Coactivation by OCA-B: Definition of Critical Regions and Synergism with General Cofactors

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Mol Cell Biol, July 1998, p. 3803-3810, Vol. 18, No. 7
0270-7306/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Coactivation by OCA-B: Definition of Critical Regions and Synergism with General Cofactors

Yan Luo, Hui Ge, Sean Stevens, Hua Xiao, and Robert G. Roeder^*

Laboratory of Biochemistry and Molecular Biology, The Rockefeller University, New York, New York 10021-6399

Received 2 February 1998/Returned for modification 20 March 1998/Accepted 22 April 1998

SUMMARY
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

SUMMARY
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Molecular dissection of the B-cell-specific transcription coactivator OCA-B has revealed distinct regions important, respectively,for recruitment to immunoglobulin promoters through interactionwith octamer-bound Oct-1 and for subsequent coactivator function.Further analysis of general coactivator requirements showed thatselective removal of PC4 from the essential USA fraction severelyimpairs Oct-1 and OCA-B function in a cell-free system reconstitutedwith partially purified factors. Full activity can be restoredby the combined action of recombinant PC4 and the PC4-depletedUSA fraction, thus suggesting a joint requirement for PC4 andanother, USA-derived component(s) for optimal function of Oct-1/OCA-Bin the reconstituted system. Indeed, USA-derived PC2 was foundto act synergistically with PC4 in reproducing the function ofintact USA in the assay system. Consistent with the requirementfor PC4 in the reconstituted system, OCA-B was found to interactdirectly with PC4. Surprisingly, however, removal of PC4 fromthe unfractionated nuclear extract has no detrimental effect onOCA-B/Oct-1-dependent transcription. These results lead to a generalmodel for the synergistic function of activation domains in Oct-1and OCA-B (mediated by the combined action of the multiple USAcomponents) and, further, suggest a functional redundancy in generalcoactivators.

INTRODUCTION
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The B-cell-specific function of immunoglobulin (Ig) promoters is mediated by an octamer element (ATTTGCAT) and was thoughtoriginally to be regulated by an octamer-binding factor (Oct-2)enriched in lymphoid cells (reviewed in reference 51). However,early biochemical analyses indicated that Ig promoters could functionequally well with Oct-2 or the ubiquitous Oct-1 and that B-cell-specificpromoter function was determined by a B-cell-specific Oct-1-associatedcoactivator designated OCA-B (30, 41). These studies establisheda new paradigm for cell-specific promoter activation that involvesrecruitment of the true regulatory factor to the cell-specificpromoter element through interaction with a ubiquitous DNA bindingfactor. Subsequent genetic analyses confirmed that Oct-2 was nonessentialfor Ig promoter activation but failed to identify the responsibleB-cell-specific factor (6-8).

The discovery of OCA-B set the stage for cloning of a cognate cDNA on the basis of biochemical purification (31) and yeastgenetic screens (13, 54), which, in turn, facilitated bothgenetic and biochemical analyses of OCA-B. Targeted gene disruptiondata (19, 39, 50) revealed that OCA-B is essential for normalpatterns of Ig expression, most notably antigen-dependent responsesleading to secondary isotype production, but not for antigen-independentIg gene transcription events that might conceivably employ otherOct-1 coactivators.

Biochemical studies with recombinant OCA-B have confirmed the originally suggested mechanisms by showing that the highly relatedPOU domains (reviewed in references 15, 16, and 45-48) of Oct-1and Oct-2, but not that of Oct-3, are sufficient for OCA-B interactionand promoter recruitment (13, 31, 54). More recent studieshave shown that OCA-B also contacts octamer nucleotides throughthe major groove in the DNA-Oct-1-OCA-B complex (2, 4),consistent with a stronger OCA-B interaction with Oct-1 or Oct-2in the presence of DNA (31). Further, the demonstration thatOCA-B can discriminate among octamer variants for formation ofthe higher-order ternary complex provided a mechanism for differentialactivation of octamer-containing promoters (4, 14), whereasthe inability of OCA-B to stimulate the histone 2B (H2B) promoter(31), which contains a functional octamer element identicalto the consensus Ig promoter element, requires a different explanation.Finally, while corresponding POU domains are sufficient for OCA-Brecruitment to Ig promoters and for normal octamer-mediated transcriptionfrom the H2B promoter, an additional Oct-1 or Oct-2 activationdomain(s) is necessary for functional synergy with OCA-B and correspondingactivation of Ig promoters (31). When assayed in more purifiedreconstituted system, Ig promoter activation by OCA-B and Oct-1also required the general coactivator fraction USA in additionto the general initiation factors (31).

The availability of recombinant OCA-B and in vitro assay systems with general initiation factors (reviewed in reference 44)and cofactors (reviewed in reference 18) prompt questions aboutstructure-function relationships in relation to its interactionboth with Oct-1 (upstream interactions) and, potentially, withcomponents of the general transcription machinery (downstreaminteractions). As predicted from our previous model invoking separatedomains for these interactions (31), mutant OCA-B defectivein either interaction would, in principle, lead to defects incoactivation function. This scenario is reminiscent of that describedfor the herpes simplex virus (HSV) (co)activator VP16, which wasreported to interact with promoter-bound Oct-1 through the POUdomain (e.g., 26, 43); have a conditional DNA binding activity(25, 52, but see reference 58; reviewed in references 5and 15), a property shared by OCA-B (2, 4); and providean activation function. From this point of view, OCA-B may representa class of cellular counterparts of viral coactivators (see Discussion).

