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Establishing a density-based method to separate proliferating and senescent cells from bone marrow stromal cells

机译:建立基于密度的方法从骨髓基质细胞中分离增殖和衰老细胞

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摘要

To assist in the study of cellular aging, we established a new method of enriching physiologically aged bone marrow stromal cells (BMSCs) in animals of any age using a Percoll density gradient centrifugation technique. BMSCs from mice 2 months of age were isolated, and their cellular age determined (over 80% Scal-1 CD29 CD11b CD45 CD105 and able to differentiate into osteoblasts, adipocytes, and chondrocytes). As proof –of principle, cells were aged in vitro and confirmed by low bromodeoxyuridine (BrdU) incorporation and senescence-associated β-galactosidase (SA-β-gal) staining. Proliferating cells were enriched in high-density gradient layers, and senescent cells were enriched in low-density gradient layers. We confirmed that over 80% of cells from the low-density gradient layer were senescent with SA-β-gal staining and telomere dysfunction-induced foci (TIF) assay. This density-based method, which can separate proliferating and senescent BMSCs, could be used to study mechanisms of physiologic cell aging and may have implications for the use of BMSCs in clinical transplant applications.
机译:为了协助研究细胞衰老,我们使用Percoll密度梯度离心技术建立了在任何年龄的动物中富集生理上老化的骨髓基质细胞(BMSC)的新方法。分离出2个月2个月的小鼠的BMSC,并且测定细胞年龄(超过80%SCOL-1 CD29 CD11B CD45 CD105,并且能够分化成骨灌注细胞,脂肪细胞和软骨细胞)。作为证明原理,细胞在体外老化并通过低溴氧氧基氨基(BRDU)掺入和衰老相关的β-半乳糖苷酶(SA-β-GAL)染色来证实。在高密度梯度层中富集增殖细胞,富含衰老细胞在低密度梯度层中。我们确认,来自低密度梯度层的超过80%的细胞与SA-β-加仑染色和端粒功能障碍诱导的焦点(TIF)测定的衰老。这种基于密度的方法可以分离增殖和衰老BMSCs,可用于研究生理细胞老化机制,并且可能对临床移植应用中使用BMSC的影响可能具有影响。

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