HONDA MSX125的問題,透過圖書和論文來找解法和答案更準確安心。 我們找到下列包括價格和評價等資訊懶人包

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國立臺灣大學 臨床牙醫學研究所 劉步遠、侯連團所指導 邱慧緣的 人類牙齦纖維母細胞之培養與分化潛力及效能之探討 (2008),提出HONDA MSX125關鍵因素是什麼,來自於間葉幹細胞、牙齦纖維母細胞、牙齒幹細胞、牙周韌帶幹細胞、人類皮膚纖維母細胞、人類骨膜細胞。

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HONDA MSX125進入發燒排行的影片

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人類牙齦纖維母細胞之培養與分化潛力及效能之探討

為了解決HONDA MSX125的問題,作者邱慧緣 這樣論述:

Background: Recently, the discovery of multipotent stem cell populations residing in periodontal ligament (PDL) and dental pulp provides exciting prospects of resource for periodontal or tooth regeneration. The expense of a tooth and difficulty in cultivating PDL and pulp cells, however, hinders th

e clinical application of PDL and pulp cells in tissue engineering for repairing dental tissues. In contrast, gingival cells could be easily harvested and expanded in vitro. Furthermore, gingiva has been reported to develop from an ectomesenchymal origin rather than a mesenchymal one, and ectomesenc

hymal stem cells are believed to be pluripotent during early development. Thus, the possible existence of ectomesenchymal stem cells in gingiva makes it of great importance to investigate the putative stem cell or progenitor cell populations in gingival fibroblasts. The purpose of this study is thro

ugh flow cytometry and induced differentiation to prove the existence of putative stem cell populations in gingiva.Materials and Methods: Primary human gingiva-derived fibroblast-like cells (GFs) was obtained from palatal gingiva of seven healthy adults. For phenotypic characterization, cells from p

assages two or three were harvested to identify stem cells or mesenchymal progenitor cells-specific surface molecules, such as CD29, CD44, CD90, CD105, CD146 and STRO-1 by flow cytometry. For investigation of osteogenic and adipogenic differentiation capacity, cells were treated with osteogenic or a

dipogenic induction medium. After stimulation, the results were analyzed by histochemistry staining, such as alkaline phosphatase (ALP) staining and Alizarin Red-S staining for osteogenic lineage cells and Oil Red-O staining for adipogenic lineage cells. Besides, the findings were further examined b

y RT-PCR for expression of osteogetic markers, such as Runx2, ALP and OCN (Osteocalcin), and adipogenic markers, such as PPARγ2 (Peroxisome proliferative activated receptor gamma 2) and LPL (lipoprotein lipase).Result: GFs demonstrated not only similar morphology to mesenchymal stem cells (MSCs), up

on phenotypic characterization, they also shared almost the same cell surface markers profile with MSCs. Furthermore, under the stimulation of osteogenic or adipogenic induction medium, the positive results of ALP, Alizarin Red-S, and Oil Red-O stainings revealed that GFs possessed the capability to

differentiated into osteogenic and adipogenic lineages, and these findings were further confirmed by the expression of osteoblastic and adipocytic lineage genes by RT-PCR.Conclusions: We speculate that GFs comprise of not only fibroblasts but also mesenchymal progenitor cells (MPCs) of osteogenic a

nd adipogenic lineages and possibly some MSCs, to some extent. These observations provide clues in clinical applications of gingival cells in cell-based regeneration for dental tissue repair in future.