The Number of a U3 Repeat Box Acting as an Enhancer in Long Terminal Repeats of Polytropic Replication-Competent Porcine Endogenous Retroviruses Dynamically Fluctuates during Serial Virus Passages in Human Cells

doi:10.1128/JVI.75.15.6933-6940.2001

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Journal of Virology, August 2001, p. 6933-6940, Vol. 75, No. 15
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.15.6933-6940.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

The Number of a U3 Repeat Box Acting as an Enhancer in Long Terminal Repeats of Polytropic Replication-Competent Porcine Endogenous Retroviruses Dynamically Fluctuates during Serial Virus Passages in Human Cells

Gregor Scheef, Nicole Fischer, Ulrich Krach, and Ralf R. Tönjes^*

Paul-Ehrlich-Institut, D-63225 Langen, Germany

Received 22 December 2000/Accepted 2 May 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The organization and transcriptional regulation of porcine endogenous retrovirus (PERV) long terminal repeats (LTRs) are unknown.We have studied the activity of LTRs from replication-competentmolecular clones by performing luciferase reporter assays. TheLTRs differ in the presence and number of 39-bp repeats locatedin U3 that confer strong promoter activity in human, simian, canine,feline, and porcine cell lines, whereas for LTRs devoid of therepeats, the promoter strength was significantly reduced. As theactivity of a heterologous simian virus 40 promoter and a homologousrepeat-deficient LTR was elevated by four 39-bp repeats independentlyof its orientation and location, the repeat box complies withthe definition of an enhancer. During serial virus passaging ofmolecular PERV clones on human 293 cells, proviral LTRs demonstratedadaptation of transcriptional activity by dynamic changes of thenumber of 39-bp repeats in the course of up to 12 passagingcycles.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The discovery of porcine endogenous retroviruses (PERV) (25) and other pig microorganisms, such as herpesviruses (9),has strengthened objections to the clinical use of pig xenografts(11, 21, 28), which is intended to alleviate the limitedsupply of allografts for the treatment of human disorders. PERVdisplay approximately 50 proviral integration sites in the piggenome (1, 25), and recent reports have demonstrated thatPERV which are released from different pig cell lines infect humancells in vitro (19, 25, 34, 33).

The organization and transcriptional regulation of PERV long terminal repeats (LTRs), particularly those of human-tropic viruses,are unknown. We have studied the promoter activity of a numberof distinct PERV LTRs in transiently transfected mammalian celllines by using a Dual-Luciferase Reporter Assay System (Promega,Mannheim, Germany). LTRs were derived from different PERV molecularclones, including those replication-competent and human-tropicviruses that we have described recently (7, 14, 30). LTRsequences of clones 293-PERV-A(42) [hereafter, clones derivedfrom cell line 293 PERV-PK (18) will be referred to as 293-PERV-(A)42,293-PERV-B(33), 293-PERV-B(43), 293-PERV-B(43)-746, 293-PERV-B(43)-590,293-PERV-B(43)- $Delta$ , and 293-PERV-B(43)-Zero], 293-PERV-B(33), and293-PERV-B(43) differ by distinct numbers of a 39-bp repeat boxwhich is located in U3. The existence of repeat elements in viralpromoters which often act as enhancer elements is well known (10).In this report, we demonstrate that the level of promoter activitycorrelates with the number of 39-bp repeat boxes, which fluctuatesin the course of serial passaging of PERV in human cells. In addition,the repeat box represents a viral enhancer that modulates theactivity of heterologous and homologouspromoters.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cloning of PERV LTRs. LTRs were isolated from replication-competent molecular clones 293-PERV-A(42), 293-PERV-B(33)/ATG, 293-PERV-B(43) (7),and PK15-PERV-A(58) (14) by PCR using oligonucleotides 5'-PERV-LTRI and 3'-PERV-LTR/PBS I (Fig. 1). A PERV-C LTR was isolated fromminipig genomic DNA by using primers 5'-PERV-C-LTR and 3'-PERV-C-LTR(Fig. 1). To generate LTR 293-PERV-B(43)-Zero lacking the repeatbox, primers 5'-PERV-LTR I and 3'-PERV-Zero were used, as wellas oligonucleotides 5'-PERV-Zero and 3'-PERV-LTR/PBS I. Both amplificationproducts were fused by PCR using primers 5'-PERV-LTR I and 3'-PERV-LTR/PBSI. The 293-PERV-B(43)- $Delta$ LTR containing one 18-bp subrepeat wasproduced by using oligonucleotides 5'-PERV-LTR I and 3'-PERV-DelI in a first step. The generated amplification product was usedas the template for a PCR using primers 5'-PERV-LTR I and 3'-PERV-DelII in a second step. Together with the amplification product generatedby primers 5'-PERV-Del II and 3'-PERV-LTR/PBS I, that second productwas fused by using primers 5'-PERV-LTR I and 3'-PERV-LTR/PBS I.The sequences of the oligonucleotides used for PCR are availableupon request.

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FIG. 1. Organization and structure of PERV LTRs used for the Dual-Luciferase Reporter Assay. Except for those of the PERV-C, PK15-PERV-A(58), and deletion mutant 293-PERV-B(43)-Zero and 293-PERV-B(43)- $Delta$ LTRs, U3 regions harbor different numbers of the same 39-bp repeat, consisting of an 18-bp subrepeat and a 21-bp subrepeat. U3, R, and U5 are shown as open boxes, and repeats are shown as gray (18-bp subrepeat) and dark gray (21-bp subrepeat) boxes. The cap site (black triangle) and TATA box (open triangle) are indicated. Numbers indicate the locations of elements in the LTRs. Nucleotide positions refer to 293-PERV-B(33) (7).

Construction of expression vectors. To construct PERV LTR reporter vectors, primers 5'-PERV-LTR II bearing a KpnI site and 3'-PERV-LTR/PBS II bearing a BglIIsite were used. In addition to the LTRs mentioned above, LTR sequences293-PERV-B(43)-590 and 293-PERV-B(43)-746 were amplified withthe same primers by using as templates PCR products that weregenerated after serial passages of molecular clones in 293 cells(see below). As a control, a Rous sarcoma virus (RSV) LTR wasderived from pREP4 (Invitrogen, Groningen, The Netherlands) byusing primers 5'-RSV-LTR and 3'-RSV-LTR, bearing KpnI and BglIIsites, respectively. All PCR products were subcloned into pGEM-TEasy (Promega). KpnI and BglII inserts were further cloned intothe luciferase reporter vector pGL3 Basic(Promega).

