Blue- and Green-Absorbing Visual Pigments of Drosophila: Ectopic Expression and Physiological Characterization of the R8 Photoreceptor Cell-Specific Rh5 and Rh6 Rhodopsins

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The Journal of Neuroscience, December 15, 1999, 19(24):10716-10726

Blue- and Green-Absorbing Visual Pigments of Drosophila: Ectopic Expression and Physiological Characterization of the R8 Photoreceptor Cell-Specific Rh5 and Rh6 Rhodopsins
Ernesto Salcedo¹, Armin Huber², Stefan Henrich², Linda V. Chadwell¹, Wen-Hai Chou¹, Reinhard Paulsen², and Steven G. Britt¹
¹ Institute of Biotechnology and Department of Molecular Medicine, University of Texas Health Science Center, San Antonio, Texas 78245, and ² University of Karlsruhe, Institute of Zoology, Department of Cell and Neurobiology, Kornblumenstrasse 13, D-76128 Karlsruhe, Germany

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Color discrimination requires the input of different photoreceptor cells that are sensitive to different wavelengths of light.The Drosophila visual system contains multiple classes of photoreceptorcells that differ in anatomical location, synaptic connections,and spectral sensitivity. The Rh5 and Rh6 opsins are expressedin nonoverlapping sets of R8 cells and are the only Drosophilavisual pigments that remain uncharacterized. In this study, weectopically expressed Rh5 and Rh6 in the major class of photoreceptorcells (R1-R6) and show them to be biologically active in theirnew environment. The expression of either Rh5 or Rh6 in "blind"ninaE¹⁷ mutant flies, which lack the gene encoding the visual pigmentof the R1-R6 cells, fully rescues the light response. Electrophysiologicalanalysis showed that the maximal spectral sensitivity of the R1-R6cells is shifted to 437 or 508 nm when Rh5 or Rh6, respectively,is expressed in these cells. These spectral sensitivities arein excellent agreement with intracellular recordings of the R8pand R8y cells measured in Calliphora and Musca. Spectrophotometricanalyses of Rh5 and Rh6 in vivo by microspectrophotometry, andof detergent-extracted pigments in vitro, showed that Rh5 is reversiblyphotoconverted to a stable metarhodopsin ( $lambda$ _max = 494 nm), whereasRh6 appears to be photoconverted to a metarhodopsin ( $lambda$ _max = 468nm) that is less thermally stable. Phylogenetically, Rh5 belongsto a group of short-wavelength-absorbing invertebrate visual pigments,whereas Rh6 is related to a group of long-wavelength-absorbingpigments and is the first member of this class to be functionallycharacterized.

Key words: Drosophila melanogaster; fruit fly; rhodopsin; visual pigment; spectral tuning; green-absorbing rhodopsin; blue-absorbing rhodopsin; protein expression

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Color vision is the ability of an organism to distinguish differences in wavelength independent of differences in light intensity(Jacobs, 1981). With the exception of the use of oil dropletsor screening pigments in some photoreceptor cells, color visionis dependent on the expression of spectrally distinct forms ofthe visual pigment rhodopsin in different photoreceptor cells(Jacobs, 1981; Hardie, 1985; Nathans et al., 1986a,b; Nathans,1992). This prerequisite for color vision is fulfilled in theDrosophila compound eye, which is composed of ~750 ommatidia (forreview, see Wolff and Ready, 1993). Each ommatidium contains abundle of 8 photoreceptor cells and 12 auxiliary cells. The photoreceptorcells differ in their position within the ommatidium, their synapticconnections within the optic lobes of the brain, and the opsingenes they express. Each photoreceptor cell contains a rhabdomere,a microvillar structure that contains the visual pigment and servesas the compartment for visual transduction. The rhabdomeres arearranged concentrically with the six peripheral rhabdomeres ofthe R1-R6 cells surrounding one central rhabdomere formed by theR7 or R8 cells in the distal or proximal portion of the ommatidium,respectively. The rhabdomeres of the R1-R6 photoreceptor cellsspan the length of the ommatidium and contain the major visualpigment of the Drosophila compound eye, the blue-absorbing Rh1rhodopsin (ninaE) (O'Tousa et al., 1985; Zuker et al., 1985; Feileret al., 1988). The R7 cells express either Rh3 or Rh4, UV-absorbingvisual pigments, in nonoverlapping subsets of cells (Fryxell andMeyerowitz, 1987; Montell et al., 1987; Zuker et al., 1987; Feileret al., 1992). The R8 cells express either Rh5 or Rh6 in nonoverlappingsubsets of cells (Chou et al., 1996, 1999; Huber et al., 1997;Papatsenko et al., 1997). A minor class of ommatidia, locatedalong the dorsal margin, contains R7 and R8 cells that both expressRh3 (Fortini and Rubin, 1990; Feiler et al., 1992). Rh2 encodesa violet-absorbing visual pigment that is expressed in the ocelli,simple eyes located on the vertex of the head (Cowman et al.,1986; Feiler et al., 1988).

The present studies were undertaken to characterize the spectral and photochemical properties of the R8 photoreceptor cell-specificrhodopsins Rh5 and Rh6. Previous work in larger flies, Calliphoraand Musca, suggested that these visual pigments are likely tohave unique spectral properties (for review, see Hardie, 1985,1986). The characterization of these pigments provides insightinto the relationship between visual pigment structure and theregulation of spectral tuning. Furthermore, phylogenetic analysesof Rh5 and Rh6 place both of these pigments into newly definedclades of visual pigment genes that have not been well characterized.Thus the characterization of Rh5 and Rh6 provides a basis forexamining other cloned invertebrate pigments and completes thespectral characterization of the visual pigments of the Drosophilaeye that is essential for a detailed examination of color visionin Drosophila.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Ectopic expression of the Rh5 and Rh6 opsin genes. Flies expressing the Rh5 opsin gene in the R1-R6 photoreceptor cells ofninaE¹⁷ mutants (y w; ninaE¹⁷; P[Rh1 + 5, y⁺]) have been described previously (Chou et al., 1996). Flies expressingthe Rh6 opsin gene (y w; ninaE¹⁷; P[Rh1 + 6, y⁺]) were generated in a similar manner. Briefly, the Rh6 cDNA (a1.4 kb EcoRI/KpnI fragment from clone 4.1A, containing the entireRh6-coding region and polyA tail) was inserted immediately 3'of an expression cassette containing the Rh1 promoter (2.4 kbincluding 33 bp of the 5'-untranslated region). The transcriptionalfusion was subcloned into the y⁺-marked P-element vector "C4" obtained from Pam Geyer (Universityof Iowa, Ames, IA). The construct was injected into y w; sr ninaE¹⁷ mutant embryos, and multiple independent P-element-mediated germlinetransformants were obtained using standard techniques (Karessand Rubin, 1984).

Histology. The immunohistochemistry and confocal imaging were performed as described previously (Chou et al., 1996). Headsections were incubated overnight at 4°C with rabbit anti-Rh1(1:250 dilution), monoclonal anti-Rh5 (clone 7F1; IgG1 subclass;1:20 dilution), and monoclonal anti-Rh6 (clone 14C5; IgM subclass;1:20 dilution). After washes in PBS containing 0.1% saponin, thesections were incubated for 1 hr at room temperature with threesecondary antibodies: Texas Red-conjugated goat anti-rabbit IgG(1:100 dilution), Cy5-conjugated goat anti-mouse IgG1 (1:100 dilution),and FITC-conjugated goat anti-mouse IgM (1:100 dilution). Theconfocal images were collected using a Bio-Rad MRC-1024 (Hercules,CA) with a Nikon Labphot-2 microscope (Melville, NY). Secondaryantibodies and other immunological reagents were obtained fromJackson ImmunoResearch (West Grove, PA) and Southern Biotechnology(Birmingham,AL).

