小鼠大小肠表皮细胞 | 单细胞测序-526互联

2023年07月05日

分析单细胞数据已有5年的经验，但竟然没有从头生成过自己的数据。

小鼠基本是机制类探索项目的必备实验，不需要太复杂，只要简单的杂交取样即可。

小鼠模型：

Aberrant cell state plasticity mediated by developmental reprogramming precedes colorectal cancer initiation

这篇文章基本涵盖了CRC常见的小鼠模型

Lgr5^eGFP; Apc^f/f;tdT (Tam induction)

AOM/DSS
MNU Tx
CDX2

这部分是小鼠的购买和育种，并且检测是否是特定的基因型。

The generation of Lgr5eGFP-IRES-CreERT2 mouse was described earlier (69). Lgr5eGFP-IRES-CreERT2 mice were backcrossed in C57bL/6J mice and subsequently single-nucleotide polymorphism (SNP)–tested to ensure >97% pure background (Taconic). To inactivate Apc in intestinal tissue, we crossed Apcf/f mice (a gift from C. Perret) to Lgr5eGFP-IRES-CreERT2. These mice were further crossed to R26-LSL-tdTomato purchased from the Jackson Laboratory (JAX, stock #007905) (70) for conditional tdT labeling of Lgr5+ stem cells and their progeny. To delete Sox9, mice were crossed to Sox9flox mice (JAX, stock #013106) (53).
To activate conditional alleles, experimental mice aged 6 to 8 weeks were injected intraperitoneally with a single-dose tamoxifen (50 μl of sunflower oil at 10 mg/ml) unless otherwise indicated. For MNU model, Lgr5eGFP-IRES-CreERT2 mice were treated with drinking water containing 240 parts per million of MNU (bioKEMIX) scheduled every other week for 10 weeks and followed for 1 year. For AOM/DSS model, AOM/DSS treatment was performed as previously described (71). Briefly, at 8 to10 weeks of age, mice were injected intraperitoneally with AOM (10 mg/kg; Sigma-Aldrich) and treated with 2% DSS (30 to 50 kDa; colitis grade; MP Biomedicals) in drinking water for 5 days. DSS treatment was repeated three times once per 4 weeks. Mice were euthanized 11 weeks after AOM injection.

mice高度依赖Cre/LoxP系统来敲除指定的基因，比如Apc，或者Kras^G12D突变