Sponge-derived Ageladine A affects the in vivo fluorescence emission spectra of microalgae

Carolin Peter; Silke Thoms; Florian Koch; Franz Josef Sartoris; Ulf Bickmeyer

doi:10.1371/journal.pone.0242464

Abstract

In several marine hosts of microalgae, fluorescent natural products may play an important role. While the ecological function of these compounds is not well understood, an interaction of these molecules with the photosynthesis of the symbionts has been suggested. In this study, the effect of Ageladine A (Ag A), a pH-dependent fluorophore found in sponges of the genus Agelas, on microalgal fluorescence was examined. The spectra showed an accumulation of Ag A within the cells, but with variable impacts on fluorescence. While in two Synechococcus strains, fluorescence of phycoerythrin increased significantly, the fluorescence of other Synechococcus strains was not affected. In four out of the five eukaryote species examined, chlorophyll a (Chl a) fluorescence intensity was modulated. In Tisochrysis lutea, for example, the position of the fluorescence emission maximum of Chl a was shifted. The variety of these effects of Ag A on microalgal fluorescence suggests that fluorophores derived from animals could play a crucial role in shaping the composition of marine host/symbiont systems.

Citation: Peter C, Thoms S, Koch F, Sartoris FJ, Bickmeyer U (2020) Sponge-derived Ageladine A affects the in vivo fluorescence emission spectra of microalgae. PLoS ONE 15(11): e0242464. https://doi.org/10.1371/journal.pone.0242464

Editor: Joseph Selvin, Pondicherry University, INDIA

Received: June 12, 2020; Accepted: November 2, 2020; Published: November 19, 2020

Copyright: © 2020 Peter et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.

Data Availability: All relevant data are within the manuscript and its Supporting Information files.

Funding: FK SPP1158, KO5563/1-1‘ViTMeD’ Deutsche Forschungsgemeinschaft www.dfg.de The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.

Competing interests: The authors have declared that no competing interests exist.

Introduction

Many sponges harbour photosynthetic symbionts, such as cryptophytes, diatoms, dinoflagellates, and members of the cyanobacterial genus Synechococcus, [1–8]. While ultraviolet, violet and blue light penetrate seawater the farthest, longer wavelengths, readily absorbed by typical algal pigments, are attenuated at shallower depths [9]. In 1968, Read et al. [10] discovered fluorophores which, when excited by ultraviolet/blue light, emit blue to green light in demosponges. Schlichter et al. [11, 12] found pigments in the deep-water coral Leptoseris fragilis that also transformed light of shorter wavelengths to longer wavelengths. It was proposed that this wavelength-transforming system by the host, enabled photosynthesis under otherwise suboptimal light qualities and intensities. Thus, it may be the case, that only a combination of low light adapted endosymbionts and a light-amplifying mechanism by the host enables phototrophic growth at depths of 95–145 m, where L. fragilis is typically found [13]. In addition, fluorescing pigments, which change the spectral composition of incoming light to be more suitable for algal photosynthesis, have been found in sponges as well as deep-water corals. While this was hypothesised by Schlichter et al. [11–13] to occur in corals, no empirical studies have been performed.

This principle may also apply to sponges, where light transmission modulation is known for spongin and Ageladine A (Ag A) found in sponges of the genus Agelas [14–16]. Ag A is a brominated pyrrole-imidazole alkaloid with different protonated states. While at neutral to slightly alkalic pH of 7–9, the uncharged species dominates, at a pH of 5–7, the first nitrogen becomes protonated. At higher acidity, pH 3–5, a second proton is gained, and the molecule becomes twice positively charged [17]. Ag A is a pH dependent fluorophore, with its fluorescence reaching maximal intensity at pH 3–4. The peak in excitation wavelength is at 370 nm with the emission ranging from 415 nm to 500 nm with a maximum at 415 nm [18], both measured in water. The excitation/emission profile changes with the environment [19]. Its specific function within the sponge holobiont, has not been identified.

While the uncharged form of Ag A is membrane permeable, once protonated it becomes membrane impermeable. This leads to an efficient accumulation of Ag A in acidic cellular compartments, such as thylakoids [17]. In the latter its fluorescence could potentially affect algal photosynthesis, by making a greater proportion of the incident light available to algal pigments. In addition, according to the Förster theory of energy transfer [20], a close proximity of two fluorophores can change the fluorescence characteristics of both [21], with the resulting fluorescence spectrum differing from the assumed additive spectrum. Since many algal pigments are known to be fluorophores, the presence of Ag A could potentially change the fluorescence signature of algal cells in more complex ways than simply yielding an additional Ag A specific fluorescence peak. While Ag A could alter algal photosynthesis in different ways and to differing extents, this has not been investigated before, and potential interactions between Ag A and algal pigments are unknown.

