Nuclear Entry Mechanism of Rat PER2 (rPER2): Role of rPER2 in Nuclear Localization of CRY Protein

doi:10.1128/MCB.21.19.6651-6659.2001

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Molecular and Cellular Biology, October 2001, p. 6651-6659, Vol. 21, No. 19
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.19.6651-6659.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Nuclear Entry Mechanism of Rat PER2 (rPER2): Role of rPER2 in Nuclear Localization of CRY Protein

Koyomi Miyazaki,¹ Miho Mesaki,¹ and Norio Ishida¹^,²^,^*

Clock Cell Biology Group, Institute of Molecular and Cell Biology, National Institute of Advanced Industrial Science and Technology, Tsukuba, Ibaraki 305-8566,¹ and Faculty of Bioscience and Biotechnology, Tokyo Institute of Technology, Midoriku, Yokohama 226-8501,² Japan

Received 6 June 2001/Accepted 2 July 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Mammalian PERIOD2 protein (PER2) is the product of a clock gene that controls circadian rhythms, because PER2-deficient micehave an arrhythmic phenotype. The nuclear entry regulation ofclock gene products is a key step in proper circadian rhythm formationin both Drosophila and mammals, because the periodic transcriptionof clock genes is controlled by an intracellular, oscillating,negative feedback loop. The present study used deletion mutantsof rat PER2 (rPER2) to identify the functional nuclear localizationsignal (NLS) in rPER2. The elimination of putative NLS (residues778 to 794) from the rPER2 fragment resulted in the loss of nuclearentry activity. Adding the NLS to the cytosolic protein (bacterialalkaline phosphatase) translocates the fusion protein to the nuclei.The data indicate the presence of a functional NLS in rPER2. Furthermore,intact rPER2 was preferentially translocated from the cytoplasmto the nucleus when coexpressed with human CRY1 (hCRY1). However,rPER2 mutants lacking a carboxyl-terminal domain could not enterthe nucleus even in the presence of hCRY1. In addition, coexpressionof the nuclear localization domain (residues 512 to 794) lackingrPER2 and CRY1 changed the subcellular localization of CRY1 fromthe nucleus to the cytoplasm. In vitro protein interaction studiesdemonstrated that the carboxyl-terminal domain of rPER2 is essentialfor binding to CRY1. The data suggested that both the rPER2 NLSand carboxyl-terminal CRY binding domain are essential for nuclearentry of the rPER2-CRY1complex.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Circadian rhythms in organisms ranging from bacteria to humans are driven by endogenous biological clocks that regulate manybiochemical, physiological, and behavioral processes with approximate24-h periodicity (3). Three mammalian period genes (per1, per2,and per3) that resemble the clock-regulating gene of Drosophilamelanogaster, period (per) (1, 19, 21-23, 29), have beencloned. Structural similarity indicated that the mammalian genesare components of a central oscillating mechanism. Transcriptlevels of all three per genes oscillate in the hypothalamic suprachiasmaticnucleus (SCN), where the principal mammalian circadian oscillatorlies (8), as well as in peripheral tissues (2, 6, 15,29). Among the three putative mammalian homologues, the per2gene encodes a functional component of the mammalian clock, becausemPER2^brdm1 mutant mice lose circadian rhythms 2 weeks after release intoconstant darkness (28).

Circadian clocks are also apparently located in the peripheral tissues of mammals that are synchronized by the SCN (2,6, 15, 22, 23). In both SCN and peripheral tissues, clock-relatedgene products including PER proteins precisely oscillate, andthis oscillation is required to generate circadian rhythms (4,10, 13, 17). Even in cultured cells, serum shock can inducethe rhythmic expression of clock genes and clock-controlled genes(2), indicating that individual cells contain a set of moleculesthat drive their ownoscillator.

Molecular dissection has revealed that circadian oscillation is driven by a transcription- and translation-based negativefeedback loop, wherein positive elements induce the expressionof negative regulators that in turn inhibit the transactivationof positive regulators (3). Thus, the timing of nuclear entryis critical to maintain the correct time of the biological clockin both Drosophila and mammals. In Drosophila, Drosophila PER(dPER) and dTIMELESS (dTIM) are located in the nuclei of pacemakercells at night but not during the day. These two molecules accumulatein the cytoplasm until heterodimerization, which is a triggerfor the nuclear entry of this complex that inhibits CLOCK/BMALtransactivation after dPER/dTIM expression decreases (14).

Mammalian PER proteins localize in the nucleus of SCN cells (5) and partially inhibit CLOCK-BMAL-dependent transactivation(7), which may proceed in the nucleus. Mammalian CRY proteins(CRY1 and CRY2), which were originally considered blue-light photoreceptors(cryptochromes), are essential components of the central clockmechanism, because mice lacking both murine CRY1 (mCRY1) and mCRY2completely lose circadian rhythms (25). Kume et al. found thatmCRY1 and mCRY2 form a complex with mouse PERs (mPERs) and appearedto facilitate the nuclear entry of mPERs (10). However, thenuclear entry mechanism and the binding domain of this complexhave not been clarified. Another report suggested that nuclearentry can be accomplished by serum shock-induced heterodimerizationof mPER1 and mPER2 with mPER3 (27). On the other hand, the phosphorylationof PER proteins by casein kinase I $varepsilon$ can modulate the nuclear localizationof mPER1 and mPER3 but not of mPER2 (20, 26). These findingsindicate that the pathway by which mPERs enter the nucleus ismore complicated than that of Drosophila (14).

The domain structures of PER2 protein are predicted from the primary sequence. Based on the similarity of sequences to dPER,mammalian PER2 has PAS (PER-ARNT-SIM) domains near the amino terminus,which can interact with and regulate the activity of PAS domaintranscriptional factors, such as CLOCK and BMAL (1, 15, 21).The region similar to the dPER cytoplasmic localization domainis located at the carboxyl region of the PAS domain (21). Thenuclear localization signals (NLS) in mPER1 (26) and mPER3 (27)have been identified; the functional NLS in mPER2 remains unknown.Computer-aided motif prediction programs show a bipartite-typeNLS in mPER2 and rat PER2 (rPER2) (15, 18).

