Dow AgroSciences, 9330 Zionsville Rd., Indianapolis, IN 46268, USA.
Plant Mol Biol. 2010 Aug;73(6):617-28. doi: 10.1007/s11103-010-9641-4. Epub 2010 May 8.
A transgene, flanked by zinc finger nuclease (ZFN) cleavage sites, was deleted from a stably transformed plant by crossing it with a second plant expressing a corresponding ZFN gene. A target construct, containing a GUS reporter gene flanked by ZFN cleavage sites, a GFP reporter gene and a PAT selectable marker gene, was transformed into tobacco. Basta-resistant plants were regenerated and screened for GUS and GFP expression. A second construct, containing a ZFN gene driven by the constitutive CsVMV promoter and an HPT selectable marker gene, was also transformed into tobacco. Selected T(0) plants were grown to maturity and allowed to self-pollinate. Homozygous target plants, which expressed GUS and GFP, were crossed with homozygous ZFN plants, which expressed the ZFN gene. Numerous GUS-negative plants were observed among the hybrids with one particular cross displaying approximately 35% GUS-negative plants. Evidence for complete deletion of a 4.3 kb sequence comprising the GUS gene was obtained and sequence confirmed. Co-segregation in F(2) progenies of 'truncated' and 'intact' target sequences with expected reporter gene phenotypes were observed. Since ZFNs can be designed to bind and cleave a wide range of DNA sequences, these results constitute a general strategy for creating targeted gene deletions.
通过与表达相应锌指核酸酶(ZFN)基因的第二株植物杂交,从稳定转化的植物中删除侧翼带有 ZFN 切割位点的转基因。将含有侧翼带有 ZFN 切割位点的 GUS 报告基因、GFP 报告基因和 PAT 选择标记基因的靶构建体转化到烟草中。抗性植株再生并筛选 GUS 和 GFP 表达。将第二个构建体转化到烟草中,该构建体含有由组成型 CsVMV 启动子驱动的 ZFN 基因和 HPT 选择标记基因。选择的 T(0) 植物成熟并自花授粉。表达 GUS 和 GFP 的纯合靶植物与表达 ZFN 基因的纯合 ZFN 植物杂交。在杂种中观察到许多 GUS 阴性植株,其中一个特定杂交种显示约 35%的 GUS 阴性植株。获得并证实了包含 GUS 基因的 4.3kb 序列完全缺失的证据。在 F(2)后代中观察到“截断”和“完整”靶序列与预期报告基因表型的共分离。由于 ZFN 可以设计为结合和切割广泛的 DNA 序列,因此这些结果构成了创建靶向基因缺失的通用策略。
