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Electric-Field Dependent Decays of Two Spectroscopically Different M-States of Photosensory Rhodopsin II from Natronobacterium pharaonis

Laura Rivas ^*, Silke Hippler-Mreyen , Martin Engelhard  and Peter Hildebrandt ^* 

^* Instituto de Tecnologia Química e Biológica, Universidade Nova de Lisboa, P-2781-901 Oeiras, Portugal; Max-Planck-Institut für Molekulare Physiologie, D-44227 Dortmund, Germany; and Technische Universität Berlin, Institut f. Chemie, D-10623 Berlin, Germany

Correspondence: Address reprint requests to Peter Hildebrandt, Tel.: +49-30-314-21419; Fax: +49-30-314-21122; E-mail: hildebrandt{at}chem.tu-berlin.de.

	ABSTRACT

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Sensory rhodopsin II (NpSRII) from Natronobacterium pharaonis was studied by resonance Raman (RR) spectroscopic techniques. Using gated 413-nm excitation, time-resolved RR measurements of the solubilized photoreceptor were carried out to probe the photocycle intermediates that are formed in the submillisecond time range. For the first time, two M-like intermediates were identified on the basis of their C=C stretching bands at 1568 and 1583 cm^-1, corresponding to the early M(L)₄₀₀ state with a lifetime of 30 µs and the subsequent M(1)₄₀₀ state with a lifetime of 2 ms, respectively. The unusually high C=C stretching frequency of M(1)₄₀₀ has been attributed to an unprotonated retinal Schiff base in a largely hydrophobic environment, implying that the M(L)₄₀₀ M(1)₄₀₀ transition is associated with protein structural changes in the vicinity of the chromophore binding pocket. Time-resolved surface enhanced resonance Raman experiments of NpSRII electrostatically bound onto a rotating Ag electrode reveal that the photoreceptor runs through the photocycle also in the immobilized state. Surface enhanced resonance Raman spectra are very similar to the RR spectra of the solubilized protein, ruling out adsorption-induced structural changes in the retinal binding pocket. The photocycle kinetics, however, is sensitively affected by the electrode potential such that at 0.0 V (versus Ag/AgCl) the decay times of M(L)₄₀₀ and M(1)₄₀₀ are drastically slowed down. Upon decreasing the potential to -0.4 V, that corresponds to a decrease of the interfacial potential drop and thus of the electric field strength at the protein binding site, the photocycle kinetics becomes similar to that of NpSRII in solution. The electric-field dependence of the protein structural changes associated with the M-state transitions, which in the present spectroscopic work is revealed on a molecular level, appears to be related to the electric-field control of bacteriorhodopsin's photocycle, which has been shown to be of functional relevance.

	INTRODUCTION

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Bacteria have evolved intricate mechanisms to respond adequately and efficiently to environmental challenges. Archaea like Halobacterium salinarum or Natronobacterium pharaonis can react toward chemical stimuli as well as toward light. The latter input signal triggers a phototactic transduction pathway which is mediated by two receptors, sensory rhodopsin I (SRI) and sensory rhodopsin II (SRII), which are responsible for directing the bacteria toward favorable light conditions (Spudich and Luecke, 2002; Spudich, 1998; Schäfer et al., 1999). SRI and SRII are structurally closely related to each other and to the two other archaeal rhodopsins, the ion pumps bacteriorhodopsin (BR) and halorhodopsin (HR). All four archaeal pigments contain an all-trans retinal bound to the seven-helix membrane protein via a protonated Schiff base. Whereas BR, HR, and SRI absorb at wavelengths above 560 nm, SRII from H. salinarum has its absorption maximum at around 490 nm. On excitation by light the archaeal rhodopsins undergo characteristic photoreaction cycles, which are coupled to the physiological response, i.e., signal transduction or ion pumping. Sensory rhodopsins from H. salinarum have been sequenced (Blanck et al., 1989; Zhang et al., 1996) and in the case of the photophobic receptor also from the phylogenetically distinct N. pharaonis (NpSRII) (Seidel et al., 1995). The biochemical and physiological properties of NpSRII are quite similar to those of SRII from H. salinarum, as demonstrated in measurements of the photocycle (Scharf et al., 1992).

