ADP/ATP Translocator from Pea Root Plastids (Comparison with Translocators from Spinach Chloroplasts and Pea Leaf Mitochondria)

The kinetic properties of the adenosine 5[prime]-diphosphate/adenosine 5[prime]-triphosphate (ADP/ATP) translocator from pea (Pisum sativum L.) root plastids were determined by silicone oil filtering centrifugation and compared with those of spinach (Spinacia oleracea L.) chloroplasts and pea leaf mitochondria. In addition, the ADP/ATP transporting activities from the above organelles were reconstituted into liposomes. The Km(ATP) value of the pea root ADP/ATP translocator was 10 [mu]M and that for ADP was 46 [mu]M. Corresponding values of the spinach ADP/ATP translocator were 25 [mu]M and 28 [mu]M, respectively. Comparable results were obtained for the reconstituted ATP transport activities. The transport was highly specific for ATP and ADP. Adenosine 5[prime]-monophosphate (AMP) caused only a slight inhibition and phosphoenolpyruvate and inorganic pyrophosphate caused no inhibition of ATP uptake. With pea root plastids and spinach chloroplasts, Km values >1 mM were obtained for ADP-glucose. Since the concentrations of ATP and ADP-glucose in the cytosolic compartment of spinach leaves have been determined as 2.5 and 0.6 mM, respectively, a transport of ADP-glucose by the ADP/ATP translocator does not appear to have any physiological significance in vivo. Although both the plastidial and the mitochondrial ADP/ATP translocators were inhibited to some extent by carboxyatractyloside, no immunological cross-reactivity was detected between the plastidial and the mitochondrial proteins. It seems probable that these proteins derive from different ancestors.     

Chemical Modification of the Membrane-bound ATP Synthetase of Spinach Chloroplasts with Pyridoxal Phosphate in Light

Photosynthetic activities of the thylakoid membranes modifiedwith pyridoxal phosphate (PLP) and sodium borohydride in lightwere studied and compared with those modified in the dark. PLPmodified the membrane-bound chloroplast coupling factor 1 (CF₁)and inhibited photophosphorylation. Only PLP modification inlight stimulated basal electron transport. This stimulationof electron transport was prevented by the presence of ATP orcarbonylcyanide m-chlorophenylhydrazone in the modificationmixture. Magnesium ion was required for PLP modification. Theextent of lightinduced proton uptake was decreased by PLP modificationin light. N,N'-Dicyclohexylcarbodiimide lowered the stimulatedelectron transport to the basal level of unmodified chloroplastsand restored proton uptake. When chloroplasts were modified with 4 mM PLP in light and dark,11.6 and 11.0 mol of PLP were incorporated into mol of CF₁,respectively. ATP could bind with high affinity to CF₁ isolatedafter PLP modification in light. The results indicate that PLP modifies membrane-bound CF₁ whichhas a conformation altered by energization of the thylakoidsin light, and causes an apparent uncoupling of phosphorylation(stimulation of basal electron transport). The results suggestthat this uncoupling is induced by the loss of the regulatoryfunction of CF₁ for proton translocation after PLP modificationin light. ¹ Presented at the ISRACON on Control Mechanisms in Photosynthesis.Aug. 31-Sept. 4, 1980, Acre, Israel (Received June 22, 1981; Accepted August 28, 1981)     

Uptake of l-Ascorbate by Intact Spinach Chloroplasts

Uptake of l-[1-¹⁴C]ascorbate by intact ascorbate-free spinach (Spinacia oleracea L. cv Vital^r) chloroplasts has been investigated using the technique of silicone oil filtering. Rates greater than 100 micromoles per milligram chlorophyll per hour (external concentration, 10 millimolar) of ascorbate transport were observed. Ascorbate uptake into the sorbitol-impermeable space (stroma) followed the Michaelis-Menten-type characteristic for substrate saturation. A K_m of 18 to 40 millimolar was determined. Transport of ascorbate across the chloroplast envelope resulted in an equilibrium of the ascorbate concentrations between stroma and medium. A pH optimum of 7.0 to 7.5 and the lack of alkalization of the medium upon ascorbate uptake suggest that only the monovalent ascorbate anion is able to cross the chloroplast envelope. The activation energy of ascorbate uptake was determined to be 65.8 kilojoules (16 kilocalories) per mole (8 to 20°C). Interference of ascorbate transport with substrates of the phosphate or dicarboxylate translocator could not be detected, but didehydroascorbate was a competitive inhibitor. Preloading of chloroplasts with didehydroascorbate resulted in an increase of V_max but did not change the K_m for ascorbate. Millimolar concentrations of the sulfhydryl reagent p-chloromercuriphenyl sulfonate inhibited ascorbate uptake. The data are interpreted in terms of ascorbate uptake into chloroplasts by the mechanism of facilitated diffusion mediated by a specific translocator.     