Sequence alignment and phylogenetic analysis. Amino acid sequences were aligned using Clustal X (Thompson et al., 1997). Phylogenetictrees were constructed with PAUP* 4.0b2a (Swofford, 1998) usingmaximum parsimony (unweighted) and neighbor-joining methods. Toensure robustness of the results and to estimate confidence intervals,we bootstrapped all trees 100 times. For each parsimony bootstrapreplicate, five random additions and tree-bisection reconnectionbranch swapping were performed. In all analyses, bovine rhodopsinwas designated anoutgroup.

Electrophysiology. Electroretinogram (ERG) recordings were obtained from immobilized white-eyed (w) flies using glass microelectrodesfilled with normal saline (0.9% NaCl, w/v) as described previously(Chou et al., 1996; Townson et al., 1998). Flies were stimulatedwith light from a xenon arc lamp (450 W; Osram; Oriel, Stratford,CT), using interference and neutral density filters to selectspecific wavelengths and intensities of light. Light intensitywas measured using a calibrated silicon photodiode (model 71883;Oriel) and an optical power meter (OPM model 70310;Oriel).

Spectral sensitivity was measured using a modification of the voltage-clamp method of Franceschini (1979, 1984), which wehave described in detail elsewhere (Townson et al., 1998). Briefly,the amplitude of the ERG response to a flickering (10 Hz) monochromaticstimulus was maintained at a criterion level by continuously adjustingthe light intensity, as the wavelength of stimulating light wasvaried during a scan. In previous experiments, we have found thatdirectly measuring and "clamping" the area (amplitude) of theERG response can be problematic. This is because the scans requireseveral minutes to complete and there is a significant problemin defining the baseline from which the ERG area or amplitudeis calculated, especially when the baseline drifts. In the measurementsin this study, for each ~0.3 sec window (ERG response to approximatelythree flickers), we averaged all of the ERG voltages during thisperiod and used the SD as an estimate of the amplitude (width)of the response (Press et al., 1992). The SD is a function ofthe variance between the individual data points and the mean voltageduring the sinusoidal ERG response. Thus, the SD is related tothe response amplitude, although we have found that it is muchless sensitive to baseline drift andnoise.

During an experiment, as the monochrometer was stepped through a scan, the SD of the ERG response to three pulses of light(during 0.3 sec) was calculated and compared with a criterionset point. The ERG response was maintained near the set pointduring the scan by constantly adjusting the light intensity usinga proportional-integral-derivative algorithm (Corripio, 1990).Spectral sensitivity (SS) was defined as the inverse of the lightflux required to produce the criterion response, taking into accountthe wavelength and intensity of the stimulating light [i.e., SS $proportional to$ 1/(light intensity (µW/cm²) × wavelength)]. Raw sensitivity data were normalized to an amplitudeof 1.0 at the wavelength of maximum sensitivity, multiple individualmeasurements were averaged, and values that differed by >10% fromthe mean value of a 10 nm window were filtered out. The filteredspectra were then smoothed with a window of 12nm.

Microspectrophotometry. Heads from white-eyed flies were bisected (maintaining the retinas intact) and mounted between quartzcoverslips in PBS. A single eye was illuminated antidromicallyso that light passed through the specimen into the objective lensof the single-beam microspectrophotometer [Leitz (MPV2; Wetzler,Germany) equipped with Zeiss ultrafluar optics and a Productsfor Research photomultiplier (RCA model C31034A02; Danvers, MA)].To adapt the specimen, light emitted from a super-pressure mercuryarc lamp (HBO 100 W; Osram, Berlin, Germany) and passed throughan interference filter was used to photoconvert the visual pigmentfrom its rhodopsin (R) to its metarhodopsin (M) state. The wavelength( $lambda$ ₁) of the adapting light was selected to shift the photosteadystate preferentially between R and M. To measure the transmissionthrough the specimen, light from a tungsten halogen source (12V/100 W; model 64623; Osram) was passed through a 1/8-m monochromator(model 7420; Oriel) and directed through the specimen. Transmissionwas measured continuously with a photomultiplier as the monochromatorscanned from 350 to 700 nm. The measuring light did not significantlyalter the steady state between the two photopigment states. Asecond adapting light at a different wavelength ( $lambda$ ₂) was thenused to shift the photosteady state of the R and M states backtoward the R state, and the transmission of the specimen was measuredagain. A difference spectrum $Delta$ E ( $lambda$ ) was calculated from thesemeasurements: $Delta$ E( $lambda$ ) = [log (I₂( $lambda$ )/I₁( $lambda$ )], where I₁( $lambda$ )and I₂( $lambda$ ) are the light intensities transmitted through thespecimen after adaptation at $lambda$ ₁ and $lambda$ ₂, respectively. The differencespectra were normalized, averaged, and smoothed with a windowof 10nm.

Electrophysiological and spectroscopic data acquisition and instrument control were performed with a Power Macintosh 7600/120(Apple Computer, Cupertino, CA) equipped with a National Instruments(Austin, TX) PCI-MIO-16XE-50 multifunction input/output boardrunning LabView 5.0.

Preparation of visual pigment extracts and spectrophotometry. Drosophila ninaE¹⁷ mutants, white-eyed (w¹¹¹⁸) control flies, and transgenic strains expressing different Drosophilavisual pigments in a ninaE¹⁷ mutant background were dark adapted for 48 hr. Between 200 and1000 eyes were dissected under dim red light (>665 nm) and collectedin water. The water was removed, and 200 µl of homogenizationbuffer (10% sucrose and 0.1 M sodium phosphate buffer, pH 6.0)was added. The samples were homogenized and then centrifuged for20 sec at low speed (1000 × g) to spin down the chitin debrisand unhomogenized tissue. The supernatant was removed, and theprocedure was repeated twice. The combined supernatants were centrifugedfor 10 min at 100,000 × g, and the membrane pellet was extractedwith 40 µl of 4% digitonin in sodium phosphate buffer, pH 6.0,for 40 min at 20°C in the dark. Difference spectra were recordedwith a Kontron Uvikon 930 spectrophotometer at 10°C (for measuringabsorbance changes of extracts containing Rh1, Rh3, Rh4, or Rh5rhodopsin) or at 1°C (for extracts containing Rh6 rhodopsin orextracts obtained from ninaE¹⁷ mutants). The extracts were irradiated in the cuvette with monochromaticlight (Schott interference filters) using a 50 W xenon lamp untila steady state was achieved (2-4 min) at the wavelengths indicatedin the figure legends. To ensure that there was little or no effecton the photosteady state of the pigment caused by measuring thespectrum, before each experiment we measured and then immediatelymeasured again the spectrum of the dark-adapted pigment. The differencespectrum of these two measurements is shown as the "baseline"in relevant figurepanels.

Rhodopsin nomogram modeling. Rhodopsin and metarhodopsin absorption spectra were calculated from the difference spectra recordedfrom the microspectrophotometry (MSP) and detergent-extractedpigments using the exponential function described by Stavengaet al. (1993). Briefly, the spectral shape of the rhodopsin $alpha$ -bandabsorption can be described by the following log normal function: $alpha$ = A exp[ $-$ a₀x²(1 + a₁x + a₂x²)], where x = ¹⁰log( $lambda$ / $lambda$ _max), A = 1, a₀ = 380, a₁ = 6.09, and a₂ = 3a₁²/8. Taking this relationship and assuming that the spectral shapeof metarhodopsin is also described by this equation (but withdifferent A and $lambda$ _max), we fit the measured difference spectrato an equation in which the $alpha$ -band absorption of rhodopsin wassubtracted from that of metarhodopsin. A curve-fitting routinewas implemented in KaleidaGraph (version 3.08d; Synergy Software,Reading, PA) using the Levenberg-Marquardt (nonlinear least-squares)algorithm (Press et al., 1992). The computer solved for the $lambda$ _maxand amplitude of both the rhodopsin and metarhodopsin absorptionspectra and calculated the SD for each variable and the correlationcoefficient (Pearson's r).

