CHLOROPHYLL PHOTOSENSITIZED ELECTRON TRANSFER REACTIONS IN LIPID BILAYER VESICLES: VECTORIAL ELECTRON TRANSFER ACROSS THE BILAYER FROM REDUCED CYTOCHROME c IN THE INNER COMPARTMENT TO OXIDIZED FERREDOXIN IN THE OUTER COMPARTMENT

A negatively charged large unilamellar vesicle system containing a membrane-bound photo-sensitizer (chlorophyll, Chi), a reduced redox protein [cytochrome c, cyt c(red)] in the inner aqueous compartment, an oxidized redox protein [ferredoxin, Fd(ox)] in the outer aqueous compartment, and propylene diquat (PDQ²⁺) as a mediator, was investigated using both flash and steady-state photolysis techniques. The results demonstrate that the light-generated triplet state of Chi (³Chl) was initially quenched by PDQ²⁺ at the outer membrane surface to form Chi cation radical (Chl⁺) and the reduced diquat (PDQ⁺). This was succeeded by a biphasic recombination between Chi⁺ and PDQ⁺. The slow phase of the recombination process, which represents reverse electron transfer between Chl⁺ and those PDQ⁺ molecules which escaped from the membrane surface, could be suppressed effectively both by the reduction of Chl^ in the inner monolayer of the vesicles by cyt c(red), and by the reoxidation of PDQ⁺ by Fd(ox) in the outer aqueous compartment. These reactions lead to the permanent accumulation of oxidized and reduced product proteins, i.e. cyt c(ox) in the inner compartment and Fd(red) in the outer compartment. The yields of such accumulation were 11%, based on the ³Chl quenched, and 1.4%, based on absorbed quanta, under the conditions used in the present study. This system mimics one of the key events in natural photosynthesis and results in an appreciable storage of electromagnetic energy in the reaction products.     

KINETICS OF CHLOROPHYLL PHOTOSENSITIZED ELECTRON TRANSFER REACTIONS IN PHOspHOLIPID BILAYER VESICLES

Abstract The effects of electrostatic surface charge and valinomycin addition in the presence of K* on the kinetics and the inside-outside asymmetry properties of light-induced electron transfer reactions between chlorophyll triplet state and benzoquinone, ferricyanide and methyl viologen in large unilamellar vesicles have been investigated using laser flash photolysis. Modifying the surface charge of the bilayers by incorporating charged surfactants or decreasing the ionic strength of the suspending medium caused large changes in the dynamics of the electron transfer reactions, which could be interpreted in terms of electrostatic interactions between reactants, products and membrane components, and the existence of a spontaneous transmembrane electrical potential corresponding to an excess of negative charge at the outer surface of the vesicle bilayer. The presence of valinomycin had more specific effects on these reactions, which were consistent with an electrostatic influence of the presence of the positively-charged K⁺-valinomycin complex within the bilayer on the dynamics of only those triplet quenching and radical formation and decay processes which occur in this region of the vesicle structure.     

CHLOROPHYLL PHOTOSENSITIZED ELECTRON TRANSFER REACTIONS IN LIPID BILAYER VESICLES: GENERATION OF PROTON GRADIENTS ACROSS THE BILAYER COUPLED TO QUINONE REDUCTION AND HYDROQUINONE OXIDATION

Abstract— A chlorophyll-containing small unilamellar lipid bilayer vesicle system with a sulfonated quinone molecule (MQS) in one aqueous compartment and a sulfonated hydroquinone molecule (H₂QS) in the other has been investigated, using laser flash photolysis and steady-state irradiation, as a means of storing light energy in the form of a proton gradient across the lipid bilayer. Under optimal conditions, an efficiency of 39% based on the chlorophyll triplet state quenched has been achieved for vectorial electron transfer across the bilayer; this corresponds to a quantum yield of 23% based on absorbed photons. As a consequence of irradiation by a single laser flash, 0.2 μ M of protons were taken up by quinone reduction (MQS → H₂MQS) in the outer compartment. The same number of protons were released in the inner compartment by hydroquinone oxidation (H₂QS → QS). Since the volume occupied by the vesicles was only 1/1000 of the total volume of the sample, the local concentration of protons in the inner compartment was 1000 times larger ( i.e. ≅ 200 μ M ), resulting in the generation of an appreciable proton gradient across the bilayer.     

