An Extraretinally Expressed Insect Cryptochrome with Similarity to the Blue Light Photoreceptors of Mammals and Plants

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The Journal of Neuroscience, May 15, 1999, 19(10):3665-3673

An Extraretinally Expressed Insect Cryptochrome with Similarity to the Blue Light Photoreceptors of Mammals and Plants
Elizabeth S. Egan , Tina M. Franklin , Marla J. Hilderbrand-Chae , Gerard P. McNeil , Mary A. Roberts , Andrew J. Schroeder , Xiaolan Zhang, and F. Rob Jackson
Department of Neuroscience, Tufts University School of Medicine, Boston, Massachusetts 02111

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Photic entrainment of insect circadian rhythms can occur through either extraretinal (brain) or retinal photoreceptors, whichmediate sensitivity to blue light or longer wavelengths, respectively.Although visual transduction processes are well understood inthe insect retina, almost nothing is known about the extraretinalblue light photoreceptor of insects. We now have identified andcharacterized a candidate blue light photoreceptor gene in Drosophila(DCry) that is homologous to the cryptochrome (Cry) genes of mammalsand plants. The DCry gene is located in region 91F of the thirdchromosome, an interval that does not contain other genes requiredfor circadian rhythmicity. The protein encoded by DCry is ~50%identical to the CRY1 and CRY2 proteins recently discovered inmammalian species. As expected for an extraretinal photoreceptormediating circadian entrainment, DCry mRNA is expressed withinthe adult brain and can be detected within body tissues. Indeed,tissue in situ hybridization demonstrates prominent expressionin cells of the lateral brain, which are close to or coincidentwith the Drosophila clock neurons. Interestingly, DCry mRNA abundanceoscillates in a circadian manner in Drosophila head RNA extracts,and the temporal phasing of the rhythm is similar to that documentedfor the mouse Cry1 mRNA, which is expressed in clock tissues.Finally, we show that changes in DCry gene dosage are associatedpredictably with alterations of the blue light resetting responsefor the circadian rhythm of adult locomotoractivity.

Key words: circadian; cryptochrome; photoreceptor; blue light; Drosophila; extraretinal

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Molecular genetic studies in the mold Neurospora, the fruit fly Drosophila, and the mouse have shown that phylogeneticallyconserved biochemical mechanisms underly the generation of biologicalrhythms (Dunlap, 1996; Darlington et al., 1998; Gekakis et al.,1998; Hall, 1998; Young, 1998). The same analysis has culminatedin a detailed model describing the circadian timing device. Thetiming mechanism now can be described in terms of an autoregulatoryfeedback loop in which circadian changes in the abundance of clockproteins negatively regulate clock gene transcription. Similarly,the clock resetting mechanism can be understood at the molecularlevel: resetting stimuli such as light or temperature lead torapid alterations in the abundance of a clock component, effectivelyshifting the clock to a new time of day (Crosthwaite et al., 1995;Hunter-Ensor et al., 1996; Lee et al., 1996; Myers et al., 1996;Zeng et al., 1996; Liu et al., 1998; Sidote et al., 1998). However,the photopigments that function in the circadian system and thephototransduction pathways that serve to reset the circadian clocksof animal species have not yet been subjected to a detailed molecularanalysis.

Studies in the fruit fly Drosophila and other holometabolous insect species indicate that an extraretinal blue light photoreceptormediates light input to the circadian clock regulating behavioralrhythmicity (Zimmerman and Ives, 1971; Truman, 1972; Helfrich,1986; Blaschke et al., 1996; Suri et al., 1998; Yang et al., 1998).In silkmoths, for example, brain transplantation studies demonstratedthat both the circadian clock and a photoreceptor for entrainmentwere located in the CNS (Truman, 1972). Similarly, retinally blindand eyeless mutants of Drosophila retain the capacity to entrainto environmental light/dark cycles (Helfrich, 1986), indicatingthat an extraretinal photoreceptor mediates circadian resetting.Indeed, recent studies show that degradation of the timeless (TIM)clock protein, which is correlated with light-induced circadianresetting, occurs in visual transduction mutants of Drosophila(Yang et al., 1998). Finally, spectral resetting curves for theDrosophila activity rhythm show that the circadian clock is sensitiveto both blue/green light and longer wavelengths (Blaschke et al.,1996; Suri et al., 1998). Sensitivity to the two portions of thespectrum is thought to be mediated by the retinally based opsinsystem and an extraretinal blue/greenphotoreceptor.

