(Received for publication, August 6, 1996, and in revised form, October 4, 1996)
From the Unitat de Bioquímica, Departament de
Ciències Fisiològiques Humanes i de la Nutriciò,
Universitat de Barcelona, Avinguda Diagonal 643, Barcelona 08028, Catalunya, Spain and the Department of
Biochemistry, University of Minnesota, Minneapolis, Minnesota
55455-0347
The activation of glycolytic flux is a biochemical characteristic of growing cells. Several reports have demonstrated the role of fructose 2,6-bisphosphate in this process. In this paper we show that the levels of 6-phosphofructo-2-kinase/fructose-2,6-bisphosphatase (6PF2K/Fru-2,6-P2ase) mRNA are modulated in response to serum and growth factors and this effect is due to regulation of its transcription rate. The modulation of the expression of this enzyme by growth factors differs according their mitogenic effect; both lysophosphatidic acid and epidermal growth factor, when added alone, increased the mRNA levels, but endothelin had no effect. Furthermore, cAMP, which acts as an antimitogenic signal in Rat-1 fibroblasts, produced a decrease in 6PF2K/Fru-2,6-P2ase mRNA and inhibited the effects of lysophosphatidic acid and epidermal growth factor on 6PF2K/Fru-2,6-P2ase expression. PD 098059, a specific inhibitor of the activation of the mitogen-activated protein kinase, was able to prevent the effect of EGF on 6PF2K/Fru-2,6-P2ase gene expression. These results imply that activation of mitogen-activated protein kinase is required for the stimulation of the transcription of 6PF2K/Fru-2,6-P2ase by EGF.
Quiescent cells can be stimulated to recommence DNA synthesis by distinct and interactive signal transduction pathways. These signaling pathways trigger a cascade of molecular events required for progression of DNA replication (1, 2). One of the essential processes for this progression is the activation of the glycolytic flux (3, 4). It is known that glycolysis is stimulated both when growth promoting agents are added to quiescent cells and in many types of transformed cells (5-7). The major regulatory step in the glycolytic pathway is 6-phosphofructo-1-kinase activity. Activation of glycolysis involves the increase of fructose 2,6-bisphosphate (Fru-2,6-P2)1 levels, a potent allosteric stimulator of 6-phosphofructo-1-kinase (reviewed in Refs. 8 and 9). Fru-2,6-P2 content is regulated by the bifunctional enzyme 6-phosphofructo-2-kinase/fructose-2,6-bisphosphatase (6PF2K/Fru-2,6-P2ase; EC 2.7.1.105/3.1.3.46), which catalyzes both its synthesis and its degradation (8, 9). Different 6PF2K/Fru-2,6-P2ase isoenzymes have been described depending on the tissues and cell specificity. In rat, the liver, the muscle, and the F-type isoforms are encoded by the same gene arising from distinct promoters (10, 11). These isoenzymes differ with respect to their N-terminal sequence, regulation by phosphorylation, and kinetic properties. It has been shown that the F-type is the isoform expressed in several proliferative tissues and in serum-stimulated Rat-1 fibroblasts (10). Although extensive studies have been performed on the regulation of liver and muscle isoforms, this is not the case of F-type.
Different reports have demonstrated that Fru-2,6-P2 levels increase after stimulation of fibroblasts with fetal bovine serum, insulin, epidermal growth factor (EGF), or tumor promoter phorbol esters (12-21). In some cases, the increase in this metabolite has been correlated with an increase in the Vmax of 6-phosphofructo-2-kinase activity (19-24). Although this metabolic effect is clear, the mechanism by which it is achieved is not known. Recently, a study of the regulation of Fru-2,6-P2 metabolism through different signal transduction pathways has been performed using murine Swiss 3T3 fibroblasts as a model (21). However, the attempts to measure regulation of 6PF2K/Fru-2,6-P2ase mRNA levels and transcription rate were not successful because the cDNA probes available did not recognize Swiss 3T3 6PF2K/Fru-2,6-P2ase mRNA.
The aim of this work is to study the signaling pathways that control the transcription of the 6PF2K/Fru-2,6-P2ase gene during cell proliferation. For this propose, we have investigated the effect of EGF, lysophosphatidic acid (LPA), endothelin, and cholera toxin (CTx) on 6PF2K/Fru-2,6-P2ase gene expression in Rat-1 fibroblasts and the role of mitogen-activated kinase (MAPK) in this regulation.
