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HomeStem Cell CultureMouse Embryonic Stem Cell Culture Procedures & Protocols

Mouse Embryonic Stem Cell Culture Procedures & Protocols

Introduction

The development of transgenic and gene knockout technology has provided an effective tool for the analysis of gene function. Critical to this has been the ability to isolate and culture murine embryonic stem (ES) cells in vitro. Derived from the inner cell mass of early mouse embryos, ES cells contribute to all tissues including germline tissue. Efficient procedures for the in vitro culture and maintenance of mouse pluripotent ES cells have been crucial to the success of gene targeting experiments. We offer a wide range of mouse ES qualified products providing researchers with convenient and cost effective solutions for the reliable culture of mouse ES cells including ESGRO mLIF supplement, primary mouse embryonic fibroblasts, mouse ES cell lines, stem cell screened FBS and proprietary serum-free media.

The cell culture protocol described here includes the in vitro culture of mouse ES cells in serum-containing media using mouse embryonic fibroblasts and ESGRO mLIF. It should be noted that the protocols included in this manual are intended to serve as a guide only, and optimization of culture protocols is encouraged to ensure success.

Experimental Outline for Targeting ES Cells –Step by Step

Plan out a flow chart from day 1 to day 16–19. Note, depending upon the growth of the ES cells, the days may have to be shifted. Electroporation, screening, picking and preparation of DNA will take 2–3 weeks, including weekends.

Day No.ApplicationSection No.
0Prepare culture plates for plating.III
1Prepare PMEF Feeder cell plates for ES cell expansion Et electroporation, if applicable.IV.
2Check PMEF Feeder cell plates, and thaw ES cells.V., XII.
3Feed ES cells; passage if required.V., XII.
4Feed ES cells; passage if required. Prepare Targeting Vector: Linearize ..-100 pg of targeting vector (each electroporation requires 15-30 pg of linearized vector), and precipitate with EtOH (no need to phenolize).V., XII.
5Electroporation of ES cells.VI., XIII.
6-10Select for ES cell transformants.VII., XIV.
9-11Pick ES cells.VIII., XV.
12-13Feed picked ES cells.VIII., XV.
14Freeze ES cell clones Et retain duplicate wells to grow ES cells for DNA isolation.IX., X.
Prepare Genomic DNA for Southern blot analysis.IX
16-19Recover clones following analysis using RESGRO. Culture Medium.XXI.

Coating Plates with Gelatin Solution

  1. Warm 0.1% Gelatin Solution to room temperature prior to use.
  2. In a culture hood, under sterile conditions, add Gelatin Solution to each well of the plate as suggested in the table to the right.
    Note: Add enough Gelatin Solution to adequately cover the plasticware surface.
  3. Leave the Gelatin Solution in the wells for at least 30 minutes at room temperature, with dish lids on in the laminar flow hood.
  4. Remove the Gelatin Solution by aspiration and discard. Immediately add media and cells to the dish. Do not allow the dishes to dry before adding cells.
PlateAmount / Well
96-well100 μL
48-well300 μL
24-well0.5 mL
12-well1.0 mL
6-well1.5-2.0 mL
30 mm1.5-2.0 mL
60 mm3.0 mL
100 mm4.0-5.0 mL 

Plating PMEF Feeder Cells

EmbryoMax® Primary Mouse Embryo Fibroblasts (PMEF) feeder cells are supplied as frozen vials containing 5–6 x 106 cells per vial at passage 3 (2–3 population doublings per passage). It is recommended that PMEF feeder cells be plated one day prior to plating ES cells, which guarantees approximately 95% confluence of the PMEF cells. If ES cells are plated earlier than one day after PMEF plating, there may be some small gaps in the feeder layer. Although plating ES cells when gaps are present may not have any detrimental effects on the ES cells, it is not recommended.

