The hematopoietic regulator, ELF-1, enhances the transcriptional response to Interferon-β of the OAS1 anti-viral gene

Interferon (IFN) therapy is effective in treating cancers, haematological and virus induced diseases. The classical Jak/Stat pathway of IFN signal transduction leading to changes in transcriptional activity is well established but alone does not explain the whole spectrum of cellular responses to IFN. Gene promoters contain cis-acting sequences that allow precise and contextual binding of transcription factors, which control gene expression. Using the transcriptional response to IFN as a starting point we report a high frequency of tandem GGAA motifs in the proximal promoters of Interferon stimulated genes, suggesting a key regulatory action. Utilizing the well-characterized anti-viral gene, OAS1, as an example Interferon stimulated gene promoter containing such a duplicated GGAA motif, we have demonstrated a regulatory role of this promoter in response to IFN by mutation analysis. Furthermore, we identified ELF-1 as a direct binding factor at this motif. Additionally, recruitment of RB1 and SP1 factors to the promoter following IFN stimulation is shown. ELF-1 overexpression enhanced and knockdown of ELF-1 inhibited full activation of OAS1 by IFN stimulation. Collectively, ELF-1 binds an important duplicated GGAA cis-acting element at the OAS1 promoter and in cooperation with RB1 and SP1 recruitment contributes to regulation in response to IFN stimulation.

A duplicated GGAA motif in the human OAS1 promoter is required for effective IFN-mediated activation. The OAS1 gene is an important ISG encoding an enzyme with essential functions in anti-viral defense 26 . Even though an Interferon-stimulated response element (ISRE) is essential for the OAS1 gene to respond to IFN but alone it is not responsible for full activation 27 . Therefore, we focused on the role of duplicated GGAA motifs in regulation of ISG induction by IFNs, analyzing the contribution of this motif to OAS1 promoter activation. As depicted in Fig. 1, we have isolated a 541 bp region surrounding the reported TSS (accession number, NM_016816.2), which responds well to IFN stimulation (5 h), and examined its activity by Luciferase (Luc) reporter assay with serial deletion constructs of this region (Fig. 2). Deletion of the region containing the duplicated GGAA motif (− 423 to − 288) from the pGL4_OAS1 construct impaired the IFN-mediated promoter activation in both HeLa S3 and Jurkat cells. Cis-acting elements, such as in the promoters of ISGs are also responsible, at least in part, for the differential transcription profiles in response to IFN stimulation and hence the pleiotropic effects of IFNs 28 . Therefore, we speculate that the response may additionally originate from other GGAA (TTCC) containing elements, such as binding sites for STAT4, IRF-1 and ETS-family factors. The above result suggests that the deleted sequence from nucleotide − 423 to − 288 contains cis-acting element in the response to IFN-β and -γ . In order to determine the contribution of the duplicated GGAA motif to activation of the OAS1 promoter, the motif in the 541 bp region was disrupted to make the pGL4_OAS1mtdupGGAA construct (Fig. 2). This substitution comparatively inhibited IFN-induced promoter activation, indicating that the duplicated GGAA motif (− 326 to − 307; 5′ -gatctttccacttcctggtt-3′ ) is required for full promoter activation following IFN-treatment.
Sequence specific DNA-binding complexes at a duplicated GGAA motif in the OAS1 promoter.
