4.3 Article

Simplification of aggregate culture of human mesenchymal stem cells as a chondrogenic screening assay

期刊

BIOTECHNIQUES
卷 42, 期 6, 页码 732-+

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INFORMA HEALTHCARE
DOI: 10.2144/000112451

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  1. NIAMS NIH HHS [R01 AR050208-01A2, R01 AR050208, 5R01-AR050208] Funding Source: Medline
  2. NATIONAL INSTITUTE OF ARTHRITIS AND MUSCULOSKELETAL AND SKIN DISEASES [R01AR050208] Funding Source: NIH RePORTER

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Aggregate culture provides a three-dimensional (3-D) environment for differentiating or differentiated cells; it is particularly useful to study in vitro chondrogenesis and cartilage biology. We have recently ported this method from a conical tube-based format to a 96-well plateformat for the study of mesenchymal stem cell (MSC) chandrogenesis. The microplate format has greatly reduced the workload and materials cost, while maintaining reproducible chondrogenic differentiation. A long-term goal is to fully automate aggregate culture-this requires critically identifying all the indispensable steps of the protocol. Robotic laboratory equipment for manipulating microplate assays are commercially available; however, centrifugation steps are difficult to implement automatically. We, therefore, tested whether the centrifugation step can be eliminated, thus significantly streamlining the assay work-flow. By comparing aggregates prepared from human bone marrow-derived MSCs (hMSCs) that were formed either through centrifugation or through free sedimentation, we found that both methods produce aggregates with similar formation kinetics, and that there was no perceptible difference in the timing of the appearance of markers of chondrogenesis. Thus, 1. t appears safe to eliminate the centrifugation step from the aggregate culture protocol. This results in significant time and effort savings and paves the way for future full automation o the aggregate assay.

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