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首页> 外文期刊>Proteins: Structure, Function, and Genetics >An NMR study of the N-terminal domain of wild-type hERG and a T65P trafficking deficient hERG mutant.
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An NMR study of the N-terminal domain of wild-type hERG and a T65P trafficking deficient hERG mutant.

机译:对野生型hERG和T65P转运缺陷型hERG突变体的N端结构域进行NMR研究。

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摘要

The human Ether-a-go-go Related Gene (hERG) potassium channel plays an important role in the heart by controlling the rapid delayed rectifier current. The N-terminal 135 residues (NTD) contain a Per-Arnt-Sim (PAS) domain and an N-terminal amphipathic helix. NMR relaxation analysis and H/D exchange experiments on the NTD demonstrated that the amphipathic helix is rigid and solvent accessible. An NTD containing a T65P mutation, which causes a hERG channel trafficking deficiency, was purified from E.coli. The mutant protein did not aggregate in gel filtration analysis and the amide cross peaks of its residues disappeared in an HSQC spectrum indicating the possibility of structural changes. A carbon chemical shift comparison of the residues with cross peaks in the HSQC spectrum showed no clear difference between the purified wild-type protein and the purified mutant. There were multiple conformations observed for the T65P mutant protein at high temperatures from HSQC experiments and a thermal stability assay showed that the T65P mutation reduced the thermal stability of NTD. This instability may affect protein folding or structural dynamics of other regions.
机译:人类以太相关基因(hERG)钾离子通道通过控制快速延迟的整流器电流在心脏中发挥重要作用。 N末端135个残基(NTD)包含Per-Arnt-Sim(PAS)域和N末端两亲性螺旋。在NTD上进行NMR弛豫分析和H / D交换实验表明,两亲性螺旋是刚性的,并且可以接近溶剂。从大肠杆菌中纯化出含有导致hERG通道运输缺陷的T65P突变的NTD。突变蛋白在凝胶过滤分析中未聚集,其残基的酰胺交叉峰在HSQC光谱中消失,表明可能发生结构变化。在HSQC谱图中具有交叉峰的残基的碳化学位移比较表明,纯化的野生型蛋白和纯化的突变体之间没有明显的差异。通过HSQC实验在高温下观察到T65P突变蛋白的多种构象,热稳定性分析表明T65P突变降低了NTD的热稳定性。这种不稳定性可能影响蛋白质折叠或其他区域的结构动力学。

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