[-32P]dCTP (3000 Ci/mmol),
[
-32P]UTP (3000 Ci/mmol),
[6-3H]thymidine (5 Ci/mmol), ECL Western kit, and
Hybond-N membranes were from Amersham International (Amersham, Bucks.,
United Kingdom (UK)). The random-primer DNA-labeling kit was from
Boehringer Mannheim. Fetal calf serum, minimum essential medium, and
penicillin/streptomycin were from Bio-Whittaker. EGF, LPA, insulin, and
endothelin-1 were from Sigma. Anti-phosphotyrosine
monoclonal antibody PY20 was from Affiniti Research Products Ltd.
(Nottingham, UK), and anti-MAPK monoclonal antibody was from Zymed
Laboratories, Inc. (San Francisco, CA). PD 098059 was a gift from Dr.
A. Saltiel, Parke-Davis Pharmaceutical Division (Detroit, MI). Other
materials and chemicals were of the highest quality available.
Rat-1 fibroblasts were routinely grown in minimum essential medium (MEM) supplemented with 10% (v/v) fetal calf serum (FCS), 100 units of penicillin/ml, and 100 µg of streptomycin/ml at 37 °C in a 5% CO2 atmosphere. For experimental purposes, cells were subcultured in six-well plates or 100-mm dishes and their quiescence was induced by maintaining the cells in serum-free medium during 24 h. After this, cells were stimulated with either FCS or different growth factors.
Measurement of DNA SynthesisQuiescent Rat-1 cells were activated with 10% FCS and different growth factors. At the indicated times, cells were exposed to [6-3H]thymidine (0.5 µCi/ml) for the last 1 h of stimulation. Trichloroacetic acid-precipitable material was dissolved in 0.1 M NaOH and quantified by liquid scintillation counting.
Fructose 2,6-Bisphosphate DeterminationTo measure Fru-2,6-P2 levels, Rat-1 cells were homogenized in 0.1 M NaOH, heated at 80 °C for 15 min, and centrifuged at 12,000 × g for 5 min. Fru-2,6-P2 was determined in supernatants by its ability to activate pyrophosphate-dependent 6-phosphofructo-1-kinase from potato tubers as described by Van Schaftingen et al. (25).
Western Blot AnalysisImmunoblot analysis were performed essentially as described by Burnette (26). For 6PF2K/Fru-2,6-P2ase, we used a 1:1000 dilution of a polyclonal antibody raised against the rat liver protein (27). Western blot analysis of MAPK phosphorylation was performed as described previously (28) using anti-phosphotyrosine or anti-MAPK monoclonal antibodies. Bound antibodies were detected by enhanced chemiluminescence method. The amount of protein was determined by densitometric scanning of the autoradiograms.
RNA Isolation and AnalysisTotal RNA was extracted from Rat-1 cells by the LiCl/urea method (29). Northern blot analyses were carried out by standard procedures (30). To detect 6PF2K/Fru-2,6-P2ase mRNA, a 1.4-kilobase EcoRI fragment from pPKB plasmid was used as a probe (31). The integrity of the RNA was verified by observing the rRNA bands in the ethidium bromide gel under UV irradiation. The level of mRNA was evaluated by densitometric scanning of the autoradiograms and corrected for the amount of 18 S rRNA using a ribosomic cDNA probe (32).
Transfection and CAT AssaysStable transfections were
performed by the CaPO4 method as described by Sambrook
et al. (30). Rat-1 cells were plated at 106
cells/100-mm culture dish 24 h before transfection. The DNA
precipitate (50 µg of the HindIII/BspmI 5
flanking region of the F isoform of 6PF2K/Fru-2,6-P2ase
cloned into pBLCAT3 plasmid as described by Lange (11) and 5 µg of
pSV2Neo) were left overnight. After 24 h, the cells were
trypsinized and replated at 1:4 dilution. G418 (400 µg/ml) was added
24 h later. Transfections containing resistant colonies were
pooled for experimentation. CAT activity determinations were carried
out as described by Ausebel et al. (33).
Protein was determined as described by Bradford (34) with bovine serum albumin as a standard. Statistical significance of difference was assessed by Student's unpaired t test.