Therefore, the nuclear entry mechanism of rPER2 was studied intensively by making deletion constructs. First, we developedsystems with which to express truncated rPER2 protein in COS-1cells and identified the sequence required for its nuclear localization.The nuclear import of cytosolic protein tagged with rPER2 NLSwas observed. Coexpression of rPER2 with human CRY1 (hCRY1) inducedthe nuclear localization of both proteins. Deletion at the nuclearlocalization domain (NLD), which includes the NLS at the C terminusor carboxyl-terminal domain inhibited rPER2 nuclear localizationfacilitated by hCRY1. Subcellular localization analysis of hCRY1and binding assays of each protein showed that the carboxyl-terminaldomain of rPER2 is necessary for binding CRY1 and that the NLDof rPER2 is important in establishing the nuclear accumulationof both rPER2 andhCRY1.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Construction of plasmids for overexpression. To generate the rPER2 expression plasmid, cDNA encoding rPER2 (GenBank accession no. AB016532 [15]) was subcloned intothe CAG-promoter-driven expression vector pCXN2 (a gift from J.Miyazaki [12]). The precise deletions of rPER2 were achievedusing conventional restriction enzyme digestion and ligation.The FLAG-tagged carboxyl-terminal fragment of rPER2 was generatedby excising the MroI-to-BglII (acids 1638 to 3878) or MroI-to-SmaI(acids 1638 to 3576) fragments of pCXN2-rPER2 and blunting andre-ligating them into the SmaI site of pFLAG-CMV2 (Sigma). TheNLD and CRY1 binding domain fragments were amplified using oligonucleotideswith EcoRI or BamHI sites and were sequenced and ligated intopFLAG-CMV2. rPER2 NLS insertion into the carboxyl-terminal endof bacterial alkaline phosphatase (BAP) was carried out by PCRamplification with oligonucleotides containing rPER2 nucleotidesequences coding the NLS. All constructs were verified by sequenceanalysis. hCRY1 was expressed by the plasmid pcDNA3.1-His (Invitrogen)containing the coding region for hCRY1 (GenBank accession no.NM004075). This expression plasmid was a gift from T.Todo.

Cell culture and transfection. COS-1 cells were maintained in Dulbecco's modified Eagle's medium supplemented with 10% fetal calf serum and antibiotics in5% CO₂. Cells were seeded in 6- or 12-well plates, were culturedovernight to 30 to 50% confluence, and were then transfected with1 or 0.5 µg of total plasmid DNA, respectively, using Fugene6(Roche) according to the manufacturer's instructions. After 48h, transfected cells were assayed as describedbelow.

To determine the molecular sizes of overexpressed proteins, transfected cells were rinsed with phosphate-buffered saline (PBS)twice, lysed with sodium dodecyl sulfate (SDS) sample buffer,resolved by SDS-polyacrylamide gel electrophoresis, and transferredonto ProBlots (Applied Biosystems). The blots were blocked with3% nonfat milk and were incubated with antibodies for 1 h at roomtemperature. After three rinses with 0.05% Tween 20 in PBS (T-PBS),proteins were detected using goat anti-rabbit or anti-mouse immunoglobulinG (IgG) antibody conjugated with horseradish peroxidase combinedwith enhanced chemiluminescence(NEN).

Immunocytochemistry. Cells were cultured on glass coverslips in 12-well plates and were then transfected as indicated above. The cells were thenrinsed once with PBS, fixed with 4% paraformaldehyde for 30 min,and permeabilized with 0.05% Triton X-100 in PBS including 300nM 4',6'-diamidino-2-phenylindole (DAPI) (Sigma) for 15 min. Aftertwo washes with PBS, cells were blocked with 5% bovine serum albuminfor 30 min at room temperature. Anti-rPER2 antiserum (a gift fromT. Nagase), anti-FLAG antibody (M2; Sigma), and/or anti-Xpressantibody (Invitrogen) were diluted in blocking solution and wereincubated with the cells for 1 h at room temperature. The cellswere then washed three times with T-PBS and incubated with fluoresceinisothiocyanate- and/or rhodamine-conjugated secondary antibody.Coverslips containing the stained cells were washed with T-PBSand were mounted for fluorescencemicroscopy.

Coimmunoprecipitation. Coimmunoprecipitation proceeded as described by Kume and colleagues (10) with some modifications. Forty-eight hours aftertransfection, cells in six-well plates were washed twice withPBS, were lysed with lysis buffer (150 mM NaCl, 5 mM EDTA, 0.5%NP-40, and 50 mM Tris-HCl [pH 7.5]) including protease inhibitorcocktail tablets (Complete; Roche) on ice for 30 min, and werethen clarified by centrifugation for 10 min at 15,000 × g.

Protein A/G agarose beads (Santa Cruz Biotechnology, Inc.) were incubated with anti-rPER2 antibodies for 1 h at 4°C; thenantibody-conjugated beads were collected by centrifugation, rinsedtwice with PBS, and resuspended in lysis buffer. Protein A/G agarose-antibodycomplexes were incubated with the clarified cell lysate overnightat 4°C. Subsequently, beads were washed for 10 min at 4°C threetimes and boiled in 2× SDS sample buffer. Bound proteins weretheneluted.

The supernatant was separated by SDS-polyacrylamide gel electrophoresis and immunoblotted against anti-rPER2 antiserum (1:2,000),anti-FLAG M2 antibodies (1:5,000), or anti-Xpress antibody (1:5,000)as describedabove.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Identification of region essential for nuclear localization of rPER2. Although the primary structure of rPER2 shows a bipartite NLS in the central domain of rPER2 (residues 778 to 795), whetheror not this putative sequence is functional remains unknown. Toidentify the precise molecular feature required for the nuclearentry system of rPER2, we expressed a series of deleted rPER2proteins (Fig. 1A) and determined their subcellular localizationin COS-1 cells.

