Structural Basis of Efficient Electron Transport between Photosynthetic Membrane Proteins and Plastocyanin in Spinach Revealed Using Nuclear Magnetic Resonance

In the photosynthetic light reactions of plants and cyanobacteria, plastocyanin (Pc) plays a crucial role as an electron carrier and shuttle protein between two membrane protein complexes: cytochrome b₆f (cyt b₆f) and photosystem I (PSI). The rapid turnover of Pc between cyt b₆f and PSI enables the efficient use of light energy. In the Pc-cyt b₆f and Pc-PSI electron transfer complexes, the electron transfer reactions are accomplished within <10⁻⁴ s. However, the mechanisms enabling the rapid association and dissociation of Pc are still unclear because of the lack of an appropriate method to study huge complexes with short lifetimes. Here, using the transferred cross-saturation method, we investigated the residues of spinach (Spinacia oleracea) Pc in close proximity to spinach PSI and cyt b₆f, in both the thylakoid vesicle–embedded and solubilized states. We demonstrated that the hydrophobic patch residues of Pc are in close proximity to PSI and cyt b₆f, whereas the acidic patch residues of Pc do not form stable salt bridges with either PSI or cyt b₆f, in the electron transfer complexes. The transient characteristics of the interactions on the acidic patch facilitate the rapid association and dissociation of Pc.     

Activation of the Stt7/STN7 Kinase through Dynamic Interactions with the Cytochrome b6f Complex

Photosynthetic organisms have the ability to adapt to changes in light quality by readjusting the cross sections of the light-harvesting systems of photosystem II (PSII) and photosystem I (PSI). This process, called state transitions, maintains the redox poise of the photosynthetic electron transfer chain and ensures a high photosynthetic yield when light is limiting. It is mediated by the Stt7/STN7 protein kinase, which is activated through the cytochrome b₆f complex upon reduction of the plastoquinone pool. Its probable major substrate, the light-harvesting complex of PSII, once phosphorylated, dissociates from PSII and docks to PSI, thereby restoring the balance of absorbed light excitation energy between the two photosystems. Although the kinase is known to be inactivated under high-light intensities, the molecular mechanisms governing its regulation remain unknown. In this study we monitored the redox state of a conserved and essential Cys pair of the Stt7/STN7 kinase and show that it forms a disulfide bridge. We could not detect any change in the redox state of these Cys during state transitions and high-light treatment. It is only after prolonged anaerobiosis that this disulfide bridge is reduced. It is likely to be mainly intramolecular, although kinase activation may involve a transient covalently linked kinase dimer with two intermolecular disulfide bonds. Using the yeast two-hybrid system, we have mapped one interaction site of the kinase on the Rieske protein of the cytochrome b₆f complex.Photosynthetic organisms are subjected to constant changes in light quality and quantity and need to adapt to these changes in order to optimize, on the one hand, their photosynthetic yield, and to minimize photo-oxidative damage on the other. The photosynthetic electron transfer chain consists of photosystem II (PSII), the plastoquinone (PQ) pool, the cytochrome b₆f complex (Cyt b₆f), plastocyanin, and photosystem I (PSI). All of these complexes and components are integrated or closely associated with the thylakoid membrane. The two antenna systems of PSII and PSI capture and direct the light excitation energy to the corresponding reaction centers in which a chlorophyll dimer is oxidized and charge separation occurs across the thylakoid membrane. These processes lead to the onset of electron flow from water on the donor side of PSII to ferredoxin on the acceptor side of PSI coupled with proton translocation across the thylakoid membrane. In order to sustain optimal electron flow along this electron transfer chain, the redox poise needs to be maintained under changing environmental conditions. Several mechanisms have evolved for the maintenance of this redox balance. In the case of over-reduction of the acceptor side of PSI, excess electrons can reduce molecular oxygen through the Mehler reaction to superoxide, which is then converted to hydrogen peroxide by a plastid superoxide dismutase and ultimately to water by a peroxidase (Asada, 2000). Over-reduction of the PQ pool can be alleviated by PTOX, the plastid terminal oxidase responsible for oxidizing PQH₂ to form hydrogen peroxide, which is subsequently converted to water (Carol et al., 1999; Cournac et al., 2000; Wu et al., 1999).In addition to these electron sinks that prevent the over-reduction of the electron transfer chain, the photosynthetic apparatus is able to maintain the redox poise of the PQ pool by readjusting the relative cross sections of the light harvesting systems of PSII and PSI upon unequal excitation of the two photosystems. This readjustment can occur both in the short term through state transitions and in the long term by changing the stoichiometry between PSII and PSI (Bonaventura and Myers, 1969; Murata, 1969; Pfannschmidt, 2003). State transitions occur because of perturbations of the redox state of the PQ pool due to unequal excitation of PSII and PSI, limitations in electron acceptors downstream of PSI, and/or in CO₂ availability. Excess excitation of PSII relative to PSI leads to reduction of the PQ pool and thus favors the docking of PQH₂ to the Qo site of the Cyt b₆f complex. This process activates the Stt7/STN7 protein kinase (Vener et al., 1997; Zito et al., 1999), which is closely associated with this complex and leads to the phosphorylation of some LHCII proteins and to their detachment from PSII and binding to PSI (Depège et al., 2003; Lemeille et al., 2009). Although both Lhcb1 and Lhcb2 are phosphorylated, only the phosphorylated form of Lhcb2 is associated with PSI whereas phosphorylated Lhcb1 is excluded from this complex (Longoni et al., 2015). This state corresponds to state 2. In this way the change in the relative antenna sizes of the two photosystems restores the redox poise of the PQ pool. The process is reversible as over-excitation of PSI relative to PSII leads to the oxidation of the PQ pool and to the inactivation of the kinase. Under these conditions, phosphorylated LHCII associated with PSI is dephosphorylated by the PPH1/TAP38 phosphatase (Pribil et al., 2010; Shapiguzov et al., 2010) and returns to PSII (state 1). It should be noted, however, that a strict causal link between LHCII phosphorylation and its migration from PSII to PSI has been questioned recently by the finding that some phosphorylated LHCII remains associated with PSII supercomplexes and that LHCII serves as antenna for both photosystems under most natural light conditions (Drop et al., 2014; Wientjes et al., 2013).State transitions are important at low light but do not occur under high light because the LHCII kinase is inactivated under these conditions (Schuster et al., 1986). It was proposed that inactivation of the kinase is mediated by the ferredoxin-thioredoxin system and that a disulfide bond in the kinase rather than in the substrate may be the target site of thioredoxin (Rintamäki et al., 1997, 2000). Analysis of the Stt7/STN7 protein sequences indeed reveals the presence of two conserved Cys residues close to the N-terminal end of this kinase, which are conserved in all species examined and both are essential for kinase activity although they are located outside of the kinase catalytic domain (Fig. 1) (Depège et al., 2003; Lemeille et al., 2009). Based on protease protection studies, this model of the Stt7/STN7 kinase proposes that the N-terminal end of the kinase is on the lumen side of the thylakoid membrane separated from the catalytic domain on the stromal side by an unusual transmembrane domain containing several Pro residues (Lemeille et al., 2009). This configuration of the kinase allows its catalytic domain to act on the substrate sites of the LHCII proteins, which are exposed to the stroma. Although in this model the conserved Cys residues in the lumen are on the opposite side from the stromal thioredoxins, it is possible that thiol-reducing equivalents are transferred across the thylakoid membrane through the CcdA and Hcf164 proteins, which have been shown to operate in this way during heme and Cyt b₆f assembly (Lennartz et al., 2001; Page et al., 2004) or through the LTO1 protein (Du et al., 2015; Karamoko et al., 2011).Figure 1.Conserved Cys in the Stt7/STN7 kinase. Alignment of the sequences of the Stt7/STN protein kinase from Selaginella moelendorffii (Sm), Physcomitrella patens (Pp), Oryza sativa (Os), Populus trichocarpa (Pt), Arabidopsis thaliana (At), Chlamydomonas reinhardtii ...Here we have examined the redox state of the Stt7/STN7 kinase during state transitions and after illumination with high light to test the proposed model. We find that the Stt7/STN7 kinase contains a disulfide bridge that appears to be intramolecular and maintained not only during state transitions but also in high light when the kinase is inactive. Although these results suggest at first sight that the disulfide bridge of Stt7/STN7 is maintained during its activation and inactivation, we propose that a transient opening of this bridge occurs during the activation process followed by the formation of an intermolecular disulfide bridge and the appearance of a short-lived, covalently linked kinase dimer.     

The Redox Potential of the Plastoquinone Pool of the Cyanobacterium Synechocystis Species Strain PCC 6803 Is under Strict Homeostatic Control

A method is presented for rapid extraction of the total plastoquinone (PQ) pool from Synechocystis sp. strain PCC 6803 cells that preserves the in vivo plastoquinol (PQH₂) to -PQ ratio. Cells were rapidly transferred into ice-cold organic solvent for instantaneous extraction of the cellular PQ plus PQH₂ content. After high-performance liquid chromatography fractionation of the organic phase extract, the PQH₂ content was quantitatively determined via its fluorescence emission at 330 nm. The in-cell PQH₂-PQ ratio then followed from comparison of the PQH₂ signal in samples as collected and in an identical sample after complete reduction with sodium borohydride. Prior to PQH₂ extraction, cells from steady-state chemostat cultures were exposed to a wide range of physiological conditions, including high/low availability of inorganic carbon, and various actinic illumination conditions. Well-characterized electron-transfer inhibitors were used to generate a reduced or an oxidized PQ pool for reference. The in vivo redox state of the PQ pool was correlated with the results of pulse-amplitude modulation-based chlorophyll a fluorescence emission measurements, oxygen exchange rates, and 77 K fluorescence emission spectra. Our results show that the redox state of the PQ pool of Synechocystis sp. strain PCC 6803 is subject to strict homeostatic control (i.e. regulated between narrow limits), in contrast to the more dynamic chlorophyll a fluorescence signal.The photosynthetic apparatus of oxygenic phototrophs consists of two types of photosynthetic reaction centers: PSII and PSI. Both photosystems are connected in series, with electrons flowing from PSII toward PSI through an intermediate electron transfer chain, which comprises the so-called plastoquinone (PQ) pool, plastocyanin and/or cytochrome c₅₅₃, and the cytochrome b₆f complex. The redox potential of the PQ pool is clamped by the relative rates of electron release into and uptake from this pool. Within the PSII complex, electrons are extracted from water at the lumenal side of the thylakoid membrane and transferred to the primary accepting quinone (Q_A) at the stromal side. The electron is subsequently transferred to a PQ molecule in the secondary accepting quinone (Q_B) of PSII. The intermediate Q_B semiquinone, which is formed accordingly, is stable in the Q_B site for several seconds (Diner et al., 1991; Mitchell, 1993) and subsequently can be reduced to plastoquinol (PQH₂). The midpoint potential of Q_A reduction is approximately −100 mV (Krieger-Liszkay and Rutherford, 1998; Allakhverdiev et al., 2011), whereas the corresponding midpoint potential of the Q_B semiquinone is close to zero (Nicholls and Ferguson, 2013). PQH₂ equilibrates with the PQ pool in the thylakoid membranes, which has a size that is approximately 1 order of magnitude larger than the number of PSII reaction centers (Melis and Brown, 1980; Aoki and Katoh, 1983).PQ is a lipophilic, membrane-bound electron carrier, with a midpoint potential of +80 mV (Okayama, 1976), that can accept two electrons and two protons to form PQH₂ (Rich and Bendall, 1980). PQH₂ can donate both electrons to the cytochrome b₆f complex, one to low-potential cytochrome b₆, by which reduced high-potential cytochrome b₆ is formed, and one to the cytochrome f moiety on the lumenal side of the thylakoid membrane, where the two protons are released. High-potential cytochrome b₆ then donates an electron back to PQ on the stromal side of the membrane, rendering a semiquinone in the PQ-binding pocket on the cytoplasmic face of the b₆f complex ready as an acceptor of another electron from PSII, and reduced cytochrome f feeds an electron to a water-soluble electron carrier (i.e. either plastocyanin or cytochrome c₅₅₃) for subsequent transfer to the reaction center of PSI or to cytochrome c oxidase, respectively (Rich et al., 1991; Geerts et al., 1994; Schubert et al., 1995; Paumann et al., 2004; Mulkidjanian, 2010).Electron transfer through the cytochrome b₆f complex proceeds according to the Q-cycle mechanism (Rich et al., 1991). As a result, maximally two protons from the stroma are released into the lumen per electron transferred. This electrochemical proton gradient can be used for the synthesis of ATP by the ATP synthase complex (Walker, 1998). In PSI, another transthylakoid membrane charge separation process is energized by light. Electron transfer within the PSI complex involves iron-sulfur clusters and quinones and leads to the reduction of ferredoxin, the reduced form of which serves as the electron donor for NADPH by the ferredoxin:NADP+ oxidoreductase enzyme (van Thor et al., 1999). The ATP and NADPH generated this way are used for CO₂ fixation in a mutual stoichiometry that is close to the stoichiometry at which these two energy-rich compounds are formed at the thylakoid membrane. Normally, this ratio is ATP:NADPH = 3:2 (Behrenfeld et al., 2008).Photosynthetic and respiratory electron transport in cyanobacteria share a single PQ pool (Aoki and Katoh, 1983; Aoki et al., 1983; Matthijs et al., 1984; Scherer, 1990). Respiratory electron transfer provides cells the ability to form ATP in the dark, but this ability is not limited to those conditions. Transfer of electrons into the PQ pool is the result of the joint activity of PSII, respiratory dehydrogenases [in particular those specific for NAD(P)H and succinate], and cyclic electron transport around PSI (Mi et al., 1995; Cooley et al., 2000; Howitt et al., 2001;Yeremenko et al., 2005), whereas oxidation of PQH₂ is catalyzed by the PQH₂ oxidase, the cytochrome b₆f complex, the respiratory cytochrome c oxidase (Nicholls et al., 1992; Pils and Schmetterer, 2001; Berry et al., 2002), and possibly plasma terminal oxidase (Peltier et al., 2010). Multiples of these partial reactions can proceed simultaneously, including respiratory electron transfer during illumination (Schubert et al., 1995), which includes oxygen uptake through a Mehler-like reaction (Helman et al., 2005; Allahverdiyeva et al., 2013).Because of its central location between the two photosystems, the redox state of the PQ pool has been identified as an important parameter that can signal photosynthetic imbalances (Mullineaux and Allen, 1990; Allen, 1995; Ma et al., 2010; Allen et al., 2011). Yet, an accurate estimation of the in vivo redox state of this pool has not been reported in cyanobacteria so far. Instead, the redox state of the PQ pool is widely assumed to be reflected in, or related to, the intensity of the chlorophyll a fluorescence emissions (Prasil et al., 1996; Yang et al., 2001; Gotoh et al., 2010; Houyoux et al., 2011). Imbalance in electron transport through the two photosystems may lead to a loss of excitation energy and, hence, to a loss of chlorophyll a fluorescence emission (Schreiber et al., 1986). Therefore, patterns of chlorophyll a fluorescence (pulse-amplitude modulated [PAM] fluorimetry; Baker, 2008) have widely been adopted for the analysis of (un)balanced photosynthetic electron transfer and, by inference, for indirect recording of the redox state of the PQ pool. However, the multitude of electron transfer pathways in the thylakoid membranes of cyanobacteria (see above) makes it much more complex to explain PAM signals in these organisms than in chloroplasts (Campbell et al., 1998). Additional regulatory mechanisms of nonphotochemical quenching, via the xanthophyll cycle in chloroplasts (Demmig-Adams et al., 2012) and the orange carotenoid protein (Kirilovsky and Kerfeld, 2012) in cyanobacteria, and energy redistribution via state transitions (Allen, 1995; Van Thor et al., 1998) complicate such comparisons even further.Several years ago, an HPLC-based technique was developed for the detection of the redox state of PQH₂ in isolated thylakoids (Kruk and Karpinski, 2006), but these results have neither been related to physiological conditions nor to the results of chlorophyll a fluorescence measurements. In this report, we describe an adaptation of this method with elements of a method for estimation of the redox state of the ubiquinone pool in Escherichia coli (Bekker et al., 2007). This modified method allows for reliable measurements of the redox state of the PQ pool of Synechocystis sp. strain PCC 6803 under physiologically relevant conditions. The method uses rapid cell lysis in an organic solvent to arrest all physiological processes, followed by extraction and identification of PQH₂ by HPLC separation with fluorescence detection. Next, we manipulated the redox state of the PQ pool with various redox-active agents, with inhibitors of photosynthetic electron flow, and by illumination with light specific for either PSII or PSI. The measured redox state of the PQ pool was then related to the chlorophyll a fluorescence signal and 77 K fluorescence emission spectra of cell samples taken in parallel and to oxygen-exchange rates measured separately. These experiments reveal that, despite highly fluctuating conditions of photosynthetic and respiratory electron flow, a remarkably stable redox state of the PQ pool is maintained. This homeostatically regulated redox state correlates poorly in many of the conditions tested with the more dynamic signal of chlorophyll a fluorescence emission, as measured with PAM fluorimetry. The latter signal only reflects the redox state of Q_A and not that of the PQ pool.     