Furthermore, the four 39-bp repeats of the 293-PERV-B(33) LTR (Fig. 1) were cloned into vector pGL3 Control (Promega) (seeFig. 4) in the forward and reverse orientations upstream of thesimian virus 40 (SV40) promoter and downstream of the gene forluciferase by using primers 5'-Repeat and 3'-Repeat, both containingKpnI and BamHI or BglII and SalI sites,respectively.

Cloning of the repeat box upstream of the 293-PERV-B(43)-Zero LTR (see Fig. 5) was performed by using primers 5'-Repeat and3'-Repeat, both containing a KpnI site. Cloning downstream ofthe LTR was performed by using the same primers containing BamHIand BglII sites, respectively. Those primers were also used forcloning of the repeat box into pGL3 Basic. All PCR amplificationproducts were subcloned into pGem-T Easy. Subsequently, insertswere cloned into the corresponding restriction sites of pGL3 Control,pGL3 Basic/293-PERV-B(43)-Zero, and pGL3 Basic,respectively.

Sequence analyses. DNA sequences of both strands of constructs were confirmed by primer walking with the double-stranded dideoxy-chain terminationmethod using Thermo Sequence fluorescent dye terminator cyclesequencing and precipitation kits (Amersham-Pharmacia, Freiburg,Germany). Sequencing reactions were performed with a Vistra DNALabstation 625 (Molecular Dynamics, Krefeld, Germany), and cyclesequencing was done on an ABI 373A or 377 DNA sequencing system(Applied Biosystems, Weiterstadt, Germany). Putative transcriptionfactor binding sites were analyzed by using MatInspector software(Genomatix, Munich,Germany).

Cell lines and transfection. The cell lines 293, ST-Iowa, and PK 15 were kindly provided by R. Weiss (London, England), and cell line A3.01 was obtainedfrom E. Flory at our institute. HeLa cells were purchased fromthe European Collection of Cell Cultures (ECACC 93021013), aswere MRC-5 cells (ECACC 84101801), Cos-7 cells (ECACC 87021302),PG-4 cells (ECACC 94102703), and D17 cells (ECACC 8909043). Allcell lines tested negative for mycoplasms. Plasmids used for transfectionwere prepared by using the EndoFree system (Qiagen, Hilden, Germany).Transfection was carried out with Lipofectamine (Life Technologies,Karlsruhe, Germany) for adherent cells, while DMRIE-C (Life Technologies)was used for the suspension cell line A3.01. Transfection wasperformed with six-well plates by using 1 µg of plasmid DNA cotransfectedwith 333 pg of internal standard pRL-CMV (Promega). At 5 h posttransfection,the transfection medium was replaced with appropriate culturemedium and the cells were grown for 43h.

Serial passaging of molecular PERV clones. Replication-competent molecular clones 293-PERV-B(33)/ATG and 293-PERV-B(43) (7) were used to transfect the human embryonickidney cell line 293. Cell-free supernatants filtered throughmembranes (0.45-µm pore size; Sartorius, Göttingen, Germany)were analyzed for reverse transcriptase (RT) activity by usingthe type C RT activity assay (protocol B; Cavidi Tech AB, Uppsala,Sweden). Cells were tested for expression of viral proteins byan indirect immunofluorescence assay using PERV Gag p10 antibody(15). Supernatants of productively infected cells were transferredto fresh 293 cells every 4 weeks for up to 12 months. At thosetime points, genomic nuclear DNA was purified from infected 293cells and integrated proviral LTRs were amplified by PCR usingprimers 5'-PERV-LTR I and 3'-PERV-LTR/PBSI.

Dual-Luciferase Reporter Assay System. The Dual-Luciferase Reporter Assay System (Promega) was used to investigate LTR activities. Transfected cells were washedwith phosphate-buffered saline and lysed with 300 or 100 µl (adherentor suspension cells, respectively) of passive lysis buffer (Promega)at room temperature for 10 min. Cell lysates were centrifugedat 13,000 × g for 1 min at room temperature, and supernatantswere stored at $-$ 20°C for testing. The luciferase assay was performedwith a MicroLumat Plus LB 96 V (EG&G Berthold, Bad Wildbad, Germany).Each measurement was carried out by using 20 µl of cell lysateafter addition of 50 µl of LAR II (Promega) and 50 µl of Stop& Glo (Promega) for a light-counting time of 10 s. For indicationof luciferase reactions exceeding the linear range, the luminometerwas adjusted to a diagnostic warninglevel.

Statistical analysis. For each cell line and each vector, at least three separate transfection experiments were carried out in triplicate. To normalizethe activity of the experimental reporter with regard to the activityof the internal control (pRL-CMV), the values of the internalcontrol were set as 1 and the ratio RLU_{experimental
reporter}/RLU_pRL-CMV(RLU is relative light units) was calculated. For each triplicateexperiment, the mean value and standard deviation were calculated.To assess the modulation of the SV40 promoter and the 293-PERV-B(43)-ZeroLTR by insertion of four 39-bp repeats, the mean values of bothwere set as 1 and the relative increase or decrease in luciferaseactivity was calculated. Formal statistical comparisons were notperformed, as, due to the small number of observations per constructand cell line, the power of the corresponding tests was consideredto be toolow.

