The Human Factors YY1 and LSF Repress the Human Immunodeficiency Virus Type 1 Long Terminal Repeat via Recruitment of Histone Deacetylase 1

doi:10.1128/JVI.74.15.6790-6799.2000

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Journal of Virology, August 2000, p. 6790-6799, Vol. 74, No. 15
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

The Human Factors YY1 and LSF Repress the Human Immunodeficiency Virus Type 1 Long Terminal Repeat via Recruitment of Histone Deacetylase 1

Jason J. Coull,¹ Fabio Romerio,² Jian-Min Sun,³ Janet L. Volker,⁴ Katherine M. Galvin,⁵^, James R. Davie,³ Yang Shi,⁵ Ulla Hansen,⁴^, and David M. Margolis¹^,^*

Division of Infectious Diseases, University of Texas Southwestern Medical Center, Dallas, Texas 75390-9113¹; Institute of Human Virology, University of Maryland Biotechnology Institute, Baltimore, Maryland 21201²; Department of Biochemistry and Molecular Biology, Faculty of Medicine, University of Manitoba, Winnipeg, Manitoba, Canada R3E OW3³; and Division of Molecular Genetics, Dana-Farber Cancer Institute and Harvard Medical School,⁴ and Department of Pathology, Harvard Medical School,⁵ Boston, Massachusetts 02115

Received 4 November 1999/Accepted 27 April 2000

	ABSTRACT

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Enigmatic mechanisms restore the resting state in activated lymphocytes following human immunodeficiency virus type 1 (HIV-1)infection, rarely allowing persistent nonproductive infection.We detail a mechanism whereby cellular factors could establishvirological latency. The transcription factors YY1 and LSF cooperatein repression of transcription from the HIV-1 long terminal repeat(LTR). LSF recruits YY1 to the LTR via the zinc fingers of YY1.The first two zinc fingers were observed to be sufficient forthis interaction in vitro. A mutant of LSF incapable of bindingDNA blocked repression. Like other transcriptional repressors,YY1 can function via recruitment of histone deacetylase (HDAC).We find that HDAC1 copurifies with the LTR-binding YY1-LSF repressorcomplex, the domain of YY1 that interacts with HDAC1 is requiredto repress the HIV-1 promoter, expression of HDAC1 augments repressionof the LTR by YY1, and the deacetylase inhibitor trichostatinA blocks repression mediated by YY1. This novel link between HDACrecruitment and inhibition of HIV-1 expression by YY1 and LSF,in the natural context of a viral promoter integrated into chromosomalDNA, is the first demonstration of a molecular mechanism of repressionof HIV-1. YY1 and LSF may establish transcriptional and virologicallatency of HIV, a state that has recently been recognized in vivoand has significant implications for the long-term treatment ofAIDS.

	INTRODUCTION

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A subpopulation of stably infected CD4⁺ T lymphocytes containing integrated proviral DNA capable of producing virus upon stimulationhas been identified in human immunodeficiency virus (HIV)-positiveindividuals (6, 7, 8, 15, 69). As antiretroviraltherapy now allows significant inhibition of active HIV type 1(HIV-1) replication, an understanding of factors that establishor maintain the integrated proviral state takes on new relevance.Potent repression of long terminal repeat (LTR) transcriptioncould allow an activated, infected cell to return to the restingstate and establish a stable nonproductive infection. This mayoccur via changes in local chromatin architecture surroundingthe HIV promoter. While activation of the HIV LTR has been shownto be associated with changes in chromatin structure (13, 46,51, 61-64), factors that result in durable repression of LTRexpression are less wellknown.

We have identified two cellular factors, YY1 ( $delta$ , NF-E1, UCRBP, or CF1 [45, 52, 56, 40, 70]) and LSF (CP-2, LBP-1c,or UBP-1 [22, 26, 38, 40, 70]), that cooperate uniquelyin recognition of the region $-$ 10 to +27 of the HIV-1 LTR (referredto as the RCS [repressor complex sequence]). These have been shownto specifically and synergistically repress HIV LTR expressionand viral production (41, 49). Antibodies to either YY1 orLSF inhibit RCS complex formation, and mutations within the LTRthat eliminate LSF binding and RCS complex formation ablate repressionmediated by YY1 and/or LSF (41).

YY1, a zinc finger-containing transcriptional regulator with homology to the GLI-Krüppel family of proteins, is a ubiquitouscellular factor with the ability both to activate and repressgene expression (16, 32, 52, 56). YY1 has two N-terminaltransactivation domains, while the C-terminal domain is requiredfor direct DNA binding and for repression of some promoters (2,4, 17). This broad spectrum of activity has been attributedto bending of DNA, interactions with other factors, or posttranscriptionalmodification of YY1 (52). However, activity depends on the promotercontext and specific protein-protein interactions that YY1 establisheswith other regulatory proteins (23, 32-34, 49, 50, 53,71-73, 77) and with general transcription factors (5, 61).

LSF is the predominantly expressed member of a family of proteins (also termed LBP-1a, -1b, -1c, and -1d) that are producedfrom the differential splicing from two related genes (55, 74).All bind DNA except for LSF-ID (LBP1-d), which lacks a centralencoding exon. LSF can bind the HIV LTR, and binding is associatedwith direct repression of transcription in vitro (18, 29,44). However, this effect has not been observed in vivo, astransient expression of LSF alone had no observable effect onexpression from the HIV LTR (49, 74, 76).

