脐带间充质干细胞移植对免疫性卵巢早衰的影响

目的探讨脐带间充质干细胞(UCMSCs)移植对自身免疫性卵巢早衰小鼠卵巢结构、功能的影响。方法以透明带3(ZP3)作为免疫原建立小鼠自身免疫性卵巢早衰动物模型。实验分为4组:空白对照组、模型组、实验对照组及移植组。空白对照组不注射ZP3及UCMSCs;模型组建立动物模型,不予移植;实验对照组建模后,双卵巢内注射生理盐水;移植组在建模成功即予每侧卵巢约注射1×106个UCMSCs。于移植后15、30、45及60 d分批处死小鼠,收集血标本检测性激素[雌二醇(E2)、卵泡刺激素(FSH)]浓度;留取卵巢标本,荧光显微镜下观察有无绿色荧光及其分布,计数卵泡数目。结果 UCMSCs移植后15 d,移植组卵巢组织内可见到绿色荧光,且持续至移植后2个月。绿色荧光主要分布在卵巢的间质组织,而卵泡内则见不到绿色荧光的分布。移植组部分小鼠恢复正常的动情周期。移植后各个时间点内,移植组E2浓度高于模型组及实验对照组,FSH浓度则降低。移植45、60 d时,移植组的各级卵泡数目均高于模型组及实验对照组,但低于空白对照组。结论 UCMSCs可以在透明带抗原免疫损伤的小鼠卵巢组织内存活并迁移,但其分化为卵泡组分的可能性较小。UCMSCs移植可修复透明带免疫损伤的卵巢组织,从而部分改善其内分泌功能。

人脐带与骨髓来源间充质干细胞miRNA的差异表达

采用基因芯片技术检测了人脐带与骨髓两种不同来源间充质干细胞中miRNA的表达.结果表明:有26个miRNA差异表达,其中miR-29b、miR-20a、miR-31、miR-20b及miR-106a在人脐带间充质干细胞(UMSCs)中表达显著上调,差异倍数均高于3,miR-138则表达下调.在此基础上,采用实时荧光定量PCR技术对差异性显著的6个miRNA进行验证,检测结果一致.最后对特异性基因进行靶点预测,发现靶基因与mRNA转录、翻译以及细胞增殖、分裂、信号转导等功能相关.

Comparison of human amniotic fluid-derived and umbilical cord Wharton＇s Jelly-derived mesenchymal stromal cells： Characterization and myocardial differentiation capacity

Objective To compare the characterization and myocardial differentiation capacity of arnniotic fluid-derived mesenchymal stromal cells （AF MSCs） and umbilical cord Wharton＇s Jelly-derived mesenchymal stromal cells （WJ MSCs）. Methods The human AF MSCs were cultured from amniotic fluid samples obtained by amniocentesis. The umbilical cord WJ MSCs were obtained from Wharton＇s Jelly of umbilical cords of infants delivered full-term by normal labor. The morphology, growth curves, and analyses by flow cytometry of cell surface markers were compared between the two types of cells. Myocardial genes （GATA-4, c-TnT, a-actin, and Cx43） were detected by real-time PCR and the corresponding protein expressions were detected by Western blot analysis after myocardial induced in AF MSCs and WJ MSCs. Results Our findings revealed AF MSCs and WJ MSCs shared similar morphological characteristics of the fibroblastoid shape. The AF MSCs were easily obtained than the WJ MSCs and had a shorter time to reach adherence of 2.7 ± 1.6 days to WJ MSCs of 6.5 ± 1.8 days. The growth curves by MTT cytotoxic assay showed the AF MSCs had a similar proliferative capacity at passage 5 and passage 10. However, the proliferative capacities ofWJ MSCs were decreased at 5 passage relative to 10 passage. Both AF stem cells and WJ stem cells had the characteristics of mesenchymal stromal cells with some characteristics of embryonic stem cells. They express CD29 and CD105, but not CD34. They were positive for Class I major histocompatibility （MHC I） antigens （HLA-ABC）, and were negative, or mildly positive, for MHC Class II （HLA-DR） antigen. Oct-4 was positive in all the two cells types. Both AF MSCs and WJ MSCs could differentiate along myocardium. The differentiation capacities were detected by the expression of GATA-4, c-TnT, a-actin, Cx43 after myocardial induction. Conclusions Both AF MSCs and WJ MSCs have the potential clinical application for myogenesis in cardiac regenerative therapy.