Alternative mRNA Splicing of Corepressors Generates Variants That Play Opposing Roles in Adipocyte Differentiation*

Background: The SMRT and NCoR corepressors play key biological roles in transcriptional repression. Results: Alternative mRNA splicing produces corepressor variants that can exert opposite effects on adipocyte differentiation. Conclusion: Corepressors are diversified by alternative mRNA splicing, allowing one locus to encode multiple proteins with distinct functions. Significance: Changes in alternative splicing may help drive the differentiation and customize the physiology of specific cell types. The SMRT and NCoR corepressors partner with, and help mediate repression by, a wide variety of nuclear receptors and non-receptor transcription factors. Both SMRT and NCoR are expressed by alternative mRNA splicing, resulting in the production of a series of interrelated corepressor variants that differ in their tissue distribution and in their biochemical properties. We report here that different corepressor splice variants can exert opposing transcriptional and biological effects during adipocyte differentiation. Most notably, the NCoRω splice variant inhibits, whereas the NCoRδ splice variant promotes, adipogenesis. Furthermore, the ratio of NCoRω to NCoRδ decreases during adipogenic differentiation. We propose that this alteration in corepressor splicing helps convert the cellular transcriptional program from one that maintains the pre-adipocyte in an undifferentiated state to a new transcriptional context that promotes differentiation and helps establish the proper physiology of the mature adipocyte.

We report here a dissection of the specific roles that individual SMRT and NCoR splice variants play in regulating the 3T3-L1 adipogenesis pathway. Our results indicate that the different corepressor variants are expressed at different levels in pre-adipocytes and that the relative abundance of certain variants changes as these cells differentiate into terminal adipocytes. We determined that these different corepressor variants display disparate affinities for the nuclear receptors that regulate adipogenesis, and, most notably, certain corepressor variants accelerate, whereas others suppress 3T3-L1 differentiation. Consistent with these divergent effects on the overall adipogenesis program, different corepressor variants regulate distinct panels of target genes. Our results indicate that alternative splicing of the SMRT and NCoR corepressors serves to diversify their biological functions, with different splice variants serving different roles in adipogenesis. Furthermore, we propose that programmed alterations in corepressor splicing may help switch the transcriptional environment from one that maintains the pre-adipocyte in an undifferentiated state to a new transcriptional context that permits differentiation and helps establish the proper physiology of the mature adipocyte.

EXPERIMENTAL PROCEDURES
Plasmids-The plasmid pFN21Ahyg-EGFP was created by first introducing the enhanced green fluorescent protein coding sequence from pEGFP-C1 (GenBank TM accession number U55763) into the mammalian HaloTag expression plasmid, pFN21A (Promega, Madison, WI), using PCR to add the required SgfI and PmeI sites to EGFP. The CMV promoterdriven hygromycin resistance cassette was then cloned from pCI-hygro into the AgeI and PciI sites of pFN21A-EGFP using PCR to add the required restriction site sequences and an additional SwaI site at the 3Ј end of the of the hygromycin resistance cassette to facilitate linearization of the plasmid prior to transfection. HaloTag fusion protein versions of full-length corepressor isoforms were created using PCR to add the required SgfI and PmeI restriction sites to the open reading frame of each corepressor isoform and subsequently cloning into pFN21Ahyg-EGFP, removing the GFP encoding DNA fragment.
Cell Culture and Stable Transfection of 3T3-L1 Cells-Undifferentiated murine 3T3-L1 cells were grown in DMEM containing 9% newborn calf serum (JR Scientific, Woodland, CA) at 37°C and 5% CO 2 . Cells were passaged or re-fed every 3 days and never allowed to reach Ͼ80% confluence prior to differentiation. Stable 3T3-L1 transformants were created by transfecting 5 ϫ 10 4 3T3-L1 cells/35-mm plate with 2.5 g of SwaI-linearized pFN21Ahyg-EGFP, pFN21Ahyg-NCoR␦, or pFN21Ahyg-NCoR, using 7.5 l of TransIT-LT1 (Mirus Bio, Madison WI) according to the manufacturer's protocol. After 24 h the transfected cells were trypsinized and plated into a 100-mm plate. After an additional 24 h, hygromycin B was added to a final concentration of 500 g/ml. Media (containing 500 g/ml hygromycin B) was replenished every 7 days until visible colonies formed. After colony formation was observed, cells were passaged to a new 100-mm plate and grown until the cells reached ϳ80% confluence, at which point the cells were plated for differentiation.
