番茄和马铃薯植株相关细菌可转化性的评估。

Environmental biosafety research Pub Date : 2007-01-01 Epub Date: 2007-09-12 DOI:10.1051/ebr:2007030
Leo van Overbeek, Jessica Ray, Jan Dirk van Elsas
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引用次数: 3

摘要

植物DNA转化植物相关细菌从未在农业领域得到证实。采用pSKTG DNA质粒和同源DNA提取物,对从茄枯菌感染的健康番茄植株和健康马铃薯植株茎叶分离的552株细菌进行了自然遗传能力检测。对照菌株baylyacinetobacter ADP1均可转化这两种DNA提取物。质粒pSKTG DNA处理后,未观察到可转化的分离株。我们选择了两个分离株P34(鉴定为琐碎假单胞菌)和A19(鉴定为fragi假单胞菌),这两个分离株是基于rp耐药细胞DNA处理后的抗rp CFU数始终高于野生型细胞。与野生型细胞相比,同源抗rp细胞DNA处理后,P34和A19的抗rp CFU数分别高出2.1倍和1.5倍。由此得出结论,在与番茄和马铃薯植物相关的可培养细菌群落中,能够在体外捕获外源DNA并将其整合到其基因组中的细菌相对较少,或者在转化试验中不满足有利于转化的条件。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Assessment of transformability of bacteria associated with tomato and potato plants.

Transformation of plant-associated bacteria by plant DNA has never been demonstrated in agricultural fields. In total 552 bacterial isolates from stems of Ralstonia solanacearum-infected and healthy tomato plants and from stems and leaves of healthy potato plants were tested for natural genetic competence using plasmid pSKTG DNA and homologous DNA extracts. Control strain Acinetobacter baylyi ADP1 was transformable with both DNA extracts. No transformable isolates were observed after treatment with plasmid pSKTG DNA. Two isolates, P34, identified as Pseudomonas trivialis and A19, identified as Pseudomonas fragi, were selected on the basis of the consistently higher Rp-resistant CFU numbers after treatment with DNA from Rp-resistant cells than with that from wild-type cells. P34 showed 2.1-fold and A19 1.5-fold higher Rp-resistant CFU numbers after treatment with DNA from homologous Rp-resistant cells versus that from wild-type cells. It is concluded that bacteria capable of in vitro capture and integration of exogenous DNA into their genomes are relatively rare in culturable bacterial communities associated with tomato and potato plants, or that conditions conducive to transformation were not met in transformation assays.

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