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大豆胚轴萌发过程中超氧阴离子和过氧化氢的代谢

Superoxide anion and hydrogen peroxide metabolism in soybean embryonic axes during germination.

作者信息

Puntarulo S, Galleano M, Sanchez R A, Boveris A

机构信息

Instituto de Química y Fisicoquímica Biológicas, Facultad de Farmacia y Bioquímica, Universidad de Buenos Aires, Argentina.

出版信息

Biochim Biophys Acta. 1991 Jul 8;1074(2):277-83. doi: 10.1016/0304-4165(91)90164-c.

Abstract

The total rate of mitochondrial O2- production in the presence of NADH as substrate increased from 200 to 1340 pmol/min per axis between 2 and 30 h of imbibition. The activities of the enzymes involved in hydroperoxide metabolism, e.g., superoxide dismutase, catalase, peroxidase and glutathione and ascorbate peroxidases, markedly changed during the germination of soybean embryonic axes. Superoxide dismutase was the enzymatic activity affected the most during the initial stages of germination. Intracellular O2- steady-state concentration, calculated from the rate of O2- production and superoxide dismutase activity, showed a 2-fold increase from 2 x 10(-8) M to 4 x 10(-8) M in germination phase I, declined in phase II to 2 x 10(-8) M and remained constant over the rest of the incubation period. The reaction of H2O2 and luminol catalyzed by Co2+ was utilized to measure H2O2 diffused out of the soybean axes after 5 to 10 min of incubation. The catalase-sensitive luminol emission of diffusates prepared from axes previously imbibed from 2 to 30 h corresponded to a H2O2 intracellular steady-state concentration in the range of 0.3 to 0.9 microM. The activity of metal-containing antioxidant enzymes was determined in the extracellular fluid. Cell wall peroxidase activity increased from 10 to 300 mumol/min per mg protein and appears as a potentially important pathway for H2O2 utilization. Hydrogen peroxide metabolism in soybean embryonic axes during early inhibition appears to have the following main features: (a) mitochondrial membranes are the most important source of cytosolic O2- and H2O2; (b) H2O2 is regulated at a steady-state concentration of 0.3-0.9 microM; (c) catalase is the main enzyme in terms of H2O2 utilization; (d) H2O2 exo-diffusion is quantitatively important destiny of intracellular H2O2; and (e) extracellular peroxidase located at the cell wall affords an enzymatic system able to use diffused H2O2.

摘要

以NADH为底物时,线粒体O₂⁻产生的总速率在吸胀2至30小时之间从每轴200皮摩尔/分钟增加到1340皮摩尔/分钟。在大豆胚轴萌发过程中,参与过氧化氢代谢的酶如超氧化物歧化酶、过氧化氢酶、过氧化物酶以及谷胱甘肽过氧化物酶和抗坏血酸过氧化物酶的活性发生了显著变化。超氧化物歧化酶是在萌发初期受影响最大的酶活性。根据O₂⁻产生速率和超氧化物歧化酶活性计算的细胞内O₂⁻稳态浓度在萌发第一阶段从2×10⁻⁸M增加了2倍至4×10⁻⁸M,在第二阶段下降至2×10⁻⁸M,并在其余孵育期保持恒定。利用Co²⁺催化的H₂O₂与鲁米诺的反应来测量孵育5至10分钟后从大豆胚轴中扩散出的H₂O₂。由先前吸胀2至30小时的胚轴制备的扩散物对过氧化氢酶敏感的鲁米诺发射对应于细胞内H₂O₂稳态浓度在0.3至0.9微摩尔范围内。在细胞外液中测定了含金属抗氧化酶的活性。细胞壁过氧化物酶活性从每毫克蛋白质10微摩尔/分钟增加到300微摩尔/分钟,似乎是H₂O₂利用的一个潜在重要途径。大豆胚轴早期抑制期间的过氧化氢代谢似乎具有以下主要特征:(a)线粒体膜是胞质O₂⁻和H₂O₂的最重要来源;(b)H₂O₂在0.3 - 0.9微摩尔的稳态浓度下受到调节;(c)就H₂O₂利用而言,过氧化氢酶是主要酶;(d)H₂O₂外扩散是细胞内H₂O₂的重要定量命运;(e)位于细胞壁的细胞外过氧化物酶提供了一个能够利用扩散的H₂O₂的酶系统。

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