Oil Red O Staining and Quantification-Differentiated 3T3-L1 transformants (day 8) were fixed and stained with Oil Red O to visualize lipid accumulation (91). Cells were then counterstained with hematoxylin. The extent of Oil Red O staining was quantified from multiple microscopic fields (n Ն 6) of each transformant using the Color Threshold and Analyze Particle functions of NIH ImageJ (version 1.45k) (92). The means Ϯ S.E. of multiple microscopy fields from three independent transformants of NCoR␦, NCoR, and GFP were plotted.
Cell Proliferation Analysis-The growth rate of 3T3-L1 stable transformants was analyzed using CellTiter 96 Aqueous One Solution (Promega). Stable corepressor isoform (or GFP) 3T3-L1 transformants were plated at 1 ϫ 10 3 cells/well in replicate wells of a 96-well plate. Cell proliferation was measured 24 and 48 h after plating according to the manufacturer's protocol. Media on the remaining wells was replaced after 48 h, and cell proliferation was measured in the remaining wells 72 and 96 h after plating.
GST Pulldown Assays-Glutathione S-transferase fusion proteins with the receptor interaction domains of SMRT (amino acids 1851-2473 of SMRT␣ (GenBank TM accession number AF113001) or equivalent) and NCoR (amino acids 1817-2453 of NCoR (GenBank TM accession number U35312) or equivalent) were expressed in Sf9 cells using the Bac-to-Bac baculovirus expression system (Invitrogen, Carlsbad, CA). Whole cell extracts were prepared from ϳ3 ϫ 10 8 infected Sf9 cells grown in 50 ml of suspension culture using Insect-XPRESS (Lonza, Walkersville, MD) medium containing 9% fetal bovine serum. Three days after infection, Sf9 cells were collected, rapidly frozen in liquid nitrogen, and thawed on ice before resuspending in WCE buffer (20 mM HEPES (pH 7.9), 200 mM KCl, 1 mM EDTA, 0.5% IGEPAL CA-630, 10% glycerol, 1 mM dithiothreitol, 1ϫ Complete Protease Inhibitor mixture (Roche Applied Science)). Resuspended cells were again frozen in liquid nitrogen and thawed on ice. Lysates were cleared by centrifuging at 14,000 ϫ g for 5 min at 4°C. In vitro "GST pulldown" protein-interaction assays were preformed as previously described (93).
RT-PCR Analysis of Corepressor Isoform Expression-RNA for corepressor isoform RT-PCR and quantitative RT-PCR was isolated using TRIzol reagent (Invitrogen) according to the manufacturer's protocol. Complimentary DNA (cDNA) was synthesized from 1 g of total RNA using a Quantitect Reverse Transcription kit (Qiagen). For corepressor isoform analysis, cDNA equivalent to 12.5 ng of RNA was amplified for 32 cycles using GoTaq DNA polymerase (Promega) and the primer sets in supplemental Table S1A. PCR products were visualized using ethidium bromide and a 1.5% agarose/TAE gel and quantified using an Alpha Innotech Fluorchem 8900 and AlphaEase software (version 3.1.2).
Quantitative PCR Assay for Adipogenic Gene Regulation-Analysis of gene expression in pre-and post-differentiated 3T3-L1 cells was performed by quantitative RT-PCR using an Opticon2 real-time thermal cycler, SsoFast EvaGreen Supermix (Bio-Rad, Hercules, CA) and the primer sets listed in supplemental Table S1B. Expression levels are expressed relative to the Day 0 GFP samples and normalized to ␤2-microglobulin expression. The means Ϯ S.E. of normalized relative expression values from three independent stable transformants were plotted.
Mouse Embryonic Fibroblast Isolation-Embryonic fibroblasts (MEFs) from wild-type C57BL/6 and transgenic mice engineered to only express the exon 37bϪ form of NCoR were isolated according to the method developed by Todaro and Green (94).

