Hippocampal Protein Analysis in Mice

Mice were sacrificed by decapitation and the brain rapidly removed, hippocampi promptly dissected and homogenized as described [25] (link). Proteins were denatured, reduced and separated on 10% Tris-Glycine SDS-PAGE gels (Anamed, Germany). After transfer, nitrocellulose membranes were probed with primary antibodies specific for protein tau and tubulin as described [25] (link) and for CNPase (Millipore - MAB326) as marker for myelin.

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Maurin H., Chong S.A., Kraev I., Davies H., Kremer A., Seymour C.M., Lechat B., Jaworski T., Borghgraef P., Devijver H., Callewaert G., Stewart M.G, & Van Leuven F. (2014). Early Structural and Functional Defects in Synapses and Myelinated Axons in Stratum Lacunosum Moleculare in Two Preclinical Models for Tauopathy. PLoS ONE, 9(2), e87605.

Publication 2014

MAB326

Antibodies Brain Cnpase Decapitation Gels Glycine Hippocampi Membranes Mice Myelin Nitrocellulose Proteins Sds page Tau protein Tris Tubulin

Corresponding Organization :

Other organizations : KU Leuven, The Open University

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Variable analysis

independent variables

Decapitation of mice

dependent variables

Protein tau levels
Tubulin levels
CNPase levels (marker for myelin)

control variables

Hippocampi dissection and homogenization
Protein denaturation, reduction, and separation on 10% Tris-Glycine SDS-PAGE gels
Nitrocellulose membrane probing with primary antibodies specific for protein tau, tubulin, and CNPase

controls

Positive control: Not explicitly mentioned
Negative control: Not explicitly mentioned

Annotations

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