A recent study by Bickmeyer et al. indicates a profound effect of Ag A on the photosynthetic performance of Synechococcus bacillaris. Cells which were exposed to UV radiation of 370–380 nm, produced 250% more oxygen when incubated with 30 μM Ag A than cells in the control. This study, however, only examined one algal strain, and whether or not the underlying mechanisms are universal and likely occur in other prokaryotic and eukaryotic microalgae, remains to be tested. Also, the ecological relevance of a host producing fluorophores which then increase the photophysiological efficiency of its endosymbionts, has not been investigated. Since such fluorophores have been found in multiple hosts/symbiont complexes [10, 12], a system turning unusable light into photosynthetically active radiation may be a new and universal currency for symbiosis.

This study investigates whether Ag A enters algal cells and interacts with the fluorescence of different algal species. The presented data suggest that the interaction depends not only on the pigments present in the different algal classes, but also on the chemical environment within the chloroplasts. Unlike previous studies, which hypothesised that the interactions might be universal, results presented here reveal a more heterogenic picture with different effects observed between algal groups and even within the same genus.

Material and methods

In this study, 4 prokaryote strains and 5 eukaryote species spanning 3 algal phyla were examined. Four cyanobacteria strains were used, belonging to two pigment types differing in the composition of their phycobilisomes (S1 Table) [22]. Synechococcus sp. RCC1084 and S. bacillaris CCMP1333 belong to the green pigment type 1, while Synechococcus sp. RCC539 and RCC791 belong to the orange pigment type 3. The five eukaryotes were comprised of three chlorophytes Chlorogonium elongatum (by courtesy of B. Seah), Micrasterias americana (SAG 151.80) and Tetraselmis chuii (SAG 8 6), plus the haptophyte Tisochrysis lutea (CCAP 927/14) and cryptophyte Rhodomonas salina (K-1487).

Culture conditions

The marine algae and freshwater algae were cultivated in K-medium [23] and DY-Vm medium (Bigelow Laboratory, National Centre for Marine Algae and Microbiota, East Boothbay, ME, USA), respectively, made from autoclaved, 0.2 μm North Sea water (salinity 34) and 0.1 μm ultrapure water, respectively. All stock cultures were grown in duplicate cell culture flasks (T25, Sarstedt, Nümbrecht, Germany and T75, TPP Techno Plastic Products AG, Trasadingen, Switzerland). The eukaryotes were cultivated at room temperature with a 18:6 h light:dark cycle of 70–80 μmol photons m^-2 s^-1. The T. chuii and T. lutea cultures were kept on a shaker (KS 130 control, IKA-Werke GmbH & Co. KG, Staufen, Germany) at 100 rpm. The Synechococcus cultures were kept under continuous light in a MIR-253 Sanyo incubator (LabX, Midland, ON, Canada) at 25°C and 30 μmol photons m^-2 s^-1. The light intensities were measured using a spherical underwater quantum sensor (SPQA) connected to a LI-1000 DataLogger (LI-COR Biosciences GmbH, Bad Homburg, Germany).

Fluorescence spectra

The fluorescence spectra were determined for cultures in the exponential growth phase after a four-hour incubation period under the respective growth conditions. The chemicals used were dimethyl sulfoxide (DMSO, Carl Roth GmbH + Co. KG, Lichtentanne, Germany), 6 mM ageladine A (Ag A, Marnas Biochemicals GmbH, Bremerhaven, Germany) dissolved in DMSO and 0.5 M sodium bicarbonate (Sigma Aldrich, St. Louis, MO, USA). The concentration of Ag A used was chosen according to the species’ or strain’s tolerance to the substance. For Synechococcus sp. RCC1084, C. elongatum, R. salina and T. lutea, a final concentration of 5 μM Ag A was used. For Synechococcus sp. RCC539, RCC791, S. bacillaris CCMP1333 and M. americana the final concentration was 10 μM Ag A. T. chuii was incubated with 30 μM Ag A. In order to eliminate potential effects of Ag A´s solvent DMSO on the cells or the fluorescence signal, the controls also had a final DMSO concentration of 0.5% vol. The final concentration of sodium bicarbonate was 2.5 mM.

Wavelength scans were performed under the confocal laser scanning microscope TCS SP5 (Leica, Wetzlar, Germany). The excitation wavelength was set to 405 nm with the measured emission ranging from 420 nm to 700 nm.

For eukaryotes, the fluorescence signal of single cells was isolated and analysed. Due to their small cell size, this was not possible for the Synechococcus samples and thus the whole field of view was analysed. The included media background fluorescence exhibited the local maximum observed in all prokaryote samples at 466 nm. Fluorescence emission data was normalised to the highest emission intensity in the controls.

