Characteristics of the Adeno-Associated Virus Preintegration Site in Human Chromosome 19: Open Chromatin Conformation and Transcription-Competent Environment

doi:10.1128/JVI.74.16.7671-7677.2000

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Journal of Virology, August 2000, p. 7671-7677, Vol. 74, No. 16
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Characteristics of the Adeno-Associated Virus Preintegration Site in Human Chromosome 19: Open Chromatin Conformation and Transcription-Competent Environment

Stefania Lamartina, Elisabetta Sporeno, Elena Fattori, and Carlo Toniatti^*

Department of Genetics, Istituto di Ricerche di Biologia Molecolare, I.R.B.M.-Piero Angeletti, 00040 Pomezia (Rome), Italy

Received 28 October 1999/Accepted 17 May 2000

	ABSTRACT

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Adeno-associated virus (AAV) establishes latency in infected cells by integrating into the cellular genome, with a high preferencefor a unique region, called AAVS1, of the human chromosome 19.The AAV proteins Rep78 and -68 are postulated to initiate thesite-specific integration process by binding to a Rep bindingsite (RBS) in AAVS1. We provide further evidence to corroboratethis model by demonstrating that the AAVS1 RBS in human cell linesis located near a DNase I hypersensitive "open" chromatin regionand therefore is potentially easily accessible to Rep proteins.This open conformation is maintained in transgenic rats whichcarry an AAVS1 3.5-kb DNA fragment and are proficient for Rep-mediatedsite-specific integration. Interestingly, the core of the DNAseI hypersensitive site in AAVS1 corresponds to a sequence displayingtranscriptional enhancer-like properties, suggesting that AAVS1constitutes a transcription-competent environment. The implicationsof our findings for AAV physiology and gene therapy arediscussed.

	TEXT

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The human adeno-associated virus (AAV) has evolved a complex strategy to propagate in its host cells: it replicates only inthe presence of helper factors, provided either by coinfectingviruses, such as adenovirus (Ad) or herpesvirus, or by genotoxicstimuli (3, 25). In the absence of these stimulatory agents,the virus integrates stably and efficiently into a specific site(called AAVS1) of the human chromosome 19 (26, 27, 45, 46),from which it is rescued following helper virus superinfection(3, 25, 45).

AAV has a linear, single-stranded DNA genome of approximately 4.7 kb which consists of two open reading frames (ORFs), namelyrep and cap, and has inverted terminal repeats (ITRs) at eachend that fold into a hairpin structure and function as originsof replication (3, 25, 49). By using alternate promoters(p5 and p19) and splicing, the rep gene encodes four overlappingproteins: two larger (Rep78 and Rep68) and two smaller (Rep52and Rep40). Rep78 and Rep68 are multifunctional proteins thatdiffer at the C terminus, but have the same DNA binding, helicase,ATPase, and endonuclease activities (3, 20, 21, 49, 59,62). Rep78 and -68 are essential for AAV replication as wellas for its integration into AAVS1 (3, 10, 45). They binda specific sequence (Rep binding site [RBS]) in the ITRs and cleavein a strand- and site-specific manner a nearby sequence calleda terminal resolution site (TRS) (6, 10, 44, 48, 58);both binding and cleavage are crucial for AAV replication (3,25, 49). An RBS flanked by a TRS is also present in AAVS1(54, 57), and in vitro experiments have demonstrated thatRep78 and -68 can mediate the formation in vitro of a complexbetween this sequence of human chromosome 19 and the AAV ITRs(57). In addition, genetic analysis performed with an Epstein-Barrvirus-based episomal vector containing various fragments of AAVS1has demonstrated that the RBS and the TRS in AAVS1 are the twocis-acting signals required for AAV site-specific integration(17, 31, 32). This evidence has led to the hypothesis thatthe simultaneous binding of Rep78 and -68 to the RBSs presentin the ITRs and in AAVS1 is the first step in the integrationmechanism (25, 31, 32). The subsequent nicking of the flankingDNA cleavage sites would then initiate the actual integrationprocess, which occurs at variable distances from the 3' end ofthe RBS and probably proceeds through a replicative type of recombination(25, 31, 32).

We speculated that a corollary to this model of the AAV integration at chromosome 19 is that the RBS in AAVS1 should be presentin a chromatin region maintained in an open conformation in orderto be easily accessible to Rep78 and -68 proteins. We thus decidedto test this hypothesis by assessing whether the RBS in AAVS1maps near or at a DNAse I hypersensitive site (DHSs). DHSs constitutea minor (ca. 1%) fraction of the bulk genome and represent regionseither which are nucleosome free or which do not carry canonicalnucleosomes and to which trans-acting factors bind (5, 12,18, 19, 38, 53). DHSs have been functionally associatedmainly with processes such as transcription, but have also beenassociated with replication, recombination, and chromosome segregation(18, 43, 61). They can thus be considered as exposed chromatinregions that allow access of trans-acting factors to importantcis-acting DNA sequences (9, 12, 18, 61).