The photocycle of NpSRII, which has been investigated in a number of studies (Chizhov et al., 1998; Hirayama et al., 1992; Miyazaki et al., 1992; Imamoto et al., 1992), is quite similar to that of BR (Lanyi and Váró, 1995), except that the turnover is slowed down by about two orders of magnitude. Recent work (Chizhov et al., 1998) has shown that the photocycle follows a scheme of irreversible first-order reactions connecting kinetically distinct protein states (P_i; I=1,2,..8). These states are formed from five spectrally distinct species (S_i), namely NpSRII₅₁₀ (K₅₁₀), NpSRII₄₉₅ (L₄₉₅), NpSRII₄₀₀ (M₄₀₀), NpSRII₄₈₅ (N₄₈₅), and NpSRII₅₃₅ (O₅₃₅). On light excitation of the retinylidene chromophore isomerization of all-trans 13-cis occurs, which is followed by thermal relaxations via the archetypical intermediates K, L, M, N, and O back to the original ground state. Accompanying these transitions are proton transfer steps which lead to vectorial proton transfer to the extracellular medium (Schmies et al., 2001). Whereas the first part of the photocycle can be readily explained by the reaction sequence

the second part in which the ground state is re-formed is more complicated as it comprises fast equilibria between the M, N, and O spectral states.

According to this model, the M spectral states are contained in three different protein states (P₃, P₄, P₅) which will be denoted M(L), M(1), and M(2), respectively. In the photocycle of BR the spectrally silent transition between M₁ and M₂ (P₄ P₅) has been correlated to a switch, which alters the accessibility of the Schiff base from the extracellular side to the cytoplasmic side, hence guaranteeing the vectorial transport of protons. A similar protein conformational change, the outward movement of helix F, has also been shown to occur in NpSRII (Wegener et al., 2000).

Vibrational spectroscopy of NpSRII revealed considerable conformational movement already at the early stages of the photocycle (Kandori et al., 2001; Engelhard et al., 1996). The L M transition is accompanied by the protonation of Asp-75 concomitantly with the deprotonation of the Schiff base (Engelhard et al., 1996). Similar experiments on SRII from H. salinarum (HsSRII) led to the same conclusions (Bergo et al., 2000). Resonance Raman (RR) spectroscopic data revealed strong hydrogen bonding interactions of the Schiff base in NpSRII₅₀₀ and in O₅₃₅ which might be one parameter controlling the absorption maxima that are distinctly blue-shifted compared to the corresponding states of other bacterial rhodopsins (Gellini et al., 2000).

In this paper, RR data on the NpSRII photocycle intermediates are presented, which provide evidence of two spectrally distinct M spectral states. Surface enhanced resonance Raman (SERR) experiments indicate that an applied potential sensitively modifies the kinetics of the photocycle.

	MATERIALS AND METHODS

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Samples
Expression and purification of NpSRII is described previously (Hohenfeld et al., 1999; Shimono et al., 1997). The protein was dissolved in solutions containing 1% dodecylmaltoside, 12.5 mM K₂SO₄ and 12.5 mM phosphate buffer (pH 7.0). The NpSRII concentration was 30 µM and 0.1 µM in RR and SERR experiments, respectively.

SERR experiments
RR and SERR spectra were measured at ambient temperature using a spectrograph (U1000) equipped with a liquid nitrogen cooled CCD camera (ISA, D-85360 Grasbrunn, Germany. Unless noted otherwise, the 413-nm excitation line of a Kr⁺-laser (Coherent Innova 302, D-64807 Dieburg, Germany) was employed and the spectral resolution was 4 cm^-1 with an increment per data point of 0.53 cm^-1. Details of the experimental set-up are given elsewhere (Oellerich et al., 2002). In SERR experiments, the laser beam was focused onto the surface of a rotating Ag electrode that was placed into a home-built electrochemical cell containing NpSRII and detergent and the supporting electrolyte. Adsorption of the protein occurred spontaneously at open circuit. The electrochemical cell and the protocol for SERR-activation of the electrode is described elsewhere (Murgida and Hildebrandt, 2001a). All potentials cited in this work refer to the Ag/AgCl electrode.