Stavenga et al. (1993) have shown that an improved fit can be obtained in the lower wavelength region by incorporating additionalterms for the rhodopsin $beta$ -band absorption. These terms were notincorporated in the curve fitting because too little is knownabout the characteristics of M $beta$ -bandabsorption.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Ectopic expression of the Rh5 and Rh6 opsins in transgenic flies

The Drosophila visual system has proven to be an extremely useful tool for studying novel invertebrate opsins in vivo (Feileret al., 1988, 1992; Britt et al., 1993; Townson et al., 1998).To characterize the spectral and biophysical properties of theRh5 and Rh6 opsins, we expressed the genes encoding these visualpigments in the R1-R6 photoreceptor cells of a mutant strain offlies (ninaE¹⁷). By coupling the structural gene of Rh5 or Rh6 to the promoterregion from the Rh1 opsin gene, we targeted the expression ofthe novel opsin to the R1-R6 photoreceptor cells. These cellscomprise the major class of photoreceptor cells in Drosophila.The R1-R6 photoreceptor cells dominate the physiological and photochemicalproperties of the compound eye and are primarily responsible forthe optomotor behavior of fruit flies (Heisenberg and Wolf, 1984).The ninaE¹⁷ mutant strain serves as an appropriate host for the expressionof the Rh5 and Rh6 opsins because these flies lack the Rh1 visualpigment that is normally expressed in the R1-R6 cells. White-eyedflies (w) were used in these experiments because the removal ofthe red-screening pigments of the eye increases the animal's sensitivityto light, allows for the measurement of rhodopsin difference spectraby MSP and from visual pigment extracts, and also simplifies theimmunofluorescence studies of visual pigment expressionpatterns.

To characterize the expression pattern of the endogenous and ectopically expressed opsins, we used specific polyclonal andmonoclonal antibodies directed against the C termini of the opsinproteins (see Materials and Methods). As shown in Figure 1A, theRh1 opsin is expressed throughout the eye of the control flies(y w; red). Specifically, these opsins are expressed in the rhabdomeresof the R1-R6 cells, which extend the full length of the retinaand constitute the majority of the photoreceptor cells found inthe compound eye (Fig. 1A). In contrast, the endogenous Rh5 (Fig.1A, blue) and Rh6 (green) opsins localize to the R8 cells, whichcomprise only a subset of the total photoreceptor cell populationand are located proximally within the retina. Not labeled in thesefigures are the endogenous opsins that localize to the R7 cells,a subset of photoreceptor cells that are located in the distalretina. The host strain (y w; ninaE¹⁷) lacks Rh1 expression in the R1-R6 photoreceptor cells becauseof a deletion within the Rh1 gene, but this strain does expressthe endogenous opsins found in the R7 and R8 cells (Fig. 1B).In the transgenic flies, the Rh5 and Rh6 opsins (y w; ninaE¹⁷ P[Rh1 + 5, y⁺] and y w; ninaE¹⁷ P[Rh1 + 6, y⁺], respectively) are expressed throughout the compound eye, inthe R1-R6 photoreceptor cells of ninaE mutant flies (Fig. 1C,D).Note that the expression of the endogenous opsins in the R8 cellsis not disrupted in the transgenic flies and there is no endogenousRh1 opsin expressed in the retina.

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Figure 1. Expression of Rh5 and Rh6 in the compound eye of Drosophila. Shown are confocal immunofluorescence images of longitudinal sections of retinas from white-eyed flies. A, In control flies (y w), Rh1 (red) is expressed in the rhabdomeres of the R1-R6 photoreceptor cells. Endogenous Rh5 (blue) and Rh6 (green) opsins are expressed in the rhabdomeres of the R8 cells, which occupy the proximal half of the retina. Rh3 and Rh4 are expressed in the rhabdomeres of R7 photoreceptor cells, which occupy the distal half of the retina (not labeled). B, In the mutant host strain (y w; ninaE¹⁷), a portion of the Rh1 gene (ninaE) has been deleted, and Rh1 is not expressed in the R1-R6 cells. However, the endogenous minor opsins, localized to the R7 (not labeled) and R8 (Rh5 and Rh6 shown as blue and green, respectively) cells, are still expressed. C, In transgenic flies that ectopically express Rh5 under the control of the Rh1 promoter (y w; ninaE¹⁷ P[Rh1 + 5, y⁺]), Rh5 (blue) is found throughout the retina in the R1-R6 photoreceptor cells. D, Similarly, in transgenic flies that ectopically express Rh6 (y w; ninaE¹⁷ P[Rh1 + 6, y⁺]), Rh6 (green) is expressed in the R1-R6 cells. Because the host strain for the expression experiment is mutant for ninaE¹⁷ (as in B), there is no detectable Rh1 opsin expressed in either of the transgenic strains (C, D). Scale bar in A, 50 µm.

To test whether Rh5 and Rh6 are biologically active in their new cellular environment, ERGs were recorded from several differentlines of control and transgenic flies. Figure 2 shows wild-typeERGs recorded from white-eyed (y w) flies, which express the Rh1opsin in the R1-R6 photoreceptor cells (Fig. 2A, top row of traces).In these ERGs, a hyperpolarizing "on-" and a depolarizing "off-"transientappears at the onset and termination of the light stimulus, respectively.In addition there is a robust depolarization that is maintainedfor the duration of the stimulus. The on- and off-transients havebeen shown to originate in the first optic neuropile (the lamina)and are induced only by activation of the R1-R6 photoreceptorcells (Heisenberg, 1971; Heisenberg and Wolf, 1984; Laughlin,1989). The maintained depolarization is generated directly atthe level of the retina by the action of all three classes ofphotoreceptors contained within the compound eye. In the ERGsrecorded from the y w; ninaE¹⁷ host strain, no on- or off-transients can be detected, and themagnitude of the depolarization is dramatically reduced (Fig.2A, second row of traces). The remnant depolarization recordedfrom these flies arises from the R7 and R8 photoreceptor cells,which still express functional opsins (Fig. 1B). When either Rh5or Rh6 is introduced into the ninaE¹⁷ mutant host strain, the light response in the ERG is completelyrestored (Fig. 2A, third, fourth rows of traces). This indicatesthat these genes encode functional opsins capable of forming rhodopsinsthat are activated by light and that couple to the downstreamcomponents of the phototransduction cascade within the R1-R6 photoreceptorcells.

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Figure 2. ERGs recorded from transgenic flies expressing Rh5 and Rh6. A, Responses to different wavelengths are arranged in columns, and responses recorded from specific genetic backgrounds are arranged in rows. Control y w flies (top row of traces), which express the Rh1 opsin in the R1-R6 photoreceptor cells, have a robust response to light at both 430 and 520 nm. The depolarization is preceded and followed by on- and off-transients, respectively, which originate in the lamina and reflect the activation of the R1-R6 cells (Heisenberg, 1971; Heisenberg and Wolf, 1984; Laughlin, 1989). The mutant host strain that lacks the Rh1 opsin, y w; ninaE¹⁷ (second row of traces from the top), has a dramatically reduced receptor potential and lacks both on- and off-transients. The residual response is derived from the R7 and R8 photoreceptor cells that are unaffected by the ninaE¹⁷ mutation. The transgenic flies that express Rh5 or Rh6, y w; ninaE¹⁷ P[Rh1 + 5, y⁺] (third row of traces from the top) and y w; ninaE¹⁷ P[Rh1 + 6, y⁺] (fourth row of traces from the top), display robust, wild-type photoresponses at either wavelength of light, demonstrating that both Rh5 and Rh6 are functional when expressed in the R1-R6 photoreceptor cells. Response amplitudes are not directly comparable between strains because of differences in the transgene expression levels. All of the strains were stimulated with the same intensity of light, which was ~1.09 µW/cm² at 430 nm and 0.9 µW/cm² at 520 nm. B, When a control fly (y w; top trace) is stimulated with intense light at 570 nm, there are a robust depolarization and immediate repolarization at the end of the stimulus. A PDA is induced when the fly is stimulated with light at 470 nm (thus producing a large amount of activated M-form). The depolarization is maintained after the cessation of the stimulus, and the photoreceptor cells are relatively inactivated to further stimuli. When the fly is again stimulated with 570 nm light, the PDA is terminated by the photoconversion of the M-form back to the R-form. Transgenic flies expressing Rh5 (y w; ninaE¹⁷ P[Rh1 + 5, y⁺]; second trace from the top) can undergo a PDA when stimulated with light at 430 nm, and this can be terminated by stimulation with light at 520 nm. Transgenic flies expressing Rh6 (y w; ninaE¹⁷ P[Rh1 + 6, y⁺]; third trace from the top) do not show a PDA when stimulated with 550 nm light. This wavelength would be expected to produce maximal conversion of Rh6 from the R- to the M-form with minimal photoconversion back to the R-form (see Fig. 4, for Rh6 extract difference spectra). Stimulation of Rh6 transgenic flies at 350, 430, 470, 520, and 570 nm was also insufficient to induce a PDA (data not shown). Light intensity was unattenuated in these experiments and was ~0.5 mW/cm² at each of the wavelengths tested. The bottom row in A and the row below each trace in B show the stimulus, with the time and voltage scales indicated on the bottom left of each panel.