Figure 1A is a schematic representation of the region of human chromosome 19 containing the AAV integration site originallydescribed by Kotin and colleagues (27). All Rep-mediated integrationsdocumented so far (27, 28, 38-41, 50, 60) have been mappedwithin the 1.6-kb EcoRI-BamHI fragment containing the RBS (Fig.1A), and we thus explored this region and its flanking sequencesfor the presence of DHSs. 293 and HeLa cells, in which Rep-mediatedsite-specific integration has been repeatedly reported, were selectedas target cells (2, 28, 36, 39, 41, 47). DNAse Isensitivity assays were performed essentially as described previously(52, 61) with minor modifications. Briefly, 293 and HeLa cellswere collected, resuspended in phosphate-buffered saline, andcentrifuged for 10 min at 4°C. They were then resuspended at adensity of 5 × 10⁶ cells per ml of TNM buffer (10 mM Tris-Cl [pH 7.5], 10 mM NaCl,3 mM MgCl₂) and incubated for 10 min in ice. Swollen cells werebroken in a tight-fitting Dounce homogenizer, and intact purifiednuclei were recovered by centrifuging the broken cells for 10min at 1,300 × g through a 0.25 M sucrose-TNM buffer cushion.Nuclei were then resuspended at a density of 2 × 10⁷ per ml of digestion buffer (15 mM Tris-Cl [pH 7.5], 15 mM NaCl,3 mM MgCl₂, 60 mM KCl, 0.25 mM sucrose, 0.5 mM dithiothreitol,1 mM, phenylmethylsulfonyl fluoride). Increasing concentrationsof DNAse I were then added to aliquots (100 µl each) of the nuclearsuspensions. After 10 min of incubation at 37°C, the reactionswere stopped by adding 400 µl of stop solution (15 mM EDTA [pH8.0], 0.6% sodium dodecyl sulfate). Forty micrograms of proteinaseK was added to each suspension, and samples were incubated for12 h at 37°C. Genomic DNA was purified by phenol extraction andethanol precipitation. After treatment with RNase, DNA sampleswere digested to completion with the appropriate enzymes, electrophoresedon a 0.8% agarose gel, and blotted onto nylon membranes. First,we checked whether DHSs mapped in the 2.6-kb BamHI fragment containingthe RBS (Fig. 1A). In the first experiment, BamHI-digested DNAwas hybridized with probe P1 (EcoRI-PstI fragment): as shown inFig. 1B, a DHS (called DHS-S1) was detectable in both cell linesas a smear centered at 1,400 bp and approximately spanning the1,250- to 1,550-bp region. This approximately mapped the DHS nearto the RBS, but since P1 was not located at either end of the2.6-kb BamHI fragment, we could not discriminate whether DHS-S1was mainly located 5' or 3' of the RBS. To further address thispoint, we performed a canonical indirect end-labelling experimentby hybridizing BamHI-digested DNA with a different probe (probeP2; DraIII-DraIII fragment) that adjoins exactly the 3' end ofthe region analyzed (Fig. 1C). As shown in Fig. 1C, also in thiscase, a smear approximately spanning the 1,250- to 1,550-bp regionwas detected, while no signal was evident at a molecular weighthigher than 1,600 bp. This pattern mapped the "core" of the DHSdownstream of the EcoRI site and mainly, if not exclusively, 5'to the RBS. Taken together, the results shown in Fig. 1B and Clocalize, within the sensitivity limits of the end-labelling technique,the core of DHS-S1 in an ~300-bp-long region (spanning approximatelynucleotides [nt] 50 to 350 of the AAVS1 sequence represented inFig. 1A) located 5' and in near proximity to the RBS (Fig. 1Band C). Notably, control DNase I digestions of the cloned andpurified AAVS1 fragment failed to detect any DHS (data not shown),thus ruling out that the DHS-S1 sequence is hypersensitive toDNase I for reasons unrelated to chromatin structure.

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FIG. 1. A DHS maps near the RBS in AAVS1. (A) Schematic representation of the region of AAVS1 analyzed. The restriction map is limited to those sites that were relevant for our studies BamHI (B), BglI (Bl), EcoRI (E), PstI (P), and DraIII (D). The bold line represents part of the published AAVS1 sequence (27), with the nucleotide numbering starting at the indicated EcoRI site (position +1) and ending at the BglI site at position +3505. The 5' and 3' sequences flanking the 1- to -3505 region are represented by dotted lines. The BamHI sites present in these flanking regions are also indicated. (B and C) Nuclei isolated from 293 or HeLa cells were digested with increasing concentrations (1, 2, 10, 20, and 40 U/ml) of DNAse I (Boehringer Mannheim, catalog no. 776785). DNA was then isolated, digested with the indicated restriction enzymes, and incubated with probe P1 (B) or P2 (C). The two probes were derived from plasmid pRVK (gift of K. Berns, Cornell Medical School, Ithaca, N.Y.), spanning nt 1 to 3525 of AAVS1 (27). P1 was obtained as an EcoRI-PstI fragment and spans nt 1 to 1427; P2 was a DraIII fragment spanning nt 953 to 1583. The diagram below each autoradiogram shows the restriction fragment being analyzed, the identity and position of each hybridization probe, the position of the RBS, and the location of DHS-S1 as identified with each specific probe. The positions of the molecular weight standards (in kilobases) are shown to the left of each gel. $-$ , lanes loaded with genomic DNA from untreated nuclei.

We next analyzed the AAVS1 segment from the BglI site at position 353 to the extreme 3' BamHI site (Fig. 1A). In the firstassay, DNAse I-treated genomic DNA of 293 cells was digested withBamHI restriction enzyme and hybridized with probe P3 (BamHI-BglIfragment; Fig. 2A), which detected the 3'-terminal 3.7 kb of theAAVS1 region (Fig. 1A). As shown in Fig. 2A, no DHS was detected.Secondly, DNase I-treated genomic DNA of 293 cells was digestedwith BglI restriction enzyme, which released a 3.2-kb fragment(Fig. 2B) that contains the RBS at a 20-bp distance from its 5'extremity and overlaps with the 2.6-kb BamHI fragment analyzedin the experiments shown in Fig. 1B and C. When this DNA was hybridizedwith probe P4 (BglI-PstI fragment; Fig. 2B), no hypersensitivesites were detectable: this confirmed that, within the sensitivitylimits of the assay, DHS-S1 is indeed centered in a region located5' to the RBS. In conclusion, in the 7.1-kb BamHI-BamHI regionanalyzed (Fig. 1A), only one DHS site (DHS-S1) was identified,and this mapped in close proximity to the RBS (Fig. 1B and C).