Results

In the two Synechococcus strains belonging to pigment type 1 (Synechococcus sp. RCC1084, S. bacillaris CCMP1333), the controls showed two maxima (Fig 1). One at wavelength 466 nm and a second peak at 657 nm. In the presence of Ag A, the first maximum shifted to 457 nm and increased in amplitude 1.6- to 1.7-fold. Neither the position nor the fluorescence intensity of the second maximum was affected significantly by the addition of Ag A.

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Fig 1.

In vivo fluorescence spectra of Synechococcus sp. RCC1084 (A) and S. bacillaris CCMP1333 (B). The solid and dotted lines represent the control and Ag A treatments, respectively. The peak positions are marked at their respective wavelengths.

https://doi.org/10.1371/journal.pone.0242464.g001

In the Synechococcus sp. strains RCC539 and RCC791, belonging to pigment type 3, the controls exhibited only one maximum at 466 nm (Fig 2). The presence of Ag A shifted the maximum to 447 nm and to 457 nm for RCC539 and RCC791, respectively. While the amplitude of the peak increased 3-fold in RCC791, it did so only by 10% for RCC539. Ag A also led to the formation of an additional maximum at 566 nm in both strains.

Download:

Fig 2.

In vivo fluorescence spectra of Synechococcus sp. RCC539 (A) and Synechococcus sp. RCC791 (B). The solid and dotted lines represent the control and Ag A treatments, respectively. The peak positions are marked at their respective wavelengths.

https://doi.org/10.1371/journal.pone.0242464.g002

The three chlorophyte species C. elongatum, M. americana and T. chuii exhibited only one maximum at 684 nm (Fig 3) in the controls. Even though its position was unaffected by Ag A, the amplitude of the peak decreased by 25% in C. elongatum and increased by 28% in M. americana. In M. americana and T. chuii, the addition of Ag A resulted in an additional, local maximum at 458 nm. C. elongatum did not show a maximum in that wavelength range.

Download:

Fig 3.

In vivo fluorescence spectra of C. elongatum (black), M. americana (dark grey) and T. chuii (light grey). The solid and dotted lines represent the control and Ag A treatments, respectively. The peak positions are marked at their respective wavelengths.

https://doi.org/10.1371/journal.pone.0242464.g003

While in the haptophyte T. lutea, only one maximum at 685 nm was observed in the control, in R. salina, a cryptophyte, two maxima, one at 584 nm and one at 685 nm were seen in the control (Fig 4). In the presence of Ag A, both species exhibited an additional maximum at 447 nm. The effect of Ag A on the original maxima differed in that in T. lutea, it shifted from 685 nm to 676 nm while the fluorescence intensity increased by 300%. In R. salina, on the other hand, the position of the original maxima remained unaffected, but the amplitudes decreased by 28 and 37%, respectively.

Download:

Fig 4.

In vivo fluorescence spectra of T. lutea (A) and R. salina (B). The solid and dotted lines represent the control and Ag A treatments, respectively. The peak positions are marked at their respective wavelengths.

https://doi.org/10.1371/journal.pone.0242464.g004

Discussion

In contrast to initial hypotheses, incubation with Ag A resulted in a variety of effects on algal fluorescence between species, likely caused by differences in the makeup of algal pigments (Table 1).

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Table 1. Some of the main pigments found in the investigated alga species.

https://doi.org/10.1371/journal.pone.0242464.t001

Fluorescence maxima

Ag A.

In four out of five eukaryotes, the uptake of Ag A resulted in an additional maximum between 440–460 nm. The maxima were located at 447 nm in T. lutea and R. salina and at 458 nm in M. americana and T. chuii. This difference in peak position between the algal species as well as its deviance from the characteristics of Ag A in water, may be due to the intracellular conditions such as differences in pH [19]. The only eukaryote which did not exhibit a local maximum in this wavelength range was C. elongatum (Fig 3). Since it was one of two freshwater chlorophytes tested and the other (M. americana) exhibited a local maximum, the absence appears to be neither a chlorophyte- nor freshwater specific response. In the Synechococcus strains, a combined peak of the Ag A maximum at 447 nm overlapping with the background maximum at 466 nm was observed (S1 Fig). In the strains RCC791, RCC1084 and CCMP1333, this maximum was located at 457 nm, while in Synechococcus sp. RCC539 the background maximum merged into the Ag A maximum at 447 nm (Fig 2). As the fluorescence of Ag A is brightest at pH 3 and 4 [18], the difference in fluorescence intensity could be caused by different pH values of the compartments into which it was incorporated.

Phycoerythrin.