Genetic and biochemical studies have established that chromatin in living cells critically affect the transcriptional competenceof a promoter sequence (3, 14, 36, 58, 68). A numberof recent reports have documented the importance of histone deacetylases(HDACs) as the effector molecules of transcriptional downregulationin many genes (11, 20, 25, 39, 47). In addition, severaltranscriptional repressors that tether HDACs to the promoter havebeen described (2, 3, 21, 28, 31, 42, 43, 72,73, 75).

To determine the domains of YY1 and LSF that participate in complex formation and regulation of the HIV promoter, we mappedthe interactions of LSF and YY1 by using a number of chimericYY1 and truncated LSF constructs. Our findings suggested a novelmolecular mechanism of repression of an integrated HIV provirusin vivo, wherein LSF is required for recruitment of YY1 to theHIV LTR, and repression is mediated by YY1 via the action ofHDAC.

We find that the YY1-LSF complex copurifies with HDAC1, identified by both Western blot analysis and enzymatic activity assay.Deletion of a glycine/alanine-rich domain of YY1, previously shownto specifically direct the interaction between YY1 and HDAC (72),ablates the ability of YY1 to repress the HIV-1 LTR. Further YY1-mediatedrepression of the LTR is ablated by the deacetylase inhibitortrichostatin A. This is the first time that the molecular mechanismby which the YY1-LSF complex represses HIV-1 transcription hasbeen described and represents another important biological circumstancewhereby the action of a transcriptional repressor is mediatedby anHDAC.

	MATERIALS AND METHODS

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Nuclear extracts. Large-scale preparation of nuclear extract from CEM cells for chromatographic purification of the RCS complex were preparedas described previously (12), with the following minor modifications:buffers A and C were supplemented with 1 mM NaF, 1 mM Na₂VO₄,10 µg of leupeptin per ml, 10 µg of aprotinin per ml, and 1 µgof pepstatin A per ml. Chymostatin (1 µg/ml) was also added tobuffer A, and 50 mM $beta$ -glycerophosphate was added to bufferC.

Ion-exchange chromatography. Activated P11 phosphocellulose (Whatman, Clifton, N.J.) was equilibrated with 50 mM NaCl-50 mM HEPES (pH 7.9)-10% glycerol-0.2mM EDTA-0.5 mM phenylmethylsulfonyl fluoride (PMSF)-0.5 mM dithiothreitol(DTT). CEM cell nuclear extract was loaded at 0.4 ml/min, washed,and eluted in a linear gradient of 50 mM to 1 M NaCl. Fractionsshown by Western blotting with anti-YY1 antibody ( $alpha$ -YY1; C-20;Santa Cruz Biotechnology, Santa Cruz, Calif.) to contain YY1,and shown by electrophoretic mobility shift assay (EMSA) to containRCS-binding activity, were pooled and dialyzed against 20 mM Tris-HCl(pH 7.9)-10% glycerol-0.2 mM EDTA-0.5 mM PMSF-0.5 mM DTT-50 mMNaCl before DEAE-cellulose chromatography. A DEAE-cellulose DE52column (Whatman) was loaded with pooled fractions at 0.2 ml/min.The column was washed and eluted, and fractions were analyzedas described above. Fractions positive both in Western blot andgel shift analyses were subjected to further purification by DNAaffinitychromatography.

DNA affinity chromatography. A double-stranded oligonucleotide spanning positions $-$ 10 to +27 of the HIV-1 LTR was ligated and coupled to cyanogen bromide-activatedSepharose CL-4B (Pharmacia, Piscataway, N.J.) as previously described(27). Active fractions from DEAE-cellulose chromatography wereequilibrated in buffer Z (25 mM HEPES [pH 7.6], 0.1 M NaCl, 20%glycerol, 12.5 mM MgCl₂, 1 mM DTT, 0.5 mM PMSF, 0.1% Nonidet P-40).Affinity resin was washed extensively with buffer Z without glyceroland Nonidet P-40. Fractions were incubated for 10 min at 4°C with10 µg of dI-dC per ml, loaded by gravity, washed, and eluted witha step gradient of 0.1 to 1 M NaCl. Western blot analysis fordetection of HDAC was performed using a rabbit polyclonal antibodyraised against a peptide corresponding to the C-terminal aminoacids 319 to 334 of the molecule (60) and against LSF usingrabbit polyclonal anti-CP2 antiserum (LSF, LBP-1c; gift from M.Sheffery). HDAC assays were performed as previously described(31).

Cell lines, transfections, and assays. Transfections of HeLa cells were performed as previously described (49). HeLa-CD4-LTR (9) cells were grown in Dulbeccomodified Eagle medium supplemented with 10% fetal calf serum andtransfected with 20 µg of plasmid DNA (prepared using an EndoFreeplasmid kit [Qiagen, Valencia, Calif.]) by calcium phosphate coprecipitationas instructed by the manufacturer (ProFection system; Promega,Madison, Wis.). After 30 min at room temperature, the solutionwas added to the cells (2.5 × 10⁵ to 4 × 10⁵ cells/plate). Twelve hours after transfection, the cells werewashed with phosphate-buffered saline (PBS) and fed fresh medium.Forty-eight hours later, the cells were harvested, cellular extractswere prepared, and chloramphenicol acetyltransferase (CAT) assaysperformed as previously described (49). To control for the effectof transcription factor overexpression on general cellular promoters,a reporter construct driven by the $beta$ -actin promoter, pH $beta$ -actin-luciferase(67), was used in cotransfection and CAT expression normalizedfor luciferase activity. Other plasmids used have been previouslydescribed (2, 49). Luciferase assays were performed at 48h as suggested by the manufacturer of the luciferase assay system(Promega), but cells were resuspended in 200 µl of lysis buffer,and one freeze-thaw step was performed. Up to 30 µl of cellularextract (normalized for protein concentration) in a final volumeof 130 µl was used for luciferasereactions.

