REST mediates resolution of HIF-dependent gene expression in prolonged hypoxia

The hypoxia-inducible factor (HIF) is a key regulator of the cellular response to hypoxia which promotes oxygen delivery and metabolic adaptation to oxygen deprivation. However, the degree and duration of HIF-1α expression in hypoxia must be carefully balanced within cells in order to avoid unwanted side effects associated with excessive activity. The expression of HIF-1α mRNA is suppressed in prolonged hypoxia, suggesting that the control of HIF1A gene transcription is tightly regulated by negative feedback mechanisms. Little is known about the resolution of the HIF-1α protein response and the suppression of HIF-1α mRNA in prolonged hypoxia. Here, we demonstrate that the Repressor Element 1-Silencing Transcription factor (REST) binds to the HIF-1α promoter in a hypoxia-dependent manner. Knockdown of REST using RNAi increases the expression of HIF-1α mRNA, protein and transcriptional activity. Furthermore REST knockdown increases glucose consumption and lactate production in a HIF-1α- (but not HIF-2α-) dependent manner. Finally, REST promotes the resolution of HIF-1α protein expression in prolonged hypoxia. In conclusion, we hypothesize that REST represses transcription of HIF-1α in prolonged hypoxia, thus contributing to the resolution of the HIF-1α response.

Hypoxia is a key microenvironmental feature of a range of physiological and pathophysiological conditions including embryonic development, exercise, cancer, ischemia and inflammation 1 . Adaptive transcriptional pathways have evolved to help an organism deal with the metabolic threat posed by hypoxia. The best-described transcriptional adaptive response in cells is mediated by the hypoxia inducible factor (HIF) signalling pathway, which up-regulates genes which restore oxygen and energy homeostasis [2][3][4] . In normoxia, HIFα is hydroxylated by the prolyl-hydroxylase domain (PHD) family of dioxygenases targeting it for proteosomal degradation 5 . This process is reversed in hypoxia and HIFα is stabilized, dimerizes with HIFβ and binds to hypoxia response elements (HRE) in the regulatory regions of target genes 6 . HIF drives an adaptive response to hypoxia by promoting the expression of genes including those that regulate erythropoiesis, angiogenesis and glycolysis 6 . However in cancer, HIF signalling can be maladaptive and contribute to tumour survival 1 . Because of the potentially deleterious effects of over-activation of the HIF pathway, a resolution mechanism is required to resolve its activity in prolonged hypoxia. In the absence of such a resolving mechanism, deleterious consequences such as pathologic angiogenesis and excessive haematocrit due to chronic HIF stabilization may occur [7][8][9] .
While several regulators of HIF expression exist, only a few have been shown to be involved in the resolution of the HIF response to hypoxia. PHD2 and PHD3 are, for example, part of an auto-regulatory mechanism, whereby HIF-1α which is stabilized in hypoxia, transcriptionally induces the expression of EGLN1 and EGLN3 genes coding for PHD2 and PHD3 proteins respectively [10][11][12] . The increased expression of the PHD enzymes in turn promotes HIFα hydroxylation, and reduction of its expression in prolonged hypoxia 10 . Less is known about the control of HIF1A mRNA stability 11 . Interestingly, while HIF-1α protein is transiently up-regulated in hypoxia, the mRNA is frequently found to be repressed [12][13][14][15] . This transcript attenuation can be conveyed through mRNA destabilization by the protein tristetraprolin in endothelial cells 14 and by miR155 in intestinal epithelial cells 12 .