Although the retinal phototransduction process is well understood in insects (Zuker, 1996), little is known about the molecularbasis of extraretinal (blue light) photoreception in these species.In contrast, blue light photoreception has been well characterizedin plants (Ahmad and Cashmore, 1996) and depends on photopigmentsknown as cryptochromes (CRY1 and CRY2), which are homologous toDNA repair (photoreactivating) enzymes known as photolyases butwhich themselves completely lack DNA repair activity (Ahmad andCashmore, 1993; Malhotra et al., 1995; Todo et al., 1996). Photoreceptionthrough CRY1 and CRY2 are required for many different blue lightresponses, including plant phototropism, the inhibition of hypocotylelongation, and the early photomorphogenesis of seedlings (Ahmadand Cashmore, 1993; Ahmad et al., 1998b). In addition, CRY1 alsohas been implicated in signaling pathways necessary for the circadianregulation of plant catalase expression (Zhong et al., 1997),and CRY2 functions in the photic regulation of flowering time(Guo et al., 1998). The phytochromes (PhyA and PhyB), anotherwell studied class of plant photopigments that are sensitive tored/far red light, participate in some of these photically stimulatedresponses (Zhong et al., 1997; Ahmad et al., 1998a; Guo et al.,1998), and it recently has been suggested that CRY1 physicallyinteracts with PhyA in vivo (Ahmad et al., 1998a).

Cry-gene homologs encoding related cryptochromes recently have been identified and characterized in mammalian species (Hsuet al., 1996). In the mouse, both Cry1 and Cry2 are expressedin the ganglion cell and inner nuclear layer of the retina, andit has been hypothesized that the encoded cryptochromes mediatelight input to the circadian clock in the suprachiasmatic nuclei(SCN; Miyamoto and Sancar, 1998). Interestingly, Cry1 also isexpressed in the SCN, and the mRNA oscillates in abundance duringthe circadian cycle (Miyamoto and Sancar, 1998), although therole of Cry1 in the SCN is not understood. Nonetheless, evidencefrom both plant and animal species implicates the cryptochromesin circadian photoreception. Therefore, we have characterizeda cryptochrome homolog in Drosophila to use a molecular geneticapproach to evaluate its role in circadianphotoreception.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Culture conditions and behavioral analysis. All fly stocks were obtained from the Indiana University Drosophila Stock Center(Bloomington, IN). Df(3R)Dl-BX12 removes region 91F1-2 to 92D3-6,whereas Df(3R)Cha7 is an overlapping deletion removing region90F1-4 to 91F5. To generate siblings carrying one or two copiesof the DCry⁺ gene, we crossed Df(3R)Dl-BX12/TM6B (DCry⁺) flies to w¹¹¹⁸ individuals, which carry two normal copies of the gene. Cultureswere reared on Drosophila cornmeal medium according to standardlab procedures (Newby and Jackson, 1993). Adult activity rhythmswere monitored and light-induced phase shifts were calculatedas previously described (Newby and Jackson, 1993; Levine et al.,1994). Blue light pulses of ~200 lux were delivered by using aKodak 47B wratten filter with a peak transmittance at 430 nm.This filter has <0.1% transmittance at wavelengths above 500nm.

RNA and DNA analyses. The Drosophila Canton-Special (C-S) strain was used for all Northern, Southern, and RNase protectionstudies. All three procedures were performed exactly as previouslydescribed (Newby and Jackson, 1993, 1996). RNA was prepared fromdifferent developmental stages and tissues according to standardprocedures (see Newby and Jackson, 1993). Samples of adult headsand bodies were prepared by freeze-fracturing adult flies (previouslyfrozen at $-$ 80°C) and separating the different body parts by sievingon ice in the cold (4°C).

RNase protection analysis was used to examine the expression of DCry RNA in different tissues and to characterize daily changesin abundance. To characterize oscillations in DCry RNA abundance,we entrained flies to a cycle of 12 hr of light and 12 hr of dark(LD 12:12) for 4-5 d before collection. As probes, we used invitro transcribed [³²P]-labeled RNAs representing a 264 base pair (bp) fragment fromthe 5' end of the HL03779 cDNA clone and a 112 bp fragment representingthe rp49 RNA. RNA probes representing DCry and rp49 were annealedovernight at 42°C to 10 µg of total RNA, and RNA/RNA duplexesthen were digested at 37°C for 1 hr with a cocktail of RNase Aand T1 according to the manufacturer's instructions (Ambion, Austin,TX). The sizes of protected fragments were determined by denaturingpolyacrylamide electrophoresis, using MspI-digested pBR322 DNAsas size standards. Gels were subjected to film autoradiography,and signals were quantitated exactly as previously described (McNeilet al., 1998) by densitometric scanning of films. DCry RNA abundancewas quantified relative to rp49 abundance, which does not changeduring the diurnalcycle.

