Abstract
As a mediator of insulin-regulated gene expression, the FoxO1 transcription factor represents a master regulator of liver glucose metabolism. We previously reported that the high-mobility group AT-hook 1 (HMGA1) protein, a molecular switch for the insulin receptor gene, functions also as a downstream target of the insulin receptor signaling pathway, representing a critical nuclear mediator of insulin function. Here, we investigated whether a functional relationship existed between FoxO1 and HMGA1, which might help explain insulin-mediated gene transcription in the liver. To this end, as a model study, we investigated the canonical FoxO1-HMGA1-responsive IGFBP1 gene, whose hepatic expression is regulated by insulin. By using a conventional GST-pull down assay combined with co-immunoprecipitation and Fluorescence Resonance Energy Transfer (FRET) analyses, we provide evidence of a physical interaction between FoxO1 and HMGA1. Further investigation with chromatin immunoprecipitation, confocal microscopy, and Fluorescence Recovery After Photobleaching (FRAP) technology indicated a functional significance of this interaction, in both basal and insulin-stimulated states, providing evidence that, by modulating FoxO1 transactivation, HMGA1 is essential for FoxO1-induced IGFBP1 gene expression, and thereby a critical modulator of insulin-mediated FoxO1 regulation in the liver. Collectively, our findings highlight a novel FoxO1/HMGA1-mediated mechanism by which insulin may regulate gene expression and metabolism.
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Introduction
The regulation of glucose metabolism and homeostasis is a central component of living systems. In mammals, this function is performed through distinct but interrelated cell signaling pathways that mediate the transduction of hormonal and nutrient stimuli to the nucleus, resulting in modifications of nuclear regulatory proteins (transcription factors), which bind to specific sites on the DNA and cause the activation or repression of genes and gene networks involved in these metabolic processes. Among the nuclear factors that act downstream of these pathways, the forkhead box protein O1 (FoxO1) is an important nutrient-sensing transcription factor that modulates the expression and activity of insulin-sensitive genes involved in gluconeogenesis, glycogenolysis and energy homeostasis1,2,3. Central to the functional regulation of FoxO1 is its nucleocytoplasmic shuttling following FoxO1 protein phosphorylation by the insulin-dependent phosphatidylinositol 3-Kinase/Akt (PI3K/Akt) signaling pathway4,5,6,7,8, a process that is further enhanced by FoxO1 acetylation9. Thus, in fasting conditions when insulin is low and the PI3K/Akt pathway is abrogated, FoxO1 binds the gluconeogenic genes10,11,12,13, and activates their expression, contributing to the maintenance of fasting euglycemia. Vice versa, in fed conditions, phosphorylation of FoxO1 by insulin, leading to the detachment of FoxO1 from DNA and its shuttling into the cytosol, represses gluconeogenesis4,14,15,16,17,18, thereby contributing to the maintenance of postprandial glucose homeostasis.
The high-mobility group A1 (HMGA1) protein is an architectural factor that binds to adenine-thymine (A-T) rich regions of DNA19. By itself, HMGA1 has no intrinsic transcriptional activity; rather, it can transactivate promoters by facilitating the assembly and stability of higher-order transcriptional complexes – so-called enhanceosomes – that drive gene transcription in response to extracellular and intracellular signals20,21. Such signals may affect HMGA1 function by inducing changes in post-translational protein modifications that markedly influence HMGA1 ability to interact with DNA substrates, other proteins and chromatin21,22. Previous studies from our laboratory have demonstrated that HMGA1 functions as a downstream nuclear target of the insulin receptor signaling pathway in vivo23. In particular, we showed that the hypoglycemic effect of insulin after meal, through the transcriptional repression of gluconeogenic genes, is mediated by HMGA123. Insulin exerts this transcriptional repression by triggering HMGA1 phosphorylation at three serine residues, via a PI3K/Akt pathway, inducing HMGA1 detachment from gluconeogenic gene promoters23. On the other hand, a relationship between HMGA1 and the insulin receptor signaling system has been demonstrated before, showing that HMGA1 is a key regulator of the expression of the insulin receptor24. Consistently with these observations, HMGA1 gene defects produce insulin resistance and type 2 diabetes in humans and mice25,26,27,28, whereas protection against insulin resistance has been reported in transgenic mice overexpressing Hmga129.
