Introduction
The mammalian circadian timing system has a hierarchical structure, in that a master pacemaker residing in the suprachiasmatic nucleus synchronizes slave oscillators existing in most body cells (Takahashi, 2004; Reppert, 2006). Cell-autonomous and self-sustained clocks were also found in cultured cells (Balsalobre et al, 1998; Nagoshi et al, 2004; Liu et al, 2007).
In 1990, Rosbash and co-workers (Hardin et al, 1990) discovered that the Drosophila clock protein Period (PER) inhibits the transcription of its own gene, and hence proposed a negative transcription/translation feedback loop as the operational principle for rhythm generation. Since then a large number of circadian clock genes have been identified in a variety of organisms from cyanobacteria to humans, and negative feedback loops are still the prevalent model for most of these organisms (Lakin-Thomas, 2006; Gallego and Virshup, 2007). In mammals, the CLOCK and BMAL1 transcription factors activate the expression of Per and Cry genes. Once PER and CRY concentrations have reached a critical threshold, they attenuate the CLOCK/BMAL1-mediated activation of their own genes in a negative feedback loop (Hastings and Herzog, 2004; Reppert, 2006). However, posttranslational events, such as the control of protein phosphorylation, acetylation, degradation, sumoylation and nucleocytoplasmic shuttling, contribute critically to the circadian rhythm generation and may affect period length, amplitude and/or magnitude of the oscillations (Lee et al, 2001; Cardone et al, 2005; Asher et al, 2008).
Although most physiological processes run faster at higher temperature, the period length of circadian oscillators remains nearly constant over a wide range of physiological temperatures (Konopka et al, 1989; Kaushik et al, 2007; Takeuchi et al, 2007). This even applies to circadian oscillators of homoeotherm organisms, such as those operative in cultured mammalian fibroblasts (Izumo et al, 2003; Tsuchiya et al, 2003). Here, we show that circadian clocks of fibroblasts are also compensated for global transcription rates. Considering that intrinsic transcription rates vary significantly in cells from different tissues (Schmidt and Schibler, 1995), transcription compensation may be an important property of peripheral circadian clocks.
Results
Long-term inhibition of RNA polymerase II-dependent transcription
Global transcription rates can be attenuated by the exposure of cells to various drugs that function at different steps. The most widely used compounds are actinomycin D and α-amanitin. Actinomycin D intercalates into double-stranded DNA and blocks transcription elongation by all three polymerases, RNA polymerase I (Pol I) being particularly sensitive. α-Amanitin is a selective and specific inhibitor of RNA polymerase II (Pol II) and RNA polymerase III (Pol III) in vitro and in vivo, with Pol II being considerably more sensitive than Pol III. α-Amanitin binds to RPB1, the largest Pol II subunit, with high affinity and thereby prevents translocation by blocking Pol II bridge helix bending (Bushnell et al, 2002). In addition, this drug induces the ubiquitination of the C-terminal domain of RPB1 and elicits proteasome-mediated RPB1 degradation in a dose-dependent manner (Nguyen et al, 1996; Mitsui and Sharp, 1999; Arima et al, 2005).
To examine the impact of overall transcription rates on circadian oscillator function, we analysed circadian gene expression in α-amanitin- and actinomycin D-treated fibroblasts. To this end, we had to identify conditions that allowed the recording of gene expression for extended time periods. Long-term treatment with α-amanitin and actinomycin D at concentrations higher than 0.5 μg/ml and 10 nM, respectively, caused significant cell death (Supplementary Figure 1A and B). However, the pretreatment of cells with sublethal doses of α-amanitin and actinomycin D for 16 and 5 h, respectively, allowed the recording of circadian bioluminescence during at least 3 days at reduced transcription rates (see Figure 1A for experimental design).