Probes representing the HL03779 or GM03047 (Drosophila 6-4 photolyase) cDNAs were [³²P]-labeled by random hexamer priming for use in Northern analysis.A labeled rp49 probe (see above) was used as a control for gelloading. Probes were hybridized to RNA blots containing 5 µg poly(A⁺) RNA or 20 µg of total RNA per lane. Hybridizations contained~0.25-1 × 10⁶ cpm probe/ml and were performed in ExpressHyb solution (Clontech,Palo Alto, CA) for 2 hr or overnight at 45°C (DNA probes) or 65°C(rp49 probe). Then the blots were washed three times (15 min each)at room temperature (~23°C) and twice (30 min each) at 50°C beforefilm autoradiography at $-$ 80°C to detect hybridizationsignals.

We performed in situ hybridization of sense and antisense DCry probes to paraffin-embedded adult tissues, using standard methods(Lehmann and Tautz, 1994). Adults were collected at the middleof the subjective day, which corresponds to the high point ofDCry RNA abundance (see Results). A 300 bp digoxigenin-labeledRNA probe representing bases 1524-1823 of the HL03779 cDNA wasgenerated for thesestudies.

Chromosome in situ hybridizations were performed as described by Engels et al. (1986). A cDNA fragment representing the entireHL03779 clone was labeled with Biotin-dATP by nick translationand was used in chromosome localization. Chromosomes were stainedlightly with Giemsa (0.4%; Sigma, St. Louis, MO) after the detectionreaction. The polytene chromosome maps of Sorsa (1988) were usedto localize the position of the DCrygene.

Sequence comparisons. Comparisons of protein sequences were performed with the software of the Genetics Computer Group (WisconsinPackage Version 9.0, Genetics Computer Group, Madison, WI). Directcomparisons among DCry and hCRY1 and hCRY2 were performed by theGAP program with a gap weight of 12 and length weight of 4. Themultiple sequence alignment was constructed by using PILEUP witha gap creation penalty of 12 and a gap extension penalty of 4.Sequences were displayed by using PRETTY, and the shading of aminoacid residues was accomplished with Microsoft Word. Distance matriceswere generated by either DISTANCES or OLDDISTANCES, using theKimura method of corrected multiple substitutions. A similarityplot for full-length sequences was generated with OLDDISTANCESand a threshold of 2; identity was calculated with a thresholdof 4. The phylogram was produced with GROWTREE to generate a UPGMAtree, using a DISTANCES matrix for full-length proteins. Resamplingof the data set with the bootstrapping technique yielded treesthat were essentially the same as that shown in Figure 1.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Identification and sequence of a Drosophila cryptochrome-like gene

On the basis of the reported sequences of mouse and human cryptochromes, we searched the Berkeley Drosophila Genome Project(BDGP) expressed sequence tag (EST) database for similar genesin Drosophila. A number of cDNA clones representing two differentDrosophila genes were identified in the initial search. One ofthese genes is the Drosophila 6-4 photolyase, which previouslywas reported to be similar to blue light photoreceptors (Todoet al., 1996). This gene is expressed at high levels only in femaleovaries, consistent with the known photolyase activity of itsencoded product and its role in the photoreactivation of damagedDNA (Todo et al., 1996). The second Drosophila gene, however,was identified from an EST representing a novel cDNA clone froma head cDNA library. That gene is represented in the BDGP databaseby two cDNA clones. One of those clones (HL03779), which appearedto contain the entire translational open reading frame, was obtainedfrom Genome Systems and sequenced in its entirety. Not countinga polyA tail of 20 adenylate residues (As), the sequence is 1823bp in length and contains a consensus polyadenylation signal atbp 1801 and an open reading frame between bp 121 and 1746 thatpredicts a cryptochrome-like protein of 542 amino acids (Fig.1A). This protein is ~50% similar and 40% identical to eitherhCRY1 or hCRY2 in direct sequence comparisons (using the GeneticsComputer Group GAP program; see Materials and Methods). Therefore,we provisionally designated the fly protein DCry for Drosophilacryptochrome and the relevant gene DCry.

