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链霉菌属橄榄绿链霉菌 ATCC11238 中的一个家族 19 几丁质酶(Chit30)在转基因豌豆中表达,影响哈茨木霉在体外的发育。

A family 19 chitinase (Chit30) from Streptomyces olivaceoviridis ATCC 11238 expressed in transgenic pea affects the development of T. harzianum in vitro.

机构信息

Institute of Plant Genetics, Leibniz University of Hannover, Herrenhäuserstr. 2, D-30419 Hannover, Germany.

出版信息

J Biotechnol. 2009 Sep 25;143(4):302-8. doi: 10.1016/j.jbiotec.2009.08.011. Epub 2009 Aug 21.

Abstract

Embryo axes excised from mature seeds of pea (Pisum sativum L.) cv. 'Sponsor' were used as explants for Agrobacterium-mediated transformation using pGreenII 0229 binary vectors. The vectors harbored a chimeric chitinase gene (chit30), driven by the constitutive 35S promoter or the elicitor inducible stilbene synthase (vst) promoter from grape (Vitis vinifera L.). The secretion signal of the bacterial chitinase gene from Streptomyces olivaceoviridis ATCC 11238 (DSM 41433) was replaced by the A. thaliana basic chitinase leader sequence. Functional properties of the recombinant gene were tested in tobacco as a model system before the long process of pea transformation was undertaken. Several transgenic pea clones were obtained and the transgenic nature confirmed by different molecular methods. The accumulation and activity of chitinase in stably transformed plants were examined by Western blot analysis and in-gel assays, which showed the presence of an additional 3 isoform bands. Using in vitro bioassays with Trichoderma harzanium as a model, we found an inhibition or delay of hyphal extension, which might indicate enhanced antifungal activity compared with non-transformed pea plants. Up to the 4th generation, the transgenic plants did not show any phenotypic alterations compared with non-transgenic control plants.

摘要

从成熟豌豆(Pisum sativum L.) cv. 'Sponsor'种子中切取的胚胎轴被用作农杆菌介导转化的外植体,使用 pGreenII 0229 二元载体。载体携带嵌合几丁质酶基因(chit30),由组成型 35S 启动子或葡萄(Vitis vinifera L.)诱导的芪合酶(vst)启动子驱动。来自链霉菌橄榄色变种(Streptomyces olivaceoviridis ATCC 11238(DSM 41433)的细菌几丁质酶基因的分泌信号被拟南芥碱性几丁质酶前导序列取代。在进行豌豆的长期转化过程之前,将重组基因的功能特性在烟草中作为模型系统进行了测试。获得了几个转基因豌豆克隆,并通过不同的分子方法证实了其转化特性。通过 Western blot 分析和胶内测定法检测了稳定转化植物中几丁质酶的积累和活性,结果显示存在另外的 3 种同工型条带。使用木霉(Trichoderma harzanium)作为模型的体外生物测定法,我们发现了菌丝延伸的抑制或延迟,这可能表明与非转化的豌豆植物相比,具有增强的抗真菌活性。与非转化对照植物相比,转基因植物在第 4 代之前没有表现出任何表型改变。

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