Culturing human Embryonic Stem Cells (hESCs)
Maintain hESCs in Nutristem medium (see Reagents & Equipment) on 0.5 µg/cm2 vitronectin N-precoated tissue culture-treated plastic (e.g. 6 well plates) in a humidified incubator (37°C, 5% CO2). Exchange the culture medium daily to fresh medium, warmed to room temperature. Culture the hESCs for at least two passages post-thawing before refreezing (See Freezing hESCs section for more information). Only maintain hESCs in vitro for up to six passages post-thawing, for efficient gastruloid generation. Culture beyond this passage number can have variable effects. Maintain stocks under antibiotic free conditions to quickly identify any microbial infections.
Note: Both Nutristem and E6 medium should be allowed to warm to room temperature on the benchtop, and not in a 37°C water-bath or incubator as some of the components are heat-sensitive.
Thawing hESCs
hESCs should be stored for long-term use at -150°C in liquid nitrogen cell banks. Before thawing, allow Nutristem media to warm to room temperature, and prepare vitronectin coated wells of a 6-well plate by putting 0.5 µg/cm2 vitronectin in PBS-/- into each well, then leave at room temperature for 1 hour before plating, or for longer periods at 4°C wrapped with parafilm.
1. Prepare enough Nutristem media for plating (3 mL per 3 cm well of a 6-well plate) with 1:1000 ROCK inhibitor. This will be your plating medium.
2. Place 9 mL Nutristem media in a 15 mL falcon tube. This will be your resuspension medium.
3. To thaw, retrieve cryovial(s) and suspend in 37°C water bath, until almost all the vial is in a liquid state (approx. 30 seconds).
4. Drop-wise, apply 1 mL of the prepared resuspension medium to the cryovial.
5. Transfer all liquid from the cryovial to the resuspension medium falcon tube.
6. Centrifuge cells in resuspension medium at 1000 rpm for 5 minutes.
7. Remove supernatant and resuspend cells in plating medium.
8. Remove vitronectin coating from wells, and transfer cell suspension to the new wells.
9. Place in a humidified incubator (37°C, 5% CO2)
10. The next day, replace media with fresh Nutristem (without ROCK inhibitor)
Freezing hESCs
Freezing of hESCs should occur when cells are 70-80% confluent.
1. Prepare 8 mL of room temperature PBS-/- in a 15 mL falcon tube, and 1 mL of room temperature Knockout Serum Replacement with 10% DMSO (KSR+DMSO), per well of a 6-well plate to be frozen.
2. Remove medium from cells, and wash cells with 3 mL PBS-/- per well of a 6-well plate
3. Add 2 mL of room-temperature 0.5 mM EDTA in PBS-/- per well of a 6-well plate
4. Place in the incubator for 4.5 minutes
5. Tap against solid surface or gently pipette to dislodge cells as clusters. Check under a dissection/benchtop microscope that this has occurred before continuing.
6. Transfer cell suspension to prepared falcon tube with PBS-/-.
7. Centrifuge cells at 1000 rpm for 5 minutes.
8. Remove supernatant and resuspend in 1 mL KSR+DMSO.
9. Transfer cell suspension to cryovial and quickly transfer to a Coolcell/’Mr. Frosty’ and to -80°C storage.
10. The next day, transfer cryovial(s) to -140/150°C liquid nitrogen storage
Passaging of hESCs
Note: Passage the hESCs to a new well of a 6-well plate once they reach 70-80% confluence (see Figure 1).
Note: Prewarm all medium to room temperature before use.
1. Prepare vitronectin-coated wells of a 6-well plate by putting 0.5 µg/cm2 vitronectin in PBS-/- into the wells. Leave at room temperature for 1 hour before plating, or for longer periods at 4°C wrapped with parafilm.
2. Wash cells once with 3 mL PBS-/- per well of a 6-well plate.
3. Add 2 mL of room-temperature 0.5 mM EDTA in PBS-/- per well of a 6-well plate.
4. Place in the incubator for 4.5 minutes.
5. Carefully remove EDTA using a suction pump, being careful not to dislodge cells from the surface.
6. Add 2 mL PBS-/- before tapping against a solid surface to dislodge the cells as clusters. Check under a dissection/benchtop microscope that this has occurred before continuing.
Note: It is vital for routine passaging that hESCs are not fully dissociated to single cells but remain as clusters of cells. To do so, minimise any pipetting and ensure exposure of cells to EDTA is just enough to dislodge cells without disrupting clusters.
7. Optional:
a) Collect cells using a P1000 and transfer to a 15 mL falcon tube containing 8 mL PBS-/-.
b) Centrifuge cell suspension at 1000 rpm for 5 minutes, remove supernatant, and resuspend in 1 mL fresh Nutristem.
c) Note: perform this step carefully so as not to disrupt cell clusters.
