From the Department of Biochemistry, Dartmouth Medical School, Hanover, New Hampshire 03755-3844
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ABSTRACT |
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Circadian clocks function to govern a wide range of rhythmic activities in organisms. An integral part of rhythmicity is the daily control of target genes by the clock. Here we describe the sequence and analysis of a novel clock-controlled gene, ccg-7, showing similarity to glyceraldehyde-3-phosphate dehydrogenase (GAPDH), a glycolytic enzyme widely used as a constitutive control in a variety of systems. That ccg-7 encodes GAPDH was confirmed by demonstrating that in vitro synthesized CCG-7 possesses GAPDH activity. Rhythms in both ccg-7 mRNA accumulation and CCG-7 (GAPDH) activity are observed in a clock wild-type strain where the peak in GAPDH activity lags several hours behind the peak in ccg-7 mRNA accumulation in the late night. Together with our previous observation that ccg-7 mRNA is not developmentally regulated, we show that ccg-7 is not induced by environmental stresses such as glucose or nitrogen deprivation (which also trigger development), heat shock, or osmotic stress. Thus, the finding that GAPDH is clock-regulated points to a specific role for the circadian clock in controlling aspects of general metabolism and provides evidence for circadian regulation of a gene found in most living organisms.
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INTRODUCTION |
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Circadian rhythms are daily rhythms that are generated and controlled by endogenous, self-sustaining, temperature-compensated biological clocks that can be reset by environmental cues (reviewed in Ref. 1). These rhythms are observed in a wide variety of organisms ranging from bacteria to mammals and are coordinated with exogenous environmental cycles to limit activities at particular times of the day. One important aspect of rhythmicity involves control of specific target genes within an output pathway on a daily basis by the circadian clock. The Neurospora circadian clock controls the timing of asexual spore (conidium) development, where conidiation is initiated once every 22 h in wild-type strains grown under constant environmental conditions. The oscillator regulating this timed behavior is a negative autoregulatory feedback loop that directs rhythmic expression of the essential clock gene, frq (frequency) (2). In addition, frq mRNA and FRQ protein have been shown to be responsive to environmental signals, providing a molecular explanation for how the clock can be reset (3, 4). This general understanding of the Neurospora crassa clock system provides an ideal background for the analysis of clock output pathways.
Analysis of clock output pathways in many organisms has focused on three general questions: what is the extent of clock regulation of gene expression, what functions do the ccg (clock-controlled gene) genes have in the cell, and how are the ccg genes regulated? To begin to address these questions in Neurospora, two clock-regulated genes were isolated using subtractive hybridization (5, 6), and six more genes were later identified using differential screening (7). Because the levels of all previously isolated N. crassa ccg genes peak in the late night to early morning corresponding to the time of day at which conidiation takes place (5-7), it has been widely assumed that the ccg genes are directly and uniquely associated with this asexual developmental pathway. This clock-regulated developmental association was viewed to be distinct from that imagined for "housekeeping genes" whose expression was expected to be relatively time-invariant; this expectation of time-invariant expression underlies the use of genes such as GAPDH1 as loading or normalization controls. Given this, it was of particular interest in the analyses of a recent set of novel ccg genes (7) to find three ccg genes that are neither light- nor developmentally regulated. This suggested that the circadian clock could be regulating cellular metabolism at a much more basic level than had been anticipated.
Here we show this to be the case. One of the clock-controlled genes, ccg-7, encodes N. crassa GAPDH, the first energy-harvesting enzyme in the glycolytic pathway and the homolog of an mRNA often used as a "constitutively expressed control" in different tissues and cell types. Although we find circadian regulation to be apparent at the level of both mRNA and enzyme activities, ccg-7 mRNA levels are refractory to changes in many common environmental stimuli, reinforcing the unique importance of this circadian influence. Through GAPDH regulation, the circadian clock may be controlling the glycolytic pathway and thereby influencing the organism's fundamental metabolic activities. ccg-7 is a clock-regulated gene encoding a product participating in basic metabolism, a function found in most living organisms. The regulation and identity of ccg-7 suggest that circadian influences may be more pervasive at the cellular level than previously anticipated.