For virus production experiments, 2 × 10⁴ HeLa cells were transfected with 10 µl of Superfect (Qiagen) and 2.5 to 3.0 µg ofDNA in a volume of 0.6 ml for 3 h, washed with PBS, and then grownin 2 ml. Aliquots of culture medium were sampled for detectionof HIV-1 p24^gag protein by antigen capture enzyme-linked immunosorbent assayas instructed by the manufacturer (Coulter Corporation, Hialeah,Fla.).

Immunoprecipitation and EMSA. Immunoprecipitation was performed with nuclear extracts prepared from a Jurkat T-cell line (49). Twenty-microliter samplesof extract were mixed with antibody (rabbit immunoglobulin G; $alpha$ -YY1-C20 [Upstate Biotechnology, Lake Placid, N.Y.] or $alpha$ -LSF[gift from M. Sheffery and S. Swendenmann]) at 4°C for 1 h; 5µl $alpha$ -rabbit IgG agarose-conjugated antibody (Sigma, St. Louis,Mo.) was added, and incubation was continued for 1 h. The complexwas precipitated by centrifugation at 3,000 rpm and 4°C for 5min. The pellet was washed three times with PBS and resuspendedin 30 µl of sodium dodecyl sulfate-polyacrylamide gel electrophoresis(SDS-PAGE) sample buffer before separation by SDS-PAGE and Westernanalysis with $alpha$ -YY1 or $alpha$ -LSF. Bands were visualized using horseradishperoxidase-conjugated $alpha$ -rabbit IgG(Sigma).

Histidine-tagged YY1 (His-YY1) and His-LSF were expressed and harvested in Escherichia coli as previously described (53,65). The RCS oligonucleotide ( $-$ 10 to +27 of HIV-1 LTR [49])was end labeled, and 10⁴ cpm was incubated with various amounts of His-LSF for 20 minat 25°C. Glutathione S-transferase (GST)-YY1 or His-YY1 was added,total protein content was normalized by the addition of bovineserum albumin, and the reaction continued for 30 min. EMSA wasthen performed as previously described (49). Supershifts wereperformed by addition of either concentrated $alpha$ -YY1 (C20-X; SantaCruz Biotechnology, Santa Cruz, Calif.) or $alpha$ -LSF (65) to thereactionmixture.

In vitro protein interaction mapping. GST-YY1/GFI-1 chimeras (17) and GST-LSF deletion (54, 55) constructs were expressed and harvested in E. coli as previouslydescribed. Proteins were visualized by Coomassie brilliant bluestaining, and protein content was normalized by densitometricanalysis. LSF was transcribed and translated in vitro by T7 RNApolymerase in rabbit reticulocyte (Promega) in the presence of[³⁵S]methionine as instructed by the manufacturer (54). Followingcapture of GST-YY1/GFI-1 chimera proteins on glutathione-agarosebeads, equal volumes of beads were incubated with [³⁵S]methionine-labeled LSF in incubation buffer (17) for 1 h at4°C. The beads were washed in incubation buffer-100 mM KCl andresuspended in 20 µl of 2× SDS loading buffer. Retained LSF wasseparated by SDS-PAGE (10% gel) dried, and visualized by autoradiography.Similarly, YY1 was transcribed and translated in vitro, and thenincubated with captured GST-LSF constructs, and retained YY1 wasvisualized by autoradiography followingelectrophoresis.

	RESULTS

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YY1 and LSF interact in vivo. Complex formation at the RCS can be ablated by either $alpha$ -YY1 or $alpha$ -LSF, suggesting that both YY1 and LSF are necessary to formthis regulatory complex (49). We sought evidence that thesefactors interacted directly in the absence of a DNA-binding sequence.Jurkat CD4⁺ T-cell nuclear extracts were incubated with $alpha$ -YY1, $alpha$ -LSF, ora nonspecific rabbit polyclonal antiserum. Antibody-protein complexeswere precipitated by addition of $alpha$ -IgG-agarose beads and centrifugation.Precipitates were then assayed for the presence of LSF by Westernblot analysis. Immunoprecipitation was specific, as only traceamounts of LSF were recovered by the nonspecific antiserum. $alpha$ -YY1precipitated approximately 75% of the LSF activity that couldbe recovered by $alpha$ -LSF (Fig. 1A). This indicates that LSF interactswith YY1 in vivo in the absence of the HIV RCS-binding site andsuggests that direct protein-protein interaction between YY1 andLSF is necessary for complex formation at the HIV LTR.

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FIG. 1. YY1 and LSF associate in vivo and in vitro, in the absence of a DNA-binding site or other factors. (A) Immunoprecipitations of Jurkat nuclear extracts using either $alpha$ -YY1, $alpha$ -LSF, or a nonspecific rabbit polyclonal antiserum. Mock immunoprecipitations (IP) were performed in the absence of antibody. Precipitates were assayed by Western blot using $alpha$ -LSF. Approximately 75% of the LSF protein recovered by $alpha$ -LSF is also immunoprecipitated by $alpha$ -YY1. To demonstrate the recognition of YY1, a Western blot of input nuclear extract is displayed at the right. (B) EMSA was performed using the RCS-binding site and the indicated amounts of LSF and YY1; total amount of protein was normalized by the addition of bovine serum albumin. The mobility of the native RCS complex formed by nuclear extract is displayed at the right. Nonspecific interactions with the RCS are indicated. (C) Complexes supershifted by the addition of either $alpha$ -YY1 or $alpha$ -LSF. Addition of $alpha$ -YY1 had no effect on the LSF complexes in the absence of YY1 protein (not shown).

