首页> 美国卫生研究院文献>The Journal of Neuroscience >Topological localization of a segment of the eel voltage-dependent sodium channel primary sequence (AA 927-938) that discriminates between models of tertiary structure
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Topological localization of a segment of the eel voltage-dependent sodium channel primary sequence (AA 927-938) that discriminates between models of tertiary structure

机译:鳗鱼电压依赖性钠离子通道一级序列(AA 927-938)的一部分的拓扑定位可区分三级结构模型

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摘要

Antibodies were raised against a synthetic peptide corresponding to residues 927–938 of the eel electroplax sodium channel primary sequence. This segment, lying between putative internal repeat domains II and III, is postulated to be exposed on the cytoplasmic surface of the membrane in several recent models of channel tertiary structure and on the external surface in another. The antiserum and affinity-purified IgG derived from it specifically recognize the peptide and the eel sodium channel in a solid-phase radioimmunoassay and bind to a single diffuse band of 260–280 kDa on Western blots of eel electroplax membrane proteins. All reactions are blocked by co-incubation of the antibodies with the synthetic peptide (1 microM). The antibody immunoprecipitates the solubilized channel in a form that retains its characteristic high-affinity binding of saxitoxin. In eel electroplax, the antibodies label only the innervated membrane known to contain sodium channels; at the ultrastructural level, this labeling is exclusively associated with the cytoplasmic surface of the membrane. Sodium channels containing the epitope are not seen in the postsynaptic membrane or in the membrane of the presynaptic nerve terminal. Segment 927–938 of the eel sodium channel is accessible on the surface of the protein in its solubilized form and is exposed in the cytoplasmic face of the innervated membrane of the electroplax in situ. This location is consistent with 3 models of channel structure but not with a fourth.
机译:产生了针对一种合成肽的抗体,该肽对应于鳗鱼电pla钠通道一级序列的第927-938位残基。在一些最新的通道三级结构模型中,假定的内部重复结构域II和III之间的该段被假定暴露在膜的细胞质表面,而在另一个模型中则暴露在外表面。衍生自其的抗血清和亲和纯化的IgG在固相放射免疫分析中特异性识别肽和鳗钠通道,并在鳗电膜蛋白的蛋白质印迹上结合到260-280 kDa的单个扩散带。通过将抗体与合成肽(1 microM)共孵育来封闭所有反应。抗体以保留其与毒素的特征性高亲和力结合的形式免疫沉淀溶解的通道。在鳗鱼电pla中,抗体仅标记已知含有钠通道的神经支膜。在超微结构水平上,该标记仅与膜的细胞质表面相关。在突触后膜或突触前神经末梢的膜中未见含有表位的钠通道。鳗鱼钠通道的第927-938段位于蛋白质表面,处于其溶解形式,并在原位电化膜神经支配膜的细胞质表面暴露。此位置与3种通道结构模型一致,但与第四个模型不一致。

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