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FIG. 1. Subcellular localization of truncated rPER2 mutants in COS-1 cells. (A) Diagrammatic representation of constructs used to identify the rPER2 NLD. PAS-A, PAS-B, and the putative bipartite NLS are shown as shaded and solid boxes. (B) Confirmation of the size of proteins expressed in COS-1 cells determined by immunoblotting. Sizes are indicated in kilodaltons. Anti-rPER2 antiserum was the first antibody. (C) Representative micrographs show the subcellular localization of rPER2. COS-1 cells were transiently transfected with truncated constructs 1-1257, 1-1157, 1-997, 1-794, 1-512, and 512-1257. Forty-eight hours later, cells were fixed and expressed proteins were visualized using anti-rPER2 antiserum and fluorescein isothiocyanate-conjugated secondary antibody. (D) Quantitative analysis of the above. Subcellular localization was categorized as cytoplasm, cytoplasm and nucleus, and nucleus. The ratio of cells with predominant localization to the total transfected cells was determined by counting 50 to 100 cells three to five times in each experiment under light microscopy.

Immunoblotting the overexpressed deletion proteins revealed that the predicted sizes of proteins were expressed in COS-1 cells(Fig. 1B). Figure 1C shows that full-length rPER2 predominatedin the cytoplasm as reported in mPERs (10, 26, 27). Twodeletions that included a mutant lacking a carboxyl-terminal domain(residues 1 to 1157) and an amino-terminal half-clone (residues1 to 512) of rPER2 were also localized in the cytoplasm (Fig.1C and D). In contrast, 1-794 and 512-1257 were located in thenuclei of 96.3 and 87.5% of transfected cells, respectively (Fig.1C and D). These findings indicated that a region important fornuclear translocation, the NLD, is located between acids 512 and794. The deletion of amino acids 998 to 1257 (1-997) intermediatelyaffected localization (Fig. 1C and D), suggesting that the C-terminaldomain affects the function of nuclear entry. Lacking the amino-terminalportion (residues 1 to 511) or carboxyl-terminal region (residues795 to 1257) of NLD led to the facilitation of rPER2 mutants'nuclear entry, indicating that both portions are masking the NLDfunction ofrPER2.

To narrow down the NLS region, we then expressed several FLAG-tagged constructs around the NLD region (Fig. 2A). The expressedproteins from two constructs (512-794 and 638-794) were localizedin the nucleus, but 512-644 was found in the cytoplasm (Fig. 2Cand D). In contrast to the nuclear localization of 638-794, thefragment of 638-777, lacking the predicted rPER2 NLS (778-794),was enriched in the cytoplasmic compartment.

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FIG. 2. Expression of NLDs of rPER2 and rPER2 NLS-tagged BAP (NLS-BAP). (A) Schematic diagrams of four constructs covering the NLD of rPER2. All fragments were tagged with FLAG at the amino terminus. rPER2 NLS was inserted at the carboxyl terminus of BAP. (B) The molecular size in kilodaltons of FLAG-tagged NLD fragments and BAP fragments was confirmed by immunoblotting using anti-FLAG M2 monoclonal antibody. (C) Subcellular localization of rPER2 NLD mutants (512-794, 512-644, 638-794, and 638-777) expressed in COS-1 cells and examined by immunofluorescence microscopy. Fragments of rPER2 NLD mutants were stained with a combination of anti-FLAG monoclonal antibody M2 and fluorescein isothiocyanate-conjugated anti-mouse IgG (green, left panels), and nuclei were visualized with DAPI (blue, right panels). The distribution of NLS-BAP and BAP was also confirmed as described above. (D) Quantitative analysis of above as described in the legend for Fig. 1D.

In order to show the ability of active nuclear transport of the predicted NLS of PER2, we inserted the NLS (778-794) intothe C-terminal end of FLAG-tagged BAP (BAP-NLS, Fig. 2A). BAP-NLSwas translocated in the nucleus, while BAP was retained in thecytoplasmic region as we expected (Fig. 2C and D). Thus, we concludedthat the latent rPER2 nuclear localization feature is derivedfrom the sequence of acids 778 to 794 rather than through coordinationwith another domain and that the predicted rPER2 NLS isfunctional.

Role of two rPER2 domains in nuclear localization of rPER2 by CRY1 coexpression. We surmised that the masking of rPER2 NLD would be disrupted by either binding or interaction with a partner molecule thatmodulates rPER2 nuclear entry like mCRY1 and mCRY2 (10). Moreover,whether or not the nuclear entry of mPERs with mCRYs is regulatedby the NLS in PERs remained unknown. Thus, we coexpressed deletionmutants of rPER2 with hCRY1 and examined their subcellularlocalization.

Intact rPER2 proteins coexpressed with hCRY1, rPER2 predominantly localized in the nucleus (Fig. 3A; 1-1257; 89.3% of transfectedcells). Deletion of the carboxyl-terminal domain (1157-1257) changedthe subcellular localization of rPER2 from the nucleus to thecytoplasm (Fig. 3C; 1-1157). Subcellular distribution of the otherdeletion mutants (Fig. 1A) was not affected by coexpression withhCRY1 (data not shown). These data suggested that the carboxyl-terminaldomain is important for the nuclear localization of rPER2 in thepresence of hCRY1. Furthermore, rPER2 lacking the NLD (Fig. 3A;1-1257; $Delta$ 512-794) also caused the cytoplasmic retention of rPER2(Fig. 3C; 92.1% of transfected cells). These findings suggestedthat the NLD of rPER2 is also important in deciding the nuclearentry of rPER2.

