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鲽鱼钙素1刺激大鼠颅骨细胞培养物中的成骨细胞分化。

Stanniocalcin 1 stimulates osteoblast differentiation in rat calvaria cell cultures.

作者信息

Yoshiko Yuji, Maeda Norihiko, Aubin Jane E

机构信息

Department of Oral Growth and Developmental Biology, Hiroshima University Graduate School of Biomedical Sciences, Kasumi 1-2-3, Minami-ku, Hiroshima 734-8553, Japan.

出版信息

Endocrinology. 2003 Sep;144(9):4134-43. doi: 10.1210/en.2003-0130.

DOI:10.1210/en.2003-0130
PMID:12933688
Abstract

Stanniocalcin 1 (STC1) is a mammalian homolog of STC, the fish calcium/phosphate-regulating polypeptide whose functions are only beginning to be elucidated. Recently, we demonstrated that STC1 stimulates, in an autocrine/paracrine fashion, bone mineralization by increasing phosphate uptake in osteoblasts apparently via the functional activity of the sodium-dependent phosphate transporter, Pit1. We have now assessed the role of STC1 on osteoblast development in fetal rat calvaria (RC) cell cultures. STC1 mRNA and protein were differentially expressed over the time course of cultures, and dexamethasone, a potent stimulator of differentiation in this model, shifted peak STC1 expression levels to earlier times. Overexpression [recombinant human (rh) STC1] and underexpression (antisense oligonucleotides) of STC1 accelerated and retarded, respectively, osteogenic development as well as osteopontin and osteocalcin mRNA expression in mature osteoblast cultures, but not osteoprogenitor cell cultures. Dexamethasone shifted the effective doses required for these effects to higher and lower concentrations of antisense oligonucleotides and rhSTC1, respectively. Concomitantly, rhSTC1 increased both sodium-dependent phosphate uptake and Pit1 gene expression in nodule formation stages, but not in primitive progenitor stages of RC cell cultures. Thus, STC1 accelerates osteoblast development in an autocrine/paracrine manner in the RC cell culture model.

摘要

骨钙素1(STC1)是鱼类钙/磷调节多肽STC在哺乳动物中的同源物,其功能才刚刚开始被阐明。最近,我们证明STC1以自分泌/旁分泌方式通过明显经由钠依赖性磷酸盐转运体Pit1的功能活性增加成骨细胞中的磷酸盐摄取来刺激骨矿化。我们现在评估了STC1在胎鼠颅骨(RC)细胞培养物中对成骨细胞发育的作用。在培养过程中,STC1 mRNA和蛋白质表达存在差异,并且在该模型中作为分化强效刺激剂的地塞米松将STC1的峰值表达水平提前。在成熟成骨细胞培养物中,而非成骨祖细胞培养物中,STC1的过表达[重组人(rh)STC1]和低表达(反义寡核苷酸)分别加速和延迟了成骨发育以及骨桥蛋白和骨钙素mRNA的表达。地塞米松分别将这些效应所需的有效剂量转移到更高和更低浓度的反义寡核苷酸和rhSTC1。同时,rhSTC1在RC细胞培养物的结节形成阶段增加了钠依赖性磷酸盐摄取和Pit1基因表达,但在原始祖细胞阶段没有增加。因此,在RC细胞培养模型中,STC1以自分泌/旁分泌方式加速成骨细胞发育。

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