Abstract
Metabolic remodeling is thought to be an important contributor towards the
development of various cardiac pathophysiologic conditions. Therefore, studies
attempting to delineate undenying mechanisms driving cardiac metabolic
remodeling represent an important initiative toward the development of novel
therapeutic interventions. To further investigate the role of metabolic substrate
switches in the heart, we focused on a pivotal, rate-limiting step of cardiac fatty
acid metabolism i.e. an upstream modulator of long-chain fatty acid importation
into the mitochondrion. In the heart, long-chain fatty acids are transported into
the mitochondrion by the rate-limiting enzyme, carnitine palmitoyl transferase 1
(CPT1). CPT1 is potently inhibited by malonyl-CoA, the product of the acetylCoA
carboxylation reaction that is catalyzed by acetyl-CoA carboxylase (ACC).
Recent studies have demonstrated that metabolic fuels such as fatty acids and
glucose can function as signaling ligands, directing transcriptional regulation of
numerous metabolic genes. However, transcriptional mechanisms directing the
gene expression of the cardiac isoform of acetyl-CoA carboxylase (ACC[3) are
less well understood. Previously, four E-box (CANNTG) sequence motifs were
identified on the human ACC[3 promoter. Since E-boxes act as binding sites for
upstream stimulatory factors (US F), putative glucose-responsive transcriptional
modulators, we hypothesized that ACC[3 is induced by USF1 in a glucosedependent
manner.
To investigate this, we began by acutely fasting and subsequently refeeding
Balb/C mice with a carbohydrate-enriched diet. Here, high carbohydrate feeding
resulted in elevated systemic glucose levels associated with increased cardiac
ACC[3 gene and protein expression. To further explore these interesting findings,
we tranSiently cotransfected neonatal card iom yocytes , H9C2 myoblasts, CV-1
fibroblasts and HepG2 hepatocytes with the full-length and deletion constructs of
the human ACC[3 gene promoter together with a putative activator and repressor expression vector, respectively: a) USF1 (glucose-responsive transcription
factor) - the rationale that it should elevate ACCI3 gene promoter activity in
accordance with the glucose-fatty acid cycle, and b) nuclear respiratory factor 1
(NRF1) - the hypothesis being that this mitochondrial biogenesis and l3-oxidation
enhancing modulator would be expected to attenuate ACCI3 promoter activity in
order to increase fatty acid oxidation capacity.
To assess whether USF1 plays a role in ACCI3 gene induction in response to
increased glucose supply, we performed cotransfection stUdies together with a
USF1 expression vector under low or high glucose exposure. We found that
USF1 overexpression markedly elevates ACCI3 promoter activity in neonatal
cardiomyocytes and CV-1 'fibroblasts under low glucose culturing conditions.
Moreover, high glucose levels Significantly increased USF1-mediated ACCI3
promoter activation compared to the low glucose exposure in CV-1 fibroblasts.
These data suggest that glucose-responsive USF1 transactivation of the human
ACCI3 gene promoter occurs in a cell-type specific manner i.e. unlike the CV-1
fibroblasts the USF1 response in neonatal cardiac myocytes appears to be
glucose-independent. We next performed transfection assays in the presence of
2-deoxyglucose, a glucose analog that is taken up into the cell and not further
metabolized. In agreement with our earlier findings, 2-deoxyglucose did not
inhibit the USF1-mediated transactivation of the human ACCI3 gene promoter
activity in neonatal cardiomyocytes. In contrast, 2-deoxyglucose administration
robustly inhibited USF1-mediated human ACCI3 promoter activity in CV-1
fibroblasts. We next tested whether phosphatase 2A (PP2A), a downstream
target of the pentose phosphate metabolite xylulose-5-phosphate. plays a role in
the USF1-mediated transcriptional activation of human ACCI3 promoter. Here,
PP2A inhibition attenuated USF1-mediated transactivation of the human ACCI3
gene promoter in CV-1 fibroblasts. Surprisingly, PP2A inhibition also reduced
USF1-mediated transactivation of the human ACCI3 gene promoter in neonatal
cardiomyocytes. Furthermore. endogenous USF1 transcriptional activity was
also reduced following exposure to okadaic add.Since four E-box sequence elements were previously identified on the human ACCI) gene promoter, we next performed cotransfection studies with a USF1 overexpression vector to determine sequence elements responsible for the USF1-mediated transactivation of the ACCI) gene promoter. Employing deletion
constructs, we found that the shortest ACCI) promoter deletion construct was
able to induce ACCI) promoter activity in both cell lines. However, the induction
was reduced compared to the full-length construct indicating that the observed
USF1 induction may be mediated via E-box 4 interacting with other upstream
regions of the promoter predominantly through E-box 4 located close to the
transcription start site. In summary, these data show that glucose-mediated
USF1 induction of the human ACCI) gene promoter occurs in a cell-specific
manner. In CV-1 fibroblasts, USF1 transactivates the human ACCI) promoter in
a glucose-dependent manner, in part via dephosphorylation of USF1 by PP2A.
