Your search keyword '"Mizoguchi, Tadashi"' showing total 16 results

1. Glycolipid analyses of light-harvesting chlorosomes from envelope protein mutants of Chlorobaculum tepidum.

Author

Tsukatani Y, Mizoguchi T, Thweatt J, Tank M, Bryant DA, and Tamiaki H

Subjects

Bacterial Proteins metabolism, Bacteriochlorophylls metabolism, Chlorobi genetics, Galactolipids chemistry, Glycolipids metabolism, Light, Models, Structural, Mutation, Organelles metabolism, Bacterial Proteins genetics, Chlorobi metabolism, Galactolipids metabolism, Glycolipids chemistry

Abstract

Chlorosomes are large and efficient light-harvesting organelles in green photosynthetic bacteria, and they characteristically contain large numbers of bacteriochlorophyll c, d, or e molecules. Self-aggregated bacteriochlorophyll pigments are surrounded by a monolayer envelope membrane comprised of glycolipids and Csm proteins. Here, we analyzed glycolipid compositions of chlorosomes from the green sulfur bacterium Chlorobaculum tepidum mutants lacking one, two, or three Csm proteins by HPLC equipped with an evaporative light-scattering detector. The ratio of monogalactosyldiacylglyceride (MGDG) to rhamnosylgalactosyldiacylglyceride (RGDG) was smaller in chlorosomes from mutants lacking two or three proteins in CsmC/D/H motif family than in chlorosomes from the wild-type, whereas chlorosomes lacking CsmIJ showed relatively less RGDG than MGDG. The results suggest that the CsmC, CsmD, CsmH, and other chlorosome proteins are involved in organizing MGDG and RGDG and thereby affect the size and shape of the chlorosome.

Published

2016

2. In Vitro Assays of BciC Showing C132-Demethoxycarbonylase Activity Requisite for Biosynthesis of Chlorosomal Chlorophyll Pigments.

Author

Teramura M, Harada J, Mizoguchi T, Yamamoto K, and Tamiaki H

Subjects

Bacterial Proteins genetics, Bacteriochlorophylls genetics, Biosynthetic Pathways, Chlorobi genetics, Escherichia coli genetics, Escherichia coli metabolism, Kinetics, Methanol, Organelles metabolism, Pigmentation, Recombinant Proteins, Substrate Specificity, Bacterial Proteins metabolism, Bacteriochlorophylls metabolism, Chlorobi enzymology

Abstract

A BciC enzyme is related to the removal of the C13(2)-methoxycarbonyl group in biosynthesis of bacteriochlorophylls (BChls) c, d and e functioning in green sulfur bacteria, filamentous anoxygenic phototrophs and phototrophic acidobacteria. These photosynthetic bacteria have the largest and the most efficient light-harvesting antenna systems, called chlorosomes, containing unique self-aggregates of BChl c, d or e pigments, that lack the C13(2)-methoxycarbonyl group which disturbs chlorosomal self-aggregation. In this study, we characterized the BciC derived from the green sulfur bacterium Chlorobaculum tepidum, and examined the in vitro enzymatic activities of its recombinant protein. The BciC-catalyzing reactions of various substrates showed that the enzyme recognized chlorophyllide (Chlide) a and 3,8-divinyl(DV)-Chlide a as chlorin substrates to give 3-vinyl-bacteriochlorophyllide (3V-BChlide) d and DV-BChlide d, respectively. Since the BciC afforded a higher activity with Chlide a than that with DV-Chlide a and no activity with (DV-)protoChlides a (porphyrin substrates) and 3V-BChlide a (a bacteriochlorin substrate), this enzyme was effective for diverting the chlorosomal pigment biosynthetic pathway at the stage of Chlide a away from syntheses of other pigments such as BChl a and Chl a The addition of methanol to the reaction mixture did not prevent the BciC activity, and we identified this enzyme as Chlide a demethoxycarbonylase, not methylesterase., (© The Author 2016. Published by Oxford University Press on behalf of Japanese Society of Plant Physiologists. All rights reserved. For permissions, please email: journals.permissions@oup.com.)

Published

2016

3. Stereochemical conversion of C3-vinyl group to 1-hydroxyethyl group in bacteriochlorophyll c by the hydratases BchF and BchV: adaptation of green sulfur bacteria to limited-light environments.