LSF and YY1 associate without cofactors in vitro. Romerio et al. (49) showed that both LSF and YY1 form a complex at the RCS site of the HIV LTR. It was not known whetherLSF and YY1 were sufficient to form this complex. We sought toreconstitute this complex in vitro, in the absence of other factors.Histidine-tagged recombinant LSF and YY1 proteins were expressedand harvested from E. coli and allowed to interact with an oligonucleotideencoding the HIV LTR RCS. Up to 100 ng of His-YY1 alone did notform a detectable specific complex with the RCS (Fig. 1B), althougha low-molecular-weight band was observed when some protein ornuclear extract preparations were used. This band became moreintense with the age of the preparation, suggesting it was theresult of protein degradation. Ten nanograms of LSF, however,formed a specific EMSA band (Fig. 1B and C). The addition of increasingamounts (20 to 100 ng) of YY1 resulted in increasing levels ofcomplex formation in the presence of 10 ng of LSF (Fig. 1B). Aslittle as 20 ng of His-LSF induced a very prominent protein-DNAcomplex (Fig. 1C), similar to previous studies (18, 26). Underthese conditions, no additional effect of YY1 was discernible.YY1 specifically enhanced RCS complex formation in the presenceof low amounts of LSF, as all reactions were normalized for totalprotein content by the addition ofBSA.

RCS protein-DNA complexes were supershifted by either $alpha$ -YY1 or $alpha$ -LSF (Fig. 1C), confirming that these complexes containedboth LSF and YY1. $alpha$ -LSF completely shifted the RCS complex, whereasunder these conditions only a fraction of complexes were supershiftedby the addition of excess $alpha$ -YY1. The quantity of $alpha$ -YY1 (5 µl)completely supershifted YY1 complexes formed on a canonical adeno-associatedvirus P5-binding site (data not shown). One interpretation ofthese results is that all complexes bound to DNA in these conditionscontain LSF multimers (54, 55), but all complexes do not containYY1 accessible to antibody. The effect of the antibody was specific,as $alpha$ -YY1 had no effect on the mobility of the complex in the absenceof YY1 protein (data not shown). Although other factors may bepresent in the RCS complex in vivo, YY1 and LSF are sufficientto form a complex at theRCS.

The addition of YY1 to LSF bound to the RCS was not associated with a further change in the mobility of the DNA-protein complex.As LSF (64 kDa) binds other sites as a tetramer (54), it ispossible that YY1 (apparent molecular mass of 68 kDa) replacesLSF molecules within the RCS complex. Alternatively, the additionof YY1 to the multimeric LSF might not significantly affect complexmobility in the native electrophoresis conditionsused.

Interaction domains of YY1 and LSF. The interaction of LSF with YY1 was mapped using constructs that contained a series of nested deletions within the codingregion of LSF (Fig. 2A). Neither the carboxyl nor amino terminusof LSF was required for interaction with YY1. However, the centralregion of the protein was required for interaction with YY1, asamino-terminal deletions beyond amino acid 164 and carboxy-terminaldeletions prior to amino acid 403 resulted in marked diminutionof the ability of LSF to bind YY1 (Fig. 2B). Binding was lostaltogether when C-terminal sequences between amino acid residues308 and 368 were removed. Further amino acid substitutions withinthis region, which impair multimerization (55), markedly decreasedthe ability of the mutant LSF to bind full-length YY1. A likelypossibility is that LSF recognizes YY1 only in its multimericconformation.

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FIG. 2. Mapping of the YY1-LSF interaction domains. (A) Representation of wild-type (wt) LSF and LSF deletion mutants used to identify the region of interaction between LSF with YY1. $Delta$ X, deletion up to codon X; X $Delta$ , deletion after codon X; XX, mutated single codons. The amount of LSF bound to GST-YY1 varied from 2.5 to 7% of the input, depending on the experiment. All values were normalized to the amount of wild-type LSF bound to GST-YY1 in the experiment. (B) Representative autoradiographs showing input LSF constructs and LSF constructs retained by GST-YY1 and by GST. (C) Graphical representation of the YY1 chimeras, all of which contained the GST tag. All constructs also contained the N-terminal region of YY1 (amino acids 1 to 294) except YY1 Zn Fingers, which lacked this region. YY1 is the full-length wild-type YY1 molecule. Nonshaded regions represent GFI-1 zinc fingers (related to Krüppel zinc finger proteins). GFI contains only GFI-1 zinc fingers, Chi 1 contained the first YY1 zinc finger, Chi 2 contained the first two YY1 zinc fingers, Chi 5 contained the last two YY1 zinc fingers, Chi 7 contained the second YY1 zinc finger only, and YY1 Zn Fingers contained all four YY1 zinc fingers without the YY1 amino-terminal region. The first two zinc fingers of YY1 are required for optimal binding of LSF. Chi 1, Chi 2, Chi 7, and YY1 bound LSF, whereas Chi 5, GFI-1, and GST exhibited background levels of LSF binding. A lane containing only a diluted aliquot of labeled LSF serves as a marker. When normalized for protein concentration, a construct expressing only the YY1 zinc fingers fused to GST binds LSF as avidly as intact GST-YY1. Background levels of binding varied between experiments, as shown.