In this report, we first show functional analyses of wild-type OCA-B versus mutant derivatives to define domains criticalfor upstream versus downstream interactions. We then present afurther definition of general cofactor requirements for the properfunction of Oct-1 and OCA-B in a reconstituted system. Finally,we use OCA-B mutants to establish a functional linkage betweenOCA-B and general cofactors.

MATERIALS AND METHODS
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In vitro transcription. For transcription in nuclear extracts, conditions described by Luo et al. (30) and Luo and Roeder (31) were used. Thereaction mixtures (25 µl) contained 5 µl of transcription premix(200 mM HEPES [pH 8.4]; 15 mM MgCl₂, 3 mM each ATP, GTP, CTP,and UTP; 20 mM dithiothreitol, 40 U of RNasin); 5 µl of H₂O containing500 ng of the BCL₁ (27) IgH template (41) and, when indicated,50 ng of the 2×Sp1 template (42); and 15 µl of a mixture ofnuclear extract maintained in BC100 (30; typically, 10 µl) andvarious amounts of cofactor OCA-B maintained in BC100-250-µg/mlbovine serum albumin (BSA) with compensating volumes of the samebuffer. For transcription in a reconstituted system, the nuclearextract-OCA-B mixture mentioned above was replaced with TFII-A,-B, -D, and -E/F/H plus RNA polymerase II and other factor andcofactor components specified in the figures and legends. Factorsin this system were stabilized by 1.5-mg/ml BSA. All of the invitro transcription reaction mixtures were incubated at 30°C for60 min, and transcripts were measured by primer extension.

Purification of factors and cofactors. Proteins were maintained in the BC buffers described by Luo et al. (30). Numbers following BC indicate millimolar KCl concentrations.Highly purified factors and cofactors (in BC100) were stabilizedwith 250-µg/ml BSA. Oct-1 (glycosylated) was purified from HeLanuclear extracts by using a combination of wheat germ agglutininand octamer binding site affinity columns as described by Pieraniet al. (41). General transcription factors and cofactors wereprepared as described by Ge et al. (10) and Kretzschmar et al.(24).

Recombinant wild-type and mutant OCA-B proteins were expressed as six-His-tagged proteins (vector 6His-pET11d; reference 17)in Escherichia coli and purified. Recombinant PC4 was expressedand purified as described by Ge et al. (10).

Immunodepletion of PC4. Immunodepletion of PC4 was carried out at 4°C. The USA fraction from the heparin-Sepharose step (see reference 34; 0.4 mlin BC100, diluted to 2 ml with BC600) was passed several timesthrough a 0.4-ml protein A-agarose column equilibrated in BC500.Half of the flowthrough fraction served as a source of mock-depletedUSA. The other half was passed several times through a 0.2-mlanti-PC4 affinity column equilibrated in BC500. Both the finalflowthrough fraction from the protein A column and that from theanti-PC4 column were dialyzed to BC100, concentrated (about fivefold)by ultrafiltration (Amicon, Inc.), and used as mock-depleted andPC4-depleted USA fractions in transcription assays. The extentof depletion was monitored by immunoblotting various fractionswith anti-PC4 sera (see Fig. 3A). Removal of PC4 from HeLa nuclearextract was carried out by a similar protocol, except for theomission of the initial dilution and final concentration steps.

Anti-PC4 antibodies were raised against a protein containing full-length PC4 fused to glutathione S-transferase (GST). Specificanti-PC4 antibodies were purified from crude antisera by usingan immunogen affinity column. The purified antibodies were thencross-linked to protein A-agarose, yielding an anti-PC4 affinitycolumn.

Protein-protein interaction assays. To detect a protein(s) that can specifically bind to the wild-type OCA-B activation domain, GST and a GST-OCA-B fusion protein(containing residues 171 to 256 in wild-type and mutant B OCA-B;Fig. 1) were expressed in E. coli and then purified by bindingto glutathione-agarose beads. Subsequently, aliquots of HeLa nuclearextract in BC100 were passed through the resultant beads equilibratedin BC100. After extensive washing of the resins with BC100, thebound proteins were eluted by BC1000. The eluates were analyzedby multiple immunoblots using available antisera against variousgeneral factors and cofactors; PC4 was the sole polypeptide detectedby immunoblotting.

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FIG. 1. (A) A simple linear description of the OCA-B molecule. The 256-residue polypeptide is rich in proline (~16%; for the complete sequence, see references 13, 31, and 54). Relevant putative functional domains include domain A (with its sequence alignment with an E1A segment shown) and domain B (with acidic residues marked by asterisks). The mutant forms of OCA-B used in this study are also described. The mutant proteins were made by a PCR-based strategy. (B) Protein profile of bacterially expressed, 6His-tagged wild-type OCA-B and mutant forms of OCA-B. A roughly calculated 0.1 ng each of the proteins was analyzed by immunoblotting with polyclonal anti-OCA-B antibodies. (Given that all three mutant proteins may have lost some epitopes compared to the wild type, the amounts of the mutant proteins might be slightly underestimated. Nevertheless, this underestimation would not complicate our analyses of, and the conclusions made about, these mutant proteins.) The amounts used for the in vitro transcription analyses in Fig. 2 were based on this estimation.