DAC Is Involved in the Accumulation of the Cytochrome b6/f Complex in Arabidopsis

The biogenesis and assembly of photosynthetic multisubunit protein complexes is assisted by a series of nucleus-encoded auxiliary protein factors. In this study, we characterize the dac mutant of Arabidopsis (Arabidopsis thaliana), which shows a severe defect in the accumulation of the cytochrome b₆/f complex, and provide evidence suggesting that the efficiency of cytochrome b₆/f complex assembly is affected in the mutant. DAC is a thylakoid membrane protein with two predicted transmembrane domains that is conserved from cyanobacteria to vascular plants. Yeast (Saccharomyces cerevisiae) two-hybrid and coimmunoprecipitation analyses revealed a specific interaction between DAC and PetD, a subunit of the cytochrome b₆/f complex. However, DAC was found not to be an intrinsic component of the cytochrome b₆/f complex. In vivo chloroplast protein labeling experiments showed that the labeling rates of the PetD and cytochrome f proteins were greatly reduced, whereas that of the cytochrome b₆ protein remained normal in the dac mutant. DAC appears to be a novel factor involved in the assembly/stabilization of the cytochrome b₆/f complex, possibly through interaction with the PetD protein.The cytochrome b₆/f (Cyt b6/f) complex is a multisubunit complex that resides in the thylakoid membrane and functions in linear and cyclic electron transport. In the linear process, the complex receives electrons from PSII and transfers them to PSI, a process that is accompanied by the generation of a proton gradient, which is essential for ATP synthesis (Mitchell, 1961; Saraste, 1999). The native form of this complex is present as a dimer with a mass of 310 kD that can be converted into a 140-kD monomer with increasing detergent concentrations (Huang et al., 1994; Breyton et al., 1997; Mosser et al., 1997; Baniulis et al., 2009). In higher plants, the Cyt b6/f monomer contains at least eight subunits: Cyt f, Cyt b₆, PetC, PetD, PetM, PetL, PetG, and PetN (Wollman, 2004). PetC and PetM are encoded by nuclear genes, whereas the others are encoded by plastid genes. It has been shown that PetG and PetN are necessary for complex stability in tobacco (Nicotiana tabacum; Schwenkert et al., 2007). By contrast, PetL is not required for the accumulation of other subunits of the Cyt b6/f complex, even though it is involved in the stability and formation of the functional dimer (Bendall et al., 1986; Schwenkert et al., 2007). Inactivation of PetC in Arabidopsis (Arabidopsis thaliana) resulted in significantly reduced amounts of Cyt b6/f subunits and completely blocked linear electron transport, indicating that PetC participates in the formation of the functionally assembled Cyt b6/f complex (Maiwald et al., 2003). In Synechocystis sp. PCC 6803, the PetM subunit has no essential role in Cyt b6/f complex electron transfer or accumulation; however, the absence of this subunit apparently affects the levels of other protein complexes involved in energy transduction (Schneider et al., 2001). In addition to the other proteins, FNR was identified as a subunit of the Cyt b6/f complex isolated from spinach (Spinacia oleracea) thylakoid membranes (Zhang et al., 2001).Previous research has revealed how the Cyt b6/f complex assembles into a functional dimer (Bendall et al., 1986; Lemaire et al., 1986; Kuras and Wollman, 1994). In the Cyt b6/f complex, Cyt b₆ and PetD form a mildly protease-resistant subcomplex that serves as a template for the assembly of Cyt f and PetG, producing a protease-resistant cytochrome moiety (Wollman, 2004). The PetC and PetL proteins then participate in the assembly of the functional dimer (Schwenkert et al., 2007). PetD becomes more unstable in the absence of Cyt b₆, and the synthesis of Cyt f is greatly reduced when either Cyt b₆ or PetD is inactivated, indicating that both Cyt b₆ and PetD are prerequisite for the synthesis of Cyt f (Kuras and Wollman, 1994). The reduced synthesis of Cyt f can be explained by the so-called CES (for controlled by epistasy of synthesis) mechanism. It is suggested that, in this mechanism, the synthesis rate of some chloroplast-encoded subunits of photosynthetic protein complexes is regulated by the availability of their assembly partners from the same complexes (Choquet et al., 2001). The mechanism of CES for Cyt f has been studied in detail in Chlamydomonas reinhardtii (Choquet et al., 1998; Choquet and Vallon, 2000). In it, the unassembled Cyt f inhibits its own translation through a negative feedback mechanism, and MCA1 and TCA1 have been demonstrated to be involved in the regulation of Cyt f synthesis (Boulouis et al., 2011).Many studies have focused on understanding the conversion of apocytochrome to holocytochrome via the covalent binding of heme in Cyt f and Cyt b₆ during the assembly of Cyt b6/f through the CCS and CCB pathways (Nakamoto et al., 2000; Wollman, 2004; de Vitry, 2011). The CCS pathway was originally discovered in the green alga C. reinhardtii through genetic studies of ccs mutants (for cytochrome c synthesis) that display a specific defect in membrane-bound Cyt f and soluble Cyt c₆, two thylakoid lumen-resident c-type cytochromes functioning in photosynthesis (Xie and Merchant, 1998). In the CCS pathway, six loci that include plastid ccsA and nuclear CCS1 to CCS5 have been found in C. reinhardtii (Xie and Merchant, 1998). In these mutants, the apocytochrome is normally synthesized, targeted, and processed, but heme attachment is perturbed. The CCB pathway is involved in the covalent attachment of heme c(i) to Cyt b₆ on the stromal side of the thylakoid membranes (Kuras et al., 2007). The ccb mutants show defects in the accumulation of subunits of the Cyt b6/f complex and covalent binding of heme to Cyt b₆ (Lyska et al., 2007; Lezhneva et al., 2008). However, heme binding is not a prerequisite for the assembly of Cyt b₆ into the Cyt b6/f complex, although the fully formed Cyt b6/f showed an increased sensitivity to protease (Saint-Marcoux et al., 2009).The assembly of the Cyt b6/f complex is a multistep process, and current studies have shown that the covalent binding of heme to Cyt f and Cyt b₆ is highly regulated. Thus, it is reasonable to speculate that, similar to the other photosynthetic protein complexes (Mulo et al., 2008; Nixon et al., 2010; Rochaix, 2011), the assembly of the Cyt b6/f complex is also assisted by many nucleus-encoded factors. In this study, we characterized an Arabidopsis protein, DAC (for defective accumulation of Cyt b6/f complex), that seems to be involved in the assembly of the Cyt b6/f complex. In addition, we provide evidence that DAC interacts directly with PetD before it assembles within the Cyt b6/f complex.     

Thylakoid Membrane Maturation and PSII Activation Are Linked in Greening Synechocystis sp. PCC 6803 Cells

Thylakoid membranes are typical and essential features of both chloroplasts and cyanobacteria. While they are crucial for phototrophic growth of cyanobacterial cells, biogenesis of thylakoid membranes is not well understood yet. Dark-grown Synechocystis sp. PCC 6803 cells contain only rudimentary thylakoid membranes but still a relatively high amount of phycobilisomes, inactive photosystem II and active photosystem I centers. After shifting dark-grown Synechocystis sp. PCC 6803 cells into the light, “greening” of Synechocystis sp. PCC 6803 cells, i.e. thylakoid membrane formation and recovery of photosynthetic electron transport reactions, was monitored. Complete restoration of a typical thylakoid membrane system was observed within 24 hours after an initial lag phase of 6 to 8 hours. Furthermore, activation of photosystem II complexes and restoration of a functional photosynthetic electron transport chain appears to be linked to the biogenesis of organized thylakoid membrane pairs.Thylakoid membranes are typical and essential features of both chloroplasts and cyanobacteria. The intracellular thylakoid membranes of cyanobacteria harbor the protein complexes of the photosynthetic electron transport chain (Nowaczyk et al., 2010; Bernat and Rögner, 2011). The photosynthetic electron transport chain is composed of three large membrane protein complexes, i.e. PSII, the cytochrome b₆f complex, and PSI. Excitation energy trapping by PSII results in water splitting at the PSII donor side within the thylakoid lumen and transport of electrons to the primary and secondary electron accepting quinone molecules Q_A and Q_B, respectively. Following double reduction and protonation, Q_B is released from PSII into the plastoquinone (PQ) pool and delivers electrons to the cytochrome b₆f complex. The cytochrome b₆f complex transfers the electrons to the soluble electron carrier plastocyanin or cytochrome c₆, which subsequently reduces PSI. For efficient light harvesting, cyanobacteria contain soluble light-harvesting antenna proteins, the phycobilisomes (PBSs), which transfer light energy to the photosynthetic reaction centers. In cyanobacteria, the PSI-to-PSII ratio is controlled by light and by the redox state of the PQ/PQH₂-pool (Fujita et al., 1987), and under high-light growth conditions, typically less PSI is present in cyanobacterial thylakoid membranes compared with low-light conditions (Fujita et al., 1994).Thylakoid membranes and photosynthetic electron transport are essential for phototrophic growth of cyanobacterial cells. Despite their importance for survival of cyanobacteria, biogenesis of thylakoid membranes is yet not well understood. It still is an ongoing debate whether the internal membrane systems (cytoplasmic and thylakoid membranes) are connected in cyanobacteria or not, and thus whether thylakoids represent a completely separated membrane entity (Liberton et al., 2006; van de Meene et al., 2006, 2012; Schneider et al., 2007). Up to now, only few proteins have been described to be involved in thylakoid membrane biogenesis. Among them the Vipp1 protein (vesicle inducing protein in plastids1) seems to play an important role in thylakoid membrane biogenesis, as in chloroplasts of Arabidopsis (Arabidopsis thaliana) and in the cyanobacterium Synechocystis sp. PCC 6803 (hereafter referred to as Synechocystis), depletion of Vipp1 results in a reduced thylakoid membrane system (Kroll et al., 2001; Westphal et al., 2001). While the exact physiological function of the protein is not yet known (Vothknecht et al., 2012), depletion of Vipp1 in Synechocystis not only results in reduced thylakoid membrane formation, but also affects the activity and structure of components of the photosynthetic electron transport chain (Fuhrmann et al., 2009; Gao and Xu, 2009).As complexes of the respiratory electron transport chain are also localized in cyanobacterial thylakoids, the photosynthetic and respiratory electron transport pathways are highly interconnected and both contribute to formation of an electrochemical gradient across the thylakoid membrane and energy production. Due to this, Synechocystis is able to grow completely heterotrophically under light-activated photoheterotrophic growth (LAHG) conditions in the presence of high Glc concentrations (Anderson and McIntosh, 1991; Smart et al., 1991).In this study, we have used dark-grown Synechocystis cells to investigate “greening” of Synechocystis cells, i.e. thylakoid membrane formation and recovery of photosynthetic electron transport reactions. Following transfer of Synechocystis cells into the light, complete restoration of a typical thylakoid membrane system was observed within 24 h. While dark-grown Synechocystis cells contained only rudimentary thylakoid membranes, they still contained a high concentration of PBSs, active PSI as well as inactive PSII complexes. Activation of PSII complexes appears to be linked to the biogenesis of organized thylakoid membrane pairs.     

