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作 者:尚霄丽[1] 冯建灿[1] 朱道圩[1] 邢东方[1] 马春华[1]
出 处:《中国细胞生物学学报》2010年第1期126-130,共5页Chinese Journal of Cell Biology
摘 要:以中华猕猴桃伏牛95-2(Actinidia chinensis‘Funiu 95-2')叶片为试验材料,对不同侵染方式、预培养时间、菌液浓度、共培养时间等影响β-葡萄糖苷酸酶基因(β-glucuronidase,GUS)瞬时表达率的因素进行了研究。结果表明,叶片预培养3天,菌液浓度A_(600)值为0.3,真空渗入方式侵染10 min,共培养4天条件下,GUS基因瞬时表达率最高,达到92.2%。对转基因抗性植株进行PCR检测和GUS组织化学染色,初步证明外源基因已整合到中华猕猴桃伏牛95-2的基因组中。Factors affecting transient expression frequency of GUS gene, including different infection methods, days of pre-culture, concentration of Agrobacterium tumefaciens, days of co-culture were studied in genetic transformation, using leaves ofAcitnidia chinensis 'Funiu 95-2' as explants. The results showed that the highest transient expression frequency (92.2%) was obtained when explants were firstly pre-cultured for 3 d, infected for 10 min with Agrobacterium tumefaciens (A600=0.3) by vacuum infiltration and finally co-cultured for 4 d. PCR detection and GUS histochemical staining proved initially that the foreign gene had been integrated into the Acitnidia chinensis genomes.
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