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User-generated protocol

Confirmation of pluripotency by spin embryoid body formation

Introduction Materials required Protocol

Introduction  

Embryoid bodies (EBs) are three-dimensional aggregates comprised of human pluripotent stem cells (hPSCs). Within EBs, hPSCs undergo differentiation and cell specification along the three germ layers, which are commonly used as an assessment of the initial hPSCs' pluripotency. The protocol for formation of spin EBs can be used as a basis for the development of protocols for directed differentiation via EBs.

Materials required  

  • 24-well plates, cell-culture treated, flat bottom
  • 96-well plates, non-treated, V bottom
  • Advanced RPMI 1640
    (with glucose, sodium pyruvate, and non-essential amino acids; without L-glutamine and HEPES)
  • B-27 Supplement (50X), serum free
  • DEF-CS COAT-1
  • GlutaMAX-I (100X; 200 mM)
  • PBS Dulbecco's with Ca2+ & Mg2+ (D-PBS +/+)
  • PBS Dulbecco's w/o Ca2+ & Mg2+ (D-PBS –/–)
  • Penicillin-streptomycin
    (PEST; 10,000 units/ml of penicillin and 10,000 µg/ml of streptomycin)
  • TrypLE Select Enzyme (1X), no phenol red
    (Thermo Fisher Scientific, Cat. # 12563011)
  • Y27632

Protocol  

Medium preparation

Preparing the in vitro differentiation (IVD) medium

Prepare the IVD medium by adding 10 ml B-27 Supplement (50X), 5 ml GlutaMAX-I (100X), and 5 ml PEST to 500 ml of Advanced RPMI 1640. Mix the solution properly and carefully. The medium expires one month after the date of preparation.

Preparing the seeding medium

Prepare the seeding medium by adding Y27632 (to a final concentration 5 µM) to the IVD medium. Prepare fresh medium on the day of intended use.

Formation of spin EBs

  1. Warm the seeding medium to 37°C ± 1°C and all other reagents to room temperature (RT, 15–25°C) before use.
  2. Wash one T25 flask containing confluent hPSCs with 5 ml D-PBS –/–.

    NOTE: The entirety of this flask will be used for spin EB formation. Ensure other flasks or banked cells of equivalent passage number exist in order to preserve the original line.

  3. Add 500 µl of TrypLE Select (20 µl/cm2) and place the cells in an incubator at 37°C ± 1°C, 5% CO2, and >90% humidity for 5 min, or until cells start to detach.
  4. Add 5 ml of seeding medium and dissociate the cells, pipetting up and down until a single-cell suspension is achieved.
  5. Count the cells to determine the initial cell concentration.
  6. Make a cell suspension of 20 ml seeding medium containing 2.5 x 105 cells/ml.
  7. Seed 200 µl of the final cell suspension into each well of a 96-well plate (non-treated, V bottom), generating a seeding density of 5 x 104 cells/well.
  8. Centrifuge at 400g at RT for 5 min.
  9. Place the 96-well plate in the incubator at 37°C ± 1°C, 5% CO2, and >90% humidity and let it sit undisturbed for 7 days to form EBs.

    NOTE: Throughout this process, the cells are undergoing spontaneous differentiation. During the incubation period, directed differentiation protocols can be optimized and applied. Alternatively, if pluripotency is to be assessed, continue to the next section.

Spontaneous differentiation of spin EBs

Coating of the cell culture plate

  1. Dilute the required volume of DEF-CS COAT-1 in D-PBS +/+ before use. Make a 1:20 dilution.
  2. Mix the diluted DEF-CS COAT-1 solution gently and thoroughly by pipetting up and down.
  3. Add the appropriate volume of diluted DEF-CS COAT-1 solution to a 24-well plate (use 0.2 ml/cm2); make sure the entire culture surface is covered.
  4. Place the plate for a minimum of 20 min in an incubator at 37°C ± 1°C, 5% CO2, and >90% humidity or 0.5–3 hr at RT.
  5. Aspirate DEF-CS COAT-1 solution from plate immediately before use.

Transferring of spin EBs

  1. Warm IVD medium to 37°C ± 1°C.
  2. Add 1.5 ml of fresh, warm IVD medium to each well of the coated 24-well plate.
  3. Carefully detach and transfer the EBs using a pipette. Transfer 5–7 EBs to each well of the 24-well plate.
  4. Place the 24-well plate in the incubator at 37°C ± 1°C, 5% CO2, and >90% humidity and let it sit undisturbed for 4 days.

Exchanging the media

NOTE: Complete a 100% media change every 2–3 days.

  1. Warm IVD medium to 37°C ± 1°C.
  2. Completely exchange the media in each well of the 24-well plate (1.5 ml/well).

    NOTE: 18–21 days after the start of spin EB formation, the cells are ready to be analyzed for the presence of specialized cells along the three germ layers. The number of days needed depends on the cell line.

Related products

Cat. # Product Size Price License Quantity Details
Y30010 Cellartis® DEF-CS™ 500 Culture System 1 Kit USD $583.00

License Statement

ID Number  
C001 This product is manufactured and sold by Takara Bio Europe SAS based on a commercial license to certain intellectual property rights held by Wisconsin Alumni Research Foundation (“WARF”). This product is covered by one or more claims of U.S. Patent No. 7,514,260 and its foreign counterparts. The purchase of this product conveys to the buyer the non-transferable right to use the product for its intended use, strictly limited to purchaser’s own internal research. No other express or implied license is granted to the purchaser. Purchaser cannot have any right to use this product or its components in humans for any purposes including but not limited to diagnostics and/or therapeutics, or otherwise clinical trials. Purchase does not include any right to resell or transfer this product to a third party regardless of whether or not compensation is received. Purchasers wishing to use this product for purposes other than internal research use should contact us.

