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缺硫培养6天的水稻幼苗,其叶片和根中的硝酸还原酶(NR)活性明显下降。用1pPm 的6-苄氨基腺嘌呤(6-BA)处理培养了10天的水稻幼苗根系,24小时后缺硫培养的水稻幼苗叶片和根系的 NR 活性升高,加硫培养的水稻幼苗叶片和根中的 NR 活性下降。用~(35)S示踪发现,6-BA 可降低加硫幼苗对~(35)S 的吸收和转化,但促进缺硫幼苗对~(35)S 的转化。  相似文献   

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超结瘤大豆(Glycine m ax (L.) Merr.) nts 382 和不结瘤大豆Nod 49 的叶和根组织水提取物经Sephadex G25 过滤、洗脱,再根据洗脱物对硝酸还原酶(NR)活性的影响可划分为4 个组分(fraction)样品,即nts 382(Nod 49) F1、nts 382(Nod 49) F2、nts 382(Nod 49) F3 和nts 382(Nod 49) F4。其中, nts382 F2 和F4 抑制NR 活性作用在接种USDA110 后明显下降, 但接种的nts 382 F2 却能提高大豆Bragg 的结瘤数达一倍, 而接种的nts 382 F3 和F4 的作用不明显。NR 活性抑制因子不是刺激结瘤的因子, 刺激结瘤的因子主要分布在接种的nts382 F2 部分中。与这一现象相反, Nod 49 F2 和F4 抑制NR活性的作用在接种后更强, 且也抑制大豆nts 382 的结瘤, 其中Nod 49 F4 抑制结瘤的作用基本不能逆转。抑制结瘤因子主要分布在接过种的Nod 49 F4 部分中  相似文献   

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NITRATE REDUCTASE ACTIVITY OF SPHAGNUM SPECIES IN THE SOUTH PENNINES   总被引:4,自引:3,他引:1  
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大豆(Glycine m ax (L.) Merr.)Bragg 及它的突变体, 超结瘤大豆nts 382 和不结瘤大豆Nod 49 的叶片提取物中含有抑制iNR活性、c1NR活性和C2NR活性的抑制成分。300 μE·m - 2·s- 1照度和接种根瘤菌strain USDA110 是形成抑制成分的重要条件。在两种条件下,Nod 49 中的抑制活性最强, nts 382 的最弱, Bragg 的居中。Bragg 的接种根提取物对3 种NR活性的抑制作用基本同于其叶片提取物; nts 382 的接种根提取物也同于其叶片提取物,基本不抑制NR的活性, 但Nod 49 的接种根提取物只抑制叶片的c2NR活性, 不同于其叶片提取物抑制3 种NR活性的作用。结果说明叶片与根两种提取物在抑制叶片NR活性的成分上相关  相似文献   

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短日照对浮萍植物中过氧化物酶和硝酸还原酶活性的影响   总被引:1,自引:0,他引:1  
短日照处理引起Lemna minor的两个日长反应不同的品系,以及Lemna paucicostata6746中硝酸还原酶的体外活性下降.在L. minorGl和L. paucicostala6746两个短日品系中,短日照导致过氧化物酶活性和抗坏血酸含量水平增高.其抗坏血酸含量水平与过氧化物酶的活性水平具有平行增长关系.对日长不敏感的品系L. minorG2中过氧化物酶活性在短日下呈现强烈起伏和随后的衰减.其抗坏血酸含量水平在同期表现连续下降.对两个L. minor品系中过氧化物酶同工酶的比较表明,在不敏感品系中缺乏迁移最快的阴离子酶带,而同一酶带存在于短日照品系中,并呈现明显的被诱导变化.    相似文献   

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DISAPPEARANCE OF NITRATE REDUCTASE ACTIVITY FROM CHLAMYDOMONAS REINHARDI   总被引:2,自引:2,他引:0  
Nitrate reductase activity was induced in Chlamydomonas reinhardi following addition of nitrate. Enzymic activity was assayed in cell-free supernatants and in whole cells whose permeability had been increased by freezing. Nitrate reductase activity in cells decreased rapidly when CO2-fixation was prevented by (a) darkening cultures, (b) aerating cultures with CO2-free air, or (c) addition of DCMU (3-(3,4-dichlorophenyl)-1,1-dimethylurea). A smaller loss of nitrate reductase activity from darkened cells occurred when (a) acetate-adapted cells were supplied with acetate, or (b) cells were allowed to accumulate carbon reserves by nitrogen starvation before darkening. It was concluded that maintenance of nitrate reductase activity was dependent upon the availability of a suitable carbon source.  相似文献   

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The activity of extracted NADH-NO3? reductase was measured in the marine dinoflagellates Amphidinium carteri Hulburt and Cachonina niei Loeblich. Its activity showed a diel periodicity and was ca. twice as great at midday as at midnight. The enzyme activity was unstable, with an in vitro half-life of 2–3 h. Values of enzyme activity were low or undetectable during lag phase but paralleled the instantaneous growth rate value during log phase. Nitrate reductase activity was not found in the stationary phase of growth, but additions of NO3? resulted in enzyme activity after 24h. When A. carteri was exposed to a series of light intensities for several weeks, the division rate and enzyme activity increased with increasing light intensity up to saturating intensities. In 6 h exposures, enzyme activity decreased with decreasing light intensities below light intensities saturating division rate. Additions of NH4+ (0.5–50 μm) to A. carteri cultures decreased the amount of extractable enzyme. The in vitro activity was not inhibited by similar NH+4 concentrations.  相似文献   

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