In R. salina, the maximum at 584 nm (Fig 4), can be attributed to phycoerythrin [24]. The other two algal strains, which also contain phycoerythrin (Synechococcus sp. RCC539 and RCC791) showed a maximum (566 nm) attributable to this pigment only in the presence of Ag A (Fig 2). For stress factors like low temperatures [25] and high light intensities [26], significantly increased phycoerythrin fluorescence has been reported to be linked to an uncoupling of the phycobilisomes from the photosystems or the thylakoid membranes. The changes in fluorescence could either be due to Ag A affecting structural components of the phycobilisomes, or specifically the pigments associated with phycoerythrin, phycoerythrobilin (PEB) and phycourobilin (PUB).

In case of R. salina, only a minor effect of Ag A on phycoerythrin fluorescence intensity was observed and the position of the maximum remained unaffected. Since in cryptophytes phycoerythrin is not organised in phycobilisomes [27], Ag A possibly affects structural components of the phycobilisomes rather than the pigment itself.

Phycocyanin.

In Synechococcus sp. RCC1084 and S. bacillaris CCMP1333, the maximum at 657 nm (Fig 1) likely belongs to phycocyanin [24]. The fact that in both strains its position and amplitude was largely unaffected by the presence of Ag A, indicates a specific interaction between Ag A and proteins associated with phycoerythrin, present only in the phycobilisomes of Synechococcus strains belonging to pigment types 2 and 3. Another possibility is variable interactions between Ag A and different types of phycocyanin (S1 Table).

Chlorophyll a.

A fluorescence maximum, attributable to Chl a [28], was observed at 684-685nm in the three chlorophytes and in T. lutea and R. salina. The addition of Ag A to T. lutea shifted the position of the maximum by 9 nm to 676 nm and increased the fluorescence intensity by 300% (Fig 4). In comparison, the increase was significantly lower (28%) in M. americana, while for C. elongatum and R. salina, the fluorescence intensity decreased by 25% and 37%, respectively. This difference in reaction to Ag A could be due to the differences in the molecular composition of the chlorophyll surroundings, including accessory pigments like Fucoxanthin, which is only present in T. lutea.

Potential impact on physiology

The additional fluorescence maxima found in all algae except C. elongatum supports the hypothesis that Ag A is taken up into the cells. The results of this study highlight that Ag A can interact with algal pigments in a multitude of ways. The significant increase in fluorescence of phycoerythrin containing phycobilisomes, for example, indicates a potential disruption in the energy transfer chain for these Synechococcus strains. This might decrease their photosynthetic efficiency, while that of strains belonging to pigment type 1 would remain unaffected.

The drastic increase of Chl a fluorescence in T. lutea and M. americana points to variable effects of Ag A and subsequent changes in photosynthetic activity. However, since photosynthetic efficiency was not assessed in the current study, the effect of Ag A on the former can only be speculated. The increase in fluorescence indicates that an increased proportion of received energy was not being utilised by the photosystems [29]. This could either be because Ag A interrupts the coupling of light harvesting antennae or because Ag A inhibits the photosystems. Given the fine-tuned collocation of absorption maxima within the photosynthetic apparatus, the shift in emission observed in T. lutea could also inhibit the efficient transfer of energy to the next molecule. However, the increase in fluorescence could also indicate a surplus of light energy made available to the chlorophyll molecules by the fluorescence emission of Ag A. In the latter, a subsequent upregulation of photosystems would be expected, increasing the overall photosynthetic efficiency.

An observed decrease in fluorescence could either hint at decreased or increased photosynthetic efficiency. It could hint at a greater proportion of absorbed light energy being used for photosynthetic activity [29], possibly due to an improved coupling of accessory pigments to the photosystems or by an increased availability of photosystems. On the other hand, decreased fluorescence could also be caused by a decrease in absorption. In this case, reduced photosynthetic efficiency would be expected.

These conflicting effects of Ag A on photosynthetic efficiency need to be investigated with targeted experiments, measuring photosynthesis and other photosynthetic parameters.

Conclusion

The effects of Ag A on algal pigments are far more complex and diverse than initially proposed by Bickmeyer et al.. While changes in fluorescence intensity could be due to an interaction of Ag A with the photosynthesis apparatus, shifts in fluorescence peak emission suggest a direct pigment-pigment interaction at least for Chl a. Since this effect is not observed for all eukaryotic algae, the chemical environment within the chloroplasts also appears to be of great importance. In addition to the interaction with Chl a, Ag A appears to have a profound effect on certain phycobilisomes. The differences in the effect of Ag A on algal fluorescence, might enable the sponge to take control over the composition of its microbiome. While in some algae the photosynthetic efficiency would be improved by the presence of sponge produced Ag A, other algae would see their photosynthetic efficiency decreased, placing them at a competitive disadvantage. In symbionts associated with sponges for a prolonged time, this could lead to a change in pigment content or composition, which would enable the algae to thrive where they otherwise could not and to subside on lower resources. It could also serve as a mechanism binding the algae to the sponge. Since fluorophores of similar characteristics as Ag A have also been found in other endosymbiont hosts, this principle might be more widely employed than is currently known.