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FIG. 3. Role of two rPER2 domains in nuclear localization by CRY1 coexpression. (A) Schematic representation of truncated rPER2 constructs. The position of the rPER2 NLD is shown by shaded boxes as PAS-A and PAS-B. The putative NLS is shown as a solid box. Internal portion of constructs 1-1257 $Delta$ 512-794 and 1-1157 $Delta$ 512-794, containing NLD, was deleted (amino acids 512 to 794, dotted line). The carboxyl-terminal portion of clones 1-1157 $Delta$ 512-794 was also deleted to form clone 1-1157. (B) Molecular size in kilodaltons of clones with a truncation of the NLD was confirmed by immunoblotting using anti-rPER2 polyclonal antibody. (C) Full-length (1-1257) or truncated (1-1157 and 1-1257 $Delta$ 512-794) clones with a deletion of rPER2 were cotransfected with hCRY1-pcDNA3.1-His (right panels, + hCRY1) in COS-1 cells. Control used the mock vector, pcDNA3, instead of hCRY1-pcDNA3.1-His (left panels, + pcDNA3). Localization was examined by immunocytochemistry using anti-rPER2 antibody. (D) Quantitation of above as described in the legend for Fig. 1D.

Role of carboxyl-terminal domain of rPER2 in nuclear localization of rPER2-CRY1 complex. When singly expressed in COS-1 cells, hCRY1 was distributed in the nucleus (data not shown). We examined the localizationof hCRY1 in COS-1 cells cotransfected with rPER2 deletion mutants.When hCRY1 was transfected with full-length rPER2 (1-1257) orcarboxyl-terminal domain lacking rPER2 (1-1157), the nucleus becamepredominantly enriched with hCRY1 (Fig. 4). On the other hand,rPER2 localization differed between 1-1257 and 1-1157 (Fig. 4),which were enriched in the nucleus and cytosol, respectively,suggesting that the carboxyl-terminal domain is the binding domainof rPER2 for CRY1. hCRY1 coexpressed with 1-1257 $Delta$ 512-794, whichlacks rPER2 NLD, accumulated in the cytoplasm (72.91% of transfectedcells). Furthermore, 1-1157 $Delta$ 512-794, which lacks both NLD andthe carboxyl-terminal domain, did not affect the nuclear entryof hCRY1 (Fig. 4). These data also indicated that the carboxyl-terminaldomain of rPER2 is the hCRY1 binding site and suggested that afterhCRY1 binds to rPER2, the NLD of rPER2 is essential for the nucleartranslocation of the rPER2-hCRY1 complex.

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FIG. 4. Subcellular distribution of hCRY1 is affected by cotransfection with rPER2 mutants in COS-1 cells. (A) Full-length (1-1257) and deletion clones truncated at NLDs and/or the carboxyl-terminal portion were coexpressed with Xpress-tagged hCRY1. Transfected cells were triply stained with anti-rPER2 antibodies (green), anti-Xpress antibodies (red), and DAPI (blue). Anti-Xpress antibodies recognized recombinant hCRY and DAPI-stained nuclei. (B) Quantitative analysis of experiment shown in Fig. 4A as described in the legend for Fig. 1D.

Binding domain of rPER2 to hCRY1. To determine whether or not the effect of rPER2 mutants on hCRY1 localization is due to the ability of each molecule to bindCRY1, we analyzed the binding activity of rPER2 mutants with hCRY1using coimmunoprecipitation. The lysates from cells of cooverexpressedrPER2 mutants and Xpress-tagged hCRY1 was incubated with anti-rPER2antibody-protein A/G agarose complex. The precipitated immunocomplexeswere analyzed by immunoblotting with anti-rPER2 antibody and anti-Xpressantibody. Intact rPER2 and all mutants containing a carboxyl-terminaldomain bound to hCRY1 (1-1257, 1-1257 $Delta$ 512-794, and 512-1257),while all deletions lacking the carboxyl-terminal domain of rPER2lost the ability to bind hCRY1 (1-1157, 1-1157 $Delta$ 512-794, and 512-1157)(Fig. 5A and B).

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FIG. 5. Coimmunoprecipitation shows that hCRY1 interacts with rPER2 carboxyl-terminal domain. (A) Schematic representation of rPER2 mutant constructs for coimmunoprecipitation. The positions of rPER2 NLD, PAS-A, and PAS-B are shown by shaded boxes. The rPRE2 NLS is shown as a solid box. The mutants with a deletion at the amino-terminal half (512-1257 and 512-1157) and at the carboxyl-terminal fragment of rPER2 (1157-1257) were tagged with FLAG at their amino-terminal ends. (B) Total lysates from cells coexpressing hCRY1 and truncation mutants of rPER2 were immunoprecipitated (IP) and blotted with anti-rPER2 antibodies (top panel) and were detected using anti-Xpress antibodies (lower panel). Results were similar in replicate experiments. Arrow indicates position of hCRY1. (C) Identification of the CRY1 binding domain of rPER2. The FLAG-tagged truncation mutants of rPER2 proteins (1157-1257, 512-1257, and 512-1157) were expressed with hCRY1. Control was vector pcDNA3 or pFLAG instead of hCRY1 or rPER2 mutants. Lysates from transfected cells were immunoprecipitated (IP) and blotted with anti-FLAG antibodies (top panel) and were visualized using anti-Xpress antibodies (lower panel). The arrow indicates the position of hCRY1. Asterisks indicate nonspecific band corresponding to Ig derived from M2 monoclonal antibodies. Numerals indicate molecular weights in thousands.