Time-resolved measurements
The laser beam used for probing the RR and SERR spectra also initiates the photocycle. The degree of photoconversion of the NpSRII during the residence time t in the laser beam is given by

(1)

The mean photochemical rate constant l₀ can be approximated by

(2)

where is the quantum yield of the primary photochemical process and () the extinction coefficient at the excitation wavelength (Lohrmann and Stockburger, 1992). The laser power is denoted by P_L, and r_L refers to the radius of the laser beam. For = 413 nm, the extinction coefficient of the parent state NpSRII₅₀₀ is 15,000 l·mol^-1·cm^-1 (Chizhov et al., 1998). The quantum yield of the primary photoprocess has not yet been determined; however, for the formation of the long-lived intermediate NpSRII₄₀₀, a value of 0.5 was published (Losi et al., 1999). Inserting these values as well as the laser beam radius of 40 µm, as defined according to Lohrmann and Stockburger (1992), into Eq. 9, one obtains

(3)

where P_L is expressed in joules x s.

The residence time of the sample in the laser beam is given by

(4)

where r_c and ₀ are the respective radius and the frequency of the rotating device that is a rotating cell and a rotating electrode in RR and SERR experiments, respectively.

To avoid quasi-photostationary conditions, the NpSRII molecules of the irradiated volume (RR) or surface (SERR) element must be allowed to relax to the parent state before entering the laser beam again. This condition requires that the minimal time interval between irradiation events is larger than the decay time of the longest-lived intermediate. For BR and HR, this requirement can be fulfilled by setting ₀ 50 s^-1, whereas for NpSRII ₀ would have to be kept smaller than 1 s^-1. Such a slow rotation would drastically increase t to 2 ms (Eq. 4), corresponding to a photoconversion parameter l₀t larger than one even at very low laser power (cf. Eq. 1). Under these conditions, a quasi-photostationary equilibrium between the parent state and the primary photoproduct would be formed in the laser beam, and the RR spectrum would include large contributions from intermediate states.

In our previous study on NpSRII (Gellini et al., 2000), we had chosen a compromise between a small photoconversion parameter and a small rotational frequency to probe the RR spectrum of the parent state, although accumulation of long-lived intermediates was inevitable. In the present work, we have employed a different approach by controlling the sample irradiation independent of the rotational frequency of the cell or the electrode. On the basis of a home-built multichannel pulse delay generator, a voltage-dependent intensity modulator (LM 202, Gsänger, D-82152 Planegg, Germany) is triggered via a pulse amplifier (LIV 8, Gsänger, Planegg) to gate the exciting laser beam such that the irradiation interval corresponds to the rotational period (1/₀) of the cell or the electrode and the dark interval is set equal to the time required for the parent state recovery. Thus, the "fresh sample" condition is fulfilled and formation of intermediates exclusively depends on l₀t. The smallest possible t depends on the maximal ₀, which was 50 s^-1 for the rotating cell but, due to technical constraints, 5 s^-1 for the rotating electrode, corresponding to a minimal t of 26 µs and 260 µs in RR and SERR experiments, respectively.

	RESULTS

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RR spectra
Fig. 1 displays the RR spectra of NpSRII in the frequency range between 1500 and 1660 cm^-1, which is dominated by the in-phase C=C stretching (_C=C) of the conjugated retinal chain (Althaus et al., 1995). The frequency of this mode is correlated with the position of the first electronic transition (_max) of the retinal chromophore (Heyde et al., 1971). On the basis of this _C=C/_max relationship, it was possible to assign component spectra determined from the analysis of the RR spectra measured at different excitation conditions to individual species of the NpSRII photocycle (Gellini et al., 2000). A representative spectrum obtained with low laser power and a short residence time of the sample in the laser beam (corresponding to a small photoconversion parameter) is shown in Fig. 1 A. Under these conditions the parent state NpSRII₅₀₀ is the prevailing species in the probe volume. Moreover, the excitation wavelength of 514 nm that was employed in this experiment is in rigorous resonance with the electronic transition of NpSRII₅₀₀ (500 nm) such that its RR bands are preferentially enhanced over those of the intermediates. In this experiment, the fresh-sample condition is not completely fulfilled and long-lived species N₄₈₅ and O₅₃₅ were accumulated, whereas the contribution of L₄₉₅ formed during the residence time of the sample in the laser beam is considered to be negligibly small. Thus, the three C=C stretching modes at 1547, 1537, and 1555 cm^-1 are attributed to NpSRII₅₀₀, N₄₈₅, and O₅₃₅, respectively, according to the _C=C/_max relationship. Contributions from M₄₀₀ could not be observed under these conditions due to the lack of sufficient resonance enhancement.

