NeuroXVivo Rat Cortical Neuron Culture Kit
R&D Systems, part of Bio-Techne | Catalog # CDK011
Key Product Details
Assay Procedure
Refer to the product datasheet for complete product details.
Briefly, primary rat cortical neurons are maintained and matured ex vivo with the NeuroXVivo™ Rat Cortical Neuron Culture Kit using the following procedure:
- Dissect prenatal or neonatal rat cortical tissue
- Dissociate rat cortical tissue
- Suspend single cells in Complete Cortical Neuron Culture Media
- Plate cells onto coated plates
- Exchange media every 3-4 days
Reagents provided in the NeuroXVivo™ Rat Cortical Neuron Culture Kit (Catalog # CDK011)
- Neuronal Base Media (500 mL)
- N21-MAX Media Supplement (50X)
- Recombinant Human BDNF
- Recombinant Human IGF-I
- Reconstitution Buffer 1
Reagents
- E17–E18 Timed Pregnant Rat or P1-P2 Rat Pups
- Poly-D-Lysine (R&D Systems®, Catalog # 3439-100-01)
- Poly-L-Lysine –coated µ-slides
- Mouse Laminin-I (R&D Systems®, Catalog # 3400-010-01)
- L-Glutamine
- Antibiotic-Antimycotic (100X)
- Phosphate Buffered Saline (PBS)
- Sterile deionized or distilled water (dH2O)
- Papain
- DNAse-I
- Ovomucoid Protease Inhibitor
- Earle’s Balanced Salt Solution
Materials
- Parafilm
- Fire-polished glass pasteur pipette
- Tissue culture plates
- Conical tubes
- Pipettes and pipette tips
Equipment
- 37 °C, 5% CO2 humidified incubator
- Laminar flow cell culture hood
- Centrifuge
- Hemocytometer
- 37 °C water bath
- Microscope
Neuronal Base Media - Thaw at 37 °C.
N21-MAX Supplement (50X) - Thaw at 2-8 °C.
Recombinant Human BDNF (1000X) - Add 560 µL of Reconstitution Buffer 1 to the vial of Recombinant Human BDNF to produce Recombinant Human BDNF (1000X).
Recombinant Human IGF-I (1000X) - Add 600 µL of Reconstitution Buffer 1 to the vial of Recombinant Human IGF-I to produce Recombinant Human IGF-I (1000X).
Complete Cortical Neuron Culture Media - Add N21-MAX Supplement (50X) at a final concentration of 1X to the desired amount of Neuronal Base Media (e.g., for every 100 mL of base media, add 2 mL of N21-MAX Supplement (50X)). Add Recombinant Human BDNF (1000X) and Recombinant Human IGF-I (1000X) at a final concentration of 1X to the desired amount of Neuronal Base Media (e.g., for every 100 mL of base media, add 100 µL each of Recombinant Human BDNF (1000X) and Recombinant Human IGF-I (1000X)). Supplement media with 0.5 mM L-Glutamine and Antibiotic-Antimycotic (1X).
Note: Complete Cortical Neuron Culture Media is stable for up to 1 month at 2-8 °C after adding all the growth supplements.
Please refer to the product datasheet for complete protocol details.
Note: Optimal culture conditions for each stem cell line must be determined by the investigator.
Day 1 Prepare tissue culture plates by coating with Poly-D-Lysine and Laminin-I.
Day 2 Isolate cortical tissue from E16-18 rat embryos or P1-2 pups following the dissection protocol outline.
Digest cortical tissue with Papain and DNase-1 for 20-30 minutes.*
*Only if using brains from postnatal rats.
Collect tissues in a conical tube containing Neuronal Base Media and dissociate into a single-cell suspension using a fire-polished pasteur pipette.
Pellet the cells by centrifugation at 200 x g. Suspend cells in Neuronal Base Media and pellet cells. Repeat a total of two times.
Suspend cell pellet in Complete Cortical Neuron Culture Media. Perform a cell count.
Verify desired amount of cells per milliliter in Complete Cortical Neuron Culture Media.
Seed cells onto Poly-D-Lysine/ Laminin-I coated tissue culture plates or µ-slides.
Culture cortical neurons for desired amount of time. Exchange media every 3-4 days.
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