  1. Prior to thawing PMEF cells, coat plates/flasks with Gelatin solution (Section III).
  2. Thaw PMEF vial(s) quickly in a 37 °C water bath and transfer to a 15 mL tube (already containing 10 mL of warm PMEF Feeder Cell Medium.
  3. Gently invert the tube to distribute, and centrifuge at 300xg for 4–5 minutes.
  4. Remove supernatant and resuspend the cell pellet in warm PMEF Feeder Cell Medium.
  5. Remove the Gelatin solution from plates/flasks, and aliquot the PMEF feeder cell suspension at the densities recommended in Table 4.1 on the following page.
  6. Incubate the PMEF Feeder cells at 37 °C with 5% CO2. Use Figures 4A, B and C as a guide for an estimate of correct PMEF density and appearance. Gelatinized plates may be used for 12–14 days.
Dish SizeVolume (mL)/flask or wellGrowth Area (cm2)No. of feeder cells/flask or well
75 cm2 flask

12

75

3.75 x 106
25 cm2 flask

6

25

1.25 x 106
. mm plate

10

56

2.8 x 106
60 mm plate

5

21

1.0 x 106
6-well plate

4

9.5

4.75 x 105
12-well plate

2

4

2.0 x 105
24-well plate

1

2

1.0 x 105
96-well plate

0.1

0.32

1.5 x 104
Plating PMEF Feeder Cells

Figure 4.A) PMEF feeder cells at the correct density B)PMEF feeder cells at too low density C)PMEF feeder cells at too high density

ES Cell Culture using ESGRO® Medium Supplement

ESGRO® supplement is a special formulation of mouse LIF protein. Unlike regular LIF, which is sold by weight, each lot of ESGRO® supplement is sold based on its biological activity. The benefits of ESGRO® mLIF medium supplement include consistent inhibition of mouse ES cell differentiation, no batch-to-batch variation and the increased ability to grow mouse ES cells in feeder-free conditions.

ES Cell Culture without PMEF Feeder Cells

  1. Thaw a vial containing 1x107 ES cells into 4 mL of ES Cell Medium (containing ESGRO® supplement at 1000 units/mL). Centrifuge (3–5 minutes) and resuspend the cells in 10 mL of ES Cell Medium. Plate the ES cells onto the gelatinized plates at a density of 1–1.5 x 106 cells/25 cm2 (~3 x 106 cells/100 mm plate). Incubate the plates at 37 °C with 5% CO2. The cells appearance should resemble Image 5A.
  2. Examine the cells daily to determine if a change of media is required (indicated by a change of media color to yellow). After 2–3 days, ES cell cultures will become crowded with large colonies (Image 5B). At this point, passage ES cells at a 1:5 ratio.
  3. To passage ES cells, prepare two 100 mm gelatinized plates in advance as described (Section III). Remove ES Cell Medium, wash plates twice with DPBS, and add 1.2 mL of Trypsin. Incubate plates at 37 °C for 2 minutes, and then add 10 mL of ES cell medium. Pipette vigorously to break up the ES cell aggregates (avoid bubble formation).
  4. Add 2 mL of the cell suspension to each gelatinized plate containing 8 mL of ES Cell Medium. Excess ES cells can
  5. be frozen at a concentration of 2–10 x 106 cells per vial for future use. Please note that ES cells should always be passaged the day before you intend to electroporate.
ES Cell Culture without PMEF Feeder Cells

