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Enzymic and Photosynthetic Characteristics of Reciprocal F1 Hybrids of Flaveria pringlei (C3) and Flaveria brownii (C4-Like Species) 1

机译:黄萎病菌(C3)和棕黄病菌(C4-like种)1的互作F1杂种的酶促和光合特性

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摘要

The activities of key C4 enzymes in gel-filtered, whole-leaf extracts and the photosynthetic characteristics for reciprocal F1 hybrids of Flaveria pringlei (C3) and F. brownii (C4-like species) were measured to determine whether any inherited C4-photosynthetic traits are responsible for their reduced CO2 compensation concentration values (AS Holaday, S Talkmitt, ME Doohan Plant Sci 41: 31-39). The activities of phosphoenolpyruvate carboxylase, pyruvate, orthophosphate dikinase, and NADP-malic enzyme (ME) for the reciprocal hybrids are only about 7 to 17% of those for F. brownii, but are three- to fivefold greater than the activities for F. pringlei. The low activities of these enzymes in the hybrids appear to be the result of a partial dominance of F. pringlei genes over certain F. brownii genes. However, no such dominance occurs with respect to the expression of genes for NADP-malate dehydrogenase, which is as active in the hybrids as in F. brownii. In contrast to the situation with the enzymes above, cytoplasmic factors appear to determine the inheritance of NAD-ME. The NAD-ME activity in each hybrid is comparable to that in the respective maternal parent. Pulse-chase 14CO2 incorporation analyses at ambient CO2 levels indicate that the hybrids initially assimilate 7 to 9% of the total assimilated CO2 into C4 acids as compared to 3.5% for F. pringlei. In the hybrids, the percentage of 14C in malate decreases from an average of 6.5 to 2.1% after a 60-second chase in 12CO2/air. However, this apparent C4-cycle activity is too limited or inefficient to substantially alter CO2 exchange from that in F. pringlei, since the values of net photosynthesis and O2 inhibition of photosynthesis are similar for the hybrids and F. pringlei. Also, the ratio of the internal to the external CO2 concentration and the initial slopes of the plot of CO2 concentration versus net photosynthesis are essentially the same for the hybrids and F. pringlei. At 45 micromoles CO2 per mole and 0.21 mole O2 per mole, the hybrids assimilate nearly fivefold more CO2 into C4 acids than does F. pringlei. Some turnover of the malate pool occurs in the hybrids, but the labelling of the photorespiratory metabolites, glycine and serine, is the same in these plants as it is in F. pringlei. Thus, although limited C4-acid metabolism may operate in the hybrids, we conclude that it is not effective in altering O2 inhibition of CO2 assimilation. The ability of the hybrids to assimilate more CO2 via phosphoenolpyruvate carboxylase at low levels of CO2 than does F. pringlei may result in an increased rate of reassimilation of photorespiratory CO2 and CO2 compensation concentrations below that of their C3 parent. If the hybrids do possess a limited C4 cycle, it must operate intracellularly. They are not likely to have inherited an intercellular compartmentation of C4 enzymes, since F. brownii has incomplete compartmentation of key C3 and C4 enzymes.
机译:通过凝胶过滤的全叶提取物中关键C4酶的活性以及黄萎病菌(C3)和棕褐病菌(C4样物种)的倒数F1杂种的光合特性来测定是否有遗传的C4光合特性降低其二氧化碳补偿浓度值的原因(AS Holaday,S Talkmitt,ME Doohan Plant Sci 41:31-39)。相互杂交的磷酸烯醇丙酮酸羧化酶,丙酮酸,正磷酸二激酶和NADP-苹果酸酶(ME)的活性仅为棕褐线虫的约7-17%,但比F.的活性高三到五倍。普林莱。这些酶在杂种中的低活性似乎是由于F.pringlei基因相对于某些F. brownii基因部分优势所致。然而,就NADP-苹果酸脱氢酶的基因表达而言,没有这样的优势,NADP-苹果酸脱氢酶在杂种中的活性与褐褐葡萄球菌一样。与上述酶的情况相反,细胞质因子似乎决定了NAD-ME的遗传。每个杂种中的NAD-ME活性与相应母本中的NAD-ME活性相当。在环境CO2水平下进行脉冲追逐14CO2掺入分析表明,杂种最初将总被吸收的CO2的7%至9%吸收到C4酸中,而F. pringlei则为3.5%。在杂种中,在12CO2 /空气中追逐60秒后,苹果酸中14C的百分比从平均6.5%下降至2.1%。但是,这种表观的C4循环活性太有限或效率低下,无法从F. pringlei实质上改变CO2交换,因为杂种和F. pringlei的净光合作用和O2抑制光合作用的值相似。同样,内部和外部CO 2浓度的比率以及CO 2浓度对净光合作用的曲线的初始斜率对于杂种和F. Fringlei基本上是相同的。在每摩尔45微摩尔的CO2和每摩尔0.21摩尔的O2的情况下,杂种将C2酸中的CO2吸收量比拟南芥提高了近五倍。在杂种中苹果酸池有一些周转,但是这些植物中的光呼吸代谢产物甘氨酸和丝氨酸的标记与F. pringlei中的相同。因此,尽管有限的C4酸代谢可能在杂种中起作用,但我们得出结论,它不能有效地改变O2对CO2同化的抑制作用。杂种通过磷酸烯醇丙酮酸羧化酶在较低水平的CO2上吸收更多的CO2的能力比F. Fringlei可能导致光呼吸CO2的重新同化率增加,并且CO2补偿浓度低于其C3亲本。如果杂种确实具有有限的C4循环,则它必须在细胞内运行。它们不太可能继承了C4酶的细胞间区隔,因为布朗氏酵母对关键C3和C4酶的区隔不完全。

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