Supporting information

S1 Fig. Non-normalised fluorescence spectra as determined by wavelength scans of Synechococcus sp. RCC1084.

The solid line represents the control, the dotted line represents the sample treated with Ag A. The dashed line represents the normalised fluorescence data of T. lutea treated with Ag A, the dash-dotted line represents the combination peak calculated as the fluorescence in the Synechococcus sp. RCC1084 control plus the T. lutea sample incubated with Ag A.

https://doi.org/10.1371/journal.pone.0242464.s001

(DOCX)

S1 Table. Composition of phycobilisomes of Synechococcus spp. depending on the pigment type.

The grey crosses indicate that pigment type 2 has either C-phycocyanin or “R-Phycocyanin II or other”, but not both [22].

https://doi.org/10.1371/journal.pone.0242464.s002

(DOCX)

S1 Data.

https://doi.org/10.1371/journal.pone.0242464.s003

(XLSX)

Acknowledgments

We thank Annegret Müller and Nancy Kühne for taking care of the algal cultures.

References

1. DucJaux G. Présence de cryptophycées symbiontiques dans trois éponges des côtes francaises. Bull Soc Phycol Fr. 1973; 18: 54–57.
- View Article
- Google Scholar
2. Hill MS. Symbiotic zooxanthellae enhance boring and growth rates of the tropical sponge Anthosigmella varians forma varians. Mar Biol. 1996; 125: 649–654.
- View Article
- Google Scholar
3. Imhoff JF, Trüper HG. Marine sponges as habitats of anaerobic phototrophic bacteria. Microb Ecol. 1976; 3: 1–9. pmid:24233392
- View Article
- PubMed/NCBI
- Google Scholar
4. Lee YK, Lee JH, Lee HK. Microbial symbiosis in marine sponges. The J Microbiol. 2001; 39: 254–264.
- View Article
- Google Scholar
5. Regoli F, Nigro M, Chierici E, Cerrano C, Schiapparelli S, Totti C, et al. Variations of antioxidant efficiency and presence of endosymbiotic diatoms in the Antarctic porifera Haliclona dancoi. Mar Environ Res. 2004; 58: 637–640. pmid:15178092
- View Article
- PubMed/NCBI
- Google Scholar
6. Schönberg CHL, Loh WKW. Molecular identity of the unique symbiotic dinoflagellates found in the bioeroding demosponge Cliona orientalis. Mar Ecol Prog Ser. 2005; 299: 157–166.
- View Article
- Google Scholar
7. Taylor MW, Radax R, Steger D, Wagner M. Sponge-associated microorganisms: Evolution, ecology, and biotechnological potential. Microbiol Mol Biol R. 2007; 71: 295–347.
- View Article
- Google Scholar
8. Unson MD, Holland ND, Faulkner DJ. A brominated secondary metabolite synthesized by the cyanobacterial symbiont of a marine sponge and accumulation of the crystalline metabolite in the sponge tissue. Mar Biol. 1994; 119: 1–11.
- View Article
- Google Scholar
9. Holmes RW. Solar radiation, submarine daylight, and photosynthesis. Treatise on marine ecology and paleoecology. 1957; 1: 109–128.
- View Article
- Google Scholar
10. Read KRH, Davidson JM, Twarog BM. Fluorescence of sponges and coelenterates in blue light. Comp Biochem Physiol. 1968; 25: 873–882.
- View Article
- Google Scholar
11. Schlichter D, Fricke HW, Weber W. Light harvesting by wavelength transformation in a symbiotic coral of the Red Sea twilight zone. Mar Biol. 1986; 91: 403–407.
- View Article
- Google Scholar
12. Schlichter D, Weber W, Fricke HW. A chromatophore system in the hermatypic, deep-water coral Leptoseris fragilis (Anthozoa: Hexacorallia). Mar Biol. 1985; 89: 143–147.
- View Article
- Google Scholar
13. Schlichter D, Fricke HW. Coral host improves photosynthesis of endosymbiotic algae. Naturwissenschaften. 1990; 77: 447–450.
- View Article
- Google Scholar
14. Assmann M, Lichte E, van Soest RWM, Köck M. New bromopyrrole alkaloid from the marine sponge Agelas wiedenmayeri. Org Lett. 1999; 1: 455–457.
