New trends in photobiology History of photoinhibition research

At the beginning of our century few scientists paid attention to the phenomenon of inactivation of photosynthesis by high light intensities which was later called photoinhibition. In the period 1925–1950, the idea was established that photoinhibition is a reversible inactivation, determined by light intensity and exposure time, followed by irreversible damage of the photosynthetic apparatus. However, the absence of a uniform terminology demonstrates that photoinhibition was not completely perceived and understood. In 1956, B. Kok gave the first definition of photoinhibition as a photochemical inactivation of pigment complexes.     

Photobiological characteristics and photosynthetic UV responses in two Ulva species (Chlorophyta) from southern Spain

The effect of different wavebands of artificial UV (UVB and UVA) and photosynthetically active radiation (PAR) was assessed in two species of the genus Ulva, U. olivascens and U. rotundata, from southern Spain in order to test for possible differences in acclimation of photosynthesis. Both species share similar morphology but are subject to different light environments: U. rotundata is an estuarine alga, inhabiting subtidal locations, while U. olivascens is an intertidal, sun-adapted organism. Algae were exposed to three different UV conditions, PAR+UVA+UVB, PAR+UVA and PAR for 7 d. Short-term exposure (6 h) was also carried out, using two PAR levels, 150 and 700 micromolm(-2)s(-1). Pigment contents and photosynthesis vs. irradiance curves from oxygen evolution were used to contrast sun- and shade adaptation between these species. O2-based net photosynthesis (Pmax) and PAM-chlorophyll fluorescence (optimal quantum yield, Fv/Fm) were used as parameters to evaluate photoinhibition of photosynthesis in the experiments. The results underline different photobiological characteristics among species: the subtidal U. rotundata had higher contents of pigments (Chl a, Chl b and carotenoids) than the sun-adapted U. olivascens, which resulted in higher thallus absorptance and P-I parameters characterized by higher photosynthetic efficiency at limiting irradiances (alpha) and lower saturating points for photosynthesis (Ek). After 7 d exposure, photoinhibition of Fv/Fm was close to 40-45% in both species. Differences between UV treatments were seen in U. rotundata after 5 d and after 7 d in U. olivascens, in which PAR+UVA impaired strongly photosynthesis (80%). Such patterns were correlated with a progressive decrease in pigment contents, specially chlorophylls. In short-term (6 h) exposures, combinations of UVA+UVB and high PAR level resulted in high rates of photoinhibition of chlorophyll fluorescence (68-92%) in U. rotundata, whereas in U. olivascens photoinhibition ranged between 42% and 53%. Photoinhibition under low PAR combined to UV radiation was lower than observed under high PAR. Net O2-Pmax revealed similar response among the species, with maximal photoinhibition rates close to 60% in algae incubated under high PAR+UVA+UVB. In the case of UV exposure in combination with low PAR, the highest photoinhibition rates were measured in U. rotundata.     

EVIDENCE FOR AN ULTRAVIOLET SUNSCREEN ROLE OF THE EXTRACELLULAR PIGMENT SCYTONEMIN IN THE TERRESTRIAL CYANOBACTERIUM Chiorogloeopsis sp.

The proposed photoprotective role of the UV-A absorbing, extracellular pigment scytonemin was studied in the terrestrial cyanobacterium Chlorogloeopsis sp. strain O-89-Cgs(1). UV-A (315-400 nm) caused growth delay, cell growth restarting only when scytonemin had accumulated in the extracellular envelopes. Cultures with scytonemin were more resistant to photoinhibition of photosynthesis than cultures without scytonemin, the differential resistance being much greater to UV-A-caused photoinhibition than to photoinhibition caused by visible light. The presence of scytonemin in the extracellular envelopes was correlated with the inability of UV-A radiation to induce strong photopigment fluorescence (685 nm emission), regardless of the specific content os photosynthetic pigments. The physical removal of the scytonemin containing extracellular envelopes brought about the loss of UV-A resistance as measured by photobleaching rates of chlorophyll a under conditions of physiological inactivity (desiccation). These observations provide strong evidence for the proposed protective role of scytonemin, as a passive UV-A sunscreen, in cyanobacteria.     