Figure 5A & B.ES Cell Culture without PMEF Feeder Cells

ES Cell Culture with PMEF Feeder Cells

  1. Thaw a vial containing 1x107 ES cells into 4 mL of ES Cell Medium (containing ESGRO® supplement at 1000 units/mL). Centrifuge (3–5 minutes) and resuspend the cells in 10 mL of ES Cell Medium.
  2. Remove the PMEF Feeder Cell Medium from a feeder plate prepared earlier (Section IV), and seed the ES cells onto the PMEF coated plate at a density of 1–1.5 x 106 cells/25 cm2 (~3 x 106 cells/100 mm plate). Incubate the plates at 37 °C with 5% CO2. The cells appearance should resemble Image 5C.
  3. Examine the cells daily to determine if a change of media is required (indicated by a change of media color to yellow). After 2–3 days, the ES cell cultures will become crowded with large colonies (Image 5D). At this point, passage the ES cells at a 1:5 ratio.
  4. To passage ES cells, prepare two 100 mm plates containing PMEF cells as previously described (Section 4). Remove the ES Cell Medium, wash plates twice with DPBS, and add 1.2 mL of Trypsin. Incubate at 37 °C for 2 minutes. Add 10 mL of ES Cell Medium and pipette vigorously to disperse the ES cell aggregates (avoid bubble formation).
  5. Add 2 mL of the cell suspension to each of the PMEF cell plates containing 8 mL of ES Cell Medium. Excess ES cells can be frozen at a concentration of 2–10 x 106 cells per vial for future use. Please note that ES cells should always be passaged the day before you intend to electroporate.
ES Cell Culture with PMEF Feeder Cells

Figure 6.

Electroporation of ES Cells

  1. The evening before the electroporation is to be performed, prepare 4 plates with PMEF cells (Section IV).
  2. The morning that the electroporation is to be performed feed the ES cells fresh ES Cell Medium.
  3. Later that afternoon, harvest the ES cells as described previously, and determine the cell count. 1x107 ES cells is the minimum number of ES cells required for electroporation. If there is excess, freeze the cells down as previously described.
  4. Centrifuge the cells required for electroporation at 300xg for 10 minutes, then aspirate the medium.
  5. Resuspend the ES cell pellet in 600 μL of Electroporation Buffer.
  6. 25–40 μg of knockout construct DNA (purified) should already be linearized, ethanol precipitated and dried as a pellet. In a sterile hood, dissolve the DNA pellet in 30 μL of Electroporation Buffer, and then add the solution to the ES cells. Mix well and leave for 5 minutes at room temperature.
  7. Place the ES cells in a 0.4 cm electroporation cuvette. Electroporate the suspension at 500 μFD, 0.24 kV. The time constant produced should be between 6.9 and 7.9 milliseconds (optimal 7.2). Following electroporation, place the cuvette on ice for 10 minutes.
  8. Transfer the electroporated ES cells to 40 mL of ES Cell Medium and mix gently using a Pasteur pipette.
  9. Plate the ES cell suspension (10 mL per feeder plate, total of 4 plates). Ensure that the PMEF Feeder Cell Medium is removed prior to the addition of cells.
  10. Incubate for approximately 36 hours at 37 °C and 5% CO2 prior to antibiotic selection.

Selection of ES Cells

Prior to selection, it is recommended that a kill curve should be determined for each ES cell line in order to determine the exact drug concentration to be used. The following selection regimes can be used as a guide:

  • Neomycin (G418) in 129SVEV and 129SVJ cells: 350 μg/mL for two days, then 150 μg/mL for the rest of the selection. Total 5–7 days selection
  • Neomycin (G418) in C57BL6/J cells: 275 μg/mL for one day, 200 μg/mL for the second day, then 150 μg/mL for the rest of the selection. Total 6–8 days selection
  • Hygromycin B in 129SVEV and 129SVJ cells: 100 μg/mL for two days, then 75 μg/mL for one day, then 50 μg/mL for the rest of the selection. Total 7–10 days selection
  1. To select for transformants, add ES cell medium containing either Neomycin (G418) or Hygromycin B.
  2. After 48 hours, cell death should be apparent. Change the culture medium daily if there is excessive debris evident or if the medium is discoloring, otherwise every other day is sufficient. If the debris is adhering to the living cells, wash the cells gently with sterile DPBS before changing the medium, taking care not to dislodge the feeder cell layer. ES cells should be cultured for approximately 10 days following electroporation.