QUINONES AS MEDIATORS OF ELECTRON TRANSFER FROM MEMBRANE-BOUND CHLOROPHYLL TO CYTOCHROME c IN THE AQUEOUS PHASE IN LIPID BILAYER VESICLES: SYNERGISTIC ENHANCEMENT OF CYTOCHROME c REDUCTION BY LIPOPHILIC/ HYDROPHILIC QUINONE PAIRS

Laser flash photolysis has been used to determine the kinetics of cytochrome c reduction by chlorophyll triplet state in negatively-charged lipid bilayer vesicles, as mediated by quinones. Large synergistic enhancements in the yield of reduced cytochrome were obtained using a pair of quinones, one of which was lipophilic (e.g. benzoquinone, 2,6-di-f-butylbenzoquinone) and the other of which was hydrophilic (e.g. l,2-naphthoquinone-4-sulfonate). The mechanism was shown to involve initial quenching of the triplet by the membrane-associated quinone to form chlorophyll cation radical and quinone anion radical. An interquinone electron transfer process followed this reaction, which occurred at the membrane-water interface, and greatly facilitated electron transport from within the bilayer to the aqueous phase. This process formed the basis of the synergistic effect. Cytochrome c reduction occurred in the water phase by reaction with the anion radical of the hydrophilic quinone. Finally, the reduced cytochrome was reoxidized by a slow reaction with chlorophyll cation radical. Under the most favorable conditions, we estimate that the quantum yield of conversion of triplet quenching events to reduction of cytochrome approached unity. The lifetime of the reduced protein and oxidized chlorophyll could be as long as 140 ms, under the best conditions. This system has properties which are thus quite favorable for solar energy conversion in a biomimetic process.     

HORSE HEART CYTOCHROME c AS AN ELECTRON ACCEPTOR FROM CHLOROPHYLL TRIPLET IN NEGATIVELY CHARGED LIPID BILAYER VESICLES*

Abstract— Cytochrome c has been shown to bind via electrostatic interactions to egg phosphatidylcholine vesicles which contain 5–30 mol percent of negatively-charged surfactant (dihexadecylphosphate) in a low ionic strength medium. Under these conditions the oxidized cytochrome can function as a direct one-electron acceptor from membrane-bound triplet state chlorophyll to produce chlorophyll cation radical and reduced cytochrome. Kinetic experiments using laser flash photolysis have demonstrated that triplet quenching and the yield of electron transfer products increase, and product lifetime decreases, with an increase in the magnitude of the negative charge on the vesicles, and with a decrease in the ionic strength of the medium. Both triplet quenching and product formation rates and yields showed saturation behavior as the cytochrome concentration was increased, and reached limiting values at 20–30 μM cytochrome when the vesicle contained 20 mol percent of the negatively-charged surfactant. This behavior is interpreted in terms of saturation of the vesicle surface binding sites. Under optimum conditions in this system, approximately 20% of the chlorophyll triplet molecules could be converted to electron transfer products which had a halftime for the reverse reaction of approximately 1.5 ms.     

VECTORIAL ELECTRON TRANSPORT ACROSS LIPID VESICLE MEMBRANES DRIVE BY TWO PHOTOREACTIONS. II. PHOTOCHEMICAL REGENERATION OF REDUCED CYTOCHROME c BY FLAVIN TRIPLET STATE AND ETHYLENEDIAMINETETRAACETIC ACID IN THE INNER COMPARTMENT AND REDUCTION OF FERREDOXIN BY CHLOROPHYLL TRIPLET STATE IN THE OUTER COMPARTMENT

