Nov 11, 2022
CALCIUM STAINING PROTOCOL
- Machlusil Husna1,
- Kusworini Handono2,
- Hidayat Sujuti3,
- Aulanni'am4,
- Ettie Rukmigarsari5
- 1Department of Neurology Faculty of Medicine, Universitas Brawijaya / dr. Saiful Anwar General Hospital, Malang, Indonesia;
- 2Department of Clinical Pathology Faculty of Medicine, Universitas Brawijaya / dr. Saiful Anwar General Hospital, Malang, Indonesia;
- 3Department of Ophthalmology Faculty of Medicine, Universitas Brawijaya / dr. Saiful Anwar General Hospital, Malang, Indonesia;
- 4Department of Chemistry, Faculty of Science Universitas Brawijaya, Malang, Indonesia;
- 5Faculty of Teacher Training and Education, Islamic University of Malang, Indonesia
Protocol Citation: Machlusil Husna, Kusworini Handono, Hidayat Sujuti, Aulanni'am, Ettie Rukmigarsari 2022. CALCIUM STAINING PROTOCOL. protocols.io https://dx.doi.org/10.17504/protocols.io.kxygx9zewg8j/v1
License: This is an open access protocol distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited
Protocol status: Working
We use this protocol and it's working
Created: October 18, 2022
Last Modified: November 11, 2022
Protocol Integer ID: 71480
Abstract
Neurodegeneration due to neurotoxicity is one of the phenomena in temporal lobe epilepsy. Experimentally, hippocampal excitotoxicity process can occur due to kainic acid exposure, especially in the CA3 area. Neuronal death, astrocyte reactivity and increased calcium also occur in hippocampal excitotoxicity, but few studies have investigated immediate effect after kainic acid exposure. The organotypic hippocampal slice culture (OHSC) is a useful model for studying the neurodegeneration process, but there are still many protocol differences. In this study, minor modifications were made in the OHSC protocol.
Calcium assay kit
Calcium assay kit
We use Fluo-4 assay kit (calcium ab 228555) that provides a homogenous fluorescense-based assay for detecting the intracellular calcium mobilization
Material supplied in kit
Material supplied in kit
Fluo-4 AM 1 vial
10x F127 Plus 1 bottle (10 mL)
HHBS (Hank's Buffer with 20 mM Hepes) 1 bottle (100 mL)
Reagent Preparation
Reagent Preparation
Briefly centrifuge small vials at low speed prior to opening
Thaw all the kit components at room temperature before use
Fluo-4 AM stock solution : add 200 μL of DMSO into the vial of Fluo-4 AM and mix well
1x Assay buffer : make 1x assay buffer by adding 1 mL of 10x F127 plus into 9 mL of HHBS buffer and mix them well
Fluo-4 AM dye-loading solution : add 20 μL of Fluo-4 AM stock solution into 10 mL of 1x assay buffer and mix them well. This working solution is stable for at least 2 hours at room temperature
Assay procedure
Assay procedure
Equilibrate all materials and prepared reagents to room temperature just prior to use and gently agitate
Add 20 μL Fluo-4 AM dye-loading solution into the cell plate
Incubate the dye-loading plate in incubator with temperature 37oC fo 1 h
Prepare the plate with HHBS
Run the calcium flux assay by monitoring the fluorescense intensity at Ex/Em = 490/525 nm with CLSM