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FIG. 2. No DHSs are present in AAVS1 downstream of the RBS. Nuclei isolated from 293 cells were digested with DNAse I, purified, digested with the indicated restriction enzymes, and incubated with probe P3 (A) or P4 (B). P3 was a BamHI-BglI fragment spanning nt 2367 to 3505; P4 was a BglI-PstI fragment extending from nt 353 to 1427. The restriction fragment being analyzed and the identity and position of each hybridization probe are shown. The positions of the molecular weight standards (in kilobases) are shown to the left of each gel. $-$ , lanes loaded with genomic DNA from untreated nuclei.

The chromatin configuration associated with functionally important DHSs is often dominant over the surrounding regions andis maintained in different chromosomal environments (11, 13,15, 18, 35, 36, 51). The possibility to test whetherthis rule also applies to DHS-S1 was offered by recently generatedtransgenic rats which carry the 3.5-kb region of human AAVS1 andrepresent a valid model for studying AAV site-specific integration(42). Intact nuclei from transgenic primary rat fibroblasts,in which Rep-mediated integration at AAVS1 has been documented(42), were isolated and treated with increasing concentrationsof DNase I. Southern blot analysis of BamHI-digested genomic DNAdemonstrated that DHS-S1 at human AAVS1 was maintained even inthe context of the rat genome (Fig. 3). This result strongly suggeststhat the DHS-S1 sequence imposes a position-independent chromatinconfiguration.

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FIG. 3. DHS-S1 mapping in the genome of transgenic rats carrying the AAVS1 3.5-kb DNA fragment. Primary fibroblasts from ear biopsies of transgenic rats (line 15) were isolated as described previously (42). Isolated nuclei were incubated with increasing concentrations of DNAse I as described in the legend to Fig. 1. Genomic DNA was then purified, digested with restriction enzyme BamHI, transferred to nylon membranes, and hybridized with probe P2 (see also Fig. 1C). The fine structure of the human AAVS1 region integrated in the genome of transgenic rat line 15 has been previously described (42). At the bottom of the figure is a schematic representation of the BamHI restriction fragment recognized by the probe P2: the bold line represents part of the human AAVS1 sequence with the nucleotide numbering starting at the indicated EcoRI site (position +1) and ending at the BamHI site at position +1605 (27). The positions of the molecular weight standards (in kilobases) are indicated. $-$ , genomic DNA from untreated nuclei.

DHSs mainly reside at cis-acting DNA elements that function in gene regulation, such as promoters and enhancers (12, 18,29, 53): we thus tested whether the identified DHS in AAVS1had transcription regulatory properties. The core region of DHS-S1was cloned in two opposite orientations upstream of a promoterlessreporter chloramphenicol acetyltransferase (CAT) gene (Fig. 4A)and transfected in HeLa and 293 cells. A plasmid containing theCAT gene downstream of the simian virus 40 (SV40) promoter (pCAT3-promoter vector; Promega) was used in control experiments. Asshown in Fig. 4A, DHS-S1 stimulated transcription of the CAT genein both cell lines. Activation was stronger in 293 cells (~300-to -400-fold activation) than in HeLa cells (~10- to 13-fold induction)and was mainly not orientation dependent. To verify that the transcriptionalactivity of DHS-S1 was not due to any artifact in the constructs,we tested the transcriptional properties of three randomly selectedfragments of AAVS1 adjacent but not contiguous to DHS-S1. Thesethree fragments, FR1, FR2, and FR3, spanning nt 1313 to 1616,2077 to 2371, and 2633 to 2927, respectively, were cloned upstreamof the promoterless CAT gene and analyzed in transient assays.As indicated in Fig. 4A, none of these three fragments stimulatedtranscription in 293 and HeLa cells, thus validating the resultsobtained with DHS-S1.

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FIG. 4. Transcriptional activity of DHS-S1. (A) Structure and activity of constructs containing DHS-S1 cloned upstream of the CAT gene. The whole DHS-S1 was excised as an SmaI-SmaI fragment (nt 18 to 353 of AAVS1) from plasmid pRVK and cloned in both orientations (indicated by the direction of the arrows) upstream of the intron and the CAT gene into the SmaI site of pCAT 3-basic vector (Promega). Black boxes represent the SV40 promoter. The promoterless plasmid is the pCAT 3-basic vector (Promega), and the control plasmid containing the SV40 promoter is the pCAT 3-promoter vector (Promega). Regions FR1 (nt 1313 to 1616 of AAVS1) and FR3 (nt 2633 to 2927 of AAVS1) were amplified by PCR with plasmid pRVK as a substrate and oligonucleotides carrying SmaI sites at either end. The resulting fragments were digested with restriction enzyme SmaI and cloned into the SmaI site of the pCAT 3-basic vector. Region FR2 (nt 2077 to 2371 of AAVS1) was excised from plasmid pRVK as a BamHI-flanked fragment, filled in by treatment with Klenow enzyme, and inserted into the SmaI site of pCAT 3-basic vector. Ten micrograms of each plasmid was transfected as described previously by calcium phosphate precipitation into 293 and HeLa cells (1). At 15 h posttransfection, the medium was changed: after an additional 24 h, cells were collected and CAT activity in cell extracts was measured by using the Quan-T-CAT assay system (Amersham, Pharmacia). CAT activities were normalized against the luciferase activity derived from a cotransfected cytomegalovirus-luciferase plasmid (1). Results are expressed as milliunits of CAT enzyme present in 10 µg of cell extracts and as fold induction with respect to the promoterless pCAT 3-basic vector. The data are means ± standard deviations of two independent experiments in which two separate plasmid preparations were used. (B) Enhancer activity of DHS-S1 in 293 and HeLa cells. DHS-S1 was cloned in both orientations (represented by the direction of the arrows) into the pCAT 3-promoter vector either into the SmaI site upstream of the SV40 promoter or into the BamHI site downstream of the CAT gene. Similarly, FR1, FR2, and FR3 were cloned in one orientation either into the SmaI site or into the BamHI site of pCAT 3-vector. Transfections were performed, and CAT activities were measured and normalized as described in the legend to Fig. 4A. Results are expressed as milliunits of CAT enzyme in 10 µg of cell extracts; fold induction was calculated with respect to that of the pCAT 3-promoter vector. The data are means ± standard deviations of three independent experiments in which at least two different plasmid preparations were used.

