Editing independent effects of ADARs on the miRNA/siRNA pathways
2009; Springer Nature; Volume: 28; Issue: 20 Linguagem: Inglês
10.1038/emboj.2009.244
ISSN1460-2075
AutoresBret S.E. Heale, Liam P. Keegan, Leeanne McGurk, Gracjan Michlewski, James Brindle, Chloë M. Stanton, Javier F. Cáceres, Mary A. O’Connell,
Tópico(s)CRISPR and Genetic Engineering
ResumoArticle27 August 2009Open Access Editing independent effects of ADARs on the miRNA/siRNA pathways Bret S E Heale Bret S E Heale MRC Human Genetics Unit, Institute of Genetics and Molecular Medicine, Western General Hospital, Edinburgh, UK Search for more papers by this author Liam P Keegan Liam P Keegan MRC Human Genetics Unit, Institute of Genetics and Molecular Medicine, Western General Hospital, Edinburgh, UK Search for more papers by this author Leeanne McGurk Leeanne McGurk MRC Human Genetics Unit, Institute of Genetics and Molecular Medicine, Western General Hospital, Edinburgh, UK Search for more papers by this author Gracjan Michlewski Gracjan Michlewski MRC Human Genetics Unit, Institute of Genetics and Molecular Medicine, Western General Hospital, Edinburgh, UK Search for more papers by this author James Brindle James Brindle MRC Human Genetics Unit, Institute of Genetics and Molecular Medicine, Western General Hospital, Edinburgh, UK Search for more papers by this author Chloe M Stanton Chloe M Stanton MRC Human Genetics Unit, Institute of Genetics and Molecular Medicine, Western General Hospital, Edinburgh, UK Search for more papers by this author Javier F Caceres Javier F Caceres MRC Human Genetics Unit, Institute of Genetics and Molecular Medicine, Western General Hospital, Edinburgh, UK Search for more papers by this author Mary A O'Connell Corresponding Author Mary A O'Connell MRC Human Genetics Unit, Institute of Genetics and Molecular Medicine, Western General Hospital, Edinburgh, UK Search for more papers by this author Bret S E Heale Bret S E Heale MRC Human Genetics Unit, Institute of Genetics and Molecular Medicine, Western General Hospital, Edinburgh, UK Search for more papers by this author Liam P Keegan Liam P Keegan MRC Human Genetics Unit, Institute of Genetics and Molecular Medicine, Western General Hospital, Edinburgh, UK Search for more papers by this author Leeanne McGurk Leeanne McGurk MRC Human Genetics Unit, Institute of Genetics and Molecular Medicine, Western General Hospital, Edinburgh, UK Search for more papers by this author Gracjan Michlewski Gracjan Michlewski MRC Human Genetics Unit, Institute of Genetics and Molecular Medicine, Western General Hospital, Edinburgh, UK Search for more papers by this author James Brindle James Brindle MRC Human Genetics Unit, Institute of Genetics and Molecular Medicine, Western General Hospital, Edinburgh, UK Search for more papers by this author Chloe M Stanton Chloe M Stanton MRC Human Genetics Unit, Institute of Genetics and Molecular Medicine, Western General Hospital, Edinburgh, UK Search for more papers by this author Javier F Caceres Javier F Caceres MRC Human Genetics Unit, Institute of Genetics and Molecular Medicine, Western General Hospital, Edinburgh, UK Search for more papers by this author Mary A O'Connell Corresponding Author Mary A O'Connell MRC Human Genetics Unit, Institute of Genetics and Molecular Medicine, Western General Hospital, Edinburgh, UK Search for more papers by this author Author Information Bret S E Heale1, Liam P Keegan1, Leeanne McGurk1, Gracjan Michlewski1, James Brindle1, Chloe M Stanton1, Javier F Caceres1 and Mary A O'Connell 1 1MRC Human Genetics Unit, Institute of Genetics and Molecular Medicine, Western General Hospital, Edinburgh, UK *Corresponding author. MRC Human Genetics Unit, Institute of Genetics and Molecular Medicine, Western General Hospital, Crewe Road, Edinburgh EH4 2XU, UK. Tel.: +44 131 467 8417; Fax: +44 131 467 8456; E-mail: M.O'[email protected] The EMBO Journal (2009)28:3145-3156https://doi.org/10.1038/emboj.2009.244 PDFDownload PDF of article text and main figures. ToolsAdd to favoritesDownload CitationsTrack CitationsPermissions ShareFacebookTwitterLinked InMendeleyWechatReddit Figures & Info Adenosine deaminases acting on RNA (ADARs) are best known for altering the coding sequences of mRNA through RNA editing, as in the GluR-B Q/R site. ADARs have also been