We then constructed and overexpressed the three FLAG-tagged clones (1157-1257, 512-1257, and 512-1157) in COS-1 cells. Bindingto hCRY1 was tested by coimmunoprecipitation with anti-FLAG antibody.The results showed that the minimal region of rPER2 required forbinding hCRY1 was located in clone 1157-1257 (Fig. 5C). The dataindicate that the carboxyl-terminal region (1157-1257) of rPER2is the binding domain to hCRY1. These data easily explain thecytoplasmic colocalization of hCRY1 and rPER2 in Fig. 4A.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The present study focused on the nuclear entry mechanism of rPER2 and identified its latent functional NLS at acids 778 to794; that NLS has been identified as the putative bipartite-typeNLS. The full length of rPER2 overexpressed in COS-1 cells waspredominantly distributed in the cytoplasm, like mPERs in COS-7and NIH 3T3 cells (10, 27). However, the truncated mutagenesisof rPER2 (1-794 and 512-1257) promoted nuclear entry. Furthermore,the putative NLS deletion inactivated the nuclear localizationof the rPER2 fragments, and BAP tagged with rPER2 NLS promotedthe nuclear translocation of the molecule. The bipartite-typeNLS in rPER2 is well conserved in mPER2 and in hPER2 at similarpositions (1, 6, 11, 15, 18, 21). In the PER1 sequence,no obvious NLS was found, but the functional NLS was identifiedat the corresponding region to rPER2 NLS (26). In contrast,PER3 contains a simian virus 40 large-T-antigen type of NLS atthe corresponding region, which is functional (26, 27).

The NLS appeared to be masked by two other regions (1-511 and 795-1257), and the deletion of masking regions may activatethe nuclear translocating function (Fig. 1). Shearman et al. showedthat mPER2 435-1257 could not enter into the nucleus (17), whileour N-terminal deletion clone (512-1257) showed nuclear localization.We speculate that the domain for masking the NLS function or theportion for cytosolic retaining activity like NES may locate betweenresidues 435 and 512. Furthermore, mPER2^brdm1 (missing residues 348 to 434) could not be translocated in thenucleus, irrespective of the presence of mCRY1 (17). Becauseour results suggest that mPER2^brdm1 can bind with mCRY1, the arrhythmic phenotype of mPER2^brdm1 (28) may be caused by the inhibition of proper nuclear translocationof CRYproteins.

Kume et al. reported that mCRY1 and mCRY2 are nuclear proteins that interact with all three mPER proteins and translocatethem from the cytoplasm to the nucleus (10). Constitutivelyoverexpressed hCRY1 also localized in the nucleus (data not shown)like mCRY proteins (9, 10, 24) and promoted the nuclearentry of full-length rPER2 but failed to translocate rPER2 witha truncated carboxyl-terminal domain (Fig. 3). In fact, otherreports also suggest that the amino-terminal half-region is notimportant for the nuclear translocation of mPER2 and mCRY proteins(17). Furthermore, our binding assays showed that the carboxyl-terminaldomain was essential for rPER2 to bind hCRY1 followed by nucleartranslocation. Recombinant rPER2 protein lacking the NLD did notenter the nucleus, even when coexpressing hCRY1 in COS-1 cells.Moreover, hCRY1 was also retained in the cytoplasm like rPER2with a deletion of the NLD. This indicated that the rPER2 NLD,which becomes functional after binding with hCRY1, is essentialfor nuclear localization of the rPER2-hCRY1 complex. We speculatethat the binding of hCRY1 to rPER2 changes the conformation ofrPER2 and exposes the NLD to render it functional in translocatingthe complex to thenucleus.

The rat TIM-like protein (rTLP) homologous to dTIM (a partner in dPER nuclear translocation) was a candidate to expose rPER2NLS like dTIM (14). However, rTLP did not influence the subcellularlocalization of rPER2 (16), in agreement with the results ofother studies using mPER and mTIM (10). It is likely that CRYsplay more important roles in the nuclear translocation of rPER2than doesrTLP.

When singly overexpressed in COS-1, hCRY1 was distributed in the nucleus (data not shown). However, hCRY1 located in the cytosolafter coexpressing rPER2 with a deletion of the NLD. The sequencein rPER2 appeared to be abler to perform nuclear translocationthan that inhCRY1.

Several pathways for the nuclear entry of mammalian PERs have been reported. Kume et al. found that mCRY proteins act as dimerizationpartners for the nuclear localization of mPER1, mPER2, and mPER3,with activity that is more effective on mPER1 and mPER2 than onmPER3 (10). The present study revealed details of the interactionmechanism between rPER2 and hCRY1 and suggests that hCRY1 translocatesrPER2 to the nucleus by binding and inhibiting its ability tomask the rPER2 NLD. On the other hand, Yagita et al. demonstratedthat the nuclear translocation of mPER1 and mPER2 is acceleratedby serum shock after binding mPER3 (27), although the effectof mPER3 on the nuclear entry of mPER2 was weaker than that ofmPER1. Casein kinase I $varepsilon$ modulates the nuclear translocation ofmPER1 and mPER3 but not of mPER2 (20, 26). Thus, CRY appearsto be the main partner involved in the nuclear translocation ofPER2.

In the SCN of mCry1-mCry2 double-knockout mice, mPER1 weakly localizes in the nucleus (17, 27), whereas mPER2 does notaccumulate in the nuclei of SCN neurons (17). Our results areconsistent with these findings in that at least the nuclear translocationof PER2 will be mainly regulated by the CRY protein through directbinding.

The CRY1 binding domain of rPER2 shows higher homology with that of mPER2 but less with that of hPER2 and the PER subfamily,including PER1 and PER3. All mammalian PER proteins bind CRY proteins(10), suggesting that the 1156-to-1175 region, which is highlyhomologous to other PER proteins, is important for binding CRYproteins.

mCRY proteins are temporally expressed in the nucleus of SCN neurons, and the expression profile is synchronized with theaccumulation of PER1 and PER2 in the nucleus (5, 10). TheCRY proteins inhibit per1-promoter-driven reporter transactivationby the CLOCK-BMAL complex in NIH 3T3 cells (10). This inhibitionmight proceed in the nuclei of SCN neurons in vivo. Our conclusionthat the NLS of rPER2 is essential for the nuclear entry of CRY1indicates that PER2 plays an important role in the nuclear translocationof CRY, which may regulate the negative-feedback loop of the corecircadian clockmechanism.