The finding that DHS-S1 acted essentially in an orientation-independent manner suggested that this region could be a transcriptionalenhancer. To check this point, DHS-S1 was cloned into pCAT 3-promotervector either 5' to the SV40 promoter or 3' to the polyadenylationsite of the CAT gene. Control plasmids were generated by usingFR1, FR2, and FR3 fragments. The various constructs are representedin Fig. 4B, which also shows their behavior in transfected 293and HeLa cells. In both cells, DHS-S1 markedly enhanced the SV40promoter activity when cloned either upstream of the SV40 promoteror downstream of the CAT gene, although the stimulation was greaterfrom an upstream position (20- to 50-fold induction) than froma downstream position (10- to 25-fold induction) (Fig. 4B). Theenhancer effect was not orientation dependent (Fig. 4B) and notartifactual, in that control fragments FR1, FR2, and FR3 did notbehave as transcriptional enhancers (Fig. 4B). In conclusion,DHS-S1 exhibited the properties of a true enhancer in that itwas effective in both orientations and activated the SV40 promotereither from a proximal site (upstream of the promoter) or froma remote site (downstream of the CAT gene) (4).

To further characterize DHS-S1, we also analyzed the enhancer properties of two deletion mutants: E1-S1, spanning nt 18 to181 of the published AAVS1 sequence (27), and E2-S1, which runsfrom nt 181 to 353 (Fig. 5A). Each fragment was cloned in bothpossible orientations in the plasmid pCAT 3-promoter $---$ either 5'or 3' to the CAT gene $---$ and the various constructs were transfectedinto 293 and HeLa cells (Fig. 5B). As shown in Fig. 5B, E2-S1displayed almost the same enhancer activity as the full-lengthDHS-S1 (compare Fig. 4B and Fig. 5B): however, E1-S1 also wasstill active, thus suggesting that cis-acting signals are at leastpartially redundant in DHS-S1. Taken together, these results correlatewell with the presence of potential binding sites for severaltranscription factors (such as AP-1, AP-2, Sp1, and CREB) scatteredalong the entire hypersensitive site, but mainly concentrated(in particular the Sp1 sites) (27) in the 3' half of DHS-S1,as revealed by DHS-S1 sequence analysis using the MAP programand the Transcription Factor Database (Wisconsin Package, version10.0; Genetics Computer Group, Madison, Wisc.) (16).

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FIG. 5. Enhancer activity of DHS-S1 is mainly located in the 181 to 353 region. (A) Graphic representation of the two DHS-S1 subregions, E1-S1 (nt 18 to 181) and E2-S1 (nt 181 to 353), whose transcriptional activity was tested in transient transfection assays. (B) Enhancer activity of E1-S1 and E2-S1 in 293 and HeLa cells. E1-S1 and E2-S1 were obtained as PCR fragments by using plasmid pRVK (see legend to Fig. 1) as a template, and cloned in both orientations (indicated by the direction of the arrows) into plasmid pCAT 3-promoter either upstream of the SV40 promoter or downstream of the CAT gene (see the legend to Fig. 4). Transfections, CAT assays, and normalization of the results were performed as described in the legend to Fig. 4. Results are expressed as milliunits of CAT per 10 µg of cell extracts and as fold induction with respect to the pCAT 3-promoter vector. The data are means ± standard deviations of four independent experiments in which two different plasmid preparations were used.

In this report, we have demonstrated that AAV site-specific integration into chromosome 19 takes place near a DHS and in anapparently transcriptionally active region. It is known that DHSsassociated with enhancer functions confer chromatin accessibilityto proximal DNA regions (12, 22, 23). Therefore, the findingthat DHS-S1 maps in near proximity to the RBS (at less than 1nucleosomal DNA unit length from the mapped 3' end of the DHS)strongly suggests that the RBS is indeed maintained in an openchromatin conformation and hence is easily accessible to Rep proteinsin vivo (9, 12, 53, 61). This further corroborates thewidely accepted model for Rep-mediated site-specific integration:the specificity of AAV integration might thus be dictated by theDNA sequence at AAVS1 and facilitated by the chromatin configurationin that region (17, 31, 32, 57). This hypothesis is furthersupported by results obtained by Kotin and colleagues using episomalintegration substrates: in that case, the addition of an AAVS1segment corresponding to DHS-S1 led to an integration frequencythreefold higher than that observed with a substrate containingonly the RBS and the TRS (31, 32). Interestingly, one region(from nt 209 to 326 of AAVS1) overlapping with DHS-S1, and inparticular with the E2-S1 segment, has been associated with episomalDNA rearrangements by Linden et al. (31, 32). This regioncarries the motif M26, which has been characterized as an enhancerof meiotic recombination in fission yeast (14, 24, 55).A role for this sequence in AAV integration has only been hypothesized,but our finding that it co-maps with a nuclease hypersensitivesite, much as has been observed in Schizosaccharomyces pombe,is of interest and supports this conjecture (33, 34).

