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Publication : Simultaneous quantitative assessment of two distinct cell lineages with a nuclear-localized dual genetic reporter.

First Author  Tang M Year  2020
Journal  J Mol Cell Cardiol Volume  146
Pages  60-68 PubMed ID  32668281
Mgi Jnum  J:314889 Mgi Id  MGI:6820594
Doi  10.1016/j.yjmcc.2020.07.002 Citation  Tang M, et al. (2020) Simultaneous quantitative assessment of two distinct cell lineages with a nuclear-localized dual genetic reporter. J Mol Cell Cardiol 146:60-68
abstractText  Genetic lineage tracing has been widely used for studying in vivo cell fate plasticity during embryogenesis, tissue homeostasis, and disease development. Recent applications with multiple site-specific recombinases have been used in complex and sophisticated genetic fate mapping studies. However, the previous multicolor reporters for dual recombinases had limitations of precise in situ quantification of cell number, which is mainly due to the intermingling of cells in condensed tissues. Here, we generated a dual recombinase-mediated nuclear-localized GFP and tdTomato reporter line, which enables clear, simultaneous quantification of two distinct cell lineages in vivo. Combining this dual genetic reporter with Tbx18-Cre and Cdh5-Dre lines, which genetically trace epicardial and endothelial cells, respectively, we obtained high-resolution images for the anatomic distribution of the descendants of these two distinct cell lineages in the valve mesenchyme during development, remodeling, and maturation stages. This new dual genetic reporter is expected to facilitate fate tracing of two cell lineages and their objective quantification in vivo.
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