Antigen masking in routinely processed tissue is a poorly understood process caused by multiple factors. We sought to dissect the effect on antigenicity of each step of processing by using frozen sections as proxies of the whole tissue. An equivalent extent of antigen masking occurs across variable fixation times at room temperature. Most antigens benefit from longer fixation times (>24 hr) for optimal detection after antigen retrieval (AR; for example, Ki-67, bcl-2, ER). The transfer to a graded alcohol series results in an enhanced staining effect, reproduced by treating the sections with detergents, possibly because of a better access of the polymeric immunohistochemical detection system to tissue structures. A second round of masking occurs upon entering the clearing agent, mostly at the paraffin embedding step. This may depend on the non-freezable water removal. AR fully reverses the masking due both to the fixation time and the paraffin embedding. AR itself destroys some epitopes which do not survive routine processing. Processed frozen sections are a tool to investigate fixation and processing requirements for antigens in routine specimens.

Scalia, C., Boi, G., Bolognesi, M., Riva, L., Manzoni, M., Desmedt, L., et al. (2017). Antigen Masking During Fixation and Embedding, Dissected. JOURNAL OF HISTOCHEMISTRY & CYTOCHEMISTRY, 65(1), 5-20 [10.1369/0022155416673995].

Antigen Masking During Fixation and Embedding, Dissected

SCALIA, CARLA ROSSANA
Primo
;
BOI, GIOVANNA MARIA
Secondo
;
BOLOGNESI, MADDALENA MARIA;Bosisio, F;LEONE, BIAGIO EUGENIO
Penultimo
;
CATTORETTI, GIORGIO
Ultimo
2017

Abstract

Antigen masking in routinely processed tissue is a poorly understood process caused by multiple factors. We sought to dissect the effect on antigenicity of each step of processing by using frozen sections as proxies of the whole tissue. An equivalent extent of antigen masking occurs across variable fixation times at room temperature. Most antigens benefit from longer fixation times (>24 hr) for optimal detection after antigen retrieval (AR; for example, Ki-67, bcl-2, ER). The transfer to a graded alcohol series results in an enhanced staining effect, reproduced by treating the sections with detergents, possibly because of a better access of the polymeric immunohistochemical detection system to tissue structures. A second round of masking occurs upon entering the clearing agent, mostly at the paraffin embedding step. This may depend on the non-freezable water removal. AR fully reverses the masking due both to the fixation time and the paraffin embedding. AR itself destroys some epitopes which do not survive routine processing. Processed frozen sections are a tool to investigate fixation and processing requirements for antigens in routine specimens.
Articolo in rivista - Articolo scientifico
antigen retrieval; FFPE; fixation; formalin; immunostaining; Antigens; Epitopes; Fluorescent Antibody Technique; Frozen Sections; Humans; Paraffin Embedding; Staining and Labeling; Tissue Fixation; Anatomy; Histology
English
2017
65
1
5
20
partially_open
Scalia, C., Boi, G., Bolognesi, M., Riva, L., Manzoni, M., Desmedt, L., et al. (2017). Antigen Masking During Fixation and Embedding, Dissected. JOURNAL OF HISTOCHEMISTRY & CYTOCHEMISTRY, 65(1), 5-20 [10.1369/0022155416673995].
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Utilizza questo identificativo per citare o creare un link a questo documento: https://hdl.handle.net/10281/163025
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