Results
HIF-1α protein is transiently stabilized in hypoxia while its mRNA is suppressed. The HIF-1α response in prolonged hypoxia involves a rapid protein accumulation phase ( Fig. 1A-F), followed by a protein resolution phase, where HIF-1α levels decay back to close to normoxic levels ( Fig. 1A-F). In the HEK293 cell line, HIF1A mRNA expression decreased by only 21% to 32% after 8 hours of exposure to hypoxia (Figs 1G and 3E). In other cell lines including the intestinal epithelial cancer cell line CaCo-2 and in HeLa cells, HIF1A mRNA has been reported to decreased by ~ 50% after 6 to 8 hours of hypoxic exposure (1% oxygen) 12,41 . Here, we observed that in normal breast and breast cancer derived cell lines, HIF1A mRNA expression can decrease by 50 to 80% after 8 hours of hypoxic exposure (Fig. 1G). Thus, suppression of HIF1A mRNA is common in response to hypoxia.
NFκ B has been shown to be responsible for the transient and early HIF1A mRNA induction in response to hypoxia, 1% oxygen, in human pulmonary arterial smooth muscle cells 24 . Therefore we decided to test if in HEK293 cells NFκ B was recruited to the HIF1A κ B element previously shown to bind p50 and p65 in response to hypoxia and activate HIF1A transcription 24 . Using chromatin immunoprecipitation assays (ChIP), with a rabbit p65 antibody or rabbit IgG negative control antibody from pre-immune sera, chromatin pull-downs were performed, and qRT-PCR was used to quantify the chromatin containing the HIF1A κ B element. This revealed that p65 was transiently recruited to the κ B site on the HIF1A promoter in response to hypoxia, being significantly up-regulated in comparison to normoxia and IgG at 8 hours (Fig. 1H). Despite the recruitment of p65 to the κ B site on the HIF1A promoter, HIF1A mRNA is still significantly decreased in hypoxia (Figs 1G and 3E), this indicates that counter-regulatory mechanisms must be acting either at the level of regulating mRNA transcription or stability. We next investigated the possibility that a transcriptional repressor was counter-regulating NFκ B-dependent activation of HIF1A gene transcription (see below).
REST negatively regulates HIF-1α. The protein tristetraprolin 14 , the microRNA miR155, and the lncRNA aHIF 13,16 have all been shown to regulate HIF1A mRNA stability, but no example is known of a transcriptional mechanism directly acting on the HIF1A promoter. Therefore, we decided to use the ENCODE consortium ChIP-Seq datasets to determine which transcriptional repressors are bound to the human HIF1A promoter region, 4000 bp upstream and 2000 bp downstream of the ATG ( Fig. 2A,B). This revealed the presence of multiple transcription factors (Fig. S1), among which were members of the REST co-repressor complex, namely REST, mSin3A, RCOR1 (CoREST), and HDAC2 (Fig. 2B) 34 . Due to the previous implication of REST in the response to ischaemia, we decided to test if REST was involved in the repression of HIF1A gene transcription. Using the JASPAR database, we looked for putative REST binding sites (RE1) on the HIF1A promoter region covered by the ChIP-Seq hits of the REST co-repressor complex family of nuclear factors (Fig. 2C). And identified an RE1 which was evolutionarily conserved within primates, but diverged in other mammals (62 to 81% conserved base pairs in the RE1 site) and was not present in more distant animal species having REST orthologous proteins (Fig. 2D). REST binding to this RE1 site was validated in human HEK293 cells using ChIP assays coupled to qRT-PCR using primers that amplified (G) Cells where exposed to 8 hours of hypoxia (1% oxygen) or normoxia (21% oxygen), the mRNA was collected and used for qRT-PCR analysis of HIF1A mRNA expression. Results are shown as fold change to normoxia. (H) ChIP assays coupled to qRT-PCR where performed on HEK293 cells exposed to hypoxia for the indicated time points using p65 and IgG control antibodies, primers covering the NFκ B site on the HIF-1α gene where used (see sequence highlighted in blue in Fig. 3A). N = 3-4 independent experiments. Data are represented as mean ± SEM. In (G), *p < 0.05, ***p < 0.001, significant fold change over 21% O 2 . In (A), *p < 0.05, significant increase over normoxic p65 ChIP and IgG ChIP. The HIF1A gene with mammalian conservation is depicted in relation to its position on chromosome 14 q23.2 (modified from the