Analysis of the in vivo function of OCA-B and derived mutants by transfection. cDNAs encoding wild-type and mutant (A, B, and A/B) OCA-B proteins were subcloned into mammalian expression vector pRC (Invitrogen).These effector constructs were cotransfected with a reporter gene(luciferase in vector pGL3; Promega) under the control of theBCL₁ (27) IgH promoter. The transfection analyses were carriedout with HeLa cells by using conventional calcium phosphate methods,and cells were harvested after 48 h. Extracts were prepared byusing reporter lysis buffer (Promega), and expression was assayedin accordance with the manufacturer's instructions. In each case,assays were conducted in duplicate or triplicate and a constantamount of the vector CMV $beta$ gal was added as an internal controlfor transfection efficiency. The expression vector levels weretitrated carefully, and the amounts used for the data includedhere were within the linear range for activation. Western blotanalyses indicated that the OCA-B cDNA and the various mutantforms were expressed at similar levels (data not shown).

RESULTS
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Molecular dissection of OCA-B. In addition to being rich in proline (~16%), a characteristic of a number of transcription factors (reviewed in reference 35), OCA-B displays a weak sequence similarity to the viralcoactivator E1A (31; domain A in Fig. 1A) and contains a putativeacidic activation domain (domain B in Fig. 1A) reminiscent ofthat of coactivator VP16 (56). To explore the possibility thatthese domains are important for OCA-B function, three OCA-B mutantswere made as described in the legend to Fig. 1. The A mutant proteinhas domain A (amino acids [aa] 4 to 18) deleted, the B mutantprotein has the acidic stretch neutralized, and the A/B mutantprotein is a combinatorial double mutant protein. For in vitroanalyses, wild-type OCA-B and the mutant forms of OCA-B were expressedin and purified from bacteria (Fig. 1B); they then were testedfor the ability to stimulate an Ig heavy-chain (IgH, BCL₁ [27rsqb;)reporter promoter in a HeLa cell nuclear extract. In a dose-responseexperiment (Fig. 2A), all three mutant proteins showed reducedtranscriptional activity compared to wild-type OCA-B. To analyzein vivo functions, HeLa cells were cotransfected with the BCL₁IgH promoter reporter and cytomegalovirus-driven expression vectors.As expected, the in vivo activities of the wild-type and mutantOCA-B proteins on the IgH promoter paralleled those observed invitro (Fig. 2B). Both in vivo (Fig. 2B) and in vitro (Fig. 2A),the defect in the combinatorial A/B mutant protein was more severethan that of either the A or the B mutant protein. Quantitationof the activation levels is indicated in the figure legends.

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FIG. 2. Analyses of wild-type (Wt) OCA-B and mutant (Mut.) forms of OCA-B. (A) In vitro transcription assay. As indicated, three doses of wild-type OCA-B and mutant OCA-B (respectively, 10 ng [lanes 2, 5, 8, and 11]; 20 ng [lanes 3, 6, 9, and 12], and 50 ng [lanes 4, 7, 10, and 13]) were used in the titration experiment to complement a HeLa nuclear extract (10 µl for each reaction). The transcripts were analyzed by primer extension as described by Luo and Roeder (31). Lane 1 ( $-$ ) was a control (without the addition of OCA-B or its derivatives). Transcription activation levels (by the middle point dosage of OCA-B, i.e., 20 ng; an amount equivalent to that of the endogenous OCA-B present in 10 µl of the B-cell [Nam] nuclear extract), compared to lane 1 (taken as 1), are 8, 2.7, 2.2, and 1.4, respectively, for the wild type and the B, A, and A/B mutant proteins (lanes 3, 6, 9, and 12; also, see the fold stimulation shown under each corresponding lane). (B) In vivo (transfection) assay. An IgH reporter promoter construct (with the promoter inserted in front of the luciferase gene) was cotransfected with effector constructs (expressing OCA-B or its mutants under the control of the cytomegalovirus promoter) in HeLa cells. Relative IgH promoter activation levels were scored by measuring the light units of the extracts of the transfected cells 48 h posttransfection normalized to $beta$ -galactosidase controls. Taking the level with no effector as 1, the relative levels are 12, 4, 3, and 2, respectively, for the wild type and the B, A, and A/B mutant proteins. The mutant OCA-B proteins were expressed at levels similar to that of the wild-type protein in transfected cells, as assessed by immunoblotting with anti-OCA-B antibodies (data not shown). (C) Octamer DNA-POU-1 complex supershift assay. POU-1 is a truncated version of Oct-1 containing only the POU domain, sufficient to bind OCA-B either in solution or when on DNA (e.g., reference 31). The supershift condition was the same as that described by Luo and Roeder (31), except that approximately 25-fold less OCA-B (or its mutants) was used, such that only a portion of the binary complex was supershifted. To obtain the highest possible resolution, the free probe (a labeled DNA fragment containing the IgH octamer site) was allowed to run out of the gel. As can be seen, the B mutant protein (lane 3) retained the ability to form the higher-order complex, which was even denser than that formed with the wild type (lane 2) for a reason we do not know, whereas the A mutant protein (lane 4) lost the capacity to bind the binary complex. Given that the combinatorial A/B mutant protein (lane 5) could give rise to the formation of a residual level of the ternary complex, it is possible that the introduction of the B mutant protein created a conformational change that can increase the POU-OCA-B interaction even with domain A deleted. We emphasize that such a complication in the binding assay did not complicate our in vitro transcription analyses and conclusions. (D) Test of dominant negative potentials of wild-type OCA-B and its mutant forms. Eight microliters of B-cell (Nam) nuclear extract was used for each reaction (there is ~2 ng of endogenous OCA-B per µl in this nuclear extract [see above]). The nuclear extract was supplemented with either BC100 buffer (lane 1) or, as indicated, recombinant wild-type or mutant OCA-B (~100 ng, for a molar ratio of ~6:1 over the endogenous OCA-B) in BC100 (lanes 2 to 5). The transcripts were analyzed as described for panel A.