To validate this approach, we estimated the inhibitory effects of α-amanitin and actinomycin D on Pol II-dependent transcription by several methods (Figure 1B–E) and assayed transcription rates or RPB1 expression during 48–72 h after the drugs were washed away. First, in vivo transcription rates in NIH3T3 cells pretreated for 16 h with α-amanitin (3–5 μg/ml) or in untreated cells were measured by the incorporation of [3H]uridine after labelling the cells for 60 min (Figure 1B). In keeping with previous publications (Adolph et al, 1993), we found that pretreatment of NIH3T3 cells with 3 and 5 μg/ml of α-amanitin for 16 h reduced RNA synthesis to about 60 and 35%, respectively, when compared with untreated cells (Figure 1B, panel 0 h). The inhibitory effect of α-amanitin on overall transcription rates persisted for at least 48 h (Figure 1B). In the second approach, in vitro incorporation of [32P]UTP (uridine triphosphate) was measured in isolated cell nuclei by run-on transcription assays under conditions favouring efficient elongation predominantly by Pol II (Gariglio et al, 1981; Schmidt and Schibler, 1995). Pretreatment with α-amanitin (3 μg/ml) abolished about 85% of Pol II-dependent transcription immediately after drug elimination, and about 70% after 72 h (Figure 1C). Actinomycin D (50 nM) inhibited about half of Pol II-dependent transcription immediately after drug removal, with partial recovery to 73% after 72 h (Figure 1C). We noticed that the incorporation rate of uridine into RNA in α-amanitin-pretreated cells (Figure 1 B) was somewhat higher after 48 h than expected on the basis of the in vitro run-on experiments performed with cells analysed 72 h after the pretreatment (Figure 1C). This may have been caused by a reduction of the nuclear UTP pool size, which is difficult to measure experimentally.
Next, we determined the effect of α-amanitin on the induction of c-fos precursor RNA by a serum shock (Adolph et al, 1993) and found that this immediate early response was significantly dampened in drug-treated cells (Figure 1D). Finally, we evaluated α-amanitin-mediated RPB1 degradation. As shown in Figure 1E, a western blot analysis revealed a strong reduction in RPB1 protein levels after a 16-h treatment of cells with 3 μg/ml α-amanitin, and RPB1 accumulation remained low for at least 48 h (Figure 1E).
Inhibition of clock gene transcription by -amanitin
To determine the impact of α-amanitin treatment on the transcription of core clock genes, mRNA accumulation patterns for synchronized NIH3T3 cells were monitored by quantitative RT–PCR using amplicons for Bmal1, Rev-erbα, Dbp, Per1 and Per2. The values thus obtained were then normalized to Q-PCR values measured for a Gapdh amplicon in genomic DNA from duplicate plates, to express transcript accumulation levels in cellular equivalents (see Materials and methods). As shown in Figure 2, the α-amanitin treatment inhibited the cellular accumulation of transcripts specified by all examined core clock and clock-controlled genes, albeit to somewhat different extents. Genes such as Per1, Per2 and Dbp, the transcription of which is activated by BMAL1-CLOCK and repressed by PER–CRY complexes, were particularly sensitive to α-amanitin treatment. In addition, the serum-induced immediate early induction of Per1 and Per2 expression was strongly blunted in drug-treated cells (Figure 2). Although these experiments suggested that NIH3T3 clocks still function in α-amanitin-treated cells, the low magnitude, amplitude and temporal resolution observed in the temporal mRNA accumulation profiles did not allow for a more detailed characterization of circadian phenotypes caused by the reduction of global transcription rates. Hence, we resorted to more sensitive reporter gene assays with a high temporal resolution power.