shown to affect RNA interference (RNAi) and microRNA processing by deamination of specific adenosines to inosine. Here, we show that ADAR proteins can affect RNA processing independently of their enzymatic activity. We show that ADAR2 can modulate the processing of mir-376a2 independently of catalytic RNA editing activity. In addition, in a Drosophila assay for RNAi deaminase-inactive ADAR1 inhibits RNAi through the siRNA pathway. These results imply that ADAR1 and ADAR2 have biological functions as RNA-binding proteins that extend beyond editing per se and that even genomically encoded ADARs that are catalytically inactive may have such functions. Introduction The most common RNA editing event in human mRNA is deamination of adenosine to inosine. Proteins of the adenosine deaminases acting on RNA (ADAR) family catalyse this editing event. ADAR activity has been implicated in cancer, development, innate immunity and RNA interference (RNAi) (Patterson et al, 1995; George and Samuel, 1999; Beghini et al, 2000; Maas et al, 2001; Scadden and Smith, 2001; Hartwig et al, 2004; Luciano et al, 2004; Scadden, 2005; Scadden and O'Connell, 2005; Yang et al, 2005, 2006; Blow et al, 2006; Takahashi et al, 2006; Ohman, 2007; Paz et al, 2007; Kawahara et al, 2007a, 2007b; Cenci et al, 2008). In humans, the two most studied proteins of the ADAR family are ADAR1 and ADAR2. The ADAR1−/− mice are embryonic lethal with liver disintegration and a deficiency in erythropoiesis (Wang et al, 2000, 2004; Hartner et al, 2004). ADAR2 has been shown to be necessary for the editing of the GluR-B transcript at the critical Q/R site, which limits calcium entry through AMPA receptors. ADAR2−/− mice die around day p20 with seizures (Higuchi et al, 2000). ADAR1 and ADAR2 have similar domain structures (Figure 1D) but mainly display distinct editing site specificities—although their editing activities do overlap at some sites. There are two major isoforms of ADAR1 because of alternative promoter usage, the longer shuttling p150 isoform and the shorter nuclear p110 isoform. ADAR1 p150 is upregulated by interferon and can compete with PKR for double-stranded (ds)RNA. At the amino terminus ADAR1 p150 has two Z-DNA-binding domains and a nuclear export signal, which allows it to shuttle in and out of the nucleus, however it is predominantly found in the cytoplasm. Both isoforms have three dsRNA-binding domains, the third one overlaps with a nuclear localization signal (NLS) and the catalytic deaminase domain is at the carboxy terminus (Strehblow et al, 2002). ADAR1 is widely expressed throughout the body with the exception of skeletal muscle. ADAR2, on the other hand, is most highly expressed in the central nervous system, has two dsRNA-binding domains and a carboxy-terminal deaminase domain. It is localized to the nucleus by an NLS present in the N-terminal region (Desterro et al, 2003; Wong et al, 2003). To what extent each of the different domains of ADAR1 and ADAR2 contributes to their biological activities is an open question. Two other members of the ADAR family in vertebrates are catalytically inactive, ADAR3 that is brain specific and TENR that is expressed in the testis (Melcher et al, 1996; Connolly et al, 2005). Drosophila has a single Adar gene encoding a deaminase with the same domain structure as ADAR2. Adar mutant flies are viable with severe locomotion defects and loss of RNA editing in transcripts expressed in the CNS (Palladino et al, 2000a, 2000b). Figure 1.Editing levels in the human mir-376 cluster. (A) Diagram of the mir-376 cluster; nomenclature is from miRBASE http://microrna.sanger.ac.uk/sequences. Numbers at bottom indicate intervening lengths of sequences. Bold text regions are the mature microRNAs. Boxes indicate major sites of editing. There is no evidence of editing in mir-654. (B) Editing in mir-376a1 expressed from a complete mir-376 cluster. (C) Editing in mir-376a2. Ratio G/(A+G) indicates the ratio of the guanosine signal to the total (adenosine+guanosine) chromatogram signal. +4 and +44 are positions within mir-376a2 indicated in A. (D) ADAR1 and ADAR2 protein domains showing the positions and features used in the construction of the hADAR expression vectors. hADAR1 p150 contains two Z-DNA-binding domains, three dsRBDs and one deaminase