We have attempted to mimic natural photosynthesis with regard to the photogeneration of a powerful reductant, using a negatively charged lipid bilayer vesicle system incorporating two photoreactions sensitized by a flavin analog (flavin mononucleotide [FMN]) and chlorophyll (chl) in their respective triplet states. Ethylenediamine-tetraacetic acid (EDTA) in the inner aqueous compartment was used as a sacrificial electron donor to the FMN triplet, and ferredoxin in the outer aqueous compartment served as the final electron acceptor (mediated via triplet electron transfer chain in this multicomponent system to be elucidated. By itself, EDTA does not function as an effective donor to membran-bound oxidized chl (chl^+.), which is formed by electron transfer from triplet chl to the viologen follwed by transbilayer electron migration. This is a consequence of electrostatic repulsive interactions with the negatively charged membrane. This limitation is avoided when FMN is used as a photomediator between EDTA and chl^+.. The overall reaction is dramatically increased in rate by enclosing cytochrom c together with EDTA and FMN in the inner compartment. The rate constant of the key step in the reaction, i.e. elctron transfer from reduced cytochrome c, generated via photoreduction by the FMN/EDTA system, to chl^+. is increased 20-fold over that obtained with cytochrome c alone as the elctron donor. One of the important constraints that limited the net electron transfer across the bilayer to 50% of the added cytochrome, i.e. inhibition by oxidized cytochrome c formed in the inner compartment, is avoided by the inclusion of the second photoreaction in this system, thus allowing photoreduction of all of the added ferredoxin to be achieved. This system provides a model for a photochemical energy storage process that utilizes two photorections operating in series resulting in electron flow across a lipid bilayer membrane.     

REDOX PROTEINS AS ELECTRON ACCEPTORS FROM CHLOROPHYLL TRIPLET STATE IN LIPID BILAYER VESICLES: KINETICS OF REDUCTION OF MEMBRANE RECONSTITUTED CYTOCHROME c OXIDASE MEDIATED BY 2,5-DI-t-BUTYL BENZOQUINONE AND CYTOCHROME c

Laser flash photolysis was used to determine the kinetics of electron transfer between membrane-bound triplet chlorophyll (3C), cytochrome c (cyt c) located in the external water phase, and vesicle-reconstituted cytochrome c oxidase (CCO). 2,5-Di-t-butyl benzoquinone (2,5 TBQ) was used as an electron transfer mediator between 3C and cyt c. A light-induced cyclic electron transfer sequence between the redox components was observed (3C----2.5 TBQ----cyt c----CCO----C+.). Under optimum conditions of membrane surface charge and ionic strength, the overall efficiency of CCO reduction (based on 3C generated by the laser flash) was 14%. Under the anaerobic conditions used, CCO reoxidation (occurring via electron transfer to C+.) was quite slow (halftime approx. 1 s at 75 mM ionic strength). The multicomponent system displayed a high level of stability, as indicated by its ability to undergo many cycles of reduction and reoxidation without any apparent degradation of the components. These results demonstrate the feasibility of constructing complex electron transfer chains, including both soluble and membrane-bound redox proteins, in artificial lipid bilayers, whose properties can be readily controlled by manipulating parameters such as ionic strength and membrane composition.     

ELECTRON TRANSFER REACTIONS OCCURRING UPON LASER FLASH PHOTOLYSIS OF PHOSPHOLIPID BILAYER SYSTEMS CONTAINING CHLOROPHYLL,BENZOQUINONE AND CYTOCHROME c-I. NEGATIVELY-CHARGED VESICLES*

