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利用金免疫标记技术对人肌肉中抗肌萎缩蛋白进行超微结构定位。

Ultrastructural localization of dystrophin in human muscle by using gold immunolabelling.

作者信息

Cullen M J, Walsh J, Nicholson L V, Harris J B

机构信息

Muscular Dystrophy Group Research Laboratories, Newcastle General Hospital, U.K.

出版信息

Proc R Soc Lond B Biol Sci. 1990 May 22;240(1297):197-210. doi: 10.1098/rspb.1990.0034.

Abstract

Immunolabelling with a 5 nm gold probe was used to localize dystrophin at the ultrastructural level in human muscle. The primary antibody was monoclonal, raised against a segment (amino acids 1181-1388) from the rod domain of dystrophin. The antibody (Dy4/6D3) is specific for dystrophin and shows no immunoreactivity with any protein from mdx mouse muscle or from patients with a gene deletion spanning part of the molecule recognized by the antibody (Nicholson et al. 1989 a; England et al. 1990). Using this antibody, labelling was almost entirely confined to a narrow 75 nm rim at the periphery of the muscle fibres. Histograms of the distance from the gold probe to the cytoplasmic face of the plasma membrane and of the distance between gold probes (nearest neighbour in a plane parallel with the plasma membrane) displayed modes at approximately 15 nm and 120 nm, respectively. The distribution of the probe was the same in longitudinal and transverse sections of the muscle. These observations suggest that the rod portion of the dystrophin molecule is normally arranged close to the cytoplasmic face of the plasma membrane and that the molecules form an interconnecting network. Labelling was not associated with the transverse tubular system.

摘要

使用5纳米金探针进行免疫标记,以在超微结构水平上定位人肌肉中的肌营养不良蛋白。一抗是单克隆抗体,针对肌营养不良蛋白杆状结构域的一个片段(氨基酸1181 - 1388)产生。该抗体(Dy4/6D3)对肌营养不良蛋白具有特异性,与mdx小鼠肌肉中的任何蛋白质或基因缺失患者的任何蛋白质均无免疫反应性,这些患者的基因缺失跨越了该抗体所识别分子的一部分(Nicholson等人,1989年a;England等人,1990年)。使用该抗体,标记几乎完全局限于肌纤维周边75纳米宽的边缘区域。从金探针到质膜细胞质面的距离以及金探针之间的距离(与质膜平行平面中的最近邻距离)的直方图分别显示在约15纳米和120纳米处有众数。在肌肉的纵向和横向切片中,探针的分布相同。这些观察结果表明,肌营养不良蛋白分子的杆状部分通常靠近质膜的细胞质面排列,并且这些分子形成一个相互连接的网络。标记与横管系统无关。

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