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The Journal of Neuroscience, October 15, 2000, 20(20):7525-7530
Light and Glutamate-Induced Degradation of the Circadian Oscillating Protein BMAL1 during the Mammalian Clock Resetting
Teruya Tamaru1, Yasushi Isojima2, Takashi Yamada1, Masato Okada2, Katsuya Nagai2, and Ken Takamatsu1 1 Department of Physiology, Toho University School of Medicine, Tokyo 143-8540, Japan and 2 Division of Protein Metabolism, Institute for Protein Research, Osaka University, Osaka 565-0871, Japan
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Recently discovered mammalian clock genes are believed to compose the core oscillator, which generates the circadian rhythm. BMAL1/CLOCK heterodimer is the essential positive element that drives clock-related transcription and self-sustaining oscillation by a negative feedback mechanism. We examined BMAL1 protein expression in the rat suprachiasmatic nuclei (SCN) by immunoblot analysis. Anti-BMAL1 antiserum raised against rBMAL1 recognized 70 kDa mBMAL1b and detected a similar immunoreactivity (IR) as a major band in rat brains. Robust circadian BMAL1-IR oscillations with nocturnal peaks were detected in the SCN during a light/dark cycle and under constant darkness. A short duration light exposure at night acutely reduced BMAL1-IR in the SCN during photoentrainment. This might be attributable to the degradation of BMAL1 protein. Application of glutamate and NMDA to the SCN slices at projected night, a procedure mimicking photic phase delay shift, also acutely reduced BMAL1-IR in a similar manner. A rapid decrease of BMAL1 protein suggests that BMAL1 protein might be implicated in the light-transducing pathway within the SCN.
Key words: circadian clock; light; phase shift; glutamate; NMDA; suprachiasmatic nucleus
INTRODUCTION
Circadian clocks controlling various biological timings are widely observed in eukaryotes and some prokaryotes. Recent progress has revealed an important part of the mechanism, a set of mammalian circadian clock genes localized within the site of the master circadian pacemaker in the hypothalamic SCN (Dunlap, 1999
).
The molecular core of the circadian clock is thought to be the feedback loop with positive and negative limbs. The mouse Clock gene was first demonstrated to be an essential component of the mammalian circadian clock (Vitaterna et al., 1994
The negative limb in the circadian loop is believed to be composed of PER1, PER2, PER3, TIM, CRY1, and CRY2. These molecules, except TIM, show stronger circadian oscillation than that of Clock/BMAL1 (Albrecht et al., 1997
Light is the most powerful external stimulus for connecting and entraining the circadian clock to the environment. In rodents, even a single brief exposure to light in the early (subjective) night causes a phase delay shift, whereas a light pulse during late (subjective) night induces a phase advance shift. The c-Fos gene was first to be identified as one of the immediate responsive genes to light in the SCN (Rea, 1989
The function of BMAL1 in the photoentrainment and maintaining of the circadian clock is not clear. To understand further how the putative BMAL1 functions in the circadian clock cells, we have generated a specific antiserum against rBMAL1 and used it for the immunoblot analysis of the temporal regulation related to the clock mechanism. In this report, we discuss photic downregulation of BMAL1 protein during the resetting of the circadian clock.
MATERIALS AND METHODS
Animals. Male Wistar rats (Nippon Bio-Supply Center, Tokyo, Japan) aged 5-7 weeks were maintained at 25°C on a 12 hr light/dark (LD) cycle [light: zeitgeber time (ZT) 0-12; dark: ZT12-24] for at least 10 d before use. The animals were then transferred to a dim light (<1 lux) condition, and their circadian locomotor activities were monitored using the far-infrared monitor system (Supermex System, Muromachi-Kikai, Tokyo, Japan). The experiments under constant darkness (DD) conditions were performed 2-3 d after the transition. For the light pulse experiment, rats were exposed to white light (1000 lux) for 30 min, then they were killed at the experimental time point. As controls, we analyzed the locomotor activities of a number of rats under the same sampling conditions and confirmed that the phase shifts occurred only by light exposure at subjective night.
Materials. A glutathione-Sepharose, HiTrap column and pGEX-5X vector DNA were purchased from Amersham Pharmacia Biotech (Tokyo, Japan). Escherichia coli strain JM109 and pBluescript SK+ were from Clontech (Tokyo, Japan). Affi-Gel10 was from Bio-Rad (Hercules, CA). Glutathione and complete protease inhibitor cocktail tablets were from Boehringer Mannheim (Tokyo, Japan). pGEM-T Easy vector DNA and TNT T7 Quick Coupled Transcription/Translation System were from Promega (Tokyo, Japan). Bovine serum albumin, glutamate, NMDA, and tetrodotoxin (TTX) were from Sigma-Aldrich (Tokyo, Japan). TiterMax Gold was from CytRx (Atlanta, GA). The BCA protein assay system was from Pierce (Rockford, IL). Immobilon P membranes were from Millipore (Bedford, MA). HISTOFINE Simple Stain PO (MULTI) system was Nichirei (Tokyo, Japan). Anti-actin antibody was from Chemicon (Temecula, CA). Anti-c-fos antibody was from Santa Cruz Biotechnology (Santa Cruz, CA). HIBERNATE A medium and B27 supplement were from Life Technologies (Tokyo, Japan). (R,S)-3,5-dihydroxyphenylglycine (DHPG) was from Tocris Cookson (Bristol, UK).