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EXPERIMENTAL PROCEDURES |
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Strains, Plasmids, and Culture Conditions--
All experiments
described in this report were carried out using strain bd; A
(30-7, laboratory stock). Growth conditions and media of
Neurospora cultures were as described (8). The plasmid pCCG7
includes ccg-7 cDNA in pBluescript SK(+) (Stratagene)
and was isolated from differential screening of morning
versus evening ZapII cDNA libraries (7). A
4.5-kilobase PstI fragment and a 3.0-kilobase
BamHI-XhoI fragment from ccg-7 genomic
DNA were subcloned into pBluescript SK(+), resulting in plasmids
pMLS701 and pMLS702, respectively. The plasmid pKL119 (9) containing ccg-1 genomic DNA was used as a positive control for glucose
deprivation (10) and for osmotic
stress.2 As positive
controls for the nitrogen deprivation experiments (11) and heat-shock
experiments, eas (ccg-2; in the plasmid pLW1
(12)) and hsp30 (13) cDNA were used, respectively. The bacterial strain XL1-Blue (Stratagene) was used for all plasmid manipulations.
Genomic Library Screening, Sequencing, and Computer
Analyses--
A ccg-7 genomic clone, G5:7H, was isolated
from the Orbach/Sachs genomic cosmid library (pMOcosX, Fungal Genetics
Stock Center) by colony hybridization (17) using a ccg-7
cDNA probe radiolabeled with [-32P]dCTP (6000 Ci/mmol; DuPont). Two subclones, pMLS701 and pMLS702, were constructed
from the cosmid clone. Automated sequencing of both strands of
ccg-7 cDNA and genomic DNA was accomplished using the
Applied Biosystems Prism Dye deoxy sequencing kit using nested oligodeoxynucleotide primers. DNA and putative amino acid sequences were compared with other known genes and peptides using the BLAST search from the GenBankTM/EMBL non-redundant data
base.3 The program CLUSTALW
(18) was used to align amino acid sequences. Quantitation of Northern
and Western blots was performed on scanned images (Silverscanner III,
LaCie) by densitometry using the NIH Image 1.60 program (19), and
linearity of density was confirmed by loading different amounts.
Preparation, Detection, and Assays of mRNA and Protein-- mRNA extraction was carried out as described previously (2). Primer extension analysis was carried out according to the method described by Ehrenman et al. (20) using an end-labeled primer, 7-NR4 (TGACCTTCTTGCCGTTGAC, corresponding to nucleotides 886-904 downstream from the transcription initiation site; see Fig. 1). Protein extraction and detection of FRQ by Western blot analysis were accomplished as described (15).
CCG-7 in Vitro Expression and Activity Assays of GAPDH, Alkaline Phosphatase, and UDG-- The ccg-7 gene (from pCCG7) and the cmt (ccg-12; copper metallothionein (7)) gene (from pCCG12) were expressed in vitro using rabbit reticulocyte lysates (TNTTM coupled reticulocyte lysate systems, Promega) as recommended by the supplier. GAPDH and alkaline phosphatase enzymatic assays were carried out using total Neurospora protein extracts used for the FRQ Western analysis. GAPDH activity was measured as described by Hochberg and Sargent (21). Alkaline phosphatase activity was assayed using the Sigma diagnostics alkaline phosphatase reagent as recommended by the supplier. One unit of GAPDH and alkaline phosphatase activities was calculated by determining the increase of NADH concentration in a reaction mixture at 340 nm (22) and of p-nitrophenol concentration at 405 nm, respectively. UDG activity was assayed as described by Meyer-Siegler et al. (23). Lysates containing in vitro synthesized CCG-7 or CCG-12 protein were used directly in the UDG reaction mixture as described by Slupphaug et al. (24). The amounts of [3H]dUTP released from a tritiated DNA substrate were measured as UDG activity.