Characteristics of Prompt and Delayed Fluorescence from Spinach Chloroplasts

Effects of ferricyanide, dichlorophenyldimethylurea (DCMU), and uncouplers of phosphorylation on the prompt and delayed fluorescences from spinach chloroplasts are described. Any factor that affects the yield of prompt fluorescence will similarly influence the intensity of delayed fluorescence. This idea, recently investigated by Lavorel, should be expressed in terms of a “live” component of fluorescence; that is, the component from chlorophyll associated with the photochemical traps of System II. Some of the effects of ferricyanide and DCMU on delayed fluorescence can then be explained in terms of effects on the yield of prompt fluorescence. From the internal consistency of the explanation, applied to various observations, a judgment can be made that most of the prompt fluorescence observed initially when dark-adapted chloroplasts are first illuminated is “dead,” coming from chlorophyll not associated with trap II. The live fluorescence is represented almost entirely by the time-varying component that develops during illumination. The observed intensity of delayed fluorescence can be divided by the yield of live prompt fluorescence to give an intrinsic delayed fluorescence. This intrinsic delayed fluorescence is proportional to the square root of exciting light intensity (as long as the excitation is not saturating) and decays with second order kinetics. This behavior may reflect the photochemical formation and second order dissipation of an oxidized product of Photosystem II.     

The Photo-oxidation of Epinephrine by Spinach Chloroplasts and Its Inhibition by Superoxide Dismutase: Evidence for the Formation of Superoxide Radicals in Chloroplasts

The thiobarbituric acid (TBA) test for detecting lipid hydroperoxides does not require for fomation of TBA reacting compounds from hydroperoxides, but oxygen has an unfavorable effect, that is, it forms new hydroperoxides during the reaction when unoxidized lipids co-exist. Therefore, a method using a vacuum reaction tube was proposed.     

Light-induced ATP release from the lens

The recent discovery of the photoreceptor melanopsin in lens epithelial cells has opened the possibility of modulating this protein by light stimulation. Experiments carried out on New Zealand white rabbits have demonstrated that the release of ATP from the lens to the aqueous humor can be reduced either when a yellow filter or a melanopsin antagonist is used. Compared to control (1.10?±?0.15 μM ATP), the application of a yellow filter (λ465–480) reduced ATP in the aqueous humor 70%, while the melanopsin antagonist AA92593 reduced the presence of ATP 63% (n?=?5), an effect which was also obtained with the PLC inhibitor U73122. These results indicate that when melanopsin is blocked either by the lack of light, a filter, or an antagonist, the extracellular presence of ATP is significantly reduced. This discovery may be relevant, on the one hand, because many ocular physiological processes are controlled by ATP and, on the other hand, because it is possible to stimulate ATP release with just light and without using any added substance.     

Electron Transport Reactions in Grana Preparations from Spinach Chloroplasts

Fraction 2 (grana-stack) particles prepared with the French press showed absorbance changes, at room temperature and with sodium ascorbate and methyl-viologen, that were produced by the oxidation of cytochrome b-559. This oxidation was inhibited by 3-(3,4-dichlorophenyl)-1,1-dimethylurea (DCMU) and sensitized by system II of photosynthesis. The oxidation is too slow to account for the rates of the Hill reaction that have been observed with nicotinamide-adenine dinucleotide phosphate (NADP⁺). It appears that this cytochrome is not functioning in the main pathway of electron transport. In the presence of 2,3,5,6-tetramethyl-p-phenylene-diamine (DAD) and ascorbate, light-induced oxidation of cytochrome f took place within 3 msec (or faster) in the grana-stack particles. Treatment with the detergent Triton X-100 disrupted this rapid cytochrome f oxidation as well as the oxidation of cytochrome b-559. Subsequent plastocyanin addition did not restore the rapid oxidation of cytochrome f (nor of cytochrome b-559) but only slow changes of cytochrome f. In view of the fact that these particles contain almost no plastocyanin, it is unlikely that plastocyanin functions in electron transport between cytochrome f and P-700 in the particles derived from the grana-stack regions of the chloroplast.     