domain. hADAR1 p110 begins at amino-acid position 296 of hADAR1 p150. hADAR2 has two dsRBDs and one deaminase domain. hADAR2 ΔN is a deletion mutant of hADAR2 with amino acids from positions 4–72 removed. A key glutamate residue in the deaminase domain is amino acid 912 for ADAR1 and 319 for ADAR2. Mutation of this residue to alanine renders the ADAR catalytically inactive. Download figure Download PowerPoint Mutations in human ADAR1 are associated with Dyschromatosis Symmetrica Hereditaria (DSH1) (Tojo et al, 2006), an autosomal dominant hyperpigmentation of the hands and feet occurring in Chinese and Japanese families. The majority of DSH1 mutations are associated with single allele truncations of ADAR1 and the dominant phenotype seems to be due to haploinsufficiency for ADAR1. The effect may arise in migrating neural crest cells that develop into melanocytes in the affected skin areas. The point mutant ADAR1 G1007R is an unusual example of a DSH1-associated variant that produces a full-length ADAR1 protein. On the basis of the known crystal structure of the ADAR2 deaminase domain (Macbeth et al, 2005) this mutant should not affect deaminase domain folding and the protein may be capable of RNA binding. However, the mutation introduces an additional positively charged arginine residue on the RNA-binding face of the deaminase domain very close to the active site and the DSH1 phenotype suggests that the ADAR1 G1007R protein may be catalytically inactive. dsRNA is required for both RNA editing by ADARs and RNAi. Thus, it is not surprising that there have been several reports of effects of ADARs in RNAi. Most of these studies have focused on the effect of the editing base change on processing of dsRNA or edited microRNA precursors (Scadden and Smith, 2001; Luciano et al, 2004; Scadden, 2005; Scadden and O'Connell, 2005; Yang et al, 2005, 2006; Blow et al, 2006; Ohman, 2007; Kawahara et al, 2007a, 2007b). More recent studies focused on the downstream effects on target selection by edited miRNAs. For example, it was recently shown that an miRNA predicted to target the PRPS1 transcript is edited by ADAR2 and, interestingly, levels of PRPS1 protein are elevated in ADAR2-deficient mice (Kawahara et al, 2007b). This result is the only demonstration so far that miRNA modulation of protein levels is altered by ADARs. There are several key steps in the miRNA pathway, which could be affected by ADARs (for review see Tomari and Zamore, 2005; Valencia-Sanchez et al, 2006). First, primary transcripts (pri-miRNA) are processed in the nucleus by the microprocessor complex, which contains Drosha and its partner DGCR8, to pre-miRNA hairpins (Gregory et al, 2004). Nuclear ADARs could therefore affect this step through steric hindrance of Drosha/DGCR8 binding or by inhibiting Drosha action through the alteration at the edited base in the primary miRNA transcript. As pre-miRNA hairpins can be bound by ADARs it is possible that their export from the nucleus, which is mediated by Exportin 5 (Yi et al, 2003), can be disrupted by binding. The next step in miRNA processing is the Dicer complex-mediated cleavage of the pre-miRNA hairpin into a 21–23 nucleotide RNA duplex in the cytoplasm. Cytoplasmic ADARs could also influence this step through sequestering the pre-miRNA or editing the pre-miRNA. Ultimately, the mature miRNA guide strand guides RISC to mRNAs that have complementarity with the guide strand, resulting in translation inhibition or mRNA degradation. ADAR antagonism of miRNA or siRNA production should result in alteration in the functional activity elicited by miRNAs or siRNAs. In this work, we sought to determine which properties of ADARs are responsible for influencing miRNA function. Specifically, we have examined the ability of several truncation and point mutations of ADAR1 and ADAR2 to alter the function of mir-376a2 in a cell culture system optimized for analysis of the activity of a single miRNA. Our results indicate that editing can result in retargeting of human mir-376a2 as shown earlier for murine mir-376 (Kawahara et al, 2007b). Interestingly, our results also show that even in the absence of editing, ADARs can affect the processing of miRNAs at the Drosha cleavage level step, thereby altering the functional activity of miRNAs. This suggests that ADARs