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RESULTS |
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ccg-7 Encodes Neurospora GAPDH--
ccg-7 was
sequenced, and its conceptual amino acid sequence was found to have a
high degree of similarity to GAPDH peptides from diverse organisms
(Figs. 1 and
2. Based on RNA hybridization, cDNA
size, and primer extension analysis, ccg-7 encodes a single processed transcript of 1226 nucleotides (excluding the poly(A) tail)
that contains a short 5-untranslated region (43 nucleotides) followed
by a single open reading frame of 338 codons. Two introns of 567 and 76 nucleotides are processed out of the primary transcript, the former
being unusually large for N. crassa genes (25). The presence
and position of the shorter intron within the coding region are
conserved among GAPDH genes from some filamentous ascomycetes (26-31).
(While this paper was in revision, the same sequence appeared in a
clone identified during work in the Neurospora am gene and was identified as encoding GAPDH (32).) However, the longer intron
within the 5
-untranslated region was not found in previously identified GAPDH genes from other fungal species. The 3
-untranslated region contains a putative polyadenylation signal (AATAAT,
nucleotides +1828 to +1833) followed by a poly(A) tail positioned after
the last nucleotide at +1866 (Fig. 1).
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Steady-state Levels of ccg-7 mRNA and GAPDH Activity Vary Systematically over Time-- When analyzed under constant environmental conditions in the dark, ccg-7 mRNA levels showed a rhythm peaking in the late night (CT 18-0) (Fig. 3, A and B). The period length of the ccg-7 mRNA abundance rhythm changed appropriately with the strain examined, 22 h in the clock wild-type frq+ strain and 29 h in the long-period clock mutant frq7 (7) (Fig. 3B). The characteristics of stable rhythmicity with a period length reflecting the genotype of the strain (frq+ versus frq7) and of the constant phase (peak always in the subjective night) indicate that rhythmic expression of the ccg-7 gene is indeed controlled by the circadian oscillator. Amplitude of mRNA levels was often observed to be varied among different clock phenotypes. Although rhythmicity in ccg-7 transcript abundance is apparent, if CCG-7 protein had a long half-life under these conditions, rhythms in enzyme activity might not be evident. We first attempted to detect CCG-7 using antibodies directed against rabbit muscle GAPDH and against Trypanosoma glyoxosomal GAPDH, but CCG-7 was not detected by either. Therefore, to test the metabolic significance of the rhythm in ccg-7 mRNA, rhythmicity of GAPDH activity was assayed as a function of time (Fig. 3C). An ~1.5-fold rhythm in GAPDH activity was observed, with peak activity occurring in the early morning (CT 4-6) under conditions of constant darkness in liquid culture and in the absence of observable development. In control experiments using the same protein extracts, the clock component protein FRQ showed the characteristic rhythms in abundance and time-of-day-specific phosphorylation (Fig. 3A) (15), confirming a robust and functional clock in these cultures. On the other hand, alkaline phosphatase activity stayed constant (Fig. 3C), as previously suggested (21). As protein extracts were obtained from replicate samples from the same cultures used to isolate RNA samples, these data indicate that a 4-8-h time lag occurs between the peaks of ccg-7 mRNA and GAPDH enzyme activity levels. The data indicate a stable and consistent time-of-day-specific regulation of GAPDH activity that persists in the absence of environmental changes or overt developmental progression.
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ccg-7 mRNA Levels Are Refractory to Changes in Most Environmental Factors-- Circadian clocks are generally understood as being evolutionarily adaptive by virtue of the eligibility they confer on the organism to anticipate regularly observed changes in the environment. Thus, to understand better what role the observed GAPDH rhythm might play in the life of Neurospora, we examined the response of ccg-7 to acute environmental stimuli and agents of stress (Fig. 4) found to affect the expression of some other ccg genes (7). All samples were harvested at the same circadian time corresponding to approximately halfway between trough and peak of ccg-7 mRNA levels. Although positive control genes (hsp30 and ccg-1) respond in a typically robust manner to these stimuli (13),2 ccg-7 mRNA levels clearly showed no increase under heat shock or osmotic stress, and occasionally, heat shock resulted in a small but real decrease in expression levels (Fig. 4, A and B).