Increasing evidences demonstrated that FoxO1 executes its function on gene promoters by interacting with other nuclear proteins with which it assembles different transcriptional complexes13,30,31,32,33. However, the mechanisms by which these processes regulate FoxO1 activity are still largely unknown. On the base of the above considerations, here we explored the hypothesis that the insulin-mediated FoxO1-regulated metabolic pathway in the liver could be modulated by direct interactions of HMGA1 with FoxO1.
Results
Physical interaction between HMGA1 and FoxO1
We previously showed that phosphorylation of HMGA1 represents a critical event in mediating the insulin’s effect on gluconeogenic genes PEPCK and G6Pase, as well as other insulin target genes, such as the insulin receptor and the IGFBP1 genes23. On the other hand, FoxO1 is an important mediator of insulin action at these levels34,35, and cytoplasmic retention of FoxO1 via PI3K/AKT phosphorylation is considered to be a mechanism of insulin-mediated repression of insulin target genes34,35. Thus, the possibility that an interplay among HMGA1 and FoxO1 could be a fundamental prerequisite for these functions was investigated in this study. First, we tested the possibility that HMGA1 could physically interact with FoxO1, in the absence of DNA. We performed a GST pull-down assay, in which a GST-HMGA1 affinity resin was analyzed for its ability to specifically retain in vitro-translated 35S-labeled FoxO1. As shown in Fig. 1a, FoxO1 was retained by GST-HMGA1 but not GST alone, indicating that physical interaction between FoxO1 and HMGA1 occurs in vitro, in the absence of chromatin/DNA. The interaction between HMGA1 and FoxO1 was investigated further in co-immunoprecipitation studies with nuclear extracts from HepG2 cells, a cell line naturally expressing both HMGA1 and FoxO1 proteins, in the presence of an anti-HMGA1 specific antibody immobilized on protein A beads. As shown in Fig. 1b, immunoprecipitation of HMGA1 from HepG2 nuclear extracts, followed by western blot analysis for FoxO1, revealed a higher MW band (80-kDa), which migrated in a position corresponding to the size of FoxO1. When the same transfer was reprobed with an anti-HMGA1 specific antibody, a low MW band (12-kDa), which migrated in a position corresponding to the size of pure HMGA1, was detected as well (Fig. 1b). Co-immunoprecipitation between HMGA1 and FoxO1 was also observed in vivo, in liver extracts from wild-type mice (not shown), in which, however, specific signals on immunoblots were qualitatively poor as compared to those from HepG2 cells.
Thus, these results clearly indicate that HMGA1 and FoxO1 physically interact with each other in vitro, in cell free extracts, as well as in the context of intact cells and liver tissue samples.
Subcellular colocalization of HMGA1 and FoxO1
FoxO1’s activity is finely regulated by two distinct mechanisms: by post-translational modifications, which drive subcellular localization of FoxO1, and by protein-protein interactions, that mediate transcriptional activation36,37. As previously reported, both mechanisms are triggered by a wide variety of extracellular stimuli, which include oxidative stress, growth factors, and nutrients36,37,38,39. To substantiate the interaction between HMGA1 and FoxO1, and to address their subcellular localization in living cells, we performed FRET studies that finely allow the detection of associated proteins in living cells in real time. To this end, the coding sequences of both HMGA1 (HMGA1a isoform) and FoxO1 (FoxO1a isoform) were tagged with the yellow fluorescent protein (YFP) and the cyan fluorescent protein (CFP), respectively, and expressed in HEK-293 cells that were deprived of serum (starved) to prevent nuclear/cytoplasmic shuttling of the FoxO1 protein. As determined by Western blot analysis and reporter gene assay, both fusion proteins were expressed and functionally active following transfection of expression plasmids into cells (Fig. 2a). As shown in Fig. 2b, YFP-HMGA1 and CFP-FoxO1 exhibited a robust FRET signal in the nucleus of serum starved HEK-293 cells, with an almost equivalent distribution between the heterochromatin chromatin domains, found near the nuclear envelope, and the more transcriptionally active central nuclear position, which supports the physical interaction between the two proteins at this level. HEK-293 cells were ideally suited for FRET experiments since they do not express appreciable levels of endogenous HMGA1 and FoxO1, a condition that improves the analysis of transfected fluorescent proteins.
