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Introduction
Rat neural stem cells (NSCs) serve as a well-established model for investigating human brain development, disease processes, and treatment strategies for debilitating central nervous system (CNS) disorders. This protocol describes the in vitro expansion, passaging, and morphology of rat fetal NSCs in adherent or neurosphere suspension cultures.
Required Materials
Cells
Media and Reagents
Special Tools
TOPRequired Materials
Cells
- GIBCO® Rat Fetal Neural Stem Cells (Cat. no. N7744-100) or homogenous cell preparation from 14−18 days post-coitum rat brain tissue
Media and Reagents
- Dulbecco’s Phosphate-Buffered Saline (D-PBS) (Cat. no. 14040)
- Dulbecco’s Phosphate-Buffered Saline (D-PBS) without calcium or magnesium (Cat. no. 14190)
- StemPro® NSC SFM (Cat. no. A10509-01)
- StemPro® Accutase® Cell Dissociation Reagent (Cat. no. A11105-01)
- CELLstart™ CTS™ (Cat. no. A10142-01)
- Trypan blue (Cat. no. 15250) (included with the Countess®) or the LIVE/DEAD® Cell
- Vitality Assay Kit (Cat. no. L34951)
Special Tools
- Countess® Automated Cell Counter (Cat. no. C10227) or hemacytometer
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Preparing Media
Medium for Expanding Neural Stem Cells
StemPro® NSC SFM complete medium consists of KnockOut™ D-MEM/F-12 with StemPro® Neural Supplement, bFGF, EGF, and GlutaMAX™-I. Complete medium is stable for 4 weeks when stored in the dark at 2-8°C.
To prepare 100 mL of complete medium:
You may observe a white precipitate when thawing StemPro® Neural Supplement; this precipitate will disappear when the supplement is completely thawed or dissolved.
StemPro® NSC SFM complete medium consists of KnockOut™ D-MEM/F-12 with StemPro® Neural Supplement, bFGF, EGF, and GlutaMAX™-I. Complete medium is stable for 4 weeks when stored in the dark at 2-8°C.
To prepare 100 mL of complete medium:
- Reconstitute bFGF and EGF with 0.1% BSA solution (in KnockOut™ D-MEM/F-12) at a concentration of 100 μg/mL. You will need 20 μL of each per 100 mL of complete medium. Freeze unused portions in aliquots.
- Mix the following components under aseptic conditions. For larger volumes, increase the component amounts proportionally.
| Component | Final concentration | Amount |
|---|---|---|
| KnockOut™ D-MEM/F-12 | 1X | 97 mL |
| GlutaMAX™-I Supplement | 2 mM | 1 mL |
| bFGF (prepared as 100 μg/mL stock) | 20 ng/mL | 20 μL |
| EGF (prepared as 100 μg/mL stock) | 20 ng/mL | 20 μL |
| StemPro® Neural Supplement | 2% | 2 mL |
You may observe a white precipitate when thawing StemPro® Neural Supplement; this precipitate will disappear when the supplement is completely thawed or dissolved.
Coating Culture Vessels with CELLstart™
For adherent cultures, prepare plates with CELLstart™ CTS™ as described below.
Note: You may coat the plates in advance and store them at 4°C, wrapped tightly with Parafilm, for up to 2 weeks. Do not remove CELLstart™ CTS™ solution until just prior to using the coated plates. Make sure the plates do not dry out.
- Dilute CELLstart™ CTS™ 1:100 in D-PBS with calcium and magnesium (e.g., 50 μL of CELLstart™ CTS™ into 5 mL of D-PBS). Note: CELLstart™ CTS™ should not be frozen, vortexed, or exposed to vigorous agitation due to potential gel formation.
- Coat the surface of the culture vessel with the working solution of CELLstart™ CTS™ (14 mL for a T-75 flask, 7 mL for a T-25 flask, 3.5 mL for a 60-mm dish, 2 mL for a 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 at 4°C until use. Remove all CELLstart™ CTS™ solution immediately before use, and fill the vessel with complete StemPro® NSC SFM.
Note: You may coat the plates in advance and store them at 4°C, wrapped tightly with Parafilm, for up to 2 weeks. Do not remove CELLstart™ CTS™ solution until just prior to using the coated plates. Make sure the plates do not dry out.
Expanding and Passaging of Rat NSCs
Adherent Cultures
- Resuspend the rat fetal NSCs as follows:
- For freshly prepared rat fetal NSCs, after rinsing with D-PBS, resuspend in warmed complete StemPro® NSC SFM at a density of 1 × 107 viable cells/mL.
- For thawed rat fetal NSCs, after determining the viable cell count, resuspend in warmed complete StemPro® NSC SFM at a cell density of 1 × 107 viable cells/mL.
- Plate rat fetal NSCs onto CELLstart™ CTS™-coated culture vessels at a density of 5 × 104 cells/cm2. See the following table for recommended seeding densities for common culture vessels.
Vessel size Growth area Volume of media No. of cells 96-well plate 0.32 cm2/well 0.1 mL 1.6 × 104 24-well plate 1.9 cm2/well 0.5 mL 1.0 × 105 12-well plate 3.8 cm2/well 1 mL 1.9 × 105 35-mm dish 8 cm2/well 2 mL 4.0 × 105 6-well plate 9.6 cm2/well 2 mL 4.8 × 105 60-mm dish 19.5 cm2 5 mL 9.8 × 105 T-25 flask 25 cm2 5 mL 1.3 × 106 100-mm dish 55 cm2 10 mL 2.8 × 106 T-75 flask 75 cm2 15 mL 3.8 × 106 - Add the appropriate volume of cells to each culture vessel and incubate at 37°C, 5% CO2 and 90% humidity.
