Nuclear CK1δ as a critical determinant of PER:CRY complex dynamics and circadian period

Circadian clocks are molecular oscillators that regulate 24-hr physiological rhythms as an adaptive response to day–night cycles (Takahashi, 2017; Partch, 2020). In mammals, the core clock relies on a delayed negative transcription–translation feedback loop (TTFL), in which the transcriptional activators BMAL1 and CLOCK drive the expression of their inhibitors, PERIOD (PER) and CRYPTOCHROME (CRY) proteins (Lee et al., 2001; Bell-Pedersen et al., 2005; Partch et al., 2014). This core loop is reinforced by a secondary feedback loop in which the nuclear receptors RORs and REV-ERBs connect the core oscillator to cellular metabolism by activating and repressing BMAL1 transcription, respectively (Preitner et al., 2002; Sato et al., 2004). Circadian clocks are expressed in many tissues and entrained by daily recurring cues. Entraining environmental light cues are received by the suprachiasmatic nucleus (SCN), which directly and indirectly synchronizes clocks in peripheral organs via neuronal and hormonal/humoral cues. Recurring metabolic cues entrain peripheral clocks in the liver and other organs and determine their phase relative to the 24-hr light–dark cycle. The circadian system directly and indirectly controls key metabolic pathways (Ramsey et al., 2007; Dibner et al., 2010; Mohawk et al., 2012).

The prevailing ‘dual-mode of circadian repression’ model offers a robust framework for understanding the circadian clock on the molecular level, distinguishing between the so-called ‘early’ and ‘late’ repressive phases. During the early repressive phase, a complex composed of PERs, CRYs, and casein kinase 1δ (CK1δ) assembles on CLOCK:BMAL1, leading to CLOCK phosphorylation, reducing CLOCK:BMAL1 binding to DNA, and thereby resulting in ‘displacement’-type repression. In the late repressive phase, phosphorylated PER proteins are degraded and the remaining CRY1 directly suppresses CLOCK:BMAL1 by sequestering the BMAL1 transactivation domain (TAD), resulting in ‘blocking’-type repression. Upon CLOCK dephosphorylation, the CLOCK:BMAL1 complex re-associates with DNA, establishing a poised promoter state. This configuration is characterized by transcriptional readiness, awaiting CRY1 to decrease below a threshold allowing reinitiation of the circadian transcriptional cycle (Cao et al., 2023; Koike et al., 2012; Ye et al., 2014; Chiou et al., 2016; Aryal et al., 2017; Michael et al., 2017; Fribourgh et al., 2020). It has been shown recently that CLOCK:BMAL1 in the SCN remains partially repressed by CRY1 even at peak circadian transcription (Smyllie et al., 2025), a mechanism that may ensure responsiveness of the circadian clock to synchronizing cues (Smyllie et al., 2025; Brunner, 2025).

Clock component homologs generally have redundant functions but differ in expression phases and binding affinities. PER1 and PER2 are both essential for maintaining robust circadian rhythms. PER1, expressed earlier, shortens the circadian period when PER2 is absent, whereas PER2 lengthens the period when PER1 is absent; PER3 plays a less critical role (Bae et al., 2001; Zheng et al., 2001). CRY1 and CRY2 exhibit overlapping repressive functions when complexed with PER proteins. In addition, CRY1, but not CRY2, serves as a potent repressor of CLOCK:BMAL1 after PERs are degraded (Lee et al., 2001; Griffin et al., 1999; Horst et al., 1999). As a consequence, CRY1 lengthens and CRY2 shortens circadian period (Horst et al., 1999). The casein kinase 1 splice isoforms CK1δ1 and CK1δ2, and the similar CK1ε all support the clock, with their contributions varying potentially by tissue-specific expression (Fustin et al., 2018; Lee et al., 2009). Likewise, NPAS2 can partially substitute for CLOCK in a tissue-specific manner (Landgraf et al., 2016).

