C-Terminal Binding Protein (CtBP) Activates the Expression of E-Box Clock Genes with CLOCK/CYCLE in Drosophila

To screen new clock genes, we used the EP lines [18], which carries the Upstream Activation Sequence (UAS) insertion in the promoter region of a target gene. The EP lines were crossed with tim(UAS)-Gal4 as a driver [19]. Because tim is expressed in virtually all clock-related cells [20], a target gene downstream of UAS can be activated by GAL4 in these tissues. This allowed us to screen for gene candidates which contribute to the circadian system, regardless of the tissue specificity of the target gene expression. We found EP3352 strain carrying the UAS insertion in the promoter region of dCtBP altered circadian locomotor rhythm when it was crossed with tim(UAS)-Gal4. About 80% of tim(UAS)-Gal4;EP3352 flies became arrhythmic; the remaining flies demonstrated lengthening of the circadian period to over 26 h (Table 1). Because homozygous EP3352 flies were semi-lethal, the UAS insertion in the promoter region of dCtBP might affect the expression of the dCtBP gene. We newly established two lines of UAS-dCtBP transgenic flies, which enabled us to investigate the effect of dCtBP overexpression. tim(UAS)-Gal4/+; UAS-dCtBP-1/+ flies demonstrated a period length of approximately 25.5 h, significantly longer than those of the corresponding parental strains (t test, P<0.05). The other overexpression flies, tim(UAS)-Gal4/UAS-dCtBP-2, became totally arrhythmic (Figure 1 and Table 1). To further check the effect of dCtBP overexpression in limited clock cells, we used pdf-Gal4 in which GAL4 is expressed in a subset of pacemaker neurons [21]. Both pdf-Gal4/Y;+;UAS-dCtBP-1/+ and pdf-Gal4/Y;UAS-dCtBP-2/+ flies showed a significantly longer period than corresponding each parental strains (t test, P<0.05).

Neuron-specific knockdown of dCtBP also affected circadian locomotor rhythm, although the effect was relatively smaller than that of dCtBP overexpression (Table 1 and Figure 1). The periods of knockdown flies tested were slightly but significantly longer than the corresponding parental strains– (t test, P<0.05) regardless of the GAL4 driver. About 10% of flies demonstrated arrhythmicity in tim(UAS)-Gal4/+;dCtBP-IR1/+ flies.

The daily expression profile of dCtBP in the fly head was measured by quantitative PCR analyses (Q-PCR). The expression level of dCtBP in the driver line as a control showed rhythmicity with a low amplitude (Figure 2A). The statistical analysis with Tukey’s test reveals that it peaks at the end of night phase, which is close to that of Clk[22], [23] (Figure 2A). The expression level of dCtBP was also determined at ZT1 and ZT13 in the tim(UAS)-Gal4/UAS-dCtBP-2 flies, which showed arrhythmicity. The former corresponds to the trough phase of E-box clock genes expression, while the latter corresponds to the peak phase. The dCtBP expression level was 17-times higher than that of controls at both phases (Figure 2B).

Next, the expression levels of known clock genes were measured in this arrhythmic dCtBP overexpression flies at ZT1 and ZT13. In the case of Clk, whose expression is not controlled through an E-box [24], expression oscillated in antiphase to E-box clock genes. The levels of per, vri, and Pdp1ε increased at their peak phase, whereas that of cwo decreased at the trough phase (Figure 3). The expression level of tim showed no significant change at both phases (Figure 3).

Then in order to investigate whether the effect of dCtBP overexpression can be observed in output genes, we quantified the expression level of takeout (to) [25] whose expression shows circadian rhythm [26], [27]. We compared the expression level of to in three groups of flies, tim(UAS)-Gal4, UAS-dCtBP-2 and tim(UAS)-Gal4/UAS-dCtBP-2. dCtBP overexpression significantly increased to expression both at the peak and trough phases in tim(UAS)-Gal4/UAS-dCtBP-2 flies as compared to those in the parental lines (t test, P<0.05). It seemed that the expression of takeout (to) maintain rhythmicity even in the arrhythmic flies (Figure 4).

These results suggest that dCtBP overexpression affects clock-related gene expression. In general, dCtBP overexpression activates the expression of E-box clock genes at the peak phase although there are some exceptions as we observed in tim and cwo. Interestingly, circadian expression rhythm seemed to persist in all clock-related genes we tested, although dCtBP overexpression flies became arrhythmic at the behavioral level.

The luciferase assay in cultured Drosophila S2 cells was used to determine whether the gene-specific induction by dCtBP could be observed in vitro. First, we investigated whether dCtBP was able to regulate the E-box clock genes without CLK. S2 cells are reported not to express CLK [22]. Regulation by dCtBP was monitored by promoter-luc, in which firefly luciferase cDNA was linked to the promoter region including the E-box sequence of clock genes. None of those promoters were regulated by dCtBP without CLK (Figure 5). When we further co-transfected the plasmid to express CLK, per-luc, vri-luc, Pdp1-luc and cwo-luc were activated. This activation effect tended to correlate with the amount of dCtBP expression plasmid (Figure 5). However, we could not observe a significant increase of tim-luc under the expression of dCtBP with CLK (Figure 5). Thus, except for the case of cwo-luc, these results obtained in vitro are principally consistent with the results of dCtBP overexpression in vivo.

