Cyanobacterial phytochrome-like PixJ1 holoprotein shows novel reversible photoconversion between blue- and green-absorbing forms

The gene, pixJ1 (formerly pisJ1), is predicted to encode a phytochrome-like photoreceptor that is essential for positive phototaxis in the unicellular cyanobacterium Synechocystis sp. PCC 6803 [Yoshihara et al. (2000) Plant Cell Physiol. 41: 1299]. The PixJ1 protein was overexpressed as a fusion with a poly-histidine tag (His-PixJ1) and isolated from Synechocystis cells. A zinc-fluorescence assay suggested that a linear tetrapyrrole was covalently attached to the His-PixJ1 protein as a chromophore. His-PixJ1 showed novel photoreversible conversion between a blue light-absorbing form (Pb, lambdaAmax=425-435 nm) and a green light-absorbing form (Pg, lambdaAmax=535 nm). Dark incubation led Pg to revert to Pb, indicative of stability of the Pb form in darkness. Red or far-red light irradiation, which is effective for photochemical conversion of the known phytochromes, produced no change in the spectra of Pb and Pg forms. Site-directed mutagenesis revealed that a Cys-His motif in the second GAF domain of PixJ1 is responsible for binding of the chromophore. Possible chromophore species are discussed with regard to the novel photoconversion spectrum.     

Continuous Turnover of Carotenes and Chlorophyll a in Mature Leaves of Arabidopsis Revealed by 14CO2 Pulse-Chase Labeling

