In Vitro Induction of Neuromuscular Junctions from Engineered Human-Induced Pluripotent Stem Cells
Published: September 27, 2024
Abstract
Source:Lin, C. et al., In vitro Neuromuscular Junction Induced from Human Induced Pluripotent Stem Cells. J. Vis. Exp.(2020).
This experiment details a method for generating neuromuscular junctions from human-induced pluripotent stem cells. It uses a staged differentiation process to promote myotube and motor neuron development and synapse formation, yielding functional neuromuscular junctions.
Protocol
1. Preparation of extracellular matrix (ECM)-coated plates
- Dilute ECM (see Table of Materials) with ice cold 1x PBS to a final concentration of 2%
- Add 1 mL of ECM to 49 mL of 1x PBS in a 50 mL plastic tube. Mix well by pipetting up and down several times.
- Place 1 coverslip into each well of a 6-well plate. Add 1.5 mL of 2% ECM into each well.
- Incubate the well plate with 2% ECM for 2 h at 37 °C.
- Aspirate ECM from the well plate and store the plate at 4 °C before use.
2. Differentiation of iPSCs toward NMJ
- Seed 4 x 105 of iPSCs per well on the 6-well plate prepared in section 1. Make sure to seed the cells on the coverslip pre-deposited in the well.
NOTE: In this study, the 201B7MYOD iPS cell line was used.- Remove the medium from the iPSCs on the 6 cm culture dish and wash the iPSCs once with 1x PBS.
- Add 1 mL of cell detachment solution to the dish and incubate for 10 min at 37 °C.
- Add 3 mL of primate embryonic stem (ES) cell medium to the dish and gently pipette 3 times.
- Collect the supernatant, which contains detached iPSCs, into a 50 mL plastic tube and centrifuge at 160 x g at 4 °C for 5 min.
- Carefully aspirate the supernatant, resuspend the iPSCs in 3 mL primate ES cell medium with 10 µM Y27632, and count the cell number using a hemocytometer.
- Dilute the iPSCs with primate ES cell medium and 10 µM Y27632 to a concentration of 2 x 105 cells/mL. Add 2 mL of iPSCs on the coverslip pre-deposited in the well described in section 1.
3. Induction of the iPSCs to NMJ
- On day 1, 24 h after seeding the iPSCs to the 6-well plate, remove the culture medium and replace it with 2 mL of fresh primate ES cell medium containing 1 µg/mL doxycycline to each well.
- Change the medium with 2 mL of myogenic differentiation medium (MDM) (Table 1) containing 1 µg/mL doxycycline (final concentration) to each well. Refresh the medium every day from day 2 to day 10.
- From day 11, switch the medium to 2 mL of NMJ medium (Table 1) to each well. Refresh the medium every 3‒4 days thereafter until day 30.
- Observe the differentiated NMJ by phase inverted microscopy on day 30. The NMJ can be used for the following analysis.
Representative Results
Table 1: Formula of medium.
| Myogenic differentiation medium (MDM) | MEM-alpha | 500mL |
| 100mM 2-ME | 1117μL | |
| Doxycycline | 1μg/mL | |
| KSR | 56mL (final to 10%) | |
| Pen/Strep | 2.5mL | |
| total | 560mL | |
| 100mM 2-mercaptoethanol | 2-mercaptoethanol | 7μL |
| d.d. water | 993μL | |
| total | 1000μL | |
| NMJ medium | Neurobasal medium (NB) | 500mL |
| B27 | 1x (stock in 50x) | |
| BDNF | 10ng/mL | |
| GDNF | 10ng/mL | |
| N2 | 1x (stock in 100x) | |
| NT3 | 10ng/mL | |
| Pen/Strep | 2.5mL |
Disclosures
The authors have nothing to disclose.
Materials
| Medium, growth factors and reagents | |||
| 2-mercaptoethanol | Nacalai tesque | 21418-42 | |
| B27, Gibco | Gibco | 12587-001 | |
| BDNF | R & D Systems | 248-BD | |
| Cell detachment solution, Accumax | STEMCELL Technologies | #07921 | |
| Critical point dryer | Hitachi | ES-2030 | |
| Doxycycline | Takara | 631311 | |
| ECM, Matrigel (growth factor reduced) | Corning | 356230 | |
| GDNF | R & D Systems | 212-GD | |
| Gelation, IP gel | Geno Staff | PG20-1 | |
| Ions coater | JEOL | JEC3000FC | |
| iPSC medium, mTeSR | STEMCELL Technologies | 85850 | |
| KnockOut SR (KSR) | Gibco | 10828-028 | |
| live cell microscopy | Nikon | Eclipse Ti microscope | |
| MEM-alpha | Gibco | 12571-071 | |
| N2, Gibco | Gibco | 17502-048 | |
| Neurobasal medium | Gibco | 21103-049 | |
| NT3 | R & D Systems | 267-N3 | |
| Primate ES cell medium | ReproCell | RCHEMD001 | |
| SEM | Hitachi | S-4700 | |
| TEM | Hitachi | H7650 | |
| Y27632 | Wako Chemicals GmbH | 253-00513 |
Cite This Article
In Vitro Induction of Neuromuscular Junctions from Engineered Human-Induced Pluripotent Stem Cells. J. Vis. Exp. (Pending Publication), e22582, doi: (2024).