To identify protein-DNA interactions at the duplicated GGAA motif (− 326 to − 307) in the OAS1 promoter, we performed competition and supershift EMSAs with nuclear extracts prepared from IFN-stimulated (5 h) HeLa S3 cells. Specific protein-DNA interactions occurred at − 340 to − 301 of the OAS1 promoter (OAS1 − 340/− 301) with nuclear extracts from IFN-α , -β and -γ HeLa S3 cells % ISG % Randomly selected gene % Humanized random DNA sequence Duplicated GGAA motif a 81 (47) 51.7 (30) 25 (15) No duplicated GGAA motif 19 (11) 48.3 (28) 75 (45) Total 100 (58) 100 (58) 100 (60)  3A). In contrast to the promoter activation shown in Fig. 2, protein-DNA complexes were detected with the labeled OAS1 − 340/− 301 probe in binding reactions containing nuclear extracts from IFN-α and -β treated cells. This apparent difference could be the result of differences in transcriptional activation and response between IFN-α and -β . It is possible that these differences were reflected in the nuclear extracts used for EMSA assay. Additionally, fully quantitative comparisons between different nuclear extract preparations are difficult, even though prepared simultaneously. While a lot of useful information can be gained from in vitro EMSA, such experiments may not always reflect the precise temporal and spatial distribution of transcription factors in cells. Inclusion of the unlabeled specific competitor duplex in the binding reaction prevented formation of several shifted bands, demonstrating specificity of these interactions (Fig. 3B, lanes 2 to 4), whereas no competition was observed with the unlabeled adjacent sequence (OAS1 − 379/− 331; Fig. 3B, lanes 5 and 6). Although higher molar excess was required, a randomly generated synthetic duplicated GGAA motif containing unlabeled competitor inhibited formation of the same complexes (Fig. 3B, lanes 7 and 8). A competition assay using mutated probes identified only the second GGAA motif (intact in mtTTCC1) as being essential for formation of the DNA-protein complexes but not the first GGAA motif (intact in mtTTCC2, Fig. 3C). These experiments indicate that the second GGAA motif, 5′ -acTTCCtg-3′ , in the OAS1 promoter is essential for binding of IFN induced factors. Fig. 1, in silico analysis suggested several putative transcription factors, including ELK-1, ELF-1 and c-ETS-1, which may bind to the second GGAA motif. Therefore, we assessed the possible DNA-protein interactions by EMSA supershift with the relevant antibodies (Fig. 3D). Only the inclusion of an antibody targeting ELF-1 but not other antibodies in the binding reaction disrupted the formation of the GGAA specific binding complex (Fig. 3D). Thus, either ELF-1 or an ELF-1-containing complex present in the IFN-β treated (5 h) HeLa S3 cell nuclear extract can either directly or indirectly interact with the duplicated GGAA motif at the OAS1 gene promoter. Additionally, a mobility shift band, representing ELF-1/OAS1 − 340/− 301 complex (Fig. 3F, lane 5) was generated with in vitro translated ELF-1 (Fig. 3E), which was not observed with the translation reaction from empty expression vector (Fig. 3F, lane 4). This complex was super-shifted by an anti-ELF-1 antibody (Fig. 3F, lane 6) and was only competed out with a specific unlabeled competitor duplex (Fig. 3F, lanes 7 and 8).  Consistent with the results in Fig. 3C, the competition analysis using in vitro translated ELF-1 also demonstrated specificity of binding to the second GGAA motif (Fig. 3F, lanes 9 and 10). Taken together, these results demonstrate the ability of ELF-1 to form a direct physical interaction with the second GGAA motif in the OAS1 promoter, which is in close proximity to the TSS. Additionally, a band of slightly faster mobility was seen with HeLa S3 nuclear extract when compared to in vitro translated ELF-1 protein (Fig. 3F, lanes 2 and 5, respectively), signifying that additional factors in the nuclear extract may contribute to the ELF-1/GGAA complex.

ELF-1 is an IFN-inducible transcription factor in HeLa S3 cells. As shown in
We developed a sensitive non-radioisotope in vitro transcription run-off assay (NITRA) to show initiation of transcription from various cis-acting regulatory elements. Here, the sequence requirements Site-directed mutagenesis of the wild type OAS1 promoter containing pGL4_OAS1 Luc reporter plasmid was used as a template for site directed mutagenesis to create a Luc reporter plasmid with a disrupted duplicated GGAA motif, designated pGL4_mtdupGGAA. These OAS1 reporter plasmids were transfected into HeLa S3 (A) or Jurkat (B) cells and 18 h later treated with IFN-α , -β , or -γ (100, 20 and 50 ng/ml, respectively) for 5 h, followed by Luc assay. Luc activity is shown relative to the expression of a Renilla luciferase control vector and error bars represent SD from three independent transfections. Comparisons between IFN-stimulated pGL4_OAS1 transfectants and either deletion or mutant dupGGAA were made by the student's t-test; *p < 0.1; **p < 0.05; ***p < 0.01.  Identification of an ELF-1 complex(s) that specifically binds to the duplicated GGAA motif in the OAS1 promoter. (A) Nuclear extracts derived from HeLa S3 cells, which were either treated with 100 ng/ml IFN-α , 20 ng/ml -β or 50 ng/ml -γ for 5 h (lanes 3, 4 and 5, respectively) or mock stimulated (lane 2), were subjected to EMSA with 3′ -end DIG labeled probe, human OAS1 − 340/− 301 (Table 2). (B,C) The specificity of binding complexes for GGAA motifs were determined by competition assays using unlabeled specific, non-specific competitors and mutated probes ( Table 2). The molar excess of unlabeled competitor DNA duplex is either indicated by × 25 or × 50.  Table 2 and used in this figure. for transcription from the OAS1 promoter was analyzed by NITRA using nuclear extract from IFN-β treated HeLa S3 cells as a source of active transcription factors (Fig. 4). Disruption of the duplicated GGAA motif drastically reduced initiation of transcription from SpeI/PvuII fragments of pGL4_OAS1 and pGL4_OAS1mtdupGGAA (Fig. 4A,B, compare lane 3 with 5). Although it was expected that the ELF-1 antibody would interfere with transcription from the OAS1 promoter, the absence of the ELF-1 binding site affected transcription efficiency. Multiple transcripts were detectable, being consistent with previous reports of multiple transcription start sites in ISGs and TATA-less promoters 29 . Taken together these results show that the ELF-1 binding site is important for initiation of transcription, in which ELF-1 binding to the upstream duplicated GGAA motif in the OAS1 promoter is strongly implicated.