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Figure 1. Sequence of a Drosophila cryptochrome-like protein and comparison to cryptochrome and photolyase sequences from several other organisms. A, Comparison of DCry to the human cryptochromes hCRY1 and hCRY2. Gray highlighting indicates residues in cryptochrome and photolyase sequences that are identical to the new Drosophila cryptochrome-like sequence. Circles, squares, and stars indicate similarities to the Escherichia coli PHR protein. Open and filled squares indicate positions that are similar and identical, respectively, to residues known to be important for folate binding. Open and filled circles indicate positions with similarity and identity, respectively, to residues important for FAD binding. Stars indicate tryptophan (W) residues that are conserved in all blue light photoreceptors and photolyases. The first W is known to be important for CPD binding to E. coli PHR; the second is thought to be important for electron transfer involving FAD. B, Phylogram indicating relatedness of mammalian, insect, plant, and microbial cryptochromes and 6-4 photolyases. hCRY1, Human cryptochrome 1 (accession D83702); hCRY2, human cryptochrome 2 (accession AB014558); D6-4, Drosophila 6-4 photolyase (accession S74530); At6-4, Arabidopsis 6-4 photolyase (accession AB003687); AtCRY1, Arabidopsis cryptochrome 1 (accession S66909); AtCRY2, Arabidopsis cryptochrome 2 (accession U43397); SaPHR, Sinapsis alba cryptochrome (accession P40115); CrPHR, Chlamydomonas reinhardtii cryptochrome (accession S57795); EcPHR, E. coli PHR photolyase (accession P00914); AnPHR, Anacystis nidulans PHR (accession P05327); ScPHR, Saccharomyces cerevisiae PHR (accession P05066).

Cryptochromes are members of a large protein family that includes blue light photoreceptors, 6-4 photolyases (DNA photoreactivatingenzymes), and microbial Class I CPD (cyclobutane pyrimidine dimers)photolyases (Ahmad and Cashmore, 1993; Malhotra et al., 1995;Todo et al., 1996). Figure 1A shows the predicted sequence ofDCry and a comparison of the fly protein to the human CRY1 andCRY2 proteins. As indicated in the Distances Matrix of Table 1(see Materials and Methods), DCry is most similar to the humancryptochromes, with similarities of 46 and 45% to hCRY1 and hCRY2,respectively. DCry is more similar to mammalian cryptochromesthan plant cryptochromes or Class I CPD photolyases, the latterexhibiting similarities ranging from 23 to 30% (Table 1). Thegeneration of a phylogram for 12 different cryptochromes and photolyases(see Materials and Methods) underscores the relatedness of DCryto the hCRY1 and hCRY2 proteins (Fig. 1B), although DCry alsois related similarly to both the Drosophila and Arabidopsis 6-4photolyases. There is little or no homology among DCry and highereukaryotic Class II CPD photolyases (data not shown in Table 1or Fig. 1). Therefore, DCry can be considered a new member ofthe protein subfamily that includes mammalian cryptochromes and6-4 photolyases. The aggregate of our comparisons is consistentwith the idea that DCry functions as a blue light photoreceptorrather than a photolyase. This conclusion is supported by thefunctional analysis described below, which indicates that theDCry protein mediates blue light resetting of the Drosophila circadianclock.


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Table 1. Distance matrix for photolyase and Cry proteins*

Similar to other cryptochromes, DCry has conserved domains that include residues known to be important for the noncovalentbinding of the cofactors pterin (folate) and flavin adenine dinucleotide(FAD; see Fig. 1 legend). In plant and mammalian cryptochromes,these cofactors determine light absorption spectra (Lin et al.,1995; Malhotra et al., 1995; Hsu et al., 1996). Also like othercryptochromes, the DCry protein has a nonconserved C terminus(of 41 residues) that is completely unrelated to photolyases,cryptochromes, or any other sequence in the protein databases.It has been suggested that the novel C termini of cryptochromesmight be important for interactions with effector molecules (Hsuet al., 1996), and it has been demonstrated that the C terminusof the human CRY2 protein can physically interact with and inhibitthe phosphatase activity of the tetratricopeptide repeat (TPR)-containingprotein PP5 (Zhao and Sancar, 1997). The DCry protein does notcontain an N-terminal extension similar to those of microbialand plant photolyases that have been implicated in mitochondrialand nuclear targeting (Yasui et al., 1992).