Kotin et al. reported the presence of an open ORF which maps in the AAVS1 sequence from nt 1620 to nt 2318, potentially codesfor a 95-amino-acid-long polypeptide (no match with known proteinsequences), and is expressed in human foreskin fibroblasts atlow levels detectable only by reverse transcription-PCR (27).So far, this is the only report describing a transcriptional activityin AAVS1. At this stage, we do not know whether the DHS-1 is involvedin the transcriptional regulation of this potential ORF or ofany other gene (4, 7, 12). However, the presence of DHS-S1,as well as its enhancer-like properties, suggests, although itdoes not prove, that AAVS1 constitutes a transcriptionally competentenvironment (12, 29, 53, 56). AAV perpetuates its geneticinformation by establishing latency in cells: genotoxic agentsor helper virus infections activate transcription of integratedAAV genes, and this leads to recovery and replication of the AAVgenome (3). It is thus tempting to hypothesize that AAVS1 hasevolved as a preferential site for AAV integration, also becauseit locates in a region of the human genome which is proficientfor transcription and allows stably integrated exogenous genesto be reactivated. On the other side, the presence of DHS-S1 mustbe reconciled with the latency of AAV, whose genome is currentlybelieved to be transcriptionally silent when integrated at AAVS1(3). More work will thus be required to clarify whether andhow DHS-S1 affects transcription from the integrated AAV genomeduring the different phases of its lifecycle.

Our results are also of interest for gene therapy. It has been recently demonstrated that either Rep78 or Rep68 provided intrans promotes preferential integration at AAVS1 of a transgeneflanked by the AAV ITRs (2, 39, 47, 50). Several typesof viral and nonviral delivery vectors which incorporate Rep78and -68 and ITR-flanked transgenes are being designed and tested(28, 37, 40, 41). In this connection, the identificationof a DHS in AAVS1 represents a further step toward the functionalcharacterization of AAVS1. In particular, the presence of DHS-S1indicates that AAVS1 should indeed constitute a proper environmentfor transgene expression: interestingly, since DHS-S1 maps 5'to the hot-spot integration sites in AAVS1, transgene integrationshould not lead to disruption of the DHS-S1 sequence (27, 28,38-41, 50, 60). This point will clearly need to be addressedin consideration of DHS-S1 possibly playing an important rolein cell physiology, especially because rearrangements at AAVS1have been frequently associated with Rep-mediated integration(2, 37, 39, 41, 50).

	ACKNOWLEDGMENTS

We thank Gennaro Ciliberto for critically reading the manuscript. We also gratefully acknowledge Janet Clench for editingthe manuscript and Manuela Emili for work with thegraphics.

	FOOTNOTES

^* Corresponding author. Mailing address: Istituto di Ricerche di Biologia Molecolare, I.R.B.M.-P. Angeletti, Via Pontina Km30.600, 00040 Pomezia (Rome), Italy. Phone: 39-06-91093668. Fax:39-06-91093654. E-mail: toniatti{at}irbm.it.

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21. Im, D.-S., and N. Muzyczka. 1992. Partial purification of adeno-associated virus Rep78, Rep52, and Rep40 and their biochemical characterization. J. Virol. 66:1119-1128[Abstract/Free Full Text].

22. Jenuwein, T., W. C. Forrester, R.-G. Qiu, and R. Grosschedl. 1993. The immunoglobulin µ enhancer core establishes local factor access in nuclear protein independent of transcriptional stimulation. Genes Dev. 7:2016-2032[Abstract/Free Full Text].

23. Jenuwein, T., W. C. Forrester, L. A. Fernández-Herrero, G. Laible, M. Dull, and R. Grosschedl. 1997. Extension of chromatin accessibility by nuclear matrix attachment regions. Nature 385:269-272[CrossRef][Medline].

24. Kon, N., M. D. Krawchuk, B. G. Warren, G. R. Smith, and W. P. Wahls. 1997. Transcription factor Mts1/Mts2 (Atf1/Pcr1, Gad7/Pcr1) activates the M26 meiotic recombination hotspot in Schizosaccharomyces pombe. Proc. Natl. Acad. Sci. USA 94:13765-13770[Abstract/Free Full Text].

25. Kotin, R. M. 1994. Prospects for the use of adeno-associated virus as a vector for human gene therapy. Hum. Gene Ther. 5:793-891[Medline].

26. Kotin, R. M., M. Siniscalco, R. J. Samulski, X. D. Zhu, L. Hunter, C. A. Laughlin, S. M. Laughlin, N. Muzyczka, M. Rocchi, and K. I. Berns. 1990. Site-specific integration by adeno-associated virus. Proc. Natl. Acad. Sci. USA 87:2211-2215[Abstract/Free Full Text].

27. Kotin, R. M., R. M. Linden, and K. I. Berns. 1992. Characterization of a preferred site on human chromosome 19q for integration of adeno-associated virus DNA by non-homologous recombination. EMBO J. 11:5071-5078[Medline].

28. Lamartina, S., G. Roscilli, D. Rinaudo, P. Delmastro, and C. Toniatti. 1998. Lipofection of purified adeno-associated virus Rep68 protein: toward a chromosome-targeting nonviral particle. J. Virol. 72:7653-7658[Abstract/Free Full Text].

29. Li, Q., S. Harju, and K. R. Peterson. 1999. Locus control regions: coming of age at a decade plus. Trends Genet. 15:403-408[CrossRef][Medline].

30. Linden, R. M., and K. I. Berns. 1997. Site-specific integration by adeno-associated virus: a basis for a potential gene-therapy vector. Gene Ther. 4:4-5[CrossRef][Medline].

31. Linden, R. M., E. Winocour, and K. I. Berns. 1996. The recombination signals for adeno-associated virus site-specific integration. Proc. Natl. Acad. Sci. USA 93:7966-7972[Abstract/Free Full Text].