8. Plate cells in 3 mL of Nutristem per well of a vitronectin-coated 6-well plate, at between 1:4 to 1:20, depending on original cell density and cluster size.
Note: We typically passage our cultures 1:10 every 3-4 days, but ideal conditions may vary and may require optimisation for different cell lines depending on growth rate. Passaging concentration can be assessed by visual examination of cluster size after dislodging with EDTA (Step 3) and from pellet size after centrifugation (Step 7). Aim for fairly sparse, medium-sized clusters covering ~10% of the well.
Generating Human Gastruloids
The successful generation of human gastruloids requires three sequential steps, each of which needs to be carefully monitored: 1) the state of the cells at the start the protocol, 2) the Chiron pre-treatment and 3) aggregate formation.
The first, includes dependency on colony density, size and morphology. In order to achieve this state, cells can be routinely passaged and monitored so that pre-treatment is performed when cells achieve this culture state (Option 1, below). This option is the version used in the associated manuscript (Moris et. al., 2020) and the resulting gastruloids have been extensively characterised. It does not use ROCK inhibitor to alter the state of the cells, and instead utilises passaging as clusters of cells. Alternatively, we have found that cells can be seeded as a single-cell suspension before pre-treatment to standardise this starting state (Option 2, below). In our hands, this can improve reproducibility between experimentalists by providing a standardised culture method, although this requires ROCK inhibition.
Option 1: Routine passaging of hESCs before pre-treatment (~3-5 days before pre-treatment)
1. Dissociate and passage cells as described in the section describing hESC passaging.
2. Closely monitor cells daily to determine the correct timepoint to perform pre-treatment.
Note: Cell density is critical for human gastruloid generation. Cells should be at ~60% confluency on the day of aggregation, so for pre-treatment 24 hours before, cells should be at ~40-50% confluency (see Figure 1). Typically, this state is reached 3-4 days after passaging.
Note: Colony size is critical for human gastruloid generation. Ensure colonies are of medium size (not so large that they are touching each other, and not so small that they do not contain many cells). The optimal diameter of each colony is ~150-300 µm on the day of pre-treatment. See Figure 2.
Note: We have observed that cell morphology at the time of pre-treatment is a critical feature for human gastruloid generation. Cells around the edges of colonies should often appear ‘pointy’ before pre-treatment, and colonies should not yet have defined edges.
Option 2: Single-cell seeding of hESCs before pre-treatment (4 days before pre-treatment)
1. Prepare vitronectin-coated wells of a 6-well plate by putting 0.5 µg/cm2 vitronectin in PBS-/- into the wells. Leave at room temperature for 1 hour before plating, or for longer periods at 4°C wrapped with parafilm.
2. Prepare replating medium, which is Nutristem supplemented with 1:2000 ROCK inhibitor.
Note: While ROCK inhibitor is not used for routine passaging, it is critically important for survival when hESC cells are plated as a single-cell suspension.
3. Wash cells once with 3 mL PBS-/- per well of a 6-well plate.
4. Add 2 mL of room-temperature 0.5 mM EDTA per well of a 6-well plate.
5. Place in the incubator for 4.5 minutes before gently tapping against a solid surface to dislodge the cells.
6. Dissociate the colonies into a single cell suspension with a P1000 micropipette tip by pipetting up-and-down 5-10 times and ejecting the suspension forcefully against the bottom of the well.
7. Collect cells using a P1000 and then transfer to a 15 mL falcon tube with 8 mL PBS-/-.
8. Centrifuge cell suspension at 1000 rpm for 5 minutes.
9. Remove supernatant and fully resuspend in 200-1000 µL of Nutristem depending on pellet size.
10. Check under dissection microscope that the cells are in a single-cell suspension.
11. Count cells using an automated cell counter or haematocytometer.
12. For each well of a 6-well plate, add 60,000 to 80,000 cells to 3 mL of room-temperature replating medium.
Note: The exact cell number to replate depends on cell line and growth speeds. If using a new line, this number should be tested empirically, but in our hands, 60,000 cells per 3 cm well works well with most lines.
13. Remove vitronectin coating from the 6-well plate, and add cell suspension to well
14. Place cells in the incubator. Cells should be left to grow for 4 days (with fresh Nutristem exchange daily) before pre-treatment.
Pre-treatment of hPSCs (24h before aggregation)
1. Prepare Nutristem supplemented with between 3-3.5 µM Chiron, depending on cell line. An ideal concentration in our hands is 3.25 µM, but this is particularly cell line dependent.
Note: With each new cell line, optimise the Chiron concentration by performing titration experiments.
2. Aspirate Nutristem medium from cells and replace with Chiron-supplemented medium.
a. Optional: Maintain one well in Nutristem alone for routine maintenance of the cell line.
Preparation of Gastruloids (0h after aggregation)
Note: Following pre-treatment with Chiron, cell colonies should look less ‘spiky’ at the edges, and more rounded (see Figure 3). If this is not the case, consider titrating Chiron concentration further, or adjusting starting cell attributes like density and colony size.