PER proteins serve as limiting scaffolds for the assembly of the repressive complex, playing a key role in circadian timing. CK1δ is crucial in regulating PER stability and function by phosphorylating PER proteins at numerous sites. A central aspect of this regulation involves the phosphorylation of hPER2 at S662 (S659 in mPer2) within the FASP (Familial Advanced Sleep Phase) region by CK1δ bound to the Casein Kinase Binding Domain (CKBD) (Toh et al., 2001; Vanselow et al., 2006). This priming phosphorylation triggers rapid phosphorylation of four additional equally spaced residues in the FASP region. When fully phosphorylated, the FASP region inhibits CK1δ by blocking its active site (Philpott et al., 2023). This attenuation slows the phosphorylation of hPER2 S478 (S475 in mPer2), a residue within the β-TrCP phosphodegron, thereby delaying PER2 degradation, which is thus aligned with the circadian time frame (Zhou et al., 2015). This so-called ‘phosphoswitch’ mechanism is well-characterized, involving the phosphorylation of five residues in the FASP region and one in the β-TrCP degron of PER2 (Zhou et al., 2015; Narasimamurthy et al., 2018; Philpott et al., 2020). Phosphorylation of the FASP and β-TrCP regions severely impacts circadian period length but is not essential for circadian clock function per se. PER proteins are subjected to extensive hyperphosphorylation at numerous additional sites (about 80 in PER2) distributed across the protein (Hornbeck et al., 2015). The kinetics of this widespread hyperphosphorylation strongly correlate with circadian timekeeping (Marzoll et al., 2022), but the functional significance of these modifications remains largely unknown. While it has been shown that phosphorylation of mPER1 masks a nuclear localization signal (NLS; Vielhaber et al., 2000), the potential impact of PER phosphorylation on subcellular localization and interaction with other proteins has not been systematically analyzed. Furthermore, CK1δ is the main circadian kinase but is implicated in other essential cellular functions including regulation of the cell cycle and Wnt signaling (Schittek and Sinnberg, 2014; Cruciat, 2014). The regulation, subcellular distribution, and functional allocation of CK1δ to its various tasks have yet to be fully elucidated.

Circadian proteins are expressed at relatively low physiological levels, with many studies analyzing endogenous proteins contributing to our current understanding of the clock (Aryal et al., 2017; Smyllie et al., 2016; Smyllie et al., 2022; Öllinger et al., 2014; Gabriel et al., 2021; Gabriel et al., 2024; Xie et al., 2023; Guillen et al., 2020). To complement these studies and gain additional mechanistic insight, we utilized an inducible cellular overexpression approach combined with time-lapse live-cell imaging to investigate the dynamic interactions and subcellular localizations of CK1δ, PER2, and CRY1 without interference from their endogenously expressed specific binding partners. Our findings reveal that PER2 and CRY1 mutually influence their stability, as well as their nuclear–cytoplasmic shuttling dynamics and equilibrium. We demonstrate that CK1δ turnover and shuttling are modulated in a kinase activity-dependent manner such that free active nuclear CK1δ is rapidly degraded, making it a limiting factor for interactions with nuclear PER2. In contrast, CK1δ is readily available in the cytosol. Phosphorylation of PER2 by CK1δ drives, with a delay, PER2 cytosolic localization and, interestingly, disrupts PER2–CRY1 interaction. Translocation of the released CRY1 into the nucleus could then contribute to blocking-type repression of CLOCK:BMAL1.

The current dual-mode circadian repression model describes three distinct phases of CLOCK:BMAL1 activity, regulated in temporal succession by CRY1/2, PER1/2, and CK1δ (Ye et al., 2014; Chiou et al., 2016; Aryal et al., 2017; Michael et al., 2017; Fribourgh et al., 2020; Cao et al., 2021). Initially, CLOCK:BMAL1 is predominantly repressed via PER:CRY:CK1δ-mediated displacement from its target genes, followed later by CRY1-dependent blocking of DNA-bound CLOCK:BMAL1, and finally derepression of CLOCK:BMAL1 when PER proteins are degraded and CRY1 levels decline below a critical threshold. Within the framework of current circadian clock models, CK1δ is assumed to be non-limiting and readily available to PER proteins as they are synthesized in the cytosol, thereby ensuring robust and precise timekeeping.