Carotenoid turnover was investigated in mature leaves of Arabidopsis (Arabidopsis thaliana) by ¹⁴CO₂ pulse-chase labeling under control-light (CL; 130 μmol photons m⁻² s⁻¹) and high-light (HL; 1,000 μmol photons m⁻² s⁻¹) conditions. Following a 30-min ¹⁴CO₂ administration, photosynthetically fixed ¹⁴C was quickly incorporated in β-carotene (β-C) and chlorophyll a (Chl a) in all samples during a chase of up to 10 h. In contrast, ¹⁴C was not detected in Chl b and xanthophylls, even when steady-state amounts of the xanthophyll-cycle pigments and lutein increased markedly, presumably by de novo synthesis, in CL-grown plants under HL. Different light conditions during the chase did not affect the ¹⁴C fractions incorporated in β-C and Chl a, whereas long-term HL acclimation significantly enhanced ¹⁴C labeling of Chl a but not β-C. Consequently, the maximal ¹⁴C signal ratio between β-C and Chl a was much lower in HL-grown plants (1:10) than in CL-grown plants (1:4). In lut5 mutants, containing α-carotene (α-C) together with reduced amounts of β-C, remarkably high ¹⁴C labeling was found for α-C while the labeling efficiency of Chl a was similar to that of wild-type plants. The maximum ¹⁴C ratios between carotenes and Chl a were 1:2 for α-C:Chl a and 1:5 for β-C:Chl a in CL-grown lut5 plants, suggesting high turnover of α-C. The data demonstrate continuous synthesis and degradation of carotenes and Chl a in photosynthesizing leaves and indicate distinct acclimatory responses of their turnover to changing irradiance. In addition, the results are discussed in the context of photosystem II repair cycle and D1 protein turnover.Carotenoids are classified as accessory pigments in photosynthesis because they augment light harvesting in the blue spectral region by transferring the absorbed light energy to chlorophyll (Chl). However, the universal occurrence of carotenoids in photosynthetic cells, from bacteria to higher plants, indicates their essential roles, rather than mere accessory roles, in photosynthesis. Under excess light, carotenoids provide protection against photooxidative damage by facilitating dissipation of excitation energy from singlet- or triplet-state Chl and scavenging highly reactive singlet oxygen, which is generated through interaction between triplet excited Chl and oxygen (Demmig-Adams, 1990; Müller et al., 2001). These photoprotective functions make carotenoids indispensable for oxygenic photosynthesis, as demonstrated by lethal effects of inhibitors of carotenoid biosynthesis in plants (Bramley, 1993). Regulation of light harvesting and photoprotection by carotenoids requires their close proximity as well as the proper orientation to Chl molecules in pigment-protein complexes of PSI and PSII. Furthermore, a small fraction of non-protein-bound carotenoids serves as antioxidants in the lipid phase of photosynthetic membranes (Havaux and Niyogi, 1999; Havaux et al., 2004) and influences the structure and fluidity of the lipid bilayer (Gruszecki and Strzałka, 2005). Despite these and other lines of defense, the PSII reaction center polypeptide D1, and to a lesser extent also D2, undergo frequent photooxidative damage and repair in the light (Melis, 1999; Baena-González and Aro, 2002). When the repair process cannot keep up with the rate of photodamage, the overall quantum yield of PSII declines.Carotenoids are derived from isoprenoid precursors in plastids (for reviews on carotenoid biosynthesis in plants, see Lichtenthaler, 1999; Hirschberg, 2001; DellaPenna and Pogson, 2006; Giuliano et al., 2008; Tanaka et al., 2008; Cazzonelli and Pogson, 2010). Following the formation of linear C₄₀ lycopene, the pathway splits into two branches of major cyclic carotenoids: the β,β-branch gives rise to β-carotene (β-C) having two β-rings, whereas the β,ϵ-branch leads to formation of α-carotene (α-C) having one β-ring and one ϵ-ring. Hydroxylation of β-C and α-C produces the xanthophylls zeaxanthin (Z) and lutein (L), respectively. In the β,β-branch, epoxidation of the β-rings of Z results in successive synthesis of antheraxanthin (A) and violaxanthin (V); subsequently, V can be converted to neoxanthin (N), the last carotenoid product of the β,β-branch. Except for some species (García-Plazaola et al., 2007), L does not undergo β-ring epoxidation and the β,ϵ-branch thus stops with L, the most abundant carotenoid in leaves.Each of these carotenoids occupies specific binding sites in the photosynthetic apparatus to fulfill distinct roles. In both PSI and PSII, carotenes (α-C and β-C) are generally bound in core complexes, which also harbor Chl a molecules, while the majority of xanthophylls (L, Z, A, V, and N) are bound in light-harvesting antenna complexes together with Chl a and Chl b molecules (Bassi et al., 1993; Lee and Thornber, 1995). Accumulation of β-C in core complexes is a common feature of diverse photosynthetic organisms, whereas the occurrence of α-C in addition to β-C is restricted to certain taxa. For higher plants, α-C has been found in leaves of some, but not all, shade-tolerant species (Thayer and Björkman, 1990; Demmig-Adams and Adams, 1992; Demmig-Adams, 1998; Matsubara et al., 2009). Based on this photoacclimatory behavior, it has been proposed that α-C may function as a light-harvesting pigment while β-C may contribute to photoprotection (Krause et al., 2001), presumably by scavenging singlet oxygen and mediating a cyclic electron transfer around PSII (Tracewell et al., 2001; Telfer, 2005).Pronounced light-dependent changes are also observed for xanthophyll composition in light-harvesting antenna complexes. In a short term (minutes to hours), operation of the xanthophyll cycle, involving Z, A, and V, modulates levels of Z in a light-dependent manner. It is widely accepted that Z is able to enhance the dissipation of excess light energy from singlet excited Chl while V is not (Demmig-Adams, 1990; Müller et al., 2001). Long-term acclimation (days) to strong irradiance typically results in an increased pool size of the xanthophyll-cycle pigments (V + A + Z) and downsizing of PSII antenna, as indicated by a greater Chl a-to-Chl b ratio (Demmig-Adams and Adams, 1992; Demmig-Adams, 1998; Matsubara et al., 2009). Based on the observed changes in steady-state amounts of xanthophylls and carotenes following irradiance shifts, alterations in the balance between biosynthesis and degradation, or turnover, have been implicated as a mechanism for long-term adjustment of carotenoid levels in leaves (Förster et al., 2009). However, just how much biosynthesis and degradation of different carotenoids occurs in photosynthesizing green leaves is an open question to date.In order to gain insight into carotenoid turnover of mature leaves, we conducted ¹⁴CO₂ pulse-chase labeling experiments with Arabidopsis (Arabidopsis thaliana) plants. Carotenoid turnover has been studied in algae in the past by applying [¹⁴C]bicarbonate (Blass et al., 1959; Grumbach et al., 1978); for example, no more than 1% to 2% of the photosynthetically incorporated ¹⁴C was allocated to the lipophilic fraction containing Chl and carotenoid in Chlorella pyrenoidosa after a 2-h pulse application (Grumbach et al., 1978). Even lower labeling efficiency is expected for photosynthetic pigments in nongrowing green leaves, in which pigment turnover takes place almost exclusively as part of the maintenance and acclimation of photosynthetic membranes. To overcome this intrinsic but anticipated difficulty, a ¹⁴CO₂ application setup was established for efficient and reproducible ¹⁴CO₂ incorporation in detached leaves of Arabidopsis during a short (30-min) pulse period. Moreover, a method of pigment separation was developed for ¹⁴C detection in concentrated leaf pigment extracts using a radio-HPLC system. Because carotenoid composition exhibits marked sun-shade responses in leaves (Demmig-Adams and Adams, 1992; Demmig-Adams, 1998; Matsubara et al., 2009), ¹⁴CO₂ labeling patterns were studied in three different sets of Arabidopsis plants: (1) plants grown under 130 μmol photons m⁻² s⁻¹ (control light [CL]) and exposed to CL during a chase period of up to 10 h (CL plants); (2) plants acclimated to 1,000 μmol photons m⁻² s⁻¹ (high light [HL]) for 2 weeks and exposed to HL during the chase period (HL plants); and (3) plants grown under CL but exposed to HL during the chase period (CL→HL plants). These treatments simulated short-term (CL→HL) and long-term (CL or HL) responses to irradiance. Finally, as ¹⁴C was found to be rapidly incorporated in β-C and Chl a molecules in leaves of wild-type plants, in which β-C represents the only carotene species, ¹⁴C labeling experiments were also conducted with leaves of lut5 mutants containing both α-C and β-C (Fiore et al., 2006; Kim and DellaPenna, 2006) to compare turnover of the two carotenes.     