Spectral and photochemical analysis of Rh5 and Rh6

To characterize the spectral properties of the Rh5 and Rh6 opsins, we used both spectrophotometric and electrophysiologicaltechniques. To determine the spectral sensitivity of transgenicflies expressing either the Rh5 or Rh6 opsin, we used a modifiedversion of Franceschini's voltage-clamp technique (Franceschini,1979, 1984). As shown in Figure 3, top left (Rh1), white-eyedcontrol flies (y w), which express Rh1 in the R1-R6 photoreceptorcells, have a dual sensitivity in the UV and visible region ofthe spectrum. The sensitivity peak in the visible region has amaximum near 475 nm, which is well fit by a rhodopsin nomogramhaving an absorption maximum at 478 nm. The sensitivity in theUV region is thought to arise as the result of a sensitizing pigmentthat transfers the energy of an absorbed photon to the Rh1 chromophore,thereby inducing isomerization and visual pigment activation (Kirschfeldet al., 1977; Minke and Kirschfeld, 1979). In contrast, the spectralsensitivity of flies expressing the Rh5 or Rh6 minor opsins inthe R1-R6 photoreceptor cells has been markedly altered (Fig.3, bottom left). In the case of flies expressing Rh5, there isa peak of sensitivity near 440 nm, which is well fit by a rhodopsinnomogram having an absorption maximum at 437 nm. The spectralsensitivity of flies expressing Rh6 shows a peak in the greenregion near 510 nm, which is well fit by a rhodopsin nomogramhaving an absorption maximum at 508 nm.

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Figure 3. Spectral sensitivity and in vivo spectroscopy of Rh5 and Rh6. Spectral sensitivity was measured using a modification of the voltage-clamp method of Franceschini (1979, 1984) (see Materials and Methods for details). Top Left (Rh1), Recordings averaged from y w control flies (n = 2). These animals express the Rh1 (ninaE) opsin in the R1-R6 photoreceptor cells and have prominent sensitivity peaks in the blue and UV regions of the spectrum (bold trace). The single peak at ~475 nm (blue) is attributable to direct absorption by, and activation of, the Rh1 pigment. The doublet at ~355 and 370 nm (UV) is attributable to a UV-sensitizing pigment. The sensitizing pigment is thought to transfer the energy of absorbed UV quanta to the Rh1 chromophore, thereby inducing isomerization and visual pigment activation (Kirschfeld et al., 1977). The peak of Rh1 sensitivity in the blue region is fit well by a calculated rhodopsin $alpha$ -band absorption (fine trace) having a maximal absorption at 478 nm (r = 0.983) (Stavenga et al., 1993). The measured spectral sensitivity is somewhat broader than the calculated absorption, and this could be caused by waveguide or self-screening effects (Smakman and Stavenga, 1986). Bottom Left, The averaged spectral sensitivities of transgenic flies expressing either Rh5 (n = 4) or Rh6 (n = 5) in the R1-R6 cells (same genotypes indicated in Fig. 2). Flies expressing Rh5 have a prominent peak of sensitivity at ~440 nm, whereas flies expressing Rh6 have a prominent peak at ~510 nm (bold traces). The spectral sensitivities of Rh5 and Rh6 were well fit by calculated rhodopsin $alpha$ -band absorptions (fine traces) having absorption maxima at 437 nm (r = 0.995) and 508 nm (r = 0.998) for Rh5 and Rh6, respectively. When Rh5 or Rh6 is expressed in a host strain that lacks the response of the R7 and R8 cells (w norpA^P24; ninaE¹⁷ P[Rh1+norpA cDNA, w⁺]; see Results for description), we find that Rh5 transgenic flies display no UV sensitivity (data not shown). Inset, In contrast, Rh6 transgenic flies showing UV sensitivity. The fine trace shows the same curve shown in the main panel, and the bold curve is a high-resolution scan through the lower wavelength region. The amplitude of the high-resolution scan was normalized to that of the short-wavelength limb of the visible region scan (fine trace) for comparison. The y w; ninaE¹⁷ mutant host strain did not have a detectable spectral sensitivity in this assay, because the amplitude of the ERG response was not high enough to meet the criterion of the recording paradigm (see Materials and Methods). Right, Rhodopsin and metarhodopsin difference spectra measured in vivo by MSP. Top Right, Control flies (y w; Rh1; n = 3). Bottom Right, Rh5 transgenic flies (y w; ninaE¹⁷ P[Rh1 + 5, y⁺]; n = 2). Rh1-expressing flies were illuminated with adapting lights ( $lambda$ ₁ and $lambda$ ₂) of 475 and then 580 nm, to shift the photosteady state from the Rh1 R-form to the M-form, and then vice versa. Rh5 transgenic flies were illuminated with adapting lights ( $lambda$ ₁ and $lambda$ ₂) of 418 and 524 nm. No difference spectrum could be generated from flies expressing the Rh6 opsin construct after adaptation at multiple wavelengths (see Results).

To test whether either the Rh5 or Rh6 rhodopsins are capable of coupling to the sensitizing pigment and thus conferring UVsensitivity to the R1-R6 cells, we examined the spectral sensitivityof Rh5 and Rh6 when expressed in a special host strain. As describedabove and shown in Figure 2A, ninaE¹⁷ flies have functional R7 and R8 cells that are unaffected bythe ninaE¹⁷ mutation and produce a small depolarization in the ERG. The R7photoreceptor cells have a pronounced UV sensitivity that couldpotentially interfere with the analysis of Rh5 and Rh6 in theUV region of the spectrum. Therefore, in transgenic flies expressingeither Rh5 or Rh6, the norpA-encoded phospholipase C that is requiredfor visual transduction in all photoreceptor cells of the compoundeye was removed genetically (by the norpA mutation) (Bloomquistet al., 1988), and then this activity was restored only in theR1-R6 cells by expressing the norpA cDNA under the control ofthe ninaE (Rh1) promoter (Pearn et al., 1996). Because these fliesalso lack the Rh1 visual pigment gene in the R1-R6 cells (ninaE¹⁷ mutant), all of the light-induced response was derived from Rh5or Rh6 expression in the R1-R6 cells. Flies expressing Rh5 haveno detectable sensitivity in the UV region (data not shown). Wewould expect that even a small peak of UV sensitivity would bedetectable because there would be little overlap between the short-wavelengthlimb of the sensitivity peak of Rh5 transgenics and that attributableto the sensitizing pigment. By contrast, flies expressing Rh6do show a small sensitivity peak in the UV (Fig. 3, bottom left,inset). This most likely reflects the coupling of Rh6 to the sensitizingpigment in the R1-R6 cells, although the efficiency of couplingappears reduced in Rh6 transgenics in the UV region compared withRh1, as demonstrated by relative sensitivity ratios of ~2:1 (UV/visible)for Rh1 versus ~0.5:1 for Rh6. Furthermore, we did not observethe expected fine structure in the UV region for Rh6-expressingflies that is normally observed for other rhodopsins that coupleto the sensitizing pigment and has also been observed in the R8yphotoreceptor cells of larger flies (Hardie and Kirschfeld, 1983;Feiler et al., 1988). Our inability to detect any fine structuremay be caused by the relatively low UV sensitivity of the Rh6-expressingflies.