View larger version (21K): [in this window] [in a new window]   FIGURE 1  RR spectra of solubilized NpSRII in aqueous solution (pH 7.0) measured under different excitation conditions. (A) 514 nm, t·l0 = 0.35, t = 10 µs, P0 = 0.01 W, nongated excitation; (B) 413 nm, t·l0 = 0.234, t = 1300 µs, P0 = 0.01 W; gated excitation; (C) 413 nm, t·l0 = 5.85, t = 260 µs, P0 = 0.05 W; gated excitation; (D) difference spectrum "C" minus "B". The dotted lines represent the component spectrum of NpSRII500; in "A" the component spectra of the long-lived intermediates O535 and N485 are given by the dashed and solid lines, whereas in "B" and "C" the dashed-dotted, dashed, and solid lines represent the component spectra of M(L)400, M(1)400, and L495, respectively.

(5)

where _i is a constant proportional to the RR cross section of the C=C stretching mode of the species i. These constants can be determined from the RR spectrum measured with l₀t = 0.234 (Fig. 1 B) on the basis of a previous kinetic study (Chizhov et al., 1998). These authors analyzed the photocycle in terms of kinetically distinguishable states (P_j) and evaluated the rate constants for the thermal decay processes (Table 1). Using these data as well as l₀ = 9000 s^-1 derived from the excitations conditions of the RR experiment (Eqs. 3 and 4), it is possible to estimate the population of the individual states in the laser beam. The relative populations of P₀, P₂, P₃, and P₄ are calculated to be 0.795, 0.073, 0.095, and 0.037, respectively, whereas for all other states the population is <0.001. P₀, P₂, and P₄ are spectrally "pure" states and correspond to NpSRII₅₀₀, L₄₉₅, and M₄₀₀, respectively (Table 1). P₃ represents an 1:3 mixture of an L₄₉₅ and an M₄₀₀ species that form a rapid equilibrium. In the transient UV-vis absorption spectra these species are spectrally not distinguishable from the P₂ (L₄₉₅) and P₄ (M₄₀₀) states. Also the present RR spectra do not provide any indication for spectral differences between the "early" (P₂) and the "late" (P₃) L₄₉₅ species, which both contribute to the 1553-cm^-1 band. Then, the total contribution of L₄₉₅ to the RR spectrum is the sum of P₂ and 25% of P₃. Conversely, the RR spectra reveal two C=C stretching modes attributable to two different M₄₀₀ species, which appear to be related to the "early" (P₃) M₄₀₀ and "late" (P₄) M₄₀₀, denoted as M_L and M₁, respectively. Comparing relative intensities and calculated relative concentrations, the more intense 1568-cm^-1 and the weaker 1583-cm^-1 bands are assigned to M_L and M₁, respectively. Following this assignment, the relative RR cross sections evaluated according to Eq. 5 are comparable for the C=C stretching modes of both M₄₀₀ species, which is consistent with the undistinguishable absorption maxima. The corresponding values for NpSRII₅₀₀ and L₄₉₅ differ substantially from each other, which is surprising in view of the similar absorption spectra. This discrepancy may partly be due to the larger error in the intensity determination of these relatively weak bands. Thus, the quantitative analysis of the spectra according to Eq. 5 may lead to an over- and underestimation of the relative concentrations of NpSRII₅₀₀ and L₄₉₅, respectively. Since this error is systematic, it will not affect the changes of the relative concentrations in the different spectra to which the discussion will be restricted.

Upon increasing the photoconversion parameter from 0.234 to 5.85 one would expect a substantial decrease of the parent state, whereas the experimentally determined decrease is only 10% (Fig. 1 C, Table 2). These findings indicate secondary photoreactions that lead to the back-conversion of intermediates to the parent state. This may particularly refer to the M₄₀₀ species since the exciting laser beam is in rigorous resonance with their electronic transitions. For M(1)₄₀₀ the photoconversion rate is evidently higher than that of M(L)₄₀₀ since the M(L)₄₀₀/M(1)₄₀₀ ratio has increased to 3.25 from 2.0 in the absence of secondary photoreactions. Note that this increase cannot be due to the thermal decay of M(1)₄₀₀ which occurs within 2 ms and, hence, can be neglected for a residence time of 260 µs in the probe beam.

