(Received for publication, August 27, 1996, and in revised form, October 24, 1996)
From the Department of Medicine, Division of Endocrinology and Metabolism, Dartmouth Medical School, Lebanon, New Hampshire 03756
"Spot 14" protein appears rapidly in nuclei of hepatocytes exposed to glucose and thyroid hormone. Exposure of glucose- and T3-treated hepatocytes to a spot 14 antisense oligonucleotide inhibited induction of mRNAs encoding malic enzyme, ATP citrate-lyase, fatty acid synthase, liver-type pyruvate kinase, phosphoenolpyruvate carboxykinase, and type I deiodinase but not hydroxymethylglutaryl-CoA reductase, cytochrome c, and actin mRNAs. Induction of spot 14, ATP citrate-lyase, and fatty acid synthase polypeptides, but not propionyl-CoA carboxylase and mitochondrial pyruvate carboxylase, was inhibited. Antisense treatment of hepatocytes transfected with a reporter controlled by a glucose- and T3-inducible fragment of the pyruvate kinase gene promoter inhibited reporter activity, as did cotransfection of the reporter and a spot 14 antisense plasmid. Spot 14 protein acts in the induction of mRNAs coding for key lipogenic (malic enzyme, ATP citrate-lyase, fatty acid synthase), glycolytic (pyruvate kinase), and gluconeogenic enzymes (phosphoenolpyruvate carboxykinase), as well as the diet-responsive type I deiodinase, but not those involved in mitochondrial respiration (cytochrome c) or cholesterol synthesis (hydroxymethylglutaryl-CoA reductase). Transfection experiments indicated that these effects are mediated at the transcriptional level. The protein functions in the activation of genes involved in metabolic switching between the fasted and fed states in liver.
Liver, adipose, and lactating mammary tissues synthesize fatty acids for use as fuel. In those tissues lipogenesis is regulated by availability of dietary substrates and circulating hormones that control fuel metabolism. Regulated expression of genes that encode lipogenic enzymes is a major mechanism underlying this response. Spot 14 gene expression has been associated with such tissue-specific control. Spot 14 mRNA is abundant only in lipogenic tissues (1, 2), and its expression changes rapidly in response to stimuli that modulate fatty acid formation, including intake of dietary carbohydrate and polyunsaturated fat and levels of thyroid hormone and glucagon (3-9). Spot 14 protein levels paralleled those of its mRNA (10), and immunohistochemical analysis indicated that it was nuclear in location (11) with a zonal distribution in liver identical to that of the lipogenic enzymes (12).
Multifaceted regulation and nuclear localization of the spot 14 protein and its nuclear location suggested that it could function to control lipogenesis. We recently examined that hypothesis by determining the metabolic effects of antisense-mediated inhibition of spot 14 protein expression in cultured rat hepatocytes (13). Induction of lipid synthesis by glucose and triiodothyronine (T3)1 was inhibited in cells treated with a spot 14 antisense oligonucleotide, and Western analysis indicated that this resulted from diminished accumulation of lipogenic enzymes, including fatty acid synthase and ATP citrate-lyase. Activity of malic enzyme was also reduced, as was expression of malic enzyme mRNA.
We have now addressed the mechanism underlying reduced lipogenesis in hepatocytes treated with the antisense oligonucleotide. Our findings indicate that spot 14 protein participates in the tissue-specific induction of mRNAs encoding several lipogenic enzymes and of other inducible mRNAs involved in metabolic adaptation. Transfection studies further indicated that it functioned to promote pyruvate kinase gene transcription.
Collagenase perfusion of livers from male Sprague-Dawley rats (Charles River, Cambridge, MA) weighing approximately 150 g and maintained on a 12-h photoperiod (lights on at 0700 h) with ad libitum access to normal chow (Ralston Purina, St. Louis, MO) was as described previously (13, 14). Cells were plated in positively charged plastic dishes (143 × 103 cells/cm2) in serum-free modified William's E medium containing penicillin, streptomycin, 5.5 mM glucose, and no linoleic acid (Life Technologies, Inc.).
