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Plasmacytoid myoepithelioma of minor salivary glands: report of case with emphasis in the immunohistochemical findings
Authors:Esaú P Santos  Danielle RR Cavalcante  Allan UC Melo  José C Pereira  Margarete Z Gomes  Ricardo LC Albuquerque Jr
Affiliation:1. Departments of Oral and Maxillofacial Surgery, Hospital of Piacenza, Via Taverna, 49, 29100, Piacenza, Italy
2. Department of Immunohematology, Hospital of Piacenza, Via Taverna, 49, 29100, Piacenza, Italy
3. Department of Cardiology, Hospital of Piacenza, Via Taverna, 49, 29100, Piacenza, Italy
4. Department of Oncology and Hematology, Hospital of Piacenza, Via Taverna, 49, 29100, Piacenza, Italy
5. Department of Pathology, Hospital of Piacenza, Via Taverna, 49, 29100, Piacenza, Italy
Abstract:Extracorporeal formation of mineralized bone-like tissue is still an unsolved challenge in tissue engineering. Embryonic stem cells may open up new therapeutic options for the future and should be an interesting model for the analysis of fetal organogenesis. Here we describe a technique for culturing embryonic stem cells (ESCs) in the absence of artificial scaffolds which generated mineralized miromasses. Embryonic stem cells were harvested and osteogenic differentiation was stimulated by the addition of dexamethasone, ascorbic acid, and ß-glycerolphosphate (DAG). After three days of cultivation microspheres were formed. These spherical three-dimensional cell units showed a peripheral zone consisting of densely packed cell layers surrounded by minerals that were embedded in the extracellular matrix. Alizarine red staining confirmed evidence of mineralization after 10 days of DAG stimulation in the stimulated but not in the control group. Transmission electron microscopy demonstrated scorching crystallites and collagenous fibrils as early indication of bone formation. These extracellular structures resembled hydroxyl apatite-like crystals as demonstrated by distinct diffraction patterns using electron diffraction analysis. The micromass culture technique is an appropriate model to form three-dimensional bone-like micro-units without the need for an underlying scaffold. Further studies will have to show whether the technique is applicable also to pluripotent stem cells of different origin.
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