Molecular assembly of the period-cryptochrome circadian transcriptional repressor complex

PER2-CBD adopts a highly extended structure, devoid of a hydrophobic core. It folds into five α-helices of variable length, which are dispersed along an otherwise linear polypeptide (Figure 1C). In the crystal, PER2-CBD meanders along one side of CRY2-PHR and sinuously wraps around the region. With nearly half of the PER2 residues involved in binding, the two proteins bury a total 2800 Ų of solvent accessible surface area at the interface, which stretches over a distance of more than 215 Å. This unusually extensive interface provides a plausible explanation for the high-affinity binding between the two clock proteins and their insensitivity to mutational disruption.

In comparison to its FBXL3-, KL001-, and FAD-complexed forms, CRY2 adopts the same global fold when bound to PER2-CBD (Figure 4—figure supplement 2). The largest structural variations take place in two local regions, the interface loop next to the FAD-binding pocket and a serine-rich loop neighboring a secondary pocket (see below). The majority of PER2-contacting residues on CRY2 (85%) are strictly conserved between mammalian CRY1 and CRY2, suggesting that the two cryptochrome proteins share a common PER2 binding mode.

The close interaction between the C-terminal half of PER2-CBD and CRY2 C-terminal helix is immediately reminiscent of the docking mode between FBXL3 and CRY2. In the crystal structure of the FBXL3-CRY2 complex, the leucine-rich repeat (LRR) domain of FBXL3 engages CRY2 at the same site as PER2-CBD does in the PER2-CRY2 complex. The interface between FBXL3-LRR and CRY2 is also centered around the long C-terminal helix of the Cryptochrome protein. In fact, the CRY2 surface regions involved in contacting FBXL3-LRR and PER2-CBD share extensive overlapping regions (Figure 2D). Superposition analysis reveals that FBXL3 and PER2 cannot be simultaneously engaged with CRY2 without clashing into each other (Figure 2—figure supplement 1B). PERs, therefore, have the capability of protecting CRYs from FBXL3-mediated ubiquitination and degradation by directly competing with the ubiquitin ligase for binding CRYs.

To assess the role of the intermolecular zinc finger in mediating PER–CRY association, we first tested the CRY2-binding activity of a recombinant mutant PER2-CBD, which lacks the CXXC motif. In comparison to the wild-type polypeptide, the ability of the PER2-CBD mutant to bind CRY2 was substantially compromised (Figure 3B). Similarly weakened interaction was also observed in a co-immunoprecipitation assay, in which the CXXC motif of the full-length PER2 protein or the two zinc-coordinating residues of CRY2 were mutated to alanines (Figure 2—figure supplement 1A, Figure 3C). Together, these results highlight the importance of the intermolecular zinc finger in strengthening the PER–CRY interface.

In the PER2-CRY2 crystal, the N-terminal half of PER2-CBD diverges from the FBXL3-binding site of CRY2 and reaches the rim of the secondary pocket after traversing around the α-helical domain (Figure 4A). With a highly conserved sequence, the N-terminal end of PER2-CBD is embedded in a V-shaped cleft formed between the two globular domains of CRY2-PHR, burying a PER2 tryptophan residue (Trp1139) at the junction (Figure 4B, Figure 2—figure supplement 1A). One side of the cleft is constructed by a serine-rich loop in CRY2, which we name as ‘serine loop’. Distinct from its surrounding regions, this loop adopts different conformations in several available crystal structures of CRY (Figure 4—figure supplement 2). Remarkably, PER2 binding induces yet another distinct structural configuration of the loop, thereby, defining a unique structural state of the local area next to the secondary pocket.

Although CRYs are known to not engage a second cofactor (Zoltowski et al., 2011; Xing et al., 2013), our previous cell-based random mutagenesis screen has identified three residues within this secondary pocket (Gly106 and Arg109 in CRY1, Glu121 in CRY2) (Figure 4C), whose missense mutations effectively abolished the repressor activity of CRYs (McCarthy et al., 2009). Among these three residues, Arg109 is exposed to the solvent and decorates one side of the pocket. Co-immunoprecipitation analysis of the R109Q mutant showed that alteration of this single amino acid is sufficient to abrogate CLOCK-BMAL1, but not PER1 or PER2 binding (Figure 4D–F). Thus, the secondary pocket of CRYs represents an important docking site for the heterodimeric transcriptional activators. Anchoring of PER2 at the edge of this CRY pocket not only reinforces its function as a previously unrecognized locus for protein–protein interactions, but also suggests a possible role of PERs in modulating the repressor functions of CRYs.

We noticed that the two zinc finger CRY1 mutants still sustained circadian rhythms. However, they showed defects in their bioluminescence oscillations (Figure 5B,C). Such a phenotype was not observed for a mutant with a nearby residue, Cys412, mutated to alanine, which did not perturb PER or FBXL3 binding as previously documented (Figure 5D; Xing et al., 2013). The contrast between the two zinc finger-defective mutants and the wild-type-like C412A mutant confirms the functional role of the zinc-coordinating residues in the negative arm of the feedback loop.

