In this video, we demonstrate an assay that investigates monoamine release mechanisms from the neurons of metabolically active ex vivo rat brain slices, when treated with test drugs. The assay demonstrates that neurostimulant drugs induce monoamine release via the cellular monoamine transporters, whereas high KCl concentration induces synaptic vesicle exocytosis-mediated vesicular monoamine release.
Protocol
All procedures involving animal models have been reviewed by the local institutional animal care committee and the JoVE veterinary review board. 1. Ex-vivo endogenous monoamine release from brain slices or punches NOTE: The device used for this section consists of a 48-well plate and a tissue holder made of six microcentrifuge filter units without the inset filters connected to a carbogen line (Figure 1). To make the holder, use a stu…
Representative Results
Figure 1: Experimental setup for efflux experiment. (A) The efflux chamber consists of a 48-well tissue culture plate and a tissue holder tray connected to the carbogen line. (B) A diagram showing the experimental design for the endogenous monoamine efflux experiment in which the tissue activation (B1), pre-incubation with/without monoamine transporter inhibitors…
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The authors have nothing to disclose.
Materials
48-well plate
NA
NA
Assay
Calcium Chloride Anhydrous
Sigma Aldrich
C1016
Modified Artifical Cerebrospinal Fluid OR Efflux Buffer
D-(+)-Glucose
Sigma
1002608421
Dissection Buffer
L-Ascorbic Acid
Sigma Aldrich
A5960
Dissection Buffer
Magnesium Sulfate
Sigma
7487-88-9
KH Buffer
Microcentrifuge Filter Units UltraFree
Millipore
C7554
Assay – 6 to fit in 48-well plate
Pargyline Clorohydrate
Sigma Aldrich
P8013
Modified Artifical Cerebrospinal Fluid OR Efflux Buffer