Induction of ELF-1 enhances OAS1 transcription. When HeLa S3 cells were stimulated with
IFN-β from 0 to 24 h, rapid induction of ELF-1 transcription was seen within 30 min of stimulation (Fig. 5A, lane 2). Notably, the IFN-β induced transactivation of ELF-1 preceded accumulation of OAS1 mRNA, which reached a plateau at 8 h post-treatment (Fig. 5A, lane 5). Accordingly, an ELF-1 expression vector was transfected into HeLa S3 cells in increasing amounts, followed by RT-PCR analysis (Fig. 5C). Levels of OAS1 transcripts were substantially increased with ectopic expression of ELF-1, when compared to vector only transfected cells.
Western blot analysis indicated a 55 kDa band that was increased with increasing amount of transfection with ELF-1 expression plasmid (Fig. 5D), which is likely to be unmodified ELF-1 protein, whereas the previously reported 90 and 100 kDa bands 23 , which may represent phosphorylated and O-linked glycosylated ELF-1 are relatively unchanged. Induction of this faster migrating ELF-1 band was observed in HeLa S3 at 0.5 h after IFN treatment (Fig. 5B). ELF-1 was found to be predominantly nuclear with no apparent changes in sub-cellular localization following IFN treatment (data not shown). Santa Cruz C-20 is an affinity purified rabbit polyclonal antibody raised against a peptide mapping at the C-terminus of ELF-1, suggesting that the C-terminal region contains functional domain. Additionally, shRNA mediated knockdown of ELF-1 was carried out with three target sequences ( Fig. 5E; Supplementary table). Knockdown of ELF-1 resulted in reduced expression of OAS1 when compared to control vector-transfected

(B) NITRA indicates initiation of transcription from
SpeI/PvuII fragments of the pGL4_OAS1 or pGL4_OAS1mtdupGGAA plasmids. Templates were incubated with HeLa S3 nuclear extracts (HeLa NE), treated with IFN-β for 5 h, and then incubated in the presence of DIG-labeled dUTP, the de novo RNA transcripts were separated by denaturing PAGE and DIG-labeled RNAs were detected. An antibody targeting ELF-1 was included in the binding reactions (lanes 4 and 6). Non-specific bands (asterisks) originate from the ends of the template, which serve as an internal control.  (Fig. 5E). Collectively, ELF-1, whose expression is itself stimulated by IFN, may enhance rapid transcriptional activation of the OAS1 gene and protein levels in response to IFN.

ELF-1 enhances IFN-mediated OAS1 transactivation. Next the contribution of ELF-1 to OAS1
gene expression following IFN-stimulation of cells was addressed. When ELF-1 was overexpressed and then the cells were treated with IFN-β for 5 h, OAS1 gene expression was enhanced (Fig. 6A). Correspondingly, ELF-1 overexpression further enhanced IFN-induced OAS1 promoter activity in HeLa S3 cells in a dose-dependent manner (Fig. 6B) as determined by luciferase assay. Moreover, in ELF-1 knockdown cells diminished IFN-mediated activation of OAS1 expression in IFN-β stimulated cells was observed, to approximately half the level of control shRNA transfected cells (Fig. 6C). Taken together these data indicate a functional role for ELF-1 at the OAS1 promoter in its response to IFN stimulation.