Functional significance of HMGA1-FoxO1 protein-protein interaction
The functional significance of the interaction between HMGA1 and FoxO1 in vivo was then investigated at the level of the endogenous IGFBP1 genomic locus, which is recognized as a downstream target of the insulin receptor signaling pathway, and whose transcriptional regulation by either FoxO1 or HMGA1 has also been reported10,14,23,40. Using the IGFBP1 gene promoter as a target of insulin action, we performed ChIP assays in HepG2 cells, along with quantitative qRT-PCR of ChIP-ed samples. As shown in Fig. 3a, FoxO1 occupancy at the IGFBP1 chromatin target site was downregulated by insulin and was significantly reduced in cells pretreated with distamycin A, a DNA-binding agent which selectively blocks DNA binding by HMGA124. In line with our previous observations indicating that functional integrity of HMGA1 is required for normal insulin action23, insulin failed to downregulate FoxO1-DNA binding in the presence of distamycin A (Fig. 3a). DNA occupancy by FoxO1 at these sites closely paralleled the changes in IGFBP1 protein production in HepG2 cells under the same experimental conditions as those used for ChIP (Fig. 3b), thus suggesting that binding of HMGA1 to DNA is required for FoxO1-DNA interaction and transcriptional activity and may constitute a prerequisite for the functional regulation of FoxO1 by insulin.
To clarify whether HMGA1/FoxO1 interaction had a functional implication in the transcriptional activity of IGFBP1 promoter, HEK-293 cells, which barely express HMGA1, were transfected transiently with an IGFBP1 luciferase reporter construct (IGFBP1-Luc), in the presence of both HMGA1 and FoxO1 expression vectors. As shown in Fig. 4a, simultaneous overexpression of HMGA1 and FoxO1 in HEK-293 cells led to a significant increment in IGFBP1 Luc activity that exceeded that seen with either factor alone, resulting in synergistic activation of transcription. Higher amounts of HMGA1 failed to increase further IGFBP1-Luc activity probably due to the property of HMGA1 to bind non-specifically to the DNA when present at high concentrations41. As expected, treatment of transfected cells with insulin resulted in the reduction of reporter gene activity (Fig. 4a). To investigate further the functional significance of HMGA1-FoxO1 protein-protein interaction, we employed the HMGA1m expression vector coding for a mutant form of HMGA1, in which the three active serine phosphorylation sites (Ser98, Ser101 and Ser102) at the C-terminus of the HMGA1 protein were mutated to nonphosphorylatable alanines23. As previously reported, insulin elicited no effect on this mutant protein, which remained bound to DNA, thus demonstrating that phosphorylation at these sites is essential for regulating HMGA1 activity by insulin23. Consistently with this, when both HMGA1m and FoxO1 expression vectors were simultaneously cotransfected with the IGFBP1-Luc reporter plasmid in HEK-293 cells, an increase in reporter activity was detected and this activity was maintained even after insulin treatment (Fig. 4a). Conversely, when transfection with FoxO1 expression vector was preceded by siRNA-induced silencing of HMGA1 expression in HepG2 cells, a cell line naturally expressing HMGA1, IGFBP1-Luc activity was significantly reduced and this reduction was more pronounced in cells not exposed to HMGA1 siRNA but treated with insulin (Fig. 4b). Interestingly, and in line with our previous original findings that HMGA1 may represent a critical nuclear mediator of insulin action23, insulin was ineffective in lowering IGFBP1-Luc activity in HMGA1 siRNA-treated HepG2 cells (Fig. 4b).
