首页> 美国卫生研究院文献>Plant Physiology >Alcohol Dehydrogenase and Pyruvate Decarboxylase Activity in Leaves and Roots of Eastern Cottonwood (Populus deltoides Bartr.) and Soybean (Glycine max L.)
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Alcohol Dehydrogenase and Pyruvate Decarboxylase Activity in Leaves and Roots of Eastern Cottonwood (Populus deltoides Bartr.) and Soybean (Glycine max L.)

机译:东部三角叶杨(Populus deltoides Bartr。)和大豆(Glycine max L.)叶片和根中的乙醇脱氢酶和丙酮酸脱羧酶活性

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摘要

Pyruvate decarboxylase (PDC, EC 4.1.1.1) and alcohol dehydrogenase (ADH, EC 1.1.1.1) are responsible for the anaerobic production of acetaldehyde and ethanol in higher plants. In developing soybean embryos, ADH activity increased upon imbibition and then declined exponentially with development, and was undetectable in leaves by 30 days after imbibition. PDC was not detectable in soybean leaves. In contrast, ADH activity remained high in developing cottonwood seedlings, with no decline in activity during development. ADH activity in the first fully expanded leaf of cottonwood was 230 micromoles NADH oxidized per minute per gram dry weight, and increased with leaf age. Maximal PDC activity of cottonwood leaves was 10 micromoles NADH oxidized per minute per gram dry weight. ADH activity in cottonwood roots was induced by anaerobic stress, increasing from 58 to 205 micromoles NADH oxidized per minute per gram dry weight in intact plants in 48 hours, and from 38 to 246 micromoles NADH oxidized per minute per gram dry weight in detached roots in 48 hours. Leaf ADH activity increased by 10 to 20% on exposure to anaerobic conditions. Crude leaf enzyme extracts with high ADH activity reduced little or no NADH when other aldehydes, such as trans-2-hexenal, were provided as substrate. ADH and PDC are constitutive enzyme in cottonwood leaves, but their metabolic role is not known.
机译:丙酮酸脱羧酶(PDC,EC 4.1.1.1)和醇脱氢酶(ADH,EC 1.1.1.1)负责高等植物中乙醛和乙醇的厌氧生产。在发育中的大豆胚中,ADH活性在吸收后增加,然后随发育呈指数下降,并且在吸收后30天未在叶片中检测到。在大豆叶片中未检测到PDC。相反,在发育的杨木幼苗中,ADH活性仍然很高,而在发育过程中活性没有下降。三叶草的第一个完全膨胀的叶片中的ADH活性为每克干重每分钟230微摩尔NADH氧化,并随叶龄的增加而增加。三角叶杨叶的最大PDC活性是每克干重每分钟氧化10微摩尔NADH。在缺氧胁迫下,杨木根中的ADH活性由无氧胁迫诱导,在48小时内,每克干重每分钟氧化的NADH从每分钟干重氧化58到205微摩尔NADH,每克干重中氧化每分钟干重从每分钟38到246微摩尔NADH。 48小时。暴露于厌氧条件下,叶片ADH活性增加了10%至20%。当提供其他醛(例如反式-2-己醛)作为底物时,具有高ADH活性的粗叶酶提取物几乎不降低NADH或不降低NADH。 ADH和PDC是杨木叶片中的组成酶,但其代谢作用尚不清楚。

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