may influence a larger set of miRNAs than would be predicted from the numbers that are known to be edited. We have also examined the ability of the human ADARs to alter silencing of the white+ eye colour gene in Drosophila by a 300plus base-pair hairpin, which is processed into siRNA duplexes (Vagin et al, 2006). We again find that a deaminase-inactive ADAR can antagonize siRNA activity against white+. Therefore, RNA binding by itself is an important function of ADAR biology. Results Editing of the mir-376 cluster by ADAR isoforms shows asymmetric editing in pri-mir-376a2 The human mir-376 cluster comprises several miRNA hairpins encoding mir-376c, mir-376a2, mir-654, mir-376b and mir-376a1 and others (Figure 1A). It was reported earlier that in human medulla several of the adenosines in this cluster are edited (Kawahara et al, 2007b). To elucidate whether particular domains of human ADAR1 or ADAR2 have prominent roles in the effect of ADARs on miRNA function, we cotransfected HEK 293T cells with constructs that express the mir-376 cluster and with constructs that express individual human ADAR1 or ADAR2 isoforms (Figure 1D summarizes key features of ADAR1 and ADAR2). All mutant proteins were expressed to the same level as the respective wild-type protein, as detected on immunoblots probed with anti-FLAG monoclonal antibody (data not shown). HEK 293T cells do not express detectable levels of the endogenous cluster. RNA editing levels were examined initially, before endeavouring to examine the effects of these ADAR variants on precursor processing and effects on downstream microRNA targets. RNA was extracted from transfected cells, reverse transcribed with random hexamers and cDNA corresponding to individual pri-mir-376 hairpins were amplified using primers located around a 100 nucleotides before and after each hairpin within the long intervening sequences between the hairpins. RNA editing levels at sites within the pri-mir-376 hairpins were measured from mixed sequence chromatograms on the amplified sequence pools for each pri-mir-376 hairpin. We found that sites in pri-mir-376 hairpins were highly edited, as reported earlier for human medulla (Kawahara et al, 2007b). The different specificities of ADAR1 and ADAR2 account for the different patterns of editing in the pri-mir-376a1 (Figure 1B), -376a2 (Figure 1C) and -376b hairpins (Kawahara et al, 2007b). For instance, ADAR2 edits pri-mir-376a1 at the +4 and +44 site more efficiently than ADAR1 (Figure 1B). In contrast, the two naturally occurring isoforms of ADAR1, p150 and p110, showed similar efficiencies at a range of sites within pri-miR-376a1, with the nuclear ADAR1 p110 editing slightly more efficiently in all cases (Figure 1B). The larger isoform has an extended amino terminus that encodes Z-DNA-binding domains that can bind to dsRNA (Oh et al, 2002; Koeris et al, 2005; Placido et al, 2007). The editing sites that showed the strongest preferences for editing by a particular ADAR occurred in pri-mir-376a2, where hADAR2 preferentially edited the +4 site of the mature 5′ miRNA with 80–90% efficiency. ADAR1 edits this site with 40% efficiency (Figure 1C). By contrast, hADAR1 edits the +44 site within the mature 3′ miRNA with 80–90% efficiency whereas ADAR2 edits this site with only 10% efficiency. This is in contrast with the editing of miR-376a1 at the +44 site as described above (Figure 1B). RNA editing sites in other microRNA precursors within the cluster show less specificity for ADARs, the +44 site of pri-mir-376b was edited by both hADAR1 and hADAR2 (data not shown). As observed earlier in human medulla RNA, mir-654 was not edited in HEK 293T cells cotransfected with ADAR. As anticipated, cotransfection of the ADAR1 1-296 construct that expresses only the first 296 residues, containing the first Z-DNA-binding domain of ADAR or the ADAR1 1-442 construct containing both Z-DNA-binding domains did not increase RNA editing. On the other hand, cotransfection with the ADAR1 443-end construct that expresses a protein lacking both Z DNA-binding-domains gave levels of RNA editing similar to intact ADAR1 p110. To determine whether editing activity is critical for effects of ADARs on microRNA processing and/or function we tested the effects of two ADAR1 mutant proteins. First, a construct with