Abstract— In negatively-charged lipid bilayer vesicles prepared in deionized water from egg phosphatidylcholine and 25 mol % of α-eleostearic acid, and containing chlorophyll a, benzoquinone, and cytochrome c, primary electron transfer after a laser flash occurred principally from chlorophyll triplet to benzoquinone, and to a smaller extent from chlorophyll triplet to oxidized cytochrome c. Several secondary electron transfer reactions occurred subsequent to this. The most rapid of these was electron transfer from reduced cytochrome c, which was bound to the outer surface of the negatively-charged vesicle, to chlorophyll cation radical (k= 3.9 times 10³ s^-1). Subsequent to this, the cation radical was reduced by benzoquinone anion radical (k= 1.6 times 10² s^-1>) and bound oxidized cytochrome c was reduced by the remaining anion radical which was expelled into the aqueous phase by the negative charge on the vesicle surface. This latter reaction occurred at the membrane-solution interface with an observed rate constant (k= 60 s^-1) two orders of magnitude smaller than cytochrome oxidation. Net reduced cytochrome c was produced in this process. The reduced cytochrome c was slowly reoxidized by benzoquinone (k= 17 s^-1) and the system was returned to its original state. When the vesicle system was made slightly basic by adding tris(hydroxymethyl)aminomethane, the rates of both the reverse electron transfer between chlorophyll cation radical and benzoquinone anion radical (k= 5 times 10² s^-1) and the oxidation of reduced cytochrome c by chlorophyll cation radical (k= 9.4 times 10³ s^-1) were accelerated. The rate of reduction of oxidized cytochrome c by benzoquinone anion radical remained approximately the same.     

SPINACH PLASTOCYANIN AS AN ELECTRON ACCEPTOR FROM MEMBRANE-BOUND CHLOROPHYLL TRIPLET STATE IN POSITIVELY CHARGED LIPID BILAYER VESICLES*

Spinach plastocyanin is bound to egg phosphatidylcholine vesicles containing 5–25 mole percent dioctadecyldimethylammonium chloride (DODAC) via electrostatic interactions in a 50 mM betaine medium (pH=6.5). This was demonstrated by both gel filtration experiments and kinetic results using laser flash photolysis. Under those conditions, oxidized plastocyanin can function as a direct electron acceptor from membrane-bound triplet chlorophyll to produce chlorophyll cation radical and reduced plastocyanin. The fraction of chlorophyll triplet which is quenched by oxidized plastocyanin increases, and the yield of electron transfer products also increases, with an increase in the magnitude of the positive charge on the vesicles. Product decay and rise halftimes decrease with an increase in the mole percent of DODAC⁺ incorporated into egg phosphatidylcholine vesicles. However, both of these halftimes are independent of oxidized plastocyanin concentration. Even though ～50% of the Chi triplets were quenched, no electron transfer product formation was observed in 5 mM phosphate buffer (pH=7.0). Under similar conditions in betaine, approximately 13% of the Chi triplets could be converted into products.     

ELECTRON TRANSFER REACTIONS OCCURRING UPON LASER FLASH PHOTOLYSIS OF PHOSPHOLIPID BILAYER SYSTEMS CONTAINING CHLOROPHYLL,BENZOQUINONE AND CYTOCHROME c-II. ELECTRICALLY NEUTRAL AND POSITIVELY-CHARGED VESICLES*

Abstract— The primary and secondary electron transfer reactions which occurred upon laser flash photolysis of electrically neutral and positively-charged lipid bilayer vesicles containing chlorophyll, benzoquinone and cytochrome c were determined by time-resolved difference spectral and kinetic measurements, and compared with previous results obtained with negatively-charged vesicles (Y. Fang and G. Tollin, Photochem. Photobiol. 1988). The extent to which oxidized cytochrome c could function as an electron acceptor from triplet state chlorophyll, and reduced cytochrome c could act as an electron donor to chlorophyll cation radical, decreased from negatively-charged to electrically neutral to positively-charged vesicles, in agreement with expectations based on changes in the ability of cytochrome c to bind to the bilayer. In all three types of vesicles, cytochrome c reduction by benzoquinone anion radical occurred in the aqueous phase.     