ADP binding and ATP synthesis by reconstituted H-ATPase from chloroplasts

The H⁺-ATPase from chloroplasts, CF₀F₁, was isolated, purified and reconstituted into asolectin liposomes. The enzyme was brought either into the oxidized state or into the reduced state, and the rate of ATP synthesis was measured after energisation of the proteoliposomes with an acid—base transition ΔpH (pH_in = 5.0, pH_out = 8.5) and a K⁺/valinomycin diffusion potential, Δφ (K⁺_in = 0.6 mM, K⁺_out = 60 mM). A rate of 250 s⁻¹ was observed with the reduced enzyme (85 s⁻¹ in the absence of Δφ). A rate of 50 s⁻¹ was observed with the oxidized enzyme under the same conditions (15 s⁻¹ in the absence of Δφ). The reconstituted enzyme contained 2 ATP_bound per CF₀F₁ and 1 ADP_bound per CF₀F₁. Upon energisation the enzyme was activated and 0.9 ADP per CF₀F₁, was released. Binding of ADP to the active reduced enzyme was observed under different conditions. In the absence of phosphate the rate constant for ADP binding was 10⁵ M⁻¹·s⁻¹ under energized and de-energized conditions. In the presence of phosphate the rate of ADP binding drastically increased under energized conditions, and strongly decreased under de-energized conditions.     

Isolation and Characterization of Phosphatase from Thylakoid Membranes of Spinach Chloroplasts

A phosphatase from thylakoid membrane of spinach (Spinacia oleracea L. ) chloroplasts was isolated with the methods of extraction with n-ButanoL centrifugation at 100000 g for 30 min and chromatographic separation through DEAE-Cellulose (DE 52) column.The phosphatase catalyzed hydrolysis of phosphate monoesters (4-nitrophenyl phosphate). The optimal pH for enzyme catalysis was below 7. The peak rate of the enzyme reaction was obtained when it was incubated at 60℃ for 15 min. The phosphatase was inhibited by ATP and phosphate. The results from SDS-PAGE showed that the preparation of enzyme was composed of two proteins.     