View larger version (18K): [in this window] [in a new window]   FIGURE 2  SERR spectra of immobilized NpSRII on the electrode at open circuit with 413 nm and different photoexcitation parameters. (A) t·l0 = 70, t = 260 µs, P0 = 0.06 W; nongated excitation; (B) t·l0 = 58.5, t = 1300 µs, P0 = 0.05 W, gated excitation; (C) t·l0 = 2.34, t = 260 µs, P0 = 0.01 W, gated excitation; (D) t·l0 = 0.234, t = 260 µs, P0 = 0.001 W, gated excitation. The dashed-dotted and dashed lines represent the component spectra of M(L)400 and M(1)400, respectively, and the component spectra of NpSRII500 and L495 are given by the dotted and solid lines, respectively.

Even more striking are the deviations for the population of M(L)₄₀₀ as well as for the M(L)₄₀₀/M(1)₄₀₀ ratio that are predicted to be much smaller than the experimental values regardless of the true concentration of NpSRII₅₀₀ (Table 2). These findings cannot be rationalized in terms of an enhancement of the primary photochemical process, which would, at best, lead to a quasi-photostationary mixture of NpSRII₅₀₀ and K₅₁₀. Thus, it is concluded that the thermal reaction rates are altered in the adsorbed NpSRII.

An acceleration of the L₄₉₅ (P₂) decay (10 µs) cannot account for the large population of M(L)₄₀₀ and M(1)₄₀₀ during the residence time of the sample in the laser probe beam (260 µs). Instead, the most probable explanation is that the decay times of M(L)₄₀₀ (P₃, 30 µs) and M(1)₄₀₀ (P₄, 2 ms) are drastically increased (>1 s) such that they become the rate-limiting steps of the photocycle, which is thus not completed before the sample is reirradiated by the probe beam. In this case, M(L)₄₀₀ and M(1)₄₀₀ are accumulated at the expense of NpSRII₅₀₀ as observed in the SERR spectrum. Note that a further increase of the dark time and a reduction of the laser power in the SERR experiments was not possible as such conditions required a substantial increase of the total measuring time which was in conflict with the insufficient long-term stability of the adsorbed protein.

SERR spectra measured with higher photoconversion parameters support the interpretation of increased decay time of the M-states in the adsorbed protein (Fig. 2, B and C). Regardless of the different residence times in the laser beam (260 µs and 1.3 ms), the spectra reveal essentially the same distribution between the parent and intermediate states implying that the lifetimes of M₄₀₀ states are distinctly longer than 1.3 ms. In both spectra, the total amount of both M₄₀₀ states is smaller by a factor of two than in the SERR spectrum measured with a photoconversion parameter of 0.234, indicating that, like in solution, these intermediates are photochemically reconverted to the parent state. This tendency is further enhanced upon omitting the dark intervals in the measurements (Fig. 2 A). In this spectrum also the contribution of L₄₉₅ is decreased by a factor of two and contributions from M(1)₄₀₀ cannot be detected anymore, whereas the parent state contribution is further increased.

SERR spectra measured at open circuit and 0.0 V (under otherwise identical conditions) are quite similar and include approximately the same relative contributions of NpSRII₅₀₀ and the intermediate states within the experimental accuracy (Fig. 3, A and B). Upon lowering the potential to -0.4 V, however, distinct changes are observed on the high- and low-frequency side of the 1568-cm^-1 band (Fig. 3 C) as demonstrated by a difference spectrum (Fig. 3 D). These changes correspond to an increase of L₄₉₅ and a decrease of M(L)₄₀₀ such that the M(L)₄₀₀/M(1)₄₀₀ ratio is raised from 2.0 at 0.0 V to 2.8 at -0.4 V. The relative contributions of the various species to the SERR spectrum measured at -0.4 V are in good agreement to those in the RR spectrum measured under similar excitation conditions (t and t·l₀).

View larger version (21K): [in this window] [in a new window]   FIGURE 3  SERR spectra of immobilized NpSRII on the electrode measured with gated excitation at 413 nm (t·l0 = 2.34, t = 260 µs, P0 = 0.010 W) at (A) open circuit, (B) 0.0 V, and (C) -0.4 V. The dashed-dotted and dashed lines represent the component spectra of M(L)400 and M(1)400, respectively, and the component spectra of NpSRII500 and L495 are given by the dotted and solid lines, respectively. (D) is the difference spectrum "B" minus "C".

