Cho H J, Brotherton J E, Song H S, Widholm J M
Department of Crop Sciences, University of Illinois, Edward R. Madigan Laboratory, 1201 West Gregory, Urbana, Illinois 61801, USA.
Plant Physiol. 2000 Jul;123(3):1069-76. doi: 10.1104/pp.123.3.1069.
A cDNA clone that encodes a feedback-insensitive anthranilate synthase (AS), ASA2, isolated from a 5-methyl-tryptophan (Trp) (5MT)-resistant tobacco cell line under the control of the constitutive cauliflower mosaic virus 35S promoter, was introduced into the forage legume Astragalus sinicus by Agrobacterium rhizogenes with kanamycin selection. The 35S-ASA2 gene was expressed constitutively as demonstrated by northern-blot hybridization analyses and the presence of feedback-insensitive AS. Hairy root lines transformed with 35S-ASA2 grew in concentrations of up to 100 microM 5MT, whereas the controls were completely inhibited by 15 microM 5MT. Expression of the feedback-insensitive ASA2 resulted in a 1.3- to 5.5-fold increase in free Trp. Kinetic studies of the AS activity demonstrate the Trp feedback alterations and indicate that the ASA2 alpha-subunit can interact with the native A. sinicus beta-subunit to form an active enzyme. The ASA2 transcript and high free Trp were also detected in the leaves, stems, and roots of plants regenerated from the transformed hairy roots. Thus, we show for the first time that ASA2 can be used to transform plants of a different species to increase the levels of the essential amino acid Trp and impart 5MT resistance.
从5-甲基色氨酸(Trp)(5MT)抗性烟草细胞系中分离出一个编码反馈不敏感型邻氨基苯甲酸合成酶(AS)即ASA2的cDNA克隆,该克隆在组成型花椰菜花叶病毒35S启动子的控制下,通过发根农杆菌介导并经卡那霉素筛选被导入豆科牧草紫云英中。Northern杂交分析和反馈不敏感型AS的存在证明35S-ASA2基因组成型表达。用35S-ASA2转化的毛状根系能在高达100微摩尔/升的5MT浓度下生长,而对照在15微摩尔/升的5MT时就完全受到抑制。反馈不敏感型ASA2的表达使游离Trp增加了1.3至5.5倍。对AS活性的动力学研究表明了Trp反馈的改变,并表明ASA2α亚基可与天然紫云英β亚基相互作用形成一种活性酶。在从转化的毛状根再生的植株的叶、茎和根中也检测到了ASA2转录本和高含量的游离Trp。因此,我们首次表明ASA2可用于转化不同物种的植物,以提高必需氨基酸Trp的水平并赋予5MT抗性。