Nucleotide sequence accession numbers. LTR nucleotide sequences of 293-PERV-B(43)-746 (AJ298073), 293-PERV-B(43)-590 (AJ298074), and PERV-C (AJ298075) havebeen deposited in GenBank. Clones 293-PERV-A(42) (AJ133817),PK15-PERV-A(58) (AJ293656), 293-PERV-B(33) (AJ133816), and293-PERV-B(43) (AJ133818) were used for generation of LTRs.PERV-MSL (AF038600) was used for homologystudies.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Structure and organization of PERV LTRs. The structure and organization of PERV LTRs are identical to those of other type C retroviruses, containing U3, R, and U5regions (Fig. 1). Among the investigated PERV LTRs, the greatesthomologies are found in R and U5. These are identical in 293-PERV-A(42),293-PERV-B(33), and 293-PERV-B(43). The LTR of PK15-PERV-A(58)differs by 2 nucleotides (nt) in R and by 9 nt in U5 comparedto that of 293-PERV-B(33), while the PERV-C LTR shows 1 nt differencein R and 18 nt differences in U5. The R and U5 regions of the293-PERV-B(33) LTR are 76 and 55% homologous to those of typicalmammalian type C retroviruses, as established by appropriate sequencealignments (5). In U3, only the extreme 5' (nt 1 to 6) and3' (nt 538 to 544) ends of 293-PERV-B(33) show homologies to LTRsequences highly conserved among mammalian type C retroviruses(5, 12); a TATA box exists, while a CCAAT box could not beidentified. The LTRs of 293-PERV-B(33) (total length, 707 bp)(7), 293-PERV-A(42) (668 bp) (7, 14), and 293-PERV-B(43)(629 bp) (7) contain four, three, and two copies of a 39-bprepeat, respectively; otherwise, they are identical (Fig. 1).The repeat comprises an 18-bp subrepeat located upstream of a21-bp subrepeat. An additional 18-bp subrepeat is located downstreamof the 39-bp repeat box. The LTR of PK15-PERV-A(58) (702 bp) (14)contains motifs homologous to the 18-bp repeat (2 nt differences;nt 462 to 480) and to the 21-bp subrepeat (2 nt differences; nt417 to 437) but separated from each other in U3. The U3 regionof the PERV-C LTR (595 bp) harbors sequences resembling thoserepeats with an 18-bp subrepeat (nt 98 to 118) and a 21-bp subrepeat(nt 383 to 403) (Fig. 1). Comparison of the LTR of 293-PERV-B(33)with those of PK15-PERV-A(58) and PERV-C shows homologies of 68and 61%, respectively. The proviral PERV-C LTR displays close(97%) homology to the PERV-MSL sequence (1) for a segment includingthe 3' end of U3, R, and U5, whereas the upstream part of theU3 region isdifferent.

Serial passaging of molecular PERV-B clones. PERV molecular clones 293-PERV-B(33)/ATG and 293-PERV-B(43) (7) were transfected into cell line 293, and the viruses producedthereafter were serially passaged. Both viruses displayed a steepincrease in RT activity in the first 2 weeks of each passage andthe development of a plateau in week 4. With regard to the completecourse, 293-PERV-B(33)/ATG showed maximum RT activity (400 mU/ml)during the first two passages whereas 293-PERV-B(43) yielded almostunchanged activities of up to 550 mU/ml (data notshown).

Proviral LTRs were amplified by PCR using genomic DNA at the end of each passage (week 4). The amplification products revealedmultiple bands for both clones at each time point. PCR productsrepresented LTRs which differed in length (Fig. 2A and B) becausethey had different numbers of 39-bp repeats, as revealed by sequenceanalysis. The LTR of molecular clone 293-PERV-B(33)/ATG containsfour 39-bp repeats (Fig. 1 and 2A, lane 7). The multiple bands(Fig. 2A, lane 1) demonstrating products corresponding to theoriginal proviral LTR, to the LTR of 293-PERV-A(42) (three 39-bprepeats; Fig. 1 and 2A, lane 8), and to the LTR of 293-PERV-B(43)(two 39-bp repeats; Fig. 1 and 2A, lane 9). Furthermore, an LTRrepresenting one 39-bp repeat (total length, 590 bp) was detectedin lower abundance (Fig. 1). From the second passage on, smallerLTRs corresponding to the 293-PERV-A(42) and 293-PERV-B(43) LTRswere detectable in larger amounts while the other LTRs still existedin smaller amounts (Fig. 2A, lanes 2 to 5).

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FIG. 2. PCR of PERV LTR DNA sequences originating from molecular virus clones 293-PERV-B(33)/ATG (A) and 293-PERV-B(43) (B) upon passaging in 293 cells. Multiple LTR bands are denoted (arrows). Lanes: 1, virus passage 1 (4 weeks postinfection [p.i.]); 2, virus passage 2 (8 weeks p.i.); 3, virus passage 3 (12 weeks p.i.); 4, virus passage 4 (16 weeks p.i.); 5, virus passage 10 (40 weeks p.i.); 6, negative control (water); 7 to 9, LTR PCR amplification products derived from plasmids pPERV-B(33), pPERV-A(42), and pPERV-B(43) (7), respectively.

The molecular clone 293-PERV-B(43) revealed a very similar pattern of LTR distribution during serial passaging (Fig. 2B, lanes1 to 5). Descendants of that clone comprised an additional provirusthat bears a previously unknown LTR containing five 39-bp repeats(total length, 746 bp) (Fig. 1), which was barely detectable afterthe first passage (Fig. 2B, lane1).

Promoter activity of PERV LTRs. The Dual-Luciferase Reporter Assay System was used to investigate the activities of different PERV LTRs. Native and deletion-containingLTRs were investigated, and an RSV LTR and an SV40 promoter wereused as controls. In all of the human (A3.01, 293, HeLa, and MRC-5),simian (Cos-7), canine (D17), feline (PG-4), and porcine (PK 15and ST-Iowa) cell lines tested, PERV LTRs demonstrated significantpromoter activities (Fig. 3; Table 1).

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FIG. 3. Activities of PERV LTRs cloned into luciferase reporter gene vector pGL3 Basic and of control vectors with respect to that of the internal control, pRL-CMV. (A) 293 cells; (B) A3.01 cells; (C) HeLa cells; (D) MRC-5 cells. n.d., not done. RLU, relative light units.

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TABLE 1. Activities of control vectors and retroviral LTRs cloned into luciferase reporter gene vector pGL3 Basic, with respect to that of internal control pRL-CMV, in nonhuman mammalian cells

In human cell lines 293, A3.01, and HeLa, the activities of PERV LTRs containing the 39-bp repeat, i.e., 293-PERV-B(43)-746,293-PERV-B(33), 293-PERV-A(42), 293-PERV-B(43), and 293-PERV-B(43)-590,were higher than the activities of the RSV LTR [up to 25-foldand 7-fold in 293 and A3.01 cells in the case of 293-PERV-B(43)-746,respectively; Fig. 3A to C]. In 293 and A3.01 cells, those PERVLTRs displayed activities even higher than that of the SV40 promoter(Fig. 3A and B). In contrast, native LTRs lacking the 39-bp repeat,PK15-PERV-A(58) and PERV-C, showed promoter activities that wereclearly reduced compared to that of the RSV LTR. In MRC-5 cells,PERV LTRs showed moderate activity similar to that of the RSVLTR (Fig. 3D). In all of the human cell lines, the activitiesof the LTR deletion mutants 293-PERV-B(43)- $Delta$ and 293-PERV-B(43)-Zerowere clearly reduced compared to that of the parental LTR. Reductionwas up to 67-fold for 293-PERV-B(43)- $Delta$ compared with the 293-PERV-B(43)-746LTR in 293 cells and 33-fold for 293-PERV-B(43)-Zero comparedwith the 293-PERV-B(43)-746 LTR in HeLa cells (Fig. 3A and C).In Cos-7 and D17 cells, the activities of LTRs resembled thosein human cells (Table 1). Native PERV LTRs, in contrast to themutant 293-PERV-B(43)- $Delta$ LTR, showed activities clearly higherthan that of the RSV LTR. The SV40 promoter showed stronger activitythan PERV LTRs in Cos-7 cells, whereas in D17 cells, the activitiesof PERV LTRs were almost equal to that of the SV40 promoter (Table1).