We examined the transgenic flies expressing Rh5 and Rh6 using microspectrophotometry (MSP) to determine the absorption profilesof rhodopsin and metarhodopsin for each of the novel pigments.Photoconversion of R produces the activated form of the visualpigment M. For many invertebrate pigments, the M-form of the visualpigment is thermally stable, and its absorbance $lambda$ _max is dramaticallyshifted from that of the R-form of the pigment (Stavenga, 1989,1992). In addition the R- and M-forms are photointerconvertible,so that when the $lambda$ _max of R and M differ significantly the ratioof the rhodopsin molecules in the R- and M-forms can be manipulatedusing different illumination conditions. In the photosteady state,the ratio of the R- and M-forms is dependent on the spectral compositionof the illuminating light and the absorption profiles of the twostates of the pigment (Hamdorf et al., 1973; Hamdorf, 1979). Forexample, when the Rh1 rhodopsin (expressed in y w control flies)is illuminated with blue light near 480 nm, ~70% of the Rh1 R-formis converted to the M-form at steady state (Huber et al., 1990).Subsequent illumination with orange light near 580 nm photoconverts100% of the M-form back to the R-form of rhodopsin. When absorptionspectra are recorded before and after an illumination that shiftsa substantial amount of the R-form to the M-form and these spectraare subtracted from each other, the resulting difference spectrumreflects the decrease in R-form absorption and the increase inM-form absorption (Fig. 3, top right). We used MSP to measurethe difference spectrum of flies expressing the Rh5 opsin andfound that Rh5 is photoconverted to a thermally stable metarhodopsinthat absorbs maximally near 500 nm (Fig. 3, bottom right). Nodifference spectrum could be generated for Rh6-expressing fliesby MSP, suggesting either (1) that there is not enough Rh6 expressedto be detectable by MSP, (2) that the M-form of Rh6 is not stable,or (3) that there is sufficient overlap in the absorption spectraof the R- and M-forms that illumination at many different wavelengths(402, 418, 430, 442, 456, 475, 499, 524, 563, and 584 nm; datanot shown) did not lead to a detectable shift in the ratio ofR and M in the photosteadystate.

To examine the photoconversion between the R- and M-forms of Rh5 and Rh6 further, we attempted to generate prolonged depolarizingafterpotentials (PDAs) in transgenic flies expressing these pigments.A PDA is only generated in white-eyed flies when a substantialamount of rhodopsin has been photoconverted to metarhodopsin.During a PDA, the depolarization is maintained after the cessationof the light stimulus, and the response is inactivated to furtherstimuli (Pak, 1979). The PDA is thought to result from the inadequateinactivation of the activated metarhodopsin state. Metarhodopsinis inactivated in part by a stoichiometric interaction with anabundant, cytosolic protein, arrestin. Because arrestin is expressedat a fraction of the concentration of rhodopsin, excessive conversionof the visual pigment to its activated M-form is thought to overcomethe ability of arrestin to inactivate it, and this produces aPDA (Dolph et al., 1993). This requires that (1) the visual pigmentmust be expressed and activated at sufficiently high levels thatthe concentration barrier to PDA generation is overcome, (2) theabsorptions of the R- and M-forms are sufficiently different thatillumination creates a photosteady state in which a high percentageof the visual pigment is present in the M-form, and (3) the M-formof the pigment must be stable for the period of time in whichthe PDA is observed. Figure 2B, top trace, shows that when y wcontrol flies are illuminated with intense orange light at 570nm, which does not shift a significant amount of the R-form tothe M-form, there is a robust depolarization that ends abruptlyat the end of the stimulus. When the animals are illuminated withblue light at 470 nm, converting 70% of R to M, there is a robustdepolarization that is maintained after the stimulus ends, andthe fly eye is relatively inactivated to further stimuli. Whenorange light is used to photoconvert all of M to R, the PDA isimmediately terminated, and the response returns to baseline.When flies expressing Rh5 are stimulated with appropriate wavelengthsof light, a similar "retuned" PDA can be generated. The PDA canbe initiated with intense light at 430 nm, converting ~50% ofthe Rh5 R-form to M, and this response can be terminated by illuminationat 520 nm (photoconverting the M-form back to the R-form) (Fig.2B, second trace from the top). This retuning of the PDA to wavelengthsof light that can shift the steady state ratio of the R- and M-formsof ectopically expressed pigment has been demonstrated in previousstudies with transgenic flies expressing Rh2, Rh3, and Rh4 (Feileret al., 1988, 1992). Interestingly, stimulation of Rh6 transgenicflies at many wavelengths (Fig. 2B, third trace from the top;550 nm is shown) was insufficient to induce a PDA. As was thecase with the MSP studies, this suggests either that the pigmentis not being expressed or activated at high levels, that thereis a significant overlap between R- and M-form absorption, orthat the M-form is unstable. To resolve these possibilities weexamined the absorption profiles of the Drosophila Rh5 and Rh6opsins in detergent extracts prepared from the retinas of dark-adaptedflies (Fig. 4). We found that the Rh5 R-form can be reversiblyphotoconverted to a stable M-form (Fig. 4, top left), whereasphotoactivation of Rh6 at a reduced temperature (1°C) producesan M-form that was not photoconverted back to the R-form in detectableamounts, and no stable M-form could be detected in extracts athigher temperatures (10°C) (Fig. 4, top right). This finding suggeststhat the M-form of Rh6 is not as stable as that of Rh5, at leastwhen the pigments are expressed ectopically in the R1-R6 cellsand extracted in digitonin. This finding provides one possibleexplanation for our inability to detect the Rh6 M-form by MSPand to induce a PDA in Rh6-expressing flies.

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Figure 4. In vitro spectroscopy of Rh5 and Rh6 visual pigment extracts. Top, Difference spectra obtained from digitonin extracts of Rh5 (left) and Rh6 (right) transgenic flies are shown. Extracts were prepared in dim red light from 260 or 700 hand-dissected eyes of flies expressing Rh5 or Rh6, respectively, in the R1-R6 cells. Measurement of the absorption spectrum had no measurable effect on the samples, as shown by the baseline (BL) difference spectra calculated from sequential scans of the sample without other illumination. For both Rh5 and Rh6, when the extracts were illuminated with light selected to convert preferentially the R-form to the M-form (R $right-arrow$ M) (4 min at 421 nm and 2 min at 560 nm for Rh5 and Rh6, respectively), a difference spectrum is generated. For Rh5, but not Rh6, the difference spectrum could be generated at 10° C. The Rh6 difference spectrum could only be generated at a reduced temperature (1° C). When the extracts were illuminated with light selected to convert preferentially the M-form back to the R-form (M $right-arrow$ R) (4 min at 560 nm for Rh5; not shown for Rh6), a difference spectrum could be generated for Rh5 but not for Rh6. Bottom, The Rh5 and Rh6 difference spectra (DS) were fit with calculated rhodopsin and metarhodopsin absorption profiles as described in Materials and Methods (curve fits for Rh5 and Rh6 are shown as fine traces overlying the DS in the bottom right and left panels, respectively). The Rh5 difference spectrum was best fit with R- and M-form absorptions having maxima at 442 and 494 nm, respectively (r = 0.998). The calculated ratio of R- and M-form extinctions (R/M) at the $lambda$ _max for each form was 1:1.3. The Rh6 difference spectrum was best fit with R- and M-form absorptions having maxima at 515 and 468 nm, respectively (r = 0.991). The calculated ratio of R/M extinctions at the $lambda$ _max for each form was 1:2.1.