- View Article
- Google Scholar
15. Bickmeyer U, Thoms S, Koch F, Mukagatare LP, Silalahi R, Sartoris FJ. Enhancement of photosynthesis in Synechococcus bacillaris by sponge-derived Ageladine A. PloS one. 2019; 14 pmid:30913222
- View Article
- PubMed/NCBI
- Google Scholar
16. Fujita M, Nakao Y, Matsunaga S, Seiki M, Itoh Y, Yamashita J, et al. Ageladine A: an antiangiogenic matrixmetalloproteinase inhibitor from the marine sponge Agelas nakamurai. J Am Chem Soc. 2003; 125: 15700–15701. pmid:14677933
- View Article
- PubMed/NCBI
- Google Scholar
17. Bickmeyer U, Heine M, Podbielski I, Münd D, Köck M, Karuso P. Tracking of fast moving neuronal vesicles with ageladine A. Biochem Bioph Res Co. 2010; 402: 489–494. pmid:20955687
- View Article
- PubMed/NCBI
- Google Scholar
18. Bickmeyer U, Grube A, Klings KW, Köck M. Ageladine A, a pyrrole-imidazole alkaloid from marine sponges, is a pH sensitive membrane permeable dye. Biochem Bioph Res Co. 2008; 373: 419–422. Correction in Biochem Bioph Res Co. 2009; 383: 519. pmid:18588854
- View Article
- PubMed/NCBI
- Google Scholar
19. Mordhorst T, Bickmeyer U. Perspectives on the synthesis and use of ageladine A. Tetrahedron Lett. 2015; 56: 4363–4366.
- View Article
- Google Scholar
20. Förster T. Zwischenmolekulare Energiewanderung und Fluoreszenz. Ann Phys. 1948; 437: 55–75.
- View Article
- Google Scholar
21. Şener M, Strümpfer J, Hsin J, Chandler D, Scheuring S, Hunter CN, et al. Förster energy transfer theory as reflected in the structures of photosynthetic light harvesting systems. ChemPhysChem. 2011; 12: 518–531. pmid:21344591
- View Article
- PubMed/NCBI
- Google Scholar
22. Six C, Thomas JC, Garczarek L, Ostrowski M, Dufresne A, Blot N, et al. Diversity and evolution of phycobilisomes in marine Synechococcus spp.: a comparative genomics study. Genome Biol. 2007; 8 pmid:18062815
- View Article
- PubMed/NCBI
- Google Scholar
23. Keller MD, Selvin RC, Claus W, Guillard RR. Media for the culture of oceanic ultraphytoplankton. J Phycol. 1987; 23: 633–638.
- View Article
- Google Scholar
24. MacIntyre HL, Lawrenz E, Richardson TL. Taxonomic discrimination of phytoplankton by spectral fluorescence. In: Suggett DJ, Prášil O, Borowitzka MA, editors. Chlorophyll a Fluorescence in Aquatic Sciences: Methods and Applications. Springer, Berlin, Heidelberg; 2010. pp. 129–169.
25. Li Y, Zhang J, Xie J, Zhao J, Jiang L. Temperature-induced decoupling of phycobilisomes from reaction centers. Biochim Biophys Acta. 2001; 1504: 229–234. pmid:11245787
- View Article
- PubMed/NCBI
- Google Scholar
26. Tamary E, Kiss V, Nevo R, Adam Z, Bernát G, Rexroth S, et al. Structural and functional alterations of cyanobacterial phycobilisomes induced by high-light stress. Biochim Biophys Acta. 2012; 1817: 319–327. pmid:22138629
- View Article
- PubMed/NCBI
- Google Scholar
27. Spear-Bernstein L, Miller KR. Unique location of the phycobiliprotein light-harvesting pigment in the cryptophyceae. J Phycol. 1989; 25: 412–419.
- View Article
- Google Scholar
28. Millie D, Schofield O, Kirkpatrick G, Johnsen G, Evens T. Using absorbance and fluorescence spectra to discriminate microalgae. Eur J Phycol. 2002; 37: 313–322.
- View Article
- Google Scholar
29. Ralph PJ, Wilhelm C, Lavaud J, Jakob T, Petrou K, Kranz SA. Fluorescence as a tool to understand changes in photosynthetic electron flow regulation. In: Suggett DJ, Prášil O, Borowitzka MA., editors. Chlorophyll a Fluorescence in Aquatic Sciences: Methods and Applications. Springer, Berlin, Heidelberg; 2010. pp. 75–89.