In contrast to these results, in feline (PG-4) and porcine cells (ST-Iowa and PK 15), the deletion mutant 293-PERV-B(43)-Zeroshowed strong activity, reaching levels similar to those of thenative LTRs, except for the 293-PERV-B(43)-746 LTR, which demonstratedthe highest activity in these cell lines (Table 1). In contrast,the PK15-PERV-A(58) LTR, naturally lacking the 39-bp repeat, showedweak activity compared to those of the other PERVLTRs.

Modulation of heterologous and homologous promoter activities. The repeat box (four 39-bp repeats plus an additional 18-bp subrepeat) of the 293-PERV-B(33) LTR was cloned into the luciferasevector pGL3 Control upstream and downstream of the heterologousSV40 promoter and the gene for luciferase in both orientationsto evaluate possible enhancer properties of the sequencemotif.

In human 293 and A3.01 cells, these vector constructs showed markedly increased promoter activity compared to that of theunmodified vector, independently of the location and orientationof the repeat box (Fig. 4A and B). The strongest activation ofthe SV40 promoter was found for the upstream forward construct,resulting in 5.4-fold-increased activity in 293 cells and 14.7-fold-increasedactivity in A3.01 cells. The weakest activation was observed forthe downstream forward construct in A3.01 cells and the downstreamreverse construct in 293 cells. In HeLa cells, only the upstreamconstructs elevated the activity 1.6-fold in the forward orientationand 1.9-fold in the reverse orientation. Reduced activities wereobserved when the repeat box was cloned downstream of the SV40promoter (0.8-fold in the forward orientation and 0.4-fold inthe reverse orientation) (Fig. 4C). In MRC-5 cells, only a moderateincrease in promoter activity was detectable for the downstreamforward construct (1.2-fold) and the downstream reverse construct(1.1-fold), respectively (Fig. 4D).

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FIG. 4. Modulation of a heterologous promoter by the 39-bp repeat box. The repeat box was inserted upstream of the SV40 promoter and downstream of the luc gene in both orientations. The mean value of pGL3 Control luciferase activity was set as 1, and the relative increase or decrease for the given construct is shown as fold activation. (A) 293 cells; (B) A3.01 cells; (C) HeLa cells; (D) MRC-5 cells. The SV40 promoter (black box), the luciferase gene (open box), and the 39-bp repeat box (alternately light and dark gray-striped box; arrow indicates orientation) are depicted.

Further luciferase vectors contained the four 39-bp repeats cloned upstream and downstream of the 293-PERV-B(43)-Zero LTRin both orientations. In 293, A3.01, and HeLa cells, the repeatbox mediated an increase in 293-PERV-B(43)-Zero LTR activity independentlyof location and orientation, yielding a uniform pattern for allof the cell lines tested (Fig. 5). The strongest activation wasfound for the downstream reverse vector, while the lowest levelof activation was found for the upstream forward construct. In293 cells, the maximum activation of the homologous promoter wasstronger than that of the heterologous SV40 promoter, while inA3.01 cells, the opposite pattern was found (Fig. 4A and B and5A and B). In HeLa cells, the activation by the repeat box wasalmost the same for both the homologous and heterologous promoters(Fig. 4C and 5C).

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FIG. 5. Modulation of the homologous promoter 293-PERV-B(43)-Zero LTR by the 39-bp repeat box. The repeat box was cloned into the vector pGL3 Basic/293-PERV-B(43)-Zero upstream and downstream of the PERV LTR in both orientations. The mean value of pGL3 Basic/293-PERV-B(43)-Zero luciferase activity was set as 1, and the relative increase or decrease for the given construct is shown as fold activation. (A) 293 cells; (B) A3.01 cells; (C) HeLa cells. The 293-PERV-B(43)-Zero LTR (black box), the 293-PERV-B(33) LTR (black box), the luciferase gene (open box), and the 39-bp repeat box (alternately light and dark gray-striped box; arrow indicates orientation) are depicted.

When the four 39-bp repeats were inserted directly upstream of the promoterless luciferase-encoding gene in both orientations,weak promoter activity, compared to that of the PERV LTRs, wasobserved (data notshown).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In this investigation, we have studied the transcriptional activity of a variety of LTRs derived from PERV-A and PERV-B molecularclones that are replication competent in human cells. A 39-bprepeat box in U3 was identified which multimerizes dynamicallyupon replication and acts as a viralenhancer.

The number of 39-bp repeats in PERV LTRs fluctuates upon serial virus passaging. Except for LTRs of PK15-PERV-A(58) and PERV-C, the native LTRs studied here differ only in the number of 39-bp repeats, consistingof 18- and 21-bp subrepeats, located in U3 (Fig. 1). The existenceof repeat elements in viral promoters is well known (10); repeatshave been described for retroviruses such as Moloney murine leukemiavirus (31), human T-cell leukemia virus types I and II (24,27), and Mus dunni endogenous retrovirus (35).

Serial passages of PERV-B clones in human 293 cells revealed adaptation to the new host on the transcriptional level. Virusclones 293-PERV-B(33)/ATG and 293-PERV-B(43), bearing four andtwo 39-bp repeats, respectively, yielded proviral LTRs that showedreduced or multiplied numbers of 39-bp repeats (Fig. 2A and B).The multimerization of specific U3 elements in PERV LTRs and theirarrangement as repeats do not necessarily originate from viruspassaging on human cells, since analysis of PERV sequences inBAC clones derived from the porcine genome revealed that clonePERV-B (Bac-192B9) contains a complete PERV-B sequence whose LTRis very closely related to the LTR of 293-PERV-A(42) and thusbears the three 39-bp repeats in U3 (30; M. Niebert et al., unpublisheddata). In addition, PCR analysis of PK15 cellular DNA demonstratedthe presence of LTRs bearing up to four 39-bp repeats (14).