	ACKNOWLEDGMENTS

We thank Takahiro Nagase for supplying us with anti-rPER2 antibody; Takeshi Todo for providing human CRY1 expression plasmid;Junichi Miyazaki for the constitutive expression vector pCXN2;Lino Saez for useful discussion; and Kazuko Suzuki and YukakoSoya for technicalassistance.

This study was supported by a project grant for the Competition Research Program, AIST, MITI, Tokyo,Japan.

	FOOTNOTES

^* Corresponding author. Mailing address: Clock Cell Biology Group, Institute of Molecular and Cell Biology, National Instituteof Advanced Industrial Science and Technology, Tsukuba Central6, 1-1-1 Higashi, Tsukuba, Ibaraki 305-8566, Japan. Phone: 81-298-61-6053.Fax: 81-298-61-9498/6505. E-mail: n.ishida{at}aist.go.jp.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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3. Dunlap, J. C. 1999. Molecular bases for circadian clocks. Cell 96:271-290[CrossRef][Medline].

4. Field, M. D., E. S. Maywood, J. A. O'Brien, D. R. Weaver, S. M. Reppert, and M. H. Hastings. 2000. Analysis of clock proteins in mouse SCN demonstrates phylogenetic divergence of the circadian clockwork and resetting mechanisms. Neuron 25:437-447[CrossRef][Medline].

5. Hastings, M. H., M. D. Field, E. S. Maywood, D. R. Weaver, and S. M. Reppert. 1999. Differential regulation of mPER1 and mTIM proteins in the mouse suprachiasmatic nuclei: new insights into a core clock mechanism. J. Neurosci. 0:RC11 (1-7).

6. Ishida, N., M. Kaneko, and R. Allada. 1999. Biological clocks. Proc. Natl. Acad. Sci. USA 96:8819-8820[Abstract/Free Full Text].

7. Jin, X., L. P. Shearman, D. R. Weaver, M. J. Zylka, G. J. de Vries, and S. M. Reppert. 1999. A molecular mechanism regulating rhythmic output from the suprachiasmatic circadian clock. Cell 96:57-68[CrossRef][Medline].

8. Klein, D. C., R. Y. Moore, and S. M. Reppert (ed.). 1991. Suprachiasmatic nucleus: the mind's clock. Oxford University Press, New York, N.Y.

9. Kobayashi, K., S. Kanno, B. Smit, G. T. van der Horst, M. Takao, and A. Yasui. 1998. Characterization of photolyase/blue-light receptor homologs in mouse and human cells. Nucleic Acids Res. 26:5086-5092[Abstract/Free Full Text].

10. Kume, K., M. J. Zylka, S. Sriram, L. P. Shearman, D. R. Weaver, X. Jin, E. S. Maywood, M. H. Hastings, and S. M. Reppert. 1999. mCRY1 and mCRY2 are essential components of the negative limb of the circadian clock feedback loop. Cell 98:193-205[CrossRef][Medline].

11. Nagase, T., K. Ishikawa, D. Nakajima, M. Ohira, N. Seki, N. Miyajima, A. Tanaka, H. Kotani, N. Nomura, and O. Ohara. 1997. Prediction of the coding sequences of unidentified human genes. VII. The complete sequences of 100 new cDNA clones from brain which can code for large proteins in vitro. DNA Res. 4:141-150[Abstract].

12. Niwa, H., K. Yamamura, and J. Miyazaki. 1991. Efficient selection for high-expression transfectants with a novel eukaryotic vector. Gene 108:193-199[CrossRef][Medline].

13. Oishi, K., H. Fukui, and N. Ishida. 2000. Rhythmic expression of BMAL1 mRNA is altered in Clock mutant mice: differential regulation in the suprachiasmatic nucleus and peripheral tissues. Biochem. Biophys. Res. Commun. 268:164-171[CrossRef][Medline].

14. Saez, L., and M. W. Young. 1996. Regulation of nuclear entry of the Drosophila clock proteins period and timeless. Neuron 17:911-920[CrossRef][Medline].

15. Sakamoto, K., T. Nagase, H. Fukui, K. Horikawa, T. Okada, H. Tanaka, K. Sato, Y. Miyake, O. Ohara, K. Kako, and N. Ishida. 1998. Multitissue circadian expression of rat period homolog (rPer2) mRNA is governed by the mammalian circadian clock, the suprachiasmatic nucleus in the brain. J. Biol. Chem. 273:27039-27042[Abstract/Free Full Text].

16. Sakamoto, S., K. Miyazaki, H. Fukui, K. Oishi, N. Hayasaka, M. Okada, M. Kamakura, T. Taniguchi, K. Nagai, and N. Ishida. 2000. Molecular characterization and nuclear localization of rat timeless-like gene product. Biochem. Biophys. Res. Commun. 279:131-138[CrossRef][Medline].

17. Shearman, L. P., S. Sriram, D. R. Weaver, E. S. Maywood, I. Chaves, B. Zheng, K. Kume, C. C. Lee, G. T. van der Horst, M. H. Hastings, and S. M. Reppert. 2000. Interacting molecular loops in the mammalian circadian clock. Science 288:1013-1019[Abstract/Free Full Text].

18. Shearman, L. P., M. J. Zylka, D. R. Weaver, L. F. Kolakowski, Jr., and S. M. Reppert. 1997. Two period homologs: circadian expression and photic regulation in the suprachiasmatic nuclei. Neuron 19:1261-1269[CrossRef][Medline].

19. Sun, Z. S., U. Albrecht, O. Zhuchenko, J. Bailey, G. Eichele, and C. C. Lee. 1997. RIGUI, a putative mammalian ortholog of the Drosophila period gene. Cell 90:1003-1011[CrossRef][Medline].

20. Takano, A., K. Shimizu, S. Kani, R. M. Buijs, M. Okada, and K. Nagai. 2000. Cloning and characterization of rat casein kinase 1epsilon. FEBS Lett. 477:106-112[CrossRef][Medline].