Refolding and purification of recombinant OsNifU1A domain II that was expressed by Escherichia coli

OsNifU1A is a NifU-like rice (Oryza sativa) protein, discovered recently. Its amino acid sequence is very homologous to the sequence of cyanobacterial CnfU and to the sequences of NifU C-terminal domains. Based on its sequence, OsNifU1A is probably a modular structure consisting of two CnfU-like domains, with domain I (formed by residues Leu73 to Gly153) and domain II (formed by residues Leu154 to Ser226). Domain I have a conserved Cys-X-X-Cys motif, which may function as an iron-sulfur cluster assembly scaffold. Domain II lacks a Cys-X-X-Cys motif and therefore, cannot function analogously. Other NifU-like proteins, with sequences homologous to OsNifU1A domain II, have been identified during plant genomic projects; however, the biological roles of these domains remain unknown. We successfully constructed an Escherichia coli expression system for OsNifU1A domain II that enabled us to synthesize and purify milligram quantities of protein for use in structural and functional studies. Using the Gateway system, we built DNA sequences corresponding to two OsNifU1A domain II fusion proteins. One construct has a (His)6 sequence upstream of the OsNifU1A domain II sequence; the other has an upstream thioredoxin-(His)6 sequence. Recombinant OsNifU1A domain II fusion proteins were extracted from E. coli inclusion bodies by dissolving them in 6 M guanidine-HCl. About 36% of the total (His)6/OsNifU1A domain II fusion protein initially present remained soluble after guanidine-HCl was completely removed by step-wise dialysis; whereas, recovery of soluble Trx-(His)6 fusion protein was about 60% of the total cell lysate. About 2 mg of 15N-labeled OsNifU1A domain II was purified for NMR spectral studies. Examination of the OsNifU1A domain II 1H-15N HSQC NMR spectrum indicated that the purified protein was monomeric and correctly folded. Therefore, we established an efficient procedure for synthesis and purification of 15N-labeled OsNifU1A domain II in quantities sufficient for heteronuclear NMR solution structure studies.     