Circadian gene expression is resilient to large fluctuations in transcription rates
Fibroblasts expressing fire fly luciferase from circadian promoters exhibit robust circadian bioluminescence rhythms in synchronized cell populations and individual cells (Nagoshi et al, 2004; Liu et al, 2007). To assess the impact of reduced transcription on circadian gene expression, we monitored circadian bioluminescence of synchronized NIH3T3 fibroblasts stably expressing luciferase driven from Bmal1 promoter (Nagoshi et al, 2004) after a 16-h pretreatment with sublethal concentrations of α-amanitin and actinomycin D. As shown in Figure 3A, robust bioluminescence cycles could be detected in cells pretreated with 1–3 μg/ml of α-amanitin, and residual oscillation was observed in experiments with 5 μg/ml. As expected, the magnitude of Bmal1-luc expression progressively decreased with increasing α-amanitin concentrations (Figure 3A, right panel). Unexpectedly, however, period length gradually shortened with decreasing overall transcription rates (Figure 3A, middle panel). Thus, cells pretreated with 3 μg/ml α-amanitin oscillated with a 2.3-h shorter period than untreated cells. Actinomycin D pretreatment had similar effects on the bioluminescence cycles generated by Bmal1-luc cells (Figure 3B, left panel). Similar to α-amanitin, actinomycin D reduced the magnitude, amplitude and period length of circadian Bmal1-luc expression (Figure 3B). Pretreatment with α-amanitin and actinomycin D also caused a shortening of the period length and a dampening of amplitude and magnitude of bioluminescence cycles produced by skin tail fibroblasts from mPer2∷luciferase mice (Supplementary Figure 2A and B). α-Amanitin had a similar effect on NIH3T3 cells expressing luciferase from Dbp regulatory sequence oscillation pattern (Supplementary Figure 2C).
As shown in Supplementary Figure 3, α-amanitin affected circadian gene expression to a similar extent in cells synchronized by a short incubation with dexamethasone, horse serum or glucose (Balsalobre et al, 2000; Hirota et al, 2002). Thus, the alterations in circadian gene expression caused by transcription-inhibiting drugs depend neither on the signalling pathways used for the synchronization of cells nor on the expressed circadian reporter genes.
Individual fibroblast clocks exhibit robust oscillations in cells with reduced global transcription rates
At the population level, Bmal1-1uc cells exhibited progressively lower amplitude and magnitude oscillations as transcription rates dropped (Figure 3). The reduction in amplitude could have reflected a dampening of individual oscillators, and/or an inefficient synchronization between oscillators. To discriminate between these possibilities, we analysed temporal Bmal1-luc expression in individual cells treated with or without 3 or 5 μg/ml of α-amanitin, using the Olympus LV 200 bioluminescence workstation, a highly sensitive photon-counting microscope (see Materials and methods). As demonstrated by the time-lapse video recording provided in Supplementary data and at representative single-cell bioluminescence profiles (Figure 4A, B (control panel) and E), most of the recorded untreated cells (90%) exhibited robust circadian oscillations. Here, 78% of cells pretreated with 3 μg/ml of α-amanitin also displayed rhythmic Bmal1-luc expression, albeit with a 25% lower magnitude on average, in comparison to untreated counterparts (Figure 4B (α-amanitin 3 μg/ml panel) and 4E; Supplementary data). Here, 65% of cells pretreated with 5 μg/ml of α-amanitin still exhibited circadian Bmal1-luc luminescence cycles, with 50% lower magnitude in comparison to control (Figure 4B (α-amanitin 5 μg/ml panel) and 4E; Supplementary data). For both period length and signal sum intensity, the distribution was clearly shifted towards lower values for α-amanitin-treated cells versus untreated control cells, and the mean values were in good agreement with our results obtained with cell populations (Figure 4C and D).
In conclusion, our single-cell recordings suggested that the partial inhibition of transcription by α-amanitin did not arrest cell-autonomous clocks, but rather dampened the magnitude and shortened the period length. In addition, α-amanitin treatment led to a wider distribution of period lengths. The blunted amplitudes of α-amanitin-treated cells revealed by population analysis were thus caused by smaller fraction of rhythmic cells, a widened period length distribution and reduced amplitude of individual cells.
Temperature and transcription compensation: manifestations of the same underlying principle?
Circadian oscillators have long been known to be temperature-compensated for both poikilotherm and homoeotherm organisms (Pittendrigh, 1954; Konopka et al, 1989). In fact, those of mammalian fibroblasts exhibit even a temperature ‘overcompensation', that is, they run faster at lower temperatures (Izumo et al, 2003; Tsuchiya et al, 2003). In agreement with the conclusions made by these authors, our bioluminescence recordings obtained with Bmal1-luc cells (Figure 5A) and primary skin tail fibroblasts from mPer2∷luc mice (Figure 6D) suggested a decrease in period length with descending temperature. As reduced temperature and transcription had similar effects on oscillator period length, we examined whether the period shortening is additive in α-amanitin-treated cells at reduced temperature. At 37°C, the drug affected circadian amplitude and period length as expected (Figure 5B). However, as depicted in Figure 5C, transcription inhibition had only a small effect on period length in cells incubated at 33°C. Hence, transcription and temperature compensation might be manifestations of similar oscillator features (see Discussion).
