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Construction of Two Vectors for a Bypass of Monocotyledon Plants Photorespiration

机译:两个载体的构建单圈植物旁路的光素

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In order to modify the photorespiration of monocotyledonous crops, we aimed to construct vectors that will be used to introduce a bypass to the native photorespiration pathway. Firstly, we cloned the encoding sequences of glyoxylate carboligase (GCL) and tartronic semialdehyde reductase (TSR) from E. coli, glycolate dehydrogenase (GDH) from Arabidopsis thaliana and chloroplast transit peptide (cTP) from rice. Then we constructed a universal vector pEXP harboring the encoding sequence of cTP for targeting a protein into chloroplast. By insertion of these three encoding sequences into the universal vector pEXP, we obtained the expression cassettes for GCL, TSR and GDH, respectively. Finally, we inserted the cassettes for GCL and TSR in tandem into the binary vector pCAMBIA 1301, and for GDH into another binary vector, pPGN, to obtain our plant expression vectors pCAMBIA 1301-TG and pPGN-GDH, respectively. These two expression vectors possess different selection resistance and can be used to transform monocots together, to introduce the bypass pathway of photorespiration. By this way, the transgenic plants can recycle glycolate, the by-product of photosynthesis in C_3 plants, within the chloroplast, simultaneously, save energy and avoid the loss of ammonia, which will contribute to improved growth.
机译:为了改变单圈的作物的光抑制,我们旨在构造将用于引入天然光荧光途径旁路的载体。首先,我们克隆了从大肠杆菌,乙酸盐脱氢酶(GDH)的甘油酯钩状酶(GCL)和TSR)的编码序列,从亚洲稻草中,来自水稻的叶绿体过渡肽(CTP)。然后我们构建了一种普遍的载体P,含有CTP的编码序列,用于靶向蛋白质。通过将这三个编码序列插入通用载体PEXP中,我们分别为GCL,TSR和GDH获得了表达式盒。最后,我们将GCL和TSR的盒式串联插入二元载体PCAMBIA 1301,以及GDH进入另一个二元载体PPGN,以分别获得PCAMBIA 1301-TG和PPGN-GDH。这两种表达载体具有不同的选择性电阻,并且可用于将单像转换在一起,以引入光呼吸的旁路通路。通过这种方式,转基因植物可以再循环乙酸酯,在C_3植物中的光合作用副产物,同时节省能量,避免氨的丧失,这将有助于提高生长。

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