Isolation methods of human and bovine adipose tissue derived stem cells

Fhataheya Buang, M. Mohamad Shahimin
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引用次数: 1

Abstract

Mammalian adipose tissue derived stem cells have a tremendous potential in regenerative medicine for tissue engineering and somatic nuclear transfer (SNT). The isolation methods of human and bovine adipose tissue derived stem cells are compared in this paper to determine the feasibility and optimum method of isolation. The optimum isolation method will reduce the processing time, efforts and money as isolation is the first crucial and important step in stem cells research. Human abdominal subcutaneous adipose tissue and bovine abdominal subcutaneous adipose tissue are digested in three collagenase type 1 concentration 0.075%, 0.3% and 0.6% agitated at 1 hour and 2 hours under 37°C in 5% CO2 incubator. The cultures are then morphologically characterised. Human adipose tissue stem cells are found to be best isolated using abdominal subcutaneous depot, using 0.075% collagenase type 1 agitated at 1 hours under 37°C in CO2 incubator. While bovine adipose tissue derived stem cells are best isolated using abdominal subcutaneous depot, using 0.6% collagenase type 1 agitated at 2 hours under 37°C in CO2 incubator.
人与牛脂肪组织来源干细胞的分离方法
哺乳动物脂肪组织源性干细胞在组织工程和体细胞核移植等再生医学领域具有巨大的应用潜力。本文比较了人脂肪组织源性干细胞和牛脂肪组织源性干细胞的分离方法,确定了分离的可行性和最佳方法。最佳的分离方法将减少处理时间、精力和金钱,因为分离是干细胞研究中至关重要的第一步。将人腹部皮下脂肪组织和牛腹部皮下脂肪组织分别在浓度为0.075%、0.3%和0.6%的3种胶原酶1型中消化,在37℃下5% CO2培养箱中搅拌1小时和2小时。然后对培养物进行形态学表征。人脂肪组织干细胞的最佳分离方法是腹腔皮下储存,使用0.075%的1型胶原酶,在37°C的CO2培养箱中搅拌1小时。而牛脂肪组织来源的干细胞最好使用腹腔皮下储存,使用0.6%的胶原酶1型,在37°C的CO2培养箱中搅拌2小时。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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