A single Drosophila Cry gene maps to chromosome region 91F

Because there are two Cry genes present in the genomes of certain plants and mammals, we wondered whether additional cryptochromegenes existed in Drosophila. Southern hybridizations at reducedstringency, however, revealed genomic fragments correspondingto the new Drosophila cryptochrome-like gene or to the Drosophila6-4 photolyase gene, but no additional hybridizing fragments wereobserved (data not shown). Therefore, there is no evidence foradditional genes, although we cannot exclude the possibility ofmore highly divergent fly cryptochrome-like genes. However, bothin humans and Arabidopsis, the two Cry genes are much more similarto each other than they are to their counterparts in the otherspecies (see Table 1). This also suggests that the Cry gene pairsof these different species evolved from independent duplicationevents after the divergence of plants andanimals.

There are a number of Drosophila rhythm genes that have not been characterized molecularly (see Jackson, 1993). Because wewondered whether any of them corresponded to DCry, we determinedthe cytogenetic location of the Drosophila gene by hybridizationof cDNA sequences to larval salivary gland polytene chromosomes(see Materials and Methods). A single site of hybridization wasobserved within polytene region 91F of the third chromosome distalto band 91F5 (Fig. 2). No circadian rhythm genes besides DCryhave been mapped to this cytogenetic interval.

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Figure 2. Cytogenetic localization of the DCry gene. The arrow points to region 91F of the third chromosome. The numbers indicate adjacent chromosomal intervals.

The DCry mRNA is expressed in the adult brain and other nonretinal tissues

The HL03779 cDNA clone was isolated from a fly cDNA library generated from brain and sensory organ RNA (Berkeley DrosophilaGenome Project/HHMI EST Project; unpublished data), and we haveconfirmed that the DCry mRNA is expressed in head tissues. Inhead RNA preparations a doublet of ~2 kb is detected in eithertotal RNA or poly(A⁺) RNA fractions (Fig. 3A; data not shown). As the HL03779 cDNAis 1823 bp in length and most mRNAs contain 100-200 As at their3' end, we assume that this clone represents most or all of theDCry mRNA sequence.

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Figure 3. Tissue and developmental expression of DCry mRNA. A, Northern analysis showing expression in head and body tissues. H denotes 5 µg of head poly(A⁺) RNA; B denotes 5 µg of body poly(A⁺) RNA. Size markers indicate the DCry mRNA doublet (2 kb) and rp49 mRNA (0.6 kb). B, RNase protection analysis of DCry expression in different tissues and developmental stages. Protected bands representing DCry and control rp49 mRNAs are indicated. Br, Adult brain; E, 0-24 hr embryo; L, third instar larva; 3Br, third instar larval brain; B, body. The body preparation used for RNase protection analysis was examined by light microscopy to be certain that no contaminating heads were present. C, In situ hybridization to a horizontal section of an adult head. The arrow indicates the position of DCry-expressing cells in the lateral CNS. The arrowheads show specific signal in other portions of the brain. The star indicates nonspecific staining, which also was seen with the sense probe. A similar spatial pattern of expression was observed in two independent experiments. R, Retina; L, optic lamina; M, optic medulla; Lo, lobula.

In contrast to DCry expression, a probe representing the Drosophila 6-4 photolyase gene (see Materials and Methods) did notdetect a signal when hybridized to a Northern containing the samehead RNA preparations (data not shown). This result is not surprising,because our database searches found 6-4 photolyase-homologouscDNAs only in an EST collection representing a Drosophila ovarycDNA library. As previously reported (Todo et al., 1996), thefly 6-4 photolyase gene is expressed at significant levels onlyin ovarytissues.

We used RNase protection methods to examine various developmental stages and tissues for DCry expression. To determine whetherthe DCry RNA was expressed in the brain, we prepared RNA samplesfrom hand-dissected adult brains, which were completely devoidof eyes and ocelli. As judged by the control rp49 signal (Fig.3B, lane Br), DCry mRNA can be detected in a modest amount oftotal RNA (lane Br), indicating that the message is enriched inthe brain. This result also demonstrates that the message is expressedin an extraretinal manner and suggests that it encodes the cryptochromemediating circadian photoreception. Consistent with expressionin the brain, DCry mRNA was detected readily in head tissues ofeyes absent (eya) mutants, which entirely lack compound eyes (datanot shown). Interestingly, DCry mRNA can be detected in body tissues(lane B in Fig. 3A,B), which previously have been shown to containphotoreceptive clocks (Plautz et al., 1997), although the relativeabundance of the mRNA is apparently lower in the body. Finally,DCry message could not be detected in moderate-to-large amountsof total RNA from 0-24 hr embryos (Fig. 3B, lane E), whole thirdinstar larvae (lane L), or third instar larval brains (lane 3Br),suggesting that a different photoreceptor might mediate circadianresetting at these developmentalstages.