UCSC Genome Browser). The human HIF1A promoter region -4000 bp upstream to + 2000 bp downstream of the translation start site (ATG) was used to screen for the presence of REST-repressor complex components on the ENCODE ChIP-seq datasets. This is a highly conserved region surrounding EXON1. The full list of transcription factors found to be associated on this region of the HIF1A gene is described in Fig. S1. (B) Close up view on the ChIP-seq hits found for the REST co-repressor complex components: REST, mSin3A, CoREST (RCOR1) and HDAC2 on the HIF1A gene promoter. Conservation is depicted by vertical blue bars, bellow the ChIP-seq hits (horizontal grey-scale bars). (C) The genomic DNA where REST co-repressor complex ChIP-seq hits was found, was screened using the JASPAR database for the presence of RE1 elements, this revealed a putative RE1 in the -491 bp to 0 bp promoter region (highlighted in red), in close proximity to the previously reported NFκ B site on the HIF1A gene (highlighted in blue). a 62 bp amplicon containing the RE1 site (Fig. 3A). REST and its co-repressor proteins CoREST and mSin3A were found to be recruited to the HIF-1α gene with similar dynamics (Fig. 3B). Thus, we identified a functional RE1 site in the HIF1A promoter that binds REST and its co-repressors CoREST and mSin3A.
To test if REST had a functional effect on HIF1A expression, in addition to its binding to the HIF1A promoter, REST knockdown using RNAi was used in HEK293 and MCF7 cells. This led to a significant increase in HIF-1α protein ( Fig. 3C-F) and mRNA (Fig. 3G), suggesting that REST is a negative transcriptional regulator of HIF-1α expression at least in hypoxia. In HEK293 cells we did not observe up-regulation of HIF-2α in response to hypoxia 42 and MCF7 cells did not show any change in HIF-2α upon REST knockdown (Fig. 3E,F). We also observed that HEK293 cells overexpressing REST had reduced expression of HIF-1α protein ( Figure S2).
Together these findings provide evidence that REST negatively regulates HIF-1α through promoting the the assembly of a REST repressor complex on the HIF1A promoter cis-regulatory RE1 element. The data provide insight into the mechanisms underpinning attenuation of HIF1A mRNA expression in prolonged hypoxia.
REST is involved in the resolution of the HIF-1α response. Data presented thus far demonstrates that REST negatively regulates HIF-1α . We next investigated whether REST is involved in the resolution of the HIF-1α -dependent functional response. Typically, in vitro, HIF-1α protein accumulates quickly in response to hypoxia, but the response is decreased over prolonged exposure (Fig. 4A, B-black bars). Upon REST knockdown, HIF-1α protein rapidly accumulated in hypoxia, but did not decrease under prolonged hypoxia. Instead the HIF-1α response plateaued (Fig. 4A, B-red bars), indicating that REST may be involved in the resolution of the HIF-1α response. These findings were further confirmed by the increased HIF-1α -reporter activity under prolonged hypoxia when REST is knocked down (Fig. 4C), and decreased HIF-1α reporter activity when REST is overexpressed (Fig. 4D). Endogenous HIF-1α transcriptional activity under REST knock-down was also increased, as accessed by increased mRNA expression of the HIF-1α target genes PHD2 and PHD3 (Fig. 4E,F).
Our data shows that REST plays a role in the suppression of HIF-1α protein expression and transcriptional activity in prolonged hypoxia. Thus there is clear indication for the involvement of REST in the resolution of the HIF-1α response. ChIP assays on the RE1 site in the HIF1A gene promoter using the indicated antibodies in HEK293 cells exposed to the indicated time points to hypoxia (1% oxygen). Precipitated chromatin was quantified by qRT-PCR. (C-G) Cells were exposed to hypoxia (1% O 2 ) for the indicated time points. REST knockdown was performed using REST specific (REST-RNAi) or control RNAi (C-G). Whole cell extracts from HEK293 (C,D) and MCF7 (E,F) were collected and analysed for the expression of the indicated protein by immunoblotting (C,E) and densitometry analysis (D,F). HEK293 mRNA was collected and analysed for HIF mRNA expression by qRT-PCR (G). F.C. = fold change to 21% O 2 for (G) and control RNAi, 8 hours hypoxia for (C-F). Data are represented as mean ± SEM, N = 3-5 throughout. *p < 0.05, significant change over control RNAi.
