改良差时贴壁法分离培养鉴定小鼠骨髓间充质干细胞和内皮前体细胞

doi:10.16098/j.issn.0529-1356.2015.02.023

解剖学报 ›› 2015, Vol. 46 ›› Issue (2): 282-288.doi: 10.16098/j.issn.0529-1356.2015.02.023

• 技术方法 • 上一篇

改良差时贴壁法分离培养鉴定小鼠骨髓间充质干细胞和内皮前体细胞

冯文磊¹张猛¹印双红²徐芳洁²王艳杰¹陈雪玲²吴向未^1*

1. 石河子大学医学院第一附属医院普外科，新疆石河子 832008; 2. 石河子大学医学院免疫学教研室，新疆石河子 832002

收稿日期:2014-10-29 修回日期:2014-12-01 出版日期:2015-04-06 发布日期:2015-04-06
通讯作者: 吴向未 E-mail:wxwshz@126.com
基金资助:
血管内皮前体细胞调控干细胞巢的实验研究

Isolation, cultivation and identification of mesenchymal stem cells and endothelial progenitor cells from murine bone marrow with a modified differential adhesion method

FENG Wen-lei¹ZHANG Meng¹ YIN Shuang-hong² XU Fang-jie² WANG Yan-jie¹ CHEN Xue-ling² WU Xiang-wei ^1*

1. Department of General Surgery, the First Affiliated Hospital, Shihezi University Medical School, Xinjiang Shihezi 832008, China;2. Department of Immunology, Shihezi University Medical School, Xinjiang Shihezi 832002, China

Received:2014-10-29 Revised:2014-12-01 Online:2015-04-06 Published:2015-04-06
Contact: Xiang-wei WU E-mail:wxwshz@126.com

摘要/Abstract

摘要：

目的探索同时从小鼠骨髓分离培养间充质干细胞(MSCs)与内皮前体细胞(EPCs)及对其鉴定的方法。方法小鼠骨髓细胞经改良差时贴壁法分离，以48h为时间点，48h内贴壁细胞传至3代后行成骨、成软骨、成脂分化诱导实验，流式细胞术（FCM）检测其表面标记；48h后收集未贴壁细胞，传至3代后行血管形成实验，传至5代后行CD31免疫荧光细胞染色实验，FCM检测其表面标记。结果第3代48h内贴壁细胞可诱导分化为骨、软骨和脂肪细胞，FCM 检测Sca-1、CD29、CD45、CD11b 阳性率分别为（98.30±0.75）%,（97.47±1.32）%，（1.87±0.15）%，（1.03±0.71）%；第3代48h后贴壁细胞在基质胶上可形成血管样结构,第5代48h后贴壁细胞特异性表面抗原CD31呈阳性表达，FCM检测CD34、CD133、血管内皮生长因子受体（VEGFR2）阳性率分别为（88.90±1.18）%，（92.73±2.90）%，（87.63±1.79）%。结论采用改良差时贴壁法可同时分离培养扩增小鼠骨髓 MSCs和 EPCs，且简便高效稳定可重复。

关键词: 间充质干细胞, 内皮前体细胞, 骨髓, 改良差时贴壁分离法, 流式细胞术, 小鼠

Abstract:

Objective To establish a method for simultaneously isolating, culturing and identifing of murine mesenchymal stem cells (MSCs) and endothelial progenitor cells (EPCs) from bone marrow. Methods The cells were isolated by a modified differential adhesion method from murine bone marrow and cultured for 48 hours. The primary adherent cells at 48 hours were cultured in LG-DMEM and the non-adhered cells were collected and induced by EGM-2MV complete medium in human fibronectin-coated dishes. Osteogenic, chondrogenic,and adipogenic induced multi-directional differentiation potentials were performed on the primary adherent cells, their immune phenotypes were detected by flow cytometry (FCM).Tube formation experiment on the matrigelin vitro and the expression of specific surface marker CD31 determined by immunofluoresence cell staining were identified for the subsequent adherent cells, and their immune phenotypes were detected by FCM.
Results The passage 3 of the primary adherent cells were identified by induced differentiation into osteoblasts, adipocytes and chondrocytes after induction. The expression levels of Sca-1, CD29, CD45, and CD11b were (98.30±0.75)%, (97.47±1.32 )% , (1.87±0.15)% and (1.03±0.71)% respectively. The passage 3 of the subsequent adherent cells were cultured on Matrigel, which resulted in the formation of tube-like structures.The expression of the passage 5 of the subsequent adherent cells specific surface marker CD31 was positive. The expression levels of CD34, CD133 and vascular endothelial growth factor receptor(VEGFR)2 were (88.90±1.18 )% , (92.73±2.90)%, and (87.63±1.79 )% respectively. Conclusions The modified differential adhesion is an efficient, stable, and replicable method that can simultaneously isolate and amplify mouse bone marrow MSCs and EPCs.

Key words: Mesenchymal stem cells, Endothelial progenitor cells, Bone marrow, Modified differential adhesion method, Cell culture, Flow cytometry, Mouse

冯文磊张猛印双红徐芳洁王艳杰陈雪玲吴向未*. 改良差时贴壁法分离培养鉴定小鼠骨髓间充质干细胞和内皮前体细胞[J]. 解剖学报, 2015, 46(2): 282-288.

FENG Wen-lei ZHANG Meng YIN Shuang-hong XU Fang-jie WANG Yan-jie CHEN Xue-ling WU Xiang-wei*. Isolation, cultivation and identification of mesenchymal stem cells and endothelial progenitor cells from murine bone marrow with a modified differential adhesion method[J]. AAS, 2015, 46(2): 282-288.