Cellartis DEF-CS 500 Culture System is a defined culture system for efficient expansion of undifferentiated human pluripotent stem cells. This kit includes basal medium, coating substrate, and additives.

Notice to purchaser

Our products are to be used for Research Use Only. They may not be used for any other purpose, including, but not limited to, use in humans, therapeutic or diagnostic use, or commercial use of any kind. Our products may not be transferred to third parties, resold, modified for resale, or used to manufacture commercial products or to provide a service to third parties without our prior written approval.

Documents Components You May Also Like Image Data

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Expansion potential of a characterized working bank of human induced pluripotent stem (iPS) cells in the Cellartis DEF-CS Culture System

Expansion potential of a characterized working bank of human induced pluripotent stem (iPS) cells in the Cellartis DEF-CS Culture System
Expansion potential of a characterized working bank of human induced pluripotent stem (iPS) cells in the Cellartis DEF-CS Culture System. The Cellartis DEF-CS Culture System can produce 2 x 109 human iPS cells within 4 passages (18–20 days) from frozen cells (2.0–2.5 x 106 cells).

Back

Robust growth of human induced pluripotent stem (iPS) cells in the Cellartis DEF-CS Culture System

Robust growth of human induced pluripotent stem (iPS) cells in the Cellartis DEF-CS Culture System
Robust growth of human induced pluripotent stem (iPS) cells in the Cellartis DEF-CS Culture System. The number of iPS cells was quantified after being cultured for three weeks using either the Cellartis DEF-CS Culture System, a reference feeder system, or four other stem cell culture systems.

Back

Human induced pluripotent stem cells (iPS) cells grown in the Cellartis DEF-CS Culture System have the highest proportion and intensity of markers of pluripotency

Human induced pluripotent stem cells (iPS) cells grown in the Cellartis DEF-CS Culture System have the highest proportion and intensity of markers of pluripotency
Human induced pluripotent stem cells (iPS) cells grown in the Cellartis DEF-CS Culture System have the highest proportion and intensity of markers of pluripotency. Quantitative analysis of TRA1-60 (Panel A) and SSEA4 (Panel B) expression was performed on human iPS cells after five weeks culture in either the Cellartis DEF-CS Culture System, a reference feeder cell containing system, or four different stem cell culture systems.

Back

Human iPS cells grown in the Cellartis DEF-CS Culture System look different from those grown with traditional aggregate culture techniques

Human iPS cells grown in the Cellartis DEF-CS Culture System look different from those grown with traditional aggregate culture techniques
Human iPS cells grown in the Cellartis DEF-CS Culture System look different from those grown with traditional aggregate culture techniques. Freshly passaged human iPS cells were cultured for 5 days in either the Cellartis DEF-CS Culture System, on feeder cells, in mTeSR 1 medium (STEMCELL Technologies), or in Essential 8 Medium (E8; Life Technologies).

Back

Human induced pluripotent stem (iPS) cells cultured long-term in the Cellartis DEF-CS Culture System retain a normal karyotype

Human induced pluripotent stem (iPS) cells cultured long-term in the Cellartis DEF-CS Culture System retain a normal karyotype
Human induced pluripotent stem (iPS) cells cultured long-term in the Cellartis DEF-CS Culture System retain a normal karyotype. The human iPS cell line ChiPSC18 was cultured for 20 passages in the Cellartis DEF-CS Culture System. Chromosomal analysis indicates that the cells retain a normal karyotype.

Back

Human induced pluripotent stem (iPS) cells can be passaged as single cells in the Cellartis DEF-CS Culture System

Human induced pluripotent stem (iPS) cells can be passaged as single cells in the Cellartis DEF-CS Culture System

Human induced pluripotent stem (iPS) cells can be passaged as single cells in the Cellartis DEF-CS Culture System. A single GFP-actin iPS cell was isolated and placed in the well of a culture dish. Twenty-four hours after seeding, morphology was assessed by fluorescence microscopy at 20x (Panel A) and 40x (Panel B) magnification. Sixteen days later, the single GFP-actin iPS cell had proliferated into numerous cells as evidenced by microscopic observation at 4x (Panel C), 10x (Panel D), 20x (Panel E), and 40x (Panel F) magnification.

Back

Human pluripotent stem cells remain undifferentiated when cultured in the Cellartis DEF-CS Culture System

Human pluripotent stem cells remain undifferentiated when cultured in the Cellartis DEF-CS Culture System

Human pluripotent stem cells remain undifferentiated when cultured in the Cellartis DEF-CS Culture System. Human iPS cells cultured for 23 passages in the Cellartis DEF-CS Culture System were characterized by Oct-4 staining (Panel A) and nuclear staining (Panel B).

Back

Y30010: Cellartis DEF-CS 500 Culture System

Y30010: Cellartis DEF-CS 500 Culture System


User-generated protocols

User-generated protocols

User-generated protocols are based on internal proof-of-concept experiments, customer collaborations, and published literature. In some cases, relevant results are discussed in our research news BioView blog articles. While we expect these protocols to be successful in your hands, they may not be fully reviewed or optimized. We encourage you to contact us or refer to the published literature for more information about these user-generated and -reported protocols. 

If you are looking for a product-specific, fully optimized User Manual or Protocol-At-A-Glance, please visit the product's product page, open the item's product details row in the price table, and click Documents. More detailed instructions for locating documents are available on our website FAQs page.

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