MET1 Is a Thylakoid-Associated TPR Protein Involved in Photosystem II Supercomplex Formation and Repair in Arabidopsis

Photosystem II (PSII) requires constant disassembly and reassembly to accommodate replacement of the D1 protein. Here, we characterize Arabidopsis thaliana MET1, a PSII assembly factor with PDZ and TPR domains. The maize (Zea mays) MET1 homolog is enriched in mesophyll chloroplasts compared with bundle sheath chloroplasts, and MET1 mRNA and protein levels increase during leaf development concomitant with the thylakoid machinery. MET1 is conserved in C3 and C4 plants and green algae but is not found in prokaryotes. Arabidopsis MET1 is a peripheral thylakoid protein enriched in stroma lamellae and is also present in grana. Split-ubiquitin assays and coimmunoprecipitations showed interaction of MET1 with stromal loops of PSII core components CP43 and CP47. From native gels, we inferred that MET1 associates with PSII subcomplexes formed during the PSII repair cycle. When grown under fluctuating light intensities, the Arabidopsis MET1 null mutant (met1) showed conditional reduced growth, near complete blockage in PSII supercomplex formation, and concomitant increase of unassembled CP43. Growth of met1 in high light resulted in loss of PSII supercomplexes and accelerated D1 degradation. We propose that MET1 functions as a CP43/CP47 chaperone on the stromal side of the membrane during PSII assembly and repair. This function is consistent with the observed differential MET1 accumulation across dimorphic maize chloroplasts.     

HYPERSENSITIVE TO HIGH LIGHT1 Interacts with LOW QUANTUM YIELD OF PHOTOSYSTEM II1 and Functions in Protection of Photosystem II from Photodamage in Arabidopsis

Under high-irradiance conditions, plants must efficiently protect photosystem II (PSII) from damage. In this study, we demonstrate that the chloroplast protein HYPERSENSITIVE TO HIGH LIGHT1 (HHL1) is expressed in response to high light and functions in protecting PSII against photodamage. Arabidopsis thaliana hhl1 mutants show hypersensitivity to high light, drastically decreased PSII photosynthetic activity, higher nonphotochemical quenching activity, a faster xanthophyll cycle, and increased accumulation of reactive oxygen species following high-light exposure. Moreover, HHL1 deficiency accelerated the degradation of PSII core subunits under high light, decreasing the accumulation of PSII core subunits and PSII–light-harvesting complex II supercomplex. HHL1 primarily localizes in the stroma-exposed thylakoid membranes and associates with the PSII core monomer complex through direct interaction with PSII core proteins CP43 and CP47. Interestingly, HHL1 also directly interacts, in vivo and in vitro, with LOW QUANTUM YIELD OF PHOTOSYSTEM II1 (LQY1), which functions in the repair and reassembly of PSII. Furthermore, the hhl1 lqy1 double mutants show increased photosensitivity compared with single mutants. Taken together, these results suggest that HHL1 forms a complex with LQY1 and participates in photodamage repair of PSII under high light.     

PsbN Is Required for Assembly of the Photosystem II Reaction Center in Nicotiana tabacum

The chloroplast-encoded low molecular weight protein PsbN is annotated as a photosystem II (PSII) subunit. To elucidate the localization and function of PsbN, encoded on the opposite strand to the psbB gene cluster, we raised antibodies and inserted a resistance cassette into PsbN in both directions. Both homoplastomic tobacco (Nicotiana tabacum) mutants ∆psbN-F and ∆psbN-R show essentially the same PSII deficiencies. The mutants are extremely light sensitive and failed to recover from photoinhibition. Although synthesis of PSII proteins was not altered significantly, both mutants accumulated only ∼25% of PSII proteins compared with the wild type. Assembly of PSII precomplexes occurred at normal rates, but heterodimeric PSII reaction centers (RCs) and higher order PSII assemblies were not formed efficiently in the mutants. The ∆psbN-R mutant was complemented by allotopic expression of the PsbN gene fused to the sequence of a chloroplast transit peptide in the nuclear genome. PsbN represents a bitopic trans-membrane peptide localized in stroma lamellae with its highly conserved C terminus exposed to the stroma. Significant amounts of PsbN were already present in dark-grown seedling. Our data prove that PsbN is not a constituent subunit of PSII but is required for repair from photoinhibition and efficient assembly of the PSII RC.     

Self-Incompatibility-Induced Programmed Cell Death in Field Poppy Pollen Involves Dramatic Acidification of the Incompatible Pollen Tube Cytosol

Self-incompatibility (SI) is an important genetically controlled mechanism to prevent inbreeding in higher plants. SI involves highly specific interactions during pollination, resulting in the rejection of incompatible (self) pollen. Programmed cell death (PCD) is an important mechanism for destroying cells in a precisely regulated manner. SI in field poppy (Papaver rhoeas) triggers PCD in incompatible pollen. During SI-induced PCD, we previously observed a major acidification of the pollen cytosol. Here, we present measurements of temporal alterations in cytosolic pH ([pH]_cyt); they were surprisingly rapid, reaching pH 6.4 within 10 min of SI induction and stabilizing by 60 min at pH 5.5. By manipulating the [pH]_cyt of the pollen tubes in vivo, we show that [pH]_cyt acidification is an integral and essential event for SI-induced PCD. Here, we provide evidence showing the physiological relevance of the cytosolic acidification and identify key targets of this major physiological alteration. A small drop in [pH]_cyt inhibits the activity of a soluble inorganic pyrophosphatase required for pollen tube growth. We also show that [pH]_cyt acidification is necessary and sufficient for triggering several key hallmark features of the SI PCD signaling pathway, notably activation of a DEVDase/caspase-3-like activity and formation of SI-induced punctate actin foci. Importantly, the actin binding proteins Cyclase-Associated Protein and Actin-Depolymerizing Factor are identified as key downstream targets. Thus, we have shown the biological relevance of an extreme but physiologically relevant alteration in [pH]_cyt and its effect on several components in the context of SI-induced events and PCD.Programmed cell death (PCD) in plants is relatively well documented and characterized (Jones and Dangl, 1996; van Doorn, 2011; van Doorn et al., 2011). There is considerable biochemical evidence for the involvement of caspase-like activities in plant PCD (van Doorn and Woltering, 2005). For example, the vacuolar processing enzyme has YVADase (caspase-1-like) activity (Hatsugai et al., 2004; Rojo et al., 2004; Hara-Nishimura et al., 2005), DEVDase (caspase-3-like) and YVADases are associated with PCD in several plant systems (del Pozo and Lam, 1998; Korthout et al., 2000; Danon et al., 2004), and VEIDase (caspase-6-like) is the main caspase-like activity involved in embryonic pattern formation (Bozhkov et al., 2004). However, because plants have no caspase gene homologs (Sanmartín et al., 2005), the nature of their caspase-like enzymes is the subject of considerable debate. Vacuolar cell death is one of two major classes of PCD in plants (van Doorn et al., 2011). It is thought that collapse of the vacuole is a key irreversible step in several plant PCD systems, including during tissue and organ formation, such as the classic differentiation of tracheary elements (Hara-Nishimura and Hatsugai, 2011). Exactly how this is achieved and what processes are involved remain unknown. Until very recently, it was generally thought that the rupturing vacuole releases proteases, hydrolases, and nucleases, allowing cellular disassembly by an autophagy-like process. Some PCD systems cannot be assigned to either class; these include PCD triggered by the hypersensitive response to biotrophic pathogens, PCD in cereal endosperm, and self-incompatibility (SI)-induced PCD (van Doorn et al., 2011).SI is a genetically controlled pollen-pistil cell-cell recognition system. Self-pollen is recognized by the stigma as being genetically identical, resulting in inhibition of pollen tube growth. Most SI systems use tightly linked polymorphic genes: the pollen (male) and pistil (female) S-determinants. In field poppy (Papaver rhoeas), the S-determinants are a 14-kD signaling ligand field poppy stigma S (PrsS) and a unique transmembrane protein field poppy pollen S (PrpS; Foote et al., 1994; Wheeler et al., 2010). These interact in an S-specific manner, and increases in cytosolic free calcium ([Ca2+]_cyt) are triggered in incompatible pollen tubes (Franklin-Tong et al., 1993), resulting in phosphorylation of soluble inorganic pyrophosphatases (sPPases; Rudd et al., 1996; de Graaf et al., 2006), activation of a Mitogen-Activated Protein Kinase (MAPK; Rudd et al., 2003), and increases in reactive oxygen species (ROS) and nitric oxide (Wilkins et al., 2011, 2014). Most of these components are integrated into a signaling network leading to PCD (Bosch et al., 2008; Wilkins et al., 2014). The actin cytoskeleton is a key target in the field poppy SI response, undergoing depolymerization (Snowman et al., 2002) followed by polymerization into highly stable F-actin foci decorated with the actin binding proteins (ABPs) Actin-Depolymerizing Factor (ADF) and Cyclase-Associated Protein (CAP; Poulter et al., 2010, 2011), with both processes being involved in mediating PCD (Thomas et al., 2006). A major player in SI-mediated PCD is a caspase-3-like/DEVDase-like activity (Thomas and Franklin-Tong, 2004; Bosch and Franklin-Tong, 2007). The SI-induced caspase-3-like/DEVDase exhibits maximum substrate cleavage in vitro at pH 5, with peak activity 5 h after SI induction in vivo (Bosch and Franklin-Tong, 2007). The low pH optimum for this caspase-3-like/DEVDase activity is unusual, because most of the cytosolic plant caspase-like activities identified to date have optimal activity close to normal physiological pH (approximate pH, 6.5–7.0; Korthout et al., 2000; Bozhkov et al., 2004; Coffeen and Wolpert, 2004). Because the SI-induced cytosolic-located DEVDase requires a low pH for activity, this suggested that, during SI, the pollen tube cytosol undergoes dramatic acidification. In vivo pH measurements of the cytosol at 1 to 4 h after SI induction confirmed this, when cytosolic pH ([pH]_cyt) had dropped from pH 6.9 to pH 5.5 (Bosch and Franklin-Tong, 2007). This fits the in vitro pH optimum of the caspase-3-like/DEVDase almost exactly, implicating pollen cytosolic acidification as playing a vital role in creating optimal conditions for the activation of the caspase-3-like/DEVDase-like activity and progression of PCD.Under normal cellular conditions, [pH]_cyt is between approximately 6.9 and 7.5 (Kurkdjian and Guern, 1989; Felle, 2001). Pollen tubes, like other tip-growing cells, have [pH]_cyt gradients (Gibbon and Kropf, 1994; Feijó et al., 1999). The [pH]_cyt of the pollen tube shank is an approximate pH of 6.9 to 7.11 (Fricker et al., 1997; Messerli and Robinson, 1998). There has been much debate about the [pH]_cyt gradient, comprising an apical domain with an approximate pH of 6.8 and a subapical alkaline band with an approximate pH of 7.2 to 7.8 in Lilium longiflorum and Lilium formosanum pollen tubes (Fricker et al., 1997; Messerli and Robinson, 1998; Feijó et al., 2001; Lovy-Wheeler et al., 2006). Oscillations of [pH]_cyt between approximate pH values of 6.9 and 7.3 have been linked to tip growth in L. formosanum pollen tubes (Lovy-Wheeler et al., 2006). The vacuole and the apoplast have a highly acidic pH between pH 5 and pH 6 (Katsuhara et al., 1989; Feijó et al., 1999). The majority of studies of pH changes in plant cells reports modest, transient changes in [pH]_cyt of approximately 0.4 and 0.7 pH units during development, gravitropic responses, decreases in light intensity, and addition of elicitors, hormones, and other treatments. For example, during root hair development in Arabidopsis (Arabidopsis thaliana), root [pH]_cyt was elevated from an approximate pH of 7.3 to 7.7 (Bibikova et al., 1998). Root gravitropic responses stimulate small transient [pH]_cyt alterations (Scott and Allen, 1999; Fasano et al., 2001; Johannes et al., 2001). More recently, it has been shown that the [pH]_cyt drops during PCD controlling root cap development; however, exactly how many units the [pH]_cyt decreased was not measured (Fendrych et al., 2014). Other studies investigating [pH]_cyt in response to physiologically relevant signals also report small transient alterations. Light-adapted cells respond to a decrease in light intensity with a rapid transient cytosolic acidification by approximately 0.3 pH units (Felle et al., 1986). Addition of nodulation factors resulted in an increase of 0.2 pH units in root hairs (Felle et al., 1998), and abscisic acid increased the [pH]_cyt of guard cells by 0.3 pH units (Blatt and Armstrong, 1993). Changes in [pH]_cyt are thought to activate stress responses (Felle, 2001). Elicitor treatments resulted in a [pH]_cyt drop of between 0.4 and 0.7 pH units in suspension cells (Mathieu et al., 1996; Kuchitsu et al., 1997), a drop of 0.2 pH units in Nitellopsis obtusa cells treated with salt (Katsuhara et al., 1989), and a drop of 0.3 to 0.7 pH units in Eschscholzia californica (Roos et al., 1998).Here, we investigate SI-induced acidification of the cytosol, providing measurements of physiologically relevant temporal alterations in [pH]_cyt, and identify key targets of this, providing mechanistic insights into these events. The SI-induced acidification plays a pivotal role in the activation of a caspase-3-like/DEVDase activity, the formation of punctate F-actin foci, and ABP localization during SI PCD. We investigate the vacuole as a potential contributor to SI-induced [pH]_cyt acidification.     