IFN-β induces RB1 and SP1 recruitment to the OAS1 promoter and ELF-1 protein interaction with under-phosphorylated RB1 protein. As an ability of ELF-1 to form complexes with both SP1 and RB1 was previously demonstrated 24,30 , we therefore investigated the potential for these proteins to co-occupy with ELF-1 at the OAS1 promoter. Recruitment of ELF-1 to the OAS1 promoter was investigated by chromatin immunoprecipitation (ChIP) with antibodies targeting ELF-1, RB1 and SP1, followed by PCR analysis (Fig. 7A). As shown in lanes 5 and 7 respectively, ELF-1 and RB1 occupy a 390 bp region of the OAS1 promoter in mock treated cells, whereas very low occupation was observed by SP1 (lane 9). Strikingly, IFN-β treatment (2 h) resulted in increased recruitment of not only ELF-1 but also SP1 and RB1 to the region containing GGAA duplication (Fig. 7A, lanes 6, 8 and 10). Time-dependent recruitment of ELF-1 to the OAS1 promoter was then assessed by ChIP assay following IFN-β treatment (Fig. 7B). Immediate-early recruitment of ELF-1 was observed, peaking at the 30 min time point (Fig. 7B, lane 7) and gradually decreased over time. Using a DNA-affinity assay, we further observed that ELF-1 from IFN-β treated nuclear extracts can bind to the region containing the dupGGAA motif but also that SP1 can physically bind to the region immediately upstream of the OAS1 transcription start site (Fig. 7C). SP1 was found to bind in the region − 157 to + 115 nt, computational transcription factor binding site search did not reveal any putative SP1 binding sites. The biotin pulldown assay in Fig. 7C, shows a clear increase in pulldown of ELF-1 protein with probe A (which contains a known ELF-1 binding site) as compared to probe B (no known ELF-1 sites). However, it is not clear whether the fainter band seen for probe B represents the background level or additional lower affinity sites. Additionally, considering that ELF-1 and SP1 have been reported to physically interact, it is possible that indirect binding of these transcription factors was detected. Conversely, overexpression of SP1 in HeLa S3 cells repressed OAS1 transcription (Fig. 7D,E).
Subsequently we examined changes in the physical interactions between ELF-1 and RB1. As shown in Fig. 7F, co-precipitation of endogenous RB1 with ELF-1 was reduced in cell lysates from IFN treated cells (upper panel, lanes 7 and 8; lower panel lanes 5 and 6), demonstrating an IFN-dependent decrease in the ELF-1/RB1 interaction. Correspondingly, an in vitro pull-down with Myc-tagged ELF-1 demonstrated that under-phosphorylated RB1 was pulled down from HeLa S3 nuclear extracts when the cells were treated with IFN-β prior to extraction (Fig. 7G, lanes 7 and 8). Even though under-phosphorylated RB1 appeared to represent a small fraction of the total RB1 (undetectable in the input samples), this faster migrating band was seen with the addition of in vitro translated ELF-1 with HeLa S3 nuclear extract from IFN treated cells (compare lanes 7 and 8).

Discussion
Using transcriptional regulation of ISGs as a starting point, we have demonstrated that a specific DNA-binding complex(s) containing ELF-1 is co-recruited with RB1 and SP1 to a duplicated GGAA motif in the promoter of OAS1, one of the main IFN effector genes. We have demonstrated that disruption of a duplicated GGAA containing sequence approximately 300 bp from the OAS1 TSS resulted in a dramatic reduction of promoter activity. Although limited IFN response was retained, this remaining activity is presumably because of an intact ISRE, without which no activation can be observed 27 . Our data indicate the role of ELF-1 in OAS1 transcription is not a simple rate-limiting step, such as regulation by the ISRE. Similarly, knockdown of ELF-1 in IFN-stimulated cells also reduced the magnitude of IFN-mediated OAS1 induction. Such results are indicative of the duplicated GGAA motif constituting a proximal promoter, which exhibit low levels of transcription by themselves but are essential for the activity of enhancers and often function to loop distal regulatory regions to close proximity of the TSS 31 . The duplicity of GGAA motifs is a common occurrence in the promoter region of genes and the specificity of Ets binding factors to a particular GGAA-containing motif for each Ets family protein has been shown elsewhere 32 . Additionally, transcription factor binding sites often occur in close proximity to one another. A wide range of transcription factors could potentially bind sites containing a GGAA-motif. So it could be expected that additional unidentified factors can also bind this motif in addition to ELF-1, either co-operating or competing with ELF-1 depending on the cellular context. Our data show that only the second GGAA motif binds directly to ELF-1. Our results suggest that ELF-1 functions as an important adaptor molecule in modulation of the OAS1 transcriptional response to IFN stimulation.
