van der Meijden K, Buskermolen J, van Essen H W, Schuurman T, Steegenga W T, Brouwer-Brolsma E M, Langenbach G E J, van Ruijven L J, den Heijer M, Lips P, Bravenboer N
Department of Endocrinology/Internal Medicine, VU University Medical Center, MOVE Research Institute, Amsterdam, The Netherlands.
Department of Clinical Chemistry, VU University Medical Center, Research Institute MOVE, Amsterdam, The Netherlands.
J Steroid Biochem Mol Biol. 2016 Nov;164:344-352. doi: 10.1016/j.jsbmb.2015.09.004. Epub 2015 Sep 7.
Animal models show that vitamin D deficiency may have severe consequences for skeletal health. However, most studies have been performed in young rodents for a relatively short period, while in older adult rodents the effects of long-term vitamin D deficiency on skeletal health have not been extensively studied. Therefore, the first aim of this study was to determine the effects of long-term vitamin D deficiency on bone structure, remodeling and mineralization in bones from older adult mice. The second aim was to determine the effects of long-term vitamin D deficiency on mRNA levels of genes involved in vitamin D metabolism in bones from older adult mice. Ten months old male C57BL/6 mice were fed a diet containing 0.5% calcium, 0.2% phosphate and 0 (n=8) or 1 (n=9) IU vitamin D/gram for 14 months. At an age of 24 months, mice were sacrificed for histomorphometric and micro-computed tomography (micro-CT) analysis of humeri as well as analysis of CYP27B1, CYP24 and VDR mRNA levels in tibiae and kidneys using RT-qPCR. Plasma samples, obtained at 17 and 24 months of age, were used for measurements of 25-hydroxyvitamin D (25(OH)D) (all samples), phosphate and parathyroid hormone (PTH) (terminal samples) concentrations. At the age of 17 and 24 months, mean plasma 25(OH)D concentrations were below the detection limit (<4nmol/L) in mice receiving vitamin D deficient diets. Plasma phosphate and PTH concentrations did not differ between both groups. Micro-CT and histomorphometric analysis of bone mineral density, structure and remodeling did not reveal differences between control and vitamin D deficient mice. Long-term vitamin D deficiency did also not affect CYP27B1 mRNA levels in tibiae, while CYP24 mRNA levels in tibiae were below the detection threshold in both groups. VDR mRNA levels in tibiae from vitamin D deficient mice were 0.7 fold lower than those in control mice. In conclusion, long-term vitamin D deficiency in older adult C57BL/6 mice, accompanied by normal plasma PTH and phosphate concentrations, does not affect bone structure, remodeling and mineralization. In bone, expression levels of CYP27B1 are also not affected by long-term vitamin D deficiency in older adult C57BL/6 mice. Our results suggest that mice at old age have a low or absent response to vitamin D deficiency probably due to factors such as a decreased bone formation rate or a reduced response of bone cells to 25(OH)D and 1,25(OH)D. Older adult mice may therefore be less useful for the study of the effects of vitamin D deficiency on bone health in older people.
动物模型表明,维生素D缺乏可能对骨骼健康产生严重后果。然而,大多数研究是在年轻啮齿动物中进行的,时间相对较短,而在成年老龄啮齿动物中,长期维生素D缺乏对骨骼健康的影响尚未得到广泛研究。因此,本研究的首要目的是确定长期维生素D缺乏对成年老龄小鼠骨骼结构、重塑和矿化的影响。第二个目的是确定长期维生素D缺乏对成年老龄小鼠骨骼中参与维生素D代谢的基因mRNA水平的影响。将10月龄雄性C57BL/6小鼠喂食含0.5%钙、0.2%磷且每克含0(n = 8)或1(n = 9)国际单位维生素D的饲料,持续14个月。在24月龄时,处死小鼠以对肱骨进行组织形态计量学和微计算机断层扫描(micro-CT)分析,并使用RT-qPCR分析胫骨和肾脏中CYP27B1、CYP24和VDR mRNA水平。在17和24月龄时采集的血浆样本用于测量25-羟基维生素D(25(OH)D)(所有样本)、磷酸盐和甲状旁腺激素(PTH)(末期样本)浓度。在17和24月龄时,接受维生素D缺乏饲料的小鼠血浆25(OH)D平均浓度低于检测限(<4nmol/L)。两组之间血浆磷酸盐和PTH浓度无差异。对骨矿物质密度、结构和重塑的微CT和组织形态计量学分析未发现对照组和维生素D缺乏小鼠之间存在差异。长期维生素D缺乏也未影响胫骨中CYP27B1 mRNA水平,而两组胫骨中CYP24 mRNA水平均低于检测阈值。维生素D缺乏小鼠胫骨中的VDR mRNA水平比对照小鼠低0.7倍。总之,成年老龄C57BL/6小鼠长期维生素D缺乏,同时血浆PTH和磷酸盐浓度正常,并不影响骨骼结构、重塑和矿化。在骨骼中,成年老龄C57BL/6小鼠长期维生素D缺乏也不影响CYP27B1的表达水平。我们的结果表明,老年小鼠对维生素D缺乏的反应较低或无反应,可能是由于诸如骨形成率降低或骨细胞对25(OH)D和1,25(OH)D反应减弱等因素。因此,成年老龄小鼠可能不太适用于研究维生素D缺乏对老年人骨骼健康的影响。
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