Author

Harada J, Teramura M, Mizoguchi T, Tsukatani Y, Yamamoto K, and Tamiaki H

Subjects

Adaptation, Physiological genetics, Cytoplasm, Genes, Bacterial, Organelles metabolism, Photosynthesis, Sequence Deletion, Stereoisomerism, Bacterial Proteins metabolism, Bacteriochlorophylls metabolism, Chlorobi genetics, Chlorobi metabolism, Ethanol metabolism, Hydrolases metabolism, Light

Abstract

Photosynthetic green sulfur bacteria inhabit anaerobic environments with very low-light conditions. To adapt to such environments, these bacteria have evolved efficient light-harvesting antenna complexes called as chlorosomes, which comprise self-aggregated bacteriochlorophyll c in the model green sulfur, bacterium Chlorobaculum tepidum. The pigment possess a hydroxy group at the C3(1) position that produces a chiral center with R- or S-stereochemistry and the C3(1) -hydroxy group serves as a connecting moiety for the self-aggregation. Chlorobaculum tepidum carries the two possible homologous genes for C3-vinyl hydratase, bchF and bchV. In the present study, we constructed deletion mutants of each of these genes. Pigment analyses of the bchF-inactivated mutant, which still has BchV as a sole hydratase, showed higher ratios of S-epimeric bacteriochlorophyll c than the wild-type strain. The heightened prevalence of S-stereoisomers in the mutant was more remarkable at lower light intensities and caused a red shift of the chlorosomal Qy absorption band leading to advantages for light-energy transfer. In contrast, the bchV-mutant possessing only BchF showed a significant decrease of the S-epimers and accumulations of C3-vinyl BChl c species. As trans- criptional level of bchV was upregulated at lower light intensity, the Chlorobaculum tepidum adapted to low-light environments by control of the bchV transcription., (© 2015 The Authors. Molecular Microbiology published by John Wiley & Sons Ltd.)

Published

2015

4. Isolation and characterization of a new bacteriochlorophyll-c bearing a neopentyl substituent at the 8-position from the bciD-deletion mutant of the brown-colored green sulfur bacterium Chlorobaculum limnaeum.

Author

Mizoguchi T, Harada J, Tsukatani Y, and Tamiaki H

Subjects

Chlorobi genetics, Methylation, Mutation, Bacterial Proteins metabolism, Bacteriochlorophylls metabolism, Chlorobi metabolism

Abstract

We recently constructed the mutant of the brown-colored green sulfur bacterium Chlorobaculum limnaeum lacking BciD which was responsible for formation of a formyl group at the 7-position in bacteriochlorophyll(BChl)-e biosynthesis. This mutant exclusively gave BChl-c, but not BChl-e, as the chlorosome pigments (Harada et al. in PLoS One 8(4):e60026, 2013). By the mutation, the homolog and epimer composition of the pigment was drastically altered. The methylation at the 8(2)-position in the mutant cells proceeded to create BChl-c carrying large alkyl substituents at this position. Correspondingly, the content of BChls-c having the (S)-configuration at the chiral 3(1)-position remarkably increased and accounted for 80.6 % of the total BChl-c. Based on the alteration of the pigment composition in the mutant cells, a new BChl-c bearing the bulkiest, triple 8(2)-methylated neopentyl substituent at the 8-position ([N,E]BChl-c) was identified. The molecular structure of [N,E]BChl-c was fully determined by its NMR, mass, and circular dichroism spectra. The newly identified [N,E]BChl-c was epimerically pure at the chiral 3(1)-position and its stereochemistry was determined to be an (S)-configuration by modified Mosher's method. Further, the effects of the C8(2)-methylation on the optical absorption properties of monomeric BChls-c were investigated. The Soret but not Qy absorption bands shifted to longer wavelengths by the extra methylation (at most 1.4 nm). The C8(2)-methylation induced a slight but apparent effect on absorption properties of BChls-c in their monomeric states.

Published

2014

5. Biosynthesis of bacteriochlorophyll c derivatives possessing chlorine and bromine atoms at the terminus of esterifying chains in the green sulfur bacterium Chlorobaculum tepidum.

