Quicklinks
- Introduction
- Preparing Reagents and Media
- Xeno-Free Differentiation Medium
- Xeno-Free Culture Medium
- Preparing Matrix
- Xeno-Free Culture of Neural Stem Cells
- Culture and Propagation of Neural Stem Cells
- Freezing Neural Stem Cells
- Xeno-Free Differentiation of Neural Stem Cells to Neurons
- Xeno-Free Culture of Neurons
Related Product Information
As the field of neuroscience moves closer to the reality of neural stem cell-derived therapies, the importance of reagent selection early in the development of clinical-grade neural cell lines has become increasingly clear. More specifically, the use of media and supplement combinations that contain xeno-free or only human-origin or recombinant components is critical to safety and traceability of the final product.
Concerns about pathogen cross-transfer from non-human sources or contamination with non-neural cells, which limit the efficiency and specificity of the differentiation protocols, as well as the various challenges faced in maintaining healthy cultures, have lead to the development of xeno-free media systems with optimized conditions for maintaining, differentiating, and expanding neural stem cells (NSCs).
The following protocol is broken in to three parts: Xeno-Free Culture of Neural Stem Cells, Xeno-Free Differentiation of Neural Stem Cells into Neurons, and Xeno-Free Culture of Neurons.
Materials Needed
Cells
- Gibco® Human Neural Stem Cells (H9-Derived) (Cat. no. N7800-100) or an in-house produced cell line
Reagents
- CELLstart™ CTS™ Substrate (Cat. no. 10142-01)
- KnockOut™ DMEM/F12 CTS™ (Cat. no. A13708-01)
- B-27® Supplement XenoFree CTS™ (Cat. no. A14867-01)
- N-2 Supplement CTS™ (Cat. no. A13707-01)
- bFGF, Recombinant Human CTS™ (Cat. no. CTP0261)
- EGF, Recombinant Human (Cat. no. PHG0311)
- GlutaMAX™-I CTS™ Supplement (A12860-01)
- Ascorbic Acid (Sigma, Cat. no. A8960)
- TrypLE™ Select CTS™ Dissociation Enzyme (Cat. no. A12859-01)
- DPBS CTS™ without Calcium Chloride, without Magnesium Chloride (Cat. no. A1285601)
- DPBS CTS™ (with Calcium & Magnesium) (Cat. no. A1285801)
- Human Laminin (Sigma, Cat. no. L6274)
- Neurobasal® Medium CTS™ (Cat. no. A1371201)
- Poly-L-Lysine or Poly-D-Lysine (Sigma, Cat. no. p7280 or p9155)
- Water, distilled (Cat. no. 15230)
Ascorbic Acid Stock Solution
- Resuspend 500 mg of ascorbic acid powder in 8.634 mL of distilled water to make a 200 mM stock solution. Note: The molecular weight of ascorbic acid is 289.54.
- Sterilize the ascorbic acid solution by filtering it through a 0.22-μm filter.
- Aliquot the ascorbic acid solution into sterile tubes and store at –20°C in the dark for up to 6 months.
bFGF and EGF Stock Solutions
- To prepare a 20 μg/mL stock solution of bFGF or EGF, resuspend 10 μg of bFGF or EGF in 500 μL of 0.1% human serum albumin in DPBS CTS™ without Calcium Chloride, without Magnesium Chloride.
- Aliquot the bFGF or EGF stock solution into sterile tubes and store at –20°C in the dark for up to 6 months.
Xeno-Free Proliferation Medium
Complete Xeno-Free Proliferation Medium is used for culturing neural stem cells. It consists of KnockOut™ DMEM-F12 CTS™ medium with GlutaMAX™-I CTS™ supplement, ascorbic acid, bFGF, EGF, N-2 Supplement CTS™, and B-27® Supplement XenoFree CTS™.
1. To prepare 100 mL of complete Xeno-Free Proliferation Medium, aseptically mix the following components:
Component | Final concentration | Amount |
---|---|---|
KnockOut™ DMEM/F12 CTS™ Medium | 1X | 96 mL |
GlutaMAX™-I CTS™ Supplement | 2 mM | 1 mL |
bFGF (prepared as 20 μg/mL stock) | 20 ng/mL | 100 μL |
EGF (prepared as 20 μg/mL stock) | 20 ng/mL | 100 μL |
B-27® Supplement XenoFree CTS™ | 2% | 2 mL |
N-2 Supplement CTS™ | 1% | 1 mL |
Ascorbic acid | 200 μM | 100 μL |
2. Complete Xeno-Free Proliferation Medium can be stored at 2–8°C in the dark for up to 2 weeks.
Xeno-Free Differentiation Medium is used for differentiating neural stem cells into neurons, and it consists of Neurobasal® Medium CTS™ with GlutaMAX™-I CTS™ supplement, ascorbic acid, and B-27® Supplement XenoFree CTS™.
