Ex vivo Live Imaging of Single Cell Divisions in Mouse Neuroepithelium

被引:2
|
作者
Piotrowska-Nitsche, Karolina [1 ,2 ]
Caspary, Tamara [1 ]
机构
[1] Emory Univ, Sch Med, Dept Human Genet, Atlanta, GA 30322 USA
[2] IGAB Polish Acad Sci, Dept Expt Embryol, Warsaw, Poland
来源
JOVE-JOURNAL OF VISUALIZED EXPERIMENTS | 2013年 / 74期
关键词
Neuroscience; Issue; 74; Genetics; Neurobiology; Cellular Biology; Molecular Biology; Developmental Biology; ex vivo live imaging; cell division; imaging neuroepithelium; primary cilia; Shh; time-lapse confocal imaging; microscopy; immunofluorescence; cell culture; mouse; embryo; animal model; NEURAL-TUBE; IN-VIVO;
D O I
10.3791/4439
中图分类号
O [数理科学和化学]; P [天文学、地球科学]; Q [生物科学]; N [自然科学总论];
学科分类号
07 ; 0710 ; 09 ;
摘要
We developed a system that integrates live imaging of fluorescent markers and culturing slices of embryonic mouse neuroepithelium. We took advantage of existing mouse lines for genetic cell lineage tracing: a tamoxifen-inducible Cre line and a Cre reporter line expressing dsRed upon Cre-mediated recombination. By using a relatively low level of tamoxifen, we were able to induce recombination in a small number of cells, permitting us to follow individual cell divisions. Additionally, we observed the transcriptional response to Sonic Hedgehog (Shh) signaling using an Olig2-eGFP transgenic line (1-3) and we monitored formation of cilia by infecting the cultured slice with virus expressing the cilia marker, Sstr3-GFP (4). In order to image the neuroepithelium, we harvested embryos at E8.5, isolated the neural tube, mounted the neural slice in proper culturing conditions into the imaging chamber and performed time-lapse confocal imaging. Our ex vivo live imaging method enables us to trace single cell divisions to assess the relative timing of primary cilia formation and Shh response in a physiologically relevant manner. This method can be easily adapted using distinct fluorescent markers and provides the field the tools with which to monitor cell behavior in situ and in real time.
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页数:7
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