These mutant B results suggest that domain B is a major activation domain of the OCA-B molecule. Further confirming this notionis the fact that while a Gal4 (1-94)-OCA-B fusion protein functionsas an activator on promoters containing Gal4 binding sites, amutant protein with a deletion encompassing domain B loses theactivation capability (53). However, our mutant B results differsomewhat from those reported by Gstaiger et al. (14), who foundthat large C-terminal deletions (aa 193 to 256 and 123 to 256)had no detrimental effects on the coactivation function of OCA-Bin transfection assays. Furthermore, in our transfection assays,even a smaller C-terminal deletion in OCA-B (aa 209 to 256; adeletion encompassing domain B) was found to impair the coactivationfunction of OCA-B (53). One explanation for this apparent discrepancyis that the more extensive C-terminal deletion mutant proteinsof Gstaiger et al., which still had activation function in theirassay, may have also lost an intrinsic inhibitory domain thatnormally masks an otherwise silent activation function (residingbetween residues 66 and 122). Alternatively, it is possible thatin the transfection assays of Gstaiger et al., the effectors wereoverexpressed, amplifying minor activation domains whose effectsnormally would not be observed. In agreement with the second possibility,similar mutant proteins, when carefully titrated, were, in fact,defective in our studies (53). Artificial coactivation by OCA-Bor its derivatives (when in excess) may also result from theirless functionally relevant interactions with DNA or with the basalmachinery. Thus, high doses of the A and B mutant proteins and,to a lesser extent, the A/B mutant protein cause detectable stimulationin vitro and in vivo (53). This is exemplified in Fig. 2A, whichshows that the largest amounts of mutant OCA-B had measurableeffects.

The wild-type and mutant OCA-B proteins were next checked for the ability to supershift a complex containing an octamer elementand the DNA binding (POU) domain of Oct-1 in an electrophoreticmobility shift assay (Fig. 2C). In agreement with the idea thatdomain A provides a determinant for POU domain interaction, itsdeletion essentially abrogated the ability of OCA-B to form theternary complex (compare lane 4, Mut. A, to lane 2, Wt). Thisobservation suggests that the coactivation defect of mutant Ais due largely to its lack of an upstream interaction with Oct-1.In contrast, the B region mutation actually enhanced the abilityof OCA-B to bind to the DNA-POU-1 complex (compare lane 3, Mut.B, to lane 2, Wt). The reason for the enhancement is not known.(However, given that the combined A/B mutant protein [lane 5]showed a residual level of ternary complex formation, one likelyscenario [also offered in the legend to Fig. 2C] is that the domainB mutation results in a conformational change that can increasethe POU-OCA-B interaction even in the absence of domain A. Sucha conformational change may also contribute, along with the lossof acidic residues per se, to the coactivation defect of the Bmutant protein.) Nevertheless, given that the B mutant proteinmaintains the ability to supershift an octamer-POU-1 complex,its coactivation defect most likely originates from lack of adownstream interaction(s). By virtue of a lack of both interactions,it is reasonable that the A/B double mutant protein shows an evenmore reduced coactivation capacity (Fig. 2A and B).

To further establish these ideas, dominant negative potentials of wild-type versus mutant OCA-B proteins were tested. Namalwacell (Nam; a B-cell lymphoma line) nuclear extract was supplementedwith recombinant proteins at a 6:1 molar ratio of exogenous toendogenous OCA-B, and the IgH promoter activity was determinedin an in vitro transcription assay (Fig. 2D). As predicted, theB mutant protein showed a significant dominant negative effect(compare lane 3 to lane 1), in agreement with the idea that itcan bind strongly to the IgH promoter-Oct-1 complex and interfere,competitively, with the binding of endogenous OCA-B. In contrast,the A and A/B mutant proteins had no (or marginal) effects (comparelanes 4 and 5 to lane 1), whereas exogenously added wild-typeOCA-B slightly boosted IgH promoter activity (compare lane 2 tolane 1). The inability of the A mutant protein, which maintainsthe normal domain B (Fig. 1A), to exert a dominant negative effectsuggests that OCA-B may interact with a downstream target(s) morestrongly when it is on the promoter than when it is free in solution.