Photoinhibition of photosynthesis in Macrocystis pyrifera (Phaeophyceae), Chondrus crispus (Rhodophyceae) and Ulva lactuca (Chlorophyceae) in outdoor culture systems

The effect of solar radiation on photosynthesis and chlorophyll fluorescence associated to photosystem II (PS II) was determined in the Phaeophyta Macrocystis pyrifera, the Rhodophyta Chondrus crispus and the Chlorophyta Ulva lactuca by oxygen evolution and pulse-amplitude-modulated (PAM) fluorescence. The algae were maintained in 1.2 m3 outdoor tanks with constant aeration and at 8, 26 and 100% incident irradiance (E(o)). All three species showed a decrease in deltaF/F'm values during solar noon compared to values in the morning and afternoon, suggesting a photoinhibition of photosynthesis. In general, photoinhibition was negatively correlated to increasing daily irradiance in all three species. Photoinhibition in C. crispus occurred in tissue incubated at 8, 26 and 100% E(o), while in M. pyrifera and U. lactuca a decrease in deltaF/F'm values was only observed in tissue incubated at 100% E(o). This suggests that species that naturally grow at greater depths might be more susceptible to excessive light when cultured in shallow waters compared to species that naturally inhabit shallower depths. In M. pyrifera, deltaF/F'm values were lower in the afternoon than those in the morning, suggesting slower repair mechanisms of the photosystem II compared to the other species. The results suggest that photoinhibition could be reduced by reducing incident irradiance to culture systems or increasing of biomass to promote self-shading. Gross oxygenic photosynthesis increased linearly at low electron transport rates after which it saturated in all three species. This suggests that chlorophyll fluorescence could be used as an indicator of the physiological status of macroalgae maintained in dense aquaculture systems.     

Photoinhibition in the Mediterranean Green Alga Halimeda tuna Ellis et Sol Measured in situ

Abstract— Photoinhibition of photosynthesis was investigated in the Mediterranean green alga Halimeda tuna measuring pulse amplitude modulation (PAM) chlorophyll fluorescence and oxygen evolution in situ under solar radiation. Exposure to solar radiation at the surface caused a drastic decline in the photosynthetic quantum yield accompanied by a decline in the photochemical quenching, while the nonphotochemical quenching dramatically increased. The algae recovered from these effects within a few hours indicating that these are mainly due to reversible photoinhibition and only to a smaller extent to nonreversible photodamage. Individuals harvested from deeper waters were more affected than those from shallower waters. Photoinhibition occurs in this alga even in its natural habitat when the sun is at high angles as shown by measuring the fluorescence parameters at hourly intervals during the course of the day. Photoinhibition was less pronounced when the short wavelength band was increasingly removed from solar radiation using cut-off filters. After exposure of thalli to solar radiation at the water surface, oxygen production decreased drastically within 30 min; this inhibition was even more pronounced in algae harvested from deeper waters. Oxygen measurements at different depths showed optimal photosynthesis at a depth of 1 m. Also for photosynthetic oxygen production inhibited by high solar irradiance at least partial recovery could be observed within several hours. Despite the fact that UVB accounts for a very small fraction of solar radiation, it has a considerable effect on photosynthesis, whereas UVA seems to contribute only little to photoinhibition in H. tuna.     

ULTRAWEAK LIGHT EMISSION FROM RAT LIVER NUCLEI

Abstract–An extremely weak native light emission from rat liver nuclei was detected and studied using a highly sensitive single photon counting system. This emission is oxygen dependent and we attribute it to (per) oxidative processes. The effects of deuterium oxide and l,4-diazabicyclo-[2.2.2] octane on the light emission suggests the possible involvement of singlet oxygen. The kinetic features of the underlying reactions including biphasic response to both oxygen and temperature changes, could be clearly discerned. Further study of this light emission can serve as a useful adjunct to biochemical investigations of oxidative processes which play an important role in mutation, carcinogenesis and aging.     