On the other hand, USF1-mediated induction of ACCI) also occurs through
dephosphorylation of USF1 by PP2A, although unlike CV-1 fibroblasts, glucose
metabolites do not appear to mediate this process.
We also found that NRF1 overexpression markedly attenuated ACCI) promoter
activity in neonatal cardiomyocytes and cardiac-derived H9C2 myoblasts.
However, NRF1 overexpression induced ACCI) promoter activity in both CV-1
fibroblasts and HepG2 hepatocytes. Interestingly. we found that USF1-mediated
induction of ACCI) promoter activity was markedly attenuated in all cell lines
tested. We therefore propose that NRF1 may interfere with USF1 binding of the
ACCI) gene promoter binding, probably via E-box4 located close to the
transcription start site. In summary, we suggest that under energy sparing
conditions, the transcriptional modulator NRF1 not only induces genes required
for mitochondrial biogenesis, but can also negatively regulate ACCI) gene
expression. This in turn should result in reduced malonyl-CoA levels and
elevated mitochondrial fatty acid oxidation In conclusion, we have identified a novel transactivator (USF1) and repressor (NRF1) of the human ACCI3 gene promoter in the heart. Our data may eventually result in the development of novel therapeutic interventions since we
have identified unique modulators regulating ACCI3 gene transcription, and by implication malonyl-CoA levels and mitochondrial fatty acid l3-oxidation.
Makaula, S (2021). Molecular Regulation Of The Cardiacenriched Acetyl-Coa Carboxylase Isoform (Accp): A Novel Target For Therapeutic Interventions In Cardiovascular Disease. Afribary. Retrieved from https://tracking.afribary.com/works/molecular-regulation-of-the-cardiacenriched-acetyl-coa-carboxylase-isoform-accp-a-novel-target-for-therapeutic-interventions-in-cardiovascular-disease
Makaula, Siyanda "Molecular Regulation Of The Cardiacenriched Acetyl-Coa Carboxylase Isoform (Accp): A Novel Target For Therapeutic Interventions In Cardiovascular Disease" Afribary. Afribary, 15 May. 2021, https://tracking.afribary.com/works/molecular-regulation-of-the-cardiacenriched-acetyl-coa-carboxylase-isoform-accp-a-novel-target-for-therapeutic-interventions-in-cardiovascular-disease. Accessed 25 Nov. 2024.
Makaula, Siyanda . "Molecular Regulation Of The Cardiacenriched Acetyl-Coa Carboxylase Isoform (Accp): A Novel Target For Therapeutic Interventions In Cardiovascular Disease". Afribary, Afribary, 15 May. 2021. Web. 25 Nov. 2024. < https://tracking.afribary.com/works/molecular-regulation-of-the-cardiacenriched-acetyl-coa-carboxylase-isoform-accp-a-novel-target-for-therapeutic-interventions-in-cardiovascular-disease >.
Makaula, Siyanda . "Molecular Regulation Of The Cardiacenriched Acetyl-Coa Carboxylase Isoform (Accp): A Novel Target For Therapeutic Interventions In Cardiovascular Disease" Afribary (2021). Accessed November 25, 2024. https://tracking.afribary.com/works/molecular-regulation-of-the-cardiacenriched-acetyl-coa-carboxylase-isoform-accp-a-novel-target-for-therapeutic-interventions-in-cardiovascular-disease