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利用超毒力根癌农杆菌菌株转化具有不同再生能力的波兰豌豆品种(Pisum sativum L.)的效率

Efficiency of transformation of Polish cultivars of pea (Pisum sativum L.) with various regeneration capacity by using hypervirulent Agrobacterium tumefaciens strains.

作者信息

Pniewski Tomasz, Kapusta Józef

机构信息

Institute of Plant Genetics, Polish Academy of Sciences, Strzeszynska 34, 60-479 Poznań, Poland.

出版信息

J Appl Genet. 2005;46(2):139-47.

Abstract

An Agrobacterium-mediated transformation method of pea has been developed for several edible and fodder cultivars of pea (Pisum sativum L.), characterized previously in their potential for regeneration via organogenesis. The most appropriate explant, which was susceptible to Agrobacterium infection and capable of regenerating transgenic plants, turned out to be a slice of an immature embryo, including the embryo axis and the basal part of a cotyledon. Three hypervirulent strains of A. tumefaciens were tested: AgL0, AgL1 and EHA105. Each carried the binary vector pP35SGIB containing the uid gene, with an intron under control of the 35S promoter, and the bar gene conferring resistance to phosphinotricin. Strain AgL0 was found to be efficient for the majority of cultivars, followed by AgL1 and EHA105. Transformation efficiency varied from 0.7 to 4.1%, depending on cultivar and Agrobacterium strain. The transformation efficiency of particular pea cultivars did not clearly correspond to their regeneration capacity, which--although indispensable--was not a critical parameter of successful transformation. The presence of integrated genes in pea genomic DNA was detected by the PCR. T-DNA was stably transmitted to the progeny, as it was confirmed by Southern hybridization. The activity of introduced genes was analysed by the histochemical GUS assay and by painting leaves or by spraying transgenic plants with the herbicide Basta.

摘要

已为几种食用和饲料用豌豆(Pisum sativum L.)品种开发了一种农杆菌介导的豌豆转化方法,这些品种先前已被鉴定具有通过器官发生进行再生的潜力。最适合的外植体是未成熟胚切片,包括胚轴和子叶基部,它易于被农杆菌感染并能够再生转基因植株。测试了三种超毒力的根癌农杆菌菌株:AgL0、AgL1和EHA105。每个菌株都携带二元载体pP35SGIB,其中包含uid基因,该基因带有一个受35S启动子控制的内含子,以及赋予对草丁膦抗性的bar基因。发现菌株AgL0对大多数品种都有效,其次是AgL1和EHA105。转化效率在0.7%至4.1%之间,具体取决于品种和农杆菌菌株。特定豌豆品种的转化效率与其再生能力并没有明显的对应关系,尽管再生能力是不可或缺的,但它并不是成功转化的关键参数。通过PCR检测豌豆基因组DNA中整合基因的存在。通过Southern杂交证实,T-DNA稳定地传递给了后代。通过组织化学GUS分析、给叶片染色或用除草剂Basta喷洒转基因植株来分析导入基因的活性。

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