Scientific RepoRts | 5:17851 | DOI: 10.1038/srep17851 REST regulates glycolytic metabolism in hypoxia. Having observed that HIF-1α activity is increased under prolonged hypoxia when REST levels are decreased by RNAi, we next investigated whether this is reflected by altered functional responses to hypoxia. The mRNA expression levels of four well described HIF-1α target genes encoding proteins known to be involved in glucose metabolism (HK2, LDHA, SLC2A1 and PFKFB3) were measured. In hypoxia, the expression of these genes was increased upon loss of REST ( Fig. 5A-D). These results suggest that REST loss could affect glucose metabolism by increasing glucose consumption. We measured glucose consumption and lactate production in HEK293 cells and observed that, in hypoxia (1% oxygen), knockdown of REST resulted in enhanced glucose consumption and lactate production (Fig. 5E,F). Thus we show that REST supresses hypoxia-induced glucose consumption and lactate production via repression of HIF-1α . In conclusion, we identify REST as a repressor of gene expression in hypoxia which acts through the repression of HIF-1α -dependent transcription.

Discussion
The regulation of HIF-1α expression is well documented at the protein level, but much less is known about the control of its mRNA stability 11 . Interestingly, while HIF-1α protein is transiently up-regulated, the mRNA is actually repressed [12][13][14][15] . This transcript attenuation can be conveyed through mRNA destabilization by the protein tristetraprolin in endothelial cells 14 and by miR-155 in intestinal epithelial cells 12 . The HIF-1α antisense transcript (aHIF), which is widely expressed in both adult and foetal tissue 16 , has also been shown to down-regulate HIF-1α mRNA in lymphocytes, non-papillary renal cell carcinoma and lung epithelial cells 13,15 . All these different mechanisms converging to the reduction of mRNA expression in hypoxia indicate that this is an important adaptation to hypoxia, potentially to prevent an over activated HIF response that could be detrimental to cells and tissues 12 . Further supporting this protective role of reduced HIF-1α mRNA expression in prolonged hypoxia, high levels of HIF-1α mRNA have been observed in hepatocellular carcinoma, gastric cancer and prostate cancer and often associated to poor prognosis [17][18][19][20] .
Here, we demonstrate the existence of a transcriptional repressor mechanism acting on the HIF1A promoter response to prolonged hypoxia. This data together with the recruitment of p65 to the HIF1A promoter (Fig. 1H) indicates that HIF1A transcription is under the tight control of both a transcriptional activator and a repressor in response to hypoxia, and de-regulation of this balance might contribute to changes in HIF1A mRNA expression. This can be expected to occur in situations where p65 is activated including inflammatory settings 43 and when REST is down-regulated including cancer 35   observed after 8 hours of hypoxia (Fig. 1H), no induction of HIF1A mRNA is observed in REST knockdown cells (Fig. 3G), indicating REST-independent mechanisms involved in the repression of NFκ B -induced transcription (e.g. tristetraprolin, miR-155 and aHIF).
REST knockdown had no effect on HIF-2α protein expression (Fig. 3D). Of notice, miR-155 and aHIF, known regulators of HIF1A mRNA also exhibit specificity towards HIF-1α , without an effect on EPAS1 (gene coding for HIF-2α ) mRNA expression 12,13 . EPAS1 mRNA is generally not repressed by hypoxia like HIF1A mRNA 12,13 , it is therefore not entirely surprising that the mechanisms that lead to HIF1A mRNA repression in hypoxia do not affect EPAS1 mRNA expression. In conclusion, REST regulates HIF-1α , but not HIF-2α expression at least in MCF7 cells.