Preparation of recombinant BMAL1 proteins. A full-length of cDNA for mBMAL1b was amplified by PCR (94°C for 30 sec, 50°C for 1 min, 72°C for 2 min, 30 cycles), using mouse brain cDNA as a template. The PCR product was ligated into the plasmid pGEM-T Easy and analyzed. The construct was transformed into E. coli strain JM109. Recombinant mBMAL1b protein was produced from the construct by in vitro transcription and translation using the TNT T7 Quick Coupled Transcription/Translation System.
A fragment of cDNA for rBMAL1 (encoding amino acid 154-182; chosen as a region nonhomologous to rTIC, assumed to be a BMAL1 homolog or splice variant) was amplified by PCR (94°C for 30 sec, 52°C for 30 sec, 72°C for 1 min, 30 cycles), using rat brain cDNA as a template. The PCR product was ligated into the plasmid pBluescript SK+ and analyzed, and ligated into pGEX-5X1. The construct was transformed into E. coli strain JM109. Expression of glutathione S-transferase (GST)-rBMAL1 fragment fusion protein (GST-
BMAL1) was induced by a final concentration of 0.5 mM isopropyl-thiogalactoside for 12 hr at 25°C. The cells were harvested by centrifugation and disrupted by sonication in buffer A (in mM: 50 Tris-HCl, pH 8.0, 50 NaCl, 1 dithiothreitol, and 1 EGTA). After centrifugation at 10,000 × g for 20 min at 4°C, the supernatant was incubated with glutathione-Sepharose for 1 hr at 4°C. After extensive washing with buffer B (0.14 M NaCl, 3 mM KCl, 8 mM Na2HPO4, and 1.5 mM KH2PO4, pH 7.4, and 0.1% Tween 20), the bound proteins were eluted with buffer A containing 20 mM glutathione. The eluate was dialyzed against 1000-fold volume of 20 mM HEPES, pH 7.5, containing 25% glycerol, 0.01% NP-40, and 1 mM dithiothreitol for 6 hr at 4°C.
Preparation of the antiserum against rBMAL1. Primary immunizations were performed with purified GST-
Preparation of the tissue extracts. Animals were decapitated at each experimental time point. They were killed under dim light (<1 lux) during the DD cycle or the dark phase during the LD cycle. The brain was removed from the skull and quickly frozen in dry ice. As described previously, the SCN region was punched out with a 2-mm-diameter needle that was inserted to a 1 mm depth into the surface of the coronal plane, an area that included the SCN (Tamaru et al., 1999
Brains and tissues were removed from rats during the day phase and homogenized using 5 volume buffer C, as described above. Protein concentration was determined using a BCA protein assay system, with bovine serum albumin as a standard. Twenty micrograms of the extracts were subjected to immunoblot analysis.
Immunoblot analysis. The samples were separated on SDS-10% polyacrylamide gels and transferred onto Immobilon P membranes. After blocking with 5% skim milk in Tris-buffered saline with 0.1% Tween 20 (TTBS), membranes were incubated at 4°C for 16 hr with a 1:200 anti-BMAL1 antiserum dilution in TTBS containing 3% bovine serum albumin. After washing with TTBS, membranes were developed with a HISTOFINE Simple Stain PO (MULTI) system according to the manufacturer's protocol. Quantification of bands of interest was performed by densitometry in a computerized image analyzer system (AE-6920; ATTO, Tokyo, Japan). As shown in figure legends, the relative density of BMAL1-IR was normalized against actin-IR (1 = the bottom level in each experiment). Student's t test was used for the statistic analysis of the relative values.