The data presented here suggest that freely available CK1δ is limited within the nucleus. Previous work has shown that nuclear export of CK1δ depends on its kinase activity (Milne et al., 2001). We confirm these findings and extend them by demonstrating that unassembled nuclear CK1δ is subject to rapid degradation, with turnover further accelerated by its catalytic activity. Mechanistically, the activity dependence of both processes may reflect a shared mechanism, such as activity-dependent release from nuclear binding sites. Moreover, we show that CK1δ is stabilized through association with PER2. The data align with earlier findings and provide a mechanistic explanation for why nuclear CK1δ levels in mouse liver remain very low in the absence of PER proteins, but increase in parallel with the circadian accumulation of nuclear PER, while cytoplasmic CK1δ levels remain constant and higher than those in the nucleus (Cao et al., 2021). Complex formation between CK1δ and PER proteins is well established as essential for circadian timekeeping (Cao et al., 2023), with CK1δ1 overexpression known to shorten circadian period length (Marzoll et al., 2022). Our results suggest that the subcellular distribution of CK1δ is finely tuned and suggest that nuclear concentrations remain, at least temporarily, below the threshold required for PER saturation. Specifically, overexpression of NLS-tagged CK1δ shortens period length, whereas NES-tagged CK1δ has no detectable effect. This is consistent with previous studies showing that PER associates with CK1δ in the cytosol and enters the nucleus facilitated by CRY (Lee et al., 2001; Aryal et al., 2017; Cao et al., 2021). Because each PER molecule can import only one kinase, and this process likely already occurs at wild-type cytosolic CK1δ levels, overexpression of NES-tagged CK1δ does not increase the nuclear CK1δ pool. The few CK1δ molecules co-imported with PER:CRY complexes equilibrate with the unbound nuclear pool. Early in the circadian cycle, when nuclear PER levels are low, free nuclear CK1δ is more likely to be degraded or exported to the cytosol than to rebind PER. As nuclear PER accumulates, it gradually competes for rebinding of free CK1δ, introducing a delay. In contrast, overexpression of NLS-tagged CK1δ promotes PER binding already early in the circadian cycle, thereby shortening the period.

Thus, when evaluating the impact of CK1δ/ε mutants on the circadian clock, not only kinase activity but also protein stability and subcellular distribution must be taken into account. Indeed, we observed that the altered activity of the tau-like CK1δ1-R178Q mutant affects its subcellular localization and turnover, leading to its accumulation at elevated levels in the nucleus. Analysis of the PER2 phosphoswitch provides strong evidence that the tau mutation (e.g., R178C in CK1δ) shortens the circadian period by attenuating phosphorylation of the FASP region in PER2 while accelerating phosphorylation of the β-TrCP degron site (S478 in mPER2) (Zhou et al., 2015; Narasimamurthy et al., 2018; Philpott et al., 2020). We demonstrate that the period shortening induced by the tau-like CK1δ1-R178Q mutant (Marzoll et al., 2022) can be partially replicated by forcing nuclear accumulation of wild-type CK1δ1 using an NLS tag (mNG-NLS-CK1δ1). Thus, the elevated nuclear accumulation of tau-like kinase may, in addition to its altered substrate specificity (Philpott et al., 2020; Gallego et al., 2006), contribute to the period-shortening phenotype observed in tau mutant animals (Lowrey et al., 2000; Meng et al., 2008).