YY1 DNA-binding activity and many YY1-protein interactions map to the carboxyl-terminal zinc fingers of the molecule. Therefore,YY1 interaction domains were mapped using chimeric YY1 recombinants(Fig. 2C). These chimeras expressed GST fused to the N-terminaldomain of the protein and had various numbers of YY1 zinc fingerdomains replaced by the structurally homologous GFI-1 zinc fingers(17). No deleterious effect on function or stability of YY1was observed (17). Figure 2C shows that the interaction withLSF did not require the third and fourth zinc fingers of YY1.LSF bound in vitro to constructs that contained YY1 zinc finger1 or 2, or both. In these assays, chimera 2, which expresses zincfingers 1 and 2, bound LSF more avidly than intact YY1. Chimera1 bound LSF nearly as well as YY1, while chimera 7 could bindLSF in vitro but less avidly. Thus, either zinc finger allowedbinding to LSF, but binding was optimal when both fingers werepresent. Chimera 5, containing only the last two zinc fingersof YY1, did not bind LSF. The GST-Y/GFI-1 construct containingthe entire YY1 amino-terminal domain fused to the zinc fingerdomain of the GFI-1 protein retained minimal amounts of LSF. Finally,a chimera expressing only the YY1 zinc finger domains, and lackingthe entire amino-terminal YY1 region, bound LSF at least as wellas intact YY1. Therefore, YY1 requires only zinc fingers 1 and2 to recognizeLSF.

LSF competent to bind DNA is required for repression of HIV LTR expression. Shirra and Hansen (54) and Shirra et al. (55) demonstrated that LSF binds a canonical simian virus 40 late promoter sitevia the formation of homotetramers. Further, binding can be blockedby the expression of a dominant negative mutant defective in DNAbinding but with remaining ability to multimerize (LSF 234QL/236KEor dnLSF). We performed experiments to test the effect of dnLSFusing the HeLa-CD4-LTR cell line (9). The LTR reporter carriedby this cell line exists within the native chromatin structureof the genome. Transfection of YY1 inhibited Tat-activated CATactivity in these cells (Fig. 3), in agreement with previous studiesusing plasmid-based reporters (49). In the setting of a chromosomallyintegrated reporter gene, the provision of LSF augmented repressionmediated by YY1, confirming the effect of YY1 and LSF on an integratedHIV-1 promoter. Significantly, dnLSF abolished the ability ofYY1 to repress CAT expression, confirming that LSF capable ofbinding DNA is required to allow YY1 to repress HIV-1 LTR expression(Fig. 3). As in previous studies (49), these effects were specificto the HIV LTR; results are normalized to the expression of acotransfected $beta$ -actin-luciferase reporter gene, whose expressionwas not significantly affected by YY1, LSF, or dnLSF (not shown).

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FIG. 3. Repression by YY1 and LSF requires functional LSF and HDAC interaction-competent YY1. Expression of an integrated LTR-CAT reporter in HeLa-CD4-LTR cells, when activated by 200 ng of pAR-Tat, was inhibited by 2.5 µg of CMV-YY1 or 2.5 µg of both CMV-YY1 and CMV-LSF; 2.5 µg of CMV-LSF had no effect on expression of CAT; 2.5 µg of dnLSF (pCMV-LSF 234QL/236KE), incapable of binding DNA but capable of forming inactive multimers, blocked inhibition of Tat-activated LTR expression by 2.5 µg of YY1; 2.5 µg of CMV-YY1 $Delta$ 154-199, incapable of interacting with HDAC, was unable to inhibit Tat-activated expression. All transfections received a total of 5 µg of CMV promoter-driven plasmid. Data are from at least four independent transfections, normalized for expression of cotransfected $beta$ -actin-luciferase.

Copurification of HDAC with the YY1-LSF complex. YY1 can act via the recruitment of HDACs (72, 73). As a nucleosome is present near the RCS when the HIV-1 LTR is integrated(46, 51, 62), we examined whether a histone deacetylasewas present in the RCS DNA affinity chromatography fractions.The YY1-LSF complex was purified by phosphocellulose P11, DEAE-cellulosecolumn, and DNA affinity chromatography as previously described(49). YY1, LSF, and the RCS-binding activity copurified in the0.3 and 0.4 M NaCl fractions of the final step of purification(Fig. 4A). RCS-binding activity was enriched about 10,000-foldby this procedure. As shown in Fig. 4A, a rabbit polyclonal antibodyraised against amino acids 319 to 334 of HDAC1 was able to detecta protein with apparent molecular mass of 66 kDa in the 0.3 and0.4 M NaCl pooled fractions. HDAC1, a 55-kDa protein, migratesat this apparent molecular mass in our gel system (59).

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FIG. 4. YY1, LSF, and HDAC1 copurify with RCS-binding activity. (A) Activities of crude nuclear extract and elution fractions from an RCS DNA affinity chromatography column. Shown are results of EMSA using the RCS probe (top panel), and of Western blotting using rabbit polyclonal $alpha$ -YY1 (second panel), rabbit polyclonal $alpha$ -CP2 (LSF) (third panel), and rabbit polyclonal $alpha$ -HDAC1/2 (bottom panel). EMSA was performed with 4 µg of nuclear extract (NE) and 20 ng of DNA affinity column eluate. Western blotting was performed with 20 µg of nuclear extract and 200 ng of DNA affinity column eluate. An arrow indicates the YY1-specific complex, as validated by $alpha$ -YY1 interference in EMSA. Positions of molecular weight markers are indicated in kilodaltons. (B) HDAC activity of DNA affinity chromatography fractions correlates with the presence of the YY1-LSF complex.