Author

Saga Y, Hayashi K, Mizoguchi T, and Tamiaki H

Subjects

Bacteriochlorophylls chemistry, Bromine analysis, Chlorine analysis, Chlorobi chemistry, Esterification, Bacterial Proteins chemistry, Bacteriochlorophylls biosynthesis, Chlorobi metabolism

Abstract

The green sulfur photosynthetic bacterium Chlorobaculum tepidum newly produced BChl c derivatives possessing a chlorine or bromine atom at the terminus of the esterifying chain in the 17-propionate residue by cultivation with exogenous ω-halo-1-alkanols. The relative ratios of BChl c derivatives esterified with 8-chloro-1-octanol and 10-chloro-1-decanol were estimated to be 26.5% and 33.3% by cultivation with these ω-chloro-1-alkanols at the final concentrations of 300 and 150 μM, respectively. In contrast, smaller amounts of unnatural BChls c esterified with ω-bromo-1-alkanols were biosynthesized than those esterified with ω-chloro-1-alkanols: the ratios of BChl c derivatives esterified with 8-bromo-1-octanol and 10-bromo-1-decanol were 11.3% and 12.2% at the concentrations of 300 and 150 μM, respectively. These indicate that ω-chloro-1-alkanols can be incorporated into bacteriochlorophyllide c more than ω-bromo-1-alkanols in the BChl c biosynthetic pathway. The homolog compositions of the novel BChl c derivatives possessing a halogen atom were analogous to those of coexisting natural BChl c esterified with farnesol. These results demonstrate unique properties of BChl c synthase, BchK, which can utilize unnatural substrates containing halogen in the BChl c biosynthesis of Cba. tepidum., (Copyright © 2014 The Society for Biotechnology, Japan. Published by Elsevier B.V. All rights reserved.)

Published

2014

6. Isolation and structural determination of C8-vinyl-bacteriochlorophyll d from the bciA and bchU double mutant of the green sulfur bacterium Chlorobaculum tepidum.

Author

Harada J, Mizoguchi T, Nomura K, and Tamiaki H

Subjects

Chlorobi genetics, Circular Dichroism, Magnetic Resonance Spectroscopy, Mutation, Bacteriochlorophylls chemistry, Chlorobi metabolism

Abstract

The mutant lacking enzymes BciA and BchU, that catalyzed reduction of the C8-vinyl group and methylation at the C20 position of bacteriochlorophyll (BChl) c, respectively, in the green sulfur bacterium Chlorobaculum tepidum, were constructed. This mutant accumulated C8-vinyl-BChl d derivatives, and a molecular structure of the major pigment was fully characterized by its NMR, mass, and circular dichroism spectra, as well as by chemical modification: (3(1) R)-8-vinyl-12-ethyl-(R[V,E])BChl d was confirmed as a new BChl d species in the cells. In vitro chlorosome-like self-aggregates of this pigment were prepared in an aqueous micellar solution, and formed more rapidly than those of (3(1) R)-8,12-diethyl-(R[E,E])BChl d isolated from the green sulfur bacterium Chlorobaculum parvum NCIB8327d synthesizing BChl d homologs. Their red-shifted Q y absorption bands were almost the same at 761 nm, and the value was larger than those of in vitro self-aggregates of R[E,E]BChl c (737 nm) and R[V,E]BChl c (726 nm), while the monomeric states of the former gave Q y bands at shorter wavelengths than those of the latter. Red shifts by self-aggregation of the two BChl d species were estimated to be 110 nm and much larger than those by BChls c (75 nm for [E,E] and 64 nm for [V,E]).

Published

2014

7. Bacteriochlorophyll homolog compositions in the bchU mutants of green sulfur bacteria.

Author

Tsukatani Y, Harada J, Mizoguchi T, and Tamiaki H

Subjects

Bacteriochlorophylls analysis, Bacteriochlorophylls chemistry, Chromatography, High Pressure Liquid, Methylation, Methyltransferases genetics, Mutation, Stereoisomerism, Bacterial Proteins genetics, Bacterial Proteins metabolism, Bacteriochlorophylls metabolism, Chlorobi enzymology, Chlorobi genetics, Methyltransferases metabolism