Confluent Rat-1 fibroblasts were made quiescent by maintaining them in serum-free medium for 24 h and then shifted to medium supplemented with 10% fetal-calf serum. After serum addition, the cells were harvested and samples were taken to be analyzed at different times. The data reported in Table I show that, after being exposed to serum, an increase of the intracellular Fru-2,6-P2 content was detected. During this process, the amount of 6PF2K/Fru-2,6-P2ase protein also increased. This was measured by immunobloting with an antibody obtained against the liver 6PF2K/Fru-2,6-P2ase (Fig. 1). To determine whether the abundance of 6PF2K/Fru-2,6-P2ase protein was correlated with the amount of 6PF2K/Fru-2,6-P2ase mRNA, Northern blot analysis was done using a 1.4-kilobase cDNA probe (31). As shown in Fig. 2, there was a transient increase in the level of 6PF2K/Fru-2,6-P2ase mRNA with a maximum at 12-15 h (5-fold increase over serum deprivation mRNA levels) and a gradual decline to serum-free mRNA levels by 30 h. The analysis of the incorporation of [6-3H]thymidine into DNA during the course of this experiment revealed that the peak in mRNA accumulation was coincident with the onset of DNA synthesis (Fig. 2).
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To determine whether the regulation of 6PF2K/Fru-2,6-P2ase
mRNA levels was due to a regulation of its transcription rate, Rat-1 fibroblasts were stable transfected with a CAT reporter gene
under transcriptional control of a 1.7-kilobase genomic DNA fragment
that contain the F-type promoter (11). In preliminary RNase protection
experiments, we observed that the F-type isoform is the only one
expressed in these cells. Quiescent transfected cells were stimulated
with 10% of serum, and CAT activity was measured at different times.
As shown in Fig. 3, up to 4-fold induction of CAT
activity was found at 4 and 8 h after addition of serum. In
contrast, CAT activity did not change in cells incubated in the absence
of serum during this period.
Effect of Growth Factors on 6PF2K/Fru-2,6-P2ase mRNA Levels
In order to study the signal transduction pathways that control the expression of 6PF2K/Fru-2,6-P2ase in Rat-1 fibroblasts during proliferation, we determined the effect of EGF, LPA, endothelin, and cholera toxin (CTx) on 6PF2K/Fru-2,6-P2ase mRNA levels. As shown in Table II, EGF at 10 ng/ml and LPA at 70 µM increased the levels of 6PF2K/Fru-2,6-P2ase mRNA 4- and 7-fold, respectively. No significant change in 6PF2K/Fru-2,6-P2ase mRNA levels was detected after endothelin addition. Furthermore, 12-O-tetradecanoylphorbol-13-acetate (TPA), an activator of protein kinase C (PKC) also failed to increase 6PF2K/Fru-2,6-P2ase mRNA. In contrast, CTx at 10 ng/ml decreased the 6PF2K/Fru-2,6-P2ase mRNA levels by approximately 50%. In agreement with the results from measurement of mRNA levels, addition of EGF and LPA to quiescent Rat-1 fibroblasts induced an increase in Fru-2,6-P2 levels. In contrast, TPA or endothelin did not modify the concentration of this metabolite (Table III).
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Both EGF and LPA induce the activation of the mitogen-activated protein
kinases ERK1 and ERK2 (MAPKs) through the Ras-Raf-MEK pathway (35, 36).
In Rat-1 fibroblasts, cAMP can inhibit the activation of MAPKs by
inhibiting Raf activation (37). To examine the correlation between MAPK
activation and the increase in 6PF2K/Fru-2,6-P2ase mRNA
found after mitogenic responses, quiescent Rat-1 cells were preincubated with CTx for 90 min before stimulation with EGF and the
6PF2K/Fru-2,6-P2ase mRNA levels were then measured. The
phosphorylation state of ERK2 is shown in Fig. 4. As we
expected, a phosphotyrosine protein that comigrated with ERK2 was
detected after EGF and serum addition, but it was almost undetectable
with TPA. Preincubation with CTx blocked the effect of EGF on ERK2
phosphorylation (panel B). Under these experimental
conditions, EGF produced a 4-fold increase on the levels of
6PF2K/Fru-2,6-P2ase mRNA and preincubation with CTx
completely inhibited this effect (panel C). The same results
were obtained with LPA (data not shown).