Analysis using the rat SCN slices. Rats aged 4-5 weeks were killed at 9-10 hr after light onset (ZT9-10), and their brains were removed. A region containing SCN located immediately dorsal to optic chiasm was processed into two sections cut at 500 µm. SCN-containing sections were transferred to HIBERNATE A medium supplemented with B27 and placed in an incubator and slowly brought to a final temperature of 35°C. Experiments were performed in the continued presence of 1 µM TTX, which reportedly reversibly blocks electrophysiological output from the circadian clock, but does not affect the timing of the circadian clock itself (Shibata and Moore 1993
RESULTS
Characterization of anti-BMAL1-specific antibody
Polyclonal antibody was raised against recombinant GST-
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Figure 1. Characterization of anti-BMAL1 antiserum. A, Immunizing a rabbit with GST-
Circadian oscillation of BMAL1-IR content in the SCN
To investigate the roles of BMAL1 in the circadian clock, we examined the circadian profile of BMAL1-IR content in the rat SCN. By immunoblot analysis, robust circadian oscillation of BMAL1-IR content was observed in the SCN under both LD (Fig. 2A) and DD conditions (Fig. 3A). A 70 kDa major band and a slightly larger minor band were detected. Normalizing BMAL1-IR content against actin-IR content as a constitutively expressed internal control was performed as the exact quantitative analysis. Circadian BMAL1-IR profiles during LD and DD cycles exhibited evident oscillation with a nocturnal peak (Figs. 2B, 3B). The peak/trough ratios for both cycles were ~2:1.
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Figure 2. Circadian profile of BMAL1-IR in the rat SCN during the LD cycle. A, Male Wistar rats aged 5-8 weeks were maintained under a 12 hr light/dark regimen. Rats were killed at ZT2, 6, 10, 14, 18, or 22. The SCN extracts from five animals at each time point were combined and subjected to immunoblot analysis. B, The relative density of BMAL1-IR from the analysis for individual SCN was normalized against actin-IR and plotted (1 = the bottom level at ZT6). Each point represents the mean ± SEM. One-way ANOVA was used for statistical analysis. Statistical significance value: **p < 0.001.
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Figure 3. Circadian profile of BMAL1-IR in the rat SCN during the DD cycle. A, Male Wistar rats aged 5-8 weeks were maintained under a 12 hr light/dark regimen (light: ZT0-12; dark: ZT12-24), then transferred to dim light (<1 lux). Rats were killed at CT1, 5, 9, 13, 17, or 21. The SCN extracts from six animals at each time point were combined and subjected to immunoblot analysis. B, The relative density of BMAL1-IR was normalized against actin-IR and plotted (1 = the bottom level at CT5).
Light pulse-induced rapid reduction of BMAL1-IR in the SCN during the resetting of the clock
To investigate the roles of BMAL1 in the phase-shifting mechanism of the circadian clock by photic stimulus, we examined the profiles of BMAL1-IR in the rat SCN containing retinorecipient cells after light exposure of rats. Interestingly, a significant decrease in BMAL1-IR content in the SCN was observed within 30 min after 1000 lux light exposure delivered 2 hr after the onset of early night in the LD cycle (ZT14), a result known to cause behavioral phase delay shift (Fig. 4A). BMAL1-IR in the SCN also decreased after a 30 min 1000 lux light pulse delivered from ZT14, a stimulus sufficient to cause the phase shift (Fig. 4B). Without light illumination at ZT14, decrease of the basal level of BMAL1-IR was not observed from ZT14 to ZT18 (Fig. 2). A significant trough in BMAL1-IR content, 48-49% lower than basal level, was observed 1-2 hr after the exposure. BMAL1-IR content returned to near basal level 3 hr after the pulse began. A similar pattern of reduction in BMAL1-IR content was observed after a light pulse during subjective early night [circadian time 15 (CT15)] (data not shown). As positive controls, we detected an acute increase of c-fos protein after the stimulus (data not shown).
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Figure 4. Temporal profile of BMAL1-IR in the rat SCN after light exposure at early night. A, Rats (n = 4 for each lane) were exposed to 1000 lux light delivered from ZT14, then killed at the indicated time. The SCN extract (10 µg of protein) from the rat was subjected to immunoblot analysis probing with anti-BMAL1 antiserum. B, Rats (n = 4 for each lane) were exposed to a 30 min 1000 lux light pulse delivered from ZT14 to ZT14.5, then killed at the indicated time. The SCN extract from the rat was subjected to immunoblot analysis probing with anti-BMAL1 antiserum and anti-Actin antibody (a). The relative densities of BMAL1-IR in the immunoblot membranes were normalized against actin-IR and plotted (1 = the basal level at ZT14) (b).
Nocturnal-specific reduction of BMAL1-IR
Because the circadian clock is entrained by photic stimulus only during subjective night, we examined the phase dependency of the photic reduction of BMAL1-IR. A number of rats (n = 5 at each treatment) were exposed to 30 min, 1000 lux light pulses delivered at early subjective night (CT15), late subjective night (CT21), and mid subjective day (CT6) (Fig. 5A). We examined the samples at 2 hr after light exposure, because the level of BMAL1-IR became trough at that time (Fig. 4). SCN from individual rats killed 2 hr after exposure were all subjected to immunoblot analysis. A clear phase dependency was revealed in the photic reduction of BMAL1-IR. A light pulse at CT6 induced no significant change in BMAL1-IR. BMAL1-IR was significantly lower after exposure at CT15 (p < 0.001; 56% of basal level) and modestly lower after exposure at CT21 (p < 0.01; 74% of basal level).