Mechanism of action of OCA-B: essential role for PC4 and synergism with PC2 in a purified reconstituted system. Because OCA-B alone can confer B-cell level activation on Ig promoters, its function has been analyzed mainly in crude HeLanuclear extracts (see above and references 30 and 31). However,an earlier study (31) indicated that it can also function ina system reconstituted with Oct-1, highly purified HeLa-derivedbasal factors and RNA polymerase II, and general coactivator fractionUSA. This suggested that Ig promoter activation by the specializedcoactivator OCA-B requires still other general (USA-derived) cofactors(reviewed in reference 18). In the case of transcription activationby Gal4-based activators on model promoters with multiple Gal4sites, the USA-derived positive cofactor PC4 can replace, andis as potent as, the complete USA fraction (e.g., 11, 22;reviewed in reference 18). However, our earlier study showedthat PC4 alone could not substitute for USA in mediating Oct-1/OCA-Bfunction in a reconstituted system (31), thus raising the questionof whether the Gal4-based artificial system had "short-circuited"a regulatory pathway normally requiring more than one componentof the USA fraction.

To gain further insights into this question, the first objective was to determine whether PC4 is, indeed, essential for theability of USA to mediate activation by Oct-1 and OCA-B. To thisend, PC4 was immunodepleted from the USA fraction (Fig. 3A) andthe ability of the PC4-deficient USA to support OCA-B functionwith Oct-1 was assessed (Fig. 3B). The PC4-free USA was foundto be almost completely inactive in this system (compare lane7 to lane 6), suggesting that PC4 is, indeed, an essential USAcomponent for Oct-1 and OCA-B function in the reconstituted system.The transcription level was almost fully restored by additionof recombinant PC4 protein (lane 8). Given that PC4 alone couldnot replace the USA fraction to support Oct-1 and OCA-B function(31), we conclude that it must act synergistically with anothercomponent(s) in the USA fraction.

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FIG. 3. PC4 as an essential component of USA and acting synergistically with PC2, to support the function of OCA-B in a reconstituted transcription system. (A) PC4 depletion (dep.) from the USA coactivator fraction (left panel) and from the nuclear extract (NE; right panel; the treated nuclear extracts were used in the experiment shown in Fig. 5). The completion of the depletion was examined by immunoblotting with anti-PC4 antibodies. (B) IgH promoter activity was analyzed in the reconstituted system with components of general factors and RNA polymerase II (top) in the presence (+) or absence of Oct-1, OCA-B, or the USA fraction, as indicated. Lanes 1 to 5 demonstrate an IgH promoter dependency on activator Oct-1, general coactivator fraction USA, and specialized coactivator OCA-B. Oct-1 is absolutely required for the promoter activity (compare lanes 2 and 3 to lane 4, which represents a complete set of components sufficient to bring about a high level of IgH promoter transcription). In an otherwise complete system, the transcription is stimulated ~15-fold by USA and ~8-fold by OCA-B (compare lane 1, missing USA, and lane 5, missing OCA-B, respectively, to lane 4, complete). Lanes 6 to 8 demonstrate that PC4 is an essential component of USA to support the function of OCA-B in the reconstituted transcription system. The defect of the PC4-depleted USA fraction (lane 7), compared to the complete USA fraction (lane 6), can be rescued by the addition of 50 ng of recombinant PC4 (lane 8). (C) PC4-PC2 synergism for the function of OCA-B in the reconstituted system. Components (top) were used to transcribe the IgH promoter in the absence or presence (+ or ++) of a general coactivator(s), as indicated. The levels of coactivation are (compared to lane 1) ~15-fold by USA (lane 2), ~1.5- to 3-fold by PC2 (lanes 5 and 3), ~3- to 5-fold by PC4 (lanes 6 and 4), and ~10- to 15-fold by PC2 plus PC4 (lanes 8 and 7). Amounts of factors used in the reconstituted system (for both B and C) are as follows: TFII-A, 0.5 µl; recombinant TFII-B, 50 ng; TFII-D, 2 µl; TFII-E/F/H fraction, 3.5 µl; RNA polymerase II, 0.25 µl; Oct-1 (when added), 20 ng; recombinant OCA-B, 50 ng; recombinant PC4, 25 (+) and 50 (++) ng; USA, mock-depleted USA and PC4-depleted USA, 1 µl of each; PC2, 1 (+) and 2 (++) µl.

To identify the component(s) that acts in conjunction with PC4, native and PC4-depleted USA fractions were further fractionated.An activity chromatographically identical to PC2 (24) was foundto be jointly required with the recombinant PC4 to fully supportthe Oct-1- and OCA-B-dependent activation of the IgH promoter(Fig. 3C, lanes 7 and 8), whereas a fraction containing PC1 andPC3, in addition to PC4, was inactive (data not shown). As canbe seen, appropriate titration of both PC4 and PC2 produced atranscription level equivalent to that obtained with the intactUSA fraction (compare lane 7 to lane 2). On the other hand, andin agreement with prior studies of PC4 (31), the IgH promoteractivity was compromised in the transcription system containingeither PC4 or PC2 alone (compare lanes 3 to 6 to lanes 2, 7, and8). Increasing the level of PC2 did not boost the transcriptionand, in agreement with the results of earlier studies (11, 22),increasing the level of PC4 eventually repressed the transcriptionsystem (data not shown). Taken together, these results documenta synergism between PC4 and PC2 that is critical for optimal Oct-1and OCA-B function in the reconstituted system. Note that thepresent analysis, in contrast to that in our previous study describingthe cloning of OCA-B (31), used increased amounts of promotertemplate DNA, as well as larger amounts of various transcriptionfactors, to maximize the promoter activity such that, while maintaining8- to 10-fold coactivation by OCA-B, the level of IgH transcriptionin the reconstituted system is more comparable to that observedin a crude system. The considerable activation by PC4 alone observedhere (Fig. 3C, compare lanes 4 and 6 to lane 1) contrasts withthe previous report showing almost no activation by PC4 (Fig.8 in reference 31) but may reflect either genuine coactivationby PC4 intrinsic to this particular redefined system or, giventhe observed PC2-PC4 synergism, minor PC2 contamination in thepartially purified TFIID and the TFIIE/F/H fractions that wereadded at higher levels to accommodate a higher template dose.Because PC2 is still poorly defined, we cannot distinguish thesetwo possibilities. Nonetheless, the PC4-PC2 synergism was clearlyevident in this experiment.