Consistent with its impaired CLOCK-BMAL1 binding activity, the CRY1 R109Q mutant showed significant derepression in the rescue assay (Figure 5E; McCarthy et al., 2009). This single amino acid mutation highlights the key role of the secondary pocket of CRYs for repression. Intriguingly, double serine to aspartate mutations (S44D S45D) in the nearby serine loop at the opposite side of the CRY secondary pocket completely rescued the circadian rhythm, although the period of the bioluminescence rhythms rescued by the mutant was reliably shorter than the wild-type CRY1 by about 1 hr (Figure 5F). In our co-immunoprecipitation experiments, this double serine mutation weakened PER2 binding to a lesser degree than the zinc finger mutations, which did not elicit a similar period-shortening effect (Figure 2C). Therefore, the period-shortening effect induced by the double serine mutation is likely specific to the defects of the local PER–CRY interface instead of their overall binding. It is conceivable that PERs might engage with CRYs near the CLOCK-BMAL1 docking site to control a periodicity-related step of negative feedback different from what they do at the predominant PER–CRY interface.

The mouse CRY2 (amino acids 1–512) was expressed as a glutathione S-transferase (GST) fusion protein in High Five (Invitrogen, Carlsbad, CA) suspension insect cells and isolated by glutathione affinity chromatography using buffer containing 20 mM Tris–HCl pH 8, 200 mM NaCl, 10% glycerol, 5 mM DTT (dithiothreitol). The protein was cleaved on-column by tobacco etch virus (TEV) protease then purified further by cation-exchange chromatography. Proteolytically stable murine PER2 (amino acids 1095–1215) was expressed as a GST-fusion protein in Escherichia coli expression system and isolated through glutathione affinity chromatography using buffer containing 20 mM Tris–HCl pH 8, 300 mM NaCl, 5 mM DTT. The protein was cleaved on-column by TEV protease then purified further by anion-exchange and size-exclusion chromatography. Both proteins were combined, concentrated, and further purified by size-exclusion chromatography using buffer containing 20 mM Tris–HCl pH 8, 300 mM NaCl, 5 mM DTT, 10% glycerol to establish stoichiometric binding.

The crystals of the CRY2-PER2 complex were grown at 4°C by the hanging-drop vapor diffusion method, using 2 μl protein complex sample mixed 2:1 with reservoir solution containing 100 mM HEPES pH 7.5, 200 mM NaCl, 15% PEG 3350. Diffraction-quality crystals were subjected to a cryo-protectant procedure by gradually increasing the concentration of ethylene glycol to 25% (vol/vol) and then frozen in liquid nitrogen. The native and zinc anomalous data sets were collected at the BL8.2.1 beamline at the Advanced Light Source of the Lawrence Berkeley National Laboratory. Reflection data were indexed, integrated, and scaled with the HKL2000 (Otwinowski and Minor, 1997). The CRY2-PER2 complex was determined by molecular replacement using CRY2 from the murine CRY2-KL001 complex structure (PDB:4MLP) as the search model. The structural models were manually built, refined, and rebuilt with the programs COOT (Emsley et al., 2010), PHENIX (Adams et al., 2010), and CCP4 (Winn et al., 2011). PER2 was built in following density modification. All figures were made using PyMOL (Schrödinger, LLC). Buried surface area was calculated using CNS (Brunger et al., 1998).

GST-tagged mCRY2 (amino acids 1–512) was over-expressed in High Five insect cells suspension culture. GST-tagged mPER2 WT (amino acids 1095–1215) and GST-tagged mPER2ΔCXXC (amino acids 1095–1209) were over-expressed in E. coli and purified as previously described. Equal volumes CRY2-PHR was incubated with immobilized PER2 at 4°C for 1 hr. Glutathione beads were rigorously washed, and GST-PER2-CRY2 was released from the beads with SDS sample buffer, analyzed by SDS-PAGE and detected by Coomasssie stain.

N-terminal Myc-tagged Cry2 (0.25 μg) and a C-terminal V5-tagged Per2 (0.5 μg) were transfected (Fugene 6, Madison, WI) into HEK293 cells. After 48 hr, cells were harvested and lysed by centrifugation. α-MYC-conjugated beads were used to immobilize MYC-CRY2. Beads were washed with buffer containing 50 mM Tris–HCl pH 7.5, 100 mM NaCl, 5% glycerol, 0.5 mM DTT, 0.5% Triton X-100, protease inhibitor (1:50). Protein was released from beads with SDS sample buffer and analyzed by Western blot using α-MYC and α-V5 for CRY2 and PER2, respectively.

Real-time circadian rescue assays performed as described in Ukai-Tadenuma et al. (2011). Cry1^−/−/Cry2^−/− MEFs were plated in 35-mm dishes at a density of 5 × 10⁵ cells per dish. 24 hr later, cells were transfected with FuGene6 with 4 μg of pGL3-P(Per2)-dLuc reporter plasmid and 150 ng of the pMU2-mCry1 expression vector (Ukai-Tadenuma et al., 2011) or mutant forms of this vector. 72 hr after transfection, the cells were synchronized by a 2-hr incubation in medium (DMEM/10% FBS/antibiotics) with dexamethasone (1 μM). The medium was then replaced with medium prepared from powdered DMEM without phenol red (Corning 90-013-PB) containing 4.5 g/l glucose and supplemented with 10 mM HEPES pH 7.2, 100 μM luciferin, 1 mM sodium pyruvate, 0.035% sodium bicarbonate, 10% FBS, antibiotics, and 2 mM L-glutamine. Bioluminescence monitoring was performed using a LumiCycle (Actimetrics, Inc. Wilmette, IL) to record from each dish continuously for ∼70 s every 10 min using a photomultiplier tube at 37°C.