Temperature and transcription compensation in mPer1 knockout cells
As described earlier, the per gene has a key function in temperature compensation in Drosophila, and a mutation in the dimerization domain (PAS) of per renders the Drosophila oscillator temperature sensitive (Konopka et al, 1989). We thus wished to examine the possible role of Per1 in temperature and transcription compensation. As Per2-deficient fibroblasts are arrhythmic at the population level (Brown et al, 2005) and displayed unstable rhythms of low amplitude or were arrhythmic at the single-cell level (Liu et al, 2007), the role of PER2 in these processes could not be assessed. Per1 knockout mice (Zheng et al, 2001) were crossed with Per2∷luc knock-in reporter mice (Yoo et al, 2004). Per1 knockout primary fibroblasts were shown to exhibit about 3 h shorter circadian period in comparison to wild-type cells (Pando et al, 2002; Brown et al, 2005). In keeping with these observations, bioluminescence cycles produced by Per1KO/Per2∷luc fibroblasts displayed 2–3 h shorter period as compared with their Per1+/+/Per2∷luc counterparts. Interestingly, however, the period length of these cells remained similar when transcription rates were reduced by a treatment with α-amanitin or actinomycin D (Figure 6A; period lengths for control, α-amanitin- and actinomycin D-treated cell lines are indicated on the graph). These values were similar when extracted from the mathematical derivatives of the raw data curves, in which the oscillations are accentuated (Figure 6B). Unexpectedly, the amplitude—which was found to be low in untreated Per1KO/Per2∷luc cells (Brown et al, 2005; Liu et al, 2007)—became somewhat more robust in actinomycin D-pretreated cells.
To characterize the oscillator properties of Per1KO/Per2∷luc cells further, we assessed their bioluminescence cycles at different temperatures. Remarkably, the period length of these fibroblasts was about 1 hour shorter at higher temperature within the examined 32–39°C range (Figure 6C). Our analysis thus suggested that the period of Per1KO cells became slightly shorter at higher temperature, opposite from the trend observed for their wild-type counterparts (see Figure 6E for comparison of period length change as depicted in Figure 6C and D). Hence, the temperature ‘overcompensation' typical for fibroblast oscillators depended on Per1, suggesting that this protein affects the mechanisms underlying both transcription and temperature compensation in mammalian cells.
Period and amplitude behaviour in common circadian oscillator models
To assess how our experimental findings compare with mathematical models for circadian oscillators, we simulated the period and the amplitude properties in two low-dimensional models (Figure 7A and B; Supplementary Figure 4A and B), and two higher dimensional kinetic models for the mammalian oscillator (Figure 7C and D; Supplementary Figure 4C and D). We hypothesized that transcription rates were reduced uniformly by the drugs and thus introduced the scale parameter ρ that rescales all mRNA synthesis rates. The low-dimensional models implement two prototypical designs for circadian oscillators, a delayed negative feedback loop (Figure 7A), related to the Goodwin oscillator (Gonze and Goldbeter, 2006), and a relaxation oscillator (Figure 7B) as proposed by Barkai and Leibler (2000). The first shows a period lengthening and amplitude increase with increasing transcription rates, consistent with our experimental finding (Figure 7A). A similar result was also found for another implementation of a Goodwin-type model (Kurosawa and Iwasa, 2005). In addition, the oscillatory regimen persists for reduction in transcription as large as 40%. Our implementation of a relaxation oscillator shows a relatively stable period dependency in a range around ρ=1, as expected for a relaxation oscillator (Barkai and Leibler, 2000). However, the period globally decreases with transcription rate (Figure 7B) and seems thus unable to account for the experimental data presented here. We now turn to more detailed mammalian models. Even though the Leloup–Goldbeter model (Leloup and Goldbeter, 2003) exhibits the right sign in the dependency of period length on transcription, the transcription range in which the model oscillates is much narrower than observed experimentally (Figure 7C); thus, this model and its parameters are in qualitative agreement with the data. Notice, however, that alternate parameter sets for the same model have been subsequently proposed (Leloup and Goldbeter, 2003), one of which exhibits a wider oscillatory range in the function of the transcription rate. Similar to the relaxation oscillator, the detailed Forger–Peskin model has an opposite period dependency (Forger and Peskin, 2003). Moreover, the half-hour period increase in the simulated case of Per1 knockout is inconsistent with experiments performed by us and others (Zheng et al, 2001; Brown et al, 2005). These simulations thus indicate limited predictability by some of the commonly invoked kinetic models, and suggest that basic architectures based on the Goodwin model come closest to capturing qualitatively the period shortening observed on reducing transcription rates. In fact, the Bmal1 loop in the Leloup–Goldbeter model is very much reminiscent of the three species Goodwin-type model.
