。

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