The tumour suppressor role of REST in non-neuronal cells has been linked to proliferative pathways 35,38 . However, the exact mechanisms whereby REST induces these changes remain unknown 35 . In this work we have shown that REST reduces HIF-1α expression and glycolysis in hypoxia, two promising targets for cancer therapy 45 . Thus our molecular biology findings have the potential to be of clinical importance in cancer, and expands the current knowledge about the mechanisms whereby REST might exert its tumour suppressor role. Our data suggest that in the absence of REST, as it occurs in REST-less tumours, there is no repression of HIF1A transcription, therefore positive regulators like NFκ B are able to freely drive HIF1A transcription, leading to increased HIF-1α protein expression in hypoxic tumour microenvironments. Indeed, we observe that the tumour cell line HepG2, which displays HIF1A mRNA induction in hypoxia, has lower REST level than HEK293 ( Figure S3). HIF activates several processes that confer an advantage for the development of cancer 46 . Among these processes is glycolysis, which facilitates energetic adaptation to the hypoxic environment 47 .
In addition, glycolysis is also known to be correlated to increased tumour aggressiveness, as it facilitates acidosis, eliminating normal cells surrounding the acidic environment or inducing mutations that will transform these cells, and is able to stimulate in vitro invasion and in vivo metastases, potentially by inducing extracellular matrix degradation 46,47 .
REST is a tumour suppressor in non-neuronal cancers of the breast, colon and lung, therefore increasing the range of pathophysiological settings were our findings might be of importance in the regulation of the HIF-1α response and glycolysis 45 . HIF-1α regulation by oncogenic pathways has been shown to operate mostly by increasing protein expression or decreasing its degradation 45,48 . Over-activation of the PI3K/Akt/mTOR pathways leads to increased HIF1A mRNA translation and inactivation of VHL can lead to decreased HIF-1α protein degradation [27][28][29][30]45,49 .
HIF1A mRNA is also overexpressed in cancer, correlating to cancer aggressiveness 11,17,50 . However, there is no clear known mechanism explaining this overexpression 45 . The transcription factors NFκ B 24,31 and NFAT 32 are described to transcriptionally activate HIF1A in response to inflammatory stimuli and in activated mast cells, respectively. In many situations the cancer microenvironment can be inflamed, and inflammation can drive cancer development, but the roles of NFκ B and NFAT in regulating HIF1A in this context remain to be fully elucidated 11 . The V-SRC oncogene has been shown to increase HIF1A mRNA, however the mechanism remains poorly understood 27 .
In this work, we have observed that loss of REST by genetic manipulation leads to increased HIF-1α expression, while increased REST levels lead to reduced HIF-1α expression. Thus REST is a tumour suppressor gene that transcriptionally represses HIF1A. We hypothesize that loss of the tumour suppressor REST 51 being the only known transcriptional repressor of HIF1A transcription, would allow the positive transcriptional regulators of HIF1A to drive its transcription, explaining its over-expression in several cancers. Taken together these observations suggest that our findings may be of clinical importance, as they provide insight into the crosstalk between hypoxia, HIF-1α , glycolysis and REST, all of which play important roles in solid tumours 35,52 .