RESULTS
The Relative Abundance of the Different Corepressor Splice Variants Differs in Different Tissues and Cell Lines-The mRNA transcripts from both the SMRT and the NCoR loci are subject to alternative splicing (18,(63)(64)(65)(66)(67)(68)(69)(70); the NCoR and SMRT splice variants that are the focus of this study are indicated in Fig. 1. These alternative splicing events are particularly extensive within the cRID regions of these corepressors and can generate NCoR variants that contain two or three distinct cRID domains, and SMRT variants that contain one, two, or three cRIDs, plus an additional SMRT variant in which the regions flanking RID1 have been deleted while preserving the interaction motif itself (Fig. 1). Additional alternative splicing events occur within the N-terminal and central regions of the corepressors that may alter docking surfaces for other components of the corepressor complex. Our nomenclature refers to both the specific splicing events that occur at the individual exons (e.g. whether SMRT exon 40bϪ or 40bϩ is utilized) and to how these individual splice events are assembled together into the final mRNA/open reading frame (e.g. SMRT is defined as the product of the assembly of exon 28ϩ, 40bϩ, and 47bϩ). Notably, splicing at each splice site appears to not influence that at other splice sites (68).
We employed RT-PCR and primers that flank these alternative splice sites to determine the relative utilization of these different splicing events in different mouse tissues (Fig. 2). Certain alternative mRNA splicing events occurred at approximately the same frequency in all tissues examined; for example, the ratio of the SMRT 28ϩ to 28Ϫ splice form was near identical across all samples tested. Other alternative mRNA splicing events proved to be highly tissue-specific. For example, inclusion of the SMRT 40bϩ exon (and its encoded RID3) prevailed in the splicing pattern in brain and testes but was relatively rare in other tissues (Fig. 2). Inclusion of the NCoR 37bϩ exon, which encodes an RID3 related to that in the SMRT 40bϩ exon, generally paralleled the SMRT 40bϩ tissue expression pattern (Fig. 2). Reciprocally, the SMRT 47bϪ splice (which deletes flanking sequences from the S1 CoRNR box in RID1) was rare in brain and testes, but high in heart, spleen, lung, skeletal muscle, and adipose tissue (Fig. 2). Significantly, the SMRT and NCoR sequences that are generally considered to be the prototypes for these corepressors are not necessarily the most abundant or most widely expressed splice forms. For example, the 37bϩ NCoR variant, which encodes three cRIDs, is frequently cited and employed experimentally as the NCoR prototype; however, NCoR is strongly expressed only in brain and testes, whereas NCoR␦, which contains only two cRIDs, predominates in all other tissues tested (Fig. 2).
Differentiation of Pre-adipocytes to Adipocytes Is Associated with a Shift from the 37bϩ to 37bϪ NCoR Splice Variant-We next extended our RT-PCR analysis to 3T3-L1 cells, a widely used ex vivo model of adipogenesis (72) (Fig. 3). Although the pattern of corepressor variants expressed in the 3T3-L1 preadipocytes generally paralleled that observed in white adipose tissue in vivo, the ratio of the NCoR 37bϩ splice to that of the 37bϪ splice was significantly higher in the former (Fig. 2). Notably, however, inducing differentiation of the 3T3-L1 cells into terminal adipocytes progressively reduced the ratio of the NCoR 37bϩ splice to the 37bϪ splice over the 8-day differentiation period to more closely resemble that observed in differentiated white adipose tissue in vivo (Fig. 3A). This was also true in response to rosiglitazone, a PPAR␥ agonist known to enhance 3T3-L1 adipogenesis (Fig. 3B). The relative expression of the other corepressor variants examined was either minimally altered (e.g. SMRT 40bϩ/40bϪ) or not significantly altered under the same conditions. We conclude that adipocyte differentiation is accompanied by a decrease in the ratio of NCoR corepressor splice forms that include RID3 versus those that do not.