GGAA motifs are frequently found in close proximity to the TSS of the majority of ISGs and may prove to be alternative sites for the initiation of transcription 33 , often overlapping with other transcription factor binding sites that helps coordinate gene regulation 34 . Regions containing multiple ETS-binding sites (GGAA) have been shown to be critical cis-acting sequences in gene regulation 35,36 . Our experiments clearly show that ELF-1 can specifically bind the OAS1 promoter sequence in vitro  and endogenous chromatin. However, the mechanism and role of ELF-1 may not be simply defined as a rate-limiting transactivation event, more than likely ELF-1 has a regulatory function. As pre-exposure to some specific cytokines dramatically affects how cells then respond to IFNs 37 , changes to constituents of the IFN-pathway should alter ISG activation patterns. Knockdown experiments suggested that ELF-1 has a positive effect on OAS1 regulation, affecting the degree of IFN response. Previous studies have reported unchanged mRNA and protein levels of ELF-1 in resting and stimulated T-cells 38 . However, in HeLa S3 cells a rapid (30 min) and transient induction of ELF-1 in HeLa S3 cells stimulated with IFN-β was observed, with no sustained up-regulation of ELF-1 protein levels. Raising the possibility that additional transcription factors are co-recruited to the OAS1 promoter by physically interacting with ELF-1.
Transcription factor binding to ETS-binding sites and paired co-activator sites may constitute proximal promoter elements in at least some of the 5′ flanking regions of ISGs. We found recruitment of RB1 and SP1 to the region containing the duplicated GGAA motif in the OAS1 promoter, despite the lack of putative binding sites. Physical interactions of ELF-1 with RB1 or SP1 24,30 may emerge as promising drug targets for precise modulation of the IFN response. RB1 is a well characterized tumor suppressor 39,40 and its loss of function is found in a large proportion of human tumors 41 . The NH 2 -terminal of ELF-1 (amino acids 21-72) binds the pocket domain of RB1. Interestingly, hyper-phosphorylation of RB1 disrupts complex formation demonstrated by overexpression of a phosphorylation-defective RB1 protein 24 . We have found that an ELF-1/underphosphorylated RB1 interaction is induced by IFN-stimulation. The cooperation between ELF-1 and RB1 in IFN stimulated cells suggests that ELF-1 recruits under-phosphorylated RB1 to the OAS1 promoter upon IFN stimulation. Overexpression of only SP1 had a moderate repressive effect on OAS1 gene expression in unstimulated cells, even though normal SP1 levels in HeLa S3 cells are high, the exogenously expressed SP1 is likely to be relatively unmodified with respects to post-translational modifications. This suggests that other co-factors such as ELF-1, in addition to SP1 may be needed to counteract the repressive effect of SP1 following IFN stimulation.
The classical JAK-STAT signal transduction pathway alone is not sufficient for generation of the full range of IFN-mediated effects. Instead, various signaling pathways mediate the biological functions of IFNs 42 . Differential responses of cell subtypes to IFNs are reported 9,10 , consistent with this and our present findings, ELF-1 may be involved in modulation of immune responses of particular cell types. The evidence presented here implies that recruitment of ELF-1 to the OAS1 promoter enhances the response to IFNs. The appropriate response to IFNs (dependent on cell type and existing cell state) might be determined by the availability of ELF-1 for transcriptional activation, competition with other GGAA-binding factors, post-translational modifications and changes in composition of ELF-1 complexes. Clearly, ELF-1 can occupy the OAS1 promoter in unstimulated cells, but a small increase in occupation was also observed following IFN stimulation. Taken together, these data permit speculation that an increase in cellular ELF-1 levels allows for a faster or greater IFN response because of this pre-occupancy. A possible mechanism for this is that in non-stimulated cells, either an ELF-1 or an ELF-1/SP1 complex and hyper-phosphorylated RB1, are dissociated or loosely associated with the OAS1 promoter and only basal transcription levels are observed. As ELF-1 and SP1 can physically interact in the absence of DNA, we envision that upon IFN-stimulation de-phosphorylation of RB1 protein occurs, which then permits RB1 to form a complex with ELF-1/SP1. Such mechanisms could at least partly account for why particular cells of the immune system respond to the exact same extrinsic signals in very different ways. Explicitly, the extracellular IFN signal is very broad and it is the capacity and availability of specific cellular factors, such as receptors, signaling molecules and transcription factors that determine IFN-mediated cellular responses. Therefore, future work is required to investigate whether ELF-1 is an additional key molecule in the IFN signal transduction pathway, acting as a general or specific transcriptional regulator of ISG expression. Our findings suggest that in addition to the essential JAK/STAT activation of ISGs, ELF-1 as well as other GGAA motif-binding factors should be taken into account when studying IFN-mediated cellular responses. Therefore, ELF-1 mediated regulation of OAS1 may represent one way in which cell type specific differences in IFN-responses could occur. That is, prevailing expression levels of transcription factors predispose the cell to a particular ISG expression pattern and specific IFN-response.
