The Regulation of Chlorophyll Biosynthesis by the Action of Protochlorophyllide on glut-RNA-Ligase

The pigment mutant C-2A' of the green alga Scenedesmus obliquus accumulates considerable amounts of protochlorophyllide (PChlide), when grown in darkness. In this paper it is demonstrated that the accumulated PChlide directly acts on ^glut-RNA-ligase and thereby blocks further biosynthesis of ALA and chlorophyll. By increasing the amount of ligase at constant concentrations of PChlide and ^glut-RNA it could clearly be demonstrated that PChlide directly inhibits ligase activity and does not act on the t-RNA. The inhibitory effect of other tetrapyrroles like chlorophyll a, pheophytin a and protoporphyrin IX was much less effective even at oversaturating concentrations.     

Origin and evolution of the light-dependent protochlorophyllide oxidoreductase (LPOR) genes

Abstract: Light‐dependent NADPH‐protochlorophyllide oxidoreductase (LPOR) is a nuclear‐encoded chloroplast protein in green algae and higher plants which catalyzes the light‐dependent reduction of protochlorophyllide to chlorophyllide. Light‐dependent chlorophyll biosynthesis occurs in all oxygenic photosynthetic organisms. With the exception of angiosperms, this pathway coexists with a separate light‐independent chlorophyll biosynthetic pathway, which is catalyzed by light‐independent protochlorophyllide reductase (DPOR) in the dark. In contrast, the light‐dependent function of chlorophyll biosynthesis is absent from anoxygenic photosynthetic bacteria. Consequently, the question is whether cyanobacteria are the ancestors of all organisms that conduct light‐dependent chlorophyll biosynthesis. If so, how did photosynthetic eukaryotes acquire the homologous genes of LPOR in their nuclear genomes? The large number of complete genome sequences now available allow us to detect the evolutionary history of LPOR genes by conducting a genome‐wide sequence comparison and phylogenetic analysis. Here, we show the results of a detailed phylogenetic analysis of LPOR and other functionally related enzymes in the short chain dehydrogenase/reductase (SDR) family. We propose that the LPOR gene originated in the cyanobacterial genome before the divergence of eukaryotic photosynthetic organisms. We postulated that the photosynthetic eukaryotes obtained their LPOR homologues through endosymbiotic gene transfer.     

The photoenzymatic cycle of NADPH: protochlorophyllide oxidoreductase in primary bean leaves (<Emphasis Type="Italic">Phaseolus vulgaris</Emphasis>) during the first days of photoperiodic growth

The photoenzymatic cycle of the light-dependent NADPH:protochlorophyllide oxidoreductase (LPOR) was investigated in situ during early stages of development of bean leaves under light-dark cycles (LDC). In the experimental system used in this study, prolamellar bodies developed during night periods and disappeared during light periods. This was accompanied by changes in the photoactive to non-photoactive Pchlide ratio, which was higher at the end of the light period, and tended to increase with the number of LDC's. Flash-induced absorbance changes in the Chlide absorption region (700 nm) were used in order to monitor the formation of short- and long-wavelength forms of Chlide (C670-675 and C682-694), which correspond to free Chlide and aggregated Chlide-NADPH-LPOR complexes, respectively. The ratio of long-wavelength to short-wavelength Chlides after one flash increased with the number of LDC's, and was higher in leaves collected at the end of light periods, compared to leaves collected at the end of night periods. During light periods, photoactive Pchlide regeneration and Chlide phytylation were completed within 1 min after flash-induced formation of long-wavelength Chlide. The results show for the first time that the photoenzymatic LPOR cycle proceeds through similar steps, but at much faster rates, during photoperiodic greening than in the previously studied leaves of etiolated plants. In particular, the parallel formation of two Chlide species always occurs, but the ratio of the two species depends on the ratio of photoactive to non-photoactive Pchlide and on light or dark adaptation.     