Dynamic interaction of HMGA1 with FoxO1
We next sought to investigate the dynamic interaction of HMGA1 and FoxO1 proteins in living cells. To this end, FRAP experiments were carried out in cells transfected with the CFP-tagged FoxO1 construct. By bleaching CFP-FoxO1 fluorescence in a defined nuclear region, we determined the time taken for fluorescence to recover by time-lapse confocal microscopy (Fig. 5a). Taking into account that the fluorescence recovery is dependent on the movement of unbleached CFP-FoxO1 molecules from the surrounding environment into the bleached region, it was then possible to measure the mobility of FoxO1 nuclear protein in CFP-FoxO1-expressing cells. In serum-starved HEK-293 cells, the fluorescence recovery of nuclear CFP-FoxO1 was incomplete (40% recovery), with a recovery time (t1/2) of 1.26 s, indicating that a significant fraction (~60%) of the CFP-FoxO1 fluorescent protein was bound to an immobile element within heterochromatic clusters (Fig. 5b). This observation fitted well with the notion that, in basal (starved) conditions, FoxO1 preferentially bound to DNA. Overexpression of either HMGA1 or HMGA1m in HEK-293 cells did not affect neither the fraction of immobile CFP-FoxO1 molecules (P = 0.28 and P = 0.71, respectively), nor the time of recovery for CFP-FoxO1 (P = 0.32 and P = 0.38, respectively) (Fig. 5b). After insulin treatment, the fluorescence recovery of CFP-FoxO1 was up to ~60%, with a shorter recovery time (t1/2 0.91 s), as compared to unstimulated cells (P < 0.001), thus indicative of an increased nuclear mobility of the CFP-tagged FoxO1 protein (Fig. 5b), which is consistent with the insulin-induced nucleocytoplasmic shuttling of FoxO1. Overexpression of HMGA1 in HEK-293 cells under insulin treatment reduced the immobile fraction of CFP-FoxO1 to 46.7%, suggesting an increasing number of CFP-FoxO1 molecules being tethered within heterochromatic clusters, whereas similar kinetics of dissociation of CFP-FoxO1 from endogenous and over-expressed HMGA1 were observed (FRAP recovery time: t1/2 = 1.65 s) (Fig. 5b). Instead, in cells overexpressing the mutant form of HMGA1 (HMGA1m), the recovery time of CFP-FoxO1 was 3.37 s, significantly higher (P < 0.01) with respect to control cells expressing the wild-type HMGA1 protein, thus indicating a reduced mobility of FoxO1, and an impaired nucleocytoplasmic shuttling of phosphorylated FoxO1 (Fig. 5b). Increased nuclear retention of phosphorylated FoxO1 was confirmed in time course experiments of FoxO1 protein phosphorylation in cytosolic and nuclear fractions of HEK-293 cells overexpressing either the wild-type or the mutant HMGA1m protein, which underwent insulin treatment (Fig. 5c). These data were further substantiated by ChIP assays coupled with qRT-PCR of ChIP-ed samples, showing that binding of FoxO1 to the endogenous IGFBP1 chromosomal locus was increased in HEK-293 cells overexpressing HMGA1m, in which the nuclear levels of pFoxO1 were higher with respect to cells overexpressing the wild-type form of HMGA1 (Fig. 5d). In line with this, as shown in Fig. 5e, IGFBP1 mRNA and protein levels were lower in insulin-treated HEK-293 cells overexpressing HMGA1 wild-type and higher in cells overexpressing the mutant HMGA1m protein, with these latter cells turning refractory to insulin with regard to the inhibition of IGFBP1.
Thus, taken togheter, these findings well support the functional relevance of HMGA1-FoxO1 interaction and provide evidence for the involvement of HMGA1 in insulin-mediated nucleocytoplasmic shuttling of FoxO1 protein.
FoxO1 and IGFBP1 expression in primary hepatocytes from normal and Hmga1-deficient mice
To further explore the functional significance of HMGA1-FoxO1 interaction in nuclear insulin signaling, we then performed experiments in primary cultured hepatocytes from both wild-type and Hmga1−/− mice. In these experiments, mRNA expression of FoxO1 and Igfbp1 was measured in primary cultured cells that were pretreated with the casein kinase (CK) 2 inhibitor 4,5,6,7-tetrabromo-1H-benzimidazole (TBB), which selectively blocks insulin-induced HMGA1 phosphorylation, and the subsequent detachment of HMGA1 from DNA23, without affecting FoxO1, whose phosphorylation is, instead, dependent on CK1 and several other protein kinases that alter subcellular location of FoxO1, DNA binding and transcriptional activity42,43,44,45. Consistent with previous observations from our group23,40,46, mRNA expression of FoxO1 and Igfbp1 was lower in primary cultured Hmga1−/− hepatocytes than in wild-type hepatocytes (Fig. 6). Following insulin treatment, the expression of mRNA for both FoxO1 and Igfbp1 decreased to 40–50% of control in cells from wild-type mice, whereas no changes in mRNA were observed in insulin-treated cells from mutant animals. Moreover, pretreatment of wild-type hepatocytes with TBB substantially attenuated the cellular response to insulin, with a less pronounced reduction in mRNA levels (Fig. 6), thereby indicating that the insulin’s effect on these two genes is mediated by HMGA1, and that functional cooperation between HMGA1 and FoxO1 may indeed constitute an essential step in nuclear insulin action.