Different SMRT and NCoR Splice Variants Possess Different Affinities for the Different Nuclear Receptors Involved in
Adipogenesis-The differentiation and subsequent function of adipocytes are tightly regulated through a network of nuclear receptors; we therefore next examined the ability of the different splice forms of SMRT and NCoR to interact with the different members of this network; we tested these first in the absence of ligand (Fig. 4, solid bars; additional statistical analysis is presented in supplemental Table S2). Notably, each nuclear receptor displayed its own unique pattern of interaction with the different corepressor variants tested. For example, in the absence of ligand, PPAR␥ interacted significantly more strongly with corepressor splice variants containing RID3 (the 37bϩ NCoR and 40bϩ SMRT␥) compared with otherwise identical corepressor splice variants lacking RID3 (the 37bϪ NCoR␦ and 40bϪ SMRT␣) (Fig. 4). In contrast, recognition of corepressor by LXR␣ appeared to be largely independent of the presence or absence of RID3 (e.g. compare LXR␣ binding to NCoR versus NCoR␦, and SMRT␥ versus SMRT␣; Fig. 4). Conversely, excision of sequences could also increase the inter- Exons removed (ᰔ) or added (⌬) relative to the reference sequence by alternative splicing are indicated below each schematic. Note that our standardization on the RefSeq database in this report results in a change in the SMRT exon numbering system compared with our prior publications. B, schematic of individual corepressor proteins of interest. Exon sequences included in each corepressor protein are shown as thick lozenges; exon sequences deleted by alternative mRNA splicing are depicted as thin horizontal lines. RIDs are shown as ovals. Nomenclature has been described previously (69). DECEMBER 30, 2011 • VOLUME 286 • NUMBER 52 action between specific corepressor variants and specific nuclear receptors; for example, the 47bϪ SMRT variant, lacking a region flanking RID1, was bound more strongly by both PPAR␥ and LXR␣ than was the otherwise identical SMRT␣ containing this region (Fig. 4). In general, the affinity of a corepressor for a given nuclear receptor appeared to be determined at least as much by the alternative splicing to which it was subject as by its locus of origin (Fig. 4).

Corepressor Splicing and Adipogenesis
We also tested several of these nuclear receptors for the ability to release the different corepressor variants in response to ligand agonists (Fig. 4, open bars) In many cases the efficiency of release varied with the corepressor variant. For example, treating RAR␣ with saturating concentrations of all-trans retinoic acid released SMRT␥, NCoR, and NCoR␦, more completely than SMRT⑀, SMRT, or SMRT␣. Similarly, TR␣ and PPAR␥ released certain corepressor variants more efficiently than others in response to cognate agonists. LXR␣ and Farnesoid X Receptor-␣, however, displayed little or no release of any of the corepressor variants tested in response to the agonists employed. These divergent responses are likely to reflect differences in the conformational changes invoked in each nuclear receptor by its cognate agonist, and differences in the specific FIGURE 2. Relative expression of different corepressor splice variants in different murine tissues. Messenger RNA was isolated from the organs and tissues indicated and was subjected to RT-PCR using primers spanning the relevant splice sites (see Fig. 1A and supplemental Table S1A); the PCR products were resolved by gel electrophoresis and quantified to determine the percentage of each alternatively spliced mRNA produced at each splice site (total ϭ 100%). The means Ϯ S.E. (n Ն 3) are presented. Skel Mscl, skeletal muscle; WAT, white adipose tissue; BAT, brown adipose tissue. Different Corepressor Splice Variants Can Exert Opposite Effects on Adipogenesis-Given their different affinities for different nuclear receptors, and their change in relative abundance during adipocyte differentiation, we chose to examine the roles of the NCoR and NCoR␦ splice variants in greater detail. We created stable 3T3-L1 cell transformants expressing each splice variant, or a GFP control, from a stably integrated expression vector. Integration and expression were confirmed by PCR and RT-PCR, and a minimum of 10 individual hygromycin-resistant colonies was combined for each construct to minimize any potential clone to clone variability. The ectopi-cally introduced NCoR␦ and NCoR variants were expressed at comparable levels in their respective transformants and resulted in detectable changes in the overall ratio of NCoR versus NCoR␦ compared with the control cells (Fig. 5, A and B); mRNA expression and splicing at the endogenous SMRT locus was unaffected (data not shown).