Dramatic Enhancement of CO2 Photoreduction by Biodegradable Light‐Management Paper

Photocatalytic reduction of CO₂ with H₂O vapor is gaining increased interest because it is a promising “green chemistry” route for the direct conversion of CO₂ to value‐added chemicals driven by solar energy. To increase the efficiency of photocatalytic conversion, most efforts are made by exploring various photocatalysts while little effort on advanced light management. For the first time, it is demonstrated that bio‐degradable transparent paper with excellent light diffusivity can effectively enhance the light utilization of photocatalytic reactions when attached on the device surface, and thus greatly increase the conversion efficiency. As a proof‐of‐concept, a graphitic carbon nitride (g‐C₃N₄) photocatalyst with transparent paper attached, exhibited 1.5 times higher photocatalytic activity than bare g‐C₃N₄ in the reduction of CO₂ under visible light irradiation. The improved catalytic performance can be ascribed to the (1) refractive index matching and (2) enhanced light absorption via prolonged light traveling path in transparent paper, which decreases the light reflection at surface and traps the absorbed light inside, leading to an increased light absorption at the active layer of the device. The transparent paper with a controllable light management behavior has an unprecedented potential for applications in photocatalysis as a general method for improved light utilization.     

Detection of protoporphyrin IX in envelope membranes of pea chloroplasts

Envelope membranes were prepared from mature pea chloroplasts. The tetrapyrrole contents of envelope membranes were analysed. The envelope membranes of pea chloroplasts contained substantial amounts of protoporphyrin IX and trace amounts of Mg-protoporphyrin IX and its monoester in addition to protochlorophyllide. The protoporphyrin IX content of envelope membranes was 89.25 pmol (mg protein)(-1). Its content in pea envelope membrane was higher than that of protochlorophyllide. The proportion of monovinyl and divinyl forms of protochlorophyllide present in pea chloroplast envelope membrane was 3:7. The significance of the presence of protoporphyrin IX in the envelope membrane is discussed in relation to plastidic Chl biosynthesis.     

木本植物阳生和阴生叶片叶绿体O_2和NO_2~-光还原作用

在有ＰＣＲ和ＰＣＯ环活性抑制剂甘油醛和光合磷酸化解偶联剂ＮＨ４ＣＬ存在下,比较了生长于 ３种 光环境的乔木黧蒴和灌木九节幼苗阳生和阴生叶片叶绿体的Ｏ２和ＮＯ２光还原速率。全自然光下两种 植物阳生叶片的叶绿体Ｏ２的光还原速率最高,占总光合电子传递活性的６６％－６８％,ＮＯ２光还原速率 也有类似趋势占总电子传递的１１％－１５％左右。３６％和１６％自然光下阴生叶片Ｏ２和ＮＯ２光还原 速率及Ｏ２光还原电子传递的比例显著降低,但ＮＯ２光还原电子传递的比例不受影响。与ＮＯ２光还原 相关的叶片ＮｉＲ和ＮＲ活性及ＮｉＲ／ＮＲ活性比也因叶片接受光强度大小而异,随光强减弱,黧蒴的 ＮｉＲ活性降低,九节的ＮＲ活性增高,但黧蒴的ＮＲ活性和九节的ＮｉＲ活性变化未达差异显著性。     

A possible physiological function of the oxygen-photoreducing system of Rhodospirillum rubrum

Anaerobic suspensions of Rhodospirillum rubrum cells which had been grown in the dark under low oxygen tension showed only a small increase of their ATP content when illuminated for 30 s. The same suspensions failed to start immediate growth in the light. Both high light-induced ATP levels and immediate phototrophic growth were elicited by small amounts of oxygen which were insufficient by themselves to raise the ATP levels or to support growth in the dark. The oxygen requirement for growth disappeared after some time of anaerobic illumination and was not observed in suspensions of cells which had been grown in the light under anaerobiosis. Furthermore, these phototrophic cells reached the maximum levels of ATP when illuminated in the absence of oxygen.Strain F11, a mutant derivative of Rhodospirillum rubrum which lacked the ability to photoreduce oxygen in vitro, needed abnormally high amounts of oxygen to increase its ATP levels and to grow in the light. Besides, KCN inhibited the increase of ATP levels in illuminated mutant cells but not wild type cells. An additional difference between both strains was that the oxygen requirement for growth did not disappear in the mutant after some time of anaerobic incubation in the light.To explain these observations, it is proposed that the photosynthetic system of semiaerobically-grown Rhodospirillum rubrum becomes overreduced under anaerobiosis. The oxygen-photoreducing system, which is impaired in the mutant, is apparently used to oxidize the photosynthetic system to its optimal redox state, carrying electrons to oxygen or to other endogenous acceptors which are formed during incubation in the light. The mutant seems to replace the defective system by a cyanide-sensitive pathway which may reduce oxygen but not the alternative endogenous acceptors.     

