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完全定义的成脂分化 ASC 与微血管内皮细胞共培养。

Completely defined co-culture of adipogenic differentiated ASCs and microvascular endothelial cells.

机构信息

Reutlingen University, Reutlingen, Germany.

University of Hohenheim, Stuttgart, Germany.

出版信息

ALTEX. 2018;35(4):464-476. doi: 10.14573/altex.1802191. Epub 2018 Jun 13.

DOI:10.14573/altex.1802191
PMID:29901210
Abstract

Vascularized adipose tissue models are highly demanded as alternative to existing animal models to elucidate the mechanisms of widespread diseases, screen for new drugs or asses corresponding safety levels. Standardly used animal-derived sera therein, are associated to ethical concerns, the risk of contaminations and many uncertainties in their composition and impact on cells. Therefore their use should be completely omitted. In this study we developed a serum-free, defined co-culture medium and implemented it to set up an adipocyte-endothelial cell (EC) co-culture model. Human adipose-derived stem cells were differentiated under defined conditions (diffASCs) and, like human microvascular ECs (mvECs), cultured in a developed defined co-culture medium in mono-, indirect or direct co-culture for 14 days. The developed defined co-culture medium was superior to compared mono-culture media and facilitated the functional maintenance and maturation of diffASCs including perilipin A expression, lipid accumulation and glycerol and leptin release. The medium equally allowed mvEC maintenance, confirmed by the expression of CD31 and vWF and acLDL uptake. Thereby mvECs showed a strong dependency on EC-specific factors. Additionally the development of vascular structures by mvECs was facilitated when directly co-cultured with diffASCs. The completely defined co-culture system allows for the serum-free setup of adipocyte/EC co-cultures and thereby represents a valuable and ethically acceptable tool for the setup of vascularized adipose tissue models.

摘要

血管化脂肪组织模型作为现有动物模型的替代品,被广泛应用于阐明广泛疾病的机制、筛选新药或评估相应的安全水平。标准的动物来源血清存在伦理问题、污染风险以及其成分和对细胞的影响存在许多不确定性,因此应完全避免使用。在这项研究中,我们开发了一种无血清、定义明确的共培养培养基,并将其用于建立脂肪细胞-内皮细胞(EC)共培养模型。人脂肪来源干细胞在定义条件下分化(diffASCs),并像人微血管内皮细胞(mvECs)一样,在开发的定义共培养培养基中进行单核、间接或直接共培养 14 天。与比较的单核培养物相比,开发的定义明确的共培养培养基更优越,并促进了 diffASCs 的功能维持和成熟,包括 perilipin A 表达、脂质积累以及甘油和瘦素的释放。该培养基同样允许 mvEC 的维持,这通过 CD31 和 vWF 的表达以及 acLDL 的摄取得到证实。mvEC 强烈依赖于 EC 特异性因子。此外,当与 diffASCs 直接共培养时,mvECs 有助于血管结构的形成。完全定义的共培养系统允许无血清设置脂肪细胞/EC 共培养,因此代表了一种有价值且符合伦理的工具,可用于建立血管化脂肪组织模型。

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