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烟草花叶病毒标记的淋巴细胞表面抗原的扫描电子显微镜观察

Scanning electron microscopy of tobacco mosaic virus-labeled lymphocyte surface antigens.

作者信息

Hammerling U, Polliack A, Sabety L M, Harven E

出版信息

J Exp Med. 1975 Feb 1;141(2):518-23. doi: 10.1084/jem.141.2.518.

Abstract

The study of surface antigen by immunoelectron microscopy has been hampered by the fact that thin sections of cells provide only a view of the cell perimeter in an essentially two- dimensional fashion. Although the reconstruction of the entire cell from serial sections has been accomplished (1), it remains too exacting a technique and will find only exceptional application. Carbon-platinum replicas (2) allow the inspection of larger surface areas and therefore are better suited for studying the distribution of antigens (3). But since only relatively smooth surfaces will yield stable replicas, cells with large numbers of microvilli are not amenable to this technique. Despire its limited resolution, scanning electron microscopy (SEM) seems to be the method of choice because it can provide a view of almost half of the surface of a cell close to its natural configuration, particularly after critical point or freeze drying (4, 5). Immunological-labeling methods have not yet been routinely applied to SEM although both latex spheres (6) and hemocyanin (7) have been used with some success. The optimal visual marker should possess the following properties: be of a distinctive shape, chemically stable, and have per se a low binding affinity for cell surfaces. Tobacco mosaic virus (TMV), a marker with which we are familiar in transmission electron microscopy (8), seems to meet these demands; it has rod-like shape and defined dimensions (15 x 300 nm) and in addition it can easily be distinguished from surface microvilli. As the hybrid antibody technique (9) is also applicable to TMV, we have attempted to combine such immunological labeling with SEM. We present evidence that surface antigens can indeed be visualized by SEM, using the TMV marker in conjunction with the hybrid antibody technique.

摘要

免疫电子显微镜对表面抗原的研究受到了限制,因为细胞的薄切片只能以基本二维的方式展示细胞周边。虽然已经能够从连续切片重建整个细胞(1),但这仍是一项要求过高的技术,仅在特殊情况下应用。碳-铂复型(2)可以观察更大的表面积,因此更适合研究抗原的分布(3)。但由于只有相对光滑的表面才能产生稳定的复型,有大量微绒毛的细胞不适合这种技术。尽管扫描电子显微镜(SEM)分辨率有限,但它似乎是首选方法,因为它可以提供接近细胞自然形态的近半个细胞表面的图像,特别是在临界点干燥或冷冻干燥后(4,5)。免疫标记方法尚未常规应用于扫描电子显微镜,尽管乳胶球(6)和血蓝蛋白(7)已经取得了一些成功。最佳的视觉标记应具有以下特性:形状独特、化学稳定,并且本身对细胞表面的结合亲和力低。烟草花叶病毒(TMV)是我们在透射电子显微镜中熟悉的一种标记(8),似乎满足这些要求;它呈杆状,尺寸确定(15×300nm),此外还能很容易地与表面微绒毛区分开来。由于杂交抗体技术(9)也适用于TMV,我们尝试将这种免疫标记与扫描电子显微镜结合起来。我们提供的证据表明,使用TMV标记结合杂交抗体技术,表面抗原确实可以通过扫描电子显微镜观察到。

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Scanning electron microscopy of cells in culture.培养细胞的扫描电子显微镜检查。
Exp Cell Res. 1972;71(2):313-24. doi: 10.1016/0014-4827(72)90299-6.
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The fluid mosaic model of the structure of cell membranes.细胞膜结构的流动镶嵌模型。
Science. 1972 Feb 18;175(4023):720-31. doi: 10.1126/science.175.4023.720.

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