Colony Picking

Depending upon the cell line and the media used, ES cell colonies are generally ready for picking 5–10 days after electroporation. The most suitable colonies to select are those that appear rounded or oval in shape, with a phase contrast bright edge and often a dark necrotic center. Differentiated colonies are flat and often surrounded by fibroblast like cells that form cobblestone-like structures. These cells should be avoided when selecting cells. ES cells can be picked onto either gelatinized plates or a PMEF feeder cell layer depending upon the ES cell line used. If gelatinized plates are preferred, please disregard the use of feeder cells as described in the procedure below.

  1. The day before picking ES cell colonies, coat an appropriate number of 24-well plates with PMEF Cells (SectionIV) or gelatin (Section III).
  2. Prior to selecting ES cell colonies, ensure that you are wearing gloves, a gown and face mask. All surfaces including the microscope, bench, tip boxes and pipette should be wiped with ethanol prior to use.
  3. Inspect the ES cell cultures at 4x magnification. Colonies selected for picking should be spaced well enough apart to ensure no contamination from surrounding colonies. When a desired colony is found, circle the colony with a pipette tip to loosen the surrounding fibroblast layer. With the pipette set to a volume of 15 μL, scrape the colony with the pipette tip to dislodge the colony, then aspirate (the colony is often visible inside the tip). Transfer the picked colony to an empty well in a 96-well plate.
  4. Continue picking and transferring ES cell colonies to fresh wells using a new tip each time, until a suitable number is picked. Clones are often picked in batches of 48 cells to prevent fatigue.
  5. Add a single drop of Trypsin to each well and incubate at 37 °C for 2 minutes. During this period, replace the PMEF Cell Media in the 24-well plates with 500 μL of ES cell medium.
  6. 6. Disperse each ES cell colony in the 96-well plate by using a pipette to break up each colony, avoiding excessive foaming. Transfer the suspension to the 24-well plate (including foam) containing 500 μL of ES cell medium, using a fresh tip for each well.
  7. When all the colonies are transferred, mix each well using a clean pipette tip set to 400 μL. Incubate at 37 °C and 5% CO2. Feed every day with medium supplemented with Neomycin (150 μg/mL) or Hygromycin (50 μg/mL) antibiotics.
  8. New colonies should be evident within a few days. If the colonies are too close in proximity to each other, disperse them using a 1 mL pipette tip to break up the colonies and spread the cells (Trypsin is not required as colonies break up very easily). Each well should be evenly covered with colonies before harvesting.
  9. Continue changing the ES cell medium every day until a good coverage of colonies in each well is achieved (typically 7–10 days).

Troubleshooting Guide

The two most common problems encountered when generating knockout mice are (1) ES cell differentiation, and (2) the inability to generate chimeras once a targeted ES cell clone has been established. In Table 25.1 are a number of common causes of ES cell differentiation and recommendations on how to help prevent differentiation from occurring. The extent of ES cell differentiation can be determined by examining the morphology of the ES cell colonies, or more thoroughly assessed using EMD Millipore’s ES Cell Characterization Kit or Alkaline Phosphatase Detection Kit. These kits contain monoclonal antibodies to ES cell markers and reagents for Alkaline Phosphatase detection that permit a discrimination of pluripotent and differentiated ES cells. Also included in Table 25.2 are a number of reasons that often cause the slow growth of ES cells. Table 25.3 contains possible causes for the lack of generating chimeras.

Common causes of ES cell differentiation and recommendations.