Note: Dissociation and reaggregation of hPSCs should be done as quickly as possible to minimise the stress caused to the cells. We recommend that any separate samples are performed independently to ensure a quick process, which should ideally be completed in < 30 minutes.
1. Pre-warm EDTA and E6 to room temperature
2. Prepare aggregation medium, by supplementing E6 with 0.5-3 µM Chiron (routinely 0.5 µM Chiron, but titrate for new cell lines) and 1:2000 ROCK inhibitor. For each 96-well plate of aggregates, prepare 5 mL of aggregation medium.
Note: This concentration of ROCK inhibitor is half the concentration used for routinely replating single cells. We have found this to be a sufficient concentration for aggregate formation. With new cell lines, consider titrating this concentration to 1:1000 if aggregation is poor.
3. Aspirate the medium from the 6-well plate and rinse gently with 3 mL PBS-/-.
4. Aspirate the PBS and add 2 mL of pre-warmed 0.5 mM EDTA.
5. Place in the incubator for 4.5 minutes before gently tapping against a solid surface to dislodge the cells.
6. Dissociate the colonies into a single cell suspension with a P1000 micropipette tip by pipetting up-and-down 5-10 times and ejecting the suspension forcefully against the bottom of the well.
Note: A single cell suspension is essential for accurate cell counting. Errors in counting affect the size of the gastruloids, which is known to affect the level of axial elongation in mouse gastruloids (see Baillie-Johnson et. al., 2015). Observe cell suspension under an inverted benchtop microscope to check single cell suspension. Cell suspension can be passed through a filter if necessary.
7. Collect cells using a P1000 and then transfer to a 15 mL falcon tube with 8 mL PBS-/-.
8. Centrifuge cell suspension at 1000 rpm for 5 minutes.
9. Remove supernatant and fully resuspend in 200-1000 µL of E6 depending on pellet size. One well of a 6-well plate at 60-80% confluence should typically be suspended in 200 µL E6.
10. Load the counting slide of an automated cell counter (or equivalent haemocytometer) with 75 µL of cell suspension and determine the density of the suspension.
Note: Accurate counting of cell numbers is necessary to achieve reproducible aggregates between experiments, so automated and highly accurate equipment is strongly recommended.
Note: If your cell counter allows, check that the amount of debris in your suspension is minimal. With our Moxi Orflo cell counter, we aim for a Moxi Population Index (MPI) of > 0.7 (ratio of cell population relative to debris and contaminants).
11. Determine the volume of suspension required to produce a cell concentration of 10-20 cells/µL of aggregation medium.
Note: This cell concentration will determine the number of cells aggregated as gastruloids. In our hands, between 300-800 cells works well, with an optimum of 400 cells, but this is particularly cell line dependent and should be optimised empirically for each new cell line.
12. Add the calculated volume of cell suspension to the required amount of aggregation medium (see Step 2), mix well and transfer to a sterile reservoir.
a. Tip: Inverting the suspension prior to plating or pipetting it up and down within the reservoir can ensure that the cells are well mixed.
13. Pipette 40 µL of plating suspension into each well of a sterile, U-bottomed non-tissue culture-treated 96-well plate with a multichannel micropipette.
a. Tip: Take care to position the droplets in the bottom of each well and not clinging to the walls, as U-shaped droplets are required for efficient aggregation.
14. Confirm that cells can be seen within each well using the inverted benchtop microscope.
15. Centrifuge the plates using a plate centrifuge at 700 rpm for 2 minutes at room temperature.
a. Tip: Wrap the plate in parafilm before centrifugation to prevent accidental lid opening and maintain sterility.
16. Return the plate to the incubator for 24 hours to allow aggregation.
Addition of Medium (24 hours after aggregation)
Note: Adding fresh E6 medium to the aggregates 24 hours after aggregation is necessary to dilute both the Chiron and ROCK inhibitor from the aggregation medium.
17. Pre-warm E6 medium to room temperature.
18. Transfer 150 µL of E6 medium to each well using the multichannel micropipette and a sterile plastic reservoir.
19. Return the plate to the incubator for a further 24 hours.
Exchange of Medium (48 hours after aggregation)
20. Pre-warm E6 medium to room temperature.
21. Carefully remove 150 µL of the medium from each well using the multichannel micropipette, holding it at an angle to aspirate slowly from the side of each well.
a. Tip: Angle the pipette at an acute angle at the beginning of suction, rotating your wrist to become more vertical as suctioning progresses. This will ensure that the tip of your pipette is always at the top of the medium and not likely to accidently disturb/remove the gastruloid (see Figure 4).
22. Add 150 µL of fresh E6 to each well using the multichannel micropipette.
23. Return the plate to the incubator.
24. Repeat steps 20-23 each day for the extent of the protocol.