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在体外,唑来膦酸处理的钙化表面会影响破骨细胞而非成骨细胞。

Osteoclasts but not osteoblasts are affected by a calcified surface treated with zoledronic acid in vitro.

作者信息

Schindeler Aaron, Little David G

机构信息

Department of Orthopaedic Research and Biotechnology, The Children's Hospital at Westmead, Sydney, Australia.

出版信息

Biochem Biophys Res Commun. 2005 Dec 16;338(2):710-6. doi: 10.1016/j.bbrc.2005.09.198. Epub 2005 Oct 11.

DOI:10.1016/j.bbrc.2005.09.198
PMID:16243296
Abstract

Bisphosphonates are potent inhibitors of osteoclast-mediated bone resorption. Recent interest has centered on the effects of bisphosphonates on osteoblasts. Chronic dosing of osteoblasts with solubilized bisphosphonates has been reported to enhance osteogenesis and mineralization in vitro. However, this methodology poorly reflects the in vivo situation, where free bisphosphonate becomes rapidly bound to mineralized bone surfaces. To establish a more clinically relevant cell culture model, we cultured bone cells on calcium phosphate coated quartz discs pre-treated with the potent nitrogen-containing bisphosphonate, zoledronic acid (ZA). Binding studies utilizing [(14)C]-labeled ZA confirmed that the bisphosphonate bound in a concentration-dependent manner over the 1-50microM dose range. When grown on ZA-treated discs, the viability of bone-marrow derived osteoclasts was greatly reduced, while the viability and mineralization of the osteoblastic MC3T3-E1 cell line were largely unaffected. This suggests that only bone resorbing cells are affected by bound bisphosphonate. However, this system does not account for transient exposure to unbound bisphosphonate in the hours following a clinical dosing. To model this event, we transiently treated osteoblasts with ZA in the absence of a calcified surface. Osteoblasts proved highly resistant to all transitory treatment regimes, even when utilizing ZA concentrations that prevented mineralization and/or induced cell death when dosed chronically. This study represents a pharmacologically more relevant approach to modeling bisphosphonate treatment on cultured bone cells and implies that bisphosphonate therapies may not directly affect osteoblasts at bone surfaces.

摘要

双膦酸盐是破骨细胞介导的骨吸收的强效抑制剂。最近的研究兴趣集中在双膦酸盐对成骨细胞的影响上。据报道,用可溶解的双膦酸盐对成骨细胞进行长期给药可在体外增强骨生成和矿化。然而,这种方法很难反映体内情况,因为游离双膦酸盐会迅速与矿化骨表面结合。为了建立一个更符合临床实际的细胞培养模型,我们将骨细胞培养在预先用强效含氮双膦酸盐唑来膦酸(ZA)处理过的磷酸钙包被的石英盘上。利用[¹⁴C]标记的ZA进行的结合研究证实,双膦酸盐在1-50μM的剂量范围内以浓度依赖的方式结合。当在ZA处理过的盘上生长时,骨髓来源的破骨细胞的活力大大降低,而成骨细胞系MC3T3-E1的活力和矿化在很大程度上不受影响。这表明只有骨吸收细胞受到结合型双膦酸盐的影响。然而,这个系统没有考虑到临床给药后数小时内未结合双膦酸盐的短暂暴露。为了模拟这一情况,我们在没有钙化表面的情况下用ZA短暂处理成骨细胞。结果证明,成骨细胞对所有短暂处理方案都具有高度抗性,即使使用的ZA浓度在长期给药时会阻止矿化和/或诱导细胞死亡。这项研究代表了一种在培养的骨细胞上模拟双膦酸盐治疗的药理学上更相关的方法,并暗示双膦酸盐疗法可能不会直接影响骨表面的成骨细胞。

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