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在博氏鞘丝藻中过表达光依赖型原叶绿素酸酯氧化还原酶的黄化蓝藻细胞中形成类原片层体超微结构。

Formation of prolamellar-body-like ultrastructures in etiolated cyanobacterial cells overexpressing light-dependent protochlorophyllide oxidoreductase in Leptolyngbya boryana.

作者信息

Yamamoto Haruki, Kojima-Ando Hiroko, Ohki Kaori, Fujita Yuichi

机构信息

Graduate School of Bioagricultural Sciences, Nagoya University.

Department of Marine Bioscience, Faculty of Biotechnology, Fukui Prefectural University.

出版信息

J Gen Appl Microbiol. 2020 Jun 17;66(2):129-139. doi: 10.2323/jgam.2020.01.009. Epub 2020 Apr 2.

DOI:10.2323/jgam.2020.01.009
PMID:32238622
Abstract

Protochlorophyllide (Pchlide) reduction is the penultimate step of chlorophyll (Chl) biosynthesis, and is catalyzed by two evolutionarily unrelated enzymes: dark-operative Pchlide oxidoreductase (DPOR) and light-dependent Pchlide oxidoreductase (LPOR). Because LPOR is the sole Pchlide reductase in angiosperms, dark-grown seedlings of angiosperms become etiolated. LPOR exists as a ternary complex of Pchlide-NADPH-LPOR to form paracrystalline prolamellar bodies (PLBs) in etioplasts. Because LPOR is distributed ubiquitously across oxygenic phototrophs including cyanobacteria, it would be important to determine whether cyanobacterial LPOR has the ability to form PLBs. We isolated a DPOR-less transformant ΔchlL/LPORox, carrying a plasmid to overexpress cyanobacterial LPOR in the cyanobacterium Leptolyngbya boryana. The transformant did not produce Chl in the dark and became etiolated with an accumulation of Pchlide and LPOR. Novel PLB-like ultrastructures were observed in etiolated cells, which disappeared during the early stage of the light-dependent greening process. However, the rate of Chl production in the greening process of ΔchlL/LPORox was almost the same as that observed in the control cells, which carried an empty vector. An in vitro LPOR assay of extracts of dark-grown ΔchlL/LPORox cells suggested that the PLB-like structures are deficient in NADPH. Low-temperature fluorescence emission spectra of membrane fractions of the etiolated cells indicated the absence of the photoactive form of Pchlide, which was consistent with the inefficiency of the greening process. Cyanobacterial LPOR exhibited an intrinsic ability to form PLB-like ultrastructures in the presence of the co-accumulation of Pchlide; however, the PLB-like structure differed from the authentic PLB regarding NADPH deficiency.

摘要

原叶绿素酸酯(Pchlide)还原是叶绿素(Chl)生物合成的倒数第二步,由两种在进化上无关的酶催化:暗操作的Pchlide氧化还原酶(DPOR)和光依赖的Pchlide氧化还原酶(LPOR)。由于LPOR是被子植物中唯一的Pchlide还原酶,因此被子植物的黑暗生长幼苗会黄化。LPOR以Pchlide-NADPH-LPOR三元复合物的形式存在,在黄化质体中形成准晶体原片层体(PLB)。由于LPOR广泛分布于包括蓝细菌在内的产氧光合生物中,因此确定蓝细菌LPOR是否具有形成PLB的能力很重要。我们分离出了一个缺失DPOR的转化体ΔchlL/LPORox,它携带一个质粒,用于在蓝细菌博氏细鞘丝藻中过表达蓝细菌LPOR。该转化体在黑暗中不产生Chl,并且由于Pchlide和LPOR的积累而黄化。在黄化细胞中观察到了新型的类PLB超微结构,这些结构在光依赖的绿化过程早期消失。然而,ΔchlL/LPORox绿化过程中Chl的产生速率与携带空载体的对照细胞中观察到的速率几乎相同。对黑暗生长的ΔchlL/LPORox细胞提取物进行的体外LPOR测定表明类PLB结构缺乏NADPH。黄化细胞的膜部分的低温荧光发射光谱表明不存在光活性形式的Pchlide,这与绿化过程的低效性一致。在Pchlide共同积累的情况下,蓝细菌LPOR表现出形成类PLB超微结构的内在能力;然而,类PLB结构在NADPH缺乏方面与真正的PLB不同。

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