中国组织工程研究

中国组织工程研究 ›› 2012, Vol. 16 ›› Issue (45): 8394-8397.doi: 10.3969/j.issn.2095-4344.2012.45.007

• 骨髓干细胞 bone marrow stem cells • 上一篇    下一篇

一种改良人骨髓间充质干细胞分离培养的方法

刘继春1,胡红涛2,许国华2,蒋玉权2,徐 宁2,叶晓健2   

  1. 1解放军第184医院骨科,江西省鹰潭市 335000
    2解放军第二军医大学附属长征医院骨科,上海市 200003
  • 收稿日期:2012-03-19 修回日期:2012-07-15 出版日期:2012-11-04 发布日期:2012-11-04
  • 通讯作者: 叶晓健,教授,博士生导师,解放军第二军医大学附属长征医院骨科,上海市 200003 yexj2002@163.com
  • 作者简介:刘继春★,男,1983年生,安徽省淮北市人,汉族, 2012年解放军第二军医大学毕业,硕士,医师,主要从事脊柱外科研究。 3-9-8-1@163.com

A modified method of isolating and culturing human bone marrow mesenchymal stem cells

Liu Ji-chun1, Hu Hong-tao2, Xu Guo-hua2, Jiang Yu-quan2, Xu Ning2, Ye Xiao-jian2   

  • Received:2012-03-19 Revised:2012-07-15 Online:2012-11-04 Published:2012-11-04
  • Contact: Ye Xiao-jian, Professor, Doctoral supervisor, Department of Orthopedics, Changzheng Hospital of Second Military Medical University, Shanghai 200003, China yexj2002@163.com
  • About author:Liu Ji-chun★, Master, Physician, Department of Orthopedics, the 184 Hospital of Chinese PLA, Yingtan 335000, Jiangxi Province, China 3-9-8-1@163.com

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摘要:

背景:分离培养鼠、兔骨髓间充质干细胞的科研实践较多,而组织工程临床实践大多以同种属种子细胞的科研为基础。
目的:建立一种稳定、高效,满足临床和实验室需要的人骨髓间充质干细胞分离培养方法。
方法:使用骨穿针于人髂前上棘处抽取骨髓和松质骨,用15 mL培养体系冲洗松质骨并收集冲洗液,采用直接培养法,利用细胞贴壁性能初筛细胞;流式细胞仪检测细胞表面抗原(CD29、CD34、CD44、CD45、CD105),分别进行成骨、成脂肪诱导分化,在诱导过程中进行细胞形态学观察对干细胞进行初步鉴定。
结果与结论:松质骨冲洗液直接培养法在培养第5天的时候出现细胞集落,细胞稳定表达CD29、CD44、CD105,不表达CD34、CD45。成骨诱导20 d后出现明显钙结节,茜素红染色呈红色结节。成脂诱导7 d后脂滴明显形成,油红素O染色见大量脂质沉淀。结果可见采用松质骨冲洗液直接培养法可以从人松质骨中短时间内获得大量间充质干细胞,其具有良好的细胞形态,稳定表达的细胞抗原及成骨、成脂分化能力。

关键词: 松质骨, 骨髓间充质干细胞, 分离, 培养, 鉴定, 成骨分化, 成脂肪分化, 干细胞

Abstract:

BACKGROUND: Experiments for the isolation and culture of rat or rabbit bone marrow mesenchymal stem cells are more common, but the clinical experiments of tissue engineering are often on the basis of the seed cells of the same species.
OBJECTIVE: To establish a protocol for isolating and culturing human bone marrow mesenchymal stem cells which is stable and efficient and consistent with the needs of clinical and laboratory experiments.
METHODS: Bone marrow and spongy bone were obtained from the human anterior superior iliac spine, and then the bone marrow, the spongy bone was flushed by 15 mL culture medium and then the rinse solution was collected. The cells were primary screened on the basis of adhesion function by direct cultivation method; the surface antigens, including CD29, CD34, CD44, CD45 and CD105 were detected by flow cytometry. Bone marrow mesenchymal stem cells were differentiated into osteoblasts and adipocytes, and the differentiated mesenchymal stem cells were identified by morphological observation.
RESULTS AND CONCLUSION: Cell colony could be seen at 5 days after cultured with spongy bone washing liquid. These cells were uniformly negative for CD34, CD45 and positive for CD29, CD44 and CD105. Calcium nodules were observed after osteogenic induction for 20 days and positive for alizarin red staining. The lipid droplets could be seen after adipogenic induction for 7 days and oil red O staining showed a large number of lipid deposition. The study shows that a large amount of mesenchymal stem cells can be isolated and cultured from adult human spongy bone in short time by direct cultivation methods, and the mesenchymal stem cells are uniform in morphology, the cells can express the antigens stably and differentiate into osteoblasts and adipocytes.

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