CHLOROPHYLL PHOTOSENSITIZED ELECTRON TRANSFER IN PHOSPHOLIPID BILAYER VESICLE SYSTEMS: EFFECTS OF CHOLESTEROL ON RADICAL YIELDS AND KINETIC PARAMETERS*

Abstract The quenching of the triplet state of chlorophyll a (Chl) by asymmetrically located electron acceptors was examined in vesicle systems containing egg yolk phosphatidylcholine and 0–50 mole % cholesterol. The incorporation of cholesterol had two main effects: (1) the distribution of Chl within the vesicle wall shifted from one favoring the inner monolayer to one favoring the outer monolayer, and (2) the Chi molecules (both ground and excited states) became more accessible to water and to the quencher molecules. This latter property was probably due to the creation of space between the phospholipid head groups by insertion of cholesterol. These phenomena required cholesterol concentrations in excess of 15 mol %. In general, the addition of cholesterol caused increases in the apparent bimolecular rate constant for triplet quenching, in the probability that quenching produced radicals, and in the rate of radical recombination. Some of the specific effects of cholesterol depended upon whether or not the quencher molecules were amphiphilic.     

CHLOROPHYLL PHOTOSENSITIZED ELECTRON TRANSFER IN PHOSPHOLIPID BILAYER VESICLE SYSTEMS: CORRELATIONS BETWEEN KINETIC PARAMETERS AND SOLUBILITIES OF VIOLOGEN ACCEPTORS *

Abstract— Twelve viologens (quaternary 4,4′-bipyridinium ions) are investigated as electron acceptors in vesicle suspensions containing chlorophyll-a (Chl) using laser flash photolysis. The structures of the viologens, which determine how they and their reduced radicals partition between the water and bilayer membrane phases, are systematically varied in order to probe the effects of acceptor solubility on the kinetics of photosensitized electron transfer reactions. The effectiveness of the viologens as quenchers of the Chl triplet excited state increases as they become less soluble in water, because the viologens are more likely to be incorporated into the membrane, but the efficiency of radical formation decreases and the rate of the reverse electron transfer reaction increases. The data obtained with a homologous series of di-alkyl viologens are analyzed quantitatively using a kinetic model which includes the partition coefficients of the viologens and their radicals. For the most part, the reactivities of the viologen species are proportional to their concentrations in the membrane phase, but the locations and mobilities of the viologens in the membrane phase also have to be considered. In order for the Chl and viologen radicals to separate efficiently. the viologen radical has to be able to diffuse from the membrane to the water phase at a rate that competes effectively with reverse electron transfer within the radical pair complex (> 10⁵ s^?1).     

CHLOROPHYLL PHOTOSENSITIZED ELECTRON TRANSFER IN PHOSPHOLIPID VESICLE SYSTEMS: COMPARISON OF INSIDE-OUTSIDE ASYMMETRY BETWEEN LARGE AND SMALL UNILAMELLAR VESICLES*

Abstract— We have determined the chlorophyll triplet quenching efficiencies, the chlorophyll cation radical yields and the conversion efficiencies of chlorophyll triplet to radical in large and small unilamellar phosphatidylcholine vesicles (LUV and SUV, respectively) in the presence of electrically-charged electron acceptors (ferricyanide and oxidized cytochrome c) located in either the inner or outer aqueous compartments of the vesicles. Both types of vesicles displayed inside-outside asymmetry, although the properties were reversed. Triplet quenching in SUV was more efficient when ferricyanide was located within the vesicle interior, whereas the reverse was true in LUV. When ferricyanide was located on the outside of the vesicles, the extent of triplet quenching in LUV was about two times that in SUV and the amount of cation radical formed in LUV was about two times that in SUV. Under these conditions, the conversion efficiencies of chlorophyll triplet to radical were 12.2% for LUV and 8.5% for SUV. With cytochrome c as an electron acceptor in negatively charged vesicles (25 mol per cent dixhexadecylphosphate incorporated) similar results were obtained. Again, the triplet quenching and radical yield inside-outside asymmetry properties were reversed between the two types of vesicles, and radical formation efficiencies when cyt c was located outside the vesicles were higher in LUV (11.7%) than in SUV (4.2%). We conclude that the inside-outside asymmetric photochemical behavior of unilamellar phosphatidylcholine vesicles is influenced by factors in addition to the difference in radius of curvature between the inside and outside surfaces. It is suggested that transmembrane electrostatic potentials may be involved. Furthermore, in the present system the properties of LUV were more favorable to photochemical electron transfer product formation than those of SUV.     