In situ hybridization techniques were used to examine the spatial localization of DCry mRNA within the adult nervous system.As shown in Figure 3C, a low level of expression could be detectedthroughout the cell body layer of the CNS (see arrowheads in Fig.3C). A much stronger signal, however, was observed in large cellsof the lateral CNS (Fig. 3C, arrow), which are close to or coincidentwith the ventral group of Drosophila clock neurons (see Discussion).Specific expression also was detected in adult non-neural tissues,including the gut (data not shown). Importantly, sections hybridizedwith a DCry sense probe did not show any signal within brain orgut cells (data not shown). A small amount of reaction productwas observed within the retina (R) with both the sense and antisenseDCry probes; thus, we conclude there is no specific signal forDCry mRNA within retinaltissues.

The DCry mRNA oscillates in abundance during the circadian cycle

As the mouse Cry1 mRNA had been reported to oscillate in abundance during the diurnal cycle, we determined whether the samemight be true of the DCry mRNA. As shown in Figure 4, the DCrymessage is more abundant in head RNA samples during the day thanat night, relative to rp49 abundance, which does not change duringthe diurnal cycle (Hardin et al., 1990). In two independent experiments,DCry mRNA was 6- and 11-fold more abundant at peak during theday than it was at the trough of the rhythm during the night (Fig.4B). Indeed, the amplitude of the DCry rhythm was greater thanthat observed for the mouse Cry1 mRNA, which oscillates in abundancein the suprachiasmatic nuclei (SCN; Miyamoto and Sancar, 1998).Additional experiments showed that DCry mRNA did not show immediateincreases in abundance in response to the lights-on signal (datanot shown), indicating that DCry gene expression is not light-inducible.Similar to mouse Cry1 mRNA, the rhythm in DCry abundance persistedin constant conditions (Fig. 4C), demonstrating that it is undercircadian regulation.

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Figure 4. The DCry mRNA oscillates in abundance in head tissues during the diurnal cycle. A, RNase protection gel showing the relative abundances of DCry (above) and rp49 (below) RNAs at different times of the day. Numbers above the gel indicate zeitgeber time (ZT, in hours). B, Quantitation of DCry RNA abundance relative to rp49 abundance in two independent LD experiments. The open and filled rectangles above A and B show the light and dark portions of the LD 12/12 cycle to which adults were entrained. Numbers refer to zeitgeber time (ZT). Similar results were obtained in two other experiments. C, Quantitation of DCry RNA abundance in constant darkness (DD). Numbers refer to circadian time (CT). Data are shown for two independent experiments. In two other DD experiments not shown here, similar circadian changes in RNA abundance were documented, although peak RNA abundance was several hours earlier than that shown in C. In those experiments RNA abundance changed by approximately four- to fivefold during the circadian cycle.

Changes in DCry gene dosage affect the blue light resetting response

We conducted behavioral genetic experiments to test the notion that the Drosophila cryptochrome mediates blue light resettingof the circadian clock. As a prelude to these experiments, wefirst examined blue light resetting in normal flies. As shownin Figure 5A, normal individuals exhibited phase shifts of increasingmagnitude in response to ~200 lux blue light pulses of increasingduration. Flies receiving 5 min of blue light (5 min b) or 5 minof 2500 lux white light (5 min w) exhibited phase delays of identicalmagnitude, suggesting that this duration of blue light constituteda saturating light pulse. Importantly, these data indicate that10 sec and 1 min pulses of blue light cause submaximal phase shifts,and thus such resetting pulses might be appropriate for detectingbehavioral alterations that result from changes in DCry gene dosage.