a glutamate to alanine change in an essential catalytic site residue (ADAR1 E912A) was shown to cause only background levels of RNA editing similar to that seen with cotransfection of the control pcDNA3.1 construct. We also cotransfected a construct expressing the naturally occurring G1007R mutation in ADAR1 that has been linked to DSH1 with the construct expressing the mir-376 cluster and found that this protein is incapable of editing any sites in the microRNA precursors. This protein, expressed in and purified from the yeast Pichia pastoris binds long dsRNA similarly to wild-type ADAR1 as assayed by filter binding but does not deaminate long dsRNA (Supplementary Figure S1). ADAR2 ΔN is a deletion of ADAR2 amino acids 4–72 that removes the nuclear localization sequence and causes active ADAR2 to accumulate in the cytoplasm (Wong et al, 2003). Surprisingly, the ADAR2 ΔN isoform edited the pri-miRNA, which is normally found only in the nucleus (Figure 1B and C). The observed editing by the cytoplasmic ADAR2 ΔN is due to editing of the pri-miRNA transcripts that escaped to the cytoplasm without being cleaved by the Drosha complex in the nucleus (Supplementary Figure S2). ADAR2 shows strong inhibition of miRNA activity As the RNA editing sites in mir-376a2 show the highest levels of preference for editing by ADAR1 or ADAR2 within the entire miR-376 cluster, we generated a construct that expresses pri-mir-376a2 alone. This allows the effects of ADAR2 binding and editing at the +4 site and ADAR1 binding and editing at the +44 site to be studied in the absence of other microRNAs that have strong sequence similarities. We verified that the editing of mir-376a2 alone was the same as editing of mir-376a2 expressed in the intact cluster (Supplementary Figure S3A). Processing of pre-mir-376a2 by the miRNA processing machinery produces mature 5′ and 3′ microRNAs. To determine how the production and the specific targeting of the mature microRNAs is affected by the presence of ADARs we measured RNA-silencing activities with two sets of luciferase constructs containing full-length microRNA target sites in the 3′ UTR regions of the luciferase transcripts (Supplementary Figure S3B). The 5′ miR luciferase reporter and the 3′ miR luciferase reporters measure the luciferase-silencing activity of the corresponding wild-type mature unedited microRNAs. The use of target sites with perfect homology extending beyond the seed match may lead to site-directed cleavage of the target transcript as well as translational inhibition. When ADARs edit within miRNAs they have the potential of retargeting miRNAs to another transcript. The RNA-silencing activities of the mature microRNAs retargeted as a result of editing are measured using a second pair of luciferase reporters with single base changes in the target sites (Supplementary Figure S3B). We found that mir-376a2 expressed and processed in the absence of cotransfected ADAR constructs generated substantial silencing activities corresponding to the mature, unedited 5′ and 3′ miRs, as expected, (Supplementary Figure S3B), reducing luciferase levels 10-fold to approximately 0.1 of the value obtained in the absence of the miRNA. We optimized the level of mir-376a2-expressing construct so that it was sufficient to obtain this maximal level of silencing for both microRNAs. Expression of the mir-376a2 construct in the absence of ADARs produced much less silencing activity directed against the reporters for the edited microRNAs, reducing the luciferase levels by only approximately two-fold, to approximately 0.5 of the value obtained in the absence of the miRNA (Supplementary Figure S3B). This five-fold discrimination by the mature unedited microRNAs between the unedited and the edited target sites is highly specific, considering that the edited target sites in each case differ by only 1 nucleotide in the 22 base sequences. Having established conditions to maximize silencing activities of mature miRNAs from the transfected pri-mir-376a2 construct and to determine their target site preferences we cotransfected the mir-376a2 reporter with constructs expressing ADARs and ADAR mutations to assess how ADARs affect the silencing activities of resulting miRNAs. Consistent with their editing of pri-mir-376a2 at position +44, both hADAR1 