32. Linden, R. M., P. Ward, C. Giraud, E. Winocour, and K. I. Berns. 1996. Site-specific integration by adeno-associated virus. Proc. Natl. Acad. Sci. USA 93:11288-11294[Abstract/Free Full Text].

33. Mizuno, K. I., Y. Emura, M. Baur, J. Kohli, K. Ohta, and T. Shibata. 1997. The meiotic recombination hot spot created by the single-base substitution ade6-M26 results in remodeling of chromatin structure in fission yeast. Genes Dev. 11:876-886[Abstract/Free Full Text].

34. Nicolas, A. 1998. Relationship between transcription and initiation of meiotic recombination: toward chromatin accessibility. Proc. Natl. Acad. Sci. USA 95:87-89[Free Full Text].

35. Ortiz, B. D., D. Cado, V. Chen, P. W. Diaz, and A. Winoto. 1997. Adjacent DNA elements dominantly restrict the ubiquitous activity of a novel chromatin-opening region to specific tissues. EMBO J. 16:5037-5045[CrossRef][Medline].

36. Ortiz, B. D., D. Cado, and A. Winoto. 1999. A new element within the T-cell receptor $alpha$ locus required for tissue-specific locus control region activity. Mol. Cell. Biol. 19:1901-1909[Abstract/Free Full Text].

37. Palombo, F., A. Monciotti, A. Recchia, R. Cortese, G. Ciliberto, and N. La Monica. 1998. Site-specific integration in mammalian cells mediated by a new hybrid baculovirus-adeno-associated virus vector. J. Virol. 72:5025-5034[Abstract/Free Full Text].

38. Pazin, M. J., and J. T. Kadonaga. 1997. What's up and down with histone deacetylation and transcription. Cell 89:325-328[CrossRef][Medline].

39. Pieroni, L., C. Fipaldini, A. Monciotti, D. Cimini, A. Sgura, E. Fattori, O. Epifano, R. Cortese, F. Falombo, and N. La Monica. 1998. Targeted integration of adeno-associated virus-derived plasmid in transfected human cells. Virology 249:249-259[CrossRef][Medline].

40. Recchia, A., R. J. Parks, S. Lamartina, C. Toniatti, L. Pieroni, F. Palombo, G. Ciliberto, F. L. Graham, R. Cortese, N. La Monica, and S. Colloca. 1999. Site-specific integration mediated by a hybrid adenovirus/adenoassociated virus vector. Proc. Natl. Acad. Sci. USA 96:2615-2620[Abstract/Free Full Text].

41. Rinaudo, D., S. Lamartina, G. Roscilli, G. Ciliberto, and C. Toniatti. 1999. Conditional site-specific integration into human chromosome 19 using a ligand-dependent chimeric AAV/rep protein. J. Virol. 74:281-294[Abstract/Free Full Text].

42. Rizzuto, G., B. Gorgoni, M. Cappelletti, D. Lazzaro, I. Gloaguen, V. Poli, A. Sgura, D. Cimini, G. Ciliberto, R. Cortese, E. Fattori, and N. La Monica. 1999. Development of animal models for adeno-associated virus site-specific integration. J. Virol. 73:2517-2526[Abstract/Free Full Text].

43. Roeder, G. S. 1997. Meiotic chromosomes: it takes two to tango. Genes Dev. 11:2600-2621[Free Full Text].

44. Ryan, J. H., S. Zolotukhin, and N. Muzyczka. 1996. Sequence requirements for binding of Rep68 to the adeno-associated virus terminal repeats. J. Virol. 70:1542-1553[Abstract].

45. Samulski, R. J. 1993. Adeno-associated virus: integration at a specific chromosomal locus. Curr. Opin. Genet. Dev. 3:74-80[CrossRef][Medline].

46. Samulski, R. J., X. Zhu, X. Xiao, J. D. Brook, D. E. Housman, N. Epstein, and L. A. Hunter. 1991. Targeted integration of adeno-associated virus (AAV) into human chromosome 19. EMBO J. 10:3941-3950[Medline]. (Erratum, 11:1228, 1992.)

47. Shelling, A. N., and M. G. Smith. 1994. Targeted integration of transfected and infected adeno-associated virus vectors containing the neomycin resistance gene. Gene Ther. 1:165-169[Medline].

48. Snyder, R. O., D.-S. Im, T. Ni, X. Xiao, R. J. Samulski, and N. Muzyczka. 1993. Features of the adeno-associated virus origin involved in substrate recognition by the viral Rep protein. J. Virol. 67:6096-6104[Abstract/Free Full Text].

49. Srivastava, A., E. W. Lusby, and K. I. Berns. 1983. Nucleotide sequence and organization of the adeno-associated virus 2 genome. J. Virol. 45:555-564[Abstract/Free Full Text].

50. Surosky, R. T., M. Urabe, S. G. Godwin, S. A. McQuiston, G. J. Kurtzman, K. Ozawa, and G. Natsoulis. 1997. Adeno-associated virus Rep proteins target DNA sequences to a unique locus in the human genome. J. Virol. 71:7951-7959[Abstract].

51. Tanimoto, K., Q. Liu, J. Bungert, and J. D. Engel. 1999. The polyoma virus enhancer cannot substitute for DNAseI core hypersensitive sites 2-4 in the human beta-globin region. Nucleic Acids Res. 27:3130-3137[Abstract/Free Full Text].

52. Tuan, D., and I. M. London. 1984. Mapping of DNAse I-hypersensitive sites in the upstream DNA of human embryonic $varepsilon$ -globin gene in K562 leukemia cells. Proc. Natl. Acad. Sci. USA 81:2718-2722[Abstract/Free Full Text].