Next, in order to investigate whether these activations are regulated via the nicotinamide adenine dinucleotide domain (NAD⁺) -dependence of dCtBP, we supplied CLK with the mutated dCtBP which carries two amino acid substitutions in NAD⁺ binding region (dCtBP-G183A/G186A) [28]. The expression level of all E-box clock genes we tested with the mutated dCtBP was not significantly different from the value without an intact dCtBP.

tim(UAS)-Gal4 strain [19] was used as the driver to knock down and overexpress dCtBP. UAS-IR lines [33] were established at the National Institute of Genetics. Knockdown flies were obtained by mating females of the driver line to males in each of the UAS-IR lines. The EP3352 line [18] was obtained from the Harvard Stock Center. UAS-dCtBP transgenic lines were established by injection of UAS-dCtBP plasmid into w¹¹¹⁸ embryos (BestGene). dCtBP-overexpressing flies were obtained by mating the driver females to EP3352 males or UAS-dCtBP transgenic males.

Flies were kept on standard glucose-cornmeal medium under 12-h light:12-h dark cycles (LD) at 25°C. We measured the locomotor activity of the adult flies using Drosophila activity monitors (Trikinetics Inc.) for 3 days in LD cycles, then over 10 days in constant darkness (DD). A single fly was introduced into a measuring glass tube containing agar gel with 100 mg/ml glucose. The periods were calculated with a χ² periodogram [34] programmed using the Matlab R2007b software (MathWorks Inc.).

The tim(UAS)-Gal4 strain [19] was used as control. Control and dCtBP-overexpressing flies entrained for at least 3 days under LD were sampled three times at each point. Total RNA was isolated from 100 heads at each time point as described elsewhere [35]. cDNA was synthesized from 5 µg total RNA using Ready-To-Go T-Primed First-Strand Kit (Amersham) according to the standard protocol. Q-PCR was performed using Applied Biosystems 7300 and Power SYBR Green PCR Master Mix (Applied Biosystems). PCR reactions were performed with samples containing 1× Power SYBR Green PCR Master Mix (Applied Biosystems), 5 µM primers, and 1 µL synthesized cDNA in a 20 µL volume using the following amplification procedure: 10 min at 95°C, then 40 cycles of 15 s at 95°C, 30 s at 60°C, and 1 min at 72°C. Gapdh2 expression levels were quantified and used as the internal control. We purified total RNA at each time point. Each RNA was used as a template to synthesize cDNA. We repeated these steps and obtained three different cDNAs at each point. One time-series of cDNAs were analyzed by Q-PCR at once with the primer sets in Table S1. The data finally obtained were calculated with the 2^−ΔΔCt Method [36] using the following equation, ΔΔCt = (Ct target – Ct Gapdh2) _{ZT x} – (Ct target – Ct Gapdh2) _ZT1. We confirmed that all primer sets we used didn’t yield any non-specific amplification by a melting curve analysis using the products of Q-PCR.

The coding sequence of dCtBP (see http://flybase.org/reports/FBgn0020496.html↗) was cloned into a pAc5.1B-V5/His plasmid (Invitrogen) by the SA-cloning method [37] using the sets of primers in Table S2.

To construct the pAc5.1-dCtBP-G183A/G186A plasmid, mutagenesis of pAc5.1-dCtBP was performed by site-directed mutagenesis PCR method using PCR with primers 5′- CTGGTGGGACTGGCCCGCATTGCTAGCGCCGTGGCCCTG-3′ and 5′- CAGGGCCACGGCGCTAGCAATGCGGGCCAGTCCCACCAG-3′.

To construct the UAS-dCtBP plasmid for transgenic flies, dCtBP was amplified by PCR using head cDNA in w¹¹¹⁸ as a template with primers 5′-AGCGAAATGGACAAAAATCTG-3′ and 5′-CTACGGCGCCTCCGTTGACT-3′ and cloned into pCR2.1 vector (Invitrogen). To construct the UAS-dCtBP plasmid, the dCtBP PCR fragment in pCR2.1 was doubly digested by SpeI and XbaI (New England Biolabs), purified, and cloned into the XbaI site of the pUAST plasmid [38].

Cultured Drosophila S2 cells were plated in 24-well tissue culture plates with Shields and Sang M3 insect medium (Sigma-Aldrich) supplemented with 12.5% fetal bovine serum (Biowest) and antibiotics (12.5 U/mL penicillin, 12.5 mg/mL streptomycin; Invitrogen) and transfected by a standard method [22] using Effectene Transfection Reagent (QIAGEN) with 100 ng of each promoter-luc[39], [40] in the presence of 0 or 100 ng pAc5.1- dCtBP alone or 0, 100, or 400 ng pAc5.1- dCtBP in conjunction with 100 ng pAct-Clk. As a positive control for the luciferase assay, cells were transfected with 610 ng pAc5.1B empty vector (Invitrogen) with 10 ng pAc5.1-Rluc. Each Luciferase activity was measured 48 h after transfection as described elsewhere [39], [40]. The mean values were calculated from data obtained by three (or four in some cases) independent experiments.