To rule out the possibility that these fractions contained a protein immunologically similar but enzymatically unrelated toHDAC, we assayed the HDAC activity of the DNA affinity chromatographyfractions. As expected, the 0.3 and 0.4 NaCl fractions showedstrong HDAC activity, as measured by release of ³H-acetic acid (Fig. 4B). These results indicate that active HDAC1copurifies with the YY1-LSF complex and suggest that the YY1-LSFcomplex represses HIV-1 transcription via the recruitment ofHDAC.

Repression of the HIV-1 LTR by YY1 requires interaction with an HDAC. A recent report has demonstrated that the Gly/Ala-rich domain of YY1 mediates the interaction with the HDAC and is requiredfor repression of the adeno-associated virus P5 promoter by YY1(72). To test whether the mechanism of repression of the HIV-1LTR by YY1 is mediated by an HDAC, we performed a series of transienttransfection experiments using a mutant YY1 deleted of the Gly/Ala-richdomain (YY1 $Delta$ 154-199 [2]) required for interaction withHDAC.

Initial experiments were performed as previously (41, 49), demonstrating that cotransfection of YY1 inhibited Tat-activated,LTR-driven CAT expression. However, YY1 $Delta$ 154-199 was unable toinhibit CAT activity, indicating the absolute requirement of theGly/Ala-rich domain of YY1 for efficient repression of the HIV-1LTR (data not shown). Chromatin remodeling effects on gene activityhave often been imputed in studies using transfected, plasmid-encodedreporter genes that may not reflect the activity of genes containedin native chromatin. However the LTR reporter carried by the HeLa-CD4-LTRcell line (9) exists within the native chromatin structureof the genome. Significantly, YY1 $Delta$ 154-199 failed to repress CATexpression, confirming that the Gly/Ala-rich HDAC interactiondomain is required for repression of the HIV-1 LTR by YY1 (Fig.3). Although YY1 $Delta$ 154-199 activated CAT expression, this effectwas not significant when normalized for modest activation observedof a cotransfected $beta$ -actin-luciferase reporter. Repression wasalso blocked by addition of the specific HDAC inhibitor trichostatinA to the culture medium (data not shown). This is the first demonstrationof both cooperative repression by YY1 and LSF and the lack ofrepression by YY1 $Delta$ 154-199 in the context of a chromosomally integratedHIV-1 promoter. It is also the first demonstration in this contextthat YY1 requires its HDAC interaction domain to mediaterepression.

Repression of the HIV-1 virion production by YY1 requires interaction with an HDAC. Support for the role of HDAC in repression of HIV-1 virion production was demonstrated by cotransfection of HeLa cells withthe infectious molecular clone pNL4-3 (1) or pYU-2 (37) andempty cytomegalovirus (CMV) vector, CMV-YY1, or CMV-YY1 $Delta$ 154-199.As these cells support HIV replication but cannot be infected,a measurement of the effect of YY1 on a single round of viralreplication can be made. The influence of YY1 on viral productionwas assayed by testing of culture supernatant for the presenceof the viral protein p24^gag. Cotransfection with a vector expressing YY1 produced dose-dependentinhibition of either CXCR4 (pNL4-3)- or CCR5 (pYU-2)-tropic virus,whereas cotransfection of YY1 $Delta$ 154-199 failed to inhibit HIV production(Fig. 5). Again, YY1 $Delta$ 154-199 activated HIV expression above normallevels. Similar results were seen in the CD4⁺ T-cell line CEM when transfected with pNL4-3 or pYU-2 and emptyCMV vector, CMV-YY1, or CMV-YY1 $Delta$ 154-199 (data not shown). Thesefindings suggest the possibility of ongoing competition betweenconstitutive cellular YY1 and HIV LTR activating factors. However,as CMV-YY1 $Delta$ 154-199 weakly activated a $beta$ -actin-luciferase reporter,secondary activating effect of YY1 $Delta$ 154-199 on the HIV-1 LTR cannotbe excluded.

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FIG. 5. YY1 directly affects production of HIV in vitro. Production of HIV-1 is inhibited by YY1 but not by YY1 $Delta$ 154-199 lacking the HDAC interaction domain following transfection of HeLa cells with 0.5 µg of the CXCR4 prototypic clone pNL4-3 (left) or 1 µg of the CCR5 prototypic clone pYU-2 (right). Data are representative of three transfections.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

YY1 and LSF interact and cooperate in repression of HIV-1 LTR expression. We show that LSF and YY1 interact with one another both in vitro and in vivo. Interaction was observed in the absence of (i)a DNA-binding site, (ii) other cellular factors, and (iii) YY1C-terminal zinc fingers required for DNA binding to canonicalYY1 sites (Fig. 1 and 2 and reference 17). As a majority ofthe LSF that can be recovered by immunoprecipitation can alsobe recovered in association with YY1, this complex is likely tobe formed in the cell prior to binding to viral regulatory elements.Further evidence of YY1 and LSF interaction is provided by theobservation that YY1 alone does not bind the RCS site in EMSA,but $alpha$ -YY1 supershifted a significant fraction of the RCS-proteincomplex.