[ref1] 1. DucJaux G. Présence de cryptophycées symbiontiques dans trois éponges des côtes francaises. Bull Soc Phycol Fr. 1973; 18: 54–57.
View Article
Google Scholar

[2] View Article

[3] Google Scholar

[ref2] 2. Hill MS. Symbiotic zooxanthellae enhance boring and growth rates of the tropical sponge Anthosigmella varians forma varians. Mar Biol. 1996; 125: 649–654.
View Article
Google Scholar

[5] View Article

[6] Google Scholar

[ref3] 3. Imhoff JF, Trüper HG. Marine sponges as habitats of anaerobic phototrophic bacteria. Microb Ecol. 1976; 3: 1–9. pmid:24233392
View Article
PubMed/NCBI
Google Scholar

[8] View Article

[9] PubMed/NCBI

[10] Google Scholar

[ref4] 4. Lee YK, Lee JH, Lee HK. Microbial symbiosis in marine sponges. The J Microbiol. 2001; 39: 254–264.
View Article
Google Scholar

[12] View Article

[13] Google Scholar

[ref5] 5. Regoli F, Nigro M, Chierici E, Cerrano C, Schiapparelli S, Totti C, et al. Variations of antioxidant efficiency and presence of endosymbiotic diatoms in the Antarctic porifera Haliclona dancoi. Mar Environ Res. 2004; 58: 637–640. pmid:15178092
View Article
PubMed/NCBI
Google Scholar

[15] View Article

[16] PubMed/NCBI

[17] Google Scholar

[ref6] 6. Schönberg CHL, Loh WKW. Molecular identity of the unique symbiotic dinoflagellates found in the bioeroding demosponge Cliona orientalis. Mar Ecol Prog Ser. 2005; 299: 157–166.
View Article
Google Scholar

[19] View Article

[20] Google Scholar

[ref7] 7. Taylor MW, Radax R, Steger D, Wagner M. Sponge-associated microorganisms: Evolution, ecology, and biotechnological potential. Microbiol Mol Biol R. 2007; 71: 295–347.
View Article
Google Scholar

[22] View Article

[23] Google Scholar

[ref8] 8. Unson MD, Holland ND, Faulkner DJ. A brominated secondary metabolite synthesized by the cyanobacterial symbiont of a marine sponge and accumulation of the crystalline metabolite in the sponge tissue. Mar Biol. 1994; 119: 1–11.
View Article
Google Scholar

[25] View Article

[26] Google Scholar

[ref9] 9. Holmes RW. Solar radiation, submarine daylight, and photosynthesis. Treatise on marine ecology and paleoecology. 1957; 1: 109–128.
View Article
Google Scholar

[28] View Article

[29] Google Scholar

[ref10] 10. Read KRH, Davidson JM, Twarog BM. Fluorescence of sponges and coelenterates in blue light. Comp Biochem Physiol. 1968; 25: 873–882.
View Article
Google Scholar

[31] View Article

[32] Google Scholar

[ref11] 11. Schlichter D, Fricke HW, Weber W. Light harvesting by wavelength transformation in a symbiotic coral of the Red Sea twilight zone. Mar Biol. 1986; 91: 403–407.
View Article
Google Scholar

[34] View Article

[35] Google Scholar

[ref12] 12. Schlichter D, Weber W, Fricke HW. A chromatophore system in the hermatypic, deep-water coral Leptoseris fragilis (Anthozoa: Hexacorallia). Mar Biol. 1985; 89: 143–147.
View Article
Google Scholar

[37] View Article

[38] Google Scholar

[ref13] 13. Schlichter D, Fricke HW. Coral host improves photosynthesis of endosymbiotic algae. Naturwissenschaften. 1990; 77: 447–450.
View Article
Google Scholar

[40] View Article

[41] Google Scholar

[ref14] 14. Assmann M, Lichte E, van Soest RWM, Köck M. New bromopyrrole alkaloid from the marine sponge Agelas wiedenmayeri. Org Lett. 1999; 1: 455–457.
View Article
Google Scholar

[43] View Article

[44] Google Scholar

[ref15] 15. Bickmeyer U, Thoms S, Koch F, Mukagatare LP, Silalahi R, Sartoris FJ. Enhancement of photosynthesis in Synechococcus bacillaris by sponge-derived Ageladine A. PloS one. 2019; 14 pmid:30913222
View Article
PubMed/NCBI
Google Scholar

[46] View Article

[47] PubMed/NCBI

[48] Google Scholar

[ref16] 16. Fujita M, Nakao Y, Matsunaga S, Seiki M, Itoh Y, Yamashita J, et al. Ageladine A: an antiangiogenic matrixmetalloproteinase inhibitor from the marine sponge Agelas nakamurai. J Am Chem Soc. 2003; 125: 15700–15701. pmid:14677933
View Article
PubMed/NCBI
Google Scholar

[50] View Article

[51] PubMed/NCBI

[52] Google Scholar

[ref17] 17. Bickmeyer U, Heine M, Podbielski I, Münd D, Köck M, Karuso P. Tracking of fast moving neuronal vesicles with ageladine A. Biochem Bioph Res Co. 2010; 402: 489–494. pmid:20955687
View Article
PubMed/NCBI
Google Scholar