FoxO1 in vivo, in normal and Hmga1 mutant mice
As a further step toward understanding the relationship between HMGA1 and FoxO1, we extended the above in vitro studies to studies in vivo, in wild-type (Hmga1+/+) and Hmga1−/− mice. As shown in Fig. 7, mRNA and protein abundances for FoxO1 were reduced in liver from 12 h-fasted Hmga1−/− mice, compared with wild-type animals. After refeeding, when the insulin receptor signaling is reactivated, both FoxO1 mRNA and protein were significantly reduced in liver from wild-type animals, while no difference on these parameters was observed in Hmga1−/− mice (Fig. 7), thereby confirming not only that HMGA1 is necessary for FoxO1 expression in vivo, in whole animals, but also that insulin-triggered FoxO1 downregulation is mediated by HMGA1. Similar results were obtained with mRNA and protein expression of Igfbp1 in liver from wild-type and Hmga1−/− mice under the same experimental conditions than those used for FoxO1 expression (Fig. 7), thus supporting the role of HMGA1 in the transcriptional regulation of IGFBP1 through the insulin/FoxO1 pathway.
The above results were confirmed by studies examining FoxO1 DNA-binding activity in vivo, in both wild-type and Hmga1−/− mice. As measured by ChIP in whole liver tissue, and subsequent qRT-PCR of ChIP-ed samples, binding of the Igfbp1 gene promoter by endogenous FoxO1 was reduced in Hmga1−/− mice compared to Hmga1+/+ animals (Fig. 8). After insulin injection in living mice, binding of FoxO1 to DNA was significantly decreased in wild-type mice, while no differences were observed in Hmga1−/− mice (Fig. 8). The same results were replicated in mice after meal ingestion, when endogenous insulin levels are expected to increase. As shown in Fig. 8, binding of FoxO1 to the Igfbp1 locus was high in wild-type mice under fasting conditions when nutrients are limited, serum insulin is decreased and binding of HMGA1 to DNA is preferentially increased. Conversely, FoxO1-DNA interaction promptly decreased in wild-type mice after refeeding, when serum insulin increases, insulin signaling is reactivated and both FoxO1 and HMGA1 become phosphorylated (Fig. 8). In fasted HMGA1−/− mice, binding of FoxO1 to the Igfbp1 promoter was lower, compared to that in wild-type mice, but in contrast to normal animals, no change in FoxO1-DNA interaction was detected upon refeeding of mutant animals (Fig. 8), thus confirming that HMGA1 is indeed required for the functional regulation of FoxO1 by insulin in vivo. Consistent with the above observations, fasting glycemia was significantly lower in Hmga1-null mice, compared to wild-type animals (Fig. 9), confirming the results obtained in previous studies using a large number of both wild-type and Hmga1-mutant mice40,46,47.
Discussion
As a member of the forkead family of transcription factors, FoxO1 regulates the transcription of a wide variety of genes involved in fundamental biological processes, such as cell growth and differentiation, DNA repair and apoptosis, inflammation and immune response1,2. Also, FoxO1 is a critical regulator of insulin signal transduction and energy metabolism2,3. In this last context, cytoplasm retention of FoxO1 via insulin-induced phosphorylation is considered to be a mechanism of insulin-mediated gene expression and regulation3. Dysregulation of FoxO1 at this level has been linked to metabolic abnormalities, including insulin resistance and type 2 diabetes35. Therefore, the observation that an interplay among HMGA1 and FoxO1 can be a component of the insulin/FoxO1 signaling pathway constitutes a novel point of the present study, which may help in understanding the molecular basis of certain disorders where insulin action becomes compromised (e.g. obesity, type 2 diabetes and other insulin-resistant conditions).