	DISCUSSION

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The transition from the early M(L)₄₀₀ to the late M(1)₄₀₀ in NpSRII is associated with an upshift of the C=C stretching frequency by 15 cm^-1 to an unusually high value of 1583 cm^-1. Unlike for protonated retinal Schiff bases, little is known about parameters that may affect the RR spectra of the unprotonated chromophores. Early RR studies on model compounds in solution have shown that polarity and hydrophobicity of the solvent influence the C=C stretching frequency (Heyde et al., 1971). Although a unique relationship with the dielectric constant of the solvent is not evident from the experimental data, at least for all-trans retinals the highest C=C stretching frequencies (>1580 cm^-1) are observed in nonpolar solvents. We conclude, therefore, that the transition from M(L)₄₀₀ to M(1)₄₀₀ is linked to structural changes in the retinal binding pocket generating a largely hydrophobic environment in which, similar as in solution, the polyene chain adopts a fully relaxed conformation. This conclusion is corroborated by time-resolved IR spectroscopic experiments, which have shown variations of the amide bands indicating changes of the protein secondary structure (F. Siebert, personal communication, Universität Freiburg, 2002).

A largely nonpolar environment would stabilize an unprotonated Schiff base and thus may account for the relatively long lifetime of this M-state compared to that of BR. The different characteristics of the formation and decay of the late M-states in NpSRII and BR can be, at least in part, rationalized on the basis of the three-dimensional structures available for the parent states of both proteins. The retinal binding pockets of BR₅₇₀ and NpSRII₅₀₀ differ with respect to the arrangement of charged and polar amino acid residues (Luecke et al., 2001; Luecke et al., 1999; Royant et al., 2001). Specifically, Arg-72 that weakens the protonated Schiff base interactions with the counterion in BR₅₇₀ is displaced from the Schiff base in NpSRII₅₀₀. This reorientation (Ren et al., 2001) as well as the substitution of polar side chains by nonpolar amino acids (Hayashi et al., 2001), which have been suggested to be the main origin for the blue-shifted absorption maximum in NpSRII, reduces the polarity of the binding pocket already in the parent state. Protein structural changes during the M(L)₄₀₀ M(1)₄₀₀ transition in NpSRII may further enhance this effect to afford a particularly nonpolar environment for the retinal that gives rise to the unusual high C=C stretching frequency.

Upon adsorption on the metal electrode, NpSRII remains photoactive such that it runs reversibly through the photocycle. There are no indications for intermediate states that are different from those of the photocycle in solution. The C=C stretching vibrations used for identification of the parent and intermediate states are very similar for the solubilized and immobilized photoreceptor. Adsorption-induced frequency differences are as small as for proteins (e.g., cytochrome c) for which preservation of the native structure in the adsorbed state has been proven independently (Oellerich et al., 2002; Murgida and Hildebrandt, 2001a). This conclusion does not rule out local structural changes in the binding domain, which would be invisible in the SERR experiments.

In the potential range of the present SERR study, i.e., above the potential of zero charge (E_PZC -0.9 V), the Ag electrode is covered with specifically adsorbed anions that overcompensate the positive charge of the metal and hence favor electrostatic binding of proteins that exhibit a cationic region on the surface. This is also true for an electrode kept at open circuit for which the charge distribution is similar to an electrode at 0.0 V (Henglein and Lilie, 1981).

The crystal structure of NpSRII reveals a positively charged patch on the cytoplasmic side of helix F, which presumably serves as the interaction domain for the transducer protein NpHtrII (Royant et al., 2001). Since there are no other positively charged regions on the cytoplasmic or extracellular sides of the protein, this domain represents also the preferred site for electrostatic binding to the electrode. Thus, it is very likely that NpSRII adsorbs in a uniform orientation with the cytoplasmic side being in contact with the electrode. In this orientation, the retinal chromophore is separated from the metal surface by 30 Å.