The GFP control, NCoR, and NCoR␦ transformants were indistinguishable by cell morphology and by most other criteria. Interestingly, however, quantitative proliferation studies revealed that transformants expressing the NCoR variant propagated with a slower doubling time and achieved a lower  Stable transformants of 3T3-L1 cells expressing GFP, NCoR␦, or NCoR were isolated and analyzed as indicated. A, ecoptically introduced GFP control, NCoR, and NCoR␦ are expressed at comparable levels. RNA from three independent 3T3-L1 transformants (differentiation Day 0) was analyzed by quantitative RT-PCR for expression of the ectopic GFP, NCoR, or NCoR␦ using the primer pairs noted in supplemental Table S1C. Means Ϯ S.E. are shown. B, introduction of ectopic NCoR or NCoR␦ detectably alters the overall expression of the corresponding NCoR splice variants in the 3T3-L1 transformants. The relative abundance of mRNAs containing NCoR exon 37bϪ or 37bϩ was assayed in each transformant by RT-PCR, using primers that span the alternative splice sites as in Fig. 2. C, NCoR transformants proliferate slower and reach lower saturation density. Proliferating 3T3-L1 transformants expressing GFP, NCoR␦, or NCoR were plated into culture dishes as described under "Experimental Procedures" and maintained at 37°C. Viable cells were quantified at the times indicated using CellTiter 96 Aqueous One Solution and measuring absorbance at 490 nm. The means Ϯ S.E. (n Ն 6) are shown. saturation density than did the NCoR␦ or the GFP transformants (Fig. 5C).
We next induced the adipogenic program in these cells using the DMI protocol. The 3T3-L1 cells transformed by the GFP vector withdrew from the cell cycle and began accumulating lipids, as detected by Oil Red O staining. By day 8 after induction many or most of the empty vector transformants displayed the rounded morphology, weaker adhesion, and large Oil Red O-positive lipid droplets characteristic of terminally differentiated adipocytes (Fig. 6). Cells transformed by the NCoR construct, in contrast, were significantly impaired in adipogenesis based both on morphological criteria and Oil Red O staining (Fig. 6). This result is consistent with the converse accelerated adipogenesis reported using pan-specific siRNAs to suppress all forms of NCoR in these cells (89). Unexpectedly, however, cells transformed by NCoR␦ variant displayed the diametrically opposite effect, undergoing adipogenesis more rapidly and more completely than did the GFP vector control (Fig. 6). These results indicate that alternative splicing can either oppose or enhance 3T3-L1 adipogenesis depending on the incorporation, or excision, of exon 37bϩ sequences from the final NCoR protein. Similar results were observed using HA-or Myc-tagged versions of NCoR and NCoR␦ (data not shown).

The Divergent Effects of NCoR and NCoR␥ on Adipogenesis Are Also Observed Using a Splice-specific Knock-out Approach-
To further investigate the biological roles of the different NCoR splice variants, we created mice bearing a inactivating mutation of the 37bϩ splice donor, thereby preventing expression of the NCoR variant and replacing it with comparable expression of the NCoR␦ variant. Mice homozygotic for the mutation were recovered. The absence of the NCoR transcript, and the presence of the NCoR␦ transcript, were confirmed in multiple organs by RT-PCR; splicing at the SMRT locus, or elsewhere in NCoR, was not detectably affected (data not shown). Although a comprehensive phenotyping of these animals at the organismal level remains in progress, we were able to recover MEFs from these versus matched wild-type animals and compare their ability to differentiate into adipocytes ex vivo. The loss of NCoR in the MEFs resulted in a pro-adipogenesis phenotype, generating Oil Red O-positive cells at significantly higher incidence than was observed in wild-type MEFs (Fig. 7, A and B). This phenotype was reproducible in multiple MEF cultures from multiple embryos. NCoR␦, but not NCoR expression was detected in the knock-out MEFs, and the expression of SMRT splice variants was unaffected ( Fig. 7C and data not shown). These results, which are reciprocal to the inhibition of 3T3-L1 adipogenesis observed when NCoR was overexpressed, support the proposal that NCoR splice variants containing RID3 inhibit adipogenesis, whereas NCoR splice variants lacking RID3 are pro-adipogenic.