For the first time in the present work, we demonstrate that HMGA1 physically and functionally interacts with FoxO1, thereby regulating both FoxO1-DNA binding and insulin-mediated FoxO1 gene transcription. Although a direct interaction between FoxO1 and HMGA1 has been observed in our study, in the absence of DNA, we show that binding of HMGA1 to the insulin target gene IGFBP1 is necessary for FoxO1-DNA binding and transcriptional activity, and this may constitute an important requisite for the functional regulation of FoxO1 by insulin. In fact, when the ability of HMGA1 to bind DNA was prevented by distamycin A in vitro, in cultured cells, binding of FoxO1 to target DNA was markedly reduced, endogenous FoxO1-dependent gene expression was decreased, and insulin failed to downregulate FoxO1-DNA binding. Conversely, FoxO1-DNA binding and transcriptional activity were increased in cells overexpressing the mutant HMGA1m lacking the three serine phosphorylation sites responsive to insulin, in which, instead, the phosphorylation capability of FoxO1 by the PI3K/Akt pathway was not modified. Consistent with our results supporting a role for HMGA1 in nuclear FoxO1 mobility, nucleocytoplasmic shuttling of insulin-activated FoxO1 was impaired in cells overexpressing the mutant HMGA1m, whereas the nuclear trapping of FoxO1 was increased, thus providing compelling evidence that HMGA1 is indeed an important factor in modulating FoxO1 activity in the context of insulin receptor signaling and that the dynamic interaction between HMGA1 and FoxO1 plays a critical role in the control of insulin-mediated gene expression. In this regard, we previously reported that the counter-regulatory hormone glucagon, which acts in opposition to insulin to maintain fasting euglycemia, upregulated HMGA1 expression via the cAMP pathway, both in vitro and in vivo in whole mice47,48. Consistent with these previous findings, and with the observation that HMGA1 activates FoxO1 gene expression46, upregulation of FoxO1 via the glucagon-cAMP-PKA signaling has been reported in liver of fasting mice to maintain fasting euglycemia49. Based on our findings here, it is likely that upregulation of HMGA1 during fasting (when glucagon peaks) may contribute to the maintenance of fasting euglycemia through two distinct but converging mechanisms: by increasing FoxO1 expression in response to glucagon, and by directly and dinamically interacting with FoxO1, thus playing an important role in fine-tuning the activation of FoxO1’s transcriptional activity. Exactly the opposite after meal, when insulin peaks in response to high glucose availability and glucagon is suppressed. In this metabolic setting, functional inactivation of HMGA1 following insulin-induced HMGA1 protein phosphorylation, by causing the detachment of FoxO1 from DNA and its inactivation by nuclear exclusion, represses hepatic gluconeogenesis, thereby contributing to the maintenance of postprandial glucose homeostasis.
The functional affinity between HMGA1 and FoxO1 is also underlined by the fact that other than phosphorylation, both proteins are also post-translationally regulated by the same histone acetyltransferase CBP (CREB-binding protein), which was found to catalyze the acetylation of both HMGA1 and FoxO1, with subsequent inactivation of transcriptional activity of both nuclear factors50,51. On the other hand, distinct roles of HMGA1 and FoxO1 in the regulation of pancreatic beta-cell function and insulin production have been reported by us and others25,52,53. However, it cannot be excluded the possibility that functional interaction of HMGA1 with FoxO1 may be cell specifically regulated by additional factors, so that cooperation between HMGA1 and FoxO1 in the transcriptional regulation of FoxO1-target genes is essential in some cell types, but not in others.
The possibility for a functional relationship between HMGA1 and FoxO1 is further supported by some metabolic similarities between Hmga1-deficient mice and liver-specific FoxO1-deficient mice, including insulin hypersensitivity of peripheral tissues following insulin tolerance test, and lower fasting plasma glucose levels as compared with wild-type animals54,55,56,57,58,59,60. Similarities in body weight and body composition profiles are also found in both knockout mouse models, in which no changes were observed in these parameters among normal and mutant mice56,61,62. Also, similarly to what was observed before, in mice lacking liver FoxO156, a trend in increasing serum cholesterol levels was seen in Hmga1-knockout mice compared with controls, with a trend in reduction of triglycerides (unpublished data). Concerning this last point, it has to be admitted that conflicting results have been reported in liver-specific FoxO1-deficient mice, in which plasma triglycerides were either unaffected56,60,63 or increased64.
In toto, these findings establish HMGA1 as a critical element in the functional activity of FoxO1 transcription factor. Also, the data indicate that cross-talking between HMGA1 and FoxO1 is critical in relaying insulin signals down to the DNA, thereby ensuring insulin’s transcriptional regulation of glucose metabolism and homeostasis. Understanding this cross-talk is interesting from both biological and mechanistic standpoints and might be useful in understanding the molecular basis of disease states that arise from alterations in nuclear insulin signaling.
Methods
Ethics statement
The study was approved by the local ethics committee, Regione Calabria Comitato Etico Sezione Area Centro (protocol registry n. 116 of May 14, 2015), and the methods were performed in accordance with approved guidelines. All animal work was performed using approved animal protocols, according to relevant institutional guidelines for the care of laboratory animals (directive 86/609/ECC, European Community Council).