An alternative explanation of these findings may be that there is too little Rh6 expressed in the transgenic flies to inducea PDA or be detectable by MSP. The evidence that this may be thecase is based on the absorbance change, corresponding to the formationof metarhodopsin, observed in visual pigment extracts. We calculatedthe amount of rhodopsin per eye, assuming that the molar extinctioncoefficients of the M-forms of the Drosophila rhodopsins are approximatelythe same as has been determined for the Calliphora Rh1 rhodopsin,i.e., 72,000 M¹ cm¹ (Stavenga and Schwemer, 1984). Although wild-type flies contain~220 fmol of Rh1 per eye, the amount of photoconvertible Rh5 andRh6 rhodopsin expressed in the R1-R6 and R8 cells of the transgenicstrains is only 45 and 9 fmol/eye, respectively. So although therelatively low amount of Rh5 present may be at the lower limitof the amount of photoconvertible rhodopsin required to inducea PDA (~10-20% of wild-type Rh1 levels), the even smaller amountof functional Rh6 present may be the major reason for our inabilityto generate a PDA in theseflies.

The theoretical absorption spectra of the R- and M-forms of each pigment were derived from the difference spectra by fittingthe data to a model in which the absorption of the R-form wassubtracted from the absorption of the M-form. The absorptionsof the R- and M-forms were calculated using an exponential functionthat describes the shape of the rhodopsin absorption curve asa function of wavelength (described in Materials and Methods)(Stavenga et al., 1993). We found that the difference spectrumof the detergent-extracted Rh5 was fit well by R- and M-formshaving absorption maxima at 442 and 494 nm, respectively (Fig.4, bottom left). This is in fairly good agreement with a similaranalysis of the MSP data [R ( $lambda$ _max) = 450 nm; M ( $lambda$ _max) = 496 nm]and the spectral sensitivity measurements determined electrophysiologically( $lambda$ _max = 437 nm). Differences in the calculated absorption spectraof the R-form could be caused by detergent effects, or waveguideeffects within the photoreceptor rhabdomere, although they morelikely are the result of the derived nature of the differencespectrum and the fact that the extinction coefficient of the R-formis approximately one-half that of the M-form. Similar analysisof the detergent-extracted Rh6 difference spectrum showed thatit was fit well by R- and M-forms having absorption maxima at515 and 468 nm, respectively (Fig. 4, bottom right). Again, themaximal absorption of the R-form differs slightly from the spectralsensitivity determined electrophysiologically ( $lambda$ _max = 508nm).

Photoactivation of rhodopsin to metarhodopsin is associated with the isomerization of the chromophore from the 11-cis to theall-trans form as well as with conformational changes within therhodopsin protein that allow it to couple to and activate theG-protein transducin. These structural changes are associatedwith changes in the absorption of the visual pigment, which arelikely to reflect changes in the interaction of the chromophorewith amino acid residues within the chromophore-binding pocket.Thus, the study of R- and M-form absorption changes in differentvisual pigments may potentially provide important insight intothe activation process. Analyses of the difference spectra obtainedfrom extracts or MSP of transgenic flies expressing Rh1-Rh4 andthe absorption spectra of the calculated R- and M-forms are shownin Figure 5. The absorption maxima for both states of each pigmentare also indicated in tabular form (Fig. 5, top right). It isinteresting to note that all of the Drosophila rhodopsins undergoa bathochromic (red) shift after photoactivation, except for Rh6that undergoes a hypsochromic (blue) shift. This hypsochromicshift in the metarhodopsin absorption of Rh6 is typical for pigmentshaving a rhodopsin absorption maxima at wavelengths longer than500 nm (Stavenga, 1989, 1992).

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Figure 5. Spectroscopy of the Drosophila Rh1-Rh4 visual pigments. Left, Middle, Difference spectra that were measured from digitonin extracts of flies expressing Rh1, Rh3, and Rh4 and ninaE¹⁷ mutant controls and MSP of flies expressing Rh2 are shown. In each case the difference spectra were calculated from spectra measured after illumination with adapting lights (using a single-adapting light and subtracting from the dark-adapted state or with $lambda$ ₁ and $lambda$ ₂ as described above), which were 461 nm (for Rh1), 418 and 524 nm (for Rh2), 344 nm (for Rh3), 384 nm (for Rh4), and 560 and 442 nm (for ninaE). Difference spectra reflecting the R $right-arrow$ M conversion were generated from flies expressing Rh1-Rh4; however no difference spectrum was generated from the ninaE¹⁷ mutant host strain. Each difference spectrum (bold trace in each panel) was fit with calculated rhodopsin and metarhodopsin absorption profiles as described in Materials and Methods (curve fits of the difference spectrum and the R- and M-forms are shown as fine traces in each panel). Table, Top Right, The calculated absorption maxima of the R- and M-forms for each pigment are indicated. The r values for the fits and the ratio of the R- and M-form extinctions $lambda$ _max were as follows: Rh1, r = 0.996 and R/M = 1:1.6; Rh2, r = 0.0.987 and R/M = 1:1.5; Rh3, r = 0.998 and R/M = 1:1.7; and Rh4, r = 0.997 and R/M = 1:1.5. Bottom Right, The calculated rhodopsin $alpha$ -band absorptions based on the absorption maxima listed in the table are shown. As discussed in the text, the calculated R- and M-form absorption maxima differ somewhat between the different measurement methods. Difference spectroscopy would be expected to yield a fairly accurate estimate of M-form absorption, because its extinction coefficient is greater than that of the R-form. In the absence of waveguide or self-screening effects, the spectral sensitivity measured physiologically would be expected to yield a fairly accurate estimate of the R-form absorption. For reference, the maximal sensitivities of flies expressing Rh1-Rh6 are 478 nm (Rh1), 420 nm (Rh2), 345 nm (Rh3), 375 nm (Rh4), 437 nm (Rh5), and 508 nm (Rh6) (Feiler et al., 1988, 1992; this paper).

Figure 5, bottom right, shows the calculated rhodopsin absorption curves for Rh1-Rh6 based on the R-form curve fits to theMSP and extract data. The Drosophila visual pigments have absorptionmaxima that differ by almost 200 nm, ranging from the UV to thegreen region of the spectrum. This remarkable range of spectralsensitivity is shared by many invertebrate organisms; howeverfruit flies are the first invertebrate organism from which thecomplete complement of all known visual pigment genes has beenexpressed and characterized indetail.

Relationship between opsins from Drosophila and other invertebrate species

To examine the relationship between the visual pigments of Drosophila and other invertebrate species, we aligned the aminoacid sequences for many of the known genes and generated a phylogenetictree to evaluate their relatedness. As shown in Figure 6, visualpigments that are thought to have similar spectral propertiesshare a high degree of structural relatedness. The Rh5 visualpigment is most similar to other opsins that are thought to beshort-wavelength absorbing, including the locust 2, bee blue,and moth Manop3 opsins, to which Rh5 is ~46, 49, and 50% identical,respectively (Fig. 6, SW clade). In contrast, Rh5 is only 30-35%identical to the Drosophila Rh1, Rh2, and Rh6 opsins and 40-44%identical to the Rh3 and Rh4 opsins. Interestingly, a subset ofthe SW-absorbing pigments appears to share a common ancestor withthe UV-absorbing pigments. The Rh6 visual pigment belongs to agroup of opsins that are proposed to form long-wavelength-absorbingrhodopsins (Fig. 6, LW clade). As with Rh5, Rh6 shares a greatersimilarity (>55%) with opsins of the LW group than with otherDrosophila opsins. Rh6 shares a 51% identity with Rh1 and Rh2and only a 30-33% identity with Rh3-Rh5 (Chou et al., 1996; Huberet al., 1997).