21. Takumi, T., C. Matsubara, Y. Shigeyoshi, K. Taguchi, K. Yagita, Y. Maebayashi, Y. Sakakida, K. Okumura, N. Takashima, and H. Okamura. 1998. A new mammalian period gene predominantly expressed in the suprachiasmatic nucleus. Genes Cells 3:167-176[Abstract].

22. Takumi, T., K. Taguchi, S. Miyake, Y. Sakakida, N. Takashima, C. Matsubara, Y. Maebayashi, K. Okumura, S. Takekida, S. Yamamoto, K. Yagita, L. Yan, M. W. Young, and H. Okamura. 1998. A light-independent oscillatory gene mPer3 in mouse SCN and OVLT. EMBO J. 17:4753-4759[CrossRef][Medline].

23. Tei, H., H. Okamura, Y. Shigeyoshi, C. Fukuhara, R. Ozawa, M. Hirose, and Y. Sakaki. 1997. Circadian oscillation of a mammalian homologue of the Drosophila period gene. Nature 389:512-516[CrossRef][Medline].

24. Thresher, R. J., M. H. Vitaterna, Y. Miyamoto, A. Kazantsev, D. S. Hsu, C. Petit, C. P. Selby, L. Dawut, O. Smithies, J. S. Takahashi, and A. Sancar. 1998. Role of mouse cryptochrome blue-light photoreceptor in circadian photoresponses. Science 282:1490-1494[Abstract/Free Full Text].

25. van der Horst, G. T., M. Muijtjens, K. Kobayashi, R. Takano, S. Kanno, M. Takao, J. de Wit, A. Verkerk, A. P. Eker, D. van Leenen, R. Buijs, D. Bootsma, J. H. Hoeijmakers, and A. Yasui. 1999. Mammalian Cry1 and Cry2 are essential for maintenance of circadian rhythms. Nature 398:627-630[CrossRef][Medline].

26. Vielhaber, E., E. Eide, A. Rivers, Z.-H. Gao, and D. M. Virshup. 2000. Nuclear entry of the circadian regulator mPER1 is controlled by mammalian casein kinase I $varepsilon$ . Mol. Cell. Biol. 20:4888-4899[Abstract/Free Full Text].

27. Yagita, K., S. Yamaguchi, F. Tamanini, G. T. van Der Horst, J. H. Hoeijmakers, A. Yasui, J. J. Loros, J. C. Dunlap, and H. Okamura. 2000. Dimerization and nuclear entry of mPER proteins in mammalian cells. Genes Dev. 14:1353-1363[Abstract/Free Full Text].

28. Zheng, B., D. W. Larkin, U. Albrecht, Z. S. Sun, M. Sage, G. Eichele, C. C. Lee, and A. Bradley. 1999. The mPer2 gene encodes a functional component of the mammalian circadian clock. Nature 400:169-173[CrossRef][Medline].

29. Zylka, M. J., L. P. Shearman, D. R. Weaver, and S. M. Reppert. 1998. Three period homologs in mammals: differential light responses in the suprachiasmatic circadian clock and oscillating transcripts outside of brain. Neuron 20:1103-1110[CrossRef][Medline].

