两种ENU诱导的少毛小鼠及突变基因定位

Wu Bao-Jin, Shao Yi-Xiang, Mao Hui-Hua, Tang Dong, Liu Jing, Xue Zheng-Feng, Li Hou-Da

Medical College of Yangzhou University, Yangzhou, Jiangsu 225001, China.

J Dermatol Sci. 2004 Dec;36(3):149-56. doi: 10.1016/j.jdermsci.2004.08.010.

OBJECTIVE

To establish mouse models for human diseases through N-ethyl-N-nitrosourea (ENU) mutagenesis, and to provide groundwork to clone genes and study their functions after mapping the mutant genes.

METHODS

18 male D2 mice (G0) at age of 8-10 weeks old were injected intraperitoneally with ENU (100 mg/kg) once a week for three consecutive weeks. The treated male mice were mated with females of the same strain, and their offspring (G1) were used to screen for dominant and recessive mutation. After breeding the mutant F2 (D2B6 F1 intercrossing) mice, 39 microsatellites that are equally distributed on the mouse genome and are different between B6 and D2 strains were used to scan the genome. According to the log odds score (LODS) we determined whether these microsatellites were linked to the mutant genes and calculated the location of mutant genes based on their recombination ratio.

RESULTS

We screened 532 G1 mice, of which 14 exhibited mutation phenotypes. None was dominantly hereditable. Two cases of recessive inheritable scant hair mice were obtained through testing 30 G1 mice with normal phenotype and potential recessive mutant genes. All showed scant coat hair, grew slowly, and hyperkeratoses of epidermis and bollicular horn plug in histological sections. Their visceral organs were not markedly different from normal, and they were named scant hair 1 Baojin (symbol is snthr(-1Bao)) and scant hair 2 Baojin (symbol is snthr(-2Bao)). Through microsatellite screening we found that the LODS between snthr(-1Bao) and D9Mit243 was 7.73, and the linkage was determined. After analyzing the recombination ratio between snthr(-1Bao) and microsatellite D9Mit18 which was near snthr(-1Bao) based on a total number of 126 F2 mice with the scant hair phenotype, we determined that snthr(-1Bao) was located at chromosome 9 and was 71cM from centromere. Using the same technique, snthr(-2Bao) was mapped to the same position as snthr(-1Bao).

CONCLUSION

In our research, two cases of scant hair mice provide good models for the study of dermatology, and the location of mutant genes provides a solid foundation for cloning new mice scant hair genes.

目的

通过N-乙基-N-亚硝基脲（ENU）诱变建立人类疾病的小鼠模型，并为在定位突变基因后克隆基因及其功能研究奠定基础。

方法

18只8 - 10周龄的雄性D2小鼠（G0），每周腹腔注射ENU（100 mg/kg），连续注射三周。将处理后的雄性小鼠与同品系雌性小鼠交配，其后代（G1）用于筛选显性和隐性突变。繁殖突变的F2（D2B6 F1杂交）小鼠后，使用39个均匀分布于小鼠基因组且在B6和D2品系间存在差异的微卫星对基因组进行扫描。根据对数优势分数（LOD）确定这些微卫星是否与突变基因连锁，并根据重组率计算突变基因的位置。

结果

筛选了532只G1小鼠，其中14只表现出突变表型，无显性遗传现象。通过对30只表型正常且具有潜在隐性突变基因的G1小鼠进行检测，获得了2例隐性遗传的少毛小鼠。所有少毛小鼠均表现为毛发稀疏、生长缓慢，组织学切片显示表皮角化过度和毛囊角栓形成。其内脏器官与正常小鼠无明显差异，分别命名为少毛1宝金（符号为snthr(-1Bao)）和少毛2宝金（符号为snthr(-2Bao)）。通过微卫星筛选发现，snthr(-1Bao)与D9Mit243之间的LOD为7.73，确定存在连锁关系。基于总共126只具有少毛表型的F2小鼠，分析snthr(-1Bao)与靠近snthr(-1Bao)的微卫星D9Mit18之间的重组率后，确定snthr(-1Bao)位于9号染色体，距着丝粒71cM。采用相同技术，snthr(-2Bao)被定位到与snthr(-1Bao)相同的位置。