This study examines the subcellular localization and interplay between PER:CRY:CK1δ complexes and CRY1. In the prevailing circadian model, transcriptional feedback is driven initially by the nuclear accumulation of PER:CRY:CK1δ repressor complexes. This is followed in the late phase by sustained repression mediated by CRY1 alone, which persists for several hours after CK1δ-dependent degradation of PER proteins. However, evidence from mouse liver (Cao et al., 2021), SCN slices (Smyllie et al., 2025), and U2OS cells (Xie et al., 2023) and this study indicates that a substantial fraction of PER2 remains cytoplasmic, even when CRY1 is present, which normally supports nuclear import of the PER:CRY complex. While several mechanisms underlying cytoplasmic localization of PER2 have been proposed (Smyllie et al., 2016; Vielhaber et al., 2001), no circadian function has yet been attributed to the cytosolic PER2 pool.

We show by transient transfection and overexpression that the distribution of PER2 between cytoplasm and nucleus depends on the expression ratio of PER2 and CRY1. DOX-induced transient overexpression was necessary to analyze how PER2 and CRY1 influence each other’s subcellular localization and dynamics while excluding contributions from endogenous PER1 and CRY2. Our data suggest that PER2 dimers and dimers bound by a single CRY1 molecule are predominantly cytosolic, whereas dimers bound by two CRY1 molecules are enriched in the nucleus (see Figure 1E). In the physiological context of a functional clock, PER1, CRY2, PER2, and CRY1 are rhythmically expressed with consecutive peaks at different CTs (Koike et al., 2012; Narumi et al., 2016). Since their expression ratios and levels vary over the course of a circadian cycle (Narumi et al., 2016), the composition and saturation of PER complexes by CRYs depend on both their specific expression levels, subcellular localization, and binding affinities. Furthermore, our data show that CK1δ-mediated phosphorylation promotes dissociation of bound CRY1, thereby supporting the cytoplasmic accumulation of PER2 dimers containing one or no CRY1 molecule. In the context of a functional circadian clock in U2OS cells, we observe that the subcellular distribution of PER2 shifts from predominantly nuclear to increasingly cytoplasmic over the course of the circadian cycle, consistent with our overexpression data. Inhibition of CK1δ/ε reverses this process, leading to dephosphorylation of cytosolic PER2 and its accumulation in the nucleus. Consistent with these observations, hyperphosphorylated PER2 is predominantly cytoplasmic in mouse liver (Cao et al., 2021) and U2OS cells (Xie et al., 2023).

Incorporating these findings into the current circadian framework, we propose that the transition between the early and late repressive phases involves a decline in nuclear PER2:CRY1:CK1δ complex levels, driven by both PER2 degradation and cytoplasmic relocalization. PER2 degradation and reduction of nuclear PER2:CRY1:CK1δ complexes by export below a critical threshold could provide a time window for CLOCK dephosphorylation and facilitate subsequent rebinding of CLOCK:BMAL1 to DNA. In addition, cytoplasmic PER2:CRY1:CK1δ complexes could act as a reservoir, gradually releasing CRY1 in a CK1δ-dependent manner to support repression of DNA-bound CLOCK:BMAL1, complementing de novo CRY1 synthesis, which peaks as PER2 levels fall. The contribution to repression by newly synthesized CRY1 and by CRY1 released from cytosolic PER2 could vary by cell type and physiological conditions. Supporting this, our data show that nuclear CRY1 levels are markedly higher and more sustained in CRY1-expressing U2OStx cells that overexpress and accumulate PER2 and CK1δ in the cytosol.

