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Optimized Protocol for Amyloid-β Extraction from the Brain

Article type: Short Communication

Authors: Izco, Maríaa | Pesini, Pedroa; b; * | Pérez-Grijalba, Virginiaa | Fandos, Noeliab | Sarasa, Manuela; b

Affiliations: [a] Araclon Biotech, Proteomic Laboratory, CIBIR, Logroño, Spain | [b] Araclon Biotech, R & D Laboratory, Zaragoza, Spain

Correspondence: [*] Correspondence to: Pedro Pesini, Araclon Biotech (Clínica Montecanal), Franz Schubert 2, 3rd floor, 50012 Zaragoza, Spain. Tel.: +34 876 241 666; Fax: +34 976 020 011; E-mail: [email protected].

Keywords: Alzheimer's disease, amyloid-β peptides, animal models, ELISA, tissue extraction, tissue homogenization

DOI: 10.3233/JAD-121798

Journal: Journal of Alzheimer's Disease, vol. 34, no. 4, pp. 835-839, 2013

Accepted 18 December 2012
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Published: 20 March 2013
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Abstract

Brain levels of amyloid-β (Aβ) are frequently assessed in transgenic mice models of Alzheimer's disease. The procedure involves tissue sample homogenization using different buffers in a sequential process. No attempt has been made to assess if these procedures are able to extract the total amount of Aβ present in the samples. Here we present data suggesting that standard protocols can lead to a dramatic underestimation of the Aβ content. Results show that higher extraction buffer volumes and at least two repetitions of the soluble and membrane-bound extraction steps are necessary for a more accurate estimation of the Aβ content in brain tissues.

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