Hepatocyte TreatmentsCells were placed in modified
William's E medium without antibiotics 5 h after plating. Some
media contained 8 µg/ml Lipofectin (Life Technologies, Inc.) and 4 µM phosphorothioate oligonucleotides (Oligos Etc,
Wilsonville, OR). Oligonucleotides employed were S14
(GCGTTTCGTTAGCACTTGC; an antisense sequence in which the 3 residue
corresponds to the G of the translational start codon of the rat spot
14 mRNA sequence) and PPI (GAAGCGCATCCACAGGGCC; an antisense
sequence in which the 3
residue corresponds to the G of the start
codon of the rat preproinsulin I mRNA, which is not expressed in
liver). Neither oligonucleotide displayed sequence similarity to any
other mRNA studied. Media were replaced the following morning and
again 24 h later with either modified William's E medium alone or
fortified with 27.5 mM glucose and 50 nM
T3, and oligonucleotides (2 µM, without
Lipofectin); cells were harvested 24 h later. We showed previously
that the spot 14 antisense oligonucleotide specifically inhibited the
induction of triglyceride synthesis under these circumstances and that
the effect is dependent upon both the oligonucleotide sequence and the
presence of the intended target mRNA (13).
Sequential introduction of reporter
plasmids and oligonucleotides was required because simultaneous
application interfered with plasmid transfection. Following 5 h in
plating medium, plasmids (3.0 µg each of a plasmid containing base
pairs 4316 to +12 of the rat liver-type pyruvate kinase promoter
fused to the chloramphenicol acetyltransferase gene
(PK4316-CAT (15), kindly provided by H. Towle, University
of Minnesota) and a plasmid containing the firefly luciferase gene
fused to the Rous sarcoma virus promoter (RSV-LUC)) were introduced by
lipofection (Lipofectin). Media were removed 4 h later and
replaced with media containing oligonucleotides as described above. CAT
activity was quantitated in a liquid scintillation counter. Luciferase
activity was determined in a BioOrbit 1251 luminometer (Pharmacia
Biotech Inc.). In another experiment, a BglII-BamHI fragment containing a modified
full-length rat spot 14 cDNA (11) was ligated in the antisense
orientation into the BglII site of the pCMV4 vector (kindly
supplied by D. Russell, University of Southwestern Texas) and
cotransfected with the PK4316-CAT reporter (1.5 µg of
each/plate) and RSV-LUC (3.0 µg/plate) to allow correction for
transfection efficiency.
Proteins and total RNA were
extracted with Trizol reagent (Life Technologies, Inc.) and were
concentrated in Centricon-3 columns (Amicon, Beverly, MA) for Western
analysis. Affinity-purified rabbit anti-glutathione
S-transferase-spot 14 fusion protein IgG was employed as
reported previously (11). Detection of rat ATP citrate-lyase and fatty
acid synthase was as described (12). Pyruvate carboxylase and
propionyl-CoA carboxylase enzymes were visualized via their biotin
prosthetic groups with a streptavidin-alkaline phosphatase conjugate
(12). Integrity of total RNA was assured by Northern analysis using a
rat actin probe (16) (kindly supplied by B. Paterson, NIH) prior to
slot-blot analysis (data not shown). Total RNA (5 µg/slot) was
immobilized on nylon membranes, covalently bound by a Stratolinker
(Stratagene, La Jolla CA), and prehybridized and hybridized at 42 °C
as described previously (8). Washing was at 55 °C in 0.1 × standard saline citrate for 15 min × 3. The following
[-32-P]dCTP-labeled (Amersham) rat cDNA probes
(labeled by the random hexamers technique (Life Technologies, Inc.),
3 × 106 cpm/ml) were used: malic enzyme (17), fatty
acid synthase (18), ATP citrate-lyase (19) (kindly supplied by L. Witters, Dartmouth Medical School), deiodinase type I (20) (kindly
supplied by D. St. Germain, Dartmouth Medical School), pyruvate kinase
(15) (kindly supplied by H. Towle, University of Minnesota),
phosphoenolpyruvate carboxykinase (21), and cytochrome c
(22) (kindly supplied by R. Scarpulla, Northwestern University Medical
School). A hamster cDNA for hydroxymethylglutaryl-coenzyme A
reductase was obtained from ATCC. Signals were quantitated on a
PhosphorImager 445 SI (Signal Analytics, Vienna VA) using IP Lab Gel
software (Signal Analytics). Radioactivity was removed in 0.1 × standard saline citrate, 0.1% sodium dodecyl sulfate at 95 °C for
10 min × 2, and blots were reprobed with the actin cDNA to
correct for the amount of immobilized mRNA.