We have shown that in hypoxia REST is recruited to the HIF1A promoter, together with the co-repressors CoREST and mSin3A. These co-repressor complexes have associated enzymes with chromatin modifying activity including histone deacetylases, histone methytransferases and demethylases, and methyl-CpG-binding protein 2 (MeCP2) 34 , thus suggesting that REST serves as a platform for the hypoxia induced epigenetic silencing of HIF1A expression in hypoxia. This would counteract the recruitment of NFκ B to the HIF1A promoter, which has been associated to increased transcription in hypoxia 24 . Together these two regulators REST and NFκ B may act to fine tune HIF1A expression according to environmental clues, and de-regulation of the expression of one of these transcription factors is expected to affect HIF1A expression, as it can happen in inflammatory diseases 43 and REST-less tumours 35 . Of interest MeCP2, a protein often associated with the long term silencing by the REST co-repressor complex, and usually found in the vicinity of the RE1 element 34,53 , has been found in the HIF1A promoter region, upstream of the ATG, in close proximity to the RE1 we identified on HIF1A 54 .
In clear cell renal cell carcinoma (CCRCC) VHL-defective RCC4 and RCC10 cells, binding of HIF-1α /2α to the reverse HRE (rHRE) on the HIF1A promoter, leads to H3K9 methylation, H3K4 de-methylation and HIF1A repression 55 . Binding of HIF-α subunits to rHREs has been described as a mechanism to repress transcription in hypoxia 56,57 . Interestingly, these methylation changes are classical marks of REST-mediated epigenetic silencing 34 . The authors of the previous study speculate on the recruitment, through as yet unknown mechanisms, of complexes carrying histone modifying activities to mediate these epigenetic changes 55 . Of note this rHRE is located up-stream of the ATG, in close proximity to the RE1 we identified. In summary, the HIF1A promoter contains epigenetic marks associated with REST (e.g. methylated H3K9) or chromatin modifying proteins associated with the REST co-repressor complex (e.g. MeCP2), this together with our findings of the recruitment of REST and its co-repressor complexes mSin3A and CoREST to the HIF1A promoter suggests a role for REST as an epigenetic regulator of HIF1A.
In conclusion, our findings have identified REST as a key repressor of HIF1A gene transcription and it's downstream glycolytic genes, playing a key role in cellular adaptation to hypoxia.
Gaussia luciferase assay, transient and stable transfections. Gaussia luciferase assays were performed as previously described 58 . Briefly, at the selected time points, 10 μ L of media was collected from the supernatant and stored at -20 °C. Gaussia luciferase activity was measured using the Biolux Gaussia luciferase Flex Assay kit (NEB) in a plate reader (Synergy HT, Biotek) and normalized to the luciferase activity of the secreted cypridina luciferase under the control of a constitutive CMV promoter (pCMV-CLuc) or protein concentration. The pHRE-MP-GLuc HIF responsive construct has been previously described 58 . The pCMV-CLuc construct was from NEB (N0321S, pCMV-CLuc 2). Plasmid sequencing was performed by MWG Eurofins, Germany.
Transfections with siRNA to be used in luciferase assays were performed in 24 well plates, as described above. All other experiments were performed on 6 well plates unless otherwise stated. In a typical experiment 200 K cells were seeded on 6 well plates and allowed to grow until approximately 60% confluent, at this time cells were transfected with 2 μ L of Lipo, 100 μ L Optimem and a pre-optimized amount of overexpressing construct (100 ng) or siRNA (100 pmol). Cells were media changed to 2 mL of conditioned media on the day after transfection. In order to keep the same transfection times with the siRNA, in experiments were hypoxic exposures were longer than 16 hrs, cells were conditioned to hypoxia on different days and lysed on the same day. For RNA extraction experiments, siRNA was incubated for 48 hrs. For the preparation of whole cell protein extracts, siRNA was incubated for 72 hrs. For the experiments where the role of REST in the resolution of the HIF-1α response was investigated (Fig. 4A,B), HEK293 cells were stably transfected with a plasmid coding for a short-hairpin RNA (shRNA) targeting the coding sequence of REST mRNA (sc-38129-SH, Santa Cruz) or a control shRNA plasmid (sc-108060, Santa Cruz), and selected with puromycin, according to the manufacturer instructions. For experiments where REST was overexpressed using msREST-FLAG, 80 K cells were seeded on 12 well plates, and cells were transfected with 100 ng msREST-FLAG, 100 ng HREG and 50 ng pCMV-CLuc with 100 μ L Optimem and 1 μ L Lipo. The media was changed to fresh media on the day after transfection.
