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Enhancement of the Essential Amino Acid Composition of Food Crop Proteins through Biotechnology

机译:通过生物技术增强食品作物蛋白质的必需氨基酸组成

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Lack of essential amino acids (EAA) in the diet of at-risk populations could beget a state of food insecurity. Plant proteins are deficient in some essential amino acids. Animals obtain EAA from plant sources. Simple biotechnologies are being developed for improving the EAA composition of crop proteins. The aim was to integrate-discriminate glycolysis and citric-glyoxylic acid cycles to optimize biosynthesis of EAA in food crops. Permutation of diverse metabolic pathways at the mRNA level by glutamate dehydrogenase (GDH)-synthesized RNA is a common biotechnology for doubling the nutritious compositions of plants. Peanuts were planted in plots and treated with mineral salts mixed according to stoichiometric ratios. Protein-bounded and free amino acids of mature peanut seeds were determined by HPLC. GDH-synthesized RNA probes homologous to the mRNAs encoding glyceraldehyde-3-phosphate dehydrogenase (GAPDH), phosphoglycerate mutase (PGlycM), phosphoenolpyruvate carboxylase (PEPCase), enolase, malate dehydrogenase (MDH), isocitrate lyase (ICL), and malate synthase (MS) were prepared from peanut seeds using restriction fragment double differential display PCR method. Northern assays of peanut total RNA showed that the mRNAs encoding PGlycM, PEPCase, MDH, and MS shared extensive sequence homologies that produced a dense network of cross-talks, resulting to co-differential silencing of the mRNAs thereby permuting glycolysis, citric-glyoxylic acid cycles. There were 42 permutations in the NPPKtreated, 105 in control, 420 in KN-, and NPKS-treated peanuts. Because of permutations involving the mRNAs encoding ICL and MS, wherever the abundances of these mRNAs were high (control, and NPPK-treated peanuts) the concentrations of the α-ketoglutarate group of total glutamate, glutamine, arginine, proline, and histidine were minimized (28.0 mg/g). The integration of glycolysis, citric and glyoxylic acid cycles increased the quality and doubled the concentrations of the protein-bounded EAA composition of NPPK-treated (33.37 mg/g) compared with the control peanut (15.66 mg/g). The commanding biotechnology was the stoichiometric mineral salts-based induction of GDH to synthesize the RNAs that integrated glycolysis, citric-glyoxylic acid cycles to one functional unit.
机译:高危人群饮食中缺乏必需氨基酸(EAA)可能会导致粮食不安全状况。植物蛋白缺乏某些必需氨基酸。动物从植物来源获得EAA。正在开发简单的生物技术来改善农作物蛋白质的EAA组成。目的是整合-区分糖酵解和柠檬酸-乙醛酸循环,以优化粮食作物中EAA的生物合成。谷氨酸脱氢酶(GDH)合成的RNA在mRNA水平上对多种代谢途径进行置换是一种使植物营养成分加倍的常见生物技术。将花生种植在小块中,并根据化学计量比用混合的无机盐处理。通过HPLC测定成熟花生种子的蛋白质结合和游离氨基酸。 GDH合成的RNA探针与编码3-磷酸甘油醛脱氢酶(GAPDH),磷酸甘油酸酯变位酶(PGlycM),磷酸烯醇丙酮酸羧化酶(PEPCase),烯醇酶,苹果酸脱氢酶(MDH),异柠檬酸裂合酶(ICL)和苹果酸合酶的mRNA同源MS)是使用限制性片段双重差异显示PCR方法从花生种子制备的。花生总RNA的Northern分析表明,编码PGlycM,PEPCase,MDH和MS的mRNA共有广泛的序列同源性,产生了密集的串扰网络,导致mRNA的共差异沉默,从而置换了糖酵解,柠檬酸-乙醛酸。周期。 NPPK处理过的花生中有42种排列,对照中有105种,KN处理和NPKS处理过的花生有420种排列。由于涉及编码ICL和MS的mRNA的排列,无论这些mRNA的丰度很高(对照和NPPK处理的花生),总谷氨酸,谷氨酰胺,精氨酸,脯氨酸和组氨酸中α-酮戊二酸组的浓度均降至最低(28.0 mg / g)。与对照花生(15.66 mg / g)相比,糖酵解,柠檬酸和乙醛酸循环的整合提高了质量,NPPK处理的蛋白质结合的EAA组合物(33.37 mg / g)的浓度增加了一倍。主导的生物技术是基于化学计量的无机盐的GDH诱导,以合成将糖酵解,柠檬酸-乙醛酸循环整合到一个功能单元的RNA。

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