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

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...

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Detalles Bibliográficos
Autores principales: Hammerling, U, Polliack, A, Lampen, N, Sabety, M, De Harven, E
Formato: Texto
Lenguaje:English
Publicado: The Rockefeller University Press 1975
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2190526/
https://www.ncbi.nlm.nih.gov/pubmed/1089747
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author Hammerling, U
Polliack, A
Lampen, N
Sabety, M
De Harven, E
author_facet Hammerling, U
Polliack, A
Lampen, N
Sabety, M
De Harven, E
author_sort Hammerling, U
collection PubMed
description 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.
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spelling pubmed-21905262008-04-17 Scanning electron microscopy of tobacco mosaic virus-labeled lymphocyte surface antigens Hammerling, U Polliack, A Lampen, N Sabety, M De Harven, E J Exp Med Articles 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. The Rockefeller University Press 1975-02-01 /pmc/articles/PMC2190526/ /pubmed/1089747 Text en This article is distributed under the terms of an Attribution–Noncommercial–Share Alike–No Mirror Sites license for the first six months after the publication date (see http://www.rupress.org/terms). After six months it is available under a Creative Commons License (Attribution–Noncommercial–Share Alike 4.0 Unported license, as described at http://creativecommons.org/licenses/by-nc-sa/4.0/).
spellingShingle Articles
Hammerling, U
Polliack, A
Lampen, N
Sabety, M
De Harven, E
Scanning electron microscopy of tobacco mosaic virus-labeled lymphocyte surface antigens
title Scanning electron microscopy of tobacco mosaic virus-labeled lymphocyte surface antigens
title_full Scanning electron microscopy of tobacco mosaic virus-labeled lymphocyte surface antigens
title_fullStr Scanning electron microscopy of tobacco mosaic virus-labeled lymphocyte surface antigens
title_full_unstemmed Scanning electron microscopy of tobacco mosaic virus-labeled lymphocyte surface antigens
title_short Scanning electron microscopy of tobacco mosaic virus-labeled lymphocyte surface antigens
title_sort scanning electron microscopy of tobacco mosaic virus-labeled lymphocyte surface antigens
topic Articles
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2190526/
https://www.ncbi.nlm.nih.gov/pubmed/1089747
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AT deharvene scanningelectronmicroscopyoftobaccomosaicviruslabeledlymphocytesurfaceantigens