中国骨科临床与基础研究杂志
中國骨科臨床與基礎研究雜誌
중국골과림상여기출연구잡지
CHINESE JOURNAL OF CLINICAL AND BASIC ORTHO[AEDIC RESEARCH
2014年
2期
99-104
,共6页
张涛%武肖娜%尹庆水%夏虹%黄华扬%张余%李梅%蓝国波
張濤%武肖娜%尹慶水%夏虹%黃華颺%張餘%李梅%藍國波
장도%무초나%윤경수%하홍%황화양%장여%리매%람국파
镁%合金%生物相容性材料%骨髓间充质干细胞%细胞,培养的%细胞增殖%成骨分化%基因%pH值
鎂%閤金%生物相容性材料%骨髓間充質榦細胞%細胞,培養的%細胞增殖%成骨分化%基因%pH值
미%합금%생물상용성재료%골수간충질간세포%세포,배양적%세포증식%성골분화%기인%pH치
Magnesium%Alloys%Biocompatible materials%Bone marrow mesenchymal stem cells%Cells,cultrued%Cell proliferation%Osteogenic differention%Gene%pH value
目的:探讨镁合金对人骨髓间充质干细胞(BMSCs)增殖及成骨分化的影响。方法抽取人骨BMSCs并予以鉴定;采用AZ31B镁合金浸提液培养人BMSCs 1、3、5、7 d,以普通培养基为对照组,CCK-8法检测细胞增殖活性;应用浸提液培养人BMSCs,诱导分化后检测成骨分化相关基因(COLⅠ、ALP、OPN)的表达。另设置调节pH值AZ31B组(pH-AZ31B组),以观察pH值变化对实验结果的影响。结果 BMSCs表达CD34(-)、CD45(-)、CD44(+)、CD73(+)、CD90(+)、CD105(+)。浸提液培养1、3、5、7 d,AZ31B组细胞相对增殖率低于对照组(P<0.05),毒性评级为2级;对照组和pH-AZ31B组细胞活性较好,两组细胞相对增殖率比较,差异无统计学意义(P >0.05)。AZ31B组COLⅠ基因表达量与对照组比较,差异无统计学意义(P >0.05);AZ31B组ALP基因表达量较低(P<0.05),pH-AZ31B组与对照组无显著差异(P>0.05);AZ31B组OPN基因表达量在诱导分化后6 d、12 d显著高于对照组(P<0.05),pH-AZ31B组与对照组无显著差异(P>0.05)。结论镁合金对BMSCs增殖及成骨分化无不良影响,其影响可能与浸提液pH值的变化有关。
目的:探討鎂閤金對人骨髓間充質榦細胞(BMSCs)增殖及成骨分化的影響。方法抽取人骨BMSCs併予以鑒定;採用AZ31B鎂閤金浸提液培養人BMSCs 1、3、5、7 d,以普通培養基為對照組,CCK-8法檢測細胞增殖活性;應用浸提液培養人BMSCs,誘導分化後檢測成骨分化相關基因(COLⅠ、ALP、OPN)的錶達。另設置調節pH值AZ31B組(pH-AZ31B組),以觀察pH值變化對實驗結果的影響。結果 BMSCs錶達CD34(-)、CD45(-)、CD44(+)、CD73(+)、CD90(+)、CD105(+)。浸提液培養1、3、5、7 d,AZ31B組細胞相對增殖率低于對照組(P<0.05),毒性評級為2級;對照組和pH-AZ31B組細胞活性較好,兩組細胞相對增殖率比較,差異無統計學意義(P >0.05)。AZ31B組COLⅠ基因錶達量與對照組比較,差異無統計學意義(P >0.05);AZ31B組ALP基因錶達量較低(P<0.05),pH-AZ31B組與對照組無顯著差異(P>0.05);AZ31B組OPN基因錶達量在誘導分化後6 d、12 d顯著高于對照組(P<0.05),pH-AZ31B組與對照組無顯著差異(P>0.05)。結論鎂閤金對BMSCs增殖及成骨分化無不良影響,其影響可能與浸提液pH值的變化有關。
목적:탐토미합금대인골수간충질간세포(BMSCs)증식급성골분화적영향。방법추취인골BMSCs병여이감정;채용AZ31B미합금침제액배양인BMSCs 1、3、5、7 d,이보통배양기위대조조,CCK-8법검측세포증식활성;응용침제액배양인BMSCs,유도분화후검측성골분화상관기인(COLⅠ、ALP、OPN)적표체。령설치조절pH치AZ31B조(pH-AZ31B조),이관찰pH치변화대실험결과적영향。결과 BMSCs표체CD34(-)、CD45(-)、CD44(+)、CD73(+)、CD90(+)、CD105(+)。침제액배양1、3、5、7 d,AZ31B조세포상대증식솔저우대조조(P<0.05),독성평급위2급;대조조화pH-AZ31B조세포활성교호,량조세포상대증식솔비교,차이무통계학의의(P >0.05)。AZ31B조COLⅠ기인표체량여대조조비교,차이무통계학의의(P >0.05);AZ31B조ALP기인표체량교저(P<0.05),pH-AZ31B조여대조조무현저차이(P>0.05);AZ31B조OPN기인표체량재유도분화후6 d、12 d현저고우대조조(P<0.05),pH-AZ31B조여대조조무현저차이(P>0.05)。결론미합금대BMSCs증식급성골분화무불량영향,기영향가능여침제액pH치적변화유관。
Objective To investigate the influence of magnesium alloy on the cell proliferation and osteogenic differentiation of human bone marrow mesenchymal stem cells (BMSCs). Methods BMSCs were extracted and identified, then cultured for 1, 3, 5, 7 d in magnesium alloy (AZ31B) leaching liquids, normal culture medium were used as control. Cell proliferation activity was detected by CCK-8 method; Human BMSCs were cultured in the extracts, followed by induction of differentiation, the expression of osteogenic differentiation-related gene (COLⅠ、ALP、OPN) were detected. pH-adjusted AZ31B group (pH-AZ31B) was added to observe the influence of pH value changes on the experimental results. Results BMSCs expressed CD34 (-), CD45(-), CD44 (+), CD73 (+), CD90 (+), CD105 (+). Cell relative growth rate in AZ31B group was lower than that of control group at 1, 3, 5, 7 d after the co-culture with alloy extracts (P <0.05), toxicity in AZ31B group was rated as 2 grade; while cell activities were good in control group as well as in pH-AZ31B group (P >0.05). No statistical difference was found between AZ31B group and control group in COLⅠ gene expression (P >0.05); ALP expression in AZ31B group was relatively low compared with those in pH-AZ31B and control groups, and there was no statistical difference between pH-AZ31B group and control group (P >0.05); OPN gene expression in AZ31B group was significantly higher than control group at 6 and 12 d after differentiation induction (P<0.05), but no statistical difference was found between control group and pH-ZA31B group (P >0.05). Conclusion Magnesium alloy AZ31B do not have adverse effects on cell proliferation and osteogenic differentiation of BMSCs, the effects may be related to the changes of pH value in leaching liquids.