The Type II NADPH Dehydrogenase Facilitates Cyclic Electron Flow,Energy-Dependent Quenching,and Chlororespiratory Metabolism during Acclimation of Chlamydomonas reinhardtii to Nitrogen Deprivation

When photosynthetic organisms are deprived of nitrogen (N), the capacity to grow and assimilate carbon becomes limited, causing a decrease in the productive use of absorbed light energy and likely a rise in the cellular reduction state. Although there is a scarcity of N in many terrestrial and aquatic environments, a mechanistic understanding of how photosynthesis adjusts to low-N conditions and the enzymes/activities integral to these adjustments have not been described. In this work, we use biochemical and biophysical analyses of photoautotrophically grown wild-type and mutant strains of Chlamydomonas reinhardtii to determine the integration of electron transport pathways critical for maintaining active photosynthetic complexes even after exposure of cells to N deprivation for 3 d. Key to acclimation is the type II NADPH dehydrogenase, NDA2, which drives cyclic electron flow (CEF), chlororespiration, and the generation of an H⁺ gradient across the thylakoid membranes. N deprivation elicited a doubling of the rate of NDA2-dependent CEF, with little contribution from PGR5/PGRL1-dependent CEF. The H⁺ gradient generated by CEF is essential to sustain nonphotochemical quenching, while an increase in the level of reduced plastoquinone would promote a state transition; both are necessary to down-regulate photosystem II activity. Moreover, stimulation of NDA2-dependent chlororespiration affords additional relief from the elevated reduction state associated with N deprivation through plastid terminal oxidase-dependent water synthesis. Overall, rerouting electrons through the NDA2 catalytic hub in response to photoautotrophic N deprivation sustains cell viability while promoting the dissipation of excess excitation energy through quenching and chlororespiratory processes.Oxygenic photosynthesis involves the conversion of light energy into chemical bond energy by plants, green algae, and cyanobacteria and the use of that energy to fix CO₂. The photosynthetic electron transport system, located in thylakoid membranes, involves several major protein complexes: PSII (water-plastoquinone oxidoreductase), cytochrome b₆f (cyt b6f; plastoquinone-plastocyanin oxidoreductase), PSI (plastocyanin-ferredoxin oxidoreductase), and the ATP synthase (CF_oCF₁). Light energy absorbed by the photosynthetic apparatus is used to establish both linear electron flow (LEF) and cyclic electron flow (CEF), which drive the production of ATP and NADPH, the chemical products of the light reactions needed for CO₂ fixation in the Calvin-Benson-Bassham (CBB) cycle.With the absorption of light energy by pigment-protein complexes associated with PSII, energy is funneled into unique chlorophyll (Chl) molecules located in the PSII reaction center (RC), where it can elicit a charge separation that generates a large enough oxidizing potential to extract electrons from water. In LEF, electrons from PSII RCs are transferred sequentially along a set of electron carriers, initially reducing the plastoquinone (PQ) pool, then the cyt b₆f complex, and subsequently the lumenal electron carrier plastocyanin (PC). Light energy absorbed by PSI excites a special pair of Chl molecules (P700), causing a charge separation that generates the most negative redox potential in nature (Nelson and Yocum, 2006). The energized electron, which is replaced by electrons from PC, is sequentially transferred to ferredoxin and ferredoxin NADP⁺ reductase, generating reductant in the form of NADPH.Electron transport from water to NADPH in LEF is accompanied by the transport of H⁺ into the thylakoid lumen. For each water molecule oxidized, two H⁺ are released in the thylakoid lumen. In addition, H⁺ are moved into the lumen by the transfer of electrons through cyt b₆f (Q cycle). H⁺ accumulation in the thylakoid lumen dramatically alters the lumenal pH, and the transmembrane H⁺ gradient (ΔpH) together with the transmembrane ion gradient constitute the proton motive force (pmf), which drives ATP formation by ATP synthase (Mitchell, 1961, 1966, 2011). This pmf also promotes other cellular processes, including the dissipation of excess absorbed excitation energy as heat in a photoprotective process (see below; Li et al., 2009; Erickson et al., 2015). The NADPH and ATP molecules generated by LEF and CEF fuel the synthesis of reduced carbon backbones (in the CBB cycle) used in the production of many cellular metabolites and fixed carbon storage polymers.A basic role for CEF is to increase the ATP-NADPH ratio, which can satisfy the energy requirements of the cell and augment the synthesis of ATP by LEF, which is required to sustain CO₂ fixation by the CBB cycle (Allen, 2003; Kramer et al., 2004; Iwai et al., 2010; Alric, 2014). There are two distinct CEF pathways identified in plants and algae. In both pathways, electrons flow from the PQ pool through cyt b₆f to reduce the oxidized form of P700 (P700⁺). In one CEF pathway, electrons are transferred back to the PQ pool prior to the formation of NADPH. This route involves the proteins PGR5 and PGRL1 (DalCorso et al., 2008; Tolleter et al., 2011; Hertle et al., 2013) and is termed PGR5/L1-dependent CEF. A second route for CEF includes an NADPH dehydrogenase that oxidizes NADPH (product of LEF) to NADP⁺, simultaneously reducing the PQ (Allen, 2003; Kramer et al., 2004; Rumeau et al., 2007). The reduced PQ pool is then oxidized by cyt b₆f, causing H⁺ translocation into the thylakoid lumen, followed by the transfer of electrons to P700⁺ via PC. In the green alga Chlamydomonas reinhardtii, this second route for CEF involves a type II NADPH dehydrogenase (NDA2; Jans et al., 2008; Desplats et al., 2009).Oxygenic photosynthetic organisms have inhabited the planet for approximately 3 billion years and have developed numerous strategies to acclimate to environmental fluctuations. These acclimation processes confer flexibility to the photosynthetic machinery, allowing it to adjust to changes in conditions that impact the metabolic/energetic state of the organism and, most importantly, the formation of reactive oxygen species that may damage the photosynthetic apparatus and other cellular components (Li et al., 2009). Several ways in which the photosynthetic apparatus adjusts to environmental fluctuations have been established. A well-studied acclimation process, nonphotochemical quenching (NPQ), reduces the excitation pressure on PSII when oxidized downstream electron acceptors are not available (Eberhard et al., 2008; Li et al., 2009; Erickson et al., 2015). Several processes constitute NPQ, as follows. (1) qT, which involves the physical movement of light-harvesting complexes (LHCs) from one photosystem to another (this is also designated state transitions; Rochaix, 2014). (2) qE, which involves thermal dissipation of the excitation energy. This energy-dependent process requires an elevated ΔpH and involves an LHC-like protein, LHCSR3 (in C. reinhardtii) or PSBS (in plants), as well as the accumulation of specific xanthophylls (mainly lutein in C. reinhardtii and zeaxanthin in plants; Niyogi et al., 1997b; Li et al., 2000, 2004; Peers et al., 2009). (3) qZ, which is energy independent and involves the accumulation of zeaxanthin (Dall’Osto et al., 2005; Nilkens et al., 2010). (4) qI, which promotes quenching following physical damage to PSII core subunits (Aro et al., 1993). Additional mechanisms that can impact LEF and CEF are the synthesis and degradation of pigment molecules, changes in levels of RC and antenna complexes, and the control of electron distribution between LEF and CEF as the energetic demands of the cell change (Allen, 2003; Kramer et al., 2004). In addition, electrons can be consumed by mitochondrial and chlororespiratory activities (Bennoun, 1982; Peltier and Cournac, 2002; Johnson et al., 2014; Bailleul et al., 2015). The latter mainly involves the plastid terminal oxidase PTOX2, which catalyzes the oxidation of the PQ pool and the reduction of oxygen and H⁺ to form water molecules (Houille-Vernes et al., 2011; Nawrocki et al., 2015).Photosynthetic processes also must be modulated as organisms experience changes in the levels of available nutrients (Grossman and Takahashi, 2001). The macronutrient nitrogen (N), which represents 3% to 5% of the dry weight of photosynthetic organisms, is required to synthesize many biological molecules (e.g. amino acids, nucleic acids, and various metabolites) and also participates in posttranslational modifications of proteins (e.g. S-nitrosylation; Romero-Puertas et al., 2013). Importantly, N is highly abundant in chloroplasts in the form of DNA, ribosomes, Chl, and polypeptides (e.g. Rubisco and LHCs; Evans, 1989; Raven, 2013). Furthermore, there is a strong integration between N and carbon assimilation. During N limitation under photoautotrophic conditions, the inability of the organism to synthesize amino acids and other N-containing molecules necessary for cell growth and division can feed back to inhibit both carbon fixation by the CBB cycle and electron transport processes and also can negatively impact the expression of genes encoding key CBB cycle enzymes (Terashima and Evans, 1988; Huppe and Turpin, 1994; Nunes-Nesi et al., 2010).C. reinhardtii is a well-established model organism in which to study photosynthesis and acclimation processes, including acclimation to nutrient limitation (Wykoff et al., 1998; Grossman and Takahashi, 2001; Moseley et al., 2006; Grossman et al., 2009; Terauchi et al., 2010; Aksoy et al., 2013). This unicellular alga grows rapidly as a photoheterotroph (on fixed carbon in the light) or as a heterotroph (on fixed carbon in the dark), has completely sequenced nuclear, chloroplast, and mitochondrial genomes, can be used for classical genetic analyses, and is haploid, which makes some aspects of molecular manipulation (e.g. the generation of knockout mutants) easier (Merchant et al., 2007; Blaby et al., 2014). In the past few years, there have been many studies on the ways in which C. reinhardtii responds to N deprivation (Bulté and Wollman, 1992; Blaby et al., 2013; Goodenough et al., 2014; Schmollinger et al., 2014; Wei et al., 2015; Juergens et al., 2015). Cells deprived of N under photoheterotrophic conditions (i.e. acetate as an external carbon source) minimize the use of N (referred to as N sparing) and induce mechanisms associated with scavenging N from both external and internal pools, all of which eventually lead to proteome modifications and an elevated carbon-N ratio (Schmollinger et al., 2014). Acclimation under photoheterotrophic conditions also causes dramatic modifications of cellular metabolism and energetics: photosynthesis is down-regulated at multiple levels, with a portion of its N content recycled (mainly Chl and polypeptides of the photosynthetic apparatus), while there is enhanced accumulation of mitochondrial complexes leading to increased respiratory activity (Schmollinger et al., 2014; Juergens et al., 2015). Additionally, while fixed carbon cannot be used for growth in the absence of N, it may be stored as starch and triacylglycerol (Work et al., 2010; Siaut et al., 2011; Davey et al., 2014; Goodenough et al., 2014).In contrast to the acclimation of photoheterotrophically grown C. reinhardtii to N deprivation, little is known about how the photosynthetic machinery in this alga adjusts in response to N deprivation under photoautotrophic conditions, when the cells absolutely require photosynthetic energy generation for maintenance. Specifically, we sought to understand how photosynthesis adjusts to metabolic restrictions that slow down the CBB cycle, which in turn could cause the accumulation of photoreductant, particularly NADPH, as the demand for electrons declines (Peltier and Schmidt, 1991; Rumeau et al., 2007). Based on analyses of mutants and the use of spectroscopic and fluorescence measurements, we established a critical role for NDA2 in the acclimation of C. reinhardtii to N deprivation under photoautotrophic conditions, including (1) an augmented capacity for alternative routes of electron utilization (which decrease the NADPH-NADP⁺ ratio) based on increased NDA2-dependent CEF and chlororespiration, and (2) elevated qE, which relies on the H⁺ gradient generated by NDA2-dependent CEF.     