Identification of PC4 as a downstream target for OCA-B function. As mentioned earlier, the defect of the B mutant form of OCA-B is due to loss of a downstream interaction. This prompted usto search for an OCA-B downstream target(s). PC4 seemed a likelytarget in view of its essential role in the function of OCA-Bin a reconstituted system (see above). To investigate this possibility,GST fusion proteins containing residues 171 to 256 of either wild-typeOCA-B or the B mutant protein were employed in pull-down assaysto search for a nuclear extract factor(s) capable of interactingwith the OCA-B activation domain. As shown in the immunoblot analysisof Fig. 4, the functional (nonphosphorylated) form of PC4 boundto a wild-type OCA-B-GST fusion protein but not to the mutantB-GST fusion protein (or GST alone) (compare lanes 4 and 5 tolanes 2 and 3). This result is consistent with a direct role forPC4 in mediating OCA-B function through the OCA-B activation domain.Purified recombinant PC4 bound to OCA-B in the same fashion (datanot shown), suggesting that the OCA-B-PC4 interaction is direct.

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FIG. 4. Identification of PC4 as a potential downstream target for the function of OCA-B. The rationale for this experiment is explained in the text, and experimental details are described in Materials and Methods. Note that only a portion (residues 171 to 256) of wild-type (WT) OCA-B and the B mutant (Mut.) protein was fused to GST. + and ++ represent two (lower and higher, respectively) concentrations of immobilized GST or GST fusions. Inp. NE, input nuclear extract.

A redundant activity for PC4 function in a crude system. Given that OCA-B can function in crude HeLa nuclear extracts to activate the Ig promoters, it was of interest to explore apossible role of PC4 in the coactivation pathway in the crudetranscription system on the grounds that it may contain a morecomplete complement of nuclear factors. To this end, the PC4 proteinwas quantitatively removed by immunodepletion from a HeLa nuclearextract (Fig. 3A, right panel) and the PC4-depleted extract wasanalyzed for the ability to transcribe the Oct-1/OCA-B-dependentIgH promoter and a control Sp1-dependent promoter (Fig. 5). Surprisingly,the PC4-deficient nuclear extract (lanes 7 to 10) was as potentas the mock-depleted nuclear extract (lanes 3 to 6) in transcribingboth templates and OCA-B functioned equally well in PC4⁺ and PC4 extracts to stimulate the IgH promoter (compare lanes 5 and 6to lanes 9 and 10) to a level similar to that observed in a B-cellextract (lane 2). These results suggest the presence of a redundantactivity capable of compensating for the loss of PC4 in the crudenuclear extract. Such an activity is likely missing from the chromatographicallypurified USA fraction, making PC4 an essential component for thefunction of Oct-1/OCA-B in the reconstituted system.

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FIG. 5. PC4 depletion (Dep.) from a nuclear extract (NE) does not affect the transcription of either octamer/Oct-dependent (IgH) or -independent (2×Sp1) promoters, suggesting a potential redundant activity for PC4 in the nuclear extracts. Untreated HeLa (lane 1), Namalwa (B cell; lane 2), mock-depleted HeLa (lanes 3 to 6), and PC4-depleted HeLa nuclear extracts were used to transcribe the promoters in the absence or the presence (+) of PC4 (50 ng) and/or OCA-B (20 ng), as indicated. While the transcription level of the control template (2×Sp1) is constant in all lanes, the IgH promoter responds to OCA-B in either mock-depleted (lanes 5 and 6 versus lanes 3 and 4) or PC4-depleted (lanes 9 and 10 versus lanes 7 and 8) HeLa nuclear extracts to a level similar to that observed in the B-cell extract (compare lanes 5 and 6 and lanes 9 and 10 to lane 2). The control template (2×Sp1) is described in reference 42.

DISCUSSION
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In the present study, targeted mutagenesis, in conjunction with in vitro and in vivo assays, has been used to define domainsof the B-cell-specific coactivator OCA-B that are critical forits proper function with the DNA binding activator Oct-1. Furtherinvestigations aimed at gaining more insights into the mechanismof action of OCA-B revealed a synergism between general coactivatorsPC2 and PC4 in mediating the activation or coactivation by Oct-1/OCA-Band an OCA-B-PC4 interaction that is of apparent functional relevance.Finally, studies with less purified systems revealed a functionalredundancy in general coactivators. Taken together, these studieslead to a refined model of Oct-1/OCA-B function that appears toparallel that of some viral coactivators.