VECTORIAL ELECTRON TRANSPORT ACROSS LIPID VESICLE MEMBRANES DRIVEN BY TWO PHOTOREACTIONS. I. ETHYLENEDIAMINETETRAACETIC ACID AS AN ELECTRON DONOR via FLAVIN TRIPLET STATE IN THE INNER COMPARTMENT AND CYTOCHROME c AS AN ELECTRON ACCEPTOR FROM CHLOROPHYLL TRIPLET STATE IN THE OUTER COMPARTMENT

Negatively charged vesicle suspensions containing chlorophyll a (chl) dissolved in the lipid bilayer, flavin mononucleotide (FMN) and/or ethylenediaminetetraacetic acid (EDTA) enclosed in the inner compartment as electron sources and oxidized cytochrome c (cyt c[ox]) in the outer compartment as an electron acceptor have been studied using laser flash photolysis and steady-state irradiation methods. Cytochrome c initially quenches the chl triplet state (³chl) generating the chlorophyll cation radical (chi⁺′) in the membrane. Reverse electron transfer from cyt c(red) to chl^+. subsequently occurs in a kinetically biphasic reaction, with rate constants of 430 pT 30 and 21.9 pT 1.7 s^?1 for the fast and slow phases, respectively. In the absence of FMN, reduction of chl⁺′ by EDTA in the inner compartment can be observed during steady-state irradiation but not in a laser flash photolysis experiment. This is due to a low reaction yield, which is probably limited by the repulsive electrostatic interaction between EDTA and the negatively charged membrane. When FMN was enclosed together with EDTA in the inner Compartment, the reaction yield of vectorial electron transfer across the bilayer from EDTA to cyt c(oX) was increased by a factor of six during steadystate white light irradiation. Laser flash photolysis and steady-state irradiation experiments using red and blue light excitation have demonstrated that the enhancement mechanism involves the formation of fully reduced FMN by blue light-sensitized photooxidation of EDTA via the flavin triplet state, occumng simultaneously with red lightsensitized electron transfer to cyt c via the chlorophyll triplet state.     

DIRECT OBSERVATION OF ELECTRON TRANSFER ACROSS A LIPID BILAYER: PULSED LASER PHOTOLYSIS OF AN ASYMMETRIC VESICLE SYSTEM CONTAINING CHLOROPHYLL,METHYL VIOLOGEN AND EDTA*

Abstract— Suspensions of vesicles composed of chlorophyll a (Chi) and phospholipid that were asymmetric with respect to aqueous solutions of methyl viologen (MV₂₊), an electron acceptor, and EDTA, an electron donor, were investigated using both flash and steady-state photolysis techniques. It was shown that Chl-photosensitized electron transfer occurred across the walls of the vesicles from EDTA to MV₂₊. Flash photolysis indicated that MV₂₊ dissolved in the interior aqueous compartments of the vesicles oxidized only those triplet excited state Chi molecules that were dissolved in the inner monolayers of the vesicle walls. The resultant radical products, Chi₊ and MV₊, recombined with a halftime of the order of 10_-4s. EDTA, added externally to the vesicles, competed effectively with MV₊ as a reducing agent for Chl₊. This places a lower limit of 10₄ s_-1 on the rate constant for transmembrane electron transfer. Compartmentalization by the vesicle wall of the competing pathways for the reduction of Chi₊ resulted in a nonlinear dependence of the rate constant of Chl₊ decay on EDTA concentration. The magnitude of the rate constant of electron transfer through the membrane and the way that the kinetics of Chl₊ decay depended on the concentration of Chi in the membrane strongly suggest that the electron transfer occurred by electron exchange between Chi and Chl₊.     