The Use of Contact Mode Atomic Force Microscopy in Aqueous Medium for Structural Analysis of Spinach Photosynthetic Complexes

To investigate the dynamics of photosynthetic pigment-protein complexes in vascular plants at high resolution in an aqueous environment, membrane-protruding oxygen-evolving complexes (OECs) associated with photosystem II (PSII) on spinach (Spinacia oleracea) grana membranes were examined using contact mode atomic force microscopy. This study represents, to our knowledge, the first use of atomic force microscopy to distinguish the putative large extrinsic loop of Photosystem II CP47 reaction center protein (CP47) from the putative oxygen-evolving enhancer proteins 1, 2, and 3 (PsbO, PsbP, and PsbQ) and large extrinsic loop of Photosystem II CP43 reaction center protein (CP43) in the PSII-OEC extrinsic domains of grana membranes under conditions resulting in the disordered arrangement of PSII-OEC particles. Moreover, we observed uncharacterized membrane particles that, based on their physical characteristics and electrophoretic analysis of the polypeptides associated with the grana samples, are hypothesized to be a domain of photosystem I that protrudes from the stromal face of single thylakoid bilayers. Our results are interpreted in the context of the results of others that were obtained using cryo-electron microscopy (and single particle analysis), negative staining and freeze-fracture electron microscopy, as well as previous atomic force microscopy studies.Oxygenic photosynthesis supports most life on Earth through the absorption of solar energy, which powers the extraction of electrons from water and the subsequent use of those electrons to convert CO₂ into organic compounds (Nelson and Ben-Shem, 2004; Merchant and Sawaya, 2005; Nelson, 2011). The light-dependent reactions of photosynthesis occur within photosynthetic or thylakoid membranes and are catalyzed by two reaction centers, PSI and PSII. Both photosystems have associated light-harvesting complexes (LHCI and LHCII) that act as antenna to efficiently capture light energy. The oxygen-evolving complex (OEC) is an integral component of PSII, catalyzing the extraction of electrons from water. The two photosystems are connected through an intersystem electron transport chain that includes the hydrophobic electron carrier plastoquinone, the membrane-bound cytochrome b₆f complex (cyt b₆f), and the mobile electron carrier plastocyanin. The electrochemical gradient generated during light-driven electron flow is used in the synthesis of ATP by the ATP synthase complex. Components of the photosynthetic apparatus vary among photosynthetic organisms and under different environmental conditions, especially for proteins associated with light-harvesting complexes (Liu and Scheuring, 2013). However, investigations of the mechanisms associated with the dynamic acclimation of photosynthetic electron transport and light harvesting to environmental cues require real-time observations that are difficult to achieve because of limitations in our ability to view such changes (e.g. difficulties in tagging proteins with fluorophores and resolving fluorescent images; Zaks et al., 2013).In vascular plants, thylakoid membranes form a network of interconnected tubular structures enclosing a lumenal space. This membrane system can be divided into two morphologically distinct regions: the grana, which are formed by stacks of appressed membranes; and the stroma lamellae, which are unappressed membranes that form connections between grana stacks. These distinct thylakoid regions are enriched for specific photosynthetic complexes. The major complexes in grana are PSII and LHCII, which can interact and form a variety of PSII-LHCII supercomplexes (Dekker and Boekema, 2005; Kouřil et al., 2012), as well as cyt b₆f (Johnson et al., 2014). Grana stacks are also the site of water oxidation and oxygen evolution; the Mn₄CaO₅ cluster is the PSII cofactor that catalyzes this process (Umena et al., 2011). This cluster resides between the transmembrane subunits of the PSII core (formed by PSII proteins D1 and D2 and their associated pigment cofactors, with PSII reaction center proteins CP43 and CP47, α- and β-subunits of cytochrome b559, and PSII reaction center protein I [PsbI]) and the lumenal, peripheral membrane proteins of the OEC. The OEC is composed of extrinsic membrane polypeptides of 33 kD, 23 kD, and 17 kD, designated oxygen-evolving enhancer protein 1, 2, and 3 (PsbO, PsbP, and PsbQ) that protrude into the thylakoid lumen in vascular and nonvascular plants as well as in green algae. Cyanobacteria also have PsbO, with PsbV and PsbU serving as functional analogs of plant PsbP and PsbQ, respectively (Dekker and Boekema, 2005). Based on removal/reconstitution experiments, these subunits have been shown to be critical for PSII stability and oxygen evolution activity (Kuwabara and Murata, 1983; Ljungberg et al., 1983; Ghanotakis et al., 1984). They may also impact the association of Ca²⁺ and Cl⁻ with PSII, the polypeptide conformation around the manganese cluster, and the formation of channels within PSII that allow access of water to the catalytic site and the exit of protons from the complex as water is oxidized (Bricker et al., 2012).The x-ray crystal structures of purified PsbP (Kohoutová et al., 2009) and PsbQ (Balsera et al., 2005) from spinach (Spinacia oleracea) have been determined. For cyanobacteria, PSII crystals have been used to establish high-resolution structures for PsbO, PsbV, and PsbU (Umena et al., 2011), with more recent analyses at room temperature (Kern et al., 2013). To study the bound state of these peripheral proteins in spinach, electron density maps were established based on cryo-electron microscopy (cryo-EM) and single particle analysis of purified PSII-LHCII supercomplexes, with structural verification based on the removal of extrinsic polypeptides of the complexes from the membranes (Nield et al., 2002). In these structures, determined at less than 2 nm (or 20 Å) resolution, the PsbP and PsbQ subunits of OEC were assigned to a single membrane protrusion, with a second membrane protrusion assigned to PsbO (Boekema et al., 2000a); these topological structures are the most prominent protruding features of the reaction center-containing membrane protein complexes. Since two PSII reaction centers associate to form a dimeric PSII-LHCII supercomplex (Bumba and Vácha, 2003), the six OEC subunits (two PsbO, two PsbP, and two PsbQ) are visualized as four protrusions associated with each supercomplex. However, after the cyanobacterial PSII core structure was solved (including the positions of the extrinsic subunits) and aligned to the cryo-EM of PSII-LHCII supercomplexes (Nield and Barber, 2006), the structure was reevaluated. The PSII lumenal small protruding mass was assigned to the large extrinsic loop of CP47 (encoded by psbB), while the larger protrusion was assigned to PsbO, PsbP, PsbQ, and the large extrinsic loop associated with CP43 (encoded by psbC).Attempts have been made to visualize PSII complexes and proteins in their native membrane environment using transmission electron microscopy (TEM) in conjunction with freeze fracture (Johnson et al., 2011) and negative staining of grana membranes from both spinach (Boekema et al., 2000b) and Arabidopsis (Arabidopsis thaliana; Betterle et al., 2009; Wientjes et al., 2013). These techniques provide little information regarding the extent of the protrusion of the polypeptide subunits out of the plane of the membranes. Even though cryo-electron tomography of isolated chloroplasts and plunge-frozen thylakoid membranes (Daum et al., 2010) and grana stacks (Kouřil et al., 2011) can preserve sample hydration using a vitrification process during freezing, it is difficult to determine the height of the extrinsic thylakoid protein protrusions from the membrane surface. Furthermore, at the resolution obtained with these techniques, the small and large protrusions of each PSII monomer may appear merged into a single structure. This would result in the visualization of only two distinguishable topological entities for each PSII-OEC dimer.The generation of images by atomic force microscopy (AFM), which involves raster scanning by a sharp tip that is in contact with the sample, complements other structural determination methods. The vertical position of the tip is controlled in order to maintain a constant imaging force (balancing interaction forces between the tip and the scanned structure). Control is implemented by a feedback loop that continuously monitors the force with a highly sensitive force sensor that activates a high-precision actuator. Logging the vertical position of the piezoelectric actuator that controls the vertical position of the tip can provide particle height relative to the membrane at high vertical resolution; this is done concurrently with logging the lateral position of each pixel to generate the image (Bippes and Muller, 2011). Probing samples with AFM in air has been employed to image spinach grana membranes (Kirchhoff et al., 2008) to elucidate the arrangement of Arabidopsis PSII-LHCII supercomplexes associated with nonphotochemical quenching (Onoa et al., 2014) and to determine the areal density of Arabidopsis PSII-OEC during the PSII repair cycle (Puthiyaveetil et al., 2014).Most AFM studies of grana have been performed with membrane surfaces exposed to air. This raises issues concerning the extent to which membrane properties are altered during measurements in a nonaqueous environment (Zaks et al., 2013), where it may be impossible to maintain appropriate hydration and ionic conditions. However, AFM has also been used in aqueous medium to establish high-resolution topography images of membrane proteins (Bippes and Muller, 2011) and specifically to characterize the PSII-OEC, which was previously observed as an ordered array within spinach grana membranes (Sznee et al., 2011). In recent studies, a map of the lumenal surface of grana membranes was generated in aqueous medium that distinguishes cyt b₆f dimers from PSII-OEC (Johnson et al., 2014). However, the potential of AFM imaging in a liquid environment has not been realized for the high-resolution analysis of features associated with thylakoid membranes and the PSII-OEC dimer. We used contact mode atomic force microscopy (CM-AFM) to (1) image PSII-OEC topology in liquid medium at high resolution, (2) identify other features/particles associated with grana membranes, and (3) optimize the use of AFM for monitoring the dynamics of thylakoid membrane complexes as the conditions of the environment are modulated (e.g. light, specific ions, and temperature).     

Light-Harvesting Complex Protein LHCBM9 Is Critical for Photosystem II Activity and Hydrogen Production in Chlamydomonas reinhardtii

Photosynthetic organisms developed multiple strategies for balancing light-harvesting versus intracellular energy utilization to survive ever-changing environmental conditions. The light-harvesting complex (LHC) protein family is of paramount importance for this function and can form light-harvesting pigment protein complexes. In this work, we describe detailed analyses of the photosystem II (PSII) LHC protein LHCBM9 of the microalga Chlamydomonas reinhardtii in terms of expression kinetics, localization, and function. In contrast to most LHC members described before, LHCBM9 expression was determined to be very low during standard cell cultivation but strongly increased as a response to specific stress conditions, e.g., when nutrient availability was limited. LHCBM9 was localized as part of PSII supercomplexes but was not found in association with photosystem I complexes. Knockdown cell lines with 50 to 70% reduced amounts of LHCBM9 showed reduced photosynthetic activity upon illumination and severe perturbation of hydrogen production activity. Functional analysis, performed on isolated PSII supercomplexes and recombinant LHCBM9 proteins, demonstrated that presence of LHCBM9 resulted in faster chlorophyll fluorescence decay and reduced production of singlet oxygen, indicating upgraded photoprotection. We conclude that LHCBM9 has a special role within the family of LHCII proteins and serves an important protective function during stress conditions by promoting efficient light energy dissipation and stabilizing PSII supercomplexes.     

Comparative Analysis of Light-Harvesting Antennae and State Transition in chlorina and cpSRP Mutants