Slowly reversible de-epoxidation of lutein-epoxide in deep shade leaves of a tropical tree legume may 'lock-in' lutein-based photoprotection during acclimation to strong light

The kinetics of response to strong light have been examined in deeply shaded leaves of the tropical tree legume (Inga sp.) which have extraordinarily high levels of the alpha-xanthophyll lutein-epoxide that are co-located in pigment-protein complexes of the photosynthetic apparatus with the beta-xanthophyll violaxanthin. As in other species, rapidly reversible photoprotection (measured as non-photochemical chlorophyll fluorescence quenching) is initiated within the time frame of sun-flecks (minutes), before detectable conversion of violaxanthin to antheraxanthin or zeaxanthin. Photoprotection is stabilized within hours of exposure to strong light by simultaneously engaging the reversible violaxanthin cycle and a slowly reversible conversion of lutein-epoxide to lutein. It is proposed that this lutein 'locks in' a primary mechanism of photoprotection during photoacclimation in this species, converting efficient light-harvesting antennae of the shade plant into potential excitation dissipating centres. It is hypothesized that lutein occupies sites L2 and V1 in light-harvesting chlorophyll protein complexes of photosystem II, facilitating enhanced photoprotection through the superior singlet and/or triplet chlorophyll quenching capacity of lutein.     

Establishment of a detection system for demethylating agents using an endogenous promoter CpG island

Disturbances of epigenetic information that result in changes in DNA methylation patterns are involved in carcinogenesis and other human disorders. Detection of agents that can cause epigenetic alterations--i.e. epimutagens--is therefore an important objective. We have developed and now describe the first detection system for demethylating agents that involves an endogenous promoter CpG island (CGI). After screening 10 promoter CGIs of genes silenced in human cancers, a CGI of the FLJ32130 gene was found to respond sensitively to a known demethylating agent, 5-aza-2'-deoxycytidine (5-aza-dC), by abundantly re-expressing its mRNA. After introducing the Hyg(r)-EGFP fusion gene into exon 3 of the FLJ32130 gene by homologous recombination, we isolated one clone that had the expected recombination outcomes and designated it F117. Two subclones (F117-47 and F117-123) of this original clone that did not share its propensity for leaky expression of the Hyg(r)-EGFP mRNA were then isolated, and methylation of their 5' CGI was confirmed. The addition of 5-aza-dC at doses of 0.1 microM or higher led to their 5' CGI being demethylated, and to Hyg(r)-EGFP being expressed; the anticipated fluorescence was readily confirmed by fluorescence microscopy. We believe that this is the first assay system that detects agents that disturb the methylated status of a CGI that regulates an endogenous promoter.     

Characterization of cyanobacteriochrome TePixJ from a thermophilic cyanobacterium Thermosynechococcus elongatus strain BP-1

A putative photoreceptor gene, TepixJ, of a thermophilic cyanobacterium is homologous to SypixJ1 that mediates positive phototaxis in the unicellular motile cyanobacterium Synechocystis sp. PCC 6803. The putative chromophore-binding GAF domain of TePixJ protein was overexpressed as a fusion with a polyhistidine tag (His-TePixJ_GAF) in Synechocystis cells and isolated to homogeneity. The photoreversible conversion of His-TePixJ_GAF showed peaks at 531, 341 and 266 nm for the green light-absorbing form (Pg form), and peaks at 433 and 287 nm for the blue light-absorbing form (Pb form). At 77K, the Pg form fluoresced at 580 nm, while the Pb form did not emit any fluorescence. Mass spectrometry of the tryptic chromopeptide demonstrated that a phycocyanobilin isomer binds to the conserved cysteine at ring A via a thioether bond. It is established that TePixJ and SyPixJ1 are novel photoreceptors in cyanobacteria ('cyanobacteriochromes') that are similar, but distinct from the phytochromes and bacteriophytochromes.     