OCA-B domains for recruitment to the promoter. An N-terminal OCA-B domain that shares weak similarity with an E1A region was implicated in Ig promoter targeting throughinteraction with the Oct-1 POU domain. However, it appears thatOCA-B contacts surfaces of both the POU-specific and POU-homeosubdomains of Oct-1 (2, 28), as well as nucleotides in theoctamer element (2, 4), suggesting that several determinantsin OCA-B may act in concert to form a stable DNA-activator-coactivatorternary complex. Supporting this notion is the observation thatseveral OCA-B residues in a region about 20 aa C terminal to domainA (Fig. 1) were shown to be critical for ternary complex formation(14). Because the Oct-1 POU-specific and POU-homeo subdomainscontact opposite sides of the DNA double helix (20), the octamer-POU-1-OCA-Bternary complex may form a highly stable ringlike structure importantfor high level, long-term Ig promoter-enhancer function in activatedB cells.

An OCA-B domain involved in promoter activation and general coactivator requirements for its function. The acidic OCA-B region (domain B in Fig. 1) was shown to be critical for coactivator function (Fig. 2A and B) but not forbinding to Oct-1 or an Oct-1-DNA complex (Fig. 2C). Further confirmingthis notion is the fact that while a Gal4(1-94)-OCA-B fusion proteinfunctions as an activator on promoters containing Gal4 bindingsites (13, 53), a mutant with a deletion encompassing domainB loses the activation capability (53). Protein-protein interactionassays also suggest that domain B of OCA-B provides a determinantfor the interaction with the general coactivator PC4 (Fig. 4).Given its ability to interact with wild-type OCA-B but not themutant B version, PC4 appears to be a genuine downstream targetfor the function of OCA-B. This is in accordance with the essentialrole for PC4, and its synergism with general coactivator PC2,in supporting the optimal function of Oct-1/OCA-B in a reconstitutedsystem. Since PC4 alone is as potent as the USA fraction in mediatingthe function of Gal4-based artificial activators on synthetictemplates with multiple Gal4-binding sites in the same reconstitutedsystem (e.g., reference 11), the PC4-PC2 synergism that wasobserved for the function of Oct-1/OCA-B may reflect the use ofcoactivators in the more physiological context of a natural activatorand promoter. It is relevant to note that USA was originally identifiedas a crude coactivator fraction capable of mediating high levelsof activation by natural activators Sp1, USF (34), and NF $kappa$ B(23), and, at least for Sp1-dependent activation, USA-derivedfractions were not as active as partially purified USA (34).A separate study (9) also has shown synergism between PC4 andPC2 in mediating activation by thyroid hormone receptor in conjunctionwith a ligand-dependent activating complex.

A model for Oct-1/OCA-B function. On the basis of both earlier work and the new findings shown here, we present a refined model for the function of Oct-1/OCA-B(Fig. 6). OCA-B is recruited to the target Ig promoter throughprimary interaction with the Oct-1 POU domain, which may precedeOct-1-DNA interactions (30, 31), and through secondary interactionswith DNA (2, 4). In conjunction with Oct-1, OCA-B then providesan activation function. Given the documented physical and functionalinteraction between OCA-B and PC4, the OCA-B activation domainmay function by influencing the basal transcription machinerywith PC4 as an adapter (11). It is important to note that thedefined activation domain(s) (ACT; 12, 37, 55) in the Octfactors also plays a key role in promoter activation because itsremoval, while not abrogating the OCA-B recruitment, is detrimentalfor OCA-B coactivation (31), suggesting a synergism betweenthe activation domain in OCA-B and that in Oct-1 and -2. Thissynergism parallels the synergism between PC4 and PC2 that isrequired for the proper function of Oct-1/OCA-B in the reconstitutedsystem, raising the intriguing possibility of a functional (orphysical) interaction of PC2 and the Oct activation domain(s).Since PC2 is a potent but less well-characterized activity amongthe USA-derived coactivators (reviewed in reference 18), itssynergism with PC4 in mediating the function of OCA-B/Oct-1 mayprovide a useful assay for its further characterization. A redundantactivity (X in Fig. 6) is also implied by the PC4 depletion analysisin crude extracts (see below). The model also indicates the basisfor the loss of function of the OCA-B A (deficiency in interactionwith Oct-1 and -2) and B (deficiency in interaction with PC4,and potentially the redundant activity [X], that also leads toa dominant negative phenotype) mutant proteins.

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FIG. 6. Model for OCA-B function. Mut., mutant; GTF, general transcription factors; ACT, activation domain(s) of Oct-1 and -2; Pol II, RNA polymerase II. Asterisks denote the activation domains in either OCA-B or Oct-1 and -2. The dashed lines indicate that, in addition to contacting residues within the octamer motif (2, 4), OCA-B may also contact downstream sequences, as revealed by a footprinting assay (32). See the text for a full description of the model.

Functional analogy of OCA-B to viral coactivators. By several criteria, OCA-B is a cellular counterpart of at least two viral coactivators, namely, the adenovirus E1A and HSVVP16 proteins. E1A is a promiscuous coactivator capable of interactingwith a number of cellular DNA binding activators that includeUSF, Sp1, the ATF family, c-Jun (29), and Oct-4 (49) via theirdiverse DNA binding motifs and thus possesses the potential toregulate the transcription of multiple genes lacking a commonpromoter element. Of interest in relation to OCA-B is the observationthat an E1A region (residues 179 to 193 in 13S E1A) implicatedin promoter targeting (29) overlaps the E1A region (residues180 to 203) that shares weak sequence similarity with OCA-B domainA (Fig. 1), which is implicated in Ig promoter targeting throughinteraction with the Oct-1 POU domain (Fig. 2C).