State transitions in photosynthesis provide for the dynamic allocation of a mobile fraction of light-harvesting complex II (LHCII) to photosystem II (PSII) in state I and to photosystem I (PSI) in state II. In the state I-to-state II transition, LHCII is phosphorylated by STN7 and associates with PSI to favor absorption cross-section of PSI. Here, we used Arabidopsis (Arabidopsis thaliana) mutants with defects in chlorophyll (Chl) b biosynthesis or in the chloroplast signal recognition particle (cpSRP) machinery to study the flexible formation of PS-LHC supercomplexes. Intriguingly, we found that impaired Chl b biosynthesis in chlorina1-2 (ch1-2) led to preferentially stabilized LHCI rather than LHCII, while the contents of both LHCI and LHCII were equally depressed in the cpSRP43-deficient mutant (chaos). In view of recent findings on the modified state transitions in LHCI-deficient mutants (Benson et al., 2015), the ch1-2 and chaos mutants were used to assess the influence of varying LHCI/LHCII antenna size on state transitions. Under state II conditions, LHCII-PSI supercomplexes were not formed in both ch1-2 and chaos plants. LHCII phosphorylation was drastically reduced in ch1-2, and the inactivation of STN7 correlates with the lack of state transitions. In contrast, phosphorylated LHCII in chaos was observed to be exclusively associated with PSII complexes, indicating a lack of mobile LHCII in chaos. Thus, the comparative analysis of ch1-2 and chaos mutants provides new evidence for the flexible organization of LHCs and enhances our understanding of the reversible allocation of LHCII to the two photosystems.In oxygenic photosynthesis, PSII and PSI function in series to convert light energy into the chemical energy that fuels multiple metabolic processes. Most of this light energy is captured by the chlorophyll (Chl) and carotenoid pigments in the light-harvesting antenna complexes (LHCs) that are peripherally associated with the core complexes of both photosystems (Wobbe et al., 2016). However, since the two photosystems exhibit different absorption spectra (Nelson and Yocum, 2006; Nield and Barber, 2006; Qin et al., 2015), PSI or PSII is preferentially excited under naturally fluctuating light intensities and qualities. To optimize photosynthetic electron transfer, the excitation state of the two photosystems must be rebalanced in response to changes in lighting conditions. To achieve this, higher plants and green algae require rapid and precise acclimatory mechanisms to adjust the relative absorption cross-sections of the two photosystems.To date, the phenomenon of state transitions is one of the well-documented short-term acclimatory mechanisms. It allows a mobile portion of the light-harvesting antenna complex II (LHCII) to be allocated to either photosystem, depending on the spectral composition and intensity of the ambient light (Allen and Forsberg, 2001; Rochaix, 2011; Goldschmidt-Clermont and Bassi, 2015; Gollan et al., 2015). State transitions are driven by the redox state of the plastoquinone (PQ) pool (Vener et al., 1997; Zito et al., 1999). When PSI is preferentially excited (by far-red light), the PQ pool is oxidized and all the LHCII is associated with PSII. This allocation of antenna complexes is defined as state I. When light conditions (blue/red light or low light) favor exciton trapping of PSII, the transition from state I to state II occurs. The over-reduced PQ pool triggers the activation of the membrane-localized Ser-Thr kinase STN7, which phosphorylates an N-terminal Thr on each of two major LHCII proteins, LHCB1 and LHCB2 (Allen, 1992; Bellafiore et al., 2005; Shapiguzov et al., 2016). Phosphorylation of LHCII results in the dissociation of LHCII from PSII and triggers its reversible relocation to PSI (Allen, 1992; Rochaix, 2011). Conversely, when the PQ pool is reoxidized, STN7 is inactivated and the constitutively active, thylakoid-associated phosphatase TAP38/PPH1 dephosphorylates LHCII, which then reassociates with PSII (Pribil et al., 2010; Shapiguzov et al., 2010). The physiological significance of state transitions has been demonstrated by the reduction in growth rate seen in the stn7 knock-out mutant under fluctuating light conditions (Bellafiore et al., 2005; Tikkanen et al., 2010).The canonical state transitions model implies spatial and temporal regulation of the allocation of LHC between the two spatially segregated photosystems (Dekker and Boekema, 2005). PSII-LHCII supercomplexes are organized in a tightly packed form in the stacked grana regions of thylakoid membranes, while PSI-LHCI supercomplexes are mainly localized in the nonstacked stromal lamellae and grana margin regions (Dekker and Boekema, 2005; Haferkamp et al., 2010). It has been proposed that, in the grana margin regions, which harbor LHCII and both photosystems, LHCII can migrate rapidly between them (Albertsson et al., 1990; Albertsson, 2001). This idea is supported by the recent discovery of mega complexes containing both photosystems in the grana margin regions (Yokono et al., 2015). Furthermore, phosphorylation of LHCII was found to increase not only the amount of PSI found in the grana margin region of thylakoid membranes (Tikkanen et al., 2008a), but also to modulate the pattern of PSI-PSII megacomplexes under changing light conditions (Suorsa et al., 2015). Nonetheless, open questions remain in relation to the physiological significance of the detection of phosphorylated LHCII in all thylakoid regions, even under the constant light conditions (Grieco et al., 2012; Leoni et al., 2013; Wientjes et al., 2013), although LHCII phosphorylation has been shown to modify the stacking of thylakoid membranes (Chuartzman et al., 2008; Pietrzykowska et al., 2014).State I-to-state II transition is featured by the formation of LHCII-PSI-LHCI supercomplexes, in which LHCII favors the light-harvesting capacity of PSI. Recently, LHCII-PSI-LHCI supercomplexes have been successfully isolated and purified using various detergents (Galka et al., 2012; Drop et al., 2014; Crepin and Caffarri, 2015) or a styrene-maleic acid copolymer (Bell et al., 2015). These findings yielded further insights into the reorganization of supercomplexes associated with state transitions, and it was suggested that phosphorylation of LHCB2 rather than LHCB1 is the essential trigger for the formation of state transition supercomplexes (Leoni et al., 2013; Pietrzykowska et al., 2014; Crepin and Caffarri, 2015; Longoni et al., 2015). Furthermore, characterization of mutants deficient in individual PSI core subunits indicates that PsaH, L, and I are required for docking of LHCII at PSI (Lunde et al., 2000; Zhang and Scheller, 2004; Kouril et al., 2005; Plöchinger et al., 2016).Recently, the state transition capacity has been characterized in the Arabidopsis (Arabidopsis thaliana) mutants with missing LHCI components. Although the Arabidopsis knock-out mutants lacking one of the four LHCI proteins (LHCA1-4) showed enhanced accumulation of LHCII-PSI complexes, the absorption cross-section of PSI under state II conditions was still compromised in the lhca1-4 mutants, and it is suggested that LHCI mediates the detergent-sensitive interaction between ‘extra LHCII’ and PSI (Benson et al., 2015; Grieco et al., 2015). Furthermore, the Arabidopsis mutant ΔLhca lacking all LHCA1-4 proteins was shown to be compensated for the deficiency of LHCI by binding LHCII under state II conditions (Bressan et al., 2016). In spite of this finding, the significant reduction in the absorption cross-section of PSI was still observed in the ΔLhca mutant, suggesting a substantial role of LHCI in light absorption under canopy conditions (Bressan et al., 2016). However, these findings emphasize the acclimatory function of state transitions in balancing light absorption capacity between the two photosystems by modifying their relative antenna size and imply the dynamic and variable organization of PS-LHC supercomplexes.LHC proteins are encoded by the nuclear Lhc superfamily (Jansson, 1994). The biogenesis of LHCs includes the cytoplasmic synthesis of the LHC precursor proteins, their translocation into chloroplasts via the TOC/TIC complex, and their posttranslational targeting and integration into the thylakoid membranes by means of the chloroplast signal recognition particle (cpSRP) machinery (Jarvis and Lopez-Juez, 2013). The posttranslational cpSRP-dependent pathway for the final translocation of LHC proteins into the thylakoid membrane includes interaction of cpSRP43 with LHC apo-proteins and recruitment of cpSRP54 to form a transit complex. Then binding of this tripartite cpSRP transit complex to the SRP receptor cpFtsY follows, which supports docking of the transit complex to thylakoid membranes and its association with the LHC translocase ALB3. Ultimately, ALB3 inserts LHC apo-proteins into the thylakoid membrane (Richter et al., 2010). Importantly, stoichiometric amounts of newly synthesized Chl a and Chl b as well as carotenoid are inserted into the LHC apo-proteins by unknown mechanisms to form the functional LHCs that associate with the core complexes of both photosystems in the thylakoid membranes (Dall’Osto et al., 2015; Wang and Grimm, 2015).The first committed steps in Chl synthesis occur in the Mg branch of the tetrapyrrole biosynthesis pathway. 5-Aminolevulinic acid synthesis provides the precursor for the formation of protoporphyrin IX, which is directed into the Mg branch (Tanaka and Tanaka, 2007; Brzezowski et al., 2015). Chl synthesis ends with the conversion of Chl a to Chl b catalyzed by Chl a oxygenase (CAO; Tanaka et al., 1998; Tomitani et al., 1999). It has been hypothesized that coordination between Chl synthesis and the posttranslational cpSRP pathway is a prerequisite for the efficient integration of Chls into LHC apo-proteins.In this study, we intend to characterize the assembly of LHCs when the availability of Chl molecules or the integration of LHC apo-proteins into thylakoid membranes is limiting. To this end, we compared the assembly of LHCs and the organization of PS-LHC complexes in two different sets of Arabidopsis mutants. Firstly, we used the chlorina1-2 (ch1-2) mutant, which is defective in the CAO gene. The members of the second set of mutants carry knock-out mutations in genes involved in the chloroplast SRP pathway (Richter et al., 2010).Our studies revealed distinct accumulation of PS-LHC supercomplexes between the two sets of mutant relative to wild-type plants. In spite of the defect in synthesis of Chl b, ch1-2 retains predominantly intact PSI-LHCI supercomplexes but has strongly reduced amounts of LHCII. In contrast, the chaos (cpSRP43) mutant exhibits synchronously reduced contents of both LHCI and LHCII, which results in the accumulation of PS core complexes without accompanying LHCs. Thus, the distribution of LHCs in the thylakoid membranes of the two mutants, ch1-2 and chaos, were explored under varying light conditions with the aim of elucidating the influence of modified LHCI/LHCII antenna size on state transitions. Our results contribute to an expanding view on the variety of photosynthetic complexes, which can be observed in Arabidopsis plants with specified mutations in LHC biogenesis.     

The Actin-Related Protein2/3 Complex Regulates Mitochondrial-Associated Calcium Signaling during Salt Stress in Arabidopsis

Microfilament and Ca²⁺ dynamics play important roles in stress signaling in plants. Through genetic screening of Arabidopsis thaliana mutants that are defective in stress-induced increases in cytosolic Ca²⁺ ([Ca2+]_cyt), we identified Actin-Related Protein2 (Arp2) as a regulator of [Ca2+]_cyt in response to salt stress. Plants lacking Arp2 or other proteins in the Arp2/3 complex exhibited enhanced salt-induced increases in [Ca2+]_cyt, decreased mitochondria movement, and hypersensitivity to salt. In addition, mitochondria aggregated, the mitochondrial permeability transition pore opened, and mitochondrial membrane potential Ψm was impaired in the arp2 mutant, and these changes were associated with salt-induced cell death. When opening of the enhanced mitochondrial permeability transition pore was blocked or increases in [Ca2+]_cyt were prevented, the salt-sensitive phenotype of the arp2 mutant was partially rescued. These results indicate that the Arp2/3 complex regulates mitochondrial-dependent Ca²⁺ signaling in response to salt stress.     

Proton Gradient Regulation5-Like1-Mediated Cyclic Electron Flow Is Crucial for Acclimation to Anoxia and Complementary to Nonphotochemical Quenching in Stress Adaptation

To investigate the functional importance of Proton Gradient Regulation5-Like1 (PGRL1) for photosynthetic performances in the moss Physcomitrella patens, we generated a pgrl1 knockout mutant. Functional analysis revealed diminished nonphotochemical quenching (NPQ) as well as decreased capacity for cyclic electron flow (CEF) in pgrl1. Under anoxia, where CEF is induced, quantitative proteomics evidenced severe down-regulation of photosystems but up-regulation of the chloroplast NADH dehydrogenase complex, plastocyanin, and Ca²⁺ sensors in the mutant, indicating that the absence of PGRL1 triggered a mechanism compensatory for diminished CEF. On the other hand, proteins required for NPQ, such as light-harvesting complex stress-related protein1 (LHCSR1), violaxanthin de-epoxidase, and PSII subunit S, remained stable. To further investigate the interrelation between CEF and NPQ, we generated a pgrl1 npq4 double mutant in the green alga Chlamydomonas reinhardtii lacking both PGRL1 and LHCSR3 expression. Phenotypic comparative analyses of this double mutant, together with the single knockout strains and with the P. patens pgrl1, demonstrated that PGRL1 is crucial for acclimation to high light and anoxia in both organisms. Moreover, the data generated for the C. reinhardtii double mutant clearly showed a complementary role of PGRL1 and LHCSR3 in managing high light stress response. We conclude that both proteins are needed for photoprotection and for survival under low oxygen, underpinning a tight link between CEF and NPQ in oxygenic photosynthesis. Given the complementarity of the energy-dependent component of NPQ (qE) and PGRL1-mediated CEF, we suggest that PGRL1 is a capacitor linked to the evolution of the PSII subunit S-dependent qE in terrestrial plants.The conversion of solar energy into chemical energy and building material by oxygenic photosynthesis, as performed by plants, green algae, and cyanobacteria, supports much of the life on our planet. The production of oxygen and the assimilation of carbon dioxide into organic matter determines, to a large extent, the composition of our atmosphere. Plant photosynthesis is achieved thanks to a series of reactions that occur mainly in the chloroplast, resulting in light-dependent water oxidation, NADP⁺ reduction, and ATP formation (Whatley et al., 1963). Two separate photosystems (PSI and PSII) and an ATP synthase (ATPase) embedded in the thylakoid membrane catalyze these reactions. The ATPase produces ATP at the expense of the proton motive force that is generated by the light reactions (Mitchell, 1961). The cytochrome (cyt) b₆f complex assures the link between the two photosystems by transferring electrons from the membrane-bound plastoquinone to a soluble carrier, plastocyanin, or cyt c₆ and functions in the pumping of protons. NADPH and ATP that are produced by linear electron flow from PSII to PSI are fueled into the Calvin Benson Bassham cycle (Bassham et al., 1950) to fix CO₂. In parallel, cyclic electron flow (CEF) between the cyt b₆f complex and PSI may occur, which would solely lead to the production of ATP. CEF around PSI has been first recognized by Arnon (1959) and is involved in the reequilibration of the ATP poise and prevention of overreduction of the PSI acceptor side (Alric, 2010; Peltier et al., 2010; Leister and Shikanai, 2013; Shikanai, 2014). In microalgae and vascular plants, CEF operates via an NAD(P)H dehydrogenase-like complex (NDH)-dependent and/or PROTON GRADIENT REGULATION5 (PGR5)-related pathway (Alric, 2010; Peltier et al., 2010; Leister and Shikanai, 2013; Shikanai, 2014). The thylakoid protein Proton Gradient Regulation5-Like1 (PGRL1; DalCorso et al., 2008) has been first discovered as a novel component for the PGR5-dependent CEF pathway in Arabidopsis (Arabidopsis thaliana), as its knockout causes a PGR5-like photosynthetic phenotype and is suggested to operate as a ferredoxin-plastoquinone reductase (Hertle et al., 2013). PGRL1 is also important for efficient CEF in the green alga Chlamydomonas reinhardtii, which becomes particularly evident under settings where CEF is induced, such as in acclimation to iron deficiency, high light (HL), or anaerobic growth conditions (Petroutsos et al., 2009; Iwai et al., 2010; Tolleter et al., 2011; Terashima et al., 2012). Remarkably, a CEF protein supercomplex composed of PSI-light-harvesting complex I (LHCI), LHCII, the cyt b₆f complex, ferredoxin-NADPH oxidoreductase, and PGRL1 was isolated from state 2 conditions (Iwai et al., 2010). Under anaerobic conditions, the Ca²⁺ sensor CAS and Anaerobic response1 (ANR1) were shown to interact with PGRL1 in vivo (Terashima et al., 2012) and were found to be associated with the C. reinhardtii CEF supercomplex. Consistently, depletion of CAS and ANR1 by artificial microRNA expression in C. reinhardtii resulted in strong inhibition of CEF under anoxia, which could be partially rescued by an increase in the extracellular Ca²⁺ concentration, inferring that CEF is Ca²⁺ dependent (Terashima et al., 2012). Notably, the regulation of the proton motive force by a two-pore potassium channel in the thylakoid membrane of Arabidopsis (AtTPK3), is also Ca²⁺ dependent (Carraretto et al., 2013), suggesting that Ca²⁺-dependent activation of CEF and the channel may work hand in hand.qE, the energy-dependent component of nonphotochemical quenching (NPQ) that occurs due to thermal dissipation of excess absorbed light energy (Li et al., 2000; Peers et al., 2009), is dependent on rapid luminal acidification upon photosynthetic electron transfer (Wraight and Crofts, 1970; Li et al., 2000). Thus, processes such as CEF that contribute to the pH gradient across the thylakoid membrane are interrelated to NPQ, as an acidified lumen is required for efficient qE (Joliot and Finazzi, 2010). In vascular plants, PSII subunit S (PSBS) is essential for efficient qE (Li et al., 2000), whereas qE induction in the green alga C. reinhardtii is mediated by light-harvesting complex stress-related protein3 (LHCSR3), an ancient light-harvesting protein that is missing in vascular plants (Peers et al., 2009). The moss Physcomitrella patens, which possesses genes encoding for PSBS and LHCSR proteins, utilizes both types of regulatory proteins to operate qE (Alboresi et al., 2010), suggesting that land plants evolved a novel PSBS-dependent qE mechanism before losing the ancestral LHCSR-dependent qE found in algae. This makes mosses a very interesting subject for investigating the interrelation and evolution of the CEF and NPQ molecular effectors.Mosses diverged from vascular plants early after land colonization and are one of the oldest groups of land plants present on earth. This places the moss model system P. patens (Rensing et al., 2008) evolutionarily in the middle between algae and vascular plants and makes it an ideal model organism for the study of the evolution of photosynthetic organisms. Analysis of photosynthesis in P. patens can provide insights into the events leading to adaptation to the harsher physicochemical conditions of the terrestrial environment (Rensing et al., 2008), as evidenced by the presence and functional overlap of LHCSRs and PSBS (Alboresi et al., 2010).To obtain insights into the interrelation and evolution of CEF and NPQ, we knocked out the PGRL1 gene from P. patens and analyzed functional phenotypic consequences. Moreover, we compared these phenotypes with phenotypic analyses of C. reinhardtii pgrl1, npq4, and pgrl1 npq4 single and double mutants lacking PGRL1, LHCSR3, and both PGRL1 and LHCSR3, respectively. The data provided strong evidence that the green cut protein PGRL1 (Karpowicz et al., 2011) is required for acclimation to anoxia both in algae and mosses. Moreover, an involvement of PGRL1 in the evolution of PSBS-dependent qE in terrestrial plants is implied.     