However, the modulation of repeat numbers during serial passaging of PERV, indeed, reflects adaptation to the new host, aslate passages appear to yield one or two types of LTRs in majority,possibly representing the optimal number of 39-bp repeats forPERV replication in vivo (Fig. 2A and B, lanes 5). Although LTRsbearing a large number of 39-bp repeats showed increased activityin transient-transfection assays (Fig. 3; Table 1), those expandedLTRs might be disadvantageous for viral replication upon serialpassaging, as negative selection, for example, by interferencewith viral RNA packaging, may occur (20).

The mechanism of repeat multimerization is unknown. In contrast to the hypothesis which suggests the slippage of RT, as describedfor SL3 (20), we suppose that the mechanism causing repeat multimerizationin PERV is similar to that described for Mus dunni endogenousretrovirus (35). This hypothesis suggests a homologous misannealingduring reverse transcription which requires the availability ofother short repeat sequences flanking the repeat region, a patternwhich, indeed, is found for PERV where an additional 18-bp subrepeatis located downstream of the 39-bp repeat box (Fig. 1). In fact,the multimerization or reduction of PERV U3 repeats generatinga panel of different proviral LTRs already occurred during thefirst 4 weeks of virus passaging (Fig. 2A and B, lanes 1), revealingno mutation in the repeatsequence.

The number of 39-bp repeats in PERV LTRs modulates promoter activity. According to the different activities of PERV LTRs in human and mammalian cell lines (Fig. 3; Table 1), we suggest that PERVLTR expansion is caused by enhancermultimerization.

We have demonstrated that PERV LTRs containing up to five copies of a 39-bp repeat (Fig. 1) showed strong promoter activityin human and mammalian cell lines, while the activity of LTRsdevoid of the repeat was clearly decreased (Fig. 3; Table 1).The remaining activity of deletion-containing LTR constructs mightresult in a basal activity of the enhancerless promoter. Furthermore,the existence of additional enhancer elements located outsidethe repeats, as described for Moloney murine sarcoma virus (16),isconceivable.

With regard to the activities of different viral promoters in lymphoid T-cell lines (37), we conclude that the 293-PERV-B(43)-746LTR, showing stronger activity than the RSV LTR in human lymphoidA3.01 T cells, might be a useful tool for gene transfer applicationsthat depend on the level ofexpression.

The 293-PERV-B(43)-Zero LTR, however, showed strong activities in porcine and feline cells (Table 1). Obviously, in thosecell lines, the promoter activity is not influenced by the repeatunless the threshold of four 39-bp repeats is exceeded, sincethe 293-PERV-B(43)-746 LTR (five 39-bp repeats) demonstrated significantlystronger activity. As porcine cells harbor endogenous PERV-LTRs,this effect could be due to competition for specific transcriptionfactors. Alternatively, the threshold effect might be due to theexistence of negative regulatory elements located outside of theenhancer sequence, as shown for murine leukemia virus (4).

Different LTR activities cause different cell tropisms. The cell-specific activity of viral LTRs is responsible for viral cell tropism, as described for Jaagsiekte sheep retrovirus(23) and RSV (26). PERV-A and PERV-B released from pig cellsinfect human cells in vitro (19, 25, 33, 34), and molecularPERV-A and PERV-B clones are replication competent in 293, HeLa,and D17 cells (7, 14) and at lower levels in A3.01 cells(data not shown). PERV LTRs show strong activity in those celllines, which is a prerequisite for productive infection in conjunctionwith the existence of PERV-specific receptors. In contrast, MRC-5cells could not be infected with PERV (data not shown), whichis consistent with the weak activity of PERV LTRs and the lowsusceptibility of these cells to pseudotyped murine leukemia virus(29). Conversely, Cos-7 cells demonstrated strong promoter activityfor PERV; however, these cells lack PERV-specific receptors (29).Furthermore, feline PG-4 cells show strong replication rates forPERV-A (14), although the 293-PERV-A(42) LTR did not demonstrateactivity higher than those of the other PERVLTRs.

The U3 repeat box acts as an enhancer. As the repeatless 293-PERV-B(43)- $Delta$ and 293-PERV-B(43)-Zero LTRs showed clearly decreased promoter activity in human cellscompared to those of LTRs bearing the 39-bp repeat (Fig. 1 and3), we supposed that the repeat comprises enhancer elements. Apreliminary statistical transcription factor analysis revealedputative binding sites for nucleus factor Y in the 39-bp sequence(data not shown). The functional role of such repeats as enhancersis a common feature (10). For example, in the RSV LTR, deletionof enhancer elements led to a 94% reduction from the originalpromoter activity (6). In our studies, the four 39-bp repeats,indeed, mediated increased SV40 promoter activity independentlyof its orientation and location over a distance of 2,200 bp inthe case of the downstream constructs in human 293 and A3.01 cells(Fig. 4A and B). Thus, the 39-bp repeat bears known propertiesof classical enhancers (2, 13). In contrast, in HeLa cells,only weak activation of the SV40 promoter was found for both upstreamconstructs (Fig. 4C). These results may be due to the fact thatthe SV40 promoter itself showed extremely strong activity in HeLacells that was caused by the major role of transcription factorSp1, which triggers SV40 promoter activity (8), possibly notallowing significant modulation. In MRC-5 cells, all of the PERVLTRs tested showed weak activity (Fig. 3D). Likewise, the 39-bprepeat box did not activate the heterologous SV40 promoter (Fig.4D).

The influence of the 39-bp repeat box on a homologous repeat-free LTR, i.e., 293-PERV-B(43)-Zero, was further studied to substantiatethe enhancer hypothesis. The promoter constructs correspond tothe 293-PERV-B(33) LTR but bear a dislocated 39-bp repeat box(Fig. 1 and 5). In all of the cell lines tested, the dislocatedrepeat box increased the activity of the deletion mutant, irrespectivelyof location and orientation, which is additional proof of theenhancer properties of the repeat box (Fig. 5). According to theseresults, the orientation and location of the repeat box in theLTRs are important for promoter activity and the different levelsof activation reflect spacing effects, possibly leading to enhancersilencing (3).

The 39-bp repeat box itself, cloned in the promoterless luciferase vector pGL3 Basic upstream of the gene for luciferase inboth orientations, revealed weak promoter activity (data not shown).Weak transcriptional initiation in the absence of a promoter isa typical feature of enhancer elements (17) and has been described,e.g., for the SV40 72-bp enhancer repeat (22, 32).

