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Heterochronic Pellet Assay to Test Cell-cell Communication in the Mouse Retina

机译:异时球团测定法测试小鼠视网膜中的细胞间通讯

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摘要

All seven retinal cell types that make up the mature retina are generated from a common, multipotent pool of retinal progenitor cells (RPCs) (). One way that RPCs know when sufficient numbers of particular cell-types have been generated is through negative feedback signals, which are emitted by differentiated cells and must reach threshold levels to block additional differentiation of that cell type. A key assay to assess whether negative feedback signals are emitted by differentiated cells is a heterochronic pellet assay in which early stage RPCs are dissociated and labeled with BrdU, then mixed with a 20-fold excess of dissociated differentiated cells. The combined cells are then re-aggregated and cultured as a pellet on a membrane for 7–10 days in vitro. During this time frame, RPCs will differentiate, and the fate of the BrdU+ RPCs can be assessed using cell type-specific markers. Investigators who developed this pellet assay initially demonstrated that neonatal RPCs give rise to rods on an accelerated schedule compared to embryonic RPCs when the two cell types are mixed together (; ). We have used this assay to demonstrate that sonic hedgehog (Shh), which we found acts as a negative regulator of retinal ganglion cell (RGC) differentiation, promotes RPC proliferation (; ). More recently we modified the heterochronic pellet assay to assess the role of feedback signals for retinal amacrine cells, identifying transforming growth factor β2 (Tgfβ2) as a negative feedback signal, and Pten as a modulator of the Tgfβ2 response (; ). This assay can be adapted to other lineages and tissues to assess cell-cell interactions between two different cell-types (heterotypic) in either an isochronic or heterochronic manner.
机译:构成成熟视网膜的所有七种视网膜细胞类型都是从共同的,多能的视网膜祖细胞(RPC)()中产生的。 RPC知道何时已生成足够数量的特定细胞类型的一种方法是通过负反馈信号,该信号由分化的细胞发出,并且必须达到阈值水平才能阻止该细胞类型的其他分化。评估分化细胞是否发出负反馈信号的关键方法是异时沉淀法,其中早期RPC被解离并用BrdU标记,然后与20倍过量的解离的分化细胞混合。然后将合并的细胞重新聚集并在膜上以沉淀形式体外培养7-10天。在此时间范围内,RPC会有所不同,并且可以使用特定于细胞类型的标记物来评估BrdU + RPC的命运。开发这种沉淀分析法的研究人员最初证明,与两种细胞类型混合在一起的胚胎RPC相比,新生儿RPC的生成时间表更快。我们已经使用该测定法证明了我们发现的声波刺猬(Shh)作为视网膜神经节细胞(RGC)分化的负调节剂,可促进RPC增殖。最近,我们修改了异时沉淀法,以评估视网膜无长突细胞反馈信号的作用,将转化生长因子β2(Tgfβ2)识别为负反馈信号,并将Pten识别为Tgfβ2反应的调节剂(;)。该测定法可以适用于其他谱系和组织,以等时或异时方式评估两种不同细胞类型(异型)之间的细胞间相互作用。

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