Recently, PD 098059 has been identified as a specific cell-permeant
inhibitor of MEK (38). To prove that MAPK activation is involved in
mediating the effect of EGF on 6PF2K/Fru-2,6-P2ase expression, we examined the effect of this compound on
6PF2K/Fru-2,6-P2ase mRNA levels. As shown in Fig.
5, PD 098059 is able to prevent the increase on
6PF2K/Fru-2,6-P2ase mRNA by EGF. The concentration of
inhibitor required to avoid this activation was similar to the one
reported to inhibit MAPK (38).
The ability of PD 098059 to inhibit the effect EGF on
6PF2K/Fru-2,6-P2ase mRNA levels was correlated with its
ability to prevent the activation of 6PF2K/Fru-2,6-P2ase
transcription. Cells stably transfected with a CAT reporter gene under
transcriptional control of 1.7-kilobase F-type promoter, were incubated
at different concentrations of PD 098059 and CAT activity was assayed
8 h after addition of EGF. As expected, PD 098059 suppressed the
increase of CAT activity induced by EGF and the activity remaining at
basal levels at high concentration of the inhibitor (Fig.
6).
Several reports have pointed out the essential role of Fru-2,6-P2 in the activation of glycolytic flux in growing cells (3, 4). The levels of this metabolite increase in different proliferative states (12-24, 39), and this change has been correlated with an increase in 6-phosphofructo-2-kinase activity (18-24) and recently with an increase in mRNA levels (40, 41). However, the mechanisms by which growth factors regulate 6PF2K/Fru-2,6-P2ase are still unclear. The results presented here demonstrate that MAPK is involved in the regulation of 6PF2K/Fru-2,6-P2ase gene transcription in response to mitogenic signals.
The modulation of the expression of 6PF2K/Fru-2,6-P2ase by growth factors is concomitant with their mitogenic response. Serum, LPA, and EGF, complete mitogens for Rat-1 fibroblasts (42), were able to increase the mRNA levels of 6PF2K/Fru-2,6-P2ase and Fru-2,6-P2 content. In contrast, endothelin, which has a low mitogenic activity (43), had no significant effect on the expression of this enzyme. Indeed, cAMP produced a decrease in 6PF2K/Fru-2,6-P2ase mRNA levels and inhibited the effect of LPA and EGF. In agreement with these results, Darville et al. (41) have demonstrated that cAMP was also able to block the effect of serum on 6PF2K/Fru-2,6-P2ase transcription. Previous studies reported a different effect of cAMP on Fru-2,6-P2 levels in fibroblasts. In Swiss 3T3 (21) and human fibroblasts (16), cAMP induces an increase in the concentration of Fru-2,6-P2, while in chick-embryo fibroblast (19), the presence of dibutyryl cAMP did not change the levels of this metabolite. It is very likely that the discrepancy between these results is due to the different mitogenic role of cAMP in these cells; cAMP is a mitogenic signal in Swiss 3T3 cells (44), but it is a strong antimitogen in Rat-1 fibroblasts (37).
With regard to the signaling pathways that control the transcription of
the 6PF2K/Fru-2,6-P2ase gene during cell proliferation, our
results suggest that agents or growth factors (LPA, EGF) that activate
the Ras-Raf-MEK-ERK pathway also increase the levels of
6PF2K/Fru-2,6-P2ase mRNA. In Rat-1 fibroblasts, EGF
promotes the activation of ERK1 and ERK2 proteins through a
Ras-dependent pathway without affecting inositol phosphate
levels (42, 45). In the same cells, LPA activates at least three
independent signaling cascades by coupling its receptor to
Gi and Gq proteins: stimulation of
phospholipases C and D via a pertussis toxin-insensitive G protein
(Gq), inhibition of adenylate cyclase via a pertussis toxin-sensitive G protein (Gi), and activation of Ras
via a pertussis toxin-sensitive Gi protein (G
) (46).