The fact that both PER1/2:CRY1/2:CK1δ complexes and CRY1 alone repress CLOCK:BMAL1 raises the question of whether the mammalian circadian clock gains a functional advantage from maintaining both repressive modes. Published data indicate that CRY1 is present and functionally active throughout the entire circadian cycle (Smyllie et al., 2025; Park et al., 2023). Although both PER and CRY proteins are rhythmically expressed, quantitative analyses reveal that PER protein levels are very low when CLOCK:BMAL1 activity reaches its circadian maximum, whereas CRY1 remains at ~50% of its peak level (Smyllie et al., 2025; Narumi et al., 2016). Moreover, ChIP-seq analyses in mouse liver show that CRY1 is bound to circadian promoters not only during the late repressive phase (CT0-4), but also at CT8-12, when CLOCK:BMAL1 activity is maximal (Koike et al., 2012). Finally, studies of endogenously tagged PER2-LUC demonstrated that PER2 oscillates around an elevated baseline in CRY1 knock-out U2OS cells and around a reduced baseline in CRY2 knock-out cells (Park et al., 2023). These findings suggest that in U2OS cells, CRY1 partially represses CLOCK:BMAL1 even during the circadian peak of transcription. Together, these observations support the view that CRY1 attenuates CLOCK:BMAL1 activity across the entire circadian cycle. Consequently, whereas PER1/2:CRY1/2:CK1δ complexes primarily regulate the troughs of circadian gene expression, CRY1 may act to limit the peak amplitude of CLOCK:BMAL1-dependent transcription, thereby enhancing the dynamic range and responsiveness of the clock during this phase.

In summary, our data suggest that cytoplasmic CK1δ is readily available to assemble in a one-to-one complex with PER proteins. After nuclear import of the PER:CRY:CK1δ complex, the bound kinase will equilibrate with the nuclear CK1δ pool. Because the nuclear CK1δ concentration is low, rebinding of CK1δ may not allow saturation of PERs in steady state. This provides a mechanistic explanation for why overexpression of nuclear CK1δ shortens circadian period length while overexpression of cytosolic CK1δ has no effect. Moreover, our overexpression data suggest that CK1δ-mediated phosphorylation disrupts PER2–CRY1 complexes, promoting the buildup of cytosolic PER2 complexes with substoichiometric CRY1 bound, while unbound CRY1 may gradually accumulate in the nucleus, a process analogous to nuclear import of newly synthesized CRY1. In the physiological context of a functional clock, the redistribution of CRY1 could contribute to establishing the poised promoter state with CLOCK:BMAL1.

Many of our conclusions are derived from synchronized DOX-induced overexpression of tagged clock proteins combined with time-lapse live-cell microscopy. While this approach was necessary to capture mechanistic insights that would be technically challenging or impossible to resolve under physiological protein levels, it will require further validation with other methods and in other systems. Nonetheless, our findings align well with and recontextualize independent observations of clock protein levels, phosphorylation states, and subcellular localization in mouse liver (Cao et al., 2023; Cao et al., 2021) and the SCN (Smyllie et al., 2025; Smyllie et al., 2022), thereby contributing to our understanding of the repressive phase of the core circadian clock.

The data supporting the findings of this study are available within the article and its supplementary information files. This study includes no data deposited in external repositories.

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Author details

1. Fidel Emmanuel Serrano

   Heidelberg University Biochemistry Center, Heidelberg, Germany

   Contribution

   Formal analysis, Investigation, Visualization, Methodology, Writing – original draft, Writing – review and editing

   Competing interests

   No competing interests declared

   "This ORCID iD identifies the author of this article:" 0000-0001-8906-9343

2. Daniela Marzoll

   Heidelberg University Biochemistry Center, Heidelberg, Germany

   Contribution

   Methodology

   Competing interests

   No competing interests declared

3. Bianca Ruppert

   Heidelberg University Biochemistry Center, Heidelberg, Germany

   Contribution

   Investigation, Methodology

   Competing interests

   No competing interests declared

4. Axel CR Diernfellner

   Heidelberg University Biochemistry Center, Heidelberg, Germany

   Contribution

   Supervision, Methodology, Project administration

   Competing interests

   No competing interests declared

5. Michael Brunner

   Heidelberg University Biochemistry Center, Heidelberg, Germany

   Contribution

   Conceptualization, Supervision, Funding acquisition, Writing – original draft, Project administration, Writing – review and editing

   For correspondence

   michael.brunner@bzh.uni-heidelberg.de

   Competing interests

   No competing interests declared

   "This ORCID iD identifies the author of this article:" 0000-0001-9798-3047

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