StemXVivo Human/Mouse Chondrogenic Supplement, 0.5 mL

Base media for the differentiation of MSCs into chondrocytes. For use with Human/Mouse and Rat StemXVivo® Chondrogenic Supplements.

Why Induce Chondrogenesis in MSCs with a Defined Media Supplement?

Despite the well-characterized factors and protocols used to differentiate mesenchymal stem/stromal cells (MSCs) into chondrocytes, differentiation efficiencies can vary depending on the quality of the MSC starting population and the reagents used to expand and differentiate MSCs.

Human/Mouse StemXVivo^® Chondrogenic Supplement:

• Contains high quality differentiation factors to drive reproducible and efficient MSC chondrogenesis.
• Is defined to reduce unwanted experimental variability.
• Has been developed and optimized using human and mouse MSCs.

The term ‘mesenchymal stromal cells’ is commonly used to describe a heterogeneous population of cultured cells that are adherent to plastic, have a distinct morphology, and express a specific set of marker proteins. Within this heterogeneous population are cells referred to as ‘mesenchymal stem cells.’

Mesenchymal stem cells are multipotent, self-renewing cells that have the ability to differentiate into adipocytes, chondrocytes, and osteoblasts when cultured in vitro. Read More about MSC Nomenclature

Human/Mouse Chondrogenic Supplement Components

This media supplement contains defined, high quality factors to drive MSC differentiation into chondrocytes.

• This supplement requires media (not included), such as Human/Mouse/Rat StemXVivo^® Chondrogenic Base Media (Catalog # CCM005) or equivalent.
• The quantity of chondrogenic media supplement supplied is sufficient to make 50 mL of media for differentiation.

2006 Proposed Change to MSC Nomenclature

Although mesenchymal stromal cells were once referred to as ‘mesenchymal stem cells’, a change to ‘mesenchymal stromal cells’ was proposed by the International Society for Cellular Therapy in 2006.¹

The change in nomenclature originates from two important factors:

• Methods used to isolate mesenchymal stem cells yield a heterogeneous population of cells with only a fraction of these cells demonstrating multipotency.
• The absence of direct evidence that mesenchymal stem cells can self-renew and differentiate in vivo.

Use of Mesenchymal Stem and Stromal Cell Terminology

Data supporting MSC self-renewal and multipotency have been obtained using in vitro conditions, which does not adequately reflect the in vivo environment. The lack of in vivo data has led some researchers to question the validity of the term ‘mesenchymal stem cell’ providing further support for the use of ‘mesenchymal stromal cells’ to describe MSCs.² While ‘mesenchymal stromal cells’ may be the more scientifically accurate term for MSCs, the two terms are often used interchangeably in the literature. R&D Systems recognizes the use of both mesenchymal stem cells and mesenchymal stromal cells and uses ‘MSC’ to indicate mesenchymal stem/stromal cells to account for both designations.

Definitions of Mesenchymal Stromal Cells and Mesenchymal Stem Cells

• Mesenchymal Stromal Cells – A heterogeneous population of cultured cells with similar characteristics such as the ability to adhere to plastic and the expression of specific marker proteins.
• Mesenchymal Stem Cells – A subpopulation of mesenchymal stromal cells that have the capacity to self-renew and differentiate into mesodermal lineages when cultured in vitro. The capacity to self-renew and differentiate in vivo has yet to be clearly demonstrated for mesenchymal stem cells.

References

• Dominici, M. et al. (2006) Cytotherapy 8:315.
• Keating, A. (2012) Cell Stem Cell 10:709.

Scientific Data Examples for StemXVivo Human/Mouse Chondrogenic Supplement, 0.5 mL

	Detection of Aggrecan in a Human MSC-differentiated Chondrogenic Pellet Section. Human MSCs cultured with Human/Mouse/Rat StemXVivo®Chondrogenic Base Media (Catalog # CCM005) and Human/Mouse StemXVivo®Chondrogenic Supplement (Catalog # CCM006) and the resulting chondrogenic pellet was cryosectioned. Chondrocyte differentiation was verified using a Goat Anti-Human Aggrecan Antigen Affinity-purified Polyclonal Antibody (Catalog # AF1220). The cells were stained using a NorthernLights™557-conjugated Donkey Anti-Goat Secondary Antibody (Catalog # NL001) and the nuclei were counterstained with DAPI.
	MSCs Differentiated into Chondrocytes form Characteristic Cell Pellets.  Human MSCs cultured with Human/Mouse/Rat StemXVivo®Chondrogenic Base Media (Catalog # CCM005) and Human/Mouse StemXVivo®Chondrogenic Supplement (Catalog # CCM006) formed a chondrogenic pellet (ball) imaged here at day 21 of culture.
	Detection of Collagen II in a Mouse MSC-differentiated Chondrogenic Pellet Section. Mouse MSCs were cultured for 21 days using the Human/Mouse StemXVivo®Chondrogenic Base Media (Catalog # CCM005) and Human/Mouse StemXVivo®Chondrogenic Supplement (Catalog # CCM006) and the resulting chondrogenic pellet was cryosectioned. Chondrocyte differentiation was verified using a Sheep Anti-Mouse Collagen II Antigen Affinity-purified Polyclonal Antibody (Catalog # AF3615). The cells were stained using a NorthernLights™557-conjugated Donkey Anti-Sheep Secondary Antibody (Catalog # NL010).

Assay Procedure

Refer to the product datasheet for complete product details.

Briefly, human or mouse MSCs are differentiated into chondrocytes using the following in vitro differentiation procedure:

• Culture multipotent cells of interest
• Induce chondrogenic differentiation using a media supplement
• Evaluate differentiation using a mature phenotype marker antibody and fluorescent ICC

For use with Human/Mouse/Rat StemXVivo^® Chondrogenic Base Media (Catalog # CCM005).

View Graphic Procedure

 

 

Reagents Provided

Reagents supplied in the Human/Mouse StemXVivo^® Chondrogenic Supplement (Catalog # CCM006):

• 0.5 mL of StemXVivo^® Chondrogenic Supplement

 

Other Supplies Required

Reagents

• Human/Mouse/Rat StemXVivo^® Chondrogenic Base Media (Catalog # CCM005)
• Penicillin-Streptomycin-Glutamate (100X)

Materials

• MSCs
• 15 mL centrifuge tubes
• Pipettes and pipette tips
• Serological pipettes

Equipment

• 37 °C and 5% CO₂ incubator
• Centrifuge
• Hemocytometer
• Inverted microscope
• 2 °C to 8 °C refrigerator
• 37 °C water bath

 

Procedure Overview

This protocol has been tested using bone marrow- and/or adipose tissue-derived MSCs. If using a different tissue source or cell line, the protocol below may need to be optimized.

Transfer 2.5 x 10⁵ MSCs to a 15 mL conical tube.

Centrifuge and resuspend the cells in Chondrogenic Differentiation Medium.

Centrifuge the cells but do not remove the medium.

Every 2-3 days, replace with fresh Chondrogenic Differentiation Medium.

After 14-21 days, the chondrogenic pellet can be harvested and analyzed.

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