Knocking Down of Isoprene Emission Modifies the Lipid Matrix of Thylakoid Membranes and Influences the Chloroplast Ultrastructure in Poplar

Isoprene is a small lipophilic molecule with important functions in plant protection against abiotic stresses. Here, we studied the lipid composition of thylakoid membranes and chloroplast ultrastructure in isoprene-emitting (IE) and nonisoprene-emitting (NE) poplar (Populus × canescens). We demonstrated that the total amount of monogalactosyldiacylglycerols, digalactosyldiacylglycerols, phospholipids, and fatty acids is reduced in chloroplasts when isoprene biosynthesis is blocked. A significantly lower amount of unsaturated fatty acids, particularly linolenic acid in NE chloroplasts, was associated with the reduced fluidity of thylakoid membranes, which in turn negatively affects photosystem II photochemical efficiency. The low photosystem II photochemical efficiency in NE plants was negatively correlated with nonphotochemical quenching and the energy-dependent component of nonphotochemical quenching. Transmission electron microscopy revealed alterations in the chloroplast ultrastructure in NE compared with IE plants. NE chloroplasts were more rounded and contained fewer grana stacks and longer stroma thylakoids, more plastoglobules, and larger associative zones between chloroplasts and mitochondria. These results strongly support the idea that in IE species, the function of this molecule is closely associated with the structural organization and functioning of plastidic membranes.Isoprene is globally the most abundant biogenic hydrocarbon constitutively emitted from many plant species (Guenther et al., 2012). It has been proposed that leaf isoprene emission is an important adaptation for plants, conferring tolerance to different environmental constraints (Vickers et al., 2009; Loreto and Schnitzler, 2010; Loreto and Fineschi, 2014). However, biogenic isoprene emission represents a nontrivial carbon loss in plants, particularly under stress conditions (Fang et al., 1996; Brilli et al., 2007; Teuber et al., 2008; Ghirardo et al., 2014), and the reason(s) why plants emit isoprene are still ambiguous, and the true role of isoprene emission remains elusive. Different approaches and techniques have been used to determine whether and how the cost of this expensive carbon emission is matched by the accomplishment of the physiological function in planta. It has been shown that isoprene might quench and/or regulate reactive oxygen and nitrogen species formation (Behnke et al., 2010a; Velikova et al., 2012), thereby indirectly providing a general antioxidant action (for review, see Vickers et al., 2009; Loreto and Schnitzler, 2010) and stabilizing thylakoid membrane structures due to the lipophilic properties of this molecule (Sharkey et al., 2001; Velikova et al., 2011).Protein and pigment-protein complexes are assembled and embedded in a lipid matrix, which has a unique lipid composition. The thylakoid lipid bilayer of chloroplasts is characterized by a high proportion of galactolipids with one (monogalactosyldiacylglycerol [MGDG]) or two (digalactosyldiacylglycerol [DGDG]) Gal molecules (Joyard et al., 2010). MGDGs are the primary constituents (approximately 50%) of thylakoid membrane glycerolipids, followed by DGDGs (approximately 30%), sulfoquinovosyldiacylglycerol (approximately 5%–12%), and phosphatidylglycerol (approximately 5%–12%; Kirchhoff et al., 2002). Galactolipids contain a large proportion of polyunsaturated fatty acids, and consequently, the thylakoid membrane is a relatively fluid system (Gounaris and Barber, 1983) compared with other biological membranes. The fluidity of the thylakoid membrane is essential for photosynthetic processes.The thylakoid membranes are highly organized internal membrane chloroplast systems that conduct the light reactions of photosynthesis. These membranes comprise pigments and proteins organized in complexes. Thylakoid membranes are arranged into stacked and unstacked regions called grana and stroma thylakoids, respectively, differentially enriched in PSI and PSII complexes (Mustárdy et al., 2008). The spatial separation of the PSI and PSII complexes in the stacked and unstacked membrane regions and the macromolecular organization of PSII in stacked grana thylakoids are self-organizing processes and important features to maintain the functional integrity of the photosynthetic apparatus (Kirchhoff et al., 2007).It is not known how changes in the lipid matrix affect lipid-protein interactions and vice versa, and how membrane macroorganization ensures the efficient diffusion of protein complexes associated with plant adaptation to the changing environment remains elusive. The isoprene impact on thylakoid intactness and functionality has been assessed using different biophysical techniques (Velikova et al., 2011). Thermoluminescence data demonstrated that the position of the main peak (Qb peak; Sane, 2004) was upshifted approximately 10° in isoprene-emitting (IE) plants, suggesting modifications in the lipid environment due to the presence of isoprene in heterologous Arabidopsis (Arabidopsis thaliana) plants expressing the isoprene synthase gene from poplar (Populus spp.). It was also shown that isoprene improves the stability of PSII light-harvesting complex II (LHCII) through the modification of pigment-protein complex organization in thylakoid membranes (Velikova et al., 2011). Moreover, we recently showed that knocking down isoprene emission in poplar remodels the chloroplast proteome (Velikova et al., 2014). The lack of isoprene resulted in the down-regulation of proteins associated with the light reactions of photosynthesis, redox regulation, and oxidative stress defenses and several proteins responsible for lipid metabolism (Velikova et al., 2014).In this study, we focused on the lipid composition of thylakoid membranes in IE and nonisoprene-emitting (NE) poplar (Populus × canescens) leaves. Specifically, we determined whether the translational suppression of isoprene synthase in NE leaves influences the lipid matrix of thylakoids and how this phenomenon affects membrane structure and function. Here, we provide evidence that the suppression of isoprene biosynthesis in poplar (1) reduced total galactolipids, phospholipids (PLs), and linolenic fatty acid (18:3), (2) altered the chloroplast ultrastructure, and (3) stimulated photoprotective mechanisms.     

Thioredoxin m4 Controls Photosynthetic Alternative Electron Pathways in Arabidopsis

In addition to the linear electron flow, a cyclic electron flow (CEF) around photosystem I occurs in chloroplasts. In CEF, electrons flow back from the donor site of photosystem I to the plastoquinone pool via two main routes: one that involves the Proton Gradient Regulation5 (PGR5)/PGRL1 complex (PGR) and one that is dependent of the NADH dehydrogenase-like complex. While the importance of CEF in photosynthesis and photoprotection has been clearly established, little is known about its regulation. We worked on the assumption of a redox regulation and surveyed the putative role of chloroplastic thioredoxins (TRX). Using Arabidopsis (Arabidopsis thaliana) mutants lacking different TRX isoforms, we demonstrated in vivo that TRXm4 specifically plays a role in the down-regulation of the NADH dehydrogenase-like complex-dependent plastoquinone reduction pathway. This result was confirmed in tobacco (Nicotiana tabacum) plants overexpressing the TRXm4 orthologous gene. In vitro assays performed with isolated chloroplasts and purified TRXm4 indicated that TRXm4 negatively controls the PGR pathway as well. The physiological significance of this regulation was investigated under steady-state photosynthesis and in the pgr5 mutant background. Lack of TRXm4 reversed the growth phenotype of the pgr5 mutant, but it did not compensate for the impaired photosynthesis and photoinhibition sensitivity. This suggests that the physiological role of TRXm4 occurs in vivo via a mechanism distinct from direct up-regulation of CEF.In plant thylakoids, photosynthesis involves a linear electron flow (LEF) from water to NADP⁺ via PSII, cytochrome b₆/f, PSI, and soluble carriers. LEF produces NADPH and generates a transthylakoidal electrochemical proton gradient that drives the synthesis of ATP. Besides LEF, cyclic electron flow (CEF) can also occur, involving only PSI (for review, see Johnson, 2011; Kramer and Evans, 2011). These additional reactions include two main distinct pathways involving either the Proton Gradient Regulation5 (PGR5)/PGRL1 complex (Munekage et al., 2002; DalCorso et al., 2008) or the NADH dehydrogenase-like complex (NDH; for review, see Battchikova et al., 2011; Ifuku et al., 2011). The functioning of either CEF pathway, which generates a pH gradient ΔpH without any accumulation of NADPH, is thought to achieve the appropriate ATP/NADPH balance required for the biochemical needs of the plant, especially under certain environmental conditions such as low CO₂ (Golding and Johnson, 2003), heat (Clarke and Johnson, 2001), cold (Clarke and Johnson, 2001), drought (Golding and Johnson, 2003; Kohzuma et al., 2009), high light (Munekage et al., 2004), or dark-to-light transitions (Joliot and Joliot, 2005; Fan et al., 2007). CEF-generated ΔpH is also involved in photoprotection owing to the down-regulation of PSII via nonphotochemical quenching (Munekage et al., 2004; Takahashi et al., 2009). Very recently, the role of the PGR5 protein as a regulator of LEF has been established. It has proved to be essential in the protection of PSI from photodamage (Suorsa et al., 2012).The two cyclic pathways are redundant (Munekage et al., 2004), sharing ferredoxin (Fd) as a common stromal electron donor (Yamamoto et al., 2011) and electron carriers from plastoquinone (PQ) to PSI with LEF. Thus, LEF and either of the CEF pathways may be in competition. The molecular events that allow CEF to challenge LEF remain enigmatic, particularly when considering that the conditions that require CEF are also those under which LEF is in excess. Efforts to understand the appropriate functioning of CEF have led to the proposition of several models segregating cyclic and linear pathways at a structural level (for review, see Eberhard et al., 2008; Cardol et al., 2011; Johnson, 2011; Rochaix, 2011). According to the restricted diffusion model, founded on the uneven distribution of the photosynthetic protein complexes in the thylakoids, there is little competition between CEF and LEF, as CEF occurs in stroma lamellae where PSI is concentrated while LEF takes place in the grana stacks. In line with the supercomplex model, whose relevance was demonstrated in the microalga Chlamydomonas reinhardtii, CEF happens within tightly bound supercomplexes containing PSI, with its own light-harvesting complex (LHCI), the PSII light-harvesting complex (LHCII), cytochrome b₆/f, Fd, Fd NADP reductase (FNR), and the integral membrane protein PGRL1 (Iwai et al., 2010). In higher plants, an association between NDH and PSI subunits suggests the formation of such supercomplexes (Peng et al., 2009). The availability of FNR, found either free in the stroma or bound to the thylakoids (Zhang et al., 2001), has also been proposed to modulate partitioning between LEF and CEF (Joliot and Joliot, 2006; Joliot and Johnson, 2011). In addition, more dynamic models that illustrate competitive processes involved in the distribution of electrons between the cyclic and linear flows have been proposed. The competition between cytochrome b₆/f and FNR for electrons from Fd could regulate the segregation between LEF and CEF (Breyton et al., 2006; Yamamoto et al., 2006; Hald et al., 2008). A few years ago, Joliot and Joliot (2006) suggested that the ATP/ADP ratio was one of the parameters that triggered on the transition between LEF and CEF. It was also established that the redox poise of chloroplast stroma contributed to the regulation of the photosynthetic pathway and played an important role in defining the extent of CEF. Breyton et al. (2006) scrutinized this redox regulation and established that the fraction of PSI complexes engaged in CEF could be modulated by changes in the stromal redox state. Overreduction of the NADPH pool was involved in the repartition between LEF and CEF (Joliot and Joliot, 2006). The NADPH/NADP⁺ ratio was proposed as a regulator of PGR-dependent CEF in vivo (Okegawa et al., 2008).All the published data supporting a role for the redox status in the regulation of CEF urged us to investigate a putative role of thioredoxins (TRX) in the regulation of CEF. TRX are ubiquitous disulfide reductases regulating the redox status of target proteins (for review, see Lemaire et al., 2007; Meyer et al., 2009). In chloroplast, TRX mediate the light regulation of numerous enzymes, among which some belong to the Calvin cycle (for review, see Schürmann and Buchanan, 2008; Montrichard et al., 2009; Lindahl et al., 2011). Global proteomic approaches have revealed that well-known photosynthetic complex subunits may be partners of TRX, such as PsbO in PSII, plastocyanin, Rieske Fe-S protein in cytochrome b₆/f, and PsaK and PsaN in PSI (for review, see Montrichard et al., 2009; Lindahl et al., 2011). Furthermore, regarding the regulation of photosynthesis, TRX have also been involved in state transitions (Rintamäki et al., 2000; Buchanan and Balmer, 2005), and their participation in the control of the redox poise of the electron transport chain has also been suggested (Johnson, 2003).In this work, we have investigated the possible role of TRX in the regulation of CEF. Using Arabidopsis (Arabidopsis thaliana) mutants with altered expression of genes encoding different plastid TRX, we have established in vivo the inhibitor activity of TRXm4 on the NDH-dependent pathway for plastoquinone reduction. This result was confirmed in transplastomic tobacco (Nicotiana tabacum) plants overexpressing the TRXm4 orthologous gene. Moreover, in vitro assays performed with isolated chloroplasts indicated that TRXm4 negatively controls the PGR-dependent electron flow as well.     