Cell cultures and nuclear extracts
Human embryonic kidney 293 (HEK-293) cells and HepG2 human hepatoma cells were cultured in DMEM and RPMI 1640 medium, respectively, supplemented with 10% fetal bovine serum (FBS) (Gibco Laboratories), 2 mM glutamine, penicillin (100 U/ml), and streptomycin (100 µg/ml) in a humidified 5% CO2 atmosphere at 37 °C. Cytoplasmic and nuclear protein extracts were prepared as previously24,65 and final protein concentration in the extracts was determined by the modified Bradford method (Bio-Rad Laboratories)66.
Glutathione S-transferase (GST) pull-down assay and co-immunoprecipitation
35S-labeled FoxO1 protein was synthesized by using the TNT-T7 quick-coupled in vitro transcription/translation system (Promega). GST tagged human HMGA1 was obtained using the pcDNA1-GST/HMGA1 expression vector, a kind gift from D. Thanos (Institute of Molecular Biology, Genetics and Biotechnology, Athens, Greece)24. Covalent coupling of antibody to protein A-Sepharose (GE Healthcare) was performed as previously described67. Antibody-coupled protein A beads were washed twice in phosphate-buffered saline and used in immunoprecipitation studies. Briefly, aliquots of HepG2 cell nuclear extract or pure HMGA1 were incubated for 3 h with rotation at 4 °C with 10 µl of antibody coupled protein A beads. Beads were recovered by gentle centrifugation and washed three times with 500 µl of NETN wash buffer [50 mM Tris-HCl (pH 8.0), 0.1% NP-40, 150 mM NaCl, 1 mM EDTA] for 5 min. Protein was removed from the beads by boiling in sample buffer for 5 min and analyzed by SDS-PAGE and immunoblotting67. Antibodies used for these studies were as follows: anti-HMGA124 and anti-FoxO1 (sc-11350) (Santa Cruz Biotechnology).
Plasmid construction and transfections, Fluorescence Resonance Energy Transfer (FRET), Fluorescence Recovery After Photobleaching (FRAP) analysis and confocal microscopy
Recombinant Luc reporter construct containing the human IGFBP1 gene promoter has been described previously23. The construct was transiently transfected into HEK-293 or HepG2 cells, using the LipofectAMINE 2000 reagent (Invitrogen Life Technology Corporation), in the presence or absence of effector vector for HMGA1 (HMGA1a isoform protein)23 and/or FoxO168, or HMGA1am23, and Luc activity was assayed 48 h later in a luminometer (Turner Biosystems Inc.), using the dual-luciferase reporter assay system (Promega). siRNA targeted to human HMGA1 (sc-37115) was purchased from Santa Cruz Biotechnology, whereas nonspecific siRNA controls with a similar GC content was obtained from Dharmacon (GE Dharmacon). 100–200 pmol siRNA duplex was transfected into cells at 40–50% confluency. After knockdown for 72 h, cells were trypsinized, pooled, and resuspended for a second transfection using the same targeting siRNA. After an additional 72 h, cells were prepared for analysis. Renilla control vector served as an internal control of transfection efficiency, together with measurements of protein expression levels.
To produce YFP-HMGA1a and CFP-FoxO1 expression plasmids, the human HMGA1a ORF (NCBI Ref. Seq. NM_145899.2) was cloned into BamHI/XbaI sites of pYFP (Clontech) and the human FoxO1 ORF (NCBI Ref. Seq. NM_002015.3) was cloned into BamHI/XbaI sites of pCFP (Clontech). Confocal imaging was performed with Leica SP2 inverted confocal microscope (Leica Mycrosystems), using 63 × Apo PLA oil immersion objective (NA 1.4) and 476 nm laser line. A 1 mm2 squared ROI within nucleus in heterochromatic region was set up for bleaching, 4 mm2 ROI for bleaching correction, and additionally 4 mm2 control ROI outside of cell area was acquired for background subtraction. The laser intensity was set up at 15%. Ten images were taken before the bleach pulse (15 laser iterations with bleaching intensity output 100%) and 60 images were taken after the bleaching with image acquisition each 0.3 s with 15% laser transmission. All FRAP experiments were performed in temperature-controlled CO2 supplied chamber. All FRAP plots were generated from background subtracted images using the public domain software ImageJ as previously described69. Shortly, the signal I was calculated in the area of interest (AOI) and normalized to the change in the total fluorescence due to the bleach pulse and the imaging: I = (To/Io) * It/Tt, where To and Tt are the total cellular fluorescence in the pre-bleach and post-bleach images, respectively, whereas Io is the average intensity in the AOI in the pre-bleach image.
