Pu Yong, Veiga-Lopez Almudena
Department of Animal Science, Michigan State University, 474 S. Shaw Lane Rm 1230 F, East Lansing, MI 48824 USA.
Cell Mol Biol Lett. 2017 Mar 23;22:6. doi: 10.1186/s11658-017-0037-1. eCollection 2017.
Although the 3T3-L1 preadipocyte cell line represents an informative model for adipogenesis research, primary cultured cells are often needed to understand particular human or animal metabolic phenotypes. As demonstrated by cultured preadipocytes from large mammalian species, primary cultured cells require specific adipogenic differentiation conditions different to that of the 3T3-L1 cell line. These conditions are also species-specific and require optimization steps. However, efficient protocols to differentiate primary preadipocytes using alternative species to rodents are scarce. Sheep represent an amenable animal model for fetal biology and developmental origins of health and disease studies. In this work, we present with the first detailed procedure to efficiently differentiate primary fetal and adult ovine preadipocytes.
Fetal and adult ovine adipose and skin tissue harvest, preadipocyte and fibroblast isolation, proliferation, and standardization and optimization of a new adipogenic differentiation protocol. Use of commercial cell lines (3T3-L1 and NIH-3T3) for validation purposes. Oil red O stain and gene expression were used to validate adipogenic differentiation. ANOVA and Fisher's exact test were used to determine statistical significance.
Our optimized adipogenic differentiation method included a prolonged adipogenic cocktail exposure time from 2 to 8 days, higher insulin concentration, and supplementation with the peroxisome proliferator-activated receptor gamma (PPARγ) agonist, rosiglitazone. This protocol was optimized for both, fetal and adult preadipocytes.
Our protocol enables successful adipogenic differentiation of fetal and adult ovine preadipocytes. This work demonstrates that compared to the 3T3-L1 cell line, fetal ovine preadipocytes require a longer exposure to the differentiation cocktail, and the need for IMBX, dexamethasone, and/or the PPARγ agonist rosiglitazone through the terminal differentiation phase. They also require higher insulin concentration during differentiation to enhance lipid accumulation and similar to human primary preadipocytes, PPARγ agonist supplementation is also required for ovine adipogenic differentiation. This work highlights species-specific differences requirements for adipogenic differentiation and the need to develop standardized methods to investigate comparative adipocyte biology.
尽管3T3-L1前脂肪细胞系是脂肪生成研究的一个信息丰富的模型,但通常需要原代培养细胞来了解特定的人类或动物代谢表型。正如大型哺乳动物物种的培养前脂肪细胞所表明的那样,原代培养细胞需要与3T3-L1细胞系不同的特定脂肪生成分化条件。这些条件也是物种特异性的,需要优化步骤。然而,使用啮齿动物以外的其他物种来分化原代前脂肪细胞的有效方案很少。绵羊是用于胎儿生物学以及健康与疾病发育起源研究的合适动物模型。在这项工作中,我们展示了首个有效分化原代胎儿和成年绵羊前脂肪细胞的详细程序。
采集胎儿和成年绵羊的脂肪和皮肤组织,分离前脂肪细胞和成纤维细胞,进行增殖,并对新的脂肪生成分化方案进行标准化和优化。使用商业细胞系(3T3-L1和NIH-3T3)进行验证。采用油红O染色和基因表达来验证脂肪生成分化。使用方差分析和费舍尔精确检验来确定统计学意义。
我们优化的脂肪生成分化方法包括将脂肪生成鸡尾酒的暴露时间从2天延长至8天,提高胰岛素浓度,并添加过氧化物酶体增殖物激活受体γ(PPARγ)激动剂罗格列酮。该方案针对胎儿和成年前脂肪细胞均进行了优化。
我们的方案能够成功地使胎儿和成年绵羊前脂肪细胞发生脂肪生成分化。这项工作表明,与3T3-L1细胞系相比,胎儿绵羊前脂肪细胞需要更长时间暴露于分化鸡尾酒中,并且在终末分化阶段需要吲哚美辛、地塞米松和/或PPARγ激动剂罗格列酮。它们在分化过程中还需要更高的胰岛素浓度以增强脂质积累,并且与人类原代前脂肪细胞类似,绵羊脂肪生成分化也需要补充PPARγ激动剂。这项工作突出了脂肪生成分化的物种特异性差异要求以及开发标准化方法来研究比较脂肪细胞生物学的必要性。
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