Discussion
Fibroblast circadian oscillators are resilient to large reductions in transcription rates
We demonstrate here that circadian oscillators keep running in mouse fibroblasts in which overall Pol II-dependent transcription rates are reduced up to three-fold. Inhibition of transcription dampened the magnitudes and amplitudes of clock gene expression cycles but did not eliminate them. The observed resilience to reduced overall transcription rates cannot be readily explained by a compensation of core clock gene expression at the level of protein accumulation, as in α-amanitin-treated cells, decreased Per2 and Cry2 mRNA levels were accompanied by reduced PER2 and CRY2 protein levels (Supplementary Figure 5). Hence, the negative feedback loop does not appear to be based on a stoichiometric mechanism requiring absolute cellular threshold concentrations of CRYs and PERs. Rather, these proteins may function as cofactors in enzymatic processes, for example those involved in regulating the circadian DNA affinity of BMAL1 and/or CLOCK/NPAS2, critical activators of Per and Cry genes. BMAL1 and CLOCK and their Drosophila orthologues CLK and CYC accumulate at similar levels throughout the day, but display a rhythmic affinity for their E-box cognate sequences both in vivo and in vitro (Ripperger and Schibler, 2006; Reinke et al, 2008; Taylor and Hardin, 2008). In agreement with our statement of mammalian oscillator compensation for large changes in transcription, Fan et al (2007) have demonstrated that CRY1, CRY2 and BMAL1 protein oscillation were not necessary for proper oscillator function in mouse, Rat-1 and HEK293 cells. This report and our own findings are not supportive of the current version of canonical model of transcription–translation feedback loop.
In the circadian clock of the filamentous fungus Neurospora crassa, the repressor protein FRQ serves as a cofactor of protein kinases to modulate the cyclic DNA-binding activity of the transcription factor complex WCC (Brunner and Kaldi, 2008). A similar scenario may apply to the control of CLOCK and BMAL1 activity by PER and CRY proteins (Taylor and Hardin, 2008).
The circadian period shortening was observed irrespective of whether actinomycin D or α-amanitin was used to reduce overall transcription rates. We did observe, however, that actinomycin D also affected the phase and the sharpness of the first bioluminescence peak at the two lower concentrations (Figure 3B). At these doses, the drug is expected to completely suppress ribosomal Pol I-dependent transcription, whereas only partially inhibiting Pol II-mediated transcription. Conceivably, dexamethasone-induced immediate early expression (e.g. that of PER1)—which is responsible for the timing and duration of the first Bmal1-luc expression peak and the synchronization of cellular oscillators—is altered in cells with an increased mRNA/ribosome ratio. Alternatively, the arrest of ribosomal RNA transcription by RNA Pol I may release rate-limiting components required for immediate early gene expression. RNA Pol I accounts for a very large fraction of total nuclear RNA synthesis, and some regulatory proteins (e.g. TBP, TFIIH) are shared by the RNA Pol I and II transcription machineries (Eberhard et al, 1993; Iben et al, 2002).
