Characterization of a cis-Acting Sequence in the pol Region Required To Transfer Human Foamy Virus Vectors

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Heinkelein, M.
	Articles by Rethwilm, A.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Heinkelein, M.
	Articles by Rethwilm, A.

Previous Article | Next Article

J Virol, August 1998, p. 6307-6314, Vol. 72, No. 8
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Characterization of a cis-Acting Sequence in the pol Region Required To Transfer Human Foamy Virus Vectors

Martin Heinkelein, Michael Schmidt, Nicole Fischer, Astrid Moebes, Dirk Lindemann, Jörg Enssle, and Axel Rethwilm^*

Institut für Virologie und Immunbiologie, Universität Würzburg, Würzburg, Germany

Received 25 February 1998/Accepted 20 April 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

To identify cis-acting elements in the foamy virus (FV) RNA pregenome, we developed a transient-vector-production system basedon cotransfection of indicator gene-bearing vector and gag-poland env expression plasmids. Two elements which were criticalfor vector transfer were found and mapped approximately. The firstelement was located in the RU5 leader and the 5' gag region (approximatelyup to position 650 of the viral RNA). The second element was locatedin an approximately 2-kb sequence in the 3' pol region. Althoughsmall 5' and 3' deletions, as well as internal deletions of thelatter element, were tolerated, both elements were found to beabsolutely required for vector transfer. The functional characterizationof the pol region-located cis-acting element revealed that itis essential for efficient incorporation or the stability of particle-associatedvirion RNA. Furthermore, virions derived from a vector lackingthis sequence were found to be deficient in the cleavage of theGag protein by the Pol precursor protease. Our results suggestthat during the formation of infectious virions, complex interactionsbetween FV Gag and Pol and the viral RNA take place.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

The identification of cis-acting RNA elements is a prerequisite for the establishment of safe retroviral vectors and packagingcell lines (28, 33). In retroviruses, cis-acting sequences(CASs) may be involved in RNA dimerization and genome packaging(4, 28), in reverse transcription (50), and in the regulationof gene expression at the transcriptional or posttranscriptionallevel (11). Some of these sequences, such as the transcriptionaltrans-activator response element or the Rev response element oflentiviruses, interact with viral regulatory proteins (11).While these elements can be replaced by constitutive promotersor constitutive RNA transport elements (CTEs), respectively, RU5and U3R sequences of the long terminal repeat (LTR), adjacentsequences (the polypurine tract [PPT] and the primer binding site,and RNA dimerization and packaging sequences must invariantlybe present on the retrovirus vector genome (7, 22, 33,54). Fortunately, some of these elements overlap at least partiallyin the retrovirus vectors, which have been characterized in detail(4, 33).

The use of foamy virus (FV)-derived vectors in gene transfer experiments may be more advantageous than murine leukemia virus-derivedvectors, and preliminary constructs have already been used (5,18, 39, 45, 47). However, the FV CASs have not been characterized.Furthermore, the replication strategy of FVs appears to differmarkedly from those of all other retroviruses (34, 44, 52,53). We therefore wished to improve FV vectors and to learnmore about the unusual mode of replication of this virus groupby characterizing the cis-acting RNA elements of the so-calledhuman FV (HFV) isolate.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Cells and viruses. Baby hamster kidney cells (BHK-21), human fibroblasts (KMST6) (37), and simian virus 40 T-antigen-expressing human embryonalkidney cells (293T) (12) were cultivated in Eagle's minimalessential medium or Dulbecco's modified Eagle's medium supplementedwith 5 to 10% fetal calf serum and antibiotics.

Recombinant DNA. The pcHSRV2 (27, 34)-derived and human cytomegalovirus (CMV) immediate-early enhancer- and promoter-directed HFV expressionplasmids (pMH4, pMH5, and pMH5/M54) and the HFV gag-pol and envgene expression plasmids (pCgp-1 and pCenv-1) have been describedpreviously (16). The pol gene expression plasmid, pCpol-2, wasmade by substituting a 4.28-kb XbaI fragment of pPZ-2 (21) fora 5.74-kb XbaI fragment of pHSRV2 (47). Thus, this plasmid containsthe CMV enhancer and promoter directing the expression of a polgene transcript with a spliced leader sequence (21). Vectorswere made by deleting pMH5 or pMH5/M54 constructs with suitablerestriction enzyme sites and by religation after treatment ofthe ends with Klenow enzyme or phage T4 polymerase as appropriate.All vectors bear an expression cassette made up of the spleenfocus-forming virus (SFFV) U3 region (2) and the gene codingfor green fluorescent protein (GFP), as described previously (16).

