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Anti synaptophysin antibody

Manufactured by Agilent Technologies
Sourced in Poland

The Anti-synaptophysin antibody is a laboratory tool used for the detection and localization of the synaptophysin protein in biological samples. Synaptophysin is a protein found in the synaptic vesicles of neurons and is commonly used as a marker for synapses. The antibody can be employed in various techniques, such as immunohistochemistry and Western blotting, to study the distribution and expression of synaptophysin in cells and tissues.

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2 protocols using anti synaptophysin antibody

1

Comprehensive Immunolabelling Protocol for Neuromuscular Junction Analysis

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Immunolabelling was carried out after in situ zymography, as described (Yeghiazaryan et al. 2012 (link)). Goat polyclonal anti-calreticulin, and anti-golgin antibodies were a gift from Dr. Marek Michalak from the University of Alberta (Canada). The anti-calreticulin antibody labels endoplasmic reticulum with high specificity, whereas the anti-golgin antibody detects Golgi structure. To visualize nerves and to analyze their internal architecture, we used antibodies against neurofilament (marker of axons) (Dako, Gdynia, Poland), S100β protein (marker of Schwann cells) (Sigma-Aldrich, Poznan, Poland), or myelin basic protein (MBP, marker of myelin sheath) (Sigma-Aldrich). To label presynaptic structure we used anti-synaptophysin antibody (Dako, Gdynia, Poland). To localize NMJ, the specimens were co-stained with an Alexa 488 or 555 fluorophore-conjugated αBt (Invitrogen/Molecular Probes). To visualize basement membrane, a monoclonal mouse anti-β-dystroglycan was used, 1:10 (Novocastra). The immunoreactions were visualized using species-specific secondary antibodies, coupled with a range of Alexa fluorophores (Alexa 488 or Alexa 555 or Alexa 647, all from Invitrogen/Molecular Probes), diluted 1:200. Nuclei were counterstained with 4,6-diamidino-2-phenylindole (DAPI) or TO-PRO-3 (Invitrogen/Molecular Probes).
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2

Hippocampal Synaptophysin Immunostaining

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Human autopsy hippocampal tissue embedded in paraffin was obtained from St. Louis University Medical Center (St. Louis, MO) and Presbyterian / St. Luke’s Medical Center (Denver, CO). Sections were first deparaffinized and then boiled in 10 mM sodium citrate buffer for 30 min, for antigen retrieval before staining with anti-synaptophysin antibody (DAKO, 1:50).
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