- Re-feed the rat fetal NSC cultures every 2−3 days with fresh complete StemPro® NSC SFM. The morphology of rat fetal NSCs should exhibit short stellate-like processes with uniform density (see Figure 1 below).
Figure 1. Rat fetal NSCs at passage 3 in adherent culture using StemPro® NSC SFM.
- When cells reach 75–90% confluency (3–4 days after seeding), the rat fetal NSC cultures are ready to be passaged.
- Rinse the culture vessel once with D-PBS without calcium and magnesium, then remove the medium.
- Add pre-warmed StemPro® Accutase® and let the cells detach from the culture surface (within approximately 30 seconds).
- After detachment, gently pipet the cells up and down to break the clumps into a uniform cell suspension and add four volumes of complete StemPro® NSC SFM to the culture vessel.
- Disperse the cells by pipetting over the culture surface several times to generate a homogenous cell solution.
- Transfer the cells to a sterile centrifuge tube and centrifuge at 300 × g for 4 minutes at room temperature. Aspirate and discard the medium.
- Resuspend the cell pellet in a minimal volume of pre-warmed complete StemPro® NSC SFM and remove a sample for counting.
- Determine the total number of cells and percent viability using trypan blue stain or the LIVE/DEAD® Cell Vitality Assay Kit.
- Add enough complete StemPro® NSC SFM to tube for a final cell solution of 1 × 106 viable cells/mL. Incubate at 37°C, 5% CO2 and 90% humidity. Rat fetal NSC cultures should not be maintained for more than 3 passages.
Important: If you are re-feeding rat fetal NSC in a growth medium other than complete StemPro® NSC SFM, ensure that the medium is supplemented with 10 ng/mL bFGF to maintain the undifferentiated state of the rat fetal NSCs.
Neurosphere Suspension Cultures
- Resuspend the rat fetal NSCs as follows:
- For freshly prepared rat fetal NSCs, after rinsing with D-PBS, resuspend in warmed complete StemPro® NSC SFM at a cell density of 1 × 107 viable cells/mL.
- For thawed rat fetal NSCs, after determining the viable cell count, resuspend in warmed complete StemPro® NSC SFM at a cell density of 1 × 107 viable cells/mL.
- Plate the rat fetal NSCs onto uncoated or low-attachment culture vessels at a density of 2 × 105 viable cells/cm2. See the table below for recommended seeding densities.
Vessel size Growth area Volume of media No. of cells 96-well plate 0.32 cm2/well 0.1 mL 6.4 × 104 24-well plate 1.9 cm2/well 0.5 mL
3.8 × 10512-well plate 3.8 cm2/well 1 mL 7.6 × 105 35-mm dish 8 cm2/well 2 mL 1.6 × 106 6-well plate 9.6 cm2/well 2 mL 1.9 × 106 60-mm dish 19.5 cm2 5 mL 3.9 × 106 T-25 flask 25 cm2 5 mL 5.0 × 106 100-mm dish 55 cm2 10 mL 1.1 × 107 - Add the appropriate volume of cells to each culture vessel and incubate at 37°C, 5% CO2 and 90% humidity.
- Carefully re-feed the neurosphere suspension of rat fetal NSCs every 2−3 days with fresh complete StemPro® NSC SFM without removing any developing neurospheres. The morphology of the neurospheres should exhibit spherical and transparent multicellular complexes (see Figure 2).
Figure 2 Rat fetal NSCs at passage 3 in neurosphere culture using StemPro® NSC SFM.
- When the neurospheres reach a diameter of 3.5 mm or larger, the rat fetal NSCs are ready to be passaged.
- Transfer the neurosphere suspension into a sterile centrifuge tube and let the neurospheres settle by gravity or centrifuge at 200 × g for 2 minutes. Aspirate the supernatant carefully to leave the neurospheres in a minimal volume of medium.
- Rinse the neurospheres once with D-PBS without calcium and magnesium and leave a minimal volume of D-PBS.
- Add 1 mL of pre-warmed StemPro® Accutase® to the neurospheres and incubate for 10 minutes at room temperature.
- After incubation, gently pipette the cells up and down to get a single-cell suspension and add 4 mL of complete StemPro® NSC SFM to the tube.
- Centrifuge at 300 × g for 4 minutes at room temperature, carefully aspirate the supernatant, resuspend in a minimal volume of pre-warmed complete StemPro® NSC SFM, and remove a sample for counting on a hemacytometer or Countess® Automated Cell Counter.
- Determine the total number of cells and percent viability.
- Add enough complete StemPro® NSC SFM to the tube for a final cell solution of 1 × 107 viable cells/mL. Incubate at 37°C, 5% CO2 and 90% humidity. Neurosphere suspension cultures should not be maintained for more than 3 passages.
Important: If you are re-feeding rat fetal NSCs in a growth medium other than complete StemPro® NSC SFM, ensure that the medium is supplemented with 10 ng/mL bFGF to maintain the undifferentiated state of the rat fetal NSCs.
LT149 17-Mar-2011
