水飞蓟素对羊胎骨髓间充质干细胞向成骨谱系分化的影响

I. Morovati, T. Mohammadi, M. Pooyanmehr, L. Soltani
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Then, cells in one of 8 groups 1: negative control; 2: treated with 10 μmol/liter silymarin in the usual environment, 3: treated with 20 μmol/liter silymarin in the usual environment, 4: treated with 100 μmol/liter estradiol in the usual environment, 5: positive control, 6: treatment treated with 10 μmol/liter silymarin in the differentiation medium, 7: treated with 20 μmol/liter silymarin in the differentiation medium, 8: treated with 100 μmol/liter in the differentiation medium, were cultured for 21 days. To determine the osteogenic differentiation of cells, the deposition of hydroxyapatite ions was examined using alizarin staining, and also, the amount of ALP enzyme secretion was also measured in the studied groups. 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引用次数: 0

摘要

间充质干细胞,分化,成骨,水飞蓟素,碱性磷酸酶。目的:利用间充质干细胞(MSCs)进行细胞治疗是一种很有前途的再生医学工具。胚胎骨髓是间充质干细胞最丰富的来源之一。水飞蓟素具有较强的抗氧化和抗炎活性,对某些细胞的增殖和抗骨质疏松具有积极作用。本研究旨在探讨水飞蓟素对绵羊胚胎骨髓间充质干细胞向成骨系分化的影响。材料与方法:从绵羊胚胎骨髓中分离间充质干细胞。采用MTT法研究水飞蓟素在不同浓度作用24和72 h时对细胞的细胞毒性。然后,8组中的1组细胞为阴性对照;2:常规环境下10 μmol/l水飞蓟素处理,3:常规环境下20 μmol/l水飞蓟素处理,4:常规环境下100 μmol/l雌二醇处理,5:阳性对照,6:分化培养基中10 μmol/l水飞蓟素处理,7:分化培养基中20 μmol/l水飞蓟素处理,8:分化培养基中100 μmol/l水飞蓟素处理,培养21 d。采用茜素染色法检测各组细胞羟基磷灰石离子沉积及ALP酶分泌量,以测定细胞成骨分化情况。结果:比较不同浓度处理后24和72小时细胞的平均光吸收表明,使用修正剪切变形理论2先进与智能材料力学学报1(2)(2022)135 - 150与处理24小时的细胞相比,零浓度水飞蓟素处理72小时后细胞的平均光吸收减少。测定各组水飞蓟素治疗21 d后ALP酶分泌水平,以第8组酶分泌水平最高(P≤0.05)。酶分泌量以组1(阴性对照)最低,其次为组2和组3 (P0.05)。茜素红染色结果显示,与分化培养基相关的各组均有钙离子沉积,分别在8、7、6、5组钙离子沉积增多。在常规环境下培养的各组中,1组未见钙化,2、3、4组钙化量分别增加。总的来说,分化环境组的钙化量高于正常环境组。结论:在本实验中,水飞蓟素对绵羊胚胎骨髓间充质干细胞在处理24和72小时后均无毒性作用。它以浓度依赖性的方式增加了细胞向成骨谱系的分化。因此,随着水飞蓟素作用的分子途径的进一步研究和鉴定,水飞蓟素可用于细胞治疗,以修复骨损伤。هرود،تفابولولس13هرامش،2،لاس1401تاحفص،135ات150
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Silymarin Effects on Ovine Fetal Bone Marrow-Derived Mesenchymal Stem Cells Differentiation into Osteogenic Lineage
Mesenchymal stem cells, differentiatio n, osteogenic, silymarin, ALP. Aim: Cell therapy using mesenchymal stem cells (MSCs) can be a promising tool in regenerative medicine. One of the richest sources of mesenchymal stem cells is fetal bone marrow. Silymarin has strong antioxidant and anti-inflammatory activities with a positive effect on the proliferation of some cells as well as antiosteoporosis properties. This study aimed to show the effect of silymarin on the differentiation of mesenchymal stem cells derived from the bone marrow of sheep embryos into the osteogenic line. Materials and Methods: Mesenchymal stem cells were isolated from the bone marrow of sheep embryos. MTT test was performed to investigate the cytotoxicity of silymarin on cells at different concentrations for 24 and 72 hours. Then, cells in one of 8 groups 1: negative control; 2: treated with 10 μmol/liter silymarin in the usual environment, 3: treated with 20 μmol/liter silymarin in the usual environment, 4: treated with 100 μmol/liter estradiol in the usual environment, 5: positive control, 6: treatment treated with 10 μmol/liter silymarin in the differentiation medium, 7: treated with 20 μmol/liter silymarin in the differentiation medium, 8: treated with 100 μmol/liter in the differentiation medium, were cultured for 21 days. To determine the osteogenic differentiation of cells, the deposition of hydroxyapatite ions was examined using alizarin staining, and also, the amount of ALP enzyme secretion was also measured in the studied groups. Results: Comparing the average optical absorption of cells at different concentrations between 24 and 72 hours after treatment showed that the average optical absorption of cells at zero concentration of silymarin after 72 hours of treatment decreased in Piezoelectric Energy Harvesting from Functionally Graded Beams Using Modified Shear Deformation Theories 2 Mechanics of Advanced and Smart Materials Journal 1(2) (2022) 135 – 150 comparison with those treated for 24 hours (P<0.05), but no significant difference was observed in other concentrations (P>0.05). Examining the level of ALP enzyme secretion, 21 days after treatment with silymarin in the studied groups showed that the highest level of enzyme secretion was in group 8 (P≤0.05). The lowest amount of enzyme secretion was observed in group 1 (negative control) and then in group 2 and group 3 respectively (P<0.05). No significant difference was observed between groups 4, 5, and 6 (P>0.05). Based on the alizarin red staining results, calcium ions deposition was observed in all the groups related to the differentiation medium, which increased in groups 8, 7, 6, and 5, respectively. In the groups cultured in the usual environment, there was no calcification in group 1 and the amount of calcification increased in groups 2, 3, and 4, respectively. In total, the amount of calcification in the differentiation environment groups was higher in comparison with the usual environment. Conclusion: During this study, Silymarin had no toxic effect on the mesenchymal stem cells derived from the bone marrow of sheep embryos in the studied concentrations after 24 and 72 hours of treatment. It increased the differentiation of the cells into the osteogenic lineage in a concentration-dependent manner. Therefore, it seems that with further studies and identification of the molecular pathways of silymarin's effect, it can be used in cell therapy in order to repair bone lesions. هرود ،تفاب و لولس 13 هرامش ، 2 ، لاس 1401 تاحفص ، 135 ات 150
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