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The MrpA, MrpB and MrpD subunits of the Mrp antiporter complex in Bacillus subtilis contain membrane-embedded and essential acidic residues

机译:MRP枯草芽孢杆菌MRP抗原膜络合物的MRPA,MRPB和MRPD亚基含有膜 - 嵌入和必要的酸性残基

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Bacillus subtilis Mrp is a unique Na+/H+ antiporter with a multicomponent structure consisting of the mrpABCDEFG gene products. We have previously reported that the conserved and putative membrane-embedded Glu-113, Glu-657, Asp-743 and Glu-747 of MrpA (ShaA) are essential for the transport function. In this study, we further investigated the functional involvement of the equivalent conserved acidic residues of other Mrp proteins in heterologous Escherichia coli and natural B. subtilis backgrounds. Asp-121 of MrpB and Glu-137 of MrpD were additionally identified to be essential for the transport function in both systems. Glu-137 of MrpD and Glu-113 of MrpA were found to be conserved in the homologous MrpD/MrpA proteins as well as in the homologous subunits of H+-translocating primary active transporters such as Nuo and Mbh, suggesting their critical role in ion binding. The remaining essential acidic residues clustered in the C-terminal domain of MrpA (Glu-657, Asp-743 and Glu-747) and MrpB (Asp-121); these subunits are fused in some Gram-negative species. It is possible that the MrpA, MrpB and MrpD subunits, which contain essential transmembrane acidic residues, form the ion translocation site(s) of the Mrp antiporter complex.
机译:芽孢杆菌枯草芽孢杆菌MRP是一种独特的Na + / H +抗糖剂,其具有MRPABCDEFG基因产物组成的多组分结构。我们此前报道,MRPA(SHAA)的保守和推定的膜嵌入式GLU-113,GLU-657,ASP-743和GLU-747对运输功能至关重要。在本研究中,我们进一步研究了在异源大肠杆菌和天然B.枯草芽孢杆菌背景中其他MRP蛋白的等同保守酸性残基的功能介入。另外识别MRPD的MRPB和GLU-137的ASP-121对于两个系统中的运输功能至关重要。发现MRPA的MRPD和Glu-113的Glu-137在同源MRPD / MRPA蛋白中以及H + -Transcocating初级活性转运蛋白的同源亚基中保存,如Nuo和MBH,表明它们在离子结合中的关键作用。将剩余的必需酸性残基聚集在MRPA(Glu-657,ASP-743和Glu-747)和MRPB(ASP-121)中的C-末端结构域;这些亚基在一些革兰氏阴性物种中融合。含有必需跨膜酸性残基的MRPA,MRPB和MRPD亚基可能形成MRP抗原醇复合物的离子易位位点。

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