Possible consequences of PERV integration into the human genome. The activity of PERV LTRs specifically correlates with the presence of a 39-bp repeat box in U3 which represents a viral enhancerthat activates heterologous, as well as homologous, promotersindependently of orientation andlocation.

Specific questions about the safety of porcine xenografts arise from these results. As proviral DNA integrates itself intothe host genome, replicating PERV may elicit pathogenic effectsmediated by the LTRs, as described for exogenous retroviruses(11, 13), endogenous retroviruses (18), and transposonsin general (36). In the case of xenotransplantation, the recipientwould be immunosuppressed to avoid rejection of the donor organ.As no steroid hormone-responsive element or NF- $kappa$ B sites couldbe identified in the PERV LTRs, it remains to be shown whetherimmunosuppressive drugs such as prednisolone and cyclosporinehave direct or indirect effects on LTR activities which mightadd to the safety concerns aboutPERV.

	ACKNOWLEDGMENTS

This study was supported by a grant from the German Ministry of Health (Bundesministerium für Gesundheit), Bonn,Germany.

We thank Egbert Flory for support regarding promoter assays and Peter Volkers for consultation about statistical analysis.The technical assistance of Gundula Braun is gratefullyacknowledged.

	FOOTNOTES

^* Corresponding author. Mailing address: Paul-Ehrlich-Institut, Paul-Ehrlich-Strasse 51-59, D-63225 Langen, Germany. Phone:49 6103 775304. Fax: 49 6103 771255. E-mail: toera{at}pei.de.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Akiyoshi, D. E., M. Denaro, H. Zhu, J. L. Greeenstein, P. T. Banerjee, and J. A. Fishman. 1998. Identification of full-length cDNA for an endogenous retrovirus of miniature swine. J. Virol. 72:4503-4507[Abstract/Free Full Text].

2. Blackwood, E. M., and J. Kadonaga. 1998. Going the distance: a current view of enhancer action. Science 281:60-63[Abstract/Free Full Text].

3. Bonifer, C. 2000. Developmental regulation of eukaryotic gene loci $---$ which cis-regulatory information is required? Trends Genet. 16:310-315[CrossRef][Medline].

4. Ch'ang, L.-Y., W. K. Yang, F. E. Myer, and D.-M. Yang. 1989. Negative regulatory element associated with potentially functional promoter and enhancer elements in the long terminal repeats of endogenous murine leukemia virus-related proviral sequences. J. Virol. 63:2746-2757[Abstract/Free Full Text].

5. Chen, H. R., and W. C. Baker. 1984. Nucleotide sequences of the retroviral long terminal repeats and their adjacent regions. Nucleic Acids Res. 12:1767-1778[Abstract/Free Full Text].

6. Cullen, B. R., K. Raymond, and G. Ju. 1985. Functional analysis of the transcription control region located within the avian retroviral long terminal repeat. Mol. Cell. Biol. 5:438-447[Abstract/Free Full Text].

7. Czauderna, F., N. Fischer, K. Boller, R. Kurth, and R. R. Tönjes. 2000. Establishment and characterization of molecular clones of porcine endogenous retroviruses replicating on human cells. J. Virol. 74:4028-4038[Abstract/Free Full Text].

8. Dynan, W. S., and R. Tjian. 1983. The promoter-specific transcription factor Sp1 binds to upstream sequences in the SV40 early promoter. Cell 35:79-87[CrossRef][Medline].

9. Ehlers, B., S. Ulrich, and M. Golz. 1999. Detection of two novel porcine herpesviruses with high similarity to gammaherpesviruses. J. Gen. Virol. 80:971-978[Abstract].

10. Fan, H. 1990. Influences of the long terminal repeats on retrovirus pathogenicity. Semin. Virol. 1:165-174.

11. Fishman, J. A. 1997. Xenosis and xenotransplantation: addressing the infectious risks posed by an emerging technology. Kidney Int. 51(Suppl. 58):41-45.

12. Golemis, E. A., N. A. Speck, and N. Hopkins. 1990. Alignment of U3 region sequences of mammalian type C viruses: identification of highly conserved motifs and implications for enhancer design. J. Virol. 64:534-542[Abstract/Free Full Text].

13. Khoury, G., and P. Gruss. 1983. Enhancer elements. Cell 33:313-314[CrossRef][Medline].

14. Krach, U., N. Fischer, F. Czauderna, and R. R. Tönjes. 2001. Comparison of replication-competent molecular clones of porcine endogenous retrovirus class A and class B derived from pig and human cells. J. Virol. 75:5465-5472[Abstract/Free Full Text].

15. Krach, U., N. Fischer, F. Czauderna, R. Kurth, and R. R. Tönjes. 2000. Generation and testing of highly specific anti-serum directed against porcine endogenous retrovirus nucleocapsid. Xenotransplantation 7:221-229[CrossRef][Medline].

16. Laimins, L. A., P. Gruss, R. Pozzatti, and G. Khoury. 1984. Characterization of enhancer elements in the long terminal repeat of Moloney murine sarcoma virus. J. Virol. 49:183-189[Abstract/Free Full Text].

17. Lang, J. C., and D. A. Spandidos. 1986. The structure and function of eukaryotic enhancer elements and their role in oncogenesis. Anticancer Res. 6:437-450[Medline].

18. Löwer, R. 1999. The pathogenic potential of endogenous retroviruses: facts and fantasies. Trends Microbiol. 7:350-356[CrossRef][Medline].

19. Martin, U., V. Kiessig, J. H. Blusch, A. Haverich, K. von der Helm, T. Herden, and G. Steinhoff. 1998. Expression of pig endogenous retrovirus by primary porcine endothelial cells and infection of human cells. Lancet 352:692-694[CrossRef][Medline].

20. Martiney, M. J., K. Rulli, R. Beaty, L. S. Levy, and J. Lenz. 1999. Selection of reversion and suppressors of a mutation in the CBF binding site of a lymphomagenic retrovirus. J. Virol. 73:7599-7606[Abstract/Free Full Text].

21. Michaels, M. G., and R. L. Simmons. 1994. Xenotransplant-associated zoonoses. Transplantation 57:1-7[Medline].

22. Moreau, P., R. Hen, B. Wasylyk, R. Everett, M. P. Gaub, and P. Chambon. 1981. The SV40 72 base pair repeat has a striking effect on gene expression both in SV40 and other chimeric recombinants. Nucleic Acids Res. 9:6047-6068[Abstract/Free Full Text].