1. To prepare 100 mL of complete Xeno-Free Differentiation Medium, aseptically mix the following components:
Component | Final concentration | Amount |
---|---|---|
Neurobasal® Medium CTS™ | 1X | 97 mL |
GlutaMAX™-I CTS™ Supplement | 2 mM | 1 mL |
B-27® Supplement XenoFree CTS™ | 2% | 2 mL |
Ascorbic acid | 200 μM | 100 μL |
2. Complete Xeno-Free Differentiation Medium can be stored at 2–8°C in the dark for up to 2 weeks.
Complete Xeno-Free Culture Medium is used for culturing neurons, and it consists of Neurobasal® Medium CTS™ with GlutaMAX™-I CTS™ supplement, ascorbic acid, and B-27® Supplement XenoFree CTS™.
1. To prepare 100 mL of complete Xeno-Free Culture Medium, aseptically mix the following components:
Component | Final concentration | Amount |
---|---|---|
Neurobasal® Medium CTS™ | 1X | 97 mL |
GlutaMAX™-I CTS™ Supplement | 2 mM | 1 mL |
B-27® Supplement XenoFree CTS™ | 2% | 2 mL |
Ascorbic acid | 200 μM | 100 μL |
2. Complete Xeno-Free Culture Medium can be stored at 2–8°C in the dark for up to 2 weeks.
Coating Culture Vessels with CELLstart™ CTS™ Substrate
- Dilute CELLstart™ CTS™ substrate 1:100 in DPBS CTS™ (with Calcium & Magnesium) (i.e., 50 μL of substrate into 5 mL of DPBS). Note: CELLstart™ CTS™ substrate should not be frozen, vortex or exposed to vigorous agitation due to potential gel formation.
- Coat the surface of the culture vessel with the working solution of CELLstart™ CTS™ substrate (14 mL for T-75, 7 mL for T-25, 3.5 mL for 60-mm dish, 2 mL for 35-mm dish).
- Incubate the culture vessel at 37°C in a humidified atmosphere of 5% CO2 for 1 hour.
- Remove the vessel from the incubator and store it until use. Remove all CELLstart™ CTS™ substrate solution immediately before use, and fill the vessel with complete Xeno-Free Proliferation Medium. Note: You may coat the plates in advance and store them at 4°C, wrapped tightly with Parafilm® laboratory film, for up to 2 weeks. Do not remove CELLstart™ CTS™ solution until just prior to use. Make sure the plates do not dry out.
Coating Culture Vessels with Human Laminin
- Thaw the laminin slowly at 2–8°C and prepare a 10-μg/mL working solution in sterile, distilled water. Aliquot the working solution into polypropylene tubes, and store the tubes at –20°C until use. Avoid repeated freeze/thaw cycles. Note: Laminin may form a gel if thawed too rapidly.
- Coat the surface of the culture vessel with the laminin working solution (14 mL for T-75, 7 mL for T-25, 3.5 mL for 60-mm dish, 2 mL for 35-mm dish).
- Incubate the culture vessel overnight at 4°C or for 2 hours at 37°C.
- Rinse the culture vessel with DPBS CTS™ without Calcium Chloride, without Magnesium Chloride, and store the vessel covered with DPBS until use. Immediately before use, remove all DPBS and replace it with complete medium. Note: You may coat the plates in advance and store them at 4°C, wrapped tightly with Parafilm® laboratory film, for up to 2 weeks. Do not remove DPBS until just prior to use. Make sure the plates do not dry out. Do not use the laminin-coated plate if discoloration or spider web formations appear on its surface.
Coating Culture Vessels with Poly-L-Lysine or Poly-D-Lysine
- Prepare a 10-μg/mL working solution of Poly-L-Lysine or Poly-D-Lysine in sterile, distilled water.
- Coat the surface of the culture vessel with the working solution of Poly-L-Lysine or Poly-D-Lysine (14 mL for T-75, 7 mL for T-25, 3.5 mL for 60-mm dish, 2 mL for 35-mm dish).
- Incubate the culture vessel at room temperature for 1 hour.
- Aspirate the Poly-L-Lysine or Poly-D-Lysine solution from the coated vessel and rinse the surface of the vessel twice with sterile, distilled water.