Obtaining a deeper understanding and further insights into the basic mechanisms required for effective gene expression in response to IFN will enable us to rationally design innovative therapeutic agents. IFN therapy is currently used for the treatment of some cancers, viral infections and immune were transfected with increasing amounts pcDNA3.1_SP1 expression plasmid or empty pcDNA3.1 plasmid for 24 hours. PCR amplification of cDNA was carried out with the indicated primer sets (Supplementary  Table). (F) RB1/ELF-1 interaction following IFN-β stimulation. HeLa S3 cells were treated with either mock (− ) or IFN-β (+ ) treated for 5 h, then subjected to co-immunoprecipitation with ELF-1, RB1 antibodies or normal mouse serum (NMS). The co-immunoprecipitated proteins were analyzed by Western blot. (G) Immunoprecipitation of proteins from Hela S3 nuclear extracts with in vitro translated Myc-tagged ELF-1. The binding reaction included in vitro transcription/translation reaction product from either empty pcDNA3.1Myc/his or pcDNA3.1Myc/his_ELF-1, and nuclear extract prepared from HeLa S3 cells mock treated or IFN-β treated (5 h). ELF-1 containing complexes were co-immunoprecipitated with c-Myc antibody for 2 h at 4 °C, and then detection of ELF-1 and RB1 by Western blot. diseases but the serious side effects [43][44][45] limit the number and spectrum of patients that may benefit from it. Although IFN-β therapy in multiple sclerosis is hailed as a breakthrough 12 , it is only partially effective and therefore greater advances on IFN therapy are required 13 . Recent reports have suggested a link between single nucleotide polymorphisms (SNPs) in the OAS1 gene that strongly contribute to the prognosis of the disease 46 , implying that OAS1 may play a fundamental role in the ability of IFNs to treat multiple sclerosis. GGAA-containing motifs and host ELF-1 have a demonstrated role in the gene transcription of the Human Immunodeficiency Virus 2 47 . Interestingly, ELF-1 has been identified as a cellular target of Epstein Barr Virus, which is associated with Burkitt's lymphoma 48 . ELF-1 is a predominant cellular factor that binds to the enhancer of the human T-cell leukemia virus type 1 (HTLV-1), the etiological agent of T-cell lymphoma/leukemia. Mutation analysis of this site markedly reduced inducible activity of the HTLV-1 enhancer 49 . Exploratory studies are required to understand the role of ELF-1 in anti-viral immunity, at present we speculate that targeting of ELF-1 in virus related diseases maybe useful as some viruses may have either evolved dependence on, or impede ELF-1 function. To conclude, understanding the action of IFN-β on the expression of OAS1 and other ISGs may help establish alternative and enhanced therapies, making IFN-derived treatments available for a wider spectrum of patients and diseases. This could be achieved by mimicking distinct IFN effects, for example by gene-therapy or small molecule compounds targeting protein-protein interactions in diseases where previously only treatment with IFNs has been effective.
Here we have identified sequence dependent binding of the ELF-1 transcription factor and a role in transactivation of the OAS1 promoter. We have provided additional supporting data that suggest the ELF-1 interacting partners, SP1 and RB1 proteins are also recruited to the OAS1 promoter. We are currently investigating in full the dynamics and contributions of SP1 and RB1 with ELF-1 in activation/ regulation of Interferon stimulated genes.

