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利用基因打靶技术进行高色氨酸水稻的设计突变育种。

Application of gene targeting to designed mutation breeding of high-tryptophan rice.

机构信息

Plant Genome Engineering Research Unit, Agrogenomics Research Center, National Institute of Agrobiological Sciences, Tsukuba, Ibaraki 305-8602, Japan.

出版信息

Plant Physiol. 2011 Jul;156(3):1269-77. doi: 10.1104/pp.111.175778. Epub 2011 May 4.

Abstract

Site-directed mutagenesis via gene targeting (GT) based on homologous recombination is the ultimate mutation breeding technology because it enables useful information acquired from structural- and computational-based protein engineering to be applied directly to molecular breeding, including metabolic engineering, of crops. Here, we employed this rationale to introduce precise mutations in OASA2--an α-subunit of anthranilate synthase that is a key enzyme of tryptophan (Trp) biosynthesis in rice (Oryza sativa)--via GT, with subsequent selection of GT cells using a Trp analog. The expression level of OASA2 in plants homozygous and heterozygous for modified OASA2 was similar to that of nontransformants, suggesting that OASA2 transcription in GT plants was controlled in the same manner as endogenous OASA2, and that GT could lead to a lower risk of gene silencing than in conventional overexpression approaches. Moreover, we showed that enzymatic properties deduced from protein engineering or in vitro analysis could be reproduced in GT plants as evidenced by Trp accumulation levels. Interestingly, mature seeds of homozygous GT plants accumulated Trp levels 230-fold higher than in nontransformants without any apparent morphological or developmental changes. Thus, we have succeeded in producing a novel rice plant of great potential nutritional benefit for both man and livestock that could not have been selected using conventional mutagenesis approaches. Our results demonstrate the effectiveness of directed crop improvement by combining precision mutagenesis via GT with a knowledge of protein engineering.

摘要

通过基于同源重组的基因靶向(GT)进行的定点突变是最终的突变育种技术,因为它使我们能够将从基于结构和计算的蛋白质工程中获得的有用信息直接应用于作物的分子育种,包括代谢工程。在这里,我们通过 GT 在水稻(Oryza sativa)中天冬氨酸氨甲酰基转移酶 2(OASA2)--色氨酸(Trp)生物合成的关键酶--的α亚基中引入精确的突变,随后使用 Trp 类似物选择 GT 细胞。修饰的 OASA2 纯合和杂合植物中 OASA2 的表达水平与非转化体相似,这表明 GT 植物中 OASA2 的转录与内源性 OASA2 以相同的方式控制,并且 GT 可能比传统的过表达方法导致基因沉默的风险更低。此外,我们表明,从蛋白质工程或体外分析推断出的酶学特性可以在 GT 植物中重现,这可以从 Trp 积累水平上得到证明。有趣的是,纯合 GT 植物的成熟种子积累的 Trp 水平比非转化体高 230 倍,而没有任何明显的形态或发育变化。因此,我们成功地生产出了一种新型的水稻植物,它对人类和家畜具有巨大的潜在营养价值,这是传统诱变方法无法选择的。我们的结果表明,通过将 GT 介导的精确诱变与蛋白质工程知识相结合,可以有效地进行定向作物改良。

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