Integrating proton coupled electron transfer (PCET) and excited states

In many of the chemical steps in photosynthesis and artificial photosynthesis, proton coupled electron transfer (PCET) plays an essential role. An important issue is how excited state reactivity can be integrated with PCET to carry out solar fuel reactions such as water splitting into hydrogen and oxygen or water reduction of CO₂ to methanol or hydrocarbons. The principles behind PCET and concerted electron–proton transfer (EPT) pathways are reasonably well understood. In Photosystem II antenna light absorption is followed by sensitization of chlorophyll P₆₈₀ and electron transfer quenching to give P₆₈₀⁺. The oxidized chlorophyll activates the oxygen evolving complex (OEC), a CaMn₄ cluster, through an intervening tyrosine–histidine pair, Y_Z. EPT plays a major role in a series of four activation steps that ultimately result in loss of 4e^?/4H⁺ from the OEC with oxygen evolution. The key elements in photosynthesis and artificial photosynthesis – light absorption, excited state energy and electron transfer, electron transfer activation of multiple-electron, multiple-proton catalysis – can also be assembled in dye sensitized photoelectrochemical synthesis cells (DS-PEC). In this approach, molecular or nanoscale assemblies are incorporated at separate electrodes for coupled, light driven oxidation and reduction. Separate excited state electron transfer followed by proton transfer can be combined in single semi-concerted steps (photo-EPT) by photolysis of organic charge transfer excited states with H-bonded bases or in metal-to-ligand charge transfer (MLCT) excited states in pre-associated assemblies with H-bonded electron transfer donors or acceptors. In these assemblies, photochemically induced electron and proton transfer occur in a single, semi-concerted event to give high-energy, redox active intermediates.     

ELECTROCHEMICAL GENERATION OF SOLUTION LUMINESCENCE—III.: EFFECT OF OXYGEN ON QUANTUM YIELD AND KINETICS OF LUMINOL

Abstract -The growth and decay of light emission were examined for luminol as a funtion of oxygen concentration in aqueous alkaline solutions during and after the application of a controlled potential, square-wave electrochemical pulse. The results indicate that, in the rise portion of the light, the rate of electrochemical oxidation of luminol governs the light emission rate; while in the decay portion, the rate is first order and is independent of oxygen concentration. Quantum yields based on integration of the total light emitted also appear to be independent of oxygen above a threshold value. These results are consistent with evidence that the emitting state is an excited singlet.     

Effects of (60)Co gamma radiation on thylakoid membrane functions in Anacystis nidulans

In photosynthetic organisms oxidative stress is known to result in photoinactivation of photosynthetic machinery. We investigated effects of ⁶⁰Co γ radiation, which generates oxidative stress, on thylakoid structure and function in cyanobacteria. Cells of unicellular, non-nitrogen fixing cyanobacterium Anacystis nidulans (Synechococcus sp.) showed D₁₀ value of 257 Gy of ⁶⁰Co γ radiation. When measured immediately after exposure, cells irradiated with 1500 Gy (lethal dose) of ⁶⁰Co γ radiation did not show any differences in photosynthetic functions such as CO₂ fixation, O₂ evolution and partial reactions of photosynthetic electron transport in comparison to unirradiated cells. Incubation of irradiated cells for 24 h in light or dark resulted in decline in photosynthesis. The decline in photosynthesis was higher in the cells incubated in light as compared to the cells incubated in dark. Among the partial reactions of electron transport, only PSII activity declined drastically after incubation of irradiated samples. This was also supported by the analysis of membrane functions using thermoluminescence. Exposure of cyanobacteria to high doses of ⁶⁰Co γ radiation did not affect the thylakoid membrane ultrastructure immediately after exposure as shown by electron microscopy. The level of reactive oxygen species (ROS) in irradiated cells was 20 times higher as compared to control. In irradiated cells de novo protein synthesis was reduced considerably immediately after irradiation. Treatment of cells with tetracycline also affected photosynthesis as in irradiated cells. The results showed that photoinhibition of photosynthetic apparatus after incubation of irradiated cells was probably augmented due to reduced protein synthesis. Active photosynthesis is known to require uninterrupted replenishment of some of the proteins involved in electron transport chain. The defective thylakoid membrane biogenesis may be leading to photosynthetic decline post-irradiation.     

ACTION SPECTRUM FOR THE PHOTOINHIBITION OF BIOLUMINESCENCE IN THE MARINE DINOFLAGELLATE DISSODINIUM LUNULA

Abstract— The fractional photoinhibition of the mechanically stimulable bioluminescence in the vacuolar dinoflagellate Dissodinium lunula is proportional to the logarithm of the exposure. The action spectrum for this photoinhibition has been determined by measuring threshold exposures in absolute units of photons cm⁻². The threshold exposure at the wavelength of maximum sensitivity, 450 nm, was 2 ± 10⁻² photons cm⁻². The action spectrum is consistent with absorption by a blue light receptor pigment shielded by a nonphotoactive pigment which absorbs in the region of the bioluminescence emission spectrum. It is suggested that there may be some selective advantage for this absorbing pigment in the vacuolar dinoflagellates in order to prevent the organisms from being photoinhibited by their own bioluminescence.     