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1.	Albrecht, U., Z. S. Sun, G. Eichele, and C. C. Lee. 1997. A differential response of two putative mammalian circadian regulators, mper1 and mper2, to light. Cell 91:1055-1064[CrossRef][Medline].
2.	Balsalobre, A., F. Damiola, and U. Schibler. 1998. A serum shock induces circadian gene expression in mammalian tissue culture cells. Cell 93:929-937[CrossRef][Medline].
3.	Dunlap, J. C. 1999. Molecular bases for circadian clocks. Cell 96:271-290[CrossRef][Medline].
4.	Field, M. D., E. S. Maywood, J. A. O'Brien, D. R. Weaver, S. M. Reppert, and M. H. Hastings. 2000. Analysis of clock proteins in mouse SCN demonstrates phylogenetic divergence of the circadian clockwork and resetting mechanisms. Neuron 25:437-447[CrossRef][Medline].
5.	Hastings, M. H., M. D. Field, E. S. Maywood, D. R. Weaver, and S. M. Reppert. 1999. Differential regulation of mPER1 and mTIM proteins in the mouse suprachiasmatic nuclei: new insights into a core clock mechanism. J. Neurosci. 0:RC11 (1-7).
6.	Ishida, N., M. Kaneko, and R. Allada. 1999. Biological clocks. Proc. Natl. Acad. Sci. USA 96:8819-8820[Abstract/Free Full Text].
7.	Jin, X., L. P. Shearman, D. R. Weaver, M. J. Zylka, G. J. de Vries, and S. M. Reppert. 1999. A molecular mechanism regulating rhythmic output from the suprachiasmatic circadian clock. Cell 96:57-68[CrossRef][Medline].
8.	Klein, D. C., R. Y. Moore, and S. M. Reppert (ed.). 1991. Suprachiasmatic nucleus: the mind's clock. Oxford University Press, New York, N.Y.
9.	Kobayashi, K., S. Kanno, B. Smit, G. T. van der Horst, M. Takao, and A. Yasui. 1998. Characterization of photolyase/blue-light receptor homologs in mouse and human cells. Nucleic Acids Res. 26:5086-5092[Abstract/Free Full Text].
10.	Kume, K., M. J. Zylka, S. Sriram, L. P. Shearman, D. R. Weaver, X. Jin, E. S. Maywood, M. H. Hastings, and S. M. Reppert. 1999. mCRY1 and mCRY2 are essential components of the negative limb of the circadian clock feedback loop. Cell 98:193-205[CrossRef][Medline].
11.	Nagase, T., K. Ishikawa, D. Nakajima, M. Ohira, N. Seki, N. Miyajima, A. Tanaka, H. Kotani, N. Nomura, and O. Ohara. 1997. Prediction of the coding sequences of unidentified human genes. VII. The complete sequences of 100 new cDNA clones from brain which can code for large proteins in vitro. DNA Res. 4:141-150[Abstract].
12.	Niwa, H., K. Yamamura, and J. Miyazaki. 1991. Efficient selection for high-expression transfectants with a novel eukaryotic vector. Gene 108:193-199[CrossRef][Medline].
13.	Oishi, K., H. Fukui, and N. Ishida. 2000. Rhythmic expression of BMAL1 mRNA is altered in Clock mutant mice: differential regulation in the suprachiasmatic nucleus and peripheral tissues. Biochem. Biophys. Res. Commun. 268:164-171[CrossRef][Medline].
14.	Saez, L., and M. W. Young. 1996. Regulation of nuclear entry of the Drosophila clock proteins period and timeless. Neuron 17:911-920[CrossRef][Medline].
15.	Sakamoto, K., T. Nagase, H. Fukui, K. Horikawa, T. Okada, H. Tanaka, K. Sato, Y. Miyake, O. Ohara, K. Kako, and N. Ishida. 1998. Multitissue circadian expression of rat period homolog (rPer2) mRNA is governed by the mammalian circadian clock, the suprachiasmatic nucleus in the brain. J. Biol. Chem. 273:27039-27042[Abstract/Free Full Text].
16.	Sakamoto, S., K. Miyazaki, H. Fukui, K. Oishi, N. Hayasaka, M. Okada, M. Kamakura, T. Taniguchi, K. Nagai, and N. Ishida. 2000. Molecular characterization and nuclear localization of rat timeless-like gene product. Biochem. Biophys. Res. Commun. 279:131-138[CrossRef][Medline].
17.	Shearman, L. P., S. Sriram, D. R. Weaver, E. S. Maywood, I. Chaves, B. Zheng, K. Kume, C. C. Lee, G. T. van der Horst, M. H. Hastings, and S. M. Reppert. 2000. Interacting molecular loops in the mammalian circadian clock. Science 288:1013-1019[Abstract/Free Full Text].
18.	Shearman, L. P., M. J. Zylka, D. R. Weaver, L. F. Kolakowski, Jr., and S. M. Reppert. 1997. Two period homologs: circadian expression and photic regulation in the suprachiasmatic nuclei. Neuron 19:1261-1269[CrossRef][Medline].
19.	Sun, Z. S., U. Albrecht, O. Zhuchenko, J. Bailey, G. Eichele, and C. C. Lee. 1997. RIGUI, a putative mammalian ortholog of the Drosophila period gene. Cell 90:1003-1011[CrossRef][Medline].
20.	Takano, A., K. Shimizu, S. Kani, R. M. Buijs, M. Okada, and K. Nagai. 2000. Cloning and characterization of rat casein kinase 1epsilon. FEBS Lett. 477:106-112[CrossRef][Medline].
21.	Takumi, T., C. Matsubara, Y. Shigeyoshi, K. Taguchi, K. Yagita, Y. Maebayashi, Y. Sakakida, K. Okumura, N. Takashima, and H. Okamura. 1998. A new mammalian period gene predominantly expressed in the suprachiasmatic nucleus. Genes Cells 3:167-176[Abstract].
22.	Takumi, T., K. Taguchi, S. Miyake, Y. Sakakida, N. Takashima, C. Matsubara, Y. Maebayashi, K. Okumura, S. Takekida, S. Yamamoto, K. Yagita, L. Yan, M. W. Young, and H. Okamura. 1998. A light-independent oscillatory gene mPer3 in mouse SCN and OVLT. EMBO J. 17:4753-4759[CrossRef][Medline].
23.	Tei, H., H. Okamura, Y. Shigeyoshi, C. Fukuhara, R. Ozawa, M. Hirose, and Y. Sakaki. 1997. Circadian oscillation of a mammalian homologue of the Drosophila period gene. Nature 389:512-516[CrossRef][Medline].
24.	Thresher, R. J., M. H. Vitaterna, Y. Miyamoto, A. Kazantsev, D. S. Hsu, C. Petit, C. P. Selby, L. Dawut, O. Smithies, J. S. Takahashi, and A. Sancar. 1998. Role of mouse cryptochrome blue-light photoreceptor in circadian photoresponses. Science 282:1490-1494[Abstract/Free Full Text].
25.	van der Horst, G. T., M. Muijtjens, K. Kobayashi, R. Takano, S. Kanno, M. Takao, J. de Wit, A. Verkerk, A. P. Eker, D. van Leenen, R. Buijs, D. Bootsma, J. H. Hoeijmakers, and A. Yasui. 1999. Mammalian Cry1 and Cry2 are essential for maintenance of circadian rhythms. Nature 398:627-630[CrossRef][Medline].
26.	Vielhaber, E., E. Eide, A. Rivers, Z.-H. Gao, and D. M. Virshup. 2000. Nuclear entry of the circadian regulator mPER1 is controlled by mammalian casein kinase I $varepsilon$ . Mol. Cell. Biol. 20:4888-4899[Abstract/Free Full Text].
27.	Yagita, K., S. Yamaguchi, F. Tamanini, G. T. van Der Horst, J. H. Hoeijmakers, A. Yasui, J. J. Loros, J. C. Dunlap, and H. Okamura. 2000. Dimerization and nuclear entry of mPER proteins in mammalian cells. Genes Dev. 14:1353-1363[Abstract/Free Full Text].
28.	Zheng, B., D. W. Larkin, U. Albrecht, Z. S. Sun, M. Sage, G. Eichele, C. C. Lee, and A. Bradley. 1999. The mPer2 gene encodes a functional component of the mammalian circadian clock. Nature 400:169-173[CrossRef][Medline].
29.	Zylka, M. J., L. P. Shearman, D. R. Weaver, and S. M. Reppert. 1998. Three period homologs in mammals: differential light responses in the suprachiasmatic circadian clock and oscillating transcripts outside of brain. Neuron 20:1103-1110[CrossRef][Medline].