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首页> 外文期刊>Hormone and Metabolic Research >Modifying RANKL/OPG mRNA expression in differentiating and growing human primary osteoblasts.
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Modifying RANKL/OPG mRNA expression in differentiating and growing human primary osteoblasts.

机译:在分化和生长的人类原代成骨细胞中修饰RANKL / OPG mRNA表达。

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The OPG/RANKL system in primary cultures of human osteoblasts has been studied by different authors. However, very few studies have been performed on gene expression of RANKL and OPG at different stages of maturation on human osteoblast cultures. The effect of 17- beta-estradiol and 1,25dihydroxyvitamin D3 on the OPG/RANKL system is not known during the different states of cellular maturation. In this work we quantified OPG and RANKL protein levels (ELISA) and the mRNA of OPG, RANKL, collagen type I, alkaline phosphatase, and osteocalcin (semi-quantitative RT-PCR) in human osteoblasts. We analyzed these in basal conditions and after incubation with 17- beta-estradiol and 1,25dihydroxyvitamin D3 in the first and second phases. We found that OPG secretion and expression levels increased throughout cellular growth. RANKL proteins were detected only in the first stage, and the expression increased throughout the first phase. Thus, the RANKL/OPG ratio was higher in immature osteoblasts than in mature osteoblasts. The evolution of RANKL gene expression was related to collagen I and alkaline phosphatase, while OPG was related to osteocalcin. We observed no modifications after estradiol and 1,25dihydroxyvitamin D3 treatment. Our results suggest that the OB is a positive stimulator at precocious stages of differentiation on osteoclastogenic modulates.
机译:不同作者已经研究了人类成骨细胞原代培养物中的OPG / RANKL系统。然而,关于成骨细胞培养的不同成熟阶段的RANKL和OPG基因表达的研究很少。在细胞成熟的不同状态期间,尚不了解17-β-雌二醇和1,25-二羟基维生素D3对OPG / RANKL系统的作用。在这项工作中,我们定量了人类成骨细胞中OPG和RANKL的蛋白水平(ELISA)以及OPG,RANKL,I型胶原,碱性磷酸酶和骨钙素的mRNA(半定量RT-PCR)。我们在基础条件下以及与第一阶段和第二阶段与17-β-雌二醇和1,25二羟基维生素D3孵育后对这些物质进行了分析。我们发现OPG的分泌和表达水平在整个细胞生长过程中都增加了。 RANKL蛋白仅在第一阶段被检测到,表达在整个第一阶段均增加。因此,未成熟成骨细胞中的RANKL / OPG比要高于成熟成骨细胞。 RANKL基因表达的进化与胶原蛋白I和碱性磷酸酶有关,而OPG与骨钙蛋白有关。我们观察到雌二醇和1,25二羟基维生素D3处理后没有任何改变。我们的结果表明,在破骨细胞生成调节的早熟阶段,OB是一种积极刺激剂。

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