Methods
Bioinformatic analysis. For occurrences of duplicated GGAA motifs, genomic sequences − 500 to + 100 bp surrounding the putative TSS of ISGs were retrieved from the Ensembl database using the web-based Regulatory Sequence Analysis Tools (RSA-Tools; http://rsat.ulb.ac.be/) [50][51][52] . The DNA pattern search tool was utilized to search for the presence of the duplicated GGAA motifs with the following string descriptions: GGAAN{0,10}GGAA and GGAAN{0,10}TTCC; where N{0,10} indicates a spacer of between 0 and 10 nucleotides, results for both sense and anti-sense strands were retrieved. The results were then displayed graphically using the RSAT feature map tool. For comparison, two sets of control sequences were acquired, one of humanized random DNA sequences of 600 bp; and the second from − 500 to + 100 bp of the TSSs for the promoters of randomly selected human genes.
Cell lines, transfection and Luciferase assays. Jurkat and HL-60 cell lines cultured in RPMI 1640 medium and HeLa S3 cells in DMEM, were maintained at 37 °C/5% CO 2 . Culture media was supplemented with 10% FBS, 100 IU/ml penicillin and 100 μ g/ml streptomycin. For overexpression experiments, cells were transfected with expression plasmids using XtremeGene 9 transfection reagent (Roche Applied Science, Indianapolis, IN) according to the manufacturers' recommendations. Total amount of transfected plasmid DNA was adjusted to constant levels with empty parental vector. For multi well Luc reporter assays in 96-well plates, a DEAE-dextran based transfection method was used, as described previously 53 , cell lysate was prepared with 1× cell culture lysis reagent and subjected to Luc assay (Promega, Madison, IN). Table), containing KpnI and XhoI restriction sites with template cDNAs from HL-60 cells, and ligated into the multi-cloning site of pcDNA3.1Myc/His-B mammalian expression vector (Invitrogen, Carlsbad, CA). Sequencing of the ELF-1 ORF identified two SNPs in HL-60 derived ELF-1, which are reported in the NCBI dbSNP database (rs7799 and rs1056820). The resultant plasmids were designated, pcDNA3.1_ELF-1 and pcDNA3.1_SP1. pGL4 Luc reporter vectors (Promega) carrying the human OAS1 promoter and its deletions were constructed in the manner previously described 53 . Mutations were introduced using site directed mutagenesis of the pGL4_OAS1 plasmid based on 54 . Briefly, PCR was performed with opposing primers (Supplementary Table) containing the desired mutation and the entire plasmid was amplified using Phusion polymerase (Finnzymes oy, Vantaa, Finland) in high fidelity (HF) buffer, the parental hemi-methylated strand was digested with DpnI before being used for transformation of E. Coli. All plasmid constructs were confirmed by sequencing (FASMAC, Yokohama, Japan).

Construction of plasmids. The ELF-1 and SP1 open reading frames (ORF) and was amplified by PCR with primers, (Supplementary
Reverse transcription-PCR (RT-PCR) and real-time quantitative PCR. Total RNAs were isolated from cells using Isogen (Nippon Gene, Tokyo, Japan). The RNAs were quantified and equivalent amounts subjected to reverse transcription with ReverTra Ace (Toyobo, Tokyo, Japan), the resultant first strand cDNA was subjected to PCR using the gene specific primer sets (Supplementary Table) as indicated in figure legends. Amplification of GADPH cDNA was used as an internal control. For analysis of mRNA transcripts in shRNA-mediated knockdown experiments, real-time quantitative PCR was carried out using SYBR green real time PCR mix (Toyobo) and analyzed on ABI 7300 real-time PCR machine (Applied Biosystems). The efficiency of the primers in the PCR reactions was checked against a standard curve using serially diluted pooled cDNA. All reactions were performed in triplicate and normalized to GAPDH expression levels, calculations were performed using pyQPCR analysis suite (http://pyqpcr. sourceforge.net/) by the Δ Δ Ct method.