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Figure 6. Phylogenetic relationships between selected invertebrate opsins. The deduced amino acid sequences of cloned invertebrate opsin genes were aligned and used to generate a phylogenetic tree, as described in Materials and Methods. Both maximum parsimony (unweighted) and neighbor-joining methods were used, and the values at each node represent the percentage of 100 bootstrap replicates that yielded the indicated structure (parsimony/neighbor-joining). Nodes with bootstrap values <60% are indicated as $-$ and if <60% for both analyses were collapsed. Visual pigments were grouped into three families based on their spectral properties. The ultraviolet (UV) pigment family includes those with maximal absorptions below 400 nm. The short-wavelength (SW) family includes those pigments having maximal absorptions between 400 and 500 nm. The long-wavelength (LW) family includes those pigments with maximal absorptions above 500 nm. Inclusion within a family was based on one or more of three criteria: (1) direct characterization of the rhodopsin after ectopic expression in Drosophila, (2) well characterized spectral sensitivity or absorption measured from the native organism that is consistent with the placement within the tree, and (3) position within the phylogenetic tree with respect to other better-characterized visual pigments. The first criterion was met by Drosophila (fruit fly) Rh1-Rh6, bee blue and UV, and the horseshoe crab 1 pigments (indicated with $left-arrow$ ) (Feiler et al., 1988, 1992; Townson et al., 1998) (Knox, Salcedo, Smith, Chou, Chadwell, Britt, and Barlow, unpublished results; this paper). The second criterion was met by the following pigments. Squid 1 and 2 are thought to have a $lambda$ _max of 494 and 480 nm, respectively (Suzuki et al., 1976; Morris et al., 1993). The desert and carpenter ant UV pigments are thought to have a $lambda$ _max of 360 nm, whereas the desert and carpenter ant LW pigments are thought to have a $lambda$ _max of 510 nm (Popp et al., 1996; Smith et al., 1997). The bee green pigment is thought to have a $lambda$ _max of 526 nm (Chang et al., 1996). The octopus pigment is thought to have a $lambda$ _max of 475 nm (Koutalos et al., 1989). One or both of the crab pigments are thought to have a $lambda$ _max of ~480 nm (Sakamoto et al., 1996). The crayfish pigment appears to have a $lambda$ _max of 533 nm (Hariyama et al., 1993; Zeiger and Goldsmith, 1994). Locust 1 and 2 are thought to have a $lambda$ _max of 520 and 430 nm, respectively (Towner et al., 1997). The moth Manop1, Manop2, and Manop3 pigments are thought to have a $lambda$ _max of 520, 357, and 450 nm, respectively (Chase et al., 1997). Butterfly Pxu Rh1 and Rh2 are thought to have a $lambda$ _max of 515 nm, whereas Pxu Rh3 is thought to have a $lambda$ _max of 575 nm (Kitamoto et al., 1998; Arikawa et al., 1999). The horseshoe crab 2 pigment is thought to have a $lambda$ _max of 530 nm (Smith et al., 1993). The remaining pigments were organized on the basis of the third criterion. This group includes the visual pigments cloned from Papilio glaucus (Pgl Rh1-Rh6) that are closely related to the Pxu Rh1-Rh3 or the moth Manop1 and Manop2 opsins (Briscoe, 1998, 1999) (A. D. Briscoe, personal communication) and the Mantis opsin, which is closely related to Locust 1. The phylogenetic tree shows that opsins are typically more closely related to pigments that share similar spectral properties than to pigments from the same species. Rh5 belongs to a group of related visual pigments that appear to be SW absorbing, whereas Rh6 belongs to a class of LW-absorbing pigments. Rh6 is the first opsin of this class to be functionally characterized. GenBank accession numbers: Apis mellifera (Bee UV, AF004169; blue, AF004168; green, U26026), Camponotus abdominalis (Carpenter Ant UV, AF042788; LW, U32502), Cataglyphis bombycina (Desert Ant UV, AF042787; LW, U32501), Drosophila melanogaster (Fruit Fly Rh1, P06002; Rh2, P08099; Rh3, P04950; Rh4, P29404; Rh5, U67905; Rh6, Z86118), Hemigrapsus sanguineus (Crab Rh1, D50583; Rh2, D50584), Limulus polyphemus [Horseshoe crab 1 (lateral eye), L03781; 2 (ventral eye), L03782], Loligo forbesi (Squid 1, X56788), Octopus dofleini (Octopus, X07797), Papilio xuthus (Butterfly Pxu Rh1, AB007423; Pxu Rh2, AB007424; Pxu Rh3 AB007425), Papilio glaucus (Butterfly Pgl Rh1, AF077189; Pgl Rh2, AF077190; Pgl Rh3, AF067080; Pgl Rh4, AF077193; Pgl Rh5, AF077191; Pgl Rh6, AF077192), Procambrus clarkii (Crayfish, S53494), Schistocerca gregaria (Locust 1, X80071; Locust 2, X80072), Sphodromantis sps (Mantis, X71665), and Todarodes pacificus (Squid 2, X70498). Genome Sequence Database (GSDB) accession numbers (www.ncgr.org/cgi-bin/ff): Manduca Sexta (Moth Manop1, 76082; Manop2, 109852; Manop3, 1249561).

It is noteworthy that the only cloned invertebrate pigments that have been functionally expressed and characterized are theDrosophila rhodopsins Rh1-Rh6 (Feiler et al., 1988, 1992) (thispaper) and the honeybee blue- and UV-absorbing pigments (Townsonet al., 1998) (Fig. 6, indicated with $left-arrow$ ). This group includesa large number of the UV- and SW-absorbing pigments shown in thetree; however Rh6 is the first and only member of the LW groupto be formally characterized. As such, Rh6 both confirms and definesthis group of pigments as likely having absorption maxima at longerwavelengths of light. In other experiments, we have found thatthe more distantly related Limulus lateral eye opsin (horseshoecrab 1) also confers LW sensitivity when ectopically expressedin Drosophila (B. E. Knox, E. Salcedo, W. C. Smith, W.-H. Chou,L. V. Chadwell, S. G. Britt, and R. Barlow, unpublishedresults).

The characterization of Rh6 as an LW-absorbing invertebrate opsin is particularly important because there is a large groupof visual pigments that are within this clade. Although none ofthese pigments have been expressed and characterized, some ofthem are thought to encode red-absorbing visual pigments on thebasis of their expression pattern (e.g., Pxu Rh3) (Kitamoto etal., 1998), whereas other long-wavelength-absorbing pigments havebeen characterized spectrophotometrically but have not yet beencloned (Schwemer and Paulsen, 1973; Langer et al., 1986). In addition,it is interesting to note that many of the SW visual pigmentsare included within clades that share common ancestors eitherwith the UV visual pigments (in the case of Rh5 and its relatedpigments) or with the LW visual pigments (in the case of Rh1 andits related pigments). This suggests that there may be specificamino acid differences between the SW pigment group (like Rh5)and the UV pigments that are responsible for their different spectralproperties. Thus our analysis of the Drosophila Rh5 and Rh6 opsinsprovides a framework in which the other invertebrate pigmentscan be grouped and studied, which is based on both structuraland functional information about thepigments.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In this paper, we have described the spectral characterization of two Drosophila visual pigments, Rh5 and Rh6. Each proteinfalls into a structurally related group of rhodopsins that aredistinguished from other groups by having absorption maxima atdifferent wavelengths of light. Both Rh5 and Rh6 were ectopicallyexpressed in the R1-R6 photoreceptor cells of blind ninaE¹⁷ flies, and we found that they are capable of restoring the lightresponse of this mutant. Rh5 encodes a visual pigment that confersa maximal spectral sensitivity at 437 nm to the R1-R6 cells, whereasRh6-expressing cells are maximally sensitive to light at 508 nm.We examined the absorption properties of the Rh5 opsin in situusing MSP and in visual pigment extracts and found that it canform a thermally stable metarhodopsin ( $lambda$ _max = 494 nm) that canbe reversibly photoconverted. After activation, Rh6 is convertedto a metarhodopsin ( $lambda$ _max = 468 nm), which appears to be less stablethan the M-forms of other Drosophilarhodopsins.