The effect of reduced transcription rates on circadian gene expression was also examined by single-cell bioluminescence analysis (Supplementary movies 1, 2 and 3). The period distribution of drug-treated cells was wider and shifted towards shorter values when compared with untreated cells. The broadening in period distributions is perfectly consistent with increased intrinsic noise resulting from a reduced number of transcripts (Gonze and Goldbeter, 2006). On average, the magnitudes of the bioluminescence cycles were reduced in drug-treated cells, as expected. In keeping with our circadian luciferase reporter data, the abundance of endogenous clock transcripts and proteins oscillated with a lower amplitude and magnitude under α-amanitin treatment. We noted, however, that reduced transcription affected the amplitude of Bmal1 and Rev-erbα mRNA accumulation cycles somewhat less than that of Per1, Per2 and Dbp accumulation cycles. Hence, the transcription control mechanisms of some clock genes might be somewhat more sensitive to this insult than those of others. Interestingly, a correlation between reduced amplitude and an increased sensitivity to phase-shifting stimuli was recently observed in primary fibroblasts from a large number of human subjects (Brown et al, 2008).
We also examined the effect of 5,6-dichloro-1-fl-D-ribobenzimidazole (DRB) on circadian gene expression. This drug inhibits transcription by preventing RPB1 phosphorylation and thereby the escape of Pol II from promoters (Dubois et al, 1994). In contrast to α-amanitin and actinomycin D, DRB actually lengthened the period by 3–3.5 h (data not shown). However, DRB is also a potent inhibitor of casein kinase 1δ/ɛ (CK1δ/ɛ) activity (Smith, 2002; Kim et al, 2008), and phosphorylation of circadian clock proteins by CK1δ/ɛ has a crucial but complex function in period length determination (Eide and Virshup, 2001; Lin et al, 2002). Although a mutation comprising PER2 phosphorylation and a hypomorphic mutation in CK1ɛ resulted in period shortening (Lowrey et al, 2000; Toh et al, 2001; Xu et al, 2005; Vanselow et al, 2006), the treatment of Rat-1 fibroblasts with the CKIδ/ɛ-selective inhibitor IC261 caused a period lengthening of circadian gene expression (Eide et al, 2005). Thus, we cannot formally exclude the possibility that the effects of actinomycin D or α-amanitin on period length is caused by protein stability changes or other, yet unknown post-translational mechanisms rather than by a general transcription reduction.
The notion that period length is determined by both transcription and post-translation regulatory mechanisms also emerged from studies on other systems. Kondo and coworkers demonstrated that in cyanobacteria circadian protein phosphorylation can persist in the absence of transcription and translation (Tomita et al, 2005) at some temperatures and even succeeded in reconstituting a circadian oscillator in vitro with only three clock proteins (KaiA, KaiB and KaiC) and ATP (Nakajima et al, 2005). However, the same group recently showed that in vivo circadian clock gene transcription is required for a fully operative clock, and that period length is determined by an interplay between KaiC phosphorylation and cyclic gene expression (Kitayama et al, 2008). Period length determination in the Drosophila circadian clock—which shares many components with the mammalian oscillator—also depends on an intricate cross-talk between transcription and post-translation events. Thus, loss of function in DBT, the fruit fly homologue of CK1δ/ɛ, can either shorten or lengthen the period, depending on the precise location of the mutation (Muskus et al, 2007). Moreover, when the transcription transactivation potential of the CLK–CYC heterodimer is increased by fusing the strong acidic activation domain of the Herpes virus protein VP16 to CYC, the circadian period length considerably shortens (Kadener et al, 2008). However, So and Rosbash (1997) also reported on the importance of post-transcriptional regulation in shaping the temporal per mRNA accumulation curve. Conceivably, at reduced overall transcription rates this mechanism controlling circadian mRNA stability over-rides the effect of transcription strength. This mechanism is actually operative in flies carrying a gene lacking the normal promoter (transgene 7.2) instead of the wild-type per allele. In these flies, per transcription from spurious promoters is constitutively low, and cyclic mRNA accumulation is driven by post-transcriptional mechanisms. As circadian cell culture systems are not yet available for the fruit fly, the impact of lowering overall transcription rates on circadian gene expression could not yet be examined in this species.