23. Palmarini, M., S. Datta, R. Omid, C. Murgia, and H. Fan. 2000. The long terminal repeat of Jaagsiekte sheep retrovirus is preferentially active in differentiated epithelial cells of the lungs. J. Virol. 74:5776-5787[Abstract/Free Full Text].

24. Paskalis, H., B. K. Felber, and G. N. Pavlakis. 1986. Cis-acting sequences responsible for the transcriptional activation of the human T-cell leukemia virus type I constitute a conditional enhancer. Proc. Natl. Acad. Sci. USA 83:6558-6562[Abstract/Free Full Text].

25. Patience, C., Y. Takeuchi, and R. A. Weiss. 1997. Infection of human cells by an endogenous retrovirus of pigs. Nat. Med. 3:282-286[CrossRef][Medline].

26. Ruddell, A. 1995. Transcription regulatory elements of the avian retroviral long terminal repeat. Virology 206:1-7[CrossRef][Medline].

27. Shimotohno, K., D. W. Golde, M. Miwa, T. Sugimura, and I. S. Y. Chen. 1984. Nucleotide sequence analysis of the long terminal repeat of human T-cell leukemia virus type II. Proc. Natl. Acad. Sci. USA 81:1079-1083[Abstract/Free Full Text].

28. Stoye, J. P., and J. M. Coffin. 1995. The danger of xenotransplantation. Nat. Med. 1:1100[Medline].

29. Takeuchi, Y., C. Patience, S. Magre, R. A. Weiss, P. T. Banerjee, P. Le Tissier, and J. P. Stoye. 1998. Host range and interference studies of three classes of pig endogenous retrovirus. J. Virol. 72:9986-9991[Abstract/Free Full Text].

30. Tönjes, R. R., F. Czauderna, N. Fischer, U. Krach, K. Boller, P. Chardon, C. Rogel-Gaillard, M. Niebert, G. Scheef, A. Werner, and R. Kurth. 2000. Molecularly cloned porcine endogenous retroviruses replicate on human cells. Transplant. Proc. 32:1158-1161[CrossRef][Medline].

31. van Beveren, C., E. Rands, S. K. Chattopadhyay, D. R. Lowy, and I. M. Verma. 1982. Long terminal repeat of murine retroviral DNAs: sequence analysis, host-proviral junctions, and preintegration site. J. Virol. 41:542-556[Abstract/Free Full Text].

32. Wasylyk, B., C. Wasylyk, P. Augereu, and P. Chambon. 1983. The SV40 72 bp repeat preferentially potentiates transcription starting from proximal natural or substitute promoter elements. Cell 32:503-514[CrossRef][Medline].

33. Wilson, C. A., S. Wong, M. van Brocklin, and M. J. Federspiel. 2000. Extended analysis of the in vitro tropism of porcine endogenous retrovirus. J. Virol. 74:49-56[Abstract/Free Full Text].

34. Wilson, C. A., S. Wong, J. Muller, C. E. Davidson, T. M. Rose, and P. Burd. 1998. Type C retrovirus released from porcine primary peripheral blood mononuclear cells infects human cells. J. Virol. 72:3082-3087[Abstract/Free Full Text].

35. Wolgamot, G., and A. D. Miller. 1999. Replication of Mus dunni endogenous retrovirus depends on promoter activation followed by enhancer multimerization. J. Virol. 73:9803-9809[Abstract/Free Full Text].

36. Yoder, J. A., C. P. Walsh, and T. H. Bestor. 1997. Cytosine methylation and the ecology of intragenomic parasites. Trends Genet. 13:335-340[CrossRef][Medline].

37. Zarrin, A. A., L. Malkin, I. Fong, K. D. Duke, A. Ghose, and N. L. Berinstein. 1999. Comparison of CMV, RSV, SV40 viral and V $lambda$ 1 cellular promoters in B and T lymphoid and non-lymphoid cell lines. Biochim. Biophys. Acta 1446:135-139[Medline].

