番茄果实特异性启动子的克隆与遗传转化研究

为了实现外源基因在番茄果实中的高效和特异表达,克隆了番茄果实特异基因多聚半乳糖醛酸酶基因( Polygalacturonase,PG)的启动子.以中蔬四号番茄为材料,建立并优化了以子叶为外植体的番茄高效再生和遗传转化体系；以GUS为报告基因,构建PG:GUS植物表达载体,转化番茄.结果表明,在1.0 mg/L ZT的MS分化培养中,番茄子叶的发芽率最高,芽的诱导率高达91％,且发生畸态芽和褐化的外植体最少；通过抗生素浓度对农杆菌的抑制效果试验发现,当头孢霉素的浓度为200 mg/L时,抑制农杆菌的效果最好；成功克隆了番茄PG启动子,将PG启动子驱动的GUS基因转入番茄,对转基因后代果实的GUS染色表明,PG启动子驱动的外源基因在果实中特异表达.

Fruit-specific Promoter Cloning and Tomato Transformation

In order to obtain fruit-specific and highly expressed foreign gene in transgenic tomato,we cloned the promoter of Poly-galacturonase(PG).The tomato regeneration and transformation system were established using "zhongshu 4".PG promoter: GUS construct was made and introduced into tomato through Agrobacterium mediated transformation.Results showed that the best callus initiation and shoot induction medium was MS + 1.0 mg/L ZT.The shoots induction rate reached 91% with low portion of abnormal shoots.200 mg/L of cefotaxime could effectively inhibit the growth of Agrobacteria.Histochemical analysis showed that GUS was specifically expressed in transgenic tomato fruit.