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蓝绿藻隐球藻6714中光系统II对大分子合成的调控

Photosystem II regulation of macromolecule synthesis in the blue-green alga Aphanocapsa 6714.

作者信息

Pelroy R A, Kirk M R, Bassham J A

出版信息

J Bacteriol. 1976 Nov;128(2):623-32. doi: 10.1128/jb.128.2.623-632.1976.

Abstract

Polymers synthesized by heterotrophically growing (glucose as carbon source) cultures of Aphanocapsa 6714 were compared with polymers synthesized in photosynthetically grown cultures. Loss of photosystem II by dark incubation, or inhibition of light-grown cells with the photosystem II-specific inhibitor dichlorophenylmethylurea, caused an 80 to 90% reduction in the rate of lipid and total ribonucleic acid synthesis, and more than a 90% reduction in the rate of protein synthesis. In contrast, glycogen synthesis was reduced only about 50% in dark cells and less than 30% in dichlorphenylmethylurea-inhibited cells. After longer heterotrophic growth, glycogen became the major component, whereas in photosynthetically grown cultures protein was the major constituent. 14C (from 14CO2 and/or [14C]glucose) assimilated into protein by heterotrophically grown cells was found in amino acids in nearly the same proportions as in photosynthetically grown cells. Thus, routes of biosynthesis available to autotropic cells were also available to heterotrophic cultures, but the supply of carbon precursors to those pathways was greatly reduced. The limited biosynthesis in heterotrophic cells was not due to a limitation for cellular energy. The adenylates were maintained at nearly the same concentrations (and hence the energy charge also) as in photosynthetic cells. The concentration of reduced nicotinamide adenine dinucleotide phosphate was higher in heterotrophic (dark) cells than in photosynthetic cells. From rates of CO2 fixation and/or glycogen biosynthesis it was determined that stationary-phase cells expended approximately 835, 165, and less than 42 nmol of adenosine 5'-triphosphate per mg (dry weight) of algae per 30 min during photosynthetic, photoheterotrophic, and chemoheterotrophic metabolism, respectively. Analysis of the soluble metabolite pools in dark heterotrophic cultures by double-labeling experiments revealed rapid equilibration of 14C through the monophosphate pools, but much slower movement of label into the diphosphate pools of fructose-1,6-diphosphate and sedoheptulose-1,7-diphosphate. Carbon did flow into 3-phosphoglycerate in the dark; however, the initial rate was low and the concentration of this metabolite soon fell to an undetectable level. In photosynthetic cells, 14C quickly equilibrated throughout all the intermediates of the reductive pentose cycle, in particular, into 3-phosphoglycerate. Analysis of glucose-6-phosphate dehydrogenase in cell extracts showed that the enzyme was very sensitive to product inhibition by reduced nicotinamide adenine dinucleotide.

摘要

将以葡萄糖为碳源异养生长的聚球藻6714培养物合成的聚合物与光合生长培养物合成的聚合物进行了比较。通过暗培养使光系统II丧失功能,或用特异性抑制光系统II的二氯苯基甲基脲处理光合生长的细胞,导致脂质和总核糖核酸合成速率降低80%至90%,蛋白质合成速率降低超过90%。相比之下,糖原合成在暗处理细胞中仅降低约50%,在二氯苯基甲基脲抑制的细胞中降低不到30%。在更长时间的异养生长后,糖原成为主要成分,而在光合生长的培养物中蛋白质是主要成分。异养生长细胞同化到蛋白质中的14C(来自14CO2和/或[14C]葡萄糖)在氨基酸中的比例与光合生长细胞中几乎相同。因此,自养细胞可用的生物合成途径异养培养物也可用,但这些途径的碳前体供应大大减少。异养细胞中有限的生物合成并非由于细胞能量受限。腺苷酸维持在与光合细胞几乎相同的浓度(因此能量电荷也相同)。还原型烟酰胺腺嘌呤二核苷酸磷酸的浓度在异养(暗)细胞中高于光合细胞。根据二氧化碳固定和/或糖原生物合成速率确定,在光合、光异养和化能异养代谢过程中,静止期细胞每毫克(干重)藻类每30分钟分别消耗约835、165和不到42纳摩尔的腺苷5'-三磷酸。通过双标记实验分析暗异养培养物中的可溶性代谢物库发现,14C通过单磷酸库快速平衡,但标记进入果糖-1,6-二磷酸和景天庚酮糖-1,7-二磷酸的二磷酸库的移动要慢得多。碳在黑暗中确实流入了3-磷酸甘油酸;然而,初始速率很低,这种代谢物的浓度很快降至无法检测的水平。在光合细胞中,14C在还原戊糖循环的所有中间体中迅速平衡,特别是进入3-磷酸甘油酸。对细胞提取物中葡萄糖-6-磷酸脱氢酶的分析表明,该酶对还原型烟酰胺腺嘌呤二核苷酸的产物抑制非常敏感。

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