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氮饥饿导致莱茵衣藻的光合作用产氢。

Nitrogen deprivation results in photosynthetic hydrogen production in Chlamydomonas reinhardtii.

机构信息

AG Photobiotechnologie, Fakultät für Biologie und Biotechnologie, Lehrstuhl für Biochemie der Pflanzen, Ruhr-Universität Bochum, 44780 Bochum, Germany.

出版信息

Planta. 2012 Apr;235(4):729-45. doi: 10.1007/s00425-011-1537-2. Epub 2011 Oct 22.

Abstract

The unicellular green alga Chlamydomonas reinhardtii is able to use photosynthetically provided electrons for the production of molecular hydrogen by an [FeFe]-hydrogenase HYD1 accepting electrons from ferredoxin PetF. Despite the severe sensitivity of HYD1 towards oxygen, a sustained and relatively high photosynthetic hydrogen evolution capacity is established in C. reinhardtii cultures when deprived of sulfur. One of the major electron sources for proton reduction under this condition is the oxidation of starch and subsequent non-photochemical transfer of electrons to the plastoquinone pool. Here we report on the induction of photosynthetic hydrogen production by Chlamydomonas upon nitrogen starvation, a nutritional condition known to trigger the accumulation of large deposits of starch and lipids in the green alga. Photochemistry of photosystem II initially remained on a higher level in nitrogen-starved cells, resulting in a 2-day delay of the onset of hydrogen production compared with sulfur-deprived cells. Furthermore, though nitrogen-depleted cells accumulated large amounts of starch, both hydrogen yields and the extent of starch degradation were significantly lower than upon sulfur deficiency. Starch breakdown rates in nitrogen or sulfur-starved cultures transferred to darkness were comparable in both nutritional conditions. Methyl viologen treatment of illuminated cells significantly enhanced the efficiency of photosystem II photochemistry in sulfur-depleted cells, but had a minor effect on nitrogen-starved algae. Both the degradation of the cytochrome b₆ f complex which occurs in C. reinhardtii upon nitrogen starvation and lower ferredoxin amounts might create a bottleneck impeding the conversion of carbohydrate reserves into hydrogen evolution.

摘要

单细胞绿藻莱茵衣藻能够利用光合作用提供的电子,通过接受来自铁氧还蛋白 PetF 的电子的 [FeFe]-氢化酶 HYD1 来生产氢气。尽管 HYD1 对氧气非常敏感,但在 C. reinhardtii 培养物中剥夺硫时,仍能建立持续且相对较高的光合作用产氢能力。在这种情况下,质子还原的主要电子来源之一是淀粉的氧化和随后的电子向质体醌库的非光化学转移。在这里,我们报告了氮饥饿诱导衣藻光合作用产氢,氮饥饿是一种已知会触发绿藻中大量淀粉和脂质积累的营养条件。光合作用系统 II 的光化学最初在氮饥饿细胞中保持在较高水平,导致与硫剥夺细胞相比,产氢的起始延迟了 2 天。此外,尽管氮饥饿细胞积累了大量的淀粉,但氢气产量和淀粉降解的程度都明显低于硫缺乏。在黑暗中转移到黑暗中的氮或硫饥饿培养物中的淀粉分解速率在两种营养条件下都相当。在硫剥夺细胞中,光照细胞的甲紫精处理显著提高了光合作用系统 II 光化学的效率,但对氮饥饿藻类的影响较小。在氮饥饿时发生在莱茵衣藻中的细胞色素 b₆ f 复合物的降解和铁氧还蛋白数量的减少都可能造成瓶颈,阻碍碳水化合物储备转化为氢气的转化。

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