Differences between means were assessed by analysis of variance (23).
Western blot verified that the treatments resulted in the expected
changes in expression of spot 14 protein and three lipogenic enzymes,
whereas levels of two other specific enzymes were unaltered (Fig.
1). Maintenance of hepatocytes in 5.5 mM
glucose and no T3 for 72 h resulted in nearly
undetectable levels of spot 14 protein (panel a, lanes
1 and 2), whereas exposure to 27.5 mM glucose and 50 nM T3 for 48 h (lanes
3 and 4) induced expression to a level comparable to
that observed in liver from a hyperthyroid, carbohydrate-fed rat
(lane 7). In contrast to the effect of the control
oligonucleotide (PPI, lane 6), treatment with the spot 14 antisense oligonucleotide markedly inhibited induction of the protein
(AS, lane 5).
Western analysis of the same protein preparations using antibodies directed against fatty acid synthase (panel b) or ATP citrate-lyase (panel c) confirmed our previous report of the effect of the treatments (13). High glucose and T3 concentrations caused a marked induction of both enzymes, and this was inhibited by transfection of the spot 14, but not the preproinsulin I, oligonucleotide.
In contrast to fatty acid synthase and ATP citrate-lyase, levels of mitochondrial pyruvate carboxylase and propionyl-CoA carboxylase were not induced by glucose and T3 and also were not lowered in antisense-treated cells (panel d). We were unable to detect acetyl-CoA carboxylase in the extracts.
To determine whether reduced expression of lipogenic enzymes in spot 14 antisense-treated cells resulted from lowered levels of their
mRNAs, we undertook slot-blot analysis of mRNA extracted from
the same hepatocytes used for Western analyses (Fig. 2). Each signal was corrected for that observed upon reanalysis with an
actin cDNA probe. The mean level of malic enzyme mRNA increased 7-fold after exposure to high glucose and T3
concentrations. The spot 14 antisense oligomer caused a 43% reduction
(p < 0.05) in the accumulation of this mRNA. ATP
citrate-lyase and fatty acid synthase mRNAs were induced
approximately 14- and 6-fold, respectively. Transfection of the
antisense oligonucleotide caused a 60 and 56% reduction in the
expression of these respective mRNAs (p < 0.05).
The 8-fold induction of pyruvate kinase mRNA was inhibited by 36%
(p < 0.05) Phosphoenolpyruvate carboxykinase mRNA
exhibited a small (1.7-fold, p < 0.05) induction that
was inhibited by antisense treatment. Hydroxymethylglutaryl-CoA
reductase mRNA was not induced by glucose and T3, nor
was its expression affected by the antisense oligonucleotide.
Cytochrome c mRNA exhibited a small (32%) but statistically significant (p < 0.05) induction that
was not differentially affected by the olgonucleotides. The 11-fold
increase in type I 5-deiodinase mRNA was reduced by 54% in
antisense-transfected cells.
Promoter activity of a construct containing nucleotides 4316 to +12
of the rat liver-type pyruvate kinase gene fused to the chloramphenicol
acetyltransferase gene (PK4316-CAT) (15) was assessed to
determine the cause of the antisense effect on mRNA levels. We
employed two different approaches to this question. In the first,
PK4316-CAT-transfected cells were treated with antisense oligonucleotides (Fig. 3). Mean CAT activity, corrected
for the activity of a cotransfected luciferase reporter (RSV-LUC), in cells maintained in 5.5 mM glucose without T3
or any oligonucleotide, was indistinguishable from the background level
in untransfected cells. Transfected hepatocytes treated with the
control oligonucleotide exhibited a significant (p < 0.05) induction of CAT activity in response to 27.5 mM
glucose plus 50 nM T3, whereas induced cells treated with the antisense oligonucleotide expressed 76% less CAT
activity (p < 0.05). In another experiment we
cotransfected a construct containing a full-length spot 14 cDNA in
the antisense orientation with respect to the cytomegalovirus promoter
(S14-anti) or the nonrecombinant vector (CMV4)
with PK4316-CAT and RSV-LUC (Fig. 4). The
antisense plasmid caused a 60% reduction in the activity of the
pyruvate kinase promoter compared with that observed in the control
group (p < 0.05).