Abstract

Chlorosomes of the green sulfur bacterium Chlorobaculum limnaeum contain a large number of self-aggregated bacteriochlorophyll (BChl) e molecules. The ΔbchU mutant of this organism lacks BchU, a C20-methyltransferase, and therefore produces BChl f, which is the C20-unsubstituted form of BChl e. The BChl e homolog compositions, in terms of degrees of C8(2)-methylation, were not changed in the wild type during growth, while the BChl f homolog patterns in the mutant were significantly altered at various time periods of growth. BChl f with an isobutyl group at the C8 position was dominant at the early stage of growth, whereas the proportion of BChl f with the C8-ethyl group increased in the late exponential phase. We also constructed the ΔbchU mutant of C. tepidum which originally produces BChl c: the mutant therefore produces BChl d. BChl d homologs highly methylated at the C8(2) position also increased in the ΔbchU mutant of C. tedium compared to those in the wild type. These phenomena suggest that BchU interferes with the methylation ability of BchQ, a C8(2)-methyltransferase, and that the enzymes might compete in terms of obtaining S-adenosyl-methionine, the source of a methyl group. As a result, when grown to the late log phase, the ΔbchU mutant of C. limnaeum had similar heterogeneities of pigment homolog compositions compared to those in the wild type. Chlorosomes with a high proportion of C8-ethylated BChl homologs might be important for fine-tuning the light-harvesting or energy-transfer efficiency. Chlorosomes of the ΔbchU mutants at the various growth stages will be good materials for investigating effects of C8(2)-methylations on supramolecular structures of self-aggregated pigments.

Published

2013

8. Cyclopropane-ring formation in the acyl groups of chlorosome glycolipids is crucial for acid resistance of green bacterial antenna systems.

Author

Mizoguchi T, Tsukatani Y, Harada J, Takasaki S, Yoshitomi T, and Tamiaki H

Subjects

Acylation, Bacterial Proteins chemistry, Bacteriochlorophylls chemistry, Chlorobi chemistry, Cyclopropanes chemistry, Fatty Acids chemistry, Glycolipids chemistry, Bacterial Proteins metabolism, Bacteriochlorophylls metabolism, Chlorobi cytology, Chlorobi metabolism, Cyclopropanes metabolism, Fatty Acids metabolism, Glycolipids metabolism

Abstract

Green photosynthetic bacteria have unique light-harvesting antenna systems called chlorosomes. Chlorobaculum tepidum, a model organism of the bacteria, biosynthesized monogalactosyl- and rhamnosylgalactosyldiacylglycerides possessing a methylene-bridged palmitoleyl group characterized by a cis-substituted cyclopropane ring as the dominant glycolipids of its chlorosome surface. The formation of the cyclopropane ring was chemically inhibited by supplementation of sinefungin, an analog of S-adenosyl-L-methionine, into the bacterial cultivation. The presence of the cyclopropane ring reinforced acid resistance of the light-harvesting chlorosomes and suppressed acidic demetalation (pheophytinization) of bacteriochlorophyll-c pigments constructing the core part of chlorosomes. The ring-formation would represent direct and post-synthetic modifications of chlorosome membrane properties and was tolerant of acidic environments., (Copyright © 2013 Elsevier Ltd. All rights reserved.)

Published

2013

9. Specific gene bciD for C7-methyl oxidation in bacteriochlorophyll e biosynthesis of brown-colored green sulfur bacteria.

Author

Harada J, Mizoguchi T, Satoh S, Tsukatani Y, Yokono M, Noguchi M, Tanaka A, and Tamiaki H

Subjects

Bacterial Proteins genetics, Bacteriochlorophylls genetics, Chlorobi genetics, Chlorobium genetics, Gene Expression, Mutagenesis, Insertional, Bacterial Proteins biosynthesis, Bacteriochlorophylls biosynthesis, Chlorobi enzymology, Chlorobium enzymology

Abstract

The gene named bciD, which encodes the enzyme involved in C7-formylation in bacteriochlorophyll e biosynthesis, was found and investigated by insertional inactivation in the brown-colored green sulfur bacterium Chlorobaculum limnaeum (previously called Chlorobium phaeobacteroides). The bciD mutant cells were green in color, and accumulated bacteriochlorophyll c homologs bearing the 7-methyl group, compared to C7-formylated BChl e homologs in the wild type. BChl-c homolog compositions in the mutant were further different from those in Chlorobaculum tepidum which originally produced BChl c: (3(1) S)-8-isobutyl-12-ethyl-BChl c was unusually predominant.

Published

2013

10. Characterization of chlorophyll pigments in the mutant lacking 8-vinyl reductase of green photosynthetic bacterium Chlorobaculum tepidum.