[54] View Article

[55] PubMed/NCBI

[56] Google Scholar

[ref18] 18. Bickmeyer U, Grube A, Klings KW, Köck M. Ageladine A, a pyrrole-imidazole alkaloid from marine sponges, is a pH sensitive membrane permeable dye. Biochem Bioph Res Co. 2008; 373: 419–422. Correction in Biochem Bioph Res Co. 2009; 383: 519. pmid:18588854
View Article
PubMed/NCBI
Google Scholar

[58] View Article

[59] PubMed/NCBI

[60] Google Scholar

[ref19] 19. Mordhorst T, Bickmeyer U. Perspectives on the synthesis and use of ageladine A. Tetrahedron Lett. 2015; 56: 4363–4366.
View Article
Google Scholar

[62] View Article

[63] Google Scholar

[ref20] 20. Förster T. Zwischenmolekulare Energiewanderung und Fluoreszenz. Ann Phys. 1948; 437: 55–75.
View Article
Google Scholar

[65] View Article

[66] Google Scholar

[ref21] 21. Şener M, Strümpfer J, Hsin J, Chandler D, Scheuring S, Hunter CN, et al. Förster energy transfer theory as reflected in the structures of photosynthetic light harvesting systems. ChemPhysChem. 2011; 12: 518–531. pmid:21344591
View Article
PubMed/NCBI
Google Scholar

[68] View Article

[69] PubMed/NCBI

[70] Google Scholar

[ref22] 22. Six C, Thomas JC, Garczarek L, Ostrowski M, Dufresne A, Blot N, et al. Diversity and evolution of phycobilisomes in marine Synechococcus spp.: a comparative genomics study. Genome Biol. 2007; 8 pmid:18062815
View Article
PubMed/NCBI
Google Scholar

[72] View Article

[73] PubMed/NCBI

[74] Google Scholar

[ref23] 23. Keller MD, Selvin RC, Claus W, Guillard RR. Media for the culture of oceanic ultraphytoplankton. J Phycol. 1987; 23: 633–638.
View Article
Google Scholar

[76] View Article

[77] Google Scholar

[ref24] 24. MacIntyre HL, Lawrenz E, Richardson TL. Taxonomic discrimination of phytoplankton by spectral fluorescence. In: Suggett DJ, Prášil O, Borowitzka MA, editors. Chlorophyll a Fluorescence in Aquatic Sciences: Methods and Applications. Springer, Berlin, Heidelberg; 2010. pp. 129–169.

[ref25] 25. Li Y, Zhang J, Xie J, Zhao J, Jiang L. Temperature-induced decoupling of phycobilisomes from reaction centers. Biochim Biophys Acta. 2001; 1504: 229–234. pmid:11245787
View Article
PubMed/NCBI
Google Scholar

[80] View Article

[81] PubMed/NCBI

[82] Google Scholar

[ref26] 26. Tamary E, Kiss V, Nevo R, Adam Z, Bernát G, Rexroth S, et al. Structural and functional alterations of cyanobacterial phycobilisomes induced by high-light stress. Biochim Biophys Acta. 2012; 1817: 319–327. pmid:22138629
View Article
PubMed/NCBI
Google Scholar

[84] View Article

[85] PubMed/NCBI

[86] Google Scholar

[ref27] 27. Spear-Bernstein L, Miller KR. Unique location of the phycobiliprotein light-harvesting pigment in the cryptophyceae. J Phycol. 1989; 25: 412–419.
View Article
Google Scholar

[88] View Article

[89] Google Scholar

[ref28] 28. Millie D, Schofield O, Kirkpatrick G, Johnsen G, Evens T. Using absorbance and fluorescence spectra to discriminate microalgae. Eur J Phycol. 2002; 37: 313–322.
View Article
Google Scholar

[91] View Article

[92] Google Scholar

[ref29] 29. Ralph PJ, Wilhelm C, Lavaud J, Jakob T, Petrou K, Kranz SA. Fluorescence as a tool to understand changes in photosynthetic electron flow regulation. In: Suggett DJ, Prášil O, Borowitzka MA., editors. Chlorophyll a Fluorescence in Aquatic Sciences: Methods and Applications. Springer, Berlin, Heidelberg; 2010. pp. 75–89.

Figures

Abstract

Introduction

Material and methods

Culture conditions

Fluorescence spectra

Results

Discussion

Fluorescence maxima

Ag A.

Phycoerythrin.

Phycocyanin.

Chlorophyll a.

Potential impact on physiology

Conclusion

Supporting information

S1 Fig. Non-normalised fluorescence spectra as determined by wavelength scans of Synechococcus sp. RCC1084.

S1 Table. Composition of phycobilisomes of Synechococcus spp. depending on the pigment type.

S1 Data.

Acknowledgments

References