53. Udavrdy, A. 1999. Dividing the empire: boundary chomatin elements delimit the territory of enhancers. EMBO J. 18:1-8[CrossRef][Medline].

54. Urcelay, E., P. Ward, S. M. Wiener, B. Safer, and R. M. Kotin. 1995. Asymmetric replication in vitro from a human sequence element is dependent on adeno-associated virus Rep protein. J. Virol. 69:2038-2046[Abstract].

55. Wahls, W. P., and G. R. Smith. 1994. A heterodimeric protein that binds to a meiotic homologous recombination hot spot: correlation of binding and hot spot activity. Genes Dev. 8:1693-1702[Abstract/Free Full Text].

56. Walters, M. C., S. Fierung, J. Eidemiller, W. Magis, M. Groudine, and D. I. K. Martin. 1995. Enhancers increase the probability but not the level of gene expression. Proc. Natl. Acad. Sci. USA 92:7125-7129[Abstract/Free Full Text].

57. Weitzman, M. D., S. R. Kyöstiö, R. M. Kotin, and R. A. Owens. 1994. Adeno-associated virus (AAV) Rep proteins mediate complex formation between AAV DNA and its integration site in human DNA. Proc. Natl. Acad. Sci. USA 91:5808-5812[Abstract/Free Full Text].

58. Weitzman, M. D., S. R. M. Kyöstiö, B. J. Carter, and R. A. Owens. 1996. Interaction of wild-type and mutant adeno-associated virus (AAV) Rep proteins on AAV hairpin DNA. J. Virol. 70:2440-2448[Abstract].

59. Wonderling, R. S., S. R. M. Kyöstiö, and R. A. Owens. 1996. A maltose-binding protein/adeno-associated virus Rep68 fusion protein has DNA-RNA helicase and ATPase activities. J. Virol. 69:3542-3548[Abstract].

60. Yang, C. C., X. Xiao, X. Zhu, D. C. Ansardi, N. D. Epstein, M. R. Frey, A. G. Matera, and R. J. Samulski. 1997. Cellular recombination pathways and viral terminal repeat hairpin structures are sufficient for adeno-associated virus integration in vivo and in vitro. J. Virol. 71:9231-9247[Abstract].

61. Zaret, K. 1999. In vivo analysis of chromatin structure. Methods Enzymol. 304:612-626[Medline].

62. Zhou, X., I. Zolotukhin, D.-S. Im, and N. Muzyczka. 1999. Biochemical characterization of adeno-associated virus Rep68 DNA helicase and ATPase activity. J. Virol. 73:1580-1590[Abstract/Free Full Text].

