DeChiara Thomas M, Poueymirou William T, Auerbach Wojtek, Frendewey David, Yancopoulos George D, Valenzuela David M
VelociGene Division, Regeneron Pharmaceutical, Inc., Tarrytown, New York, USA.
Methods Enzymol. 2010;476:285-94. doi: 10.1016/S0076-6879(10)76016-X.
In conventional methods for the generation of genetically modified mice, gene-targeted embryonic stem (ES) cells are injected into blastocyst-stage embryos or are aggregated with morula-stage embryos, which are then transferred to the uterus of a surrogate mother. F0 generation mice born from the embryos are chimeras composed of genetic contributions from both the modified ES cells and the recipient embryos. Obtaining a mouse strain that carries the gene-targeted mutation requires breeding the chimeras to transmit the ES cell genetic component through the germ line to the next (F1) generation (germ line transmission, GLT). To skip the chimera stage, we developed the VelociMouse method, in which injection of genetically modified ES cells into eight-cell embryos followed by maturation to the blastocyst stage and transfer to a surrogate mother produces F0 generation mice that are fully derived from the injected ES cells and exhibit a 100% GLT efficiency. The method is simple and flexible. Both male and female ES cells can be introduced into the eight-cell embryo by any method of injection or aggregation and using all ES cell and host embryo combinations from inbred, hybrid, and outbred genetic backgrounds. The VelociMouse method provides several unique opportunities for shortening project timelines and reducing mouse husbandry costs. First, as VelociMice exhibit 100% GLT, there is no need to test cross chimeras to establish GLT. Second, because the VelociMouse method permits efficient production of ES cell-derived mice from female ES cells, XO ES cell subclones, identified by screening for spontaneous loss of the Y chromosome, can be used to generate F0 females that can be bred with isogenic F0 males derived from the original targeted ES cell clone to obtain homozygous mutant mice in the F1 generation. Third, as VelociMice are genetically identical to the ES cells from which they were derived, the VelociMouse method opens up myriad possibilities for creating mice with complex genotypes in a defined genetic background directly from engineered ES cells without the need for inefficient and lengthy breeding schemes. Examples include creation of F0 knockout mice from ES cells carrying a homozygous null mutation, and creation of a mouse with a tissue-specific gene inactivation by combining null and floxed conditional alleles for the target gene with a transgenic Cre recombinase allele controlled by a tissue-specific promoter. VelociMice with the combinatorial alleles are ready for immediate phenotypic studies, which greatly accelerates gene function assignment and the creation of valuable models of human disease.
在传统的转基因小鼠制备方法中,将基因靶向的胚胎干细胞(ES细胞)注射到囊胚期胚胎中,或与桑葚胚期胚胎聚合,然后将其移植到代孕母鼠的子宫中。由这些胚胎出生的F0代小鼠是嵌合体,由修饰的ES细胞和受体胚胎的基因组成。要获得携带基因靶向突变的小鼠品系,需要将嵌合体进行繁殖,以便通过种系将ES细胞遗传成分传递到下一代(F1)(种系传递,GLT)。为了跳过嵌合体阶段,我们开发了VelociMouse方法,其中将转基因ES细胞注射到八细胞胚胎中,然后使其发育到囊胚期并移植到代孕母鼠体内,从而产生完全源自注射的ES细胞且种系传递效率为100%的F0代小鼠。该方法简单且灵活。雄性和雌性ES细胞都可以通过任何注射或聚合方法引入八细胞胚胎中,并可使用来自近交、杂交和远交遗传背景的所有ES细胞和宿主胚胎组合。VelociMouse方法为缩短项目时间线和降低小鼠饲养成本提供了几个独特的机会。首先,由于VelociMouse小鼠表现出100%的种系传递率,因此无需通过测交嵌合体来确定种系传递。其次,因为VelociMouse方法允许从雌性ES细胞高效生产ES细胞来源的小鼠,通过筛选Y染色体的自发丢失鉴定出的XO ES细胞亚克隆可用于产生F0代雌性小鼠,这些雌性小鼠可与源自原始靶向ES细胞克隆的同基因F0代雄性小鼠交配,以在F1代中获得纯合突变小鼠。第三,由于VelociMouse小鼠在基因上与其来源的ES细胞相同,VelociMouse方法为直接从工程化ES细胞在确定的遗传背景下创建具有复杂基因型的小鼠开辟了无数可能性,而无需低效且冗长的育种方案。例如,从携带纯合无效突变的ES细胞创建F0代敲除小鼠,以及通过将靶基因的无效和loxP条件等位基因与由组织特异性启动子控制的转基因Cre重组酶等位基因组合,创建具有组织特异性基因失活的小鼠。具有组合等位基因的VelociMouse小鼠可立即用于表型研究,这大大加速了基因功能的确定和人类疾病有价值模型的创建。
