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R26-WntVis报告基因小鼠对Wnt信号水平呈现出分级反应。

R26-WntVis reporter mice showing graded response to Wnt signal levels.

作者信息

Takemoto Tatsuya, Abe Takaya, Kiyonari Hiroshi, Nakao Kazuki, Furuta Yasuhide, Suzuki Hitomi, Takada Shinji, Fujimori Toshihiko, Kondoh Hisato

机构信息

Fujii Memorial Institute of Medical Sciences, Tokushima University, 3-18-15 Kuramoto-cho, Tokushima, 770-8503, Japan.

Graduate School of Frontier Biosciences, Osaka University, 1-3 Yamadaoka, Suita, Osaka, 565-0871, Japan.

出版信息

Genes Cells. 2016 Jun;21(6):661-9. doi: 10.1111/gtc.12364. Epub 2016 Mar 31.

Abstract

The canonical Wnt signaling pathway plays a major role in the regulation of embryogenesis and organogenesis, where signal strength-dependent cellular responses are of particular importance. To assess Wnt signal levels in individual cells, and to circumvent the integration site-dependent bias shown in previous Wnt reporter lines, we constructed a new Wnt signal reporter mouse line R26-WntVis. Heptameric TCF/LEF1 binding sequences were combined with a viral minimal promoter to confer a graded response to the reporter depending on Wnt signal strengths. The histone H2B-EGFP fusion protein was chosen as the fluorescent reporter to facilitate single-cell resolution analyses. This WntVis reporter gene was then inserted into the ROSA26 locus in an orientation opposite to that of the endogenous gene. The R26-WntVis allele was introduced into Wnt3a(-/-) and Wnt3a(vt/-) mutant mouse embryos and compared with wild-type embryos to assess its performance. The R26-WntVis reporter was activated in known Wnt-dependent tissues and responded in a graded fashion to signal intensity. This analysis also indicated that the major Wnt activity early in embryogenesis switched from Wnt3 to Wnt3a around E7.5. The R26-WntVis mouse line will be widely useful for the study of Wnt signal-dependent processes.

摘要

经典Wnt信号通路在胚胎发育和器官形成的调控中起主要作用,其中信号强度依赖性细胞反应尤为重要。为了评估单个细胞中的Wnt信号水平,并规避先前Wnt报告基因系中显示的整合位点依赖性偏差,我们构建了一种新的Wnt信号报告基因小鼠系R26-WntVis。七聚体TCF/LEF1结合序列与病毒最小启动子相结合,使报告基因根据Wnt信号强度产生分级反应。选择组蛋白H2B-EGFP融合蛋白作为荧光报告基因,以促进单细胞分辨率分析。然后将这个WntVis报告基因以与内源基因相反的方向插入ROSA26位点。将R26-WntVis等位基因导入Wnt3a(-/-)和Wnt3a(vt/-)突变小鼠胚胎中,并与野生型胚胎进行比较以评估其性能。R26-WntVis报告基因在已知的Wnt依赖性组织中被激活,并以分级方式对信号强度作出反应。该分析还表明,胚胎发育早期的主要Wnt活性在大约E7.5时从Wnt3转换为Wnt3a。R26-WntVis小鼠系将广泛应用于Wnt信号依赖性过程的研究。

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