PER1 is involved in both temperature and transcription compensation
In keeping with recently published reports (Izumo et al, 2003; Tsuchiya et al, 2003), our data demonstrate that circadian clocks of NIH3T3 mouse fibroblasts and primary mouse tail fibroblasts are compensated—or rather overcompensated—for temperature. In Drosophila, the Per protein has a key function in temperature compensation, and perL mutant flies loose temperature compensation and exhibit longer periods at higher temperature (Konopka et al, 1989). Our results suggest that Per proteins also have an important function in the temperature control of circadian oscillators in mammalian cells. Thus, Per1KO primary mouse tail fibroblasts are not temperature-(over)compensated, and in contrast to their wild-type counterparts oscillate with similar or even slightly shorter periods at higher temperatures. Interestingly, the effects of reduced Pol II transcription rates and decreased temperature on period length shortening were not additive. Likewise, Per1KO fibroblasts, normally oscillating with a 20-h period, did not exhibit further period shortening upon reduced transcription. These results would be compatible with a model surmising that the same molecular mechanisms underlie transcription and temperature compensation, and that PER1 has a function in these mechanisms. It was suggested for Drosophila that temperature-sensitive PER protein homodimerization, phosphorylation, protein degradation or alternative splicing of pre-mRNAs might account for temperature compensation (Hong and Tyson, 1997; Leloup and Goldbeter, 1997). Moreover, the role of PER in temperature compensation seems to be tightly linked to CRY proper function (Kaushik et al, 2007). Similar mechanisms might be responsible for temperature compensation in mammals, and we are planning to address Per1 phosphorylation patterns and Per–CRY complex formation at different temperatures.
Unexpectedly, weak oscillation amplitudes in Per1KO mouse fibroblasts could be rendered more robust by an actinomycin D treatment, suggesting the need of an optimal balance between the levels of different clock components for circadian oscillator function. A similar conclusion has been reached in another study examining the cooperation between PER and CRY proteins (Oster et al, 2002). Unexpectedly, circadian rhythmicity and normal clock gene expression patterns were restored in Per2 mutant mice by the inactivation of Cry2 (but not Cry1).
The impact of global transcription rates on period length in mathematical models
Global changes in transcription and translation rates arise in the body from variations in nutrition, growth condition or temperature. The ability of circadian clocks to keep running accurately despite significant variation in transcription rates appears necessary for the oscillator to maintain synchrony under different physiological conditions. The influence of fluctuations on period length and period dispersion in simple and complex models for the mammalian clock emphasized the role of post-translational regulation on oscillator stability (Rougemont and Naef, 2007). Here, we showed how low-dimensional models for prototypical nonlinear oscillators based on delayed negative feedback or relaxation oscillators tolerate a large range in transcription rates for which self-sustained oscillations are maintained, similar to what we observed experimentally. Although both models show regimens in which the period is rather insensitive to transcription rates (Barkai and Leibler, 2000), their global period dependence on transcription shows opposite signs, with Goodwin-type models being in qualitative agreement with our experiments. The more detailed mammalian models studied here were only partially consistent with our data, suggesting that the complexity of mammalian circadian clockworks is not yet fully captured by commonly invoked models. Future analysis will clarify the generality of our conclusions. Taken together, our data are consistent with the scenario that both the elimination of Per1 and the reduction of general transcription destabilize the limit cycles by bringing the system closer to the bifurcation boundaries. At the population level, low circadian amplitudes were observed in both cases, and additional single-cell analysis will thus further clarify the underlying mechanisms.
Materials and methods
RNA synthesis measurement by uridine pulse assay
Uridine pulse assay was performed as described by Balajee et al (1997). Briefly, NIH3T3 cells were pre-labeled with [14C]thymidine, treated for 16 h with 0–5 μg/ml of α-amanitin and pulse-labeled with [3H]uridine for 60 min at the indicated time points. Radioactivity incorporated into TCA-precipitated fraction was measured by scintillation counting. Transcription rates were calculated as the ratio of [3H]uridine incorporation per unit time divided by [14C]thymidine incorporation into each sample, corresponding to DNA content. Relative [3H]uridine incorporation corresponds to the ratio of values obtained for untreated and drug-treated cells.