Author

Mizoguchi T, Harada J, and Tamiaki H

Subjects

Bacteriochlorophylls metabolism, Chlorobi chemistry, Chlorobi metabolism, Gene Deletion, Oxidation-Reduction, Bacteriochlorophylls chemistry, Chlorobi enzymology, Chlorobi genetics, Oxidoreductases genetics

Abstract

The mutant lacking the enzyme BciA (renamed CT1063), which catalyzed reduction of the 8-vinyl group of a porphyrinoid-type 3,8-divinyl-(proto)chlorophyllide-a [DV-(P)Chlide-a] in the green sulfur bacterium Chlorobaculum (Cba.) tepidum, was reconstructed on the basis of the previous study reported by Chew and Bryant [J. Biol. Chem.2007, 282, 2967-2975]. Cba. tepidum biosynthesizes the following three different types of chlorophylls (Chls) through their common precursory DV-(P)Chlide-a as its photosynthetically active pigments: bacteriochlorophyll(BChl)-c and Chl-a with the partially reduced 17,18-trans-dihydroporphyrin and BChl-a with the further reduced 7,8-trans-17,18-trans-tetrahydroporphyrin. The structures of Chls thus produced were characterized in detail by various spectroscopic techniques. In the mutant, both BChl-c and Chl-a possessing the alkyl group at the 8-position were exclusively replaced by their 8-vinylated derivatives, whereas BChl-a possessed the original 8-ethyl group. The present observations were inconsistent with the previous report. However, it was apparently confirmed that the enzyme BciA was responsible for the reduction of DV-(P)Chlide-a to produce BChl-c and Chl-a. Noteworthily, exclusive accumulation of the reduced (8-ethylated) form of BChl-a, not its 8-vinylated derivative, in the mutant indicates the presence of another enzyme catalyzing the 8-vinyl reduction as yet unidentified or any other reduction mechanism using a known enzyme to yield BChl-a., (Copyright © 2012 Elsevier Ltd. All rights reserved.)

Published

2012

11. A seventh bacterial chlorophyll driving a large light-harvesting antenna.

Author

Harada J, Mizoguchi T, Tsukatani Y, Noguchi M, and Tamiaki H

Subjects

Bacterial Proteins genetics, Bacteriochlorophylls isolation & purification, Bacteriochlorophylls metabolism, Chlorobi genetics, Chlorobi growth & development, Gene Knockout Techniques, Genes, Bacterial, Methyltransferases genetics, Photosynthesis, Phycobiliproteins isolation & purification, Phycobiliproteins metabolism, Spectrophotometry, Ultraviolet, Bacteriochlorophylls chemistry, Chlorobi metabolism, Phycobiliproteins chemistry

Abstract

The discovery of new chlorophyllous pigments would provide greater understanding of the mechanisms and evolution of photosynthesis. Bacteriochlorophyll f has never been observed in nature, although this name was proposed ~40 years ago based on structurally related compounds. We constructed a bacteriochlorophyll f-accumulating mutant of the green sulfur bacterium Chlorobaculum limnaeum, which originally produced bacteriochlorophyll e, by knocking out the bchU gene encoding C-20 methyltransferase based on natural transformation. This novel pigment self-aggregates in an in vivo light-harvesting antenna, the chlorosome, and exhibits a Q(y) peak of 705 nm, more blue-shifted than any other chlorosome reported so far; the peak overlaps the maximum (~700 nm) of the solar photon flux spectrum. Bacteriochlorophyll f chlorosomes can transfer light energy from core aggregated pigments to another bacteriochlorophyll in the chlorosomal envelope across an energy gap of ~100 nm, and is thus a promising material for development of new bioenergy applications.

Published

2012

12. Biosynthesis of unnatural bacteriochlorophyll c derivatives esterified with α,ω-diols in the green sulfur photosynthetic bacterium Chlorobaculum tepidum.

Author

Nishimori R, Mizoguchi T, Tamiaki H, Kashimura S, and Saga Y

Subjects

Circular Dichroism, Farnesol chemistry, Farnesol metabolism, Photosynthesis, Bacterial Proteins biosynthesis, Bacteriochlorophylls biosynthesis, Chlorobi metabolism, Sulfur metabolism