We showed previously that induction of long chain fatty acid synthesis and of two major lipogenic enzymes, fatty acid synthase and ATP citrate-lyase, was impaired in hepatocytes treated with the antisense oligonucleotide (13). Levels of malic enzyme activity were also reduced, in conjunction with lowered relative expression of malic enzyme mRNA. These findings were confirmed in the present study. In concert with our previous immunohistochemical demonstration of nuclear localization of spot 14 protein (11), this prompted the proposal that spot 14 could function in the transduction of glucose- and T3-initiated signals for increased lipogenesis at the pretranslational level. The major finding in the current experiments was that the reduced expression of fatty acid synthase and ATP citrate-lyase polypeptides was accompanied by diminished expression of their respective mRNAs.
Expression of three mRNAs encoding inducible enzymes not directly involved in lipogenesis, pyruvate kinase, phosphoenolpyruvate carboxykinase, and type I deiodinase, was also inhibited by antisense treatment. Hepatic pyruvate kinase and type I deiodinase mRNAs are known to increase during refeeding in vivo, as is the case for the lipogenic enzymes, whereas phosphoenolpyruvate carboxykinase mRNA declines in that circumstance. Pyruvate kinase induction is mediated at the transcriptional level by a signal initiated by glucose metabolism (15). The signal is transduced via a major late transcription-like factor, hepatic nuclear factor-4 (24), and an accessory factor acting in cis with a CACGTG motif (25). We speculate that spot 14 protein could be involved, directly or indirectly, in modulating the interaction of one or more of these factors with the pyruvate kinase promoter.
In contrast to pyruvate kinase, phosphoenolpyruvate carboxykinase gene transcription is induced by glucagon-mediated increases in cAMP, T3, and glucocorticoids (26-28) and inhibited by insulin (29) in vivo. Our hepatocytes were cultured without glucagon or cAMP analogs with constant glucocorticoid (10 nM dexamethasone) and insulin (0.01 unit/ml) concentrations. The culture conditions therefore do not reproduce the reduced cellular cAMP and rising insulin levels associated with refeeding in vivo. This provides an explanation for the apparent paradox of simultaneous induction of pyruvate kinase and phosphoenolpyruvate carboxykinase in T3- and glucose-treated cells. The observed 1.7-fold induction in phosphoenolpyruvate carboxykinase mRNA may be attributed to T3, and this effect was abrogated by antisense treatment. In view of the effect on antisense treatment on pyruvate kinase mRNA expression, it appears that spot 14 protein plays a role in both T3- and glucose-mediated signaling pathways, although we did not address this issue in the current experiments.
The mechanism underlying the regulation of the deiodinase is less well characterized, although it occurs at the pretranslational level. Deiodinase mRNA in liver declines during fasting, experimental diabetes mellitus, and hypothyroidism and is induced by T3 treatment (30). Our data show that T3 and glucose act to stimulate deiodinase expression directly at the hepatocellular level and that spot 14 protein functions in this response.
T3 administration causes accumulation of some, but not all, mitochondrial polypeptides in liver. The observation that cytochrome c mRNA was induced, whereas pyruvate carboxylase polypeptide was not, is consistent with previous reports of uncoordinate regulation by T3 of mitochondrial components encoded in the nuclear genome (31). The lack of any effect of the spot 14 antisense oligonucleotide on either pyruvate carboxylase polypeptide or cytochrome c mRNA expression indicates that the protein does not participate in the regulation of mitochondrial function by carbohydrate or T3.
Because of considerations discussed in the Introduction, we focused previously on the fatty acid synthetic pathway as the locus of spot 14 protein function (13). Reduced expression of genes encoding enzymes involved in lipogenesis, glycolysis, and T3 production in antisense-treated hepatocytes in the current studies suggests a broader role for the protein in metabolic adaptation. At least in the case of pyruvate kinase, the protein functions at the level of transcription. Immunohistochemical studies from our laboratory showed that the induction of both spot 14 protein and lipogenic enzymes by T3 in rat liver is limited to the perivenous zone of the hepatic lobule (12), whereas others have demonstrated uniform distribution of hepatic nuclear T3 receptors (32). The current findings prompt the hypothesis that spot 14 could serve as a tissue- or zone-specific adaptor between generic transcription factors and their potential target genes.