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A novel-type substrate-selectivity filter and ER-exit determinants in the UapA purine transporter.

机译:UapA嘌呤转运蛋白中的新型底物选择性过滤器和ER出口决定因素。

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We present a functional analysis of the last alpha-helical transmembrane segment (TMS12) of UapA, a uric acid-xanthine/H+ symporter in Aspergillus nidulans and member of the nucleobase-ascorbate transporter (NAT) family. First, we performed a systematic mutational analysis of residue F528, located in the middle of TMS12, which was known to be critical for UapA specificity. Substitution of F528 with non-aromatic amino acid residues (Ala, Thr, Ser, Gln, Asn) did not affect significantly the kinetics of UapA for its physiological substrates, but allowed high-capacity transport of several novel purines and pyrimidines. Allele-specific combinations of F528 substitutions with mutations in Q408, a residue involved in purine binding, led to an array of UapA molecules with different kinetic and specificity profiles. We propose that F528 plays the role of a novel-type selectivity filter, which, in conjunction with a distinct purine-binding site, control UapA-mediated substrate translocation. We further studied the role of TMS12 by analysing the effect of its precise deletion and chimeric molecules in which TMS12 was substituted with analogous domains from other NATs. The presence of any of the TMS12 tested was necessary for ER-exit while their specific amino acid composition affected the kinetics of chimeras.
机译:我们介绍功能分析的UapA,构巢曲霉中的尿酸黄嘌呤/ H +转运蛋白和核碱基抗坏血酸转运蛋白(NAT)成员的最后一个UapA的α-螺旋跨膜段(TMS12)。首先,我们对位于TMS12中部的F528残基进行了系统的突变分析,这对于UapA特异性至关重要。用非芳香族氨基酸残基(Ala,Thr,Ser,Gln,Asn)取代F528不会显着影响UapA对其生理底物的动力学,但允许高容量转运几种新型嘌呤和嘧啶。 F528置换的等位基因特异性组合与Q408中的突变有关,Q408是嘌呤结合中涉及的一个残基,导致形成一系列具有不同动力学和特异性的UapA分子。我们建议F528发挥新型过滤器的作用,结合独特的嘌呤结合位点,控制UapA介导的底物易位。我们通过分析TMS12的精确缺失和嵌合分子(其中TMS12被其他NAT的类似域取代)的作用,进一步研究了TMS12的作用。存在任何被测试的TMS12对于ER出口都是必需的,而它们的特定氨基酸组成会影响嵌合体的动力学。

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