| Literature DB >> 17852085 |
Abstract
Three fixation issues related to immunostaining are discussed here: 1) Generally, a tissue block is fixed, then embedded and sectioned (pre-fixation). The type of fixative applied, crosslinking or coagulating, has an impact on selecting an epitope retrieval method. Individual antigens have a fixation-retrieval characteristic. 2) A long fixation time, especially with crosslinking fixatives, may compromise the result of immunostaining. This negative effect varies among different antigens and can be partially restored by applying a more sensitive/efficient detection system such as tyramide amplification. 3) Sections cut from a fresh frozen tissue block usually are acetone fixed(post-fixation). This was accepted as the "gold standard" for a long time. Post-fixation, however,may have serious consequences for preservation of small peptides leaking from the cut open cells,whereas this is not the case with pre-fixed intact cells. Consequently, the concept of an acetone post-fixed cryostat tissue section as "gold standard" no longer exists and a more appropriate use of the terms immunohistochemistry and immunocytochemistry therefore seems justified. For many antibodies, it is not known whether a formalin fixed, paraffin embedded tissue specimen is appropriate. Suggestions are made for creating a positive control cell block for testing such antibodies.Entities:
Mesh:
Substances:
Year: 2007 PMID: 17852085 DOI: 10.1080/10520290701375302
Source DB: PubMed Journal: Biotech Histochem ISSN: 1052-0295 Impact factor: 1.718