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In Vitro Expressed CCG-7 Shows GAPDH Activity, but Not Detectable UDG Activity-- GAPDH activities were compared among in vitro expression reaction mixtures containing the protein products of either ccg-7 or, as controls, cmt (ccg-12) or lysate only. The translation mixture to which ccg-7 was added had significant GAPDH activity compared with controls (Fig. 5A), confirming that ccg-7 encodes N. crassa GAPDH. Another possible role for the ccg-7 rhythm is suggested by the finding that a human GAPDH peptide, UDG/GAPDH, can function in DNA repair as UDG (23). This possibility is supported by the striking similarity between CCG-7 and human UDG/GAPDH (65.0%) (Fig. 2). Therefore, the same translation mixture was examined for UDG activity; however, reactions containing CCG-7 released amounts of [3H]dUTP equivalent to the negative controls (either lysate without expressed protein or lysate with CCG-12) (Fig. 5B). If the Neurospora GAPDH possessed UDG activity and the same ratio of GAPDH to UDG applied as in the human enzyme, then based on the amount of GAPDH activity seen in the translation mixture, we would have expected to observe UDG activity corresponding to a signal ~32-fold above background levels. Instead, our results indicate that CCG-7 has no significant UDG activity; this suggests that the ccg-7 gene functions exclusively or predominantly as the Neurospora GAPDH, as distinct from human UDG/GAPDH.
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DISCUSSION |
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Both sequence and functional analyses show that the clock-controlled gene ccg-7 encodes GAPDH, a key enzyme in glycolysis. Although numerous ccg genes have been linked to organism-specific behaviors such as photosynthesis (34), aspects of development (7, 14), or animal reproduction (35, 36), this study provides an example of a clock-regulated gene that participates in an aspect of fundamental metabolism that is common to most living organisms. Circadian rhythmicity is observed both for ccg-7 mRNA levels (peaking around the night, CT 18-0) and for GAPDH activity levels (peaking around the early morning, CT 4-6) under constant conditions in the dark. This time-of-day-specific variation in GAPDH enzyme expression is made more interesting by the fact that GAPDH mRNA and proteins are often used as "constitutive" controls in a variety of studies. Our data indicate a 4-8-fold amplitude in the ccg-7 mRNA rhythm and a low amplitude rhythm in GAPDH activity, consistent with the presence of additional post-transcriptional and/or post-translational factors affecting expression of enzyme activity. A rhythm in GAPDH activity (albeit with a different peak time) was suggested by one previous study (21) in cultures grown on solid media, where circadian development (conidiation) occurs. Although the presence of clock-controlled development in the study made it appear likely that the rhythm was reflecting the rhythm in development and mass accumulation, our data show that levels of GAPDH mRNA and enzyme activity are influenced by a circadian clock. Thus, ccg-7 appears not to be regulated by development (7); and the gene is also not induced by environmental factors such as heat shock, osmotic stress, or carbon/nitrogen starvation. Indeed, we found ccg-7 mRNA levels in general to be refractory to change except for the observed modulation by the biological clock.
Clock regulation of GAPDH is particularly interesting in view of the emerging numbers of reports regarding non-glycolytic roles for the GAPDH polypeptides. These include DNA repair (23, 37, 38); DNA, mRNA, and protein binding (39-41); a possible role in RNA export (42); translational control (43); protein kinase activity (44); interactions with microtubules (45); and interactions with cell membranes (46). While these activities were reported mainly in mammalian GAPDH, such roles for the GAPDH protein in lower eukaryotes cannot be ruled out a priori considering the high degree of sequence conservation of GAPDH among these organisms. Of these, we examined this possibility only with UDG activity, which was not detected in CCG-7. However, it may be that the Neurospora enzyme also shows one or more of the other activities and that this is the primary reason for its rhythmic activity.
