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Fibroblast growth factor receptor–Frs2α signaling is critical for nephron progenitors

机译:成纤维细胞生长因子受体-Frs2α信号对于肾祖细胞至关重要

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Previous studies using transgenic Pax3cre mice have revealed roles for fibroblast growth factor receptors (Fgfrs) and Fgfr substrate 2α (Frs2α) signaling in early metanephric mesenchyme patterning and in ureteric morphogenesis. The role of Fgfr/Frs2α signaling in nephron progenitors is unknown. Thus, we generated mouse models using BAC transgenic Six2EGFPcre (Six2cre) mediated deletion of Fgfrs and/or Frs2α in nephron progenitors. Six2cre mediated deletion of Fgfr1 or Fgfr2 alone led to no obvious kidney defects. Six2creFgfr1flox/floxFgfr2flox/flox (Fgfr1/2NP−/−) mice generate a discernable kidney; however, they develop nephron progenitor depletion starting at embryonic day 12.5 (E12.5) and later demonstrate severe cystic dysplasia. To determine the role of Frs2α signaling downstream of Fgfr2 in Fgfr1/2NP−/− mice, we generated Six2cre,Fgfr1flox/floxFgfr2LR/LR (Fgfr1NP−/−Fgfr2LR/LR) mice that have point mutations in the Frs2α binding site of Fgfr2. Like Fgfr1/2NP−/− mice, Fgfr1NP−/−Fgfr2LR/LR develop nephron progenitor depletion, but it does not start until E14.5 and older mice have less severe cystic dysplasia than Fgfr1/2NP−/− To determine the role of Frs2α alone in nephron progenitors, we generated Six2creFrs2′Aflox/flox (Frs2aNP−/−) mice. Frs2aNP−/− mice also develop nephron progenitor depletion and renal cysts, although these occurred later and were less severe than in the other Six2cre mutant mice. The nephron progenitor loss in all Six2cre mutant lines was associated with decreased Cited1 expression and increased apoptosis versus controls. FAC-sorted nephron progenitors in Six2cre Frs2Aflox/flox mice demonstrated evidence of increased Notch activity versus controls, which likely drives the progenitor defects. Thus, Fgfr1 and Fgfr2 have synergistic roles in maintaining nephron progenitors; furthermore, Fgfr signaling in nephron progenitors appears to be mediated predominantly by Frs2α.
机译:先前使用转基因Pax3cre小鼠进行的研究表明,成纤维细胞生长因子受体(Fgfrs)和Fgfr底物2α(Frs2α)信号在早期后肾间充质模式和输尿管形态发生中的作用。 Fgfr /Frs2α信号在肾单位祖细胞中的作用尚不清楚。因此,我们在肾单位祖细胞中使用BAC转基因Six2EGFPcre(Six2cre)介导的Fgfrs和/或Frs2α缺失产生了小鼠模型。 Six2cre介导的Fgfr1或Fgfr2单独缺失不会导致明显的肾脏缺陷。 Six2creFgfr1 flox / flox Fgfr2 flox / flox (Fgfr1 / 2 NP -/-)小鼠产生可识别的肾脏;然而,它们在胚胎第12.5天(E12.5)开始发展肾单位祖细胞耗竭,后来表现出严重的囊性异型增生。为了确定Fgfr2下游的Frs2α信号在Fgfr1 / 2 NP -/-小鼠中的作用,我们生成了Six2cre Fgfr1 flox / flox Fgfr2 LR / LR (Fgfr1 NP -/- Fgfr2 LR / LR )小鼠在Fgfr2的Frs2α结合位点具有点突变。像Fgfr1 / 2 NP -/-小鼠一样,Fgfr1 NP -/- Fgfr2 LR / LR 发生肾单位祖细胞耗竭,但直到E14.5和年龄较大的小鼠的囊性异型症严重程度低于Fgfr1 / 2 NP -// 才开始单独使用Frs2α在肾祖细胞中的作用,我们产生了Six2creFrs2′A flox / flox Frs2a NP -/-)小鼠。 Frs2a NP -/-小鼠也发生肾单位祖细胞耗竭和肾囊肿,尽管它们发生的时间较晚,并且不如其他Six2cre突变体严重老鼠。与对照相比,所有 Six2cre 突变株中肾单位祖细胞的丢失与Cited1表达降低和凋亡增加有关。在 Six2cre Frs2 ' A flox / flox 小鼠中,FAC分选的肾单位祖细胞显示出Notch活性高于对照组的证据,这可能导致了祖细胞缺陷。因此,Fgfr1和Fgfr2在维持肾单位祖细胞中具有协同作用。此外,肾单位祖细胞中的Fgfr信号似乎主要由Frs2α介导。

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