A Five‐year Study of Solar Ultraviolet Radiation in Southern Chile (39° S): Potential Impact on Physiology of Coastal Marine Algae?

This study reports 5 years of (1998-2003) data on continuous solar-irradiation measurements from a scanning spectroradiometer (SUV-100) in Valdivia, Chile (39 degrees S), accompanied by evaluation of the impact of ultraviolet radiation (UVR) on marine macroalgae of this site. UVR conditions showed a strong seasonal variation, which was less pronounced toward longer wavelengths. Daily maximum dose rates (clear days) averaged in winter-summer: UV-B(290-315 nm) 0.30-2.1, UV-B(290-320 nm) 0.70-3.7, UV-A(315-400 nm) 20.6-62.1, UV-A(320-400 nm) 20.2-60.5 W m(-2), and photosynthetically active radiation (PAR) 969-2423 micromol m(-2) s(-1). The corresponding daily doses (all the days) ranged: UV-B(290-315 nm) 2.6-40.7, UV-B(290-320 nm) 6.7-78.5, UV-A(315-400 nm) 228-1539, UV-A(320-400 nm) 224-1501, and PAR 2008-13308 kJ m(-2) d(-1). Taking into consideration action spectra of a biological interest, the risk of UV exposure could be up to 37 times higher in summer than in winter. The photosynthetic activity (as maximum quantum yield of chlorophyll fluorescence, F(v)/F(m)) of the brown alga Lessonia nigrescens from the infralittoral zone was markedly more sensitive to UVR than of the green alga Enteromorpha intestinalis from the upper midlittoral, and the UV-B wave band increased markedly photoinhibition. In L. nigrescens, maximal photoinhibition (40%) took place at weighted (the action spectrum for photoinhibition of photosynthesis) UVR doses of 800 kJ m(-2), irrespective of the season (corresponding midsummer daily dose in Valdivia is 480 kJ m(-2)). In winter, when this alga was at its most sensitive, the weighted UV dose causing 35-40% photoinhibition was around 200 kJ m(-2). In E. intestinalis, weighted doses of 800 kJ m(-2) resulted in low photoinhibition (<10 %) and no clear seasonal patterns could be inferred. These results confirm that midday summer levels of UV-B and their daily doses in southern Chile are high enough to produce stress to intertidal macroalgae.     

CHEMIEXCITATION IN THE PEROXIDATIVE METABOLISM OF N- METHYLCARBAZOLE: MECHANISTIC IMPLICATIONS

Abstract –The peroxidative metabolism of TV-methylcarbazole emits light independently of the presence of oxygen. It is likely that two chemiexcited transients are formed by electron transfer to the activated peroxidase, the cation radical by one electron transfer and a cation biradical by two electron transfer consistent with the failure to observe horseradish peroxidase-II in the steady state of the reaction. In the spectral range investigated (390–700 nm) the observed emission (570–700 nm) is ascribed to the biradical, as the latter is equivalent to an excited state of the postulated iminium cation.
While lipoxygenase has no effect upon JV-methylcarbazole, it markedly enhances the emission if peroxidase is present. This effect requires oxygen and is ascribed to an excited product formed by lipoxygenase acting upon an intermediate hydroperoxide of the aerobic process promoted by peroxidase.     

The Use of Solar Radiation by the Photosynthetic Bacterium,Rhodopseudomonas palustris: Model Simulation of Conditions Found in a Shallow Pond or a Flatbed Reactor

