Immunofluorescence Detection of the Cytoskeleton and Extracellular Matrix in Tissue and Cultured Cells

免疫染色 免疫荧光 抗原性 细胞骨架 细胞外基质 细胞生物学 表位 生物 抗原 化学 细胞 生物化学 免疫学 抗体 免疫组织化学
作者
Josiane Smith-Clerc,Boris Hinz
出处
期刊:Methods in molecular biology [Springer Science+Business Media]
卷期号:: 43-57 被引量:26
标识
DOI:10.1007/978-1-60327-345-9_4
摘要

"A picture is worth a thousand words" goes the proverb. A poor picture however can be worse than saying nothing at all. This is particularly true for immunofluorescence pictures that in addition to their informative character bear an esthetic component. We here provide a panel of straightforward methods to process tissue sections and cultured cells for immunostaining of cytoskeletal elements, primarily those associated with actin filaments. We want to emphasize to the reader the fact that the choice of the processing method will have an important influence on the outcome of the immunostaining and thus on the interpretation of the results. Fixation of cultured cells with cross-linking reagents such as paraformaldehyde efficiently preserves structural elements at the expense of reduced antigenicity. The degree and timing of cell permeabilization with detergents, along with chemical cross-linking, contributes to the clarity and resolution of distinct structures but can also lead to loss of information. Fixation with organic solvents like methanol will, in most cases, better preserve antigens but will produce a higher background and impact on structural integrity. Therefore, it is recommended to test different protocols for a "new" protein or epitope - the results will pay back your investment.
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