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活细胞共聚焦分析中脂肪生成和成骨分化干细胞的同时标记。

Simultaneous Labeling of Adipogenic and Osteogenic Differentiating Stem Cells for Live Confocal Analysis.

机构信息

PASS-Bio Med, Centro Grandi Strumenti, University of Pavia, Pavia, Italy.

Department of Molecular Medicine, University of Pavia, Pavia, Italy.

出版信息

Methods Mol Biol. 2023;2566:53-62. doi: 10.1007/978-1-0716-2675-7_5.

Abstract

Adipocytes and osteoblasts derive from a common mesenchymal progenitor present in a range of connective tissues. Differentiation of the progenitors toward the two cell lineages can be induced in vitro through well-established protocols, and leads to the appearance of lipid-laden adipocytes and osteoblasts embedded in a mineralized matrix. The formation of these two lineages in cell cultures can be monitored using lipophilic dyes such as Oil Red O and substances binding to mineral deposits such as Alizarin Red S, respectively. However, these common staining techniques require cell fixation and are thus incompatible with live analyses. Recently, alternative approaches using vital stains have allowed the dual visualization and fluorescence imaging of adipogenic and osteogenic lineages in live cultures. Here we present the concomitant analysis of cultures containing adipogenic and osteogenic cell types using live staining, combining LipidTox Red and tetracycline with NucRed nuclear counterstain for confocal imaging. This approach can be applied to visualize the kinetics and 3D structure of differentiating mesenchymal cultures over time and highlights the interaction of adipose and mineralized compartments associated with bone marrow stroma.

摘要

脂肪细胞和骨细胞都来源于存在于多种结缔组织中的一种共同的间充质祖细胞。通过成熟的方案,可以在体外诱导祖细胞向这两个细胞谱系分化,并导致富含脂质的脂肪细胞和嵌入矿化基质中的成骨细胞的出现。可以使用亲脂性染料(如油红 O)和与矿物质沉积物结合的物质(如茜素红 S)分别监测细胞培养物中这两种谱系的形成。然而,这些常见的染色技术需要细胞固定,因此与活体分析不兼容。最近,使用活细胞染料的替代方法允许在活培养物中对脂肪生成和成骨谱系进行双重可视化和荧光成像。在这里,我们使用活细胞染色法同时分析含有脂肪生成和成骨细胞类型的培养物,将 LipidTox Red 和四环素与 NucRed 核复染结合使用,进行共聚焦成像。这种方法可用于随时间可视化分化间充质培养物的动力学和 3D 结构,并突出与骨髓基质相关的脂肪和矿化区室的相互作用。

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