Different Corepressor Variants Target Distinct Genes-Given their opposing biological effects in our Oil
Red O experiments, we next examined the effects of the NCoR versus NCoR␦ splice variants at the transcriptional level. We analyzed the mRNA expression profiles of our GFP, NCoR, and NCoR␦ 3T3-L1 transformants at Days 0 and 8 after DMI induction. We used RT-PCR and focused on a panel of genes previously shown to be associated with adipogenesis. As expected from prior studies of adipogenesis, the majority of the genes in this panel were induced by Day 8 in our control transformants ( Fig. 8; additional statistical analysis is provided in supplemental Table  S3); the corresponding gene products include proteins involved in carbohydrate/lipid metabolism, storage, or transport (e.g. Acsl1, ATGL, CD36, Fabp4, FAS, Hmgcl, HSL, Lpl, Me1, Pck1, Pcx, Plin, and Srebf1), adipocyte-encoded cytokines (e.g. Adipoq and Retn), mitochondrial uncoupling proteins (e.g. UCP3), and a series of nuclear receptors and related transcriptional factors known to participate in adipocyte differentiation and function (e.g. Cebpa, LXRa, PGC1a, PPARg, and Zfp423). Consistent with the ability of NCoR to inhibit adipogenesis in our Oil Red O assay, the expression of the majority of these genes was reduced in the NCoR transformants relative to the GFP control (Fig. 8). Similarly, given the enhanced Oil Red O phenotype of our NCoR␦ transformants, the expression of many of these genes was elevated, or at least equal, in the NCoR␦ transformants compared with the GFP control and were clearly distinct from the NCoR transformants (Fig. 8). Nonetheless, the extent of repression by NCoR, or of induction by NCoR␦, appeared to vary somewhat from gene to gene. These results indicate that the individual corepressor splice variants exert distinct, often opposing effects on gene expression that, by dif-

Alternative mRNA Splicing in Different Tissues and Cell
Types Creates Extensive Corepressor Diversity-The NCoR and SMRT loci are the products of a gene duplication/divergence event that occurred early in vertebrate evolution. These paralogs share ϳ50% conservation at the codon level and encode proteins that can assemble into near-identical corepressor complexes, interact with overlapping sets of transcription fac-tor partners, and display very similar biochemical properties in vitro. Nonetheless, since their divergence, NCoR and SMRT have been maintained as distinct loci over a subsequent 10 8 years of gnathostomata evolution, suggesting that the two paralogs perform biologically distinguishable roles (67). This conclusion is supported by gene ablation experiments that demonstrate NCoR and SMRT are independently required for murine viability and produce distinct phenotypes when mutated (49,68,(87)(88)(89)(95)(96)(97)(98)(99)(100). Adding to this diversity at the genetic level, both NCoR and SMRT are alternatively spliced to produce a series of corepressor splice variants (18,(63)(64)(65)(66)(67)(68)(69)(70). This alternative splicing is particularly evident over the C-terminal regions of these corepressors and extensively modifies the cRID sequences responsible for interacting with nuclear receptor partners. As a consequence, different corepressor variants display different affinities for different nuclear receptors (and presumably, for other, non-receptor transcription factor partners as well).
As shown here, certain of these alternative corepressor splicing events appear to be relatively invariant across different mouse tissues. However, others occur at very different rates in different tissues and in different cell lines, indicating that cells must possess active mechanisms to regulate the corresponding splicing events. One of the more interesting of these is the 37bϩ/40bϩ splice, which introduces a third cRID (RID3) into NCoR and SMRT, respectively. As described in more detail below, the presence of this third RID significantly increases the affinity of the corresponding corepressors for certain nuclear receptors, such as PPAR␥, compared with corepressor variants lacking RID3 (39, 51, 52, 54 -56, 58, 59, 62, 101-103). The NCoR and SMRT 37bϩ/40bϩ splice variants are abundant in brain and in testes, and in the undifferentiated 3T3-L1 cells studied here, but are relatively minor species in most other adult mouse tissues examined. We speculate that the unusually rich abundance of the 37bϩ/40bϩ splice forms of SMRT and NCoR in these tissues confers anatomically restricted functions on PPAR␥ (and other N3/S3-dependent nuclear receptors or non-receptor transcription factors) to yield tissue-specific biological effects (104 -109). Intriguingly, another splice, denoted SMRT 47Ϫ, deletes RID1 and behaves in many ways reciprocally to SMRT 40bϩ; corepressor variants lacking the 47 exon, such as SMRT⑀, are rare in brain and testes and are impaired in binding to many nuclear receptors compared with variants containing the 47bϩ exon, such as SMRT␣.
It is interesting to note that, despite encompassing similar RID3 sequences, the NCoR37bϩ and SMRT 40bϩ splicing events occur at non-homologous splice donor and acceptor sites, indicating that the ability to generate these corepressor variants is probably the result of a convergent evolution that occurred after the duplication and divergence of the NCoR and SMRT loci. Similarly, the extensive alternative splicing associated with RID1 in SMRT was not observed for NCoR, indicating that the SMRT 47bϪ and SMRT 47Ϫ splicing events also appeared after the evolutionary divergence of NCoR and SMRT, and has been subsequently confined to the latter locus.
