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[利用根癌农杆菌获得转基因水稻植株及其后代]

[Obtaining transgenic rice plants and their progenies using Agrobacterium tumefaciens].

作者信息

Yin Z C, Yang F, Xu Y, Li B J

机构信息

Biotechnology Research Center, Zhongshan University, Guangzhou.

出版信息

Yi Chuan Xue Bao. 1998 Dec;25(6):517-24.

PMID:10465898
Abstract

Rice (Oriza sativa L.) suspension cells of Taipei 309 were co-cultivated with A. tumefaciens stran EHA101 harbouring binary vector pBYT2 for 3 days in the presence of vir inducer, 100 mumol/L acetosyringone (AS). After 2 months of continuous selection, 17 stable hygromycin-resistant, GUS-positive calli were recovered from 364 suspension cell clusters co-cultivated with A. tumefaciens. 10 putative transgenic R0 plants obtained from 8 tansformed calli and their progenies were analyzed for the integration and expression of foreign genes. Southern blot analysis of R0 and R1 generations indicated that foreign genes had been stably integrated in the genome of transgenic rice and sexually transmitted. One of the transgenic lines showed 5 copies of T-DNA integration, while the others had only one copy. Histochemical staining observation and fluorometric assay of GUS activity in transgenic rice cells and plants showed ubiquitin promoter from maize was highly effective in driving the expression of gus reporter gene in transgenic rice cells. GUS protein and its activity were also investigated through ndPAGE-X-Gluc staining assay, and it was found that the GUS protein in transgenic rice cells was smaller in size than the standard GUS protein (Sigma Co. G0786) but as large as that from E.coli HB101 (pBI121). This study suggested that Agrobacterium-mediated transformation of plant is an efficient and reliable method to introduce foreign genes into rice.

摘要

将台北309水稻(Oriza sativa L.)悬浮细胞与携带双元载体pBYT2的根癌农杆菌菌株EHA101在100 μmol/L乙酰丁香酮(AS)这种vir诱导剂存在的条件下共培养3天。在连续筛选2个月后,从与根癌农杆菌共培养的364个悬浮细胞团中获得了17个稳定的潮霉素抗性、GUS阳性愈伤组织。对从8个转化愈伤组织获得并产生后代的10株假定转基因R0植株进行了外源基因整合和表达分析。R0和R1代的Southern杂交分析表明,外源基因已稳定整合到转基因水稻基因组中并能进行有性传递。其中一个转基因株系显示有5个T-DNA整合拷贝,而其他株系只有一个拷贝。对转基因水稻细胞和植株进行组织化学染色观察及GUS活性荧光测定,结果表明玉米泛素启动子在驱动gus报告基因在转基因水稻细胞中表达方面非常有效。还通过非变性聚丙烯酰胺凝胶-X-葡萄糖苷酸染色法研究了GUS蛋白及其活性,发现转基因水稻细胞中的GUS蛋白大小比标准GUS蛋白(Sigma公司G0786)小,但与大肠杆菌HB101(pBI121)中的GUS蛋白大小相同。本研究表明,农杆菌介导的植物转化是一种将外源基因导入水稻的高效且可靠的方法。

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