Photochemical Behavior of 2-Azidopurine Tri-O-Acetylribonucleoside in Aqueous Solution: Unprecedented Transformation into 1-(5′-O-Acetyl-β-D-Ribofuranosyl)-5-[(2-Oxo-1,3,5-Oxadiazocan-4-Ylidene)Amino]-1H-Imidazole-4-Carbaldehyde

The photochemical behavior of 2-azidopurine 2′,3′,5′-tri-O-acetylribonucleoside has been investigated in aqueous solution under aerobic and anaerobic conditions. The two major processes under anaerobic irradiation of 2-azidopurine 2′,3′,5′-tri-O-acetylribonucleoside involve unprecedented transformation into 1-(5′-O-acetyl-β-D-ribofuranosyl)-5-[(2-oxo-1,3,5-oxadiazocan-4-ylidene)amino]-1H-imidazole-4-carbaldehyde and photoreduction to respective 2-aminopurine derivative, whereas under aerobic conditions these two processes occur to a much lesser extent and photooxidation to respective 2-nitropurine derivative dominates. The structures of photoproducts formed were confirmed by NMR and high-resolution electrospray ionization mass spectral data.     

Evidence for the contribution of pseudocyclic photophosphorylation to the energy requirement of the mechanism for concentrating inorganic carbon in Chlamydomonas

Mass-spectrometric measurements of ¹⁶O₂ and ¹⁸O₂ were made to compare the rates of light-dependent O₂ evolution and uptake by Chlamydomonas reinhardtii Dang. grown in air (0.035% CO₂; low-C_i cells) or CO₂-enriched air (5% CO₂; high-C_i cells) at pH 5.5 and 8.0. While at pH 5.5, no differences were observed in the isotopic O₂-gas exchange of high- and low-C_i cells, at pH 8.0 the rates of true O₂ evolution and uptake were considerably higher in low-C_i than in high-C_i cells. The enhanced rates of O₂ uptake and evolution by low-C_i cells were completely inducible within 6 h after transferring high-C_i cells to ambient air. At pH 8.0, O₂ uptake in the light was inhibited by 2 M 3-(3,4-dichlorophenyl)-1,1 dimethylurea in both types of alga, but this effect was more pronounced in low-C_i than in high-C_i cells.When the cells were grown at pH 5.5 the activities of the superoxide-radical-degrading enzymes, superoxide dismutase, ascorbate peroxidase, monodehydroascorbate reductase, dehydroascorbate reductase and glutathione reductase, were similar regardless of the CO₂ concentration provided during growth. At pH 8.0, however, the activities of these enzymes were 4 to 20 times higher in low-C_i than in high-C_i cells. When high-C_i cells were allowed to acclimate to ambient air for 6 h at pH 8.0, the activities of superoxide dismutase, ascorbate peroxidase and monodehydroascorbate dehydrogenase increased to more than 50% of the level observed with low-C_i cells. These results are consistent with an enhanced operation of O₂ photoreduction which could provide energy to the inorganic-carbon-concentrating mechanism via pseudo-cyclic photophosphorylation.     

Synthesis and Characterization of Eugenia uniflora L. Silver Nanoparticles and L-Cysteine Sensor Application

L-Cysteine (Cys) is a non-essential sulfur-containing amino acid, crucial for protein synthesis, detoxification, and several metabolic functions. Cys is widely used in the agricultural, food, cosmetic, and pharmaceutical industries. So, a suitable sensitive and selective sensing approach is of great interest, and a low-cost sensor would be necessary. This article presents silver nanoparticles (EuAgNPs) synthesized by a green synthesis method using Eugenia uniflora L. extracts and photoreduction. The nanoparticles were characterized by UV/VIS, transmission electron microscopy, high-performance liquid chromatography (HPLC), FTIR, and Zeta potential. With the addition of Cys in the EuAgNPs solution, the terminal thiol part of L-cysteine binds on the surface of nanoparticles through Ag−S bond. The EuAgNPs and CysAgNPs coexist until flavonoids bound the amino group of Cys, enhancing the red color of solutions. The EuAgNPs provided selectivity to detect Cys among other amino acids, and its detection limit was found to be 3.8 nM. The sensor has the advantages of low-cost synthesis, fast response, high selectivity, and sensitivity.