Cause of ES Cell DifferentaitionRecommendations
Incorrect concentration of mLIFESGRO® mLIF medium supplement should be used at the recommended concentration of 1000 units/mL in ES cell media.
Expiry date of ESGRO® MediaAlways check the date of each batch prior to use. Medium should be less than 4 weeks old as glutamine by-products could be toxic to ES cells. ES cells should be fed with fresh media every 2–3 days or when media discolors.
SerumNew batches of Fetal Bovine Serum should be tested for the effect of inducing differentiation. ES cell medium usually requires a serum concentration between 10% and 20%. We recommend the use of EmbryoMax ES cell qualified serum.
Lack of passagingES cells should be passaged every 2–3 days as frequent passaging removes differentiated cells. Only undifferentiated ES cells will survive frequent passaging. Refer to Images 25A–25G for illustrations of ES cell confluency and differentiated ES cells.
DisinfectantsDisinfectants such as Roccal® or Lysol® preparations should be avoided in the Tissue Culture Room and incubator where ES cells are cultured. Some disinfectants have been suspected to cause differentiation by use in water baths and aerosols created by spray wiping. The use of 70% ethanol to clean tissue culture surfaces is recommended.
Feeder cellsIf differentiation cannot be controlled using ESGRO® mLIF medium supplement with gelatinized plates, it may be necessary to culture ES cells on a feeder layer. Please refer to Section 4 for the recommended number of growth arrested fibroblasts. ESGRO® supplement should be added at a concentration of 1000 units/mL to assist in maintaining undifferentiated ES Cells.
Incubator settingsEnsure that the incubator readings are correct at 37 °C and 5% CO2.
Rate of growth of ES cellsSlow growing ES cells will be most likely to undergo differentiation. Increase serum concentration if cells are not growing quickly enough.
GelatinIt is preferable to use cell culture grade gelatin at all times (even if using feeder layers) as gelatin minimizes surface differences on the tissue culture plates. EmbryoMax® ES cell qualified 0.1% gelatin solution is recommended.
Low level of contaminationRegular use of Pen/Strep in media can often mask a low level contamination with agents such as mycoplasma. It is recommended to routinely test your ES cell lines for mycoplasma contamination on a periodic basis.
Table 25.1.

Causes of slow growth of ES cells and recommendations

Cause of Slow ES Cell GrowthRecommendations
Insufficient serumIdeally a concentration of between 10% and 20% serum is used; however, this will vary according to each ES cell strain. It is recommended to routinely test new batches of serum to determine the optimum concentration required for fast growth without inducing excessive differentiation. We recommend the use of EmbryoMax® ES cell qualified serum.
Low number of ES cellsES cells grow optimally when slightly crowded. Plate a higher density from frozen stocks or passage cells to increase individual colony numbers. Refer to the images below for illustrations of ES cell confluency.
Table 25.2.

Causes for the lack of chimeras

Cause of Lack
of Chimeras
Recommendations
Time taken to culture the ES
cells
Once the targeted ES cell clone is identified, minimize thetime that the ES cells remain in culture. It is preferable  to passage ES cell lines no more than 1–2 times prior to microinjection and/or aggregation.
Karyotype the ES cellsThe routine karyotype analysis of ES cells is recommended, particularly when the ES cell lines are reaching a high passage number.
Undetected differentiationSome degree of differentiation may go undetected by routine microscopic examination, and therefore regular passage of the ES cells is necessary. For a detailed assessment of ES cell differentiation, EMD Millipore’s ES Cell Characterization Kit or Alkaline Phosphatase Detection Kit are recommended (Section XXVII). Please refer to Section XXII of this manual for information on the use of RESGRO™ Culture Medium for the removal of differentiated ES cells within a cell line.
ES cell passage numberIn general, the best chimeras are generated from low passage number ES cells. If cell lines have been cultured for a high number of passages, it is recommended to use a lower passage frozen stock.
Number of ES cells
microinjected
Most often ES cell lines are microinjected at approximately 8–12 cells/blastocyst.
Time taken prior to microinjectionIt is recommended that ES cells be microinjected as soon as possible after removing them from the tissue culture plates, and not left on ice or at room temperature for extended periods of time.
Compatibility of ES cells and
mouse strain
Prior to any microinjection or aggregation procedures, please check the combination of embryo strains and ES cells, as some strains have been reported to be incompatible.
Table 25.3.

Media Formulations

PMEF Feeder Cell Culture Media
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Serum Containing Mouse ES Cell Culture Media
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Materials
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