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Figure 5. Blue light resetting responses in normal flies and individuals deficient for DCry gene product. A, Average phase delays (hr ± SEM) of w¹¹¹⁸ flies (DCry⁺/DCry⁺) in response to blue light pulses of ~200 lux ranging from 1 sec to 5 min. Flies receiving pulses for 5 min saw either blue light (5 min b) or full spectrum white light of ~2500 lux (5 min w). Sample sizes ranged from 7 to 13 flies per group. B, Phase delays of Df(3R)Dl-BX12/+ and +/+ siblings at three different pulse durations. For the 10 sec and 1 and 5 min pulses, respectively, we examined 11, 10, and 6 flies for Df(3R)Dl-BX12/+ and 14, 15, and 10 flies for the +/+ siblings. *p < 0.001 as compared with +/+ siblings. Both Df(3R)Dl-BX12/+ and +/+ siblings had white eye color, similar to the w¹¹¹⁸ flies of A. The average phase delay values shown in A and B were corrected by subtracting the small phase delay that results after transfer from LD to DD (Levine et al., 1994). The negative phase delay value for Df(3R)Dl-BX12/+ flies indicates that the delay that followed the LD to DD transition was actually slightly larger than the delay induced by the blue light pulse; effectively, these flies showed no phase delay in response to the 10 sec pulse. Even without the usual correction, however, the difference between deletion-bearing flies and siblings was statistically significant.

To determine whether changing DCry dosage affected blue light resetting, we characterized the resetting responses of fliescarrying one or two doses of the gene. We used two different thirdchromosome deletions in these experiments: Df(3R)Dl-BX12 and Df(3R)Cha7.Based on our localization of the DCry gene (in distal 91F), theDl-BX12 deletion was predicted to remove the gene, whereas Cha7was expected to delete a region adjacent to the gene (see Materialsand Methods). Control flies heterozygous for the Cha7 deletionexhibited phase delays at all three pulse durations that werewithin the wild-type range and not significantly different fromthose of normal flies (data not shown), which confirmed that thisdeletion did not remove the DCry gene. For Df(3R)Dl-BX12, resettingresponses were characterized in sibling flies of similar geneticbackground (see Materials and Methods), which were either heterozygousfor the deletion (Df/+) or homozygous for the normal DCry⁺ allele (+/+). As shown in Figure 5B, flies heterozygous for Df(3R)Dl-BX12had significantly smaller phase delays than normal siblings inresponse to a 10 sec pulse of blue light (p < 0.001). Phase delaysfor such flies were progressively larger in response to longerpulses (Fig. 5B), but not significantly different from those ofsiblings, presumably because the system was at or near saturationat the longer pulse durations. These data indicate that fliesdeficient for DCry product have decrements in blue lightresetting.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Identification of a Drosophila Cry homolog

Cryptochrome (Cry) proteins lacking photolyase activity have been identified in mammals and plants (Ahmad and Cashmore, 1993;Malhotra et al., 1995), and these proteins have been demonstratedto mediate blue light photoreception in Arabidopsis. We have identifiedand characterized a new Drosophila gene (DCry) encoding a cryptochromeprotein (DCry) with significant similarity to the cryptochromespreviously described in plant and animal species. Although DCryalso has similarity to 6-4 photolyase proteins, it is most similarto the mammalian cryptochromes (hCRY1 and hCRY2) that have beenimplicated in circadian photoreception (Miyamoto and Sancar, 1998).

Given that the DCry gene is expressed in Drosophila brain and body tissues, we postulate that the encoded protein serves asthe extraretinal blue light photoreceptor mediating the entrainmentof circadian behavioral rhythms. Previous studies have indicatedthat a circadian photoreceptor is localized in the insect brain(Truman, 1972; Helfrich, 1986), and recent work has demonstratedthe existence of photoreceptive circadian clocks in a varietyof Drosophila tissues (Plautz et al., 1997). Consistent with arole for cryptochrome in light resetting of the circadian clock,Drosophila strains that are deficient for DCry product show correlatedchanges in the resetting response to blue light. In addition,work reported by Stanewsky et al. (1998a) indicates that a mutationin the DCry gene we have characterized leads to altered lightresetting of circadian rhythms. The aggregate of these resultssuggests that the DCry photoreceptor mediates extraretinal lightinput to the Drosophila circadian clock. Because brain-localizedphotoreceptors mediate clock resetting in other holometabolousinsect species (Truman, 1972), it is likely that cryptochromessimilar to DCry function in circadian phototransduction in suchspecies.

How might Cry-mediated phototransduction reset the circadian clock?

Although DCry mRNA is expressed within the CNS, the identities of the cell types relevant for extraretinal photoreceptionhave not been positively determined. However, relative to otherparts of the nervous system, DCry mRNA is expressed at high levelsin large cells of the lateral CNS. Although we have not yet performeddouble-labeling experiments with clock cell antibodies, on thebasis of the size and position of the hybridizing cells we postulatethat they correspond to the ventral group of the so-called "lateralclock neurons." These cells are known to be critical for circadianfunction (Frisch et al., 1994; Helfrich-Förster, 1998) and containthe clock proteins Period and Timeless (Young, 1998) as well asa neuropeptide known as pigment-dispersing hormone (PDH; Helfrich-Förster,1995). We hypothesize that the clock neurons themselves are directlylight-sensitive by virtue of containing the DCry cryptochrome.Perhaps less likely, DCry protein might be localized within dedicatedcircadian photoreceptor cells that are close to the clock neuronsand innervatethem.