Chromatin immunoprecipitation (ChIP)
ChIP assay was performed in cultured HepG2 and HEK-293 cells, either untreated or pretreated with siRNA targeting HMGA1, as described previously23,70. For in vivo ChIP, at the end of the indicated treatments, mice were killed by cervical dislocation, the liver was rapidly removed, prewarmed with PBS, and treated with 0.2% collagenase for 15 min. The liver was then diced, forced through a 60 µm stainless steel sieve, the hepatocytes were collected directly into DMEM containing 1% formaldehyde, and the formaldehyde-fixed DNA-protein complexes were immunoprecipitated with the anti-FoxO1 antibody sc-11350 from Santa Cruz Biotechnology. Sequence-specific primers for the IGFBP1 gene promoter used for PCR amplification of ChIP-ed DNA (30 cycles), using PCR ready-to-go beads (Amersham Pharmacia Biotech): human IGFBP1 (NT_007819) for 5′-CAGAAAGAGAAGCAATTCCG-3′, rev 5′-TACCAGCCAGACGCGAGCAA-3′; mouse Igfbp1 (NT_039515) for 59-CCTGGGGAGGGAGAAACAACT-39, rev 59-GCAGTGTTCAATGCTCGCTGG-39. PCR products were electrophoretically resolved on 1.5% agarose gel and visualized by ethidium bromide staining.
Immunoprecipitation and Western blot
A polyclonal-specific antibody against HMGA123 was used to analyze HMGA1 protein expression in HEK-293 and HepG2 cells, and in liver nuclear extracts from normal and Hmga1 mutant mice. An anti-FoxO1 antibody (Santa Cruz Biotechnology) was employed to measure total FoxO1 in both human cell lines and animal tissues. An anti phospho-FoxO1 (Thr24) (Cell Signaling Technology) was used to analyze the levels of pFoxO1 protein in both nuclear and cytoplasmatic extracts.
Studies in animals
Male Hmga1-deficient mice and wild-type littermates aged 6–9 months were studied. The generation of these animals has been described previously25. We have thoroughly investigated male mice to exclude the known effects linked to estrogen cyclicity, thereby limiting variability62. FoxO1 and Igfbp1 mRNA and protein levels were analyzed in liver from age and weight matched 12-h fasted mice and after 4 h refeeding. ChIP of the Igfbp1 gene was performed in liver from 12 h-fasted animals following intraperitoneal injection of insulin (1U/kg bw) or saline, and after fasting and refeeding conditions. Cryopreserved primary hepatocytes from Hmga1−/− and wild-type mice were cultured as previously described23.
Statistical analysis
The non-parametric Mann-Whitney test was used for comparisons of continuous variables. A significance level of 0.05 was set for a type I error in all analyses. All bar graph data shown represent mean ± standard error of the mean (s.e.m.). All data were analyzed with SPSS 20.0 software (SPSS Inc.).
Data availability
The datasets generated during the current study are available from the corresponding author on reasonable request.
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Acknowledgements
We are very much obliged to Proff. A. Fusco and M. Fedele (University of Naples, Italy) for providing animals and laboratory facilities. Thanks to Prof. Marta Hribal for critical suggestions. This research did not receive any specific grant from any funding agency in the public, commercial or not-for-profit sector. B.A. is supported by a grant within the project PON03PE_00009_2 iCaRe; D.M.C. is a recipients of a PhD studentship from the “Magna Græcia” University.
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E.C. and A.B. conceived the study, designed the experiments, and analyzed the data; E.C. performed statistical analysis and prepared the first draft of the manuscript; B.A. performed transfection studies and ChIP; D.M.C. performed western blot analyses, pull-down and co-immunoprecipitation studies; C.P. performed FRAP and FRET experiments; V.M.M. and D.B. were involved in the data analysis and biological interpretation; M.A. provided the effector vector for FoxO1; D.P.F. was involved in data analysis, interpretation and critical reading of the manuscript; A.B., the corresponding author, provided financial support, supervised the project and wrote the final version of the paper.
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Chiefari, E., Arcidiacono, B., Palmieri, C. et al. Cross-talk among HMGA1 and FoxO1 in control of nuclear insulin signaling. Sci Rep 8, 8540 (2018). https://doi.org/10.1038/s41598-018-26968-3
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DOI: https://doi.org/10.1038/s41598-018-26968-3
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