Abstract

Unnatural bacteriochlorophyll (BChl) c derivatives possessing a hydroxy group at the terminus of a hydrocarbon chain at the 17-propionate were biosynthesized in the green sulfur photosynthetic bacterium Chlorobaculum tepidum. Addition of exogenous 1,8-octanediol, 1,12-dodecanediol, and 1,16-hexadecanediol in acetone to liquid cultures resulted in accumulation of BChl c monoesterified with the corresponding diols. The relative ratios of the novel BChl c derivatives esterified with 1,8-, 1,12-, and 1,16-diols to totally producing BChl c were 8.2, 50.2, and 57.6% in the cells grown with additive α,ω-diols at concentrations of 1.5, 0.06, and 0.06 mM, respectively, at the final concentration. The homologue composition of BChl c derivatives esterified with these α,ω-diols was similar to that of original, coexisting BChl c esterified with farnesol (BChl c(F)), suggesting that esterification of α,ω-diols occurred at the last step of the BChl c biosynthetic pathway by BChl c synthase, BchK, in the same manner as in BChl c(F). Chlorosomes, which were isolated from cells grown in the presence of exogenous α,ω-diols, contained a ratio and a composition of BChl c derivatives esterified with the diols similar to those in the whole cells, indicating that these BChl c derivatives were actually present in chlorosomes. Q(y) absorption bands of C. tepidum cells containing the novel BChl c derivatives were shifted to a shorter wavelength, although their bandwidths were analogous to those of cells obtained by normal cultivation. Circular dichroism spectra of cells that had BChl c derivatives esterified with α,ω-diols exhibited S-shaped signals in the Q(y) region, whose polarities were the reverse of those of cells grown in the normal medium and by supplementation with neat acetone as a control experiment. These spectral features of C. tepidum possessing BChl c derivatives esterified with α,ω-diols imply that the novel BChl c derivatives possessing a hydroxy group at the terminus of a hydrocarbon chain affect their self-assembly in chlorosomes.

Published

2011

13. In vitro synthesis and characterization of bacteriochlorophyll-f and its absence in bacteriochlorophyll-e producing organisms.

Author

Tamiaki H, Komada J, Kunieda M, Fukai K, Yoshitomi T, Harada J, and Mizoguchi T

Subjects

Bacteriochlorophylls chemical synthesis, Bacteriochlorophylls chemistry, Chlorophyll chemistry, Chlorophyll isolation & purification, Chromatography, High Pressure Liquid, Spinacia oleracea chemistry, Bacteriochlorophylls biosynthesis, Chlorobi metabolism

Abstract

Bacteriochlorophyll(BChl)-f which has not yet been found in natural phototrophs was prepared by chemically modifying chlorophyll-b. The retention time of reverse-phase high-performance liquid chromatography of the synthetic monomeric BChl-f as well as its visible absorption and fluorescence emission spectra in a solution were identified and compared with other naturally occurring chlorophyll pigments obtained from the main light-harvesting antenna systems of green sulfur bacteria, BChls-c/d/e. Based on the above data, BChl-f was below the level of detection in three strains of green photosynthetic bacteria producing BChl-e.

Published

2011

14. Stereochemical determination of chlorophyll-d molecule from Acaryochloris marina and its modification to a self-aggregative chlorophyll as a model of green photosynthetic bacterial antennae.

Author

Mizoguchi T, Shoji A, Kunieda M, Miyashita H, Tsuchiya T, Mimuro M, and Tamiaki H

Subjects

Bacteriochlorophylls chemical synthesis, Chromatography, High Pressure Liquid, Molecular Conformation, Pyridines chemistry, Sensitivity and Specificity, Spectrum Analysis, Stereoisomerism, Titrimetry, Bacteriochlorophylls chemistry, Chlorobi chemistry, Chlorophyll chemistry, Cyanobacteria chemistry

Abstract

Acaryochloris marina is a unique photosynthetic prokaryote containing chlorophyll(Chl)-d as a major photoactive pigment (over 95%). The molecular structure of Chl-d is proposed as the 3-formyl analog of Chl-a. However, the stereochemistry of Chl-d at the 13(2)-, 17- and 18-positions has not yet been established unambiguously. In the first part of this paper, we describe the determination of their stereochemistries to be 13(2)-(R)-, 17-(S)- and 18-(S)-configurations by using 1H-1H NOE correlations in 1H-NMR and circular dichroism spectra as well as chemical modification of Chl-a to produce stereochemically defined Chl derivatives. In the second part of the paper, we report a facile synthesis of a self-aggregative Chl by modifying isolated Chl-d. Since Chl-d was characterized by its reactive 3-formyl group, the formyl group was reduced with t-BuNH2BH3 to afford the desirable Chl, 3-deformyl-3-hydroxymethyl-pyrochlorophyll-d (3(1)-OH-pyroChl-d). The synthetic 3(1)-OH-pyroChl-d molecules spontaneously self-organized to form well-ordered aggregates in a non-polar organic solvent. The self-aggregates are a good model of major light-harvesting antenna systems of green photosynthetic bacteria, chlorosomes, in terms of the following three findings. (1) Both the red-shifted electronic absorption band above 750 nm and its induced reverse S-shape CD signal around 750 nm were observed in 0.5% (v/v) THF-cyclohexane. (2) The stretching mode of the 13-carbonyl group was downshifted by about 35 cm(-1) from the wavenumber of its free carbonyl. (3) The self-aggregates were quite stable on titration of pyridine to the suspension, in comparison with those of natural chlorosomal bacteriochlorophyll-d possessing the 3-(1-hydroxyethyl) group.

