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首页> 外文期刊>American Journal of Clinical and Experimental Urology >Single-cell RNA-Seq analysis identifies a putative epithelial stem cell population in human primary prostate cells in monolayer and organoid culture conditions
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Single-cell RNA-Seq analysis identifies a putative epithelial stem cell population in human primary prostate cells in monolayer and organoid culture conditions

机译:单细胞RNA-SEQ分析识别在单层和有机体培养条件下人原发性前列腺细胞中推定的上皮细胞群

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Human primary prostate epithelial (PrE) cells represent patient-derived in vitro models and are traditionally grown as a monolayer in two-dimensional culture. It has been recently demonstrated that expansion of primary cells into three-dimensional prostatic organoids better mimics prostate epithelial glands by recapitulating epithelial differentiation and cell polarity. Here, we sought to identify cell populations present in monolayer PrE cells and organoid culture, grown from the same patient, using single-cell RNA-sequencing. Single-cell RNA-sequencing is a powerful tool to analyze transcriptome profiles of thousands of individual cells simultaneously, creating an in-depth atlas of cell populations within a sample. Organoids consisted of six distinct cell clusters (populations) of intermediate differentiation compared to only three clusters in the monolayer prostate epithelial cells. Integrated analysis of the datasets allowed for direct comparison of the monolayer and organoid samples and identified 10 clusters, including a distinct putative prostate stem cell population that was high in Keratin 13 ( KRT13 ), Lymphocyte Antigen 6D ( LY6D ), and Prostate Stem Cell Antigen ( PSCA ). Many of the genes within the clusters were validated through RT-qPCR and immunofluorescence in PrE samples from 5 additional patients. KRT13+ cells were observed in discrete areas of the parent tissue and organoids. Pathway analyses and lack of EdU incorporation corroborated a stem-like phenotype based on the gene expression and quiescent state of the KRT13+ cluster. Other clusters within the samples were similar to epithelial populations reported within patient prostate tissues. In summary, these data show that the epithelial stem population is preserved in PrE cultures, with organoids uniquely expanding intermediate cell types not present in monolayer culture.
机译:人的原代前列腺上皮(前)细胞代表患者衍生的体外模型,传统上被作为二维培养物中的单层生长。最近据证明,通过重新承载上皮分化和细胞极性,将原发性细胞扩展到三维前列腺细胞素更好地模仿前列腺上皮腺体。在这里,我们寻求使用单细胞RNA测序从同一患者生长的单层前细胞和有机培养物中存在的细胞群。单细胞RNA测序是一种强大的工具,可以同时分析成千上万个体细胞的转录组谱,在样品中产生深入的细胞群地图集。与单层前列腺上皮细胞中的仅三簇相比,有器件由中间分化的六个不同细胞簇(种群)组成。允许的数据集进行综合分析,用于直接比较单层和有机体样品并鉴定10个簇,包括在角蛋白13(KRT13),淋巴细胞抗原6d(Ly6D),淋巴细胞抗原6d(Ly6d)和前列腺干细胞抗原中具有明显推定的前列腺干细胞群(PSCA)。簇内的许多基因通过RT-QPCR验证,来自5例患者的预样品中的预样品中的免疫荧光。在母体组织和有机体的离散区域中观察到KRT13 +细胞。途径分析和缺乏EDU掺入的基于KRT13 +簇的基因表达和静态状态证实了干燥的表型。样品中的其他簇类似于患者前列腺组织内报道的上皮群体。总之,这些数据表明上皮茎群在预培养物中保存,有器有机体唯一地扩张单层培养中不存在的中间细胞类型。

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