qRT-PCR. cDNA was synthesized from 1 μ g of RNA using MMLV (Promega), and amplified using the Prism 7900HT sequence detection system (Applied Biosystems, Foster City, CA) under default conditions. The mRNA relative expression was calculated by the ∆∆Ct method by normalizing the Ct of the samples to that of 18S rRNA (TaqMan Universal PCR Master Mix with the primer 18S rRNA-Euka, 4310893E, Life Technologies), followed by normalization to the control condition. The following qRT-PCR primers were used: Chromatin immunoprecipitation. ChIP assays where performed as previously described 60 . Briefly, HEK293 cells fully confluent on T175 flasks were conditioned to hypoxic media (1% oxygen) for the indicated time points. Cells were fixed with 2% formaldehyde in 10 mL fresh media for 10 min with agitation. Cells were removed from the hypoxic chamber and fixation was stopped with 125 mM glycine treatment for 5 min. The following mix was prepared: 1 uL of the purified DNA was used, 0.4 μ L of 20 μ M primers, 8 uL RNAse free water and 10 μ L of Power SYBR ® Green (Applied Biosystems). The quantitative Real-Time PCR was performed using the 7900HT Fast Real-Time PCR System. Precipitated chromatin was normalized to input samples and the control IgG IP's are shown as a negative control, as previously described 60 .

Glucose and lactate quantification assays. For the lactate assays (Trinity Biotechnology Lactate Assay
Kit, REF735-10), 1 μ L of the supernatant or Lactate Standard Solution was incubated with 100 μ L of the Lactate Reagent Solution (lactate oxidase, peroxidase, chromogenic precursor and a pH 7.2 buffer), incubated at room temperature for 10 min, absorbance at 540 nm was used to calculate the lactate concentration in the media, absorbance was corrected from blank. Lactate production relative to time zero was calculated and normalized to the protein concentration. For the glucose assays (Biovision, Glucose Assay Kit, REFK606-100) the media was diluted 1 in 10 in Assay Buffer, 1.5 μ L of the diluted sample were mixed with 48 μ L of the Assay Buffer, 1 μ L of the Glucose Enzyme Mix and 1 μ L of the Glucose probe. This was followed by incubation for 30 min at 37 °C, protected from light, and absorbance was measured at 570 nm to calculate glucose concentration in the media relative to a standard curve of a supplied glucose standard, absorbance was corrected from blank. Glucose consumption relative to time zero was calculated and normalized to the protein concentration. For HEK293 cells treated with siRNA, transfection was performed as described under the "Gaussia Luciferase Assays" section. Bioinformatics identification of the RE1 elements. ChIP-Seq data obtained by the ENCODE consortium across multiple cell lines and available at the UCSC genome browser (http://genome.ucsc.edu/) and the JASPAR database (http://jaspar.genereg.net/) of transcription factor binding sites, revealed the presence of a putative RE1 site on the HIF-1alpha promoter, located between 5207 and 5257 on the Homo sapiens HIF1A gene sequence on chromosome 14 (NCBI Reference Sequence: NG_029606.1). The Translation Start Site, referred to as ATG was determined by aligning the consensus coding sequence (CCDS) of HIF1A-001 (CCDS9753) to the HIF1A genomic DNA sequence. This corresponds to the uniprot entry (Q16665-1), the canonical HIF-1α isoform, with 826 amino acids (http://www.uniprot.org/uniprot/Q16665).

Statistical analysis.
All experiments were performed at least 3 independent times. All immunoblots shown are representative of biological replicates. Data is shown as mean ± SEM. Statistical significance was tested in Prism (Graphpad), using Student's t test for the comparison of two data sets or ANOVA for more than two datasets. *p < 0.05, **p < 0.01 and ***p < 0.001.