人甲状旁腺干细胞的分离与鉴定
Isolation and characterization of stem cells from the human parathyroid gland.
作者信息
Shih Y-R V, Kuo T K, Yang A-H, Lee O K, Lee C-H
机构信息
Institute of Clinical Medicine, National Yang-Ming University, Taipei, Taiwan.
出版信息
Cell Prolif. 2009 Aug;42(4):461-70. doi: 10.1111/j.1365-2184.2009.00614.x. Epub 2009 May 29.
OBJECTIVES
Somatic stem cells can be obtained from a variety of adult human tissues. However, it was not clear whether human parathyroid glands, which secrete parathyroid hormones and are essential in maintaining homeostasis levels of calcium ions in the circulation, contained stem cells. We aimed to investigate the possibility of isolating such parathyroid-derived stem cells (PDSC).
MATERIALS AND METHODS
Surgically removed parathyroid glands were obtained with informed consent. Cell cytogenetics was used to observe chromosomal abnormalities. Surface phenotypes were characterized by flow cytometry. Telomerase repeat amplification protocol (TRAP) assay was performed to observe the telomerase activity. RT-PCR and real-time PCR was was used to detect gene expressions. Real-time calcium uptake imaging was performed for extent of calcium uptake and transmission electron microscopy and immunofluorecent staining for smooth muscle actin.
RESULTS
After enzymatic digestion and primary culture, plastic-adherent, fibroblast-like cells appeared in culture and a morphologically homogeneous population was derived from subsequent limiting dilution and clonal expansion. Karyotyping was normal and doubling time of clonal cell growth was estimated to be 70.7 +/- 14.5 h (mean +/- standard deviation). The surface phenotype of the cells was positive for CD73, CD166, CD29, CD49a, CD49b, CD49d, CD44, CD105, and MHC class I, and negative for CD34, CD133, CD117, CD114, CD31, CD62P, EGF-R, ICAM-3, CD26, CXCR4, CD106, CD90 and MHC class II, similar to mesenchymal stem cells (MSC). Detectable levels of telomerase activity along with pluripotency Sall4 gene expression were observed from the isolated PDSCs. Expression of calcium-sensing receptor gene along with alpha-smooth muscle actin was induced and cellular uptake of extracellular calcium ions was observed. Furthermore, PDSCs possessed osteogenic, chondrogenic and adipogenic differentiation potentials.
CONCLUSIONS
Our results reveal that PDSCs were similar phenotypically to MSCs and further studies are needed to formulate induction conditions to differentiate PDSCs into parathyroid hormone-secreting chief cells.
目的
体细胞干细胞可从多种成人组织中获取。然而,尚不清楚分泌甲状旁腺激素且对维持循环中钙离子稳态水平至关重要的人类甲状旁腺是否含有干细胞。我们旨在研究分离此类甲状旁腺来源干细胞(PDSC)的可能性。
材料与方法
在获得知情同意后获取手术切除的甲状旁腺。采用细胞遗传学观察染色体异常情况。通过流式细胞术对表面表型进行鉴定。进行端粒酶重复序列扩增法(TRAP)检测以观察端粒酶活性。运用逆转录聚合酶链反应(RT-PCR)和实时聚合酶链反应检测基因表达。进行实时钙摄取成像以观察钙摄取程度,并采用透射电子显微镜和免疫荧光染色检测平滑肌肌动蛋白。
结果
经酶消化和原代培养后,培养物中出现了贴壁的、成纤维细胞样细胞,随后通过有限稀释和克隆扩增获得了形态学上均一的细胞群体。核型分析正常,克隆细胞生长的倍增时间估计为70.7±14.5小时(平均值±标准差)。这些细胞的表面表型对CD73、CD166、CD29、CD49a、CD49b、CD49d、CD44、CD105和MHC I类呈阳性,而对CD34、CD133、CD117、CD114、CD31、CD62P、表皮生长因子受体(EGF-R)、细胞间黏附分子3(ICAM-3)、CD26、CXC趋化因子受体4(CXCR4)、CD106、CD90和MHC II类呈阴性,类似于间充质干细胞(MSC)。从分离的PDSC中观察到可检测水平的端粒酶活性以及多能性Sall4基因表达。诱导了钙敏感受体基因以及α-平滑肌肌动蛋白的表达,并观察到细胞对细胞外钙离子的摄取。此外,PDSC具有成骨、成软骨和成脂分化潜能。
结论
我们的结果表明,PDSC在表型上与MSC相似,需要进一步研究以制定将PDSC分化为分泌甲状旁腺激素的主细胞的诱导条件。
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