Nonmitochondrial ATP/ADP Transporters Accept Phosphate as Third Substrate

Chlamydiales and Rickettsiales as metabolically impaired, intracellular pathogenic bacteria essentially rely on “energy parasitism” by the help of nucleotide transporters (NTTs). Also in plant plastids NTT-type carriers catalyze ATP/ADP exchange to fuel metabolic processes. The uptake of ATP^4-, followed by energy consumption and the release of ADP^3-, would lead to a metabolically disadvantageous accumulation of negative charges in form of inorganic phosphate (P_i) in the bacterium or organelle if no interacting P_i export system exists. We identified that P_i is a third substrate of several NTT-type ATP/ADP transporters. During adenine nucleotide hetero-exchange, P_i is cotransported with ADP in a one-to-one stoichiometry. Additionally, P_i can be transported in exchange with solely P_i. This P_i homo-exchange depends on the presence of ADP and provides a first indication for only one binding center involved in import and export. Furthermore, analyses of mutant proteins revealed that P_i interacts with the same amino acid residue as the γ-phosphate of ATP. Import of ATP in exchange with ADP plus P_i is obviously an efficient way to couple energy provision with the export of the two metabolic products (ADP plus P_i) and to maintain cellular phosphate homeostasis in intracellular living “energy parasites” and plant plastids. The additional P_i transport capacity of NTT-type ATP/ADP transporters makes the existence of an interacting P_i exporter dispensable and might explain why a corresponding protein so far has not been identified.Most organisms possess the capacity to resynthesize the fundamental energy currency ATP by fusion of ADP and P_i. Generally, in eukaryotes the major part of energy is produced in specialized organelles, the mitochondria. Mitochondrial ADP/ATP carriers (AACs)² mediate the export of newly synthesized ATP in strict counter-exchange with cytosolic ADP and therefore provide energy to the cellular metabolism (1). Plants additionally generate high amounts of ATP during photosynthesis in chloroplasts. However, under conditions of limiting or missing photosynthetic activity, plant plastids depend on external energy supply (2–4). Specific nucleotide transporters (NTTs) located in the inner plastid envelope membrane mediate the required energy import (5). These transporters structurally, functionally, and phylogenetically differ from mitochondrial AACs. They catalyze the import of cytosolic ATP in exchange with stromal ADP, are monomers consisting of 12 predicted transmembrane helices, and are related to the functionally heterogeneous group of bacterial NTTs (5).Although most prokaryotic organisms are able to regenerate ATP and therefore are considered as energetically self-sustaining, the obligate intracellular living bacterial orders Chlamydiales and Rickettsiales are impaired in energy and nucleotide synthesis or even completely lost the corresponding pathways (6–8). Therefore, these bacteria, which comprise important human pathogens (9, 10), essentially rely on nucleotide and energy import. Bacterial NTTs catalyze the required import of a broad range of nucleotides and NAD or facilitate the counter-exchange of ATP and ADP (5, 11–15). The latter process has been termed “energy parasitism” and obviously is of high importance for the survival of rickettsial and chlamydial cells (5, 16–18).Although import measurements on intact Escherichia coli cells expressing the corresponding proteins allowed characterization of many bacterial and plastidial NTTs (12–15, 19–24), a very important physiological question is still not clarified. The uptake of ATP^4- in exchange with ADP^3- in absence of a concerted P_i export would result in a charge difference and a phosphate imbalance in the bacterial cell. In mitochondria, phosphate carriers metabolically cooperate with AACs because they provide P_i for ATP synthesis (25). Similarly, it was assumed that NTT-type ATP/ADP transporters cooperate with phosphate exporters to guarantee phosphate homeostasis in the bacterium or plastid. However, a P_i exporter interacting with ATP/ADP transporters is not known in “energy parasites” or plant plastids. Bacterial and plant phosphate transport systems rather facilitate P_i import or the counter-exchange of P_i and phosphorylated compounds and therefore do not allow net P_i export (26–29). Furthermore, the newly identified plastidial (proton-driven) phosphate transporters are not preferentially expressed under conditions or in tissues that require ATP provision to the plastid (30, 31).Recently, we succeeded in the purification of the first recombinant NTT from Protochlamydia amoebophila (PamNTT1), a parachlamydial endosymbiont of the protist Acantamoeba (32). The functional reconstitution of the highly pure PamNTT1 into artificial lipid vesicles for the first time allowed the biochemical characterization of a representative nonmitochondrial ATP/ADP transporter unaffected by the complex metabolic situation of the bacterial cell. We demonstrated that in contrast to mitochondrial AACs, PamNTT1 catalyzes a membrane potential independent, electroneutral adenine nucleotide hetero-exchange (32, 33). The latter could argue for a cotransport of a counterion compensating for the electrogenic ATP^4-/ADP^3- exchange.Here, we investigated possible ions accompanying ATP or ADP transport. Interestingly, we uncovered that PamNTT1 and also rickettsial and plastidial ATP/ADP transporters accept an additional important substrate, which is P_i. We performed a comprehensive characterization of the P_i transport and gained new insights into the transport properties of ATP/ADP transporters.     

Hydrogen Peroxide is Scavenged by Ascorbate-specific Peroxidase in Spinach Chloroplasts

Intact spinach chloroplasts scavenge hydrogen peroxide witha peroxidase that uses a photoreductant as the electron donor,but the activity of ruptured chloroplasts is very low [Nakanoand Asada (1980) Plant & Cell Physiol. 21 : 1295]. Rupturedspinach chloroplasts recovered their ability to photoreducehydrogen peroxide with the concomitant evolution of oxygen afterthe addition of glutathione and dehydroascorbate (DHA). In rupturedchloroplasts, DHA was photoreduced to ascorbate and oxygen wasevolved in the process in the presence of glutathione. DHA reductase(EC 1.8.5.1 [EC] ) and a peroxidase whose electron donor is specificto L-ascorbate are localized in chloroplast stroma. These observationsconfirm that the electron donor for the scavenging of hydrogenperoxide in chloroplasts is L-ascorbate and that the L-ascorbateis regenerated from DHA by the system: photosystem IferredoxinNADPglutathione.A preliminary characterization of the chloroplast peroxidaseis given. (Received April 16, 1981; Accepted June 3, 1981)