氢化可的松促进小鼠胚胎干细胞来源的定形内胚层向肺泡上皮细胞分化。
Hydrocortisone Promotes Differentiation of Mouse Embryonic Stem Cell-Derived Definitive Endoderm toward Lung Alveolar Epithelial Cells.
作者信息
Mokhber Dezfouli Mohammad Reza, Sadeghian Chaleshtori Sirous, Moradmand Azadeh, Basiri Mohsen, Baharvand Hossein, Tahamtani Yaser
机构信息
Department of Internal Medicine, Faculty of Veterinary Medicine, University of Tehran, Tehran, Iran.
Institute of Biomedical Research, Faculty of Veterinary Medicine, University of Tehran, Tehran, Iran. Electronic Address:
出版信息
Cell J. 2019 Jan;20(4):469-476. doi: 10.22074/cellj.2019.5521. Epub 2018 Aug 1.
OBJECTIVE
The ability to generate lung alveolar epithelial type II (ATII) cells from pluripotent stem cells (PSCs) enables the study of lung development, regenerative medicine, and modeling of lung diseases. The establishment of defined, scalable differentiation methods is a step toward this goal. This study intends to investigate the competency of small molecule induced mouse embryonic stem cell-derived definitive endoderm (mESC-DE) cells towards ATII cells.
MATERIALS AND METHODS
In this experimental study, we designed a two-step differentiation protocol. mESC line Royan B20 (RB20) was induced to differentiate into DE (6 days) and then into ATII cells (9 days) by using an adherent culture method. To induce differentiation, we treated the mESCs for 6 days in serum-free differentiation (SFD) media and induced them with 200 nM small molecule inducer of definitive endoderm 2 (IDE2). For days 7-15 (9 days) of induction, we treated the resultant DE cells with new differentiation media comprised of 100 ng/ml fibroblast growth factor (FGF2) (group F), 0.5 μg/ml hydrocortisone (group H), and A549 conditioned medium (A549 CM) (group CM) in SFD media. Seven different combinations of factors were tested to assess the efficiencies of these factors to promote differentiation. The expressions of DE- and ATII-specific markers were investigated during each differentiation step.
RESULTS
Although both F and H (alone and in combination) promoted differentiation through ATII-like cells, the highest percentage of surfactant protein C (SP-C) expressing cells (~37%) were produced in DE-like cells treated by F+H+CM. Ultrastructural analyses also confirmed the presence of lamellar bodies (LB) in the ATII-like cells.
CONCLUSION
These results suggest that hydrocortisone can be a promoting factor in alveolar fate differentiation of IDE2-induced mESC-DE cells. These cells have potential for drug screening and cell-replacement therapies.
目的
从多能干细胞(PSC)生成肺泡II型上皮细胞(ATII)的能力有助于研究肺发育、再生医学以及肺部疾病建模。建立明确、可扩展的分化方法是朝着这一目标迈出的一步。本研究旨在探究小分子诱导的小鼠胚胎干细胞来源的定形内胚层(mESC-DE)细胞向ATII细胞分化的能力。
材料与方法
在本实验研究中,我们设计了一个两步分化方案。采用贴壁培养方法,将小鼠胚胎干细胞系Royan B20(RB20)诱导分化为定形内胚层(6天),然后再分化为ATII细胞(9天)。为诱导分化,我们在无血清分化(SFD)培养基中对小鼠胚胎干细胞处理6天,并用200 nM定形内胚层2小分子诱导剂(IDE2)诱导。在诱导的第7 - 15天(共9天),我们在SFD培养基中用由100 ng/ml成纤维细胞生长因子(FGF2)(F组)、0.5 μg/ml氢化可的松(H组)和A549条件培养基(A549 CM)(CM组)组成的新分化培养基处理所得的定形内胚层细胞。测试了七种不同的因子组合,以评估这些因子促进分化的效率。在每个分化步骤中研究定形内胚层和ATII特异性标志物的表达。
结果
尽管F和H单独及联合使用均通过类似ATII的细胞促进分化,但在F + H + CM处理的类似定形内胚层细胞中产生的表达表面活性蛋白C(SP - C)的细胞百分比最高(约37%)。超微结构分析也证实了类似ATII的细胞中存在板层小体(LB)。
结论
这些结果表明,氢化可的松可能是IDE2诱导的mESC - DE细胞肺泡命运分化的促进因子。这些细胞具有药物筛选和细胞替代疗法的潜力。
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