Overexpression of LSF alone does not repress transcription from the HIV LTR (49, 76). However, an LTR reporter gene isinhibited by YY1 expression, and this effect is augmented by coexpressionof LSF. This occurs in the context of both plasmid-based (49)and chromatin-based reporter genes (Fig. 3). Further, both YY1and LSF function are required for inhibition of the HIV LTR. Whileexpression of LSF does not significantly inhibit LTR expression,LSF synergizes with YY1 in repression, and dominant negative LSFprevents repression by YY1 (Fig. 3). Consistent with this model,preliminary studies show that the replication of a provirus containingTAR mutations that block RCS formation but allow Tat function(48) is unaffected by YY1 (data notshown).

YY1 is known to interact with a number of cellular factors via a Gly/Ala-rich region within residues 154 to 199 (2). LSF,however, interacts with the zinc finger domain of YY1. The Gly/Aladomain was present on all chimeric YY1 constructs, but only YY1,chimeras 1, 2, and 7, and the YY1 zinc fingers alone were ableto specifically bind LSF in vitro (Fig. 2C). These results indicatethat the first and, to a lesser extent, second zinc finger domainsof YY1 participate in interaction with LSF. While zinc fingersoften mediate DNA binding, examples of protein-protein interactionsmediated by zinc fingers have been documented (3, 19, 30,66). The interaction of YY1 with LSF via its carboxy-terminalzinc fingers creates an attractive model. Within the RCS complex,the amino terminus of YY1 might be accessible for interactingwith other factors, such as HDAC, as well as the nearby basaltranscription complex, the complex of proteins that binds TAR,or nearbynucleosomes.

Taken together, our findings show that LSF is required for recruitment of YY1 to the HIV promoter. LSF may facilitate YY1recognition of the LTR, guiding YY1 onto a site that was inaccessibleor of low affinity in its absence. Alternatively, YY1 may enterthe RCS complex solely through protein-protein interaction withLSF. Given the sensitivity of this interaction to mutations withinthe core of LSF that impair multimerization, it is likely thatYY1 recognizes a structure displayed by LSF multimers. The locationof the RCS within the HIV LTR may position YY1 to directly inhibitthe basal transcription complex or activators of the LTR, as wellas recruit mediators of repression such asHDACs.

Interaction of HDAC with the YY1-LSF repressive complex. The multiprotein complex containing the human factors YY1 and LSF, previously isolated from CEM cells, detected in primaryT cells, and shown to repress the HIV-1 LTR, copurifies with a65-kDa protein which we have identified as HDAC1 (Fig. 4A). Theanti-HDAC antibody used to perform the Western blot analysis wasreactive to both HDAC1 and HDAC2 but not to HDAC3 (73). However,based on the molecular weight found in Western blot analysis (60,72), HDAC1 is likely the protein copurified with YY1 andLSF.

We have demonstrated that the Gly/Ala-rich domain of YY1, which mediates the interaction with HDAC (72), is absolutely requiredfor efficient repression of the HIV-1 LTR by the YY1-LSF complex(Fig. 3). This was not an obvious result, given the many molecularmechanisms of repression that have been attributed to YY1. Thissuggests that recruitment of an HDAC is a necessary event in themechanism of repression of HIV-1 gene expression by YY1. Indeed,the fact that transfection of YY1 $Delta$ 154-199 resulted in modest upregulationof LTR expression and HIV production suggests that LTR expressionmay in part reflect the competing influences of cellular HDACand histone acetyltransferaseactivity.

The Gly/Ala-rich domain has also been shown to mediate interaction between YY1 and the general transcription factors TFIIB,TATA binding protein, and TAF_II55 and with the transcription factorp300/CBP (2). These interactions have been proposed to be relevantfor repression by YY1 through a mechanism of quenching or directrepression (2, 10, 24, 35). Although our studies provideno direct evidence for this speculation, YY1 might utilize multiplemechanisms to repress the HIV-1LTR.

YY1-LSF-HDAC may alter the chromatin structure of the HIV-1 LTR. Studies of the chromatin structure of the integrated HIV-1 provirus in chronically and acutely infected cells lines have detectedthe presence of a large nucleosome-free, DNase I-hypersensitiveregion spanning nucleotides 223 to 450 of the HIV-1 genome. Thiscorresponds to the portion of the LTR including the enhancer andthe promoter regions, up to the transcription start site. Upontreatment with tetradecanoyl phorbol acetate or tumor necrosisfactor alpha, the 3' boundary of the nucleosome-free region wasextended a further 140 nucleotides, indicating the alterationof the nucleosome, termed nuc-1 (51, 62-64). Additional DNaseI-hypersensitive sites and nucleosome-protected regions have beenidentified all along the integrated HIV-1 genome (62, 62).

More recently, Pazin et al. (46) have shown that binding of both Sp1 and the p50 subunit of NF- $kappa$ B to the HIV-1 LTR altersthe local nucleosomal array in vicinity of the HIV-1 promoterand produces the DNase I-hypersensitive region between nucleotides223 and 450. However, it is the p65 subunit of NF- $kappa$ B that induceschanges in the nucleosome nuc-1, perhaps through the recruitmentof a histone acetyltransferase (51), and enhances transcriptionalactivity (46).