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20.	Im, D.-S., and N. Muzyczka. 1990. The AAV origin-binding protein Rep68 is an ATP dependent site-specific endonuclease with DNA helicase activity. Cell 61:447-457[CrossRef][Medline].
21.	Im, D.-S., and N. Muzyczka. 1992. Partial purification of adeno-associated virus Rep78, Rep52, and Rep40 and their biochemical characterization. J. Virol. 66:1119-1128[Abstract/Free Full Text].
22.	Jenuwein, T., W. C. Forrester, R.-G. Qiu, and R. Grosschedl. 1993. The immunoglobulin µ enhancer core establishes local factor access in nuclear protein independent of transcriptional stimulation. Genes Dev. 7:2016-2032[Abstract/Free Full Text].
23.	Jenuwein, T., W. C. Forrester, L. A. Fernández-Herrero, G. Laible, M. Dull, and R. Grosschedl. 1997. Extension of chromatin accessibility by nuclear matrix attachment regions. Nature 385:269-272[CrossRef][Medline].
24.	Kon, N., M. D. Krawchuk, B. G. Warren, G. R. Smith, and W. P. Wahls. 1997. Transcription factor Mts1/Mts2 (Atf1/Pcr1, Gad7/Pcr1) activates the M26 meiotic recombination hotspot in Schizosaccharomyces pombe. Proc. Natl. Acad. Sci. USA 94:13765-13770[Abstract/Free Full Text].
25.	Kotin, R. M. 1994. Prospects for the use of adeno-associated virus as a vector for human gene therapy. Hum. Gene Ther. 5:793-891[Medline].
26.	Kotin, R. M., M. Siniscalco, R. J. Samulski, X. D. Zhu, L. Hunter, C. A. Laughlin, S. M. Laughlin, N. Muzyczka, M. Rocchi, and K. I. Berns. 1990. Site-specific integration by adeno-associated virus. Proc. Natl. Acad. Sci. USA 87:2211-2215[Abstract/Free Full Text].
27.	Kotin, R. M., R. M. Linden, and K. I. Berns. 1992. Characterization of a preferred site on human chromosome 19q for integration of adeno-associated virus DNA by non-homologous recombination. EMBO J. 11:5071-5078[Medline].
28.	Lamartina, S., G. Roscilli, D. Rinaudo, P. Delmastro, and C. Toniatti. 1998. Lipofection of purified adeno-associated virus Rep68 protein: toward a chromosome-targeting nonviral particle. J. Virol. 72:7653-7658[Abstract/Free Full Text].
29.	Li, Q., S. Harju, and K. R. Peterson. 1999. Locus control regions: coming of age at a decade plus. Trends Genet. 15:403-408[CrossRef][Medline].
30.	Linden, R. M., and K. I. Berns. 1997. Site-specific integration by adeno-associated virus: a basis for a potential gene-therapy vector. Gene Ther. 4:4-5[CrossRef][Medline].
31.	Linden, R. M., E. Winocour, and K. I. Berns. 1996. The recombination signals for adeno-associated virus site-specific integration. Proc. Natl. Acad. Sci. USA 93:7966-7972[Abstract/Free Full Text].
32.	Linden, R. M., P. Ward, C. Giraud, E. Winocour, and K. I. Berns. 1996. Site-specific integration by adeno-associated virus. Proc. Natl. Acad. Sci. USA 93:11288-11294[Abstract/Free Full Text].
33.	Mizuno, K. I., Y. Emura, M. Baur, J. Kohli, K. Ohta, and T. Shibata. 1997. The meiotic recombination hot spot created by the single-base substitution ade6-M26 results in remodeling of chromatin structure in fission yeast. Genes Dev. 11:876-886[Abstract/Free Full Text].
34.	Nicolas, A. 1998. Relationship between transcription and initiation of meiotic recombination: toward chromatin accessibility. Proc. Natl. Acad. Sci. USA 95:87-89[Free Full Text].
35.	Ortiz, B. D., D. Cado, V. Chen, P. W. Diaz, and A. Winoto. 1997. Adjacent DNA elements dominantly restrict the ubiquitous activity of a novel chromatin-opening region to specific tissues. EMBO J. 16:5037-5045[CrossRef][Medline].
36.	Ortiz, B. D., D. Cado, and A. Winoto. 1999. A new element within the T-cell receptor $alpha$ locus required for tissue-specific locus control region activity. Mol. Cell. Biol. 19:1901-1909[Abstract/Free Full Text].
37.	Palombo, F., A. Monciotti, A. Recchia, R. Cortese, G. Ciliberto, and N. La Monica. 1998. Site-specific integration in mammalian cells mediated by a new hybrid baculovirus-adeno-associated virus vector. J. Virol. 72:5025-5034[Abstract/Free Full Text].
38.	Pazin, M. J., and J. T. Kadonaga. 1997. What's up and down with histone deacetylation and transcription. Cell 89:325-328[CrossRef][Medline].
39.	Pieroni, L., C. Fipaldini, A. Monciotti, D. Cimini, A. Sgura, E. Fattori, O. Epifano, R. Cortese, F. Falombo, and N. La Monica. 1998. Targeted integration of adeno-associated virus-derived plasmid in transfected human cells. Virology 249:249-259[CrossRef][Medline].
40.	Recchia, A., R. J. Parks, S. Lamartina, C. Toniatti, L. Pieroni, F. Palombo, G. Ciliberto, F. L. Graham, R. Cortese, N. La Monica, and S. Colloca. 1999. Site-specific integration mediated by a hybrid adenovirus/adenoassociated virus vector. Proc. Natl. Acad. Sci. USA 96:2615-2620[Abstract/Free Full Text].
41.	Rinaudo, D., S. Lamartina, G. Roscilli, G. Ciliberto, and C. Toniatti. 1999. Conditional site-specific integration into human chromosome 19 using a ligand-dependent chimeric AAV/rep protein. J. Virol. 74:281-294[Abstract/Free Full Text].
42.	Rizzuto, G., B. Gorgoni, M. Cappelletti, D. Lazzaro, I. Gloaguen, V. Poli, A. Sgura, D. Cimini, G. Ciliberto, R. Cortese, E. Fattori, and N. La Monica. 1999. Development of animal models for adeno-associated virus site-specific integration. J. Virol. 73:2517-2526[Abstract/Free Full Text].
43.	Roeder, G. S. 1997. Meiotic chromosomes: it takes two to tango. Genes Dev. 11:2600-2621[Free Full Text].
44.	Ryan, J. H., S. Zolotukhin, and N. Muzyczka. 1996. Sequence requirements for binding of Rep68 to the adeno-associated virus terminal repeats. J. Virol. 70:1542-1553[Abstract].
45.	Samulski, R. J. 1993. Adeno-associated virus: integration at a specific chromosomal locus. Curr. Opin. Genet. Dev. 3:74-80[CrossRef][Medline].
46.	Samulski, R. J., X. Zhu, X. Xiao, J. D. Brook, D. E. Housman, N. Epstein, and L. A. Hunter. 1991. Targeted integration of adeno-associated virus (AAV) into human chromosome 19. EMBO J. 10:3941-3950[Medline]. (Erratum, 11:1228, 1992.)
47.	Shelling, A. N., and M. G. Smith. 1994. Targeted integration of transfected and infected adeno-associated virus vectors containing the neomycin resistance gene. Gene Ther. 1:165-169[Medline].
48.	Snyder, R. O., D.-S. Im, T. Ni, X. Xiao, R. J. Samulski, and N. Muzyczka. 1993. Features of the adeno-associated virus origin involved in substrate recognition by the viral Rep protein. J. Virol. 67:6096-6104[Abstract/Free Full Text].
49.	Srivastava, A., E. W. Lusby, and K. I. Berns. 1983. Nucleotide sequence and organization of the adeno-associated virus 2 genome. J. Virol. 45:555-564[Abstract/Free Full Text].
50.	Surosky, R. T., M. Urabe, S. G. Godwin, S. A. McQuiston, G. J. Kurtzman, K. Ozawa, and G. Natsoulis. 1997. Adeno-associated virus Rep proteins target DNA sequences to a unique locus in the human genome. J. Virol. 71:7951-7959[Abstract].
51.	Tanimoto, K., Q. Liu, J. Bungert, and J. D. Engel. 1999. The polyoma virus enhancer cannot substitute for DNAseI core hypersensitive sites 2-4 in the human beta-globin region. Nucleic Acids Res. 27:3130-3137[Abstract/Free Full Text].
52.	Tuan, D., and I. M. London. 1984. Mapping of DNAse I-hypersensitive sites in the upstream DNA of human embryonic $varepsilon$ -globin gene in K562 leukemia cells. Proc. Natl. Acad. Sci. USA 81:2718-2722[Abstract/Free Full Text].
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