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可特异性标记骨骼肌表面和T小管膜中钠通道的抗体的表位定位。

Localization of epitopes for antibodies that differentially label sodium sodium channels in skeletal muscle surface and T-tubular membranes.

作者信息

Cohen S A, Barchi R L

机构信息

Department of Medicine, University of Pennsylvania School of Medicine, Philadelphia 19104.

出版信息

J Membr Biol. 1992 Jun;128(3):219-26. doi: 10.1007/BF00231814.

DOI:10.1007/BF00231814
PMID:1380092
Abstract

We previously characterized two monoclonal antibodies, A/B2 and L/D3, that bind to the amino-terminus of the sodium channel but produce distinct immunocytochemical patterns in innervated adult skeletal muscle. Because these findings suggested the presence of several channel isoforms, we sought to define the epitopes for each antibody. Five peptides encompassing the amino-terminal 126 residues of the adult skeletal muscle sodium channel were synthesized and tested by radioimmunoassay against each antibody. Both monoclonals bound only to a peptide comprising residues 1-30 (I1-30). A nested set of peptides within this region was then synthesized and used to compete for antibody binding to I1-30. L/D3 binding was quantitatively inhibited by oligopeptides 1-30, 7-30, 13-30, and 19-30 but not 25-30, while binding of A/B2 was blocked only by the intact I1-30 peptide. This data implies that the epitope for L/D3 lies within residues 19-25 while the epitope for A/B2 is contained within residues 1-6. These tentative epitope localizations were confirmed using both proteolytic cleavage of I1-30 and immunoreactivity of a peptide corresponding to residues 1-12 with A/B2 but not L/D3. Therefore, epitopes for each monoclonal antibody are present in the SkM-1 sequence and are in close proximity in the amino-terminus of the protein. Their characteristic immunocytochemical labeling patterns may reflect differing accessibility of the epitopes in various membrane environments.

摘要

我们之前鉴定了两种单克隆抗体,A/B2和L/D3,它们与钠通道的氨基末端结合,但在受神经支配的成年骨骼肌中产生不同的免疫细胞化学模式。由于这些发现提示存在几种通道亚型,我们试图确定每种抗体的表位。合成了包含成年骨骼肌钠通道氨基末端126个残基的五种肽,并通过放射免疫测定法针对每种抗体进行测试。两种单克隆抗体都仅与包含残基1 - 30(I1 - 30)的肽结合。然后合成了该区域内的一组嵌套肽,并用于竞争抗体与I1 - 30的结合。L/D3的结合被寡肽1 - 30、7 - 30、13 - 30和19 - 30定量抑制,但不被25 - 30抑制,而A/B2的结合仅被完整的I1 - 30肽阻断。该数据表明L/D3的表位位于残基19 - 25内,而A/B2的表位包含在残基1 - 6内。使用I1 - 30的蛋白水解切割以及与A/B2而非L/D3对应的残基1 - 12的肽的免疫反应性证实了这些初步的表位定位。因此,每种单克隆抗体的表位存在于SkM - 1序列中,并且在蛋白质的氨基末端紧密相邻。它们独特的免疫细胞化学标记模式可能反映了表位在各种膜环境中的不同可及性。

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