The signaling pathway that transduces light information from Cry proteins to the clock mechanism has not been elucidated inany species. In Drosophila such a signaling mechanism ultimatelymust result in the degradation of Timeless (TIM) protein, whichserves as the sensor for light input to the clock (Hunter-Ensoret al., 1996; Lee et al., 1996; Myers et al., 1996; Zeng et al.,1996). Thus, Cry-mediated phototransduction must involve the activationof an appropriate protease, perhaps indirectly via a kinase orphosphatase intermediary. In this regard, it is of interest thatZhao and Sancar (1997) have shown that human CRY proteins caninteract with members of the TPR family of proteins, includingserine/threonine phosphatase 5 (PP5). Moreover, the activity ofPP5 can be inhibited by interaction with hCRY proteins, althoughthe observed inhibition is not light-dependent (Zhao and Sancar,1997). It also is known that there is a blue light-mediated andCRY-dependent autophosphorylation of an Arabidopsis protein kinaseknown as NPH1 (Ahmad et al., 1998b). Therefore, it is reasonableto suppose that a light-induced alteration of a specific phosphataseand/or protein kinase might be required for the activation ofthe protease that mediates Drosophila TIMdegradation.

Circadian oscillations in DCry mRNA abundance

DCry mRNA abundance changes in a circadian manner, with peaks of abundance occurring during the photoperiod of a light/darkcycle. Although the daily phasing of the DCry cycle is similarin Drosophila and the mouse (Miyamoto and Sancar, 1998), the significanceof the RNA oscillation is not understood in either species. Indeed,one would expect the abundance of a photoreceptor protein eitherto be constant during the circadian cycle or to be higher duringthe night, at the time when the clock is maximally sensitive toresetting stimuli. This could be the case for DCry protein ifthere is a temporal lag in translation of the DCry message. Alternatively,the DCry rhythm might be required for another aspect of circadianclock function in addition tophotoreception.

Although Cry rhythmicity might be relevant to circadian photoreception or another circadian function, it is also possiblethat the mammalian and Drosophila Cry rhythms reflect the ancestralphotolyase activity of the proteins. For photolyases, a higherDNA repair activity might be advantageous during the photoperiod.In this regard, it is known that the expression of certain photolyasegenes can be induced by light (Batschauer, 1993; Ahmad et al.,1997), although it is unclear whether the expression of thesegenes is under clock control. Irrespective of the physiologicalsignificance of the Cry mRNA rhythm, the remarkable similarityin the phasing of rhythmicity in different species suggests aconservation of function and/or gene regulatory mechanisms. Amore detailed molecular genetic analysis of the DCry RNA rhythmmay yield insights about itsfunction.

Note. While this paper was in review, other labs reported the genetic and molecular characterization of the Drosophila DCrygene (Emery et al., 1998; Stanewsky et al., 1998b). Their workreports the behavioral analysis of a DCry mutant and providesadditional molecular evidence that DCry protein functions as acircadianphotoreceptor.

  FOOTNOTES

Received Oct. 14, 1998; revised Feb. 11, 1999; accepted Feb. 17, 1999.

This work was supported by grants from the National Institutes of Health and National Science Foundation. We thank Yin Xuand Dale Hunter for performing tissue in situ hybridizations,Mike Byrne and the Tufts Biochemistry Facility for help with DNAsequencing, Rob Willson of the Tufts Imaging Facility for densitometricscanning of films, and Jeff Hall for communicating unpublishedresults. We also thank the Flybase consortium, the Berkeley DrosophilaGenome Project, and the Indiana University Drosophila Stock Centerfor access to database information and fly stocks. The DNA sequenceof cDNA clone HL03779 and the predicted protein sequence havebeen deposited inGenBank.
All authors contributed equally to this work; with the exception of the corresponding author (F.R.J.), they are listedalphabetically.

Correspondence should be addressed to Dr. F. Rob Jackson, Department of Neuroscience, Tufts University School of Medicine,136 Harrison Avenue, Boston, MA02111.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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