The Different Corepressor Splice Variants Display Different Affinities for Different Nuclear Receptor Partners-Our experiments agree with, and extend, prior observations that different  DECEMBER 30, 2011 • VOLUME 286 • NUMBER 52

JOURNAL OF BIOLOGICAL CHEMISTRY 44995
corepressor variants exhibit significant differences in their abilities to bind to different nuclear receptors. These differences, in part, reflect differences in the ability of the individual RID domains within each corepressor variant to bind to a given nuclear receptor. For example, TRs are known to bind strongly to an isolated RID3 construct and more weakly to isolated RID1 or RID2 constructs (39, 51, 52, 54 -56, 58, 59, 62, 101-103). Therefore, it is not unexpected that TR␣ binds more strongly to corepressor splice variants that contain RID3 (such as NCoR) compared with those that do not. Conversely, RAR␣ is known to bind strongly to an isolated RID2 and weakly or not at all to isolated RID1 or RID3; given that all the corepressor variants tested include RID2 (53,57), it is not surprising that RAR␣ bound relatively broadly to multiple corepressor variants. In addition to splicing, sequence differences between the two corepressor loci themselves also have an effect on the nuclear receptor partnership. For example, RAR␣ and PPAR␥ both interact more weakly with NCoR than with SMRT␥, despite these two corepressor variants representing the products of very similar splicing events.
Adipocyte Differentiation Is Accompanied by Specific Changes in Corepressor Splicing Pattern-The mouse 3T3-L1 cell line has been extensively exploited as ex vivo models of pre-adipocyte to adipocyte differentiation. We report here that inducing adipogenesis in 3T3-L1 is paralleled by a significant shift in the splicing of NCoR from the 37bϩ pattern to the 37bϪ pattern. This decreases the relative expression of NCoR variants containing three RIDs (such as NCoR) but increases the relative expression of variants containing two RIDs (such as NCoR␦). The expression of the other corepressor splice variants either was not, or was only minimally, altered. Consistent with these findings, differentiated white adipose tissue in vivo expresses a low NCoR 37bϩ to 37bϪ ratio. Given that the 37bϩ NCoR suppresses adipocyte differentiation, whereas the 37bϪ NCoR␦ promotes it (below), it is tempting to speculate that this shift in NCoR splicing may help release the block to differentiation in the pre-adipocyte and/or may help establish the transcriptional program necessary for proper physiological function of the mature adipocyte.
Different Splice Forms of the Same Corepressor Have Opposite Effects on Adipocyte Differentiation-To examine the role of alternative corepressor splicing in adipogenesis, we tested the effect of overexpressing NCoR versus NCoR␦ in the 3T3-L1 cell system. Consistent with prior demonstrations that panspecific knockdown of all NCoR (or all SMRT) mRNA enhances 3T3-L1 cell adipocyte differentiation (89), our reciprocal overexpression of ectopic NCoR inhibited 3T3-L1 differentiation (monitored by Oil Red O staining). In contrast, however, expression of comparable levels of NCoR␦ significantly enhanced 3T3-L1 adipogenesis under the same conditions. Therefore, different splice variants of the same corepressor class can mediate profoundly different effects on adipogenesis.
To complement our overexpression approach, we also examined adipogenesis in MEFs isolated from a splice-specific 37bϩ knock-out mouse model. We ablated the 37bϩ splice donor in these mice by standard site-directed mutagenesis and ES cell techniques, abolishing their ability to make NCoR, but leaving the 37bϪ splice donor, the shared splice acceptor, and the NCoR␦ reading frame intact. Mice homozygous for the mutation fail to express NCoR and display a corresponding shift to NCoR␦ expression in all tissues examined; splicing of SMRT and elsewhere in NCoR are unaffected. The NCoRϪ/Ϫ mice are viable and display a number of endocrine and metabolic phenotypes that remain under investigation. 3 Notably, MEFs isolated from these NCoR-/-mice display an enhanced adipocyte differentiation in culture compared with wild-type MEFs, a result fully consistent with the reciprocal ability of NCoR overexpression to inhibit, and NCoR␦ overexpression to enhance, 3T3-L1 adipogenesis.