The spectral and physiological properties of the Drosophila R8 photoreceptor cells have been difficult to examine becauseof their proximal location in the ommatidium and their small size.An early analysis of Drosophila photoreceptor cell function wasundertaken using adapting lights and mutations to eliminate specificclasses of photoreceptor cells (Harris et al., 1976). These studiesshowed that the R8 photoreceptor cells of Drosophila are sensitiveto blue-green light with a maximal sensitivity near 500 nm. Physiologicalstudies performed in larger flies, Calliphora or Musca, have identifiedfour different classes of R8 photoreceptor cells. Two minor classesinclude the R8marg cells, whose rhabdomeres are located beneaththose of the R7marg cells along the dorsal margin of the eye.The R8marg cells express a UV-absorbing pigment identical to thatfound in the R7marg cells (Hardie, 1984). In Drosophila, the R7margand R8marg cells express Rh3 (Fortini and Rubin, 1990; Feileret al., 1992). The R8r cells have only been found in Musca malesand express a pigment that is identical to that found in boththe R1-R6 cells and the sex-specific R7r cells whose rhabdomereslie above the R8r rhabdomeres (Hardie, 1983). The two major classesof R8 cells (R8p and R8y) are distinguished on the basis of theirpaired occurrence within ommatidia that contain the R7p or R7yphotoreceptor cells, respectively. Interestingly, we have foundthat the pairing of different classes of R7 and R8 photoreceptorcells in individual ommatidia also occurs in Drosophila. Specifically,the R7p and R8p photoreceptors correspond to the R7 and R8 cellsof Drosophila that express Rh3 and Rh5 in a pairwise manner, andR7y and R8y correspond to the Drosophila R7 and R8 cells thatexpress Rh4 and Rh6 (Chou et al., 1996, 1999). These classes ofommatidia were originally identified on the basis of their appearanceunder blue illumination and fluorescence (y for yellow; p forpale) (Kirschfeld et al., 1978; Franceschini et al., 1981). TheR8p and R8y cells of Calliphora and Musca have maximum spectralsensitivities at ~440 and 540 nm, respectively (Hardie et al.,1979; Smola and Meffert, 1979). The sensitivity of the R8y cellis thought to be shifted from the predicted rhodopsin $lambda$ _max (~520nm) to longer wavelengths (540 nm) because of the screening effectsof the overlying R7y cell rhabdomere (Hardie et al., 1979). TheR8y cells also displayed a small triplet of peaks in the UV region,indicating the presence of a sensitizing pigment similar to thatseen in the R1-R6 cells; however no UV sensitivity was found inthe R8p cells (Hardie and Kirschfeld, 1983).

The spectral sensitivities measured in the present study from transgenic flies expressing Rh5 and Rh6 are in excellent agreementwith the measurements from the R8p and R8y cells of larger flies,respectively, both in terms of their spectral sensitivities andin that Rh6 but not Rh5 appears to couple to the sensitizing pigment.Furthermore, our current results are also in good agreement withprevious studies in Drosophila. Spectral sensitivity measurementsmade from sev; ora flies, which lack the R7 photoreceptor cellsand the Rh1 opsin, demonstrated that the remaining R8 cells hadblue-green sensitivity with a maximum near 500 nm (Harris et al.,1976; Washburn and O'Tousa, 1989). Although these experimentsdid not resolve the diversity of R8 cells present in wild-typeflies, the spectral sensitivity is consistent with that of theclass of R8 cells that express Rh6 ( $lambda$ _max = 508 nm). Interestingly,in other experiments examining the basis for the paired expressionof opsin genes in the R7 and R8 cells of individual ommatidia,we have found that the expression of Rh5 versus Rh6 is dependenton the presence of an R7 cell. Indeed, in sev mutant flies (aswould be the case in sev; ora), we have found that there is adramatic decrease in the number of R8 cells that express Rh5,and virtually all of the R8 cells express Rh6 (Chou et al., 1996,1999). And just as we were unable to measure a difference spectrumby MSP in vivo or induce a PDA in transgenic flies expressingRh6, no MSP difference spectrum could be elicited from sev; oraflies, and the spectral sensitivity of sev; ora flies was unchangedby light adaptation (Harris et al., 1976). These results are consistentwith the idea that the Rh6 metarhodopsin may be short-lived andthat the primary class of R8 photoreceptor cells that is presentin sev; ora flies is that expressing Rh6. However, on the basisof the available data we cannot eliminate the possibility thatour inability to obtain an MSP spectrum and to induce a PDA inflies expressing Rh6 in R1-R6 cells simply reflects the low levelof photoconvertible rhodopsin present in the eyes of these flies.Whether or not a reduced thermal stability is characteristic ofall M-forms derived from the LW class of invertebrate rhodopsinsremains to be determined. Complete photoreversibility of the extractedpigments, i.e., photoconversion of R to M and vice versa withoutdecay of substantial amounts of rhodopsin, has only been shownat $-$ 15°C for the long-wavelength-absorbing (520 nm) visual pigmentof the moth Deilephila that forms an M-form with maximal absorbanceat 475 nm (Schwemer and Paulsen, 1973).

This work completes the characterization of all of the known, cloned, Drosophila opsin genes. Although more opsin genes maypotentially be identified as the Drosophila genome is completed,there are no known classes of photoreceptor cells that would necessarilyrequire additional genes. The characterization of Rh5 and Rh6is an important addition to the characterization of invertebratevisual pigments, because they have unique spectral propertiesand functionally define groups of related pigments that are asyet uncharacterized. As described in Results, Rh6 is the firstcloned LW-absorbing invertebrate visual pigment to be functionallycharacterized. Its position within a well supported clade of visualpigments that are thought to be LW absorbing provides the onlyavailable evidence that these genes do in fact encode LWpigments.

One of the primary interests behind the study of the invertebrate visual pigments is the study of color vision. Several invertebratespecies have been show to use color vision in specific behaviors.Honeybees are well known to use color vision in foraging and inreturning to the hive (for review, see Menzel and Muller, 1996).Swallowtail butterflies, blowflies, and the mantis shrimp havealso been shown to use color vision (Fukushi, 1985, 1989; Troje,1993; Marshall et al., 1996; Kinoshita et al., 1999). Limitedevidence suggests that Drosophila may also be able to discriminatebetween different colors (Quinn et al., 1974; Spatz et al., 1974;Menne and Spatz, 1977; Bicker and Reichert, 1978). The visualsystem of Drosophila is ideally suited to an analysis of colorvision because of the wide range of genetic and molecular approachesthat are available to identify new genes, manipulate them, andstudy the effects in vivo, in the intact fly. These approacheshave provided important insights into the basis of photoreceptorcell recruitment and phototransduction (Dickson and Hafen, 1993;Zuker, 1996; Treisman and Heberlein, 1998) and have the potentialto reveal important aspects of color vision in Drosophila. Thecharacterization of Rh1-Rh6 provides a comprehensive view of thevisual pigments and photoreceptor cell sensitivities in the Drosophilacompound eye and opens up the possibility of conducting molecularand genetic studies of color vision in a well defined, geneticallytractable experimentalsystem.

  FOOTNOTES

Received Aug. 5, 1999; revised Sept. 16, 1999; accepted Sept. 27, 1999.

This work was supported by National Eye Institute Grant R01EY10759 to S.G.B. and by funds from the European Union (BMH4-CT97-2341)to R.P. We thank J. O'Tousa for fly stocks and antibodies andA. Briscoe, R. Hardie, and D. Stavenga for comments on this manuscript.We are especially grateful to K. Kirschfeld and R. Feiler (Max-Planck-Institutfür Biologische Kybernetik, Tübingen, Germany) for helping usassemble and modify the scanning spectral sensitivity instrumentand microspectrophotometer that theydeveloped.
Correspondence should be addressed to Dr. Steven G. Britt, Departments of Cellular and Structural Biology and Ophthalmology,University of Colorado Health Sciences Center, 4200 East NinthAvenue, Box B111, Denver, CO 80262. E-mail: steve.britt{at}uchsc.edu.

Mr. Salcedo's present address: Departments of Cellular and Structural Biology and Ophthalmology, University of Colorado HealthSciences Center, 4200 East Ninth Avenue, Box B111, Denver, CO80262.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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Pubmed/NCBI databases
Gene GEO Profiles
HomoloGene UniGene
Substance via MeSH