The main difference between the solubilized and immobilized NpSRII refers to the photocycle kinetics. At 0.0 V and open circuit, the thermal decays of the M-states are drastically slowed down. Since the subsequent intermediate N₄₈₅ exhibits the same chromophore configuration as M(L)₄₀₀ and M(1)₄₀₀, the rate-limiting steps must be associated with conformational changes in the protein matrix. These structural changes include alterations of the secondary structure that require the rupture and formation of hydrogen bonds and proton translocations that eventually lead to the reprotonation of the Schiff base in N₄₈₅. Thus, the M-state decays involve the movement of protons, which can be sensitively affected by electric fields as has been shown for the redox-linked reorganization of the hydrogen bonding network in cytochrome c (Murgida and Hildebrandt, 2001b). In that case, the electric field experienced by the immobilized protein raises the activation barrier for the underlying proton transfer steps (Murgida and Hildebrandt, 2002), which consequently are slowed down significantly and become rate-limiting for the interfacial redox process. The lowest rate (<5 s^-1) is observed for proteins adsorbed directly in the electrical double layer (Lecomte et al., 1999) where the electric field is particularly high. As in this latter case, also NpSRII is bound to the layer of chemisorbed anions on the electrode presumably via the cationic domain on the cytoplasmic side of the protein (see above). Thus, the interfacial potential drop and the electric field strength in the retinal binding pocket are most likely comparable to that for cytochrome c (Lecomte et al., 1999; Murgida and Hildebrandt, 2001a). Hence, we conclude that also the ultimate origin for the retardation of the M-state decays in NpSRII is an electric-field induced increase of the energy barrier of proton transfer steps that are associated with rearrangements of the hydrogen bond network required for the conformational transitions of M(L)₄₀₀ and M(1)₄₀₀.

The magnitude of the electric field depends on the distance of the protein to the electrode that we have varied in our previous studies on cytochromes (Murgida and Hildebrandt, 2001a, 2001b, 2002; Simaan et al., 2002), and on the interfacial charge distribution that can be altered by changing the electrode potential (Lecomte et al., 1999). Shifting the potential E to negative values decreases the field strength since the difference (E - E_PZC) is reduced. In fact, at -0.4 V the distribution among the various states of NpSRII differs from that measured at 0.0 V and at open circuit, particularly with respect to the M_L/M₁ ratio. Moreover, the distribution is very similar to that found for the solubilized NpSRII under the same excitation conditions. These findings imply that at -0.4 V the electric field strength is not sufficient to affect the proton transfer kinetics substantially.

Extensive studies on the photocycle kinetics of BR have shown that the regeneration of the parent state is substantially slowed down under the influence of electric fields (Bamberg and Fahr, 1980; Dancshazy et al., 1983; Westerhoff and Dancshazy, 1984; Groma et al., 1984; Braun et al., 1988; Nagel et al., 1998). These results were attributed to the fact that the transmembrane proton transport starts with the deprotonation of the retinal Schiff base, i.e., the formation of the M-state. More detailed information has been obtained by Bamberg and co-workers who succeeded in reconstituting BR in membranes with a uniform orientation (Geibel et al., 2001). The authors demonstrated that at transmembrane potentials that prohibit proton pumping, specifically the decays of the early and late M-states are slowed down and thus opening a new pathway for the transformation to the parent state that is not associated with transmembrane proton transfer. Also for pSRI, an electric-field dependent retardation of the M-state decay was observed (Manor et al., 1988).

These findings appear to be strongly related to the present results on NpSRII although its primary function is not proton pumping. However, also, the conformational changes associated with the formation of the signaling state include proton transfer steps, and even proton pump activity cannot be ruled out. Thus, it is very likely that the electric-field dependence of the M-state transitions is a common characteristic of (archae)bacterial retinal proteins. For ion pumping proteins, the functional importance of these effects is immediately evident inasmuch as they may constitute a feedback control for the generation of ion gradients that are utilized to drive ATP synthesis. Taking into account the results of our previous studies on cytochrome c (Murgida and Hildebrandt, 2001a, 2001b, 2002), the molecular basis for such a mechanism may be attributed to the electric-field induced increase of the activation barrier for proton translocations. The implication of these findings for the sensor NpSRII which experiences in its natural host N. pharaonis a membrane potential of -250 mV (Wittenberg, 1995) has to be elucidated.

Submitted on October 25, 2002; accepted for publication January 22, 2003.

	REFERENCES

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

 
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