Different Corepressor Variants Generate Different Transcriptional Programs When Expressed in the 3T3-L1 Cells-To determine if the divergent effects of the different corepressor splice forms on adipogenesis as a whole were re-capitulated at the individual gene level, we examined the expression of a panel of adipocyte-associated gene products in our 3T3-L1 transformants. The majority of these pro-adipogenic genes was strongly induced by Day 8 after Dex/insulin/IBMX treatment in the control and NCoR␦ transformants, whereas this induction was severely muted in the NCoR transformants.
A complex transcriptional network regulates adipocyte differentiation (25,28,(73)(74)(75)(76)(77)(78)(79)(80)(81). Presumably any given corepressor variant associates with its specific nuclear receptor (and nonreceptor transcription factor) partners within this transcriptional network, each contributing to the regulation of different target genes, and each contributing to the many individual changes in the overall transcription program that result in adipocyte differentiation. The influence of a given corepressor variant on adipogenesis as a whole is therefore the combinatorial result of these individual effects. It should therefore be noted that the late stage differences in gene expression we report here (on Day 8 after induction) probably reflect both the primary effects of the different corepressor variants and the secondary effects of the divergent differentiation phenotypes. A complete study of gene expression throughout the differentiation process, most likely combined with a chromatin immunoprecipitation assay, will be necessary to fully define which of these genes are directly targeted by which corepressor variant.
Multiple Loci and Alternative mRNA Splicing Serve to Customize the Transcriptional Program for Specific Purposes in Specific Cell Types-Some of the divergent effects of NCoR and NCoR␦ on adipogenesis are likely to reflect their different affinities for the nuclear receptors characterized in the current 3 M. L. Privalsky and M. L. Goodson, unpublished observations. FIGURE 8. Different effects on adipocyte gene expression by NCoR versus NCoR␦. Cultured 3T3-L1 transformants expressing GFP, NCoR, or NCoR␦ were induced to differentiate using Dex/insulin/IBMX, and mRNA was isolated on differentiation Days 0 and 8. The mRNA was analyzed by quantitative RT-PCR for expression of 23 genes associated with adipocyte differentiation and/or function, using the primer pairs noted in supplemental Table S1B. The means Ϯ S.E. from three independent experiments are shown. p values are presented in supplemental Table S3. Although included in all plots, expression on Day 0 for many genes may have been too low to produce a visible bar on this graph. study, such as PPAR␥. Differences in the affinities of these splice variants for additional, as yet untested nuclear receptors and non-receptor transcription factors may also contribute to this phenomenon, as may aspects of corepressor function beyond that of transcription partner preference. For example, NCoR␦ function is inhibited by MAP kinase signaling, whereas NCoR is not (66). Nor do we exclude the possibility that alternative splicing of the 37bϩ exon can modify the assembly or function of the corepressor complex itself by adding or deleting binding sites for additional corepressor components.
More broadly, we propose that this diversification of both NCoR and SMRT through alternative mRNA splicing serves to adapt corepressor function for specific purposes in specific cell types. In this fashion, specific forms of corepressors can be expressed and assembled for specific tasks, then altered and re-designed when new tasks are required. This corepressor redesign can be in response to particular differentiation signals, as seen with the change in NCoR versus NCoR␦ ratios in adipocyte differentiation, or potentially in response to changes in the cell environment or to signals originating from other cells.
It is worth noting that there are many intriguing parallels between how the SMRT and NCoR corepressors, and their nuclear receptor partners, are diversified and expressed. Both are frequently encoded by multiple genetic loci that are, in turn, alternatively spliced to generate a series of distinct corepressor variants and nuclear receptor isoforms that vary in relative abundance in different cell types. The gene duplication and divergence events that initiated this diversification appeared for both corepressors and nuclear receptors during the early vertebrate radiation ϳ300 to 500 million years ago. Both sides of this diversification have served to rewrite the partnership contract: alternative corepressor splicing can alter its affinity for a given nuclear receptor isoform, and alternative nuclear receptor splicing can alter its affinity for a given corepressor variant. Taken as a whole, these mechanisms allow a limited number of receptors and coregulators to don many guises, permitting them to play the many different roles assigned to them by evolution and to change the script as events require it.