Our rhythmic ccg-7 mRNA data, together with other data on GAPDH expression, may raise questions about the use of GAPDH as a normalization control. For example, GAPDH mRNA of another filamentous fungus, Aspergillus, is osmotically induced,4 although this is not the case with ccg-7. In other systems, mRNA levels of GAPDH genes are responsive to pathogenic or cytotoxic agents; for instance, in potato, GAPDH mRNA levels are known to be induced by Phytophthora infection (causing potato blight) (47). In cultured human keratinocytes, tetrachlorodibenzo-p-dioxin, known to elicit pleiotropic toxic actions, induces mRNA levels of GAPDH (48). Other reports on mammalian GAPDHs also suggest that they are not constitutively expressed (49-52). Since GAPDH plays an important role in glycolysis and a number of non-glycolytic roles in some cases as described above, changes in GAPDH activity could influence many other cellular activities and thereby facilitate adaptation to different challenges or growth conditions.
Finally, another recent report of clock-regulated GAPDH from the dinoflagellate Gonyaulax polyedra suggests that our observation here is not an isolated phenomenon and that there might be some significance in clock-regulated GAPDH. Interestingly, as distinct from ccg-7, levels of Gonyaulax GAPDH mRNA do not show rhythmicity, but protein levels do (53), indicating post-transcriptional clock regulation. It may be possible that clocks influence the very core of glycolysis to regulate some aspects of general metabolism in a circadian fashion, although the exact role for the rhythm of GAPDH is still uncertain. If GAPDH oscillations exist to influence cellular activities, it may be that other enzymes in fundamental metabolic pathways are also clock-regulated in a manner coordinated with this GAPDH rhythmicity so as to enhance time-of-day-specific modulation of metabolism.
A number of clock-regulated genes and proteins have been identified (5-7, 34-36, 53). However, there has been a great deal of diversity seen among clock output systems reflecting different organism-specific requirements, so that no clock-controlled gene identified to date, except ccg-7, had the potential to be ubiquitous. The high degree of GAPDH sequence conservation indicates that all modern GAPDH variants arose from a single ancestral enzyme (54). Perhaps in addition to sharing a common ancestor, modern GAPDHs share the common aspect of regulation by an internal timekeeper.
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ACKNOWLEDGEMENTS |
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We thank J. W. Hastings for communication of results prior to publication. We also thank J. A. Kinsey and T. Fagan for sharing results and Western detection using Trypanosoma GAPDH antibody, respectively. We give special thanks to D. Bell-Pedersen for critical comments and for the ccg-7 frq7 densitometry, S. Crosthwaite for sharing protein samples, and members of our laboratories for useful discussions.
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FOOTNOTES |
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* This work was supported by National Institute of Mental Health Grants MH44651 (to J. C D. and J. J. L.) and MH01186 (to J. C. D.), Air Force Office of Scientific Research Grant F49620-94-1-0260 (to J. J. L.), National Science Foundation Grant MCB 9307299 (to J. J. L.), and a core grant from the Norris Cotton Cancer Center.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
The nucleotide sequence(s) reported in this paper has been submitted to the GenBankTM/EMBL Data Bank with accession number(s) U67457.
To whom correspondence should be addressed. Tel.: 603-650-1108;
Fax: 603-650-1128; E-mail: jay.c.dunlap{at}dartmouth.edu.
1 The abbreviations used are: GAPDH, glyceraldehyde-3-phosphate dehydrogenase; CT, circadian time; UDG, uracil-DNA glycosylase.
2 K. Lindgren, N. Garceau, and J. J. Loros, manuscript in preparation.
3 This can be accessed through the NCBI Web Server (http://www.ncbi.nlm.nih.gov/cgi-bin/BLAST).
4 N. K. Singh, personal communication.
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REFERENCES |
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