参考文献

［1］Laine SK,Hentunen T,Laitala-Leinonen T. Do microRNAs regulate bone marrow stem cell niche physiology［J］.Gene,2012,497(1): 1-9.
［2］Ghannam S，Bouffi C，Djouad F, et al. Immunosuppression by mesenchymal stem cells: mechanisms and clinical applications［J］. Stem Cell Res Ther,2010 ,1(1): 2.
［3］Wu X, Pang L, Lei W, et al. Inhibition of Sca-1 positve skeletal stem cell recruitment by alendronate blunts the anabolic effects of parathyroid hormone on bone remodeling［J］. Cell Stem Cell, 2010,7(5): 571-580.
［4］Abouelfetouh A, Kondoh T, Ehara K, et al. Morphological differentiation of bone marrow stromal cells into neuron like cells after co-culture with hippocampal slice［J］. Brain Res, 2004,1029(1):114-119.
［5］Sasaki M, Abe R, Fujita Y, et al. Mesenchymal stem cells are recruited into wounded skin and contribute to wound repair by transdifferentiation into multiple skin cell type［J］. Immunol, 2008,180(4):2581-2587.
［6］Chivu M, Dima SO, Stancu CI, et al. In vitro hepatic differentiation of human bone marrow mesenchymal stem cells under differential exposure to liver-specific factors［J］.Transl Res, 2009,154(3):122-132.
［7］Yan X, Lv A, Xing Y, et al. Inhibition of p53-p21 pathway promotes the differentiation of rat bone marrow mesenchymal stem cells into cardiomyocytes［J］. Mol Cell Biochem,2011, 354(1-2):21-28.
［8］Asahara T, Murohara T, Sullivan A, et al.Isolation of putative progenitor endothelial cells for angiogenesis［J］. Science,1997,275(5302):964-967.
［9］Peichev M, Naiyer AJ, Pereira D, et al.Expression of VEGFR-2 and AC 133 by circulating human CD34(+) cells identifies a population of functional endothelial precursors ［J］. Blood,2000,95(3):952-958. 
［10］Hill JM, Zalos G, Halcox JP,et al. Circulating endothelial progenitor cells, vascular function, and cardiovascular risk［J］. N Engl J Med,2003,348(7):593-600.
［11］Friedenstein AJ, Gorskaja JF, Kulagina NN. Fibroblast precursors in normal and irradiatedm ouse hematopoietic organs［ J］. Exp Hematol, 1976, 4(5) : 267-274.
［12］Asahara T, Masuda H, Takahashi T, et al. Bone marrow origin of endothelial progenitor cells responsible for postnatal vasculogenesis in physiological and pathological neovascularization［J］. Circ Res, 1999(3);85:221-228.
［13］Tongers J, Roncalli JG, Losordo DW. Role of endothelial progenitor cells during ischemia-induced vasculogenesis and collateral formation ［J］. Microvasc Res, 2010,79(3):200-206.
［14］Morikawa S，Mabuchi Y，Kubota Y，et al.Prospective identification，isolation and systemic transplantation of multipotent mesenchymal stem cells in murine bone marrow［J］.Exp Med，2009，206（11):2483-2496.
［15］Palladino M, Gatto l, Neri V, et al. Combined therapy with sonic hedgehog gene transfer and bone marrow-derived endothelial progenitor cells enhances angiogenesis and myogenesis in the ischemic skeletal muscle［J］. J Vasc Res, 2012,49(5):425-431.
［16］Kagami H, Agata H, Tojo A. Bone marrow stromal cells (bone marrow-derived multipotent mesenchymal stromal cells) for bone tissue engineering: basic science to clinical translation［J］. Int J Biochem Cell Biol, 2011,43(3):286-289.
［17］Song ZhSh, Bai ShL, Pan F,et al.Compatibility study of bone mesenchymal stem cells and ferulic acid treatment PHBV film in vitro［J］.Acta Anatomica Sinica, 2014,45(1):47-52.(in Chinese)
宋章硕,柏树令,潘峰,等.骨髓间充质干细胞与阿魏酸处理的PHBV膜的体外相容性［J］.解剖学报, 2014,45(1):47-52.
［18］Casamassimi A, Balestrieri ML, Fiorito C, et al. Comparison between total endothelial progenitor cell isolation versus enriched CD133+culture［J］. J Biochem, 2007,141(4):503-511.
［19］Lee JW，Gupta N，Serikov V，et al. Potential application of mesenchymal stem cells in acute lung injury［J］. Expert Opin Biol Ther,2009, 9(10) : 1259-1270.
［20］Sen S，McDonald S，Coates P，et al. Endothelial progenitor cells: novel biomarker andpromising cell therapy for cardiovascular disease［J］. Clin Science，2011，120（7）: 263-283.
［21］Navarro-Sobrino M,Hernández-Guillamon M,Fernandez-Cadenas I,et al.The angiogenic gene profile of circulating endothelial progenitor cells from ischemic stroke patients［J］.Vasc cell,2013,5(1):3.
［22］Li Q, Wang Z. Influence of mesenchymal stem cells with endothelial progenitor cells in co-culture on osteogenesis and angiogenesis: an in vitro study［J］.Arch Med Res ,2013 ,44(7):504-513.
［23］Barber CL, Iruela-Arispe ML. The ever-elusive endothelial progenitor cell: identities, functions and clinical implications［J］. Pediatr Res, 2006,59(4Pt 2):26R-32R.