Published

2006

15. Isolation and structure determination of a complete set of bacteriochlorophyll-d homologs and epimers from a green sulfur bacterium Chlorobium vibrioforme and their aggregation properties in hydrophobic solvents.

Author

Mizoguchi T, Saga Y, and Tamiaki H

Subjects

Chlorophyll chemistry, Chlorophyll isolation & purification, Dimerization, Mass Spectrometry, Molecular Structure, Nuclear Magnetic Resonance, Biomolecular, Stereoisomerism, Chlorobi chemistry, Chlorophyll analogs & derivatives

Abstract

Eight bacteriochlorophyll (BChl)-d homologs and epimers were isolated from a strain of the green sulfur bacterium Chlorobium vibrioforme. By a combination of mass spectrometry and 1H-NMR spectroscopy using the chemical shifts of meso- and 3(1)-protons and 1H-1H NOE correlations, the molecular structures were determined as (3(1)R)-8-ethyl-12-methyl, (3'R)-8-ethyl-12-ethyl, (3(1)R)-8-propyl-12-methyl, (3(1)S)-8-propyl-12-methyl, (3(1)R)-8-propyl-12-ethyl, (3(1)S)-8-propyl-12-ethyl, (3(1)S)-8-isobutyl-12-methyl and (3(1)S)-8-isobutyl-12-ethyl. The aggregation behavior of the epimerically pure BChls-d in hydrophobic organic solvents was examined to investigate the absolute configuration of the 3-(1-hydroxyethyl) group as well as the bulkiness of the C8 and C12 side-chains by using electronic-absorption and fluorescence-emission spectroscopies At high concentration of the BChls-d in CH2Cl2, the absolute configuration of the 3-(1-hydroxyethyl) group governed the formation of a subunit as a building block for the subsequent higher assembly. Upon dilution of the resulting subunit with hexane, the bulkiness of the C8 and C12 side-chains were found to affect the association of the subunits differently: the bulkiness of the C8 side-chain acted as a promoter for the association due to a stabilized hydrophobic interaction among the relevant larger side-chain, whereas the bulkiness of the C12 side-chain acted as an inhibitor for that association due to introduction of a particular steric-hindrance around the side-chain in the aggregates.

Published

2002

16. Spectral heterogeneity in single light-harvesting chlorosomes from green sulfur photosynthetic bacterium chlorobium tepidum.

Author

Saga Y, Wazawa T, Mizoguchi T, Ishii Y, Yanagida T, and Tamiaki H

Subjects

Spectrometry, Fluorescence, Chlorobi chemistry, Light, Microscopy, Fluorescence methods, Organelles chemistry

Abstract

The fluorescence emission properties of single chlorosomes from the green sulfur photosynthetic bacterium Chlorobium (Chl.) tepidum are studied for the first time, using a total internal reflection fluorescence microscope. The fluorescence peak positions of bacteriochlorophyll (BChl)-c self-aggregates in a single chlorosome of Chl. tepidum were widely distributed in the wavelength region between 750 and 768 nm, and the standard deviation (s.d. = 4.1 nm, n = 51) was larger than that of single chlorosomes of Chloroflexus (Cfl.) (s.d. = 1.9 nm, n = 50). The spectral heterogeneity among single chlorosomes from Chl. tepidum was in sharp contrast to those from Cfl. aurantiacus. The difference of chlorosomal spectral properties between Chl. tepidum and Cfl. aurantiacus at the single-unit level would be ascribed to the homolog composition of BChl-c--chlorosomes of Chl. tepidum have BChl substituted with various alkyl groups at both the 8- and 12-positions, whereas light-harvesting BChl-c molecules in Cfl. chlorosomes have the same substituents at the 8- (ethyl group) and 12- (methyl group) positions.

Published

2002