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Merck
CN
  • Dual Cre and Dre recombinases mediate synchronized lineage tracing and cell subset ablation in vivo.

Dual Cre and Dre recombinases mediate synchronized lineage tracing and cell subset ablation in vivo.

The Journal of biological chemistry (2022-04-25)
Haixiao Wang, Lingjuan He, Yan Li, Wenjuan Pu, Shaohua Zhang, Ximeng Han, Kathy O Lui, Bin Zhou
摘要

Genetic technology using site-specific recombinases, such as the Cre-loxP system, has been widely employed for labeling specific cell populations and for studying their functions in vivo. To enhance the precision of cell lineage tracing and functional study, a similar site-specific recombinase system termed Dre-rox has been recently used in combination with Cre-loxP. To enable more specific cell lineage tracing and ablation through dual recombinase activity, we generated two mouse lines that render Dre- or Dre+Cre-mediated recombination to excise a stop codon sequence that prevents the expression of diphtheria toxin receptor (DTR) knocked into the ubiquitously expressed and safe Rosa26 locus. Using different Dre- and Cre-expressing mouse lines, we showed that the surrogate gene reporters tdTomato and DTR were simultaneously expressed in target cells and in their descendants, and we observed efficient ablation of tdTomato+ cells after diphtheria toxin administration. These mouse lines were used to simultaneously trace and deplete the target cells of interest through the inducible expression of a reporter and DTR using dual Cre and Dre recombinases, allowing a more precise and efficient study of the role of specific cell subsets within a heterogeneous population in pathophysiological conditions in vivo.

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Roche
原位细胞死亡检测试剂盒,荧光素法, sufficient for ≤50 tests, suitable for detection
Sigma-Aldrich
白喉毒素 来源于白喉杆菌, lyophilized powder, Product is in unnicked form
Sigma-Aldrich
抗-NeuN抗体,克隆A60,Alexa Fluor488结合, clone A60, Chemicon®, from mouse