Note: Make sure to rinse the culture vessel thoroughly, because excess poly-D-lysine can be toxic to the cells. - Leave the coated vessels uncovered in the laminar hood until they have completely dried. You may use the dry plates immediately or store them at 4°C, wrapped tightly with Parafilm® laboratory film, for up to one week.
Thawing Neural Stem Cells
- Pre-warm 10 mL of complete Xeno-Free Proliferation Medium to 37°C.
- Transfer a vial of frozen NSCs from liquid nitrogen storage to a 37°C water bath. It is important to make the transfer immediately to prevent crystal formation.
- Immerse the vial in the 37°C water bath without submerging the cap to thaw the cells. Swirl the vial gently while thawing.
- When only a small crystal of ice remains, remove the vial from the water bath and sterilize the outside of it with 95% ethanol. Allow the ethanol to evaporate before opening the vial.
- Pipet the thawed cells gently into a sterile 15-mL tube and slowly add pre-warmed complete medium to a total volume of 5 mL. Note: While adding the medium, gently move the tube back and forth to mix the cells. This reduces osmotic shock to the cells.
- Centrifuge the cells at 300 × g for 4 minutes. Aspirate and discard the supernatant.
- Resuspend the cells in 5 mL of pre-warmed complete Xeno-Free Proliferation Medium, and determine the total number of cells and percent viability.
- Inoculate a CELLstart™ CTS™ substrate-coated culture vessel with the thawed cells at a final seeding density of 1 × 105 cells/cm2. Note: Aspirate the coating solution from the culture vessel immediately before using the vessel.
- Incubate the cells at 37°C in a humidified atmosphere (90%) of 5% CO2 in air.
- The next day, replace the spent medium with fresh Xeno-Free Proliferation Medium, and change the medium every other day thereafter.
- Once the culture has reached full confluency, passage the cells at a split ratio of 1:4 or at a seeding density of 1 × 105 cells/cm2. You may also freeze the cells for long-term storage in liquid nitrogen.
Culture and Propagation of Neural Stem Cells
- Prepare a CELLstart™ CTS™ substrate-coated culture vessel and pre-warm the Xeno-Free Proliferation Medium to 37°C.
- Dilute the TrypLE™ Select CTS™ dissociation enzyme to 0.5X in DPBS CTS™ without Calcium Chloride, without Magnesium Chloride.
- Rinse the cells to be passaged once with DPBS CTS™ without Calcium Chloride, without Magnesium Chloride, using approximately 2 mL DPBS per 10 cm2 of culture surface area.
- Add 0.5X TrypLE™ Select CTS™ solution to the cells at approximately 1 mL per 10 cm2 of culture surface area and incubate for 3 minutes at room temperature or in a 37°C incubator. If the culture is dense, increase the incubation time until the cells start to separate and round up.
- Gently rinse the culture vessel by pipetting the TrypLE™ Select CTS™ solution up and down onto the cells to detach them from the vessel. Avoid creating bubbles.
- Collect the cells and transfer to a 15-mL conical tube.
- Stop the cell dissociation reaction by adding complete Xeno-Free Proliferation Medium at 4X the volume of TrypLE™ Select CTS™ solution in the vessel (approximately 4 mL of medium per 10 cm2 of culture surface area). Disperse the medium by pipetting it over the cell layer surface several times.
- Centrifuge the cells at 300 × g for 4 minutes. Aspirate and discard the supernatant.
- Resuspend cells in complete Xeno-Free Proliferation Medium to a final concentration of 1 ×104 cells/μL.
- Inoculate the CELLstart™ CTS™ substrate-coated culture vessel with the thawed cells at a final seeding density of 1 × 105 cells/cm2 and place it in a 37°C incubator with a humidified atmosphere of 5% CO2 in air
- The next day, replace the spent medium with fresh Xeno-Free Proliferation Medium, and change the medium every other day thereafter.
- Prepare 2X freezing solution consisting of 20% DMSO and 80% Xeno-Free Proliferation Medium. Keep the freezing medium on ice until use.
- Harvest the cells as described in Culture and Propagation of Neural Stem Cells, above.
- Resuspend the cells in complete Xeno-Free Proliferation Medium at a concentration of 2 × 106 cells/mL.
- Add the same amount of 2X freezing medium to the resuspended cells as was used for resuspending them in a drop-wise manner. Note: The final concentration of DMSO in 1X freezing medium is 10%, and the final cell concentration is 1 × 106 cells/mL.
- Prepare 1 mL aliquots (1× 106 cells) in cryovials, and place the vials in an isopropanol chamber. Place the isopropanol chamber with the cryovials at –80°C overnight.
