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使构巢曲霉中编码高亲和力硝酸盐转运蛋白的nrtA基因失活的错义突变。

Missense mutations that inactivate the Aspergillus nidulans nrtA gene encoding a high-affinity nitrate transporter.

作者信息

Kinghorn James R, Sloan Joan, Kana'n Ghassan J M, Dasilva Edisio R, Rouch Duncan A, Unkles Shiela E

机构信息

School of Biology, University of Saint Andrews, Fife, Scotland, UK.

出版信息

Genetics. 2005 Mar;169(3):1369-77. doi: 10.1534/genetics.104.036590. Epub 2004 Nov 15.

Abstract

The transport of nitrate into prokaryotic and eukaryotic cells, of considerable interest to agriculture, ecology, and human health, is carried out by members of a distinct cluster of proteins within the major facilitator superfamily. To obtain structure/function information on this important class of nitrate permeases, a collection of chemically induced mutations in the nrtA gene encoding a 12-transmembrane domain, high-affinity nitrate transporter from the eukaryote Aspergillus nidulans was isolated and characterized. This mutational analysis, coupled with protein alignments, demonstrates the utility of the approach to predicting peptide motifs and individual residues important for the movement of nitrate across the membrane. These include the highly conserved nitrate signature motif (residues 166-173) in Tm 5, the conserved charged residues Arg87 (Tm 2) and Arg368 (Tm 8), as well as the aromatic residue Phe47 (Tm 1), all within transmembrane helices. No mutations were observed in the large central loop (Lp 6/7) between Tm 6 and Tm 7. Finally, the study of a strain with a conversion of Trp481 (Tm 12) to a stop codon suggests that all 12 transmembrane domains and/or the C-terminal tail are required for membrane insertion and/or stability of NrtA.

摘要

硝酸盐向原核细胞和真核细胞的转运对农业、生态学及人类健康具有重要意义,该过程由主要转运子超家族中一个独特的蛋白质簇成员来完成。为了获取有关这类重要硝酸盐通透酶的结构/功能信息,我们分离并鉴定了一系列在nrtA基因中化学诱导产生的突变,该基因编码来自真核生物构巢曲霉的一个具有12个跨膜结构域的高亲和力硝酸盐转运蛋白。这种突变分析与蛋白质比对相结合,证明了该方法在预测对硝酸盐跨膜转运重要的肽基序和单个残基方面的实用性。这些包括跨膜螺旋内位于第5个跨膜结构域(Tm 5)中高度保守的硝酸盐特征基序(残基166 - 173)、保守的带电荷残基精氨酸87(Tm 2)和精氨酸368(Tm 8),以及芳香族残基苯丙氨酸47(Tm 1)。在第6个和第7个跨膜结构域(Tm 6和Tm 7)之间的大中心环(Lp 6/7)中未观察到突变。最后,对一个将色氨酸481(Tm 12)转换为终止密码子的菌株的研究表明,所有12个跨膜结构域和/或C末端尾巴对于NrtA插入膜中和/或其稳定性是必需的。

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