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海洋聚球藻中叶绿素 d 的 18O 标记表明,叶绿素 a 和分子氧是前体。

18O labeling of chlorophyll d in Acaryochloris marina reveals that chlorophyll a and molecular oxygen are precursors.

机构信息

Schools of Biological Sciences, The University of Sydney, Sydney, New South Wales 2006, Australia.

出版信息

J Biol Chem. 2010 Sep 10;285(37):28450-6. doi: 10.1074/jbc.M110.146753. Epub 2010 Jul 7.

Abstract

The cyanobacterium Acaryochloris marina was cultured in the presence of either H(2)(18)O or (18)O(2), and the newly synthesized chlorophylls (Chl a and Chl d) were isolated using high performance liquid chromatography and analyzed by mass spectroscopy. In the presence of H(2)(18)O, newly synthesized Chl a and d, both incorporated up to four isotopic (18)O atoms. Time course H(2)(18)O labeling experiments showed incorporation of isotopic (18)O atoms originating from H(2)(18)O into Chl a, with over 90% of Chl a (18)O-labeled at 48 h. The incorporation of isotopic (18)O atoms into Chl d upon incubation in H(2)(18)O was slower compared with Chl a with approximately 50% (18)O-labeled Chl d at 115 h. The rapid turnover of newly synthesized Chl a suggested that Chl a is the direct biosynthetic precursor of Chl d. In the presence of (18)O(2) gas, one isotopic (18)O atom was incorporated into Chl a with approximately the same kinetic incorporation rate observed in the H(2)(18)O labeling experiment, reaching over 90% labeling intensity at 48 h. The incorporation of two isotopic (18)O atoms derived from molecular oxygen ((18)O(2)) was observed in the extracted Chl d, and the percentage of double isotopic (18)O-labeled Chl d increased in parallel with the decrease of non-isotopic-labeled Chl d. This clearly indicated that the oxygen atom in the C3(1)-formyl group of Chl d is derived from dioxygen via an oxygenase-type reaction mechanism.

摘要

海洋聚球藻在 H(2)(18)O 或 (18)O(2) 存在的条件下培养,利用高效液相色谱法分离新合成的叶绿素(Chl a 和 Chl d),并用质谱法进行分析。在 H(2)(18)O 存在的情况下,新合成的 Chl a 和 d 都掺入了多达四个同位素 (18)O 原子。时间进程 H(2)(18)O 标记实验表明,来自 H(2)(18)O 的同位素 (18)O 原子掺入到 Chl a 中,在 48 小时时,超过 90%的 Chl a 被 (18)O 标记。与 Chl a 相比,在 H(2)(18)O 孵育时,Chl d 中同位素 (18)O 原子的掺入较慢,在 115 小时时,约有 50%的 Chl d 被 (18)O 标记。新合成的 Chl a 的快速周转表明,Chl a 是 Chl d 的直接生物合成前体。在 (18)O(2)气体存在的情况下,Chl a 中掺入了一个同位素 (18)O 原子,其动力学掺入速率与 H(2)(18)O 标记实验中观察到的相同,在 48 小时时达到超过 90%的标记强度。在提取的 Chl d 中观察到两个源自分子氧的同位素 (18)O 原子的掺入,并且双同位素 (18)O 标记的 Chl d 的百分比与非同位素标记的 Chl d 的减少平行增加。这清楚地表明,Chl d 的 C3(1)-甲酰基中的氧原子源自通过加氧酶型反应机制的氧气。

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