- The next day, transfer the frozen cryovials to a liquid nitrogen tank (vapor phase) for long-term storage.
Note: You may check the viability and recovery of frozen cells 24 hours after storing cryovials in liquid nitrogen by following the procedure outlined in Thawing Neural Stem Cells, above.
Figure 1 Culture kinetics of neural stem cells in Xeno-Free Proliferation Medium prepared with B-27® Supplement XenoFree CTS™. After 10 days, the initial culture seeded with 0.5 × 106 cells produced 4.0 × 107 cells.
Figure 2 NSC proliferated (p3, upper left) using B-27® Supplement XenoFree CTS™ were characterized with NSC phenotype marker Sox1 (upper right, green) and Nestin (lower left, green), and further differentiated to neurons (lower right, red).
- Prepare a laminin-coated culture vessel and pre-warm the Xeno-Free Differentiation Medium to 37°C.
- Dilute the TrypLE™ Select CTS™ dissociation enzyme to 0.5X in DPBS CTS™ without Calcium Chloride, without Magnesium Chloride.
- Rinse the neural stem cells once with DPBS CTS™ without Calcium Chloride, without Magnesium Chloride, using approximately 2 mL DPBS per 10 cm2 of culture surface area.
- Add 0.5X TrypLE™ Select CTS™ solution to the cells at approximately 1 mL per 10 cm2 of culture surface area and incubate for 3 minutes at room temperature or in a 37°C incubator. If the culture is dense, increase the incubation time until the cells start to separate and round up.
- Gently rinse the culture vessel by pipetting the TrypLE™ Select CTS™ solution up and down onto the cells to detach them from the vessel. Avoid creating bubbles.
- Collect the cells and transfer to a 15-mL conical tube.
- Stop the cell dissociation reaction by adding complete Xeno-Free Proliferation Medium at 4X the volume of TrypLE™ Select CTS™ solution in the vessel (approximately 4 mL of medium per 10 cm2 of culture surface area). Disperse the medium by pipetting it over the cell layer surface several times.
- Centrifuge the cells at 300 × g for 4 minutes. Aspirate and discard the supernatant.
- Aspirate the laminin solution from the laminin-coated culture vessel and immediately add an appropriate amount of Xeno-Free Differentiation Medium to prevent the culture vessel from drying.
- Inoculate the laminin-coated culture vessel with the neural stem cells at a final seeding density of 1 × 105 cells/cm2 and place it in a 37°C incubator with a humidified atmosphere of 5% CO2 in air
- The next day, change the medium to fresh Xeno-Free Differentiation Medium, and replace half of the medium with fresh Xeno-Free Differentiation Medium every 2–3 days thereafter.
Figure 3 Human NSCs were differentiated for 7 days. Neurite extension was observed (left, phase-contrast image; scale bar = 200 μm) and up-regulation in the expression of neurofilament was examined by qPCR (right; expression was normalized by beta-actin).
Figure 4 Human induced pluripotent stem cells were differentiated into NSCs using B-27® Supplement XenoFree CTS™, and the derived NSCs were further differentiated in complete XenoFree Differentiation Medium (containing Neurobasal® Medium CTS™ and B-27® Supplement XenoFree CTS™) into neurons. Phase-contrast image of derived NSCs (left), phenotype marker expression of derived NSCs (middle; red = Sox1, green = Nestin), and NSCs differentiated into neurons for 2 weeks, whose neurites were stained (right; beta III tubulin = green)
- Pre-warm 10 mL of complete Xeno-Free Culture Medium to 37°C.
- Rinse the Poly-L-Lysine- or Poly-D-Lysine-coated culture vessel with sterile, distilled water twice, and add an appropriate volume of pre-warmed complete Xeno-Free Culture Medium.
- Inoculate the Poly-L-Lysine- or Poly-D-Lysine-coated culture vessel with the cells at a final seeding density of 2 × 104–5 × 104 cells/cm2 and incubate at 37°C overnight.
- The next day, change the medium to fresh Xeno-Free Culture Medium, and replace half of the medium with fresh Xeno-Free Culture Medium every 2–3 days thereafter.
Figure 5 Culture of human hippocampal neurons, cortical neurons, and Gibco® Episomal iPSC-derived neurons (right). After the hippocampal neurons (left) and cortical neurons (middle) were cultured for a week, live cells were stained with Calcein AM (green) and neurons were stained with Dcx (red). After Gibco® Episomal iPSC-derived neurons (right) were cultured for a week, the cells were stained with Dcx (green) and the nuclei were counterstained with DAPI (blue).
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LT175 rev. 02-21-2013