Diel patterns of leaf and root growth: endogenous rhythmicity or environmental response?

Plants are sessile organisms forced to adjust to their surrounding environment. In a single plant the photoautotrophic shoot is exposed to pronounced environmental variations recurring in a day-night 24?h (diel) cycle, whereas the heterotrophic root grows in a temporally less fluctuating environment. The contrasting habitats of shoots and roots are reflected in different diel growth patterns and their responsiveness to environmental stimuli. Differences between diel leaf growth patterns of mono- and dicotyledonous plants correspond to their different organization and placement of growth zones. In monocots, heterotrophic growth zones are organized linearly and protected from the environment by sheaths of older leaves. In contrast, photosynthetically active growth zones of dicot leaves are exposed directly to the environment and show characteristic, species-specific diel growth patterns. It is hypothesized that the different exposure to environmental constraints and simultaneously the sink/source status of the growing organs may have induced distinct endogenous control of diel growth patterns in roots and leaves of monocot and dicot plants. Confronted by strong temporal fluctuations in environment, the circadian clock may facilitate robust intrinsic control of leaf growth in dicot plants.     

Lutein epoxide cycle, light harvesting and photoprotection in species of the tropical tree genus Inga

Dynamics and possible function of the lutein epoxide (Lx) cycle, that is, the reversible conversion of Lx to lutein (L) in the light-harvesting antennae, were investigated in leaves of tropical tree species. Photosynthetic pigments were quantified in nine Inga species and species from three other genera. In Inga , Lx levels were high in shade leaves (mostly above 20 mmol mol⁻¹ chlorophyll) and low in sun leaves. In Virola surinamensis , both sun and shade leaves exhibited very high Lx contents (about 60 mmol mol⁻¹ chlorophyll). In Inga marginata grown under high irradiance, Lx slowly accumulated within several days upon transfer to deep shade. When shade leaves of I. marginata were briefly exposed to the sunlight, both violaxanthin and Lx were quickly de-epoxidized. Subsequently, overnight recovery occurred only for violaxanthin, not for Lx. In such leaves, containing reduced levels of Lx and increased levels of L, chlorophyll fluorescence induction showed significantly slower reduction of the photosystem II electron acceptor, Q _A, and faster formation as well as a higher level of non-photochemical quenching. The results indicate that slow Lx accumulation in Inga leaves may improve light harvesting under limiting light, while quick de-epoxidation of Lx to L in response to excess light may enhance photoprotection.     

Novel antibody to human BASP1 labels apoptotic cells post-caspase activation

Apoptosis is associated with morphological changes, including membrane blebbing, cell shrinkage, and chromatin condensation. However, the molecular mechanisms of the dynamic changes in cellular components during apoptosis are largely unknown. Here we developed a new rat monoclonal antibody, 9B1, that specifically immunolabeled dying cells in tissues and in cell cultures. The 9B1 antibody labeled the cytoplasm of apoptotic cells in a caspase-dependent manner. We identified human brain abundant membrane attached signal protein 1 (hBASP1) as the 9B1 antigen using the liquid chromatography with tandem mass spectrometry (LC/MS/MS) method. hBASP1 was present in the nucleus of HeLa cells, but relocated from the nucleus to the cytoplasm after the caspase activation step of apoptosis. Immunostaining analysis revealed that 9B1 preferentially labeled this cytoplasmic form of hBASP1. Labeling by 9B1 to distinguish apoptotic changes could be a novel criterion for determining whether cells with activated caspases are fated for survival or death.