Antigen Retrieval in Prion Protein Immunohistochemistry

Author:

Everbroeck Bart Van1,Pals Philippe12,Martin Jean-Jacques13,Cras Patrick13

Affiliation:

1. Department of Neurobiology, Born Bunge Foundation, Antwerp University, Wilrijk, Belgium

2. Department of Molecular Genetics, Born Bunge Foundation, Antwerp University, Wilrijk, Belgium

3. Department of Neuropathology, Born Bunge Foundation, Antwerp University, Wilrijk, Belgium

Abstract

Transmissible spongiform encephalopathies are a group of neurodegenerative diseases occurring in both humans and animals and are most likely caused by prions. Neuropathological confirmation of the clinical diagnosis has been a problem because of the difficulty in epitope retrieval from formalin-fixed, paraffin-embedded brain specimens. Many different protocols for the detection of prions in brain tissue have been used. Thus far, picric and/or formic acid, steam autoclaving at 121C of sections, microwave treatment, and 4 M guanidine thiocyanate treatment have been suggested. The objective of our experiment was to obtain the standard pretreatment(s) resulting in optimal immunostaining. In the experiment, successive tissue slides of brain specimens of several Creutzfeldt-Jakob disease and control patients were stained using different combinations of pretreatments. Using densitometric analysis, several well-defined locations per section were examined and prion immunostaining was quantified. The results showed that autoclaving is necessary for antigen retrieval and cannot be substituted by microwave treatment. The best results were obtained when the following combination was used in the specified order: 15 min saturated picric acid, 10 min steam autoclaving at 121C, 5 min 88% formic acid, and 2 hr 4 M guanidine thiocyanate at 4C.

Publisher

SAGE Publications

Subject

Histology,Anatomy

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