首页> 美国卫生研究院文献>Plant Physiology >Nitrogen Assimilation Pathways in Leaf Mesophyll and Bundle Sheath Cells of C4 Photosynthesis Plants Formulated from Comparative Studies with Digitaria sanguinalis (L.) Scop.
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Nitrogen Assimilation Pathways in Leaf Mesophyll and Bundle Sheath Cells of C4 Photosynthesis Plants Formulated from Comparative Studies with Digitaria sanguinalis (L.) Scop.

机译:根据与洋地黄(Digitaria sanguinalis(L.)Scop)的比较研究制定的C4光合作用植物的叶肉和束鞘细胞中的氮同化途径。

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摘要

Nitrogen assimilation in crabgrass Digitaria sanguinalis (L.) Scop., was studied by comparing leaf extracts with isolated mesophyll cell and bundle sheath strand extracts. The results show that both nitrate and nitrate reductase are localized in mesophyll cells; glutamine synthetase is nearly equally distributed in the mesophyll and bundle sheath; approximately 67% of the glutamate synthase activity is in the bundle sheath and 33% is in the mesophyll; and 80% of the glutamate dehydrogenase activity is in the bundle sheath, with the NADH-dependent form exhibiting a 2.5-fold higher activity than the NADPH-dependent form.Isolated crabgrass mesophyll cells reduce NO2 coupled to the photochemical production of O2 but are inactive with NO3. The NO2 -dependent O2 evolution is light-dependent; inhibited by 3-(3,4-dichlorophenyl)-1,1-dimethylurea; stimulated by photophosphorylation uncouplers; and exhibits a stoichiometry of O2 evolved to NO2 reduced of 1.45 and 0.67 in coupled and uncoupled experiments, respectively. Isolated bundle sheath strands are inactive in O2 evolution with NO3 or NO2.Based on these results, plus literature data, two schemes for crabgrass leaf nitrogen assimilation are presented, depending on whether the plant is using ammonium or nitrate as its nitrogen source. It is proposed that the increased nitrogen use efficiency in crabgrass and other C4 plants is due partially to a “division of labor” between mesophyll and bundle sheath cells, where NO3 and NO2 reductase in mesophyll cells act as nitrogen reduction traps in an analogous fashion to phosphoenolpyruvate carboxylase acting as a CO2 trap during C4 photosynthesis.
机译:通过比较叶提取物与分离的叶肉细胞和束鞘链提取物,研究了马齿Digi(Digitaria sanguinalis(L.)Scop。)的氮同化作用。结果表明,硝酸盐和硝酸盐还原酶均定位于叶肉细胞中。谷氨酰胺合成酶几乎均匀分布在叶肉和束鞘中。谷氨酸合酶活性中约67%位于束鞘中,而33%位于叶肉中。 80%的谷氨酸脱氢酶活性位于束鞘中,NADH依赖性形式的活性比NADPH依赖性形式高2.5倍。分离的马鞭草叶肉细胞减少NO2 -偶联至O2的光化学生成,但与NO3 -无关。依赖于NO2 -的O2的释放是光依赖的;被3-(3,4-二氯苯基)-1,1-二甲基脲抑制;由光磷酸化解偶联剂激发;并在耦合和非耦合实验中分别表现出O2的化学计量,其演变为NO2 -减少1.45和0.67。分离的束鞘链在NO3 -或NO2 -的O2释放中不起作用。基于这些结果,加上文献数据,提出了两种对马尾草叶氮同化的方案,具体取决于是否使用铵盐或硝酸盐作为氮源。有人提出,在草木和其他C4植物中提高的氮利用效率部分归因于叶肉和束鞘细胞之间的“分工”,其中NO3 -和NO2 -

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