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The effect of cell culture on age-related transcriptomic changes in dermal fibroblasts

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https://www.ncbi.nlm.nih.gov/geo/query/acc.cgi?acc=GSE117763
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During aging, stromal functions are thought to be impaired, yet little is known whether this stems from molecular and cellular changes of fibroblasts, a major component of stroma. Using population- and single-cell whole transcriptomics, and long-term lineage tracing, we studied alterations in murine dermal fibroblasts during physiological aging under different dietary regimes known to affect longevity. We show that the identity of aged fibroblasts becomes undefined, with the distinct fibroblast states present in young skin no longer clearly demarcated. In addition, old fibroblasts not only reduce the expression of genes involved in the formation of the extracellular matrix, but intriguingly, also gain adipogenic traits, paradoxically becoming similar to neonatal pro-adipogenic fibroblasts. These age-related alterations are sensitive to systemic changes in metabolism: long-term caloric restriction prevents them in old fibroblasts in a reversible manner, whereas a high-fat diet potentiates them in young fibroblasts. Finally, inhibition of the master regulator of adipogenesis, PPARgamma, attenuates fibroblast aging in vivo, providing potential anti-aging therapeutic alternatives to caloric restriction. Dermal fibroblasts were isolated from four young (2-months-old) and four old (18-months-old) female C57/Bl6 mice. For sample collection two young and two old mice were sacrificed per day (N=4).From each mouse 5000 fibroblasts were immediately profiled and 5000 fibroblasts were profiled after culturing.
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2018-11-14
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