Weak (and short) sequence similarity notwithstanding, the functional analogy between OCA-B and E1A is probably best exemplifiedby the activation of reporter genes with an octamer-containingenhancer in embryonal carcinoma (EC) cells (49). First, in differentiatedEC cells, the reporter genes can be stimulated by Oct-4 (alsonamed Oct-3) and 13S E1A in a synergistic fashion; second, asis the case for Oct-1/OCA-B function; activation domains fromboth the activator (Oct-4) and the coactivator (E1A) are jointlyrequired for optimal enhancer function; third, Oct-4, E1A, andoctamer DNA form a ternary complex, as revealed by gel shift analysis;finally, in undifferentiated EC stem cells, a high level of activationcan be achieved by endogenous Oct-4 alone. Given all of theseparallels, it is reasonable to postulate that Oct-4 functionsin undifferentiated EC stem cells with an E1A functional homologthat may be a member of a cellular coactivator family representedby OCA-B.

OCA-B also shows a remarkably close resemblance to the viral coactivator VP16 with respect to both interactions and mechanismof activation. VP16 activates HSV immediate-early genes by engagingin the formation of a multiprotein-promoter complex in conjunctionwith Oct-1 and another host cell factor (reviewed in references5 and 15). Like OCA-B, VP16 interacts with promoter-boundOct-1 through the POU domain (e.g., references 26 and 43)and has both a DNA binding activity contingent on Oct-1 bindingto DNA (25, 52; reviewed in references 5 and 15) andan acidic activation domain that has the potential to interactwith the general cofactor PC4 (11). The observation that, inboth cases, mutations in the activation domains either severelyweaken or abolish the ability to interact with PC4 (11 and thiswork) further supports the functional relevance of a PC4-activationdomain interaction. The function and direct interaction of PC4with several defined acidic activation domains, including thoseof AH, IE, E1A, VP16 (11), and OCA-B (this work) strongly arguefor the role of PC4 as an adapter that bridges promoter-boundtranscription factors and cofactors to the basal transcriptionalmachinery by interacting with TFIIA (11) and/or RNA polymeraseII (33). Finally, given the recent identification of a specializedOct-1 cofactor activity involved in the S-phase activation ofan octamer-dependent H2B promoter (32), it is probable thatat least some cellular genes are controlled by gene-specific coactivatorsthat function analogously to viral coactivators and are representedby OCA-B.

Redundancy in general coactivator function. In sharp contrast to the observation that PC4 is essential for the Oct-1/OCA-B function in a reconstituted system, PC4 isdispensable for the function of Oct-1/OCA-B in a crude (nuclearextract) system (Fig. 5). This suggests the existence of a redundantactivity that is missing in the purified components used in thereconstituted assay system. This redundant activity (X in Fig.6) may serve as an alternative adapter capable of mediating theOCA-B-general transcription factor interaction, thus bypassingthe requirement for PC4 in a crude transcription system. Indeed,a potential candidate for such an activity has been detected bypurification methods (60). Functional redundancy could be ahallmark of regulatory pathways in transcription. Thus, despitean absolute requirement of TATA box binding protein-associatedfactor (TAFS) for activator function in purified reconstitutedsystems (reviewed in, e.g., reference 57), studies with yeast(conditional knockout; 1, 36, 59) and less-purified humancell-free systems (40) challenge the view of a universal roleof TAFs in promoter activation and imply the existence of a distinctclass of functionally redundant activities (e.g., those presentin the RNA polymerase II holoenzyme [reviewed in references 3,21, and 38]) that may act through distinct mechanisms. Asis the case for the function of OCA-B, this implies alternativepathways for communication between activators and/or coactivatorsand the basal transcription machinery.

ACKNOWLEDGMENTS
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Y.L. thanks M. Kretzschmar and S. Malik for generous gifts of general factors and cofactors used in pilot experiments. Wealso thank other members of the Roeder laboratory for encouragementand stimulating discussions.

This work was funded by NIH grant CA43567 and by a Johnson and Johnson Focused Giving Award.

FOOTNOTES

^* Corresponding author. Mailing address: Laboratory of Biochemistry and Molecular Biology, The Rockefeller University, New York,NY 10021-6399. Phone: (212) 327-7600. Fax: (212) 327-7949. E-mail:roeder{at}rockvax.rockefeller.edu.

Present address: Laboratory of Molecular Embryology, National Institute of Child Health and Human Development, National Institutesof Health, Bethesda, MD 20892-5431.

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1.	Apone, L. M., C. A. Virbasius, J. C. Reese, and M. R. Green. 1996. Yeast TAF_II90 is required for cell-cycle progression through G2/M but not for general transcription activation. Genes Dev. 10:2368-2380[Abstract/Free Full Text].
2.	Babb, R., M. A. Cleary, and W. Herr. 1997. OCA-B is a functional analog of VP16 but targets a separate surface of the Oct-1 POU domain. Mol. Cell. Biol. 17:7295-7305[Abstract].
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