[1]	赵卫明李晓余国营王改平常翠芳 . 丝氨酸肽酶抑制因子Kazal型1对肝癌细胞增殖的影响及其机制 [J]. 解剖学报, 2023, 54(6): 695-702.
[2]	何可可李远迪文廷浩朱婕高杰胡蓉韩锋苏敏. 红细胞膜相关蛋白通过IL-6/STAT3/ROR-γt 信号通路抑制小鼠实验性自身免疫性脑脊髓炎中Th17细胞分化[J]. 解剖学报, 2023, 54(5): 538-545.
[3]	李薇王丽汪志华刘庆春韩荣胜 . 长链非编码RNA alpha-2-巨球蛋白反义RNA 1靶向微小RNA-106b-5p调控氧化型低密度脂蛋白诱导的人脑微血管内皮细胞损伤[J]. 解剖学报, 2023, 54(3): 319-327.
[4]	谢秋敏孙艳婷许皓刘蕙文易勤谭彬田杰朱静. 低氧低糖及血清剥夺联合处理抑制Nrf2信号通路诱发大鼠骨髓间充质干细胞氧化应激和凋亡[J]. 解剖学报, 2023, 54(3): 305-312.
[5]	孙孟坊程一升王丰金孟浩汪德秀. 佛手苷内酯通过调控长链非编码RNA 阿片样受体基因表达对糖氧剥夺诱导的PC12细胞损伤的影响[J]. 解剖学报, 2023, 54(1): 56-62.
[6]	张春博王改平王子慧臧夏炎薛奇杰林凯琳韩璐王棋文徐存拴. 大鼠肝再生的肝脏炎症反应中骨髓瘤基因mRNA、微小RNA-540-3p、环状RNA_04996的表达变化与作用[J]. 解剖学报, 2023, 54(1): 70-74.
[7]	张雅群付丽任译延乔妍梓赵冬梅. 大鼠脂肪间充质干细胞的分离、培养及其向少突胶质前体细胞的诱导分化[J]. 解剖学报, 2022, 53(5): 557-562.
[8]	李薇王丽汪志华刘庆春韩荣胜. 长链非编码RNA 细胞骨架调节RNA靶向微小RNA-1246对帕金森病模型细胞损伤的保护作用[J]. 解剖学报, 2022, 53(5): 563-570.
[9]	蔡梅芝卢宝全吴秀玲石佳马有权. 长链非编码RNA 核富集转录本1通过靶向微小RNA-761对缺氧/复氧大鼠星形胶质细胞损伤的影响[J]. 解剖学报, 2022, 53(5): 571-577.
[10]	秦阳阳许龙飞王琪韩晶洪艳. 骨髓间充质干细胞来源的外泌体对小鼠肝库普弗细胞极化的影响[J]. 解剖学报, 2022, 53(4): 447-452.
[11]	宋慧芳谈佳音刘阳张卫国郭蕊 . 低氧预处理通过激活低氧诱导因子1α增强老年人骨髓间充质干细胞促血管新生能力#br# #br# [J]. 解剖学报, 2022, 53(1): 35-41.
[12]	李永涛姜杨孙石柱王璐璐刘丹阳刘娜张晓东沈雷. 基于网络药理学探讨趋化因子-13对间充质干细胞增殖和迁移的影响[J]. 解剖学报, 2021, 52(6): 889-900.
[13]	高飞张欣欣杨冰陈素枝杨凤文檀淼檀金川. 微小RNA-193a调控Wilms瘤基因1促进小鼠糖尿病肾病足细胞凋亡[J]. 解剖学报, 2021, 52(5): 728-736.
[14]	李威周鑫谢志艳张天乐杨惠曹文宇刘志文曾佳玉. 自主跑轮运动通过促进海马神经发生改善甲醛所致小鼠的负性情绪[J]. 解剖学报, 2021, 52(5): 686-691.
[15]	林宝勇徐进超应涵韬蒋欣刘焕彩王箐王巧真陈燕春. DEAD-box RNA解旋酶5和转录因子12与肌萎缩侧索硬化症的关系[J]. 解剖学报, 2021, 52(5): 698-705.

改良差时贴壁法分离培养鉴定小鼠骨髓间充质干细胞和内皮前体细胞

Isolation, cultivation and identification of mesenchymal stem cells and endothelial progenitor cells from murine bone marrow with a modified differential adhesion method

可视化

摘要/Abstract

引用本文

使用本文

参考文献

相关文章 15

编辑推荐

Metrics

本文评价