Photosynthetic bacteria are attractive for biotechnology because they produce no oxygen and so H₂‐production is not inhibited by oxygen as occurs in oxygenic photoorganisms. Rhodopseudomonas palustris and Afifella marina containing BChl a can use irradiances from violet near‐UV (VNUV) to orange (350–650 nm) light and near‐infrared (NIR) light (762–870 nm). Blue diode‐based pulse amplitude modulation technology was used to measure their photosynthetic electron transport rate (ETR). ETR vs Irradiance curves fitted the waiting‐in‐line model—ETR = (ETR_max × E/E_opt) × exp (1 ? E/E_opt). The equation was integrated over pond depth to calculate ETR of Afifella and Rhodopseudomonas in a pond up to 30 cm deep (A₃₇₆, 1 cm = 0.1). Afifella saturates at low irradiances and so photoinhibition results in very low photosynthesis in a pond. Rhodopseudomonas saturates at ≈15% sunlight and shows photoinhibition in the surface layers of the pond. Total ETR is ≈335 μmol (e^?) m^?2 s^?1 in NUV + photosynthetically active radiation light (350–700 nm). Daily ETR curves saturate at low irradiances and have a square‐wave shape: ≈11–13 mol (e^?) m^?2 day^?1 (350–700 nm). Up to 20–24% of daily 350–700 nm irradiance can be converted into ETR. NIR is absorbed by water and so competes with the bacterial RC‐2 photosystem for photons.     

PICOSECOND TIME-RESOLVED EMISSION SPECTRA OF PHOTOINHIBITED AND PHOTOBLEACHED Anabaena variabilis

Abstract— Time resolved emission spectra have been measured of Anabaena variabilis cells which were grown under different light conditions. The spectra of algae photoinhibited with strong white light for 6 h as well as of algae irradiated with blue light are similar to those of the control (weak white light). Cells that were photobleached with strong white light or red light (5 days each) show dramatic changes in their time resolved emission spectra. The contributions of long-lived components to the time resolved emission spectra are large in photobleached cells. In both the reference sample and in photoinhibited cells the short-lived components with lifetimes in the picosecond range prevail which indicates efficient energy transfer within the antenna pigments. The results upon photobleaching are discussed in terms of a functional decoupling of the phycobilisome rods from the core while photoinhibition does not influence the pigment composition and the molecular organization of the antenna pigments.     

Variability of UVR effects on photosynthesis of summer phytoplankton assemblages from a tropical coastal area of the South China Sea

From June to September 2005, we carried out experiments to determine the ultraviolet radiation (UVR) -induced photoinhibition of summer phytoplankton assemblages from a coastal site of the South China Sea. Variability in taxonomic composition was determined throughout the summer, with a peak chlorophyll a (chl a approximately 20 microg chl a L(-1)) dominated by the diatom Skeletonema costatum that was detected early in the study period; the rest of the time samples were characterized by monads and flagellates, with low chl a values (1-5 chl a microg L(-1)). Surface water samples were placed in quartz tubes, inoculated with radiocarbon and exposed to solar radiation for 2-3 h to determine photosynthetic rates under three quality radiation treatments (i.e. PAB, 280-700 nm; PA, 320-700 nm and P, 400-700 nm) using different filters and under seven levels of ambient irradiance using neutral density screens (P vs E curves). UVR inhibition of samples exposed to maximum irradiance (i.e. at the surface) varied from -12.2% to 50%, while the daytime-integrated UVR-related photoinhibition in surface seawater varied from -62% to 7%. The effects of UVR on the photosynthetic parameters P(B)(max) and E(k) were also variable, but UV-B accounted for most of the observed variability. During sunny days, photosynthesis of microplankton (>20 microm) and piconanoplankton (<20 microm) were significantly inhibited by UVR (mostly by UV-B). However, during cloudy days, while piconanoplankton cells were still inhibited by UVR, microplankton cells used UVR (mostly UV-A) as the source of energy for photosynthesis, resulting in higher carbon fixation in samples exposed to UVR than the ones exposed only to photosynthetically active radiation (PAR). Our results indicate that size structure and cloudiness clearly condition the overall impact of UVR on phytoplankton photosynthesis in this tropical site of South China. In addition, model predictions for this area considering only PAR for primary production might have underestimated carbon fixation due to UVR contribution.     

Probing the active site of trypsin with rose bengal: insights into the photodynamic inactivation of the enzyme

In this work the active site of trypsin has been probed with the dye rose bengal. The dye binds competitively to the enzyme, and it can be used as a probe of the active site of the enzyme. On the basis of the emission wavelength, the binding site of trypsin is relatively polar and is similar to that of acetone in its polarity. The triplet state of rose bengal is quenched by trypsin. This quenching may be caused by the tryptophan and tyrosine residues that are in the near vicinity of the trypsin active site. This quenching can compete with the formation of singlet oxygen from the excited triplet state of rose bengal. We demonstrate that the singlet oxygen involved in the photoinactivation of trypsin is produced by the free rose bengal in solution and the bound dye is incapable of producing singlet oxygen. This explains the lack of correlation between photoinactivation efficiency and sensitizer binding capability previously reported by Wade and Spikes.     