p110 and hADAR1 p150 increased the silencing activity corresponding to the edited form of the 3′ miR (Figure 2B). This change was largely editing dependent, as the deaminase mutant ADARs (ADAR p150 E912A and ADAR p110 E912A) did not have this effect (Figure 2B); the effect was not dependent on the Z-DNA-binding domains of ADAR1 (ADAR1 443-end). Further, the Z-DNA-binding domains of ADAR1 (ADAR1 1-442) were not sufficient on their own to significantly increase the silencing activity of edited 3′ miRNA. Figure 2.Effects of ADARs on functional activities of mature miRNAs processed from pri-mir-376a2. (A) Inhibition of 3′ miRNA activity. A value more than 1 means that the miRNA is less active when the ADAR is present than when the pri-mir-376a2 is expressed alone. (B) Retargeting of 3′ miRNA activity. A value less than 1 means that the miRNA is more active in the presence of the ADAR than when the pri-mir-376a2 is expressed alone. Pre-edited mir-376a2 (a177g) indicates a construct expressing pri-mir-376a2 with the +44 site (position 177) mutated from an adenosine to a guanosine. (C) Inhibition of 5′ miRNA activity. (D) Retargeting of 5′ miRNA activity. The activity for pre-edited mir-376a2 (a137g) is from a construct expressing pri-mir-376a2 with the +4 site (position 137) mutated from an adenosine to a guanosine. Download figure Download PowerPoint Notably, it was ADAR2 that produced the most striking inhibitory effects on miRNA function, particularly on the activity of the unedited miRNAs (Figure 2A and C). ADAR2 edits the pri-mir-376a2 at position +4 and thereby increases the silencing activity of edited 5′ miR (Figure 2D), at the expense of unedited 5′ mir activity (Figure 2C). As ADAR2 edits the +4 site in pri-mir-376a2 with 90% efficiency it is surprising that the retargeting effect was not more complete. Silencing of the reporters for edited microRNAs was maximized by cotransfecting equivalent amounts of mir-376a2 constructs bearing A–G point mutations at the RNA editing sites so that the mature miRNAs were ‘pre-edited’ to mimic the inosine-containing product. Cotransfecting a pri-mir-376a2 construct pre-edited at the +4 site gives a silencing activity corresponding to the edited 5′ miRNA that was almost twice as great as seen with ADAR2 (Figure 2D). A possible explanation is that ADAR2 edits pri-mir-376a2 very efficiently but that it also slows Drosha processing of the pri-mir-376a2 so that less mature miRNA is produced. The hypothesis that ADAR2 inhibits Drosha processing of pri-mir-376a2 is supported, first, by the fact that ADAR2 inhibits the activity of the 3′ miRNA even though it edits the +44 site within this miRNA with only 10% efficiency. Second, the cytoplasmic protein ADAR2 ΔN has no effect either on activity or on retargeting of the 3′ micro RNA (Figure 2A and B). This is consistent with a nuclear inhibition of Drosha being responsible for the ADAR2-mediated inhibition of 3′ miR activity. ADAR2 ΔN did affect the activity of the 5′ miRNA and increased the activity of the edited form. This appears to be due to base deamination and it does not suggest further cytoplasmic influence of ADAR2 on cytoplasmic processing steps. ADAR2 ΔN, which is cytoplasmic, edits the Drosha product, the pre-miRNA, after it is exported to the cytoplasm (Figure 2 and Supplementary Figure S2). Drosha processing of pri-mir-376a2 is inhibited by ADAR2 protein and not by the RNA editing base changes As mentioned earlier ADAR interactions with miRNAs can occur at all levels of the miRNA processing pathway. We examined the processing of pri-mir-376a2 in transfected cells by northern analysis (Figure 3A and B; Supplementary Figure S4). ADARs were expressed in HEK293T cells in the presence of the mir-376a2 expression construct and the appropriate reporter construct. Only ADAR2 caused a significant reduction in the mature ∼22-nucleotide miRNA and in the ∼64-nucleotide pre-miRNA, with a reduction of over 65% in both cases. This indicates that ADAR2 activity on the pri-mir-376a2 hairpin disrupts Drosha processing in the nucleus. In further support of this hypothesis, ADAR2 ΔN, a cytoplasmically localized mutant of ADAR2, did not cause a significant reduction in the levels of either the pre-miRNA or the mature miRNA. Figure 3.Effects of ADARs on processing of