In vitro transcription run-on assay
Run-on transcription rates were determined in isolated nuclei under conditions favouring Pol II-dependent transcription (Gariglio et al, 1981; Schmidt and Schibler, 1995). In vitro transcription rates were calculated as [32P]UTP incorporation per minute per 106 cells. Relative incorporation corresponds to the ratio of values obtained for untreated and drug-treated cells.
RNA analysis by real-time quantitative PCR
Cells from triplicate plates were collected every 4 h by trypsinization, rinsed with PBS, divided into two halves from each plate and frozen at −70°C. Total RNA was prepared from half of each plate using Trizol reagent and used as a substrate for cDNA synthesis. Genomic DNA was prepared from the other half of each plate using the NucleoSpin Tissue kit (Macherey–Nagel). RNA and genomic DNA quantification by TaqMan real-time PCR was performed as described by Heid et al (1996). Briefly, 1 μg of total RNA was reverse-transcribed using M-MLV Reverse Transcriptase (Invitrogen) and random hexamers. The resulting cDNA and genomic DNA were PCR-amplified in an ABI PRISM 7700 Sequence Detection System from PE-Applied Biosystems. Primers and probes are listed in Supplementary Table 1.
Western blot experiments
Western blot experiments with whole-cell extracts were performed with antibodies against RPB1 and U2AF65 (loading control).
Cell lines and constructs
NIH3T3 Bmal1-luc cells are described by Nagoshi et al (2004). Mouse primary skin fibroblasts were prepared from mPer1−/− mPer2∷luciferase or from mPer2∷luciferase tail tips by standard procedure and grown in DMEM with 20% FCS. Where indicated, cells were immortalized by transfection with Large T Antigen SV40 (pBABE-puro SV40LT; Addgene; plasmid number 13970) and selected over several weeks.
Real-time bioluminescence monitoring
Cells were stimulated with either 50% horse serum or 100 nM dexamethasone as described (Nagoshi et al, 2004). Cultures were maintained at 37°C in a light–tight incubator and bioluminescence was monitored continuously using Hamamatsu photomultiplier tube detector assemblies. Photon counts were integrated over 1-min intervals.
Bioluminescence time-lapse microscopy and data analysis
NIH3T3 Bmal1-luc cells were plated in 35-mm glass bottom dishes (WillCo-dish, type 3522; WillCo Wells BV). After treating the cells with dexamethasone during 15 min, the medium was replaced by 2 ml phenol red-free DMEM supplemented with 10% FCS and 1 mM luciferin. Bioluminescence imaging was performed on an Olympus LV 200 bioluminescence workstation equipped with a × 20 UPLSAPO objective (NA 0.75). Bioluminescence emission was detected for several consecutive days using an EM CCD camera (Image EM C9100-13; Hamamatsu, Japan) cooled to −90°C using exposure times of 30 min. The image series were analysed using the ImageJ 1.32 software (National Institutes of Health, Bethesda, MD, USA; as described in Supplementary data).
Supplementary Material
Acknowledgments
We thank Juergen Ripperger and Urs Albrecht for mPer1 knockout mice; Hans Reinke, Gad Asher, David Gatfield and Steven Brown for critical comments; Emi Nagoshi for cell lines, Jerome Bosset for microscopy help, Andre Liani for having constructed the temperature regulated lumicycler, and Nicolas Roggli for the artwork. This research was supported by the Swiss National Foundation (through individual research grants to US, FN, DS and MU), the National Center of Competence in Research Program Frontiers in Genetics, the University of Geneva, the Ecole Polytechnique Fédérale de Lausanne (EPFL), the Louis Jeantet Foundation of Medicine (US), the Bonizzi-Theler Stiftung (US), the 6th European Framework Project EUCLOCK (US), the Hasler Foundation (DS and MU), the Gebert-Rüf Foundation (DS and MU). CD received a postdoctoral fellowship from the Roche Research Foundation.
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