The plasmid pSP/HFV-2, which was used to generate the antisense cRNA probe for the RNase protection analysis, was made byinserting a 760-bp HindIII-AvrII (blunted) fragment spanning aregion from the HindIII site in U3 of pHSRV2 (47) to the AvrIIsite in the gag leader into HindIII-EcoRI (blunted)-cut pSP65.

Analysis of vector transfer efficiency. DNAs were prepared with Maxi Kit columns (Qiagen). Equal amounts of vector-containing DNA (27 µg) and the expression plasmidsfor the HFV structural proteins were transiently transfected into2 × 10⁶ 293T cells in 6-cm-diameter dishes as calcium phosphate coprecipitates(1, 48). Twenty-four hours posttransfection, the CMV promoterwas induced with 10 mM sodium butyrate for 8 h (48). Forty-eighthours following transfection, the supernatant was harvested andpassed through a 0.45-µm-pore-size filter (Schleicher & Schuell)and 1 ml of each was applied to BHK-21 and KMST6 recipient cellsseeded the day before at a density of 3 × 10³ cells per well in 24-well plates. Seventy-two hours followingtransduction, the recipient cells were detached from the plasticsupport and washed in phosphate-buffered saline. At that time,approximately 5 × 10⁴ BHK-21 cells and 2 × 10⁴ KMST6 cells were harvested. The amounts of transduced cells weredetermined by fluorescence-activated cell sorting on a FACScandevice with the LysisII and CellQuest software packages (BectonDickinson) and expressed as the percentages of GFP-positive cellsin relation to the total number of cells analyzed. All experimentswere done with at least two independent plasmid preparations andat least four times. We always found some variation (as indicatedin the figures) from assay series to assay series, probably dueto transfection efficiencies. However, the results within a seriesof experiments were consistent.

Protein analysis. Lysates from transfected cells or from cell-free virus which was sedimented through a 20% sucrose cushion in TNE (100 mM Tris-HCl,100 mM NaCl, 1 mM EDTA [pH 8.0]) for 3 h at 25,000 rpm in an SW41rotor (Beckman) at 4°C were prepared as described previously (17).The samples were run on sodium dodecyl sulfate-polyacrylamidegels (8% polyacrylamide) and semidry blotted onto nitrocellulosemembranes (Schleicher & Schuell). The blots were allowed to reactwith rabbit antisera raised against recombinant HFV Gag (17)and RNase H (23) and were developed with the ECL detection system(Amersham).

RNase protection analysis. Supernatants from four 6-cm-diameter dishes, which were transfected with the same plasmids, were pooled and passed througha 0.45-µm-pore-size filter and the viral particles were concentratedby ultracentrifugation through a 20% sucrose cushion as describedabove. The virus particle-containing sediment was resuspendedin 60 µl of phosphate-buffered saline. Twenty microliters wasused for immunoblot analysis, and viral RNA was extracted fromthe remaining 40 µl with the Qiamp viral RNA kit (Qiagen). RNaseprotection analysis was performed with the HypSpeed RPA kit accordingto the instructions of the manufacturer (Ambion) and with 20 µlof a total volume of 50 µl of RNA eluted from the preparationcolumn. Following linearization with HindIII, an antisense 777-nucleotide(nt) riboprobe was synthesized with 25 µCi of [ $alpha$ -³²P]GTP (Amersham) by standard protocols (1). The probe was resuspendedin 50 µl of sodium dodecyl sulfate-containing buffer, and 0.05µl (containing approximately 10,000 cpm) was used per reaction.RNase digestion was performed with 20 µg of RNase A/ml and 400U of RNase T₁/ml for 40 min at 37°C. The reaction products wereresolved on 7 M urea-containing 5% polyacrylamide gels. Once dry,the gels were exposed to X-ray film, and quantification was performedwith a Molecular Dynamics PhosphorImager.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Design of the experimental strategy. HFV is a complex retrovirus (10, 43). In addition to the Gag, Pol, and Env proteins, replication of HFV requires at leastthe presence of the Tas-Bel-1 transcriptional trans-activator(3, 43). All previous HFV vector constructