Mesenchymal Stem Cells Clinical Trial
In this study, the investigators explored the hypothesis that osteoarthritic cartilage
fragments can promote chondrogenesis of MSCs. Non-wearing parts of cartilage tissues were
harvested from one osteoarthritic patient during the total knee arthroplasty surgery.
Cartilage fragments and MSCs were wrapped into fibrin glue; and the constructs were
implanted subcutaneously into nude mice.
Moreover, the investigators will collect the discard cartilage to develop an acellular
cartilage ECM-derived scaffold in the joint replacement surgery. In addition, the
investigators will harvest the redundant bone marrow from drilling or useless synovium
during the surgery to separate the mesenchymal stem cells. Furthermore, these mesenchymal
stem cells will be transfected with hTERT for rejuvenation and then will be labeled with
fluorescent dye PKH26 for application of animal study. To sum up, the investigators plan to
use human, natural, and discard materials from the joint replacement surgery to develop
appropriate allograft for cartilage repair and hope that one day this ideal would be apply
in clinical.
Extracellular matrix (ECM) is thought to participate significantly in guiding the differentiation process of mesenchymal stem cells (MSCs). In this study, we explored the hypothesis that osteoarthritic cartilage matrix can promote chondrogenesis of MSCs. Cartilage matrix was harvested from the health-like parts of osteoarthritic cartilage tissue. Cartilage fragments and MSCs were wrapped into fibrin glue; and the constructs were implanted subcutaneously into nude mice. Histological analysis showed a round and elongated cell appearance with positive Alcian blue staining of cartilage matrix formation in the constructs. However, the cells in fibrin glue only were condensed like MSCs in pellet culture. Immunohistochemical staining was abundantly positive for type II collagen in neo-cartilage regions of cartilage fragment-fibrin glue-MSC constructs, while the constructs without cartilage fragments were negative in staining for type II collagen. The gene expressions of type II collagen in the constructs with 60 mg fragments were significantly elevated after 4 weeks of implantation. Conversely, constructs without cartilage fragments failed to express type II collagen, which indicated that MSCs could not differentiate into a chondrogenic lineage. In conclusion, we demonstrated the effects of osteoarthritic cartilage matrix in promoting chondrogenic differentiation of MSCs. This was a favorable method without exogenous growth factors induction. ;
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