THE USE OF LIPID HEADGROUP CHARGE TO ENHANCE PHOTOINDUCED ELECTRON TRANSFER IN VESICLES: REACTIONS OF FUNCTIONALIZED PYRENE WITH A TWO COMPONENT VIOLOGEN SYSTEM

Abstract—
Kinetics of photoinduced electron transfer from a lipid functionalized pyrene, 1-(10-(6(8)-octadecylpyrenyl)decanoyl)-2-hexanoyl-.sn-glycero-3-phosphorylcholine (OPyPC), to a two component viologen acceptor system have been measured by laser flash photolysis. N, N'-tetramethylene-2,2'-bi-pyridinium ion (DQ²⁺) and N, N' -dipropyl-4,4'-bipyridinium sulfonate (PVS), have been utilized as the primary and secondary acceptors. It has been shown that utilization of a lipid with a net negatively charged phosphatidylglycerol headgroup provides a driving force for localizing high concentrations of primary acceptor (DQ²⁺) in the region of donor. Subsequently, the charged interface can act to maintain long-term separation between the oxidized pyrene donor (OPyPC⁺) and the reduced secondary acceptor, PVS^-. When a dioleoyl lipid is used, reaction of (OPyPC⁺) with the double bond competes significantly with back reaction. However, substitution of diphytylphosphatidylglycerol for the dioleoyl analog results in a cation lifetime of about 0.5 ms and a continued very long-lived reduced species (˜4 h). Quantum yields of ˜0.15 may be obtained in this system.     

LIGHT-INDUCED ELECTRON TRANSFER REACTIONS BETWEEN CHLOROPHYLL AND QUINONE IN ELECTRICALLY-CHARGED VESICLES: EFFECTS OF COUNTERIONS LOCATED IN EITHER THE INNER OR OUTER AQUEOUS PHASES ON RADICAL FORMATION AND DECAY*

Abstract— The presence of relatively low concentrations of counterions (millimolar in the case of univalent ions and micromolar in the case of polyvalent ions) in either the inner or outer aqueous compartments of electrically charged lipid bilayer vesicles containing chlorophyll in the presence of benzoquinone has been shown to produce large effects on radical formation and decay as measured by laser flash photolysis. With negatively charged vesicles having no added salt inside, salt ions added to the external phase caused radical yields to markedly decrease, with no change in decay kinetics. When salt was present only in the interior phase, radical decay became biphasic and the ability of externally added salt to affect radical yields was greatly diminished. With positively charged vesicles having no added salt inside, salt addition to the external medium caused both the radical decay rate and yield to decrease. The presence of interior salt, however, caused radical decay to become faster and, as was the case with negative vesicles, greatly reduced the effects of salt added externally. These results have been interpreted in terms of electrostatic and structural effects of charge neutralization by counterions on the dynamics of radical-ion separation and recombination.     

CHLOROPHYLL PHOTOSENSITIZED ELECTRON TRANSFER IN PHOSPHOLIPID BILAYER VESICLE SYSTEMS: SECONDARY OXIDATION OF REDUCED VIOLOGEN ACCEPTORS BY Ru(NH3)63+

Abstract— The kinetics of the oxidation of a homologous series of 4,4'-di(n-alkyl)-bipyridinium (viologen) radicals by Ru(NH₃)₆³⁺ in vesicle suspensions was studied using laser flash photolysis. The viologen radicals were produced photochemically in the bilayer membrane phase of the vesicles by electron transfer from the triplet state of chlorophyll-α. At high concentrations of Ru(NH₃)₆³⁺, the rate of oxidation of the viologen radicals in the aqueous phase was limited by the rate at which the radicals diffused from the membrane to the aqueous phase. The exit rate constant decreased from 2 × 10⁵ s⁻¹ for the methyl viologen radical to 4 × 10³ s⁻¹ for the pentyl viologen radical. Both the exit rate constants and the calculated values for the equilibrium association constants of the viologen radicals were unexpectedly insensitive to the length of their alkyl substituents. This, as well as other data, suggests that the radicals that diffused into the aqueous phase tended to remain associated with the membrane-water interface.