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首页> 外文期刊>European Journal of Obstetrics, Gynecology and Reproductive Biology: An International Journal >Routine isolation and expansion late mid trimester amniotic fluid derived mesenchymal stem cells in a cohort of fetuses with congenital diaphragmatic hernia
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Routine isolation and expansion late mid trimester amniotic fluid derived mesenchymal stem cells in a cohort of fetuses with congenital diaphragmatic hernia

机译:例行先天性diaphragm肌疝的胎儿常规分离和扩增中期中期羊水来源的间充质干细胞

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Objective: To assess the feasibility of routine isolation and expansion of amniotic fluid derived mesenchymal stem cells (AF-MSC) in fetuses diagnosed with isolated congenital diaphragmatic hernia (CDH). Study design: Redundant AF samples of fetuses with CDH and normal fetuses were obtained. Cell colonies were mechanically selected for each sample. Proliferation capacity was expressed as population doubling time (PDT). Cell lines were further characterized with flow cytometry, differentiation assays and qRT-PCR (OCT4 and NANOG). After cell labeling with LacZ in vivo tracking was performed after fetal tracheal injection in rabbits. Results: Fourteen consecutive CDH samples (median gestational age (GA) of 32.9 weeks; IQR: 27.8-34.3 weeks) and seven control samples beta0 weeks; IQR: 28.9-34.4 weeks) were obtained. PDT was similar in both groups (45.4h+- 1.9 vs. 52.3h+-3.4;NS). AF-MSCs expressed a typical mesenchymal CD marker profile. Clones could be differentiated in osteogenic, adipogenic and chrondrogenic lineages. Expression of multipotency markers was low in all cell lines. We confirmed the presence of injected cells inside the fetal lung three days after intratracheal injection. Conclusion: Routine isolation and expansion of AF-MSCs in CDH is feasible and cell lines generated were comparable to those of control samples. AF-MSCs from affected fetuses could potentially be used in future stem cell therapy.
机译:目的:评估常规分离和扩增羊水来源的间充质干细胞(AF-MSC)在诊断为先天性diaphragm肌疝(CDH)的胎儿中的可行性。研究设计:获得具有CDH的胎儿和正常胎儿的冗余AF样本。机械选择每个样品的细胞集落。增殖能力表示为人口倍增时间(PDT)。通过流式细胞术,分化测定和qRT-PCR(OCT4和NANOG)进一步表征细胞系。用LacZ标记细胞后,在兔子体内进行胎儿气管注射后进行体内追踪。结果:连续十四个CDH样品(中位胎龄(GA)为32.9周; IQR:27.8-34.3周)和七个对照样品beta0周; IQR:28.9-34.4周)。两组的PDT相似(45.4h±1.9 vs. 52.3h±3.4; NS)。 AF-MSC表达了典型的间充质CD标记物谱。克隆可以在成骨,成脂和成年世系中分化。在所有细胞系中多能性标记物的表达均较低。气管内注射三天后,我们确认胎儿肺内已注射细胞。结论:CDH中AF-MSC的常规分离和扩增是可行的,并且产生的细胞系与对照样品相当。来自受影响胎儿的AF-MSCs可能会在未来的干细胞治疗中使用。

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