pri-mir-376a2. (A, B) Effects of ADARs on processing in HEK 293T cells. Small RNA northern on RNA from cotransfected HEK 293T cells probed with antisense probes to (A) the 3′ miRNA and (B) the 5′ miRNA. Nothern blots were also probed with a 5S rRNA-specific probe as a loading control (data not shown). ADAR2 expression reduced both the pre-miRNA and the mature 3′ and 5′ miRNA signals. The numbers below the blot indicate the amount of both pre-mir-376a2 or mature 376a2 signal in each lane relative to that in pri-mir-376a2 expressed alone. (C) Recombinant ADAR2 inhibits Drosha cleavage in HeLa extracts in vitro. Drosha cleavage assays performed in the presence of recombinant ADAR2 and either pri-let-7a-1 or pri-mir-376a2. A double plus in the ADAR2 table indicates that a higher amount of ADAR2 was added. Cleavage of pri-mir-376a2 but not pri-let-7a-1 was inhibited by ADAR2, indicating that ADAR2 directly and specifically effects Drosha processing of mir-376a2. The percentage of pre-miRNA and mature 376a2 signal relative to cleavage in the absence of ADAR2 is indicated below the blot. (D) Lack of effect of RNA editing base changes in pri-mir-376a2 on Drosha cleavage in HeLa extracts in vitro. Drosha cleavage was not impaired by point mutations mimicking RNA editing events in mir-376a2. a137g mimics editing of the +4 site. a177g mimics editing of the +44 site. c188t closes the A–C mismatch at the +4 site in pri-mir-376a2. The amount of pre-miRNA signal relative to wild-type pri-mir-376a2 cleavage is indicated below the blot. Download figure Download PowerPoint By performing in vitro pri-miRNA processing assays with HeLa nuclear extract we found that the addition of purified ADAR2 specifically inhibited Drosha processing of pri-mir-376a2 but not pri-let-7a-1 (Figure 3C), though some pre-mir-376a2 is still produced. To determine whether Drosha cleavage in the HeLa nuclear extract is inhibited by the RNA editing base changes or by binding of ADAR2, in vitro transcribed mutant pri-mir-376a2 transcripts bearing adenosine to guanosine changes at the edited positions were assayed. Specifically, in mir-376a2 a137g, a guanosine replaced adenosine at the +4 position and in mir-376a2 a177g, a guanosine replaced adenosine at the +44 site that is the +6 position of the 3′ miR. Importantly, Drosha cleavage was not affected by either mutation (Figure 3D), clearly showing that the nucleotide changes mediated by editing are not themselves sufficient to inhibit the processing of mir-376a2. The c188t construct that removes the A-C mismatch at the +4 site also had no effect. Catalytically inactive ADAR2 disrupts pri-mir-376a2 processing To confirm that inhibition of Drosha cleavage is due to ADAR2 binding rather than because of the base change at the edited site an active site-mutant ADAR2 E319A was co-expressed. ADAR2 E319A retained the ability to reduce the silencing activity of unedited 5′ miR but, as expected, it was unable to retarget the silencing activity (Figure 4A). Furthermore, ADAR2 E319A caused inhibition of the processing of pri-miRNA-376a2, as detected on small RNA northerns with RNA from cotransfected cells (Figure 4B). ADAR2 E319A disruption of Drosha processing verifies the conclusion that ADAR2 interference with miRNA processing is independent of editing. ADAR2 ΔN E319A, a deaminase domain mutant localized to the cytoplasm, did not inhibit 3′ miR activity and only weakly affected 5′ miR activity (Figure 4A). This shows further that it is nuclear Drosha cleavage that is affected and not cytoplasmic Dicer activity. Figure 4.Deaminase-inactive ADAR2 fails to retarget miRNAs but still inhibits their processing. (A) Top panel: effects of normal versus deaminase mutant ADAR2 on production of mature unedited and edited miRNA activities. Inactive ADAR2 E319A retained the inhibitory effect of ADAR2 on the unedited 5′ miRNA activity but was unable to retarget the activity by editing. Bottom panel: effects of cytoplasmic ADAR2 ΔN and ADAR2 ΔN E319A on the activity of mir-376a2. ADAR2 ΔN E319A did not affect the 5′ reporter, indicating a loss in retargeting. Neither hADAR2 ΔN nor hADAR2 ΔN deaminase mutant affected the 3′ mature miRNA activity. (B) Effect of ADAR2 E319A on processing of mir-376a2 in cotransfect
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