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1.	Akiyoshi, D. E., M. Denaro, H. Zhu, J. L. Greeenstein, P. T. Banerjee, and J. A. Fishman. 1998. Identification of full-length cDNA for an endogenous retrovirus of miniature swine. J. Virol. 72:4503-4507[Abstract/Free Full Text].
2.	Blackwood, E. M., and J. Kadonaga. 1998. Going the distance: a current view of enhancer action. Science 281:60-63[Abstract/Free Full Text].
3.	Bonifer, C. 2000. Developmental regulation of eukaryotic gene loci $---$ which cis-regulatory information is required? Trends Genet. 16:310-315[CrossRef][Medline].
4.	Ch'ang, L.-Y., W. K. Yang, F. E. Myer, and D.-M. Yang. 1989. Negative regulatory element associated with potentially functional promoter and enhancer elements in the long terminal repeats of endogenous murine leukemia virus-related proviral sequences. J. Virol. 63:2746-2757[Abstract/Free Full Text].
5.	Chen, H. R., and W. C. Baker. 1984. Nucleotide sequences of the retroviral long terminal repeats and their adjacent regions. Nucleic Acids Res. 12:1767-1778[Abstract/Free Full Text].
6.	Cullen, B. R., K. Raymond, and G. Ju. 1985. Functional analysis of the transcription control region located within the avian retroviral long terminal repeat. Mol. Cell. Biol. 5:438-447[Abstract/Free Full Text].
7.	Czauderna, F., N. Fischer, K. Boller, R. Kurth, and R. R. Tönjes. 2000. Establishment and characterization of molecular clones of porcine endogenous retroviruses replicating on human cells. J. Virol. 74:4028-4038[Abstract/Free Full Text].
8.	Dynan, W. S., and R. Tjian. 1983. The promoter-specific transcription factor Sp1 binds to upstream sequences in the SV40 early promoter. Cell 35:79-87[CrossRef][Medline].
9.	Ehlers, B., S. Ulrich, and M. Golz. 1999. Detection of two novel porcine herpesviruses with high similarity to gammaherpesviruses. J. Gen. Virol. 80:971-978[Abstract].
10.	Fan, H. 1990. Influences of the long terminal repeats on retrovirus pathogenicity. Semin. Virol. 1:165-174.
11.	Fishman, J. A. 1997. Xenosis and xenotransplantation: addressing the infectious risks posed by an emerging technology. Kidney Int. 51(Suppl. 58):41-45.
12.	Golemis, E. A., N. A. Speck, and N. Hopkins. 1990. Alignment of U3 region sequences of mammalian type C viruses: identification of highly conserved motifs and implications for enhancer design. J. Virol. 64:534-542[Abstract/Free Full Text].
13.	Khoury, G., and P. Gruss. 1983. Enhancer elements. Cell 33:313-314[CrossRef][Medline].
14.	Krach, U., N. Fischer, F. Czauderna, and R. R. Tönjes. 2001. Comparison of replication-competent molecular clones of porcine endogenous retrovirus class A and class B derived from pig and human cells. J. Virol. 75:5465-5472[Abstract/Free Full Text].
15.	Krach, U., N. Fischer, F. Czauderna, R. Kurth, and R. R. Tönjes. 2000. Generation and testing of highly specific anti-serum directed against porcine endogenous retrovirus nucleocapsid. Xenotransplantation 7:221-229[CrossRef][Medline].
16.	Laimins, L. A., P. Gruss, R. Pozzatti, and G. Khoury. 1984. Characterization of enhancer elements in the long terminal repeat of Moloney murine sarcoma virus. J. Virol. 49:183-189[Abstract/Free Full Text].
17.	Lang, J. C., and D. A. Spandidos. 1986. The structure and function of eukaryotic enhancer elements and their role in oncogenesis. Anticancer Res. 6:437-450[Medline].
18.	Löwer, R. 1999. The pathogenic potential of endogenous retroviruses: facts and fantasies. Trends Microbiol. 7:350-356[CrossRef][Medline].
19.	Martin, U., V. Kiessig, J. H. Blusch, A. Haverich, K. von der Helm, T. Herden, and G. Steinhoff. 1998. Expression of pig endogenous retrovirus by primary porcine endothelial cells and infection of human cells. Lancet 352:692-694[CrossRef][Medline].
20.	Martiney, M. J., K. Rulli, R. Beaty, L. S. Levy, and J. Lenz. 1999. Selection of reversion and suppressors of a mutation in the CBF binding site of a lymphomagenic retrovirus. J. Virol. 73:7599-7606[Abstract/Free Full Text].
21.	Michaels, M. G., and R. L. Simmons. 1994. Xenotransplant-associated zoonoses. Transplantation 57:1-7[Medline].
22.	Moreau, P., R. Hen, B. Wasylyk, R. Everett, M. P. Gaub, and P. Chambon. 1981. The SV40 72 base pair repeat has a striking effect on gene expression both in SV40 and other chimeric recombinants. Nucleic Acids Res. 9:6047-6068[Abstract/Free Full Text].
23.	Palmarini, M., S. Datta, R. Omid, C. Murgia, and H. Fan. 2000. The long terminal repeat of Jaagsiekte sheep retrovirus is preferentially active in differentiated epithelial cells of the lungs. J. Virol. 74:5776-5787[Abstract/Free Full Text].
24.	Paskalis, H., B. K. Felber, and G. N. Pavlakis. 1986. Cis-acting sequences responsible for the transcriptional activation of the human T-cell leukemia virus type I constitute a conditional enhancer. Proc. Natl. Acad. Sci. USA 83:6558-6562[Abstract/Free Full Text].
25.	Patience, C., Y. Takeuchi, and R. A. Weiss. 1997. Infection of human cells by an endogenous retrovirus of pigs. Nat. Med. 3:282-286[CrossRef][Medline].
26.	Ruddell, A. 1995. Transcription regulatory elements of the avian retroviral long terminal repeat. Virology 206:1-7[CrossRef][Medline].
27.	Shimotohno, K., D. W. Golde, M. Miwa, T. Sugimura, and I. S. Y. Chen. 1984. Nucleotide sequence analysis of the long terminal repeat of human T-cell leukemia virus type II. Proc. Natl. Acad. Sci. USA 81:1079-1083[Abstract/Free Full Text].
28.	Stoye, J. P., and J. M. Coffin. 1995. The danger of xenotransplantation. Nat. Med. 1:1100[Medline].
29.	Takeuchi, Y., C. Patience, S. Magre, R. A. Weiss, P. T. Banerjee, P. Le Tissier, and J. P. Stoye. 1998. Host range and interference studies of three classes of pig endogenous retrovirus. J. Virol. 72:9986-9991[Abstract/Free Full Text].
30.	Tönjes, R. R., F. Czauderna, N. Fischer, U. Krach, K. Boller, P. Chardon, C. Rogel-Gaillard, M. Niebert, G. Scheef, A. Werner, and R. Kurth. 2000. Molecularly cloned porcine endogenous retroviruses replicate on human cells. Transplant. Proc. 32:1158-1161[CrossRef][Medline].
31.	van Beveren, C., E. Rands, S. K. Chattopadhyay, D. R. Lowy, and I. M. Verma. 1982. Long terminal repeat of murine retroviral DNAs: sequence analysis, host-proviral junctions, and preintegration site. J. Virol. 41:542-556[Abstract/Free Full Text].
32.	Wasylyk, B., C. Wasylyk, P. Augereu, and P. Chambon. 1983. The SV40 72 bp repeat preferentially potentiates transcription starting from proximal natural or substitute promoter elements. Cell 32:503-514[CrossRef][Medline].
33.	Wilson, C. A., S. Wong, M. van Brocklin, and M. J. Federspiel. 2000. Extended analysis of the in vitro tropism of porcine endogenous retrovirus. J. Virol. 74:49-56[Abstract/Free Full Text].
34.	Wilson, C. A., S. Wong, J. Muller, C. E. Davidson, T. M. Rose, and P. Burd. 1998. Type C retrovirus released from porcine primary peripheral blood mononuclear cells infects human cells. J. Virol. 72:3082-3087[Abstract/Free Full Text].
35.	Wolgamot, G., and A. D. Miller. 1999. Replication of Mus dunni endogenous retrovirus depends on promoter activation followed by enhancer multimerization. J. Virol. 73:9803-9809[Abstract/Free Full Text].
36.	Yoder, J. A., C. P. Walsh, and T. H. Bestor. 1997. Cytosine methylation and the ecology of intragenomic parasites. Trends Genet. 13:335-340[CrossRef][Medline].
37.	Zarrin, A. A., L. Malkin, I. Fong, K. D. Duke, A. Ghose, and N. L. Berinstein. 1999. Comparison of CMV, RSV, SV40 viral and V $lambda$ 1 cellular promoters in B and T lymphoid and non-lymphoid cell lines. Biochim. Biophys. Acta 1446:135-139[Medline].