力触发密度梯度沉降和鸡尾酒酶消化处理,用于从毛囊单位提取收获的人类毛囊中分离单个真皮乳头细胞。

IF 7.1 2区 医学 Q1 CELL & TISSUE ENGINEERING
Junfei Huang, Jian Chen, Haoyuan Li, Zhexiang Fan, Yuyang Gan, Yangpeng Chen, Lijuan Du
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引用次数: 0

摘要

背景:毛囊(HFs)是皮肤内易于获取的动态结构,其中含有各种具有广泛再生潜力的干细胞池,如真皮乳头细胞(DPCs)、真皮鞘细胞和上皮HF干细胞。真皮乳头细胞是高频再生的信号中心。目前分离人类 DPCs 的方法效率不高。这些方法难以获得新鲜分离的原始 DPCs,也不能有效保持 DPCs 的特征:本研究探索了两种简单但更有效的方法。方法:本研究探索了两种简单但更有效的方法,分别采用力触发密度梯度沉降法(FDGS)和鸡尾酒酶消化处理法(CEDT)从人高频中分离纯化DP球,从DP球中获得纯化的新鲜分离的原始DPCs。采用免疫荧光染色、RT-qPCR和Western blot检测分离DPCs的表达谱,分析DPC特异性标志物的基因表达:结果:10% Ficoll PM400被确定为FDGS法的最佳浓度。使用 FDGS 和 CEDT 方法同时分离了原代 DPCs、DSCs 和 HFSCs。使用 FDGS 和 CEDT 方法分离的新鲜 DPCs 的表达谱与传统分离的 DPCs 相似。新鲜分离的DPCs中DP特异性标记物的表达水平明显高于传统分离的DPCs:结论:与传统方法相比,所介绍的实验室方案能够高效分离新鲜 DPCs,从而提高其研究潜力。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Force-triggered density gradient sedimentation and cocktail enzyme digestion treatment for isolation of single dermal papilla cells from follicular unit extraction harvesting human hair follicles.

Background: Hair follicles (HFs) are dynamic structures which are readily accessible within the skin that contain various pools of stem cells with broad regenerative potential, such as dermal papilla cells (DPCs), dermal sheath cells, and epithelial HF stem cells. DPCs act as signalling centres for HF regeneration. The current method for isolating human DPCs are inefficient. These methods struggle to obtain freshly isolated original DPCs and do not maintain the characteristics of DPCs effectively.

Methods: In this study, two simple but more efficient methods were explored. Force-triggered density gradient sedimentation (FDGS) and cocktail enzyme digestion treatment (CEDT) were used to isolate purified DP spheres from human HFs, obtaining purified freshly isolated original DPCs from DP spheres. The expression profiles of isolated DPCs were tested, and gene expression of DPC-specific markers were analyzed using immunofluorescence staining, RT-qPCR and western blot.

Results: The 10% Ficoll PM400 was determined as the optimal concentration for FDGS method. Primary DPCs, DSCs and HFSCs were isolated simultaneously using the FDGS and CEDT method. The expression profiles of fresh DPCs isolated using the FDGS and CEDT methods were similar to those of traditionally isolated DPCs. DP-specific markers were expressed at significantly higher levels in freshly isolated DPCs than in traditionally isolated DPCs.

Conclusions: Compared to traditional methods, the presented laboratory protocols were able to isolate fresh DPCs with high efficiency, thereby improving their research potential.

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来源期刊
Stem Cell Research & Therapy
Stem Cell Research & Therapy CELL BIOLOGY-MEDICINE, RESEARCH & EXPERIMENTAL
CiteScore
13.20
自引率
8.00%
发文量
525
审稿时长
1 months
期刊介绍: Stem Cell Research & Therapy serves as a leading platform for translational research in stem cell therapies. This international, peer-reviewed journal publishes high-quality open-access research articles, with a focus on basic, translational, and clinical research in stem cell therapeutics and regenerative therapies. Coverage includes animal models and clinical trials. Additionally, the journal offers reviews, viewpoints, commentaries, and reports.
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