The activation of the Ras cascade by LPA produces the stimulation of
MAPK (36). In Rat-1 fibroblasts, Ras is a point of convergence of EGF
and LPA signaling pathways in the activation of MAPK. It has been shown that raising the cAMP levels in the cell induces the
hyperphosphorylation of Raf-1 by PKA, reducing the binding affinity of
Raf-1 to Ras and consequently inhibiting the Ras-Raf-MEK-ERK pathway
(47). Our results show that the inhibition of this pathway by cAMP also leads to an inhibition of the stimulatory effect of EGF and LPA on
6PF2K/Fru-2,6-P2ase expression. The effect of cAMP on
6PF2K/Fru-2,6-P2ase expression is probably due to
inhibition of MAPK activation. The implication of MAPK cascade on the
expression of this enzyme has been suggested previously (41). However,
definitive experiments were necessary to support this tentative
hypothesis. Our finding that a specific inhibitor of MEK can prevent
the effect of EGF on 6PF2K/Fru-2,6-P2ase mRNA levels
and on the transcriptional levels provides further evidence to confirm
the idea that MAPK is involved in regulating
6PF2K/Fru-2,6-P2ase expression during proliferative
processes.
Activation of PKC increases Fru-2,6-P2 levels in different cells (16-24). Although there is no direct evidence, several reports suggest that PKC may regulate 6PF2K/Fru-2,6-P2ase gene expression. In chick embryo fibroblasts, incubation with TPA produced an increase in 6PF2K/Fru-2,6-P2ase activity and this effect was abolished in cells incubated with actinomycin D, cycloheximide, or puromycin (19). In fetal hepatocytes (22) and Swiss 3T3 cells (21), the rise in 6PF2K/Fru-2,6-P2ase activity produced by phorbol esters was inhibited by cycloheximide, suggesting that it is due to enhanced expression of the protein. Our results demonstrate that, in Rat-1 fibroblasts, endothelin, a strong stimulator of PKC, and TPA, had no detectable effect on 6PF2K/Fru-2,6-P2ase mRNA levels and Fru-2,6-P2, suggesting that activation of PKC pathway alone is not enough to stimulate 6PF2K/Fru-2,6-P2ase expression in these cells. It has been reported that, in Rat-1 fibroblasts, endothelin fails to stimulate ERK phosphorylation, despite its potent coupling to the phospholipase C-PKC second messenger cascade (36). The different contribution of PKC to MAPK activation could explain the fact that, in Swiss 3T3 cells, bombesin, another phospholipase C-activating agonist, was able to increase 6PF2K/Fru-2,6-P2ase activity (21). In these cells, bombesin stimulates MAPK activity via a pathway that is almost entirely dependent on PKC (48).
Sequence analysis of the F promoter of 6PF2K/Fru-2,6-P2ase reveals the presence of several DNA-binding sites that could directly or indirectly regulate the transcription of the 6PF2K/Fru-2,6-P2ase gene by MAPK activation. A region containing three binding motifs for transcription factors of the ets oncogene family has been found in the F promoter (10). The transcriptional activity of various Ets-related transcription factors is regulated by MAPK. Thus, c-Ets-2 is both transcriptionally activated and phosphorylated by MAPK (49). Furthermore, phosphorylation of the Ets-related transcription factor p62TCF/Elk-1 by MAPK stimulates ternary complex formation at c-fos promoter, thus activating the fos transcription and consequently, the AP-1 DNA binding activity (50-52). Darville et al. (53) reported an AP-1 DNA-binding site about 250 bp downstream of the F promoter, and several reports show that an intronic AP-1 site could regulate gene expression (54-56). Indeed, in the same 6PF2K/Fru-2,6-P2ase gene, a potent glucocorticoid response element was identified in the first intron of liver transcript (11).
Recently, an E2F binding site localized at the 5 end of the first exon
has been suggested to be involved in the serum regulation of F promoter
(41). E2F transcriptional activity is blocked by its binding to
hypophosphorylated retinoblastoma protein (pRB). G1
cyclins, including cyclin D1, forms complexes with
cyclin-dependent kinases which can phosphorylate pRB,
causing to release E2F (57). Although there is no evidence, MAPK
pathway could regulate the dissociation of E2F from retinoblastoma
protein (pRB) leading to activation of E2F target genes. In this sense,
EGF induction of cyclin D1 transcription was antagonized by either
dominant negative MAPK or dominant negatives of Ets-2 activation,
suggesting that MAPK and Ets-2 function downstream of EGF in the
context of cyclin D1 induction (58). It would be very interesting to study whether this putative MAPK-Ets-cyclin D1-pRB-E2F pathway controls
6PF2K/Fru-2,6-P2ase expression.
We thank Dr. R. Bartrons for continued interest in this work. We also thank Dr. A. Saltiel at Parke-Davis for generously supplying PD 098059. We thank Dr. J. Hesketh for correcting the English of the manuscript.