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Figure 5. Phase-dependent effect of light exposure on BMAL1-IR in the rat SCN. A, Rats (n = 5 at each treatment) were exposed to 30 min 1000 lux light pulses delivered from CT15, CT21, and CT6 (L), then killed at the same time schedule (CT17). Control ( ) rats were kept in darkness, then killed at 2 hr after the exposure. The SCN extracts from the rats were subjected to immunoblot analyses. The relative density of BMAL1-IR was normalized against actin-IR and plotted (1 = the basal level of control). Each column represents the mean ± SEM. Two-tailed Student's t test was used for statistical analysis. Statistical significance value: **p < 0.001; *p < 0.01. B, The SCN extracts from five animals at each time point were combined and subjected to immunoblot analysis. The figure represents the typical pattern for the phase-dependent effect of light exposure on BMAL1-IR in the SCN.
Glutamate and NMDA-induced rapid BMAL1-IR reduction in the SCN slices
To explore the mechanism of photic reduction of BMAL1-IR in the SCN, we performed in vitro pharmacological experiments on the rat SCN slices. Glutamate is believed to be a major neurotransmitter which transduces retinal photic information to the SCN via retinohypothalamic projection. Application of glutamate to the SCN can mimic the photic phase shift (Ding et al., 1994
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Figure 6. Effects of glutamate receptor agonists on BMAL1-IR in the rat SCN slices. Rats (n = 4 at each treatment) aged 4 weeks were killed at ZT9 to ZT10. At projected ZT14, slices were treated with glutamate (A; 0-300 µM) or NMDA (A; 0-300 µM) for 40 min. Slices were also treated with glutamate (B; 100 µM), NMDA (C; 100 µM) or without (B, C;
The precise temporal patterns of BMAL1-IR were analyzed after the application of glutamate receptor agonists. Similar to the photic reduction, rapid BMAL1-IR reduction in the SCN slices began within 10 min after the application of glutamate and continued to decrease for at least 1 hr (Fig. 6B). Evident reduction of BMAL1-IR also was observed even 2 hr after the application of glutamate (data not shown). Acute c-fos protein induction was clearly detected after the application of glutamate, confirming the effect of glutamate on the SCN slices under our experimental conditions (data not shown). Treatment with NMDA also promptly reduced BMAL1-IR in the SCN nuclear fraction, in a pattern similar to the glutamate application (Fig. 6C). In addition to ionotropic NMDA receptors, metabotropic glutamate receptor subtypes are also clearly detected in the SCN (Gannon and Rea, 1994
DISCUSSION
Using anti-BMAL1 antiserum raised against GST-
The specificity of anti-BMAL1 antiserum is discussed from several aspects. As reported, in mice, three splice variants, mBMAL1b (mArnt3), mBMAL1b', and mBMAL1g' encode 626, 636, and 222 amino acids, whose predicted molecular weights are 68.6, 69.4, and 25 kDa, respectively (Yu et al., 1999
It is surprising that BMAL1-IR remarkably decreased promptly after a nocturnal light pulse. It has been reported that BMAL1 transcript does not change for up to ~1 hr after light pulse (Abe et al., 1998
We cannot exclude the possibility that other components of the system influence light response. Acute induction of Per1 and Per2 transcripts in the SCN by photic stimulation is assumed to be mediated by transactivation of BMAL1/CLOCK heterodimer on their E-box elements or another unknown activating pathway downstream of hypothetical LRE. Induced Per1 and Per2 transcripts peak after 1-1.5 hr of light onset, then rapidly decrease (Albrecht et al., 1997
The biochemical mechanism responsible for light-induced BMAL1 reduction (presumably degradation) is largely elusive. Glutamate is considered a major neurotransmitter mediating photoentrainment into the SCN (Ding et al., 1994
FOOTNOTES Received April 24, 2000; revised July 20, 2000; accepted July 26, 2000.
This work was supported by a Grant-in-Aid for Scientific Research from Uehara Memorial Foundation (T.T.), a Grant-in-Aid for Scientific Research from Nissan Science Foundation (T.T.), the Project Research Grant 10-20 of Toho University School of Medicine (T.T.), and the Scientific Research Promotion Fund from the Japan Private School Promotion Foundation (T.K.).
Correspondence should be addressed to Teruya Tamaru, Department of Physiology, Toho University School of Medicine, 5-21-16 Ohmori-nishi Ohta-ku, Tokyo 143-8540, Japan. E-mail: tetamaru{at}med.toho-u.ac.jp.
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