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Related Links Fluorochromes Selection for Multicolor ICC/IF Sample Preparation for ICC/IF Experiments Controls for ICC/IF Experiments Useful Links ICC Handbook
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What is the Significance of Fixation?Fixatives preserve cellular morphology, integrity and structure by preventing proteolytic enzyme induced autolysis of cells and the process of putrefaction (cellular decay). Fixatives also enhance the rigidity and mechanical strength of cells, which is critical to withstanding the various, sometimes rigorous, steps of the immunostaining procedure. Cells should be fixed immediately following removal from cell culture conditions to limit autolysis and putrefaction. If there is a delay in fixation or if fixation is incomplete, the antigen may disperse into neighboring sub-cellular regions. This results in misleading staining as shown in the example below.
Major Types of FixativesCross-linking fixativesAldehydes, such as formalin or formaldehyde, are the preferred fixative for preserving cell morphology and are well suited for immunostaining of membrane proteins. These fixatives crosslink proteins via free amine groups, forming intermolecular bridges and a network of linked antigenic proteins. Crosslinking masks antigens and reduces target antigenicity which may be perpetuated by a long fixation time. Cells are typically incubated with 4% formaldehyde or 10% formalin solution for 10-20 minutes at room temperature.Precipitating fixativesSome organic solvents, such as methanol, acetone, and picric acid, act as strong dehydrants and cause the precipitation of cellular proteins. While these fixatives are effective at preserving cellular architecture, they can remove small soluble molecules and lipids. In addition, precipitating fixatives are not recommended for use with overexpressed fluorescent proteins (e.g. GFP) because they can denature these proteins. In a standard fixation protocol, ice-cold methanol is added to cells for 10-20 minutes at 4˚C. Other protocols may involve acetone, a milder fixative compared to methanol fixation or a mixture with an equal ratio of chilled methanol and acetone (1:1). Cells undergoing acetone or methanol fixation may not require a permeabilization step.Is There a Difference Between 10% Formalin and 4% Paraformaldehyde (PFA)?Paraformaldehyde (PFA) is a powder form of polymerized formaldehyde that needs to be dissolved in PBS before it is used as a fixative. Formalin is a commercially available, saturated formaldehyde solution (37% w/v) that also contains methanol as a stabilizer to prevent the polymerization of formaldehyde. A 3.7% PFA solution is equivalent to a 10% formalin solution. What are the Major Advantages and Disadvantages of Various Fixatives?
* Always check the application notes and the customized protocols, if available, on the datasheet of antibodies for these limitations. What is Cell Permeabilization and Why is it Important in ICC/IF?Under normal conditions, antibody molecules are too large and ionic to pass through the cellular membrane to detect intracellular proteins. Permeabilizing the cells through acetone or methanol fixation, or with the use of a detergent, allows antibodies to pass through the cellular membrane and enter the cell. The most common reagent used for cell permeabilization is non-ionic detergent, Triton X-100. Other milder permeabilizing agents include digitonin or related saponin compounds.
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