shRNA mediated gene knockdown. pGeneClip U1 hairpin expression vectors (Promega) containing either control (luciferase) or ELF-1 targeting shRNAs under the control of the U1 promoter were prepared following the manufacturers instructions. Transfected HeLa S3 cells were selected with Hygromycin B for 2 weeks before either mock or IFN treatment. Sequences for shRNA templates are shown in the Supplementary Table. Electrophoretic-mobility shift assay (EMSA) and DNA-affinity purification. Nuclear extracts were prepared from either mock or IFN treated cells essentially as previously described 55 . Duplex DNA probes were created by annealing partially complementary oligos, filling in the ends with Klenow fragment (Toyobo), and then end-labeled with digoxigenin (DIG) (Roche Applied Science), the sequences for duplex DNA probes and competitors are shown in Table 2. Binding reactions were carried out in; 0.2 mM EDTA, 20% Glycerol, 20 mM Hepes-KOH (pH7.9), 100 mM KCl, 1 mM DTT, 1 mM PMSF; for 15 min at 20 °C, the resulting reaction mixture was separated by native TBE-PAGE and transferred to a positively charged nylon membrane (PALL, Port Washington, NY) in 0.5× TBE buffer and UV cross-linked with a transilluminator. Detection of labeled DNAs was performed with an alkaline phosphatase conjugated anti-DIG antibody and CSPD ECL substrate (Roche Applied Science); chemiluminescence was detected using LAS 4000 imager (Fuji Film, Tokyo, Japan). For competition-EMSAs, a molar excess of unlabeled competitor probe was included in the binding reaction, as indicated in figure legends. In vitro transcription and translation of ELF-1 was carried out using the TNT quick coupled transcription/translation system (Promega), 3 μ l of translated protein was substituted for the nuclear extract where indicated. In vitro translated ELF-1 was confirmed by Western blot. Supershift-EMSAs were performed by incubating the binding reaction with the indicated antibody for an additional 45 min at 20 °C. For biotin-mediated DNA-affinity purification and detection of ELF-1 and SP1 by western blotting, 3′ -end biotin labeled dsDNA probes were prepared by incorporating biotinylated primers (Supplementary Table) during PCR amplification of the OAS1_pGL4 plasmid, followed by cleanup with a PCR purification kit (NipponGenetics). Biotinylated probes were bound to streptavidin beads, washed twice in EMSA binding buffer and then incubated with 32 μ g IFN-β treated HeLa S3 nuclear extract in the presence of 1 μ g poly dI:dC in 200 μ l of EMSA binding buffer for 50 min at 20 °C. The beads were then washed 3× with binding buffer containing 0.1% Tween-20 and bound proteins were eluted by boiling in 2× SDS sample buffer before being separated by SDS-PAGE and detected by Western blot analysis.
Immunoprecipitation and Western blot analysis. Western blot and immunoprecipitation were essentially carried out as described previously 56 . Briefly, cell lysates were separated by denaturing SDS-PAGE, transferred to Protran nitrocellulose membrane (Millipore, Billerica, MA) and immunoblotted with the following primary antibodies targeting RB1, ELF-1, Myc and an β -actin (Santa Cruz Biotechnology, Santa Cruz, CA) proteins, followed by secondary reaction with either horse radish peroxidase (HRP) or alkaline phosphatase (AP) conjugated anti-mouse or -rabbit IgGs (Calbiochem, Billerica, MA). HRP signals were detected by enhanced ECL substrate (Perkin Elmer, Boston, MA) and AP signals with BCIP/NBT (Sigma-Aldrich, St. Louis, MO). For preparation of nuclear and cytoplasmic cell extracts, fractions were prepared by lysing the cell membrane in 700 μ l buffer per 5 × 10 6 cells containing; 10 mM Tris.HCl (pH 7.5), 1 mM EDTA, 0.5% NP-40 and proteinase inhibitor cocktail (Sigma-Aldrich) on ice for 10 min, centrifugation at 10 000 × g and the supernatant (cytoplasmic extract) was recovered, the nuclear pellet was washed twice in lysis buffer and lysed in SDS-sample buffer. For immunoprecipitation of proteins from HeLa S3 nuclear extracts with in vitro translated Myc tagged ELF-1. The reaction included 10 μ l of TNT quick coupled in vitro transcription/translation (Promega) reaction product  Table 2. dsDNA duplex probes and competitors used for EMSA. a GGAA (TTCC) motifs are underlined. Only sense strand is shown.
with either empty pcDNA3.1Myc/his or pcDNA3.1Myc/his_ELF-1 as a template, 320 μ g nuclear extract prepared from HeLa S3 cells mock treated or IFN-β treated, in PBS to a final volume of 500 μ l, 1 mM DTT and 1× proteinase inhibitor cocktail (Roche Applied Science), incubated for 1 h at 4 °C. The ELF-1 containing complexes were immunoprecipitated with 2 μ g c-Myc antibody for 2 h at 4 °C, recovered by protein G sepharose beads and separated on a SDS-PAGE, followed by Western blot analysis.