The Antarctic Psychrophile Chlamydomonas sp. UWO 241 Preferentially Phosphorylates a Photosystem I-Cytochrome b6/f Supercomplex

Chlamydomonas sp. UWO 241 (UWO 241) is a psychrophilic green alga isolated from Antarctica. A unique characteristic of this algal strain is its inability to undergo state transitions coupled with the absence of photosystem II (PSII) light-harvesting complex protein phosphorylation. We show that UWO 241 preferentially phosphorylates specific polypeptides associated with an approximately 1,000-kD pigment-protein supercomplex that contains components of both photosystem I (PSI) and the cytochrome b₆/f (Cyt b₆/f) complex. Liquid chromatography nano-tandem mass spectrometry was used to identify three major phosphorylated proteins associated with this PSI-Cyt b₆/f supercomplex, two 17-kD PSII subunit P-like proteins and a 70-kD ATP-dependent zinc metalloprotease, FtsH. The PSII subunit P-like protein sequence exhibited 70.6% similarity to the authentic PSII subunit P protein associated with the oxygen-evolving complex of PSII in Chlamydomonas reinhardtii. Tyrosine-146 was identified as a unique phosphorylation site on the UWO 241 PSII subunit P-like polypeptide. Assessment of PSI cyclic electron transport by in vivo P700 photooxidation and the dark relaxation kinetics of P700⁺ indicated that UWO 241 exhibited PSI cyclic electron transport rates that were 3 times faster and more sensitive to antimycin A than the mesophile control, Chlamydomonas raudensis SAG 49.72. The stability of the PSI-Cyt b₆/f supercomplex was dependent upon the phosphorylation status of the PsbP-like protein and the zinc metalloprotease FtsH as well as the presence of high salt. We suggest that adaptation of UWO 241 to its unique low-temperature and high-salt environment favors the phosphorylation of a PSI-Cyt b₆/f supercomplex to regulate PSI cyclic electron transport rather than the regulation of state transitions through the phosphorylation of PSII light-harvesting complex proteins.The Antarctic psychrophilic green alga Chlamydomonas sp. UWO 241 (UWO 241) originates from the lowest trophic zone of Lake Bonney, which is characterized by an extremely stable environment of low temperatures (4°C–6°C), low irradiance (less than 50 µmol photons m⁻² s⁻¹), high salt concentrations (700 mm), and a narrow spectral distribution enriched in the blue-green region (Lizotte and Priscu, 1992; Morgan-Kiss et al., 2006). Adaptation of UWO 241 to this unique natural aquatic environment has resulted in the evolution of a structurally and functionally distinct photosynthetic apparatus relative to the mesophilic strains Chlamydomonas raudensis SAG 49.72 (SAG 49.72; Pocock et al., 2004) and the model green alga Chlamydomonas reinhardtii (Morgan et al., 1998; Morgan-Kiss et al., 2006). UWO 241 is a halotolerant psychrophile (Morgan-Kiss et al., 2006; Takizawa et al., 2009) that dies at temperatures of 20°C or higher (Possmayer et al., 2011). This is consistent with the fact that temperature-response curves for light-saturated rates of CO₂-saturated oxygen evolution indicate that UWO 241 photosynthesizes maximally at 8°C at rates that are comparable to rates of the mesophile, C. reinhardtii, grown and measured at 29°C (Pocock et al., 2007). Although UWO 241 exhibits a low quantum requirement for photoinhibition and the degradation of the PSII reaction center polypeptide D1 (PsbA), this is complemented by a rapid, light-dependent recovery of PSII photochemistry associated with the de novo biosynthesis of D1 at low temperature (Pocock et al., 2007). Thus, this psychrophile appears to be photosynthetically adapted to growth at low temperature (Pocock et al., 2007).UWO 241 exhibits significantly enhanced fatty acid unsaturation associated with all of the major thylakoid lipid classes (monogalactosyldiacylglyceride, digalactosyldiacylglyceride, sulfoquinovosyldiacylglyceride, and phosphatidyldiacylglyceride) as well as a 2- to 10-fold increase in the unique, unsaturated fatty acid 16:4, depending on the specific thylakoid lipid species (Morgan-Kiss et al., 2002a). Consequently, the biophysical determination of the critical temperature for thylakoid membrane destabilization for UWO 241 (40°C) was significantly lower than that for C. reinhardtii (50°C), which is consistent with the adaptation of UWO 241 to low temperature (Morgan-Kiss et al., 2002a).Biochemical analyses of the chlorophyll-protein complexes coupled with immunoblots of their constituent polypeptides indicate that UWO 241 exhibits abundant PSII light-harvesting complex (LHCII) associated with a low chlorophyll a/b (Chl a/b) ratio (1.8–2) relative to the mesophiles, SAG 49.72 and C. reinhardtii (Chl a/b ratio = 3). In addition, UWO 241 exhibits an unusually low level of PSI such that the stoichiometry of PSI/PSII was estimated to be about 0.5 in UWO 241, whereas the mesophiles, SAG 49.72 and C. reinhardtii, grown under optimal growth conditions, exhibited a PSI/PSII of about 1. These biochemical data were confirmed by measurements of P700 photooxidation (Morgan-Kiss et al., 2002b; Szyszka et al., 2007), which indicated that UWO 241 exhibits high rates of PSI cyclic electron flow (CEF; Morgan-Kiss et al., 2002b).Recently, we reported that acclimation of UWO 241 to low temperature and low growth irradiance results in alterations in the partitioning of excess excitation energy to maintain cellular energy balance compared with the mesophile, SAG 49.72 (Szyszka et al., 2007). While SAG 49.72 favors energy partitioning for photoprotection through the induction of the xanthophyll cycle, the psychrophilic strain, UWO 241, favors energy partitioning for photoprotection through constitutive quenching processes involved in energy dissipation, even though UWO 241 exhibits an active xanthophyll cycle (Pocock et al., 2007; Szyszka et al., 2007). Although the molecular basis of the constitutive quenching process for photoprotection has not been elucidated unequivocally, this may reflect the differences in the predisposition for energy dissipation through either the Q2 or the Q1 site in PSII-LHCII supercomplexes (Jahns and Holzwarth 2012; Derks et al., 2015) or, alternatively, it may indicate quenching through PSII reaction centers, as suggested previously (Hüner et al., 2006; Sane et al., 2012). Regardless of the mechanism, one consequence of this enhanced energy-quenching capacity of UWO 241 is that the psychrophile does not exhibit any pigment change in response to photoacclimation (Morgan-Kiss et al., 2006), typically observed for other mesophilic green algae such as C. reinhardtii, Dunaliella tertiolecta (Escoubas et al., 1995), Dunaliella salina (Smith et al., 1990; Maxwell et al., 1995), and Chlorella vulgaris (Maxwell et al., 1995; Wilson et al., 2003). In addition, maximum growth rates of UWO 241 are sensitive to light quality, since rates of growth and photosynthesis are inhibited under red light, which results in increased excitation pressure in the psychrophile (Morgan-Kiss et al., 2005).However, the most unusual feature of UWO 241 is that it represents a natural variant that is deficient in state transitions (Morgan-Kiss et al., 2002b; Takizawa et al., 2009). State transitions have been well documented as a short-term mechanism for photoacclimation employed by algae and plants to balance light excitation between PSII and PSI (Allen et al., 1981; Allen, 2003; Eberhard et al., 2008; Rochaix, 2011, 2014). Overexcitation of PSII relative to PSI results in the phosphorylation of several peripheral Chl a/b-binding LHCII proteins, which causes their dissociation from the PSII core and subsequent association with PSI (Eberhard et al., 2008; Rochaix, 2011). As a result, excitation energy is redistributed in favor of PSI at the expense of PSII. Phosphorylation of LHCII polypeptides is essential in the regulation of state transitions and energy distribution between the two photosystems (Allen, 2003; Eberhard et al., 2008; Kargul and Barber, 2008; Rochaix, 2011, 2014). LHCII phosphorylation is initiated by modulation of the redox state of the plastoquinone (PQ) pool, which is sensed through the preferential binding of plastoquinol to the quinone-binding site of the cytochrome b₆/f (Cyt b₆/f) complex. As a consequence, the thylakoid protein kinases STT7 in C. reinhardtii and its ortholog, STN7, in Arabidopsis (Arabidopsis thaliana) are activated and LHCII is phosphorylated (Rochaix, 2011, 2014; Wunder et al., 2013). Similar to all other photosynthetic organisms, the LHCII polypeptides represent the major phosphorylated polypeptides detected in thylakoids of the mesophile, SAG 49.72 (Szyszka et al., 2007). Consistent with a deficiency in state transitions, UWO 241 does not phosphorylate the major LHCII polypeptides in response to changes in either growth irradiance or growth temperature (Morgan-Kiss et al., 2002b; Szyszka et al., 2007; Takizawa et al., 2009). In fact, UWO 241 exhibits a unique thylakoid membrane phosphorylation profile compared with either SAG 49.72 or C. reinhardtii (Morgan-Kiss et al., 2005; Szyszka et al., 2007; Takizawa et al., 2009). Rather than phosphorylation of LHCII polypeptides, UWO 241 preferentially phosphorylates several novel high-molecular-mass polypeptides (greater than 70 kD; Morgan-Kiss et al., 2002b; Szyszka et al., 2007).The Cyt b₆/f complex of the photosynthetic intersystem electron transport chain is essential in the regulation of state transitions and the activation of the STT7 kinase (Rochaix, 2011, 2014). The Cyt b₆/f complex of UWO 241 exhibits a unique cytochrome f (Cyt f) that is 7 kD smaller than the expected molecular mass of 41 kD exhibited by C. reinhardtii based on SDS-PAGE (Morgan-Kiss et al., 2006; Gudynaite-Savitch et al., 2006, 2007). No other differences in the structure and composition of the Cyt b₆/f complex are apparent. Sequencing of the entire Cytochrome f gene (petA) from UWO 241 indicated that the amino acid sequence of Cyt f from UWO 241 exhibited 79% identity to that of C. reinhardtii. Through domain swapping between petA of UWO 241 and that of C. reinhardtii and subsequent transformation of a ΔpetA mutant of C. reinhardtii with the chimeric gene constructs, we reported that the apparent differences in molecular masses observed for petA in UWO 241 are due to differences in the amino acid sequences of the small domain of Cyt f. However, complementation of the ΔpetA mutant of C. reinhardtii with the entire petA from either UWO 241 or C. reinhardtii completely restored the capacity for state transitions in the ΔpetA mutant. Thus, we concluded that the changes in the amino acid sequence of the small domain of Cyt f of UWO 241 cannot account for the inability of UWO 241 to undergo state transitions (Gudynaite-Savitch et al., 2006, 2007).Since state transitions are inhibited in UWO 241, we hypothesized that the unique protein phosphorylation pattern observed in UWO 241 reflects an alternative mechanism to regulate energy flow within the photosynthetic apparatus of this Antarctic psychrophile. Thus, the objective of this research was to identify and characterize the high-molecular-mass polypeptides phosphorylated in the psychrophile, UWO 241. We report that UWO 241 preferentially phosphorylates specific polypeptides associated with a PSI-Cyt b₆/f supercomplex. The role of the PSI-Cyt b₆/f supercomplex and its phosphorylation status in the regulation of PSI cyclic electron transport in UWO 241 are discussed. We suggest that adaptation of UWO 241 to its unique low-temperature and low-light environment favors the phosphorylation of a PSI-Cyt b₆/f supercomplex to regulate PSI cyclic electron transport rather than the regulation of state transitions through the phosphorylation of LHCII proteins.