含哌啶取代酞菁金属配合物的合成及其对癌细胞光灭活作用

采用“模板法”合成8种含哌啶取代酞菁金属配合物[(PEO)4PcM, M=Zn, Ni, Co, Cu, PEO=2-(哌啶-1-基)乙氧基], 采用FTIR、质谱和元素分析等技术对其进行了表征. 分别测定了它们的紫外-可见吸收光谱、荧光发射光谱和光敏化产生单线态氧的能力. 研究结果表明, 2种酞菁锌配合物均具有较高的摩尔消光系数、一定的荧光量子产率和较大的单线态氧生成速率. 通过光动力灭活BEL7402肝癌细胞的试验研究发现, β-(PEO)4PcZn的浓度为10 μmol/L时, 在670 nm激光辐照下, 光剂量为1.2 J时, 对癌细胞的抑制率可达到83%.     

Measurement of singlet-oxygen in vivo: progress and pitfalls

This article is a highlight of the paper by Jarvi et al. in this issue of Photochemistry and Photobiology as well as a brief overview of the state of the field of singlet-oxygen ((1) O(2) ) detection in vivo. The in vivo detection of (1) O(2) using its characteristic 1270 nm phosphorescence is technically challenging. Nevertheless, substantial progress has been made in this area. Major advances have included the commercial development of photomultiplier tubes sensitive to 1270 nm light, techniques for spatially resolving the location of (1) O(2) at a subcellular level and more complex mathematical models for interpreting the kinetics of (1) O(2) emission from living cells. It is now recognized that oxygen consumption, photosensitizer bleaching, oxidation of biological molecules and diffusion of (1) O(2) can significantly change the kinetics of (1) O(2) emission from living cells.     

Interactions between photosynthesis and 'light-enhanced dark respiration' (LEDR) in the flagellate Euglena gracilis after irradiation with ultraviolet radiation

The effects of ultraviolet radiation (UV-A, 315-400 nm plus UV-B, 280-315 nm) on photosynthesis and 'light-enhanced dark respiration' (LEDR) in Euglena gracilis have been investigated by using light pulses (80 s) with increasing photon fluence rates of 59, 163, 600, 1180, 2080 and 3340 micromol m(-2) s(-1) and dark periods between the light pulses. LEDR is estimated as the maximum rate of oxygen consumption after a period of light minus the rate of oxygen consumption 30 s after the maximum rate. Without any exposure to UV radiation, the photosynthetic rate and LEDR increase with increasing photon fluence rate. After 20 and 40 min exposures to UV radiation, the photosynthetic rate and LEDR as functions of photon fluence rate are reduced. After a 20 min UV treatment respiration is greater than photosynthesis after the first light pulse of 59 micromol m(-2) s(-1) radiation, and especially at higher photon fluence rates photosynthesis is lower than the control values. The inhibitory effects of UV radiation on photosynthetic rate and LEDR are greater after a 40 min UV exposure than after a 20 min exposure. Only at 600 micromol m(-2) s(-1) is the rate of oxygen evolution greater than that of oxygen consumption after a 40 min UV treatment. Both photosynthetic rate and LEDR are inhibited by the photosynthetic inhibitor DCMU (10(-5) M) in a similar way, which indicates close regulatory interactions between photosynthesis and LEDR. Potassium cyanide (KCN) inhibits dark respiration more than it inhibits LEDR. Dark respiration is not affected to the same degree by UV radiation as are photosynthesis and LEDR.     

Photocatalytic Reduction of Nicotinamide Co-factor by Perylene Sensitized RhIII Complexes**

The ambitious goal of artificial photosynthesis is to develop active systems that mimic nature and use light to split water into hydrogen and oxygen. Intramolecular design concepts are particularly promising. Herein, we firstly present an intramolecular photocatalyst integrating a perylene-based light-harvesting moiety and a catalytic rhodium center ( Rh^IIIphenPer ). The excited-state dynamics were investigated by means of steady-state and time-resolved absorption and emission spectroscopy. The studies reveal that photoexcitation of Rh^IIIphenPer yields the formation of a charge-separated intermediate, namely Rh^IIphenPer ⋅ ⁺ , that results in a catalytically active species in the presence of protons.