海南医学
海南醫學
해남의학
Hainan Medical Journal
2015年
18期
2661-2664
,共4页
康银辉%魏波%祝兆波%郭伟雄%王朝军%宋丽君%林颢%李广盛%楚佳奇%曾荣
康銀輝%魏波%祝兆波%郭偉雄%王朝軍%宋麗君%林顥%李廣盛%楚佳奇%曾榮
강은휘%위파%축조파%곽위웅%왕조군%송려군%림호%리엄성%초가기%증영
皮质酮%成骨细胞%基因表达%成骨
皮質酮%成骨細胞%基因錶達%成骨
피질동%성골세포%기인표체%성골
Corticosterone%Osteoblasts%Gene expression%Osteogenesis
目的:探讨皮质酮对离体SD大鼠成骨细胞功能的影响。方法采用多次胶原酶组织消化法获得新生SD大鼠颅骨中的成骨细胞作为研究对象,用倒置显微镜及碱性磷酸酶、钙结节染色观察成骨细胞形态, CCK-8法检测皮质酮对成骨细胞增殖的影响,根据CCK-8结果将SD大鼠成骨细胞分成四组,分别用含不同浓度的皮质酮(0μmol/L、0.1μmol/L、1.0μmol/L、10.0μmol/L)的DMEM(H)培养基培养,作用24 h后,测定成骨细胞内碱性磷酸酶含量,采用RT-PCR检测成骨细胞内COL1A、OCN、ALP基因表达,采用Western blot检测成骨细胞内COL1A、OCN、RUNX-2蛋白的表达。结果 CCK-8结果显示皮质酮能抑制成骨细胞的增殖,皮质酮能抑制成骨细胞内碱性磷酸酶的生成,与浓度明显相关;RT-PCR与Western blot检测可见COL1A、OCN、ALP基因表达及COL1A、OCN、RUNX-2蛋白的表达下降。结论皮质酮在超生理剂量的浓度下能抑制成骨细胞增殖及细胞内碱性磷酸酶的合成,减少COL1A、OCN、ALP基因及COL1A、OCN、RUNX-2蛋白的表达。
目的:探討皮質酮對離體SD大鼠成骨細胞功能的影響。方法採用多次膠原酶組織消化法穫得新生SD大鼠顱骨中的成骨細胞作為研究對象,用倒置顯微鏡及堿性燐痠酶、鈣結節染色觀察成骨細胞形態, CCK-8法檢測皮質酮對成骨細胞增殖的影響,根據CCK-8結果將SD大鼠成骨細胞分成四組,分彆用含不同濃度的皮質酮(0μmol/L、0.1μmol/L、1.0μmol/L、10.0μmol/L)的DMEM(H)培養基培養,作用24 h後,測定成骨細胞內堿性燐痠酶含量,採用RT-PCR檢測成骨細胞內COL1A、OCN、ALP基因錶達,採用Western blot檢測成骨細胞內COL1A、OCN、RUNX-2蛋白的錶達。結果 CCK-8結果顯示皮質酮能抑製成骨細胞的增殖,皮質酮能抑製成骨細胞內堿性燐痠酶的生成,與濃度明顯相關;RT-PCR與Western blot檢測可見COL1A、OCN、ALP基因錶達及COL1A、OCN、RUNX-2蛋白的錶達下降。結論皮質酮在超生理劑量的濃度下能抑製成骨細胞增殖及細胞內堿性燐痠酶的閤成,減少COL1A、OCN、ALP基因及COL1A、OCN、RUNX-2蛋白的錶達。
목적:탐토피질동대리체SD대서성골세포공능적영향。방법채용다차효원매조직소화법획득신생SD대서로골중적성골세포작위연구대상,용도치현미경급감성린산매、개결절염색관찰성골세포형태, CCK-8법검측피질동대성골세포증식적영향,근거CCK-8결과장SD대서성골세포분성사조,분별용함불동농도적피질동(0μmol/L、0.1μmol/L、1.0μmol/L、10.0μmol/L)적DMEM(H)배양기배양,작용24 h후,측정성골세포내감성린산매함량,채용RT-PCR검측성골세포내COL1A、OCN、ALP기인표체,채용Western blot검측성골세포내COL1A、OCN、RUNX-2단백적표체。결과 CCK-8결과현시피질동능억제성골세포적증식,피질동능억제성골세포내감성린산매적생성,여농도명현상관;RT-PCR여Western blot검측가견COL1A、OCN、ALP기인표체급COL1A、OCN、RUNX-2단백적표체하강。결론피질동재초생리제량적농도하능억제성골세포증식급세포내감성린산매적합성,감소COL1A、OCN、ALP기인급COL1A、OCN、RUNX-2단백적표체。
Objective To investigate the effect of different corticosterone concentration on the gene expres-sion of SD rat osteoblasts in vitro. Methods Newborn SD rat osteoblasts in the skull were obtained by many times of collagenase digestion as the object of study. The osteoblastic morphology was observed using inverted microscope, al-kaline phosphatase and calcium nodes dyeing. And the effect of corticosterone concentration on osteoblastic prolifera-tion was detected by CCK-8. According to the scores of CCK-8, the SD rat osteoblasts were divided into four groups with different corticosterone concentrations of DMEM (H) culture (0μmol/L, 0.1μmol/L, 1.0μmol/L, 10.0μmol/L). After 24 hours of DMEM (H) culture, content of osteoblastic alkaline phosphatase were measured, gene expressions of osteoblastic COL1A, OCN, ALP were detected by RT-PCR, and the protein expression of osteoblastic COL1A, OCN, RUNX-2 were measured by western blot. Results The scores of CCK-8 showed that corticosterone can re-strain the proliferation of SD rat osteoblasts and the formation of osteoblastic alkaline phosphatase, which were signifi-cantly related to concentration. And the results of RT-PCR and western blot both showed decreased expression of COL1A, OCN, ALP gene and COL1A, OCN, RUNX-2 protein. Conclusion Corticosterone beyond physical dosage can inhibit the proliferation of osteoblasts and synthesis of intracellular alkaline phosphatase, and reduce the expres-sion of COL1A, OCN, ALP gene and COL1A, OCN, RUNX-2 protein.