Our previous results suggested that LSF allows YY1 to recognize a site on the LTR that YY1 could not bind by itself (49).Therefore, LSF might primarily act as a docking molecule for YY1,which in turn acts by tethering HDAC (Fig. 6). In this model,YY1 may be a limiting factor for repression of the LTR, requiredfor the recruitment of the HDAC to the HIV-1 promoter. The findingthat overexpression of the mutant YY1 $Delta$ 154-199 results in activationof HIV expression is consistent with such a model. El Kharroubiet al. (13) have shown that activation of the integrated proviralHIV genome requires alteration of the local chromatin via acetylationof the nucleosome adjacent to the start site. The recruitmentof HDAC by YY1 might prevent such changes in the local chromatin,maintaining the nucleosome in a deacetylated state, preservinghigher-order nucleosome structure, and thereby inhibiting geneexpression (Fig. 6).

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FIG. 6. Model of recruitment by LSF of YY1 and then HDAC to the HIV promoter.

In vitro assays have shown that assembly of nuc-1 on naked HIV-1 DNA can be inhibited by the presence of LSF (51). Further,one previous report suggested that LSF is important for efficientactivation of the HIV-1 LTR (26), although this has been disputed(76). However, we find no evidence that wild-type LSF activatesLTR expression. While previous evidence that LSF is an activatorof HIV conflicts with our findings, these studies were performedin very different experimental systems. Indeed, through interactionwith other factors, in the absence of YY1, or in other cellularmilieus, LSF might direct LTRactivation.

Regulation of HIV expression within resting CD4 lymphocytes. The HIV-1 enhancer and promoter possess a multiplicity of sequences recognized by cellular and viral regulatory factors. Theroles of cellular enhancers such as Sp1 and NF- $kappa$ B and of the viralactivator Tat in active HIV gene expression have been extensivelystudied. As discussed above, changes in chromatin structure aboutan integrated HIV promoter during activation have been documented.However, mechanisms that downregulate HIV expression are largelyunknown. We have shown that YY1 and LSF are capable of cooperatingto inhibit HIV transcription. Of the many possible mechanismsthrough which YY1 might downregulate transcription, we can nowlink this function to the recruitment of an HDAC; our studiesstrongly suggest that this enzyme is HDAC1. Thus, the YY1-LSFrepressor complex recruits factors capable of potent and durableinhibition of HIV-1 LTR promoterexpression.

A large nucleosome-free, DNase I-hypersensitive region spanning nucleotides 223 to 450 of the HIV-1 has been observed in thechromatin structure of the integrated HIV-1 provirus in chronicallyand acutely infected cells lines. Activation of LTR expressionextends the 3' boundary of this nucleosome-free region a further140 nucleotides. Each nucleosome is entwined by 1.65 turns ofa left-handed superhelix of DNA that corresponds to 147 bp. Thisindicates that the DNA protected by one nucleosome has been exposed,presumably by remodeling of the nucleosome structure. The bindingof both Sp1 and the p50 or p65 subunits of NF- $kappa$ B to the HIV-1LTR alters the local nucleosomal array in vicinity of the HIV-1promoter and perhaps through the recruitment of a histone acetyltransferaseenhances transcriptional activity. El Kharroubi et al. (13)have also shown that activation of the integrated proviral HIVgenome requires alteration of the local chromatin via acetylationof the nucleosome adjacent to the start site. Our findings implythat recruitment of HDAC by YY1 might prevent such changes inthe local chromatin, maintaining the nucleosome in a deacetylatedstate and inhibiting HIVexpression.

We propose a dynamic model of HIV LTR regulation that would allow the establishment of virological latency in rare CD4 T cells.Following T-cell activation necessary for viral entry, reversetranscription, and other steps of the viral life cycle which leadto proviral integration, the rare activated cell avoids apoptosisor viral or immune-mediated destruction. Dampening of LTR expressionby YY1 and LSF may play an important role at this stage. Thiscell then follows pathways that typically reestablish the resting,memory state. The HIV-1 LTR remains silent due to the predominanteffects of repressor molecules, resulting in an inaccessible chromatinstructure about the LTR. This cell may later exit virologicallatency if it encounters stimuli that increase nuclear levelsof NF- $kappa$ B, again changing LTR chromatin structure. Levels of theviral activator Tat then increase within the cell, driving theequilibrium toward viralexpression.

Further study of cellular factors that establish or maintain the rare latent state of HIV infection may yield novel techniquesto manipulate HIV expression, allow better understanding of theHIV replication in T lymphocytes, and lead to specific therapiesdirected at the quiescent reservoir of HIVinfection.

	ACKNOWLEDGMENTS

We thank Laurel Matey and Randall Merling for excellent technical assistance. The following reagents were obtained throughthe AIDS Research and Reference Reagent Program, Division of AIDS,NIAID, NIH: HLCD4-CAT from Barbara K. Felber and George N. Pavlakis,pNL4-3 from Malcolm Martin, and pYU-2 from Beatrice Hahn and GeorgeShaw.

This work was supported by an Ortho-McNeil Young Investigator award from the IDSA and NIH grants AI 41366 and AI 45297 toD.M.M.; Medical Research Council of Canada grant MT-9186 to J.R.D.,an MRC Senior Scientist; NIH grant GM53874 to Y.S.; and a DFCI/SandozDiscovery grant to U.H.

	FOOTNOTES

^* Corresponding author. University of Texas Southwestern Medical Center, 5323 Harry Hines Blvd., Dallas, TX 75390-9113. Phone:(214) 648-3593. Fax: (214) 648-0231. E-mail: david.margolis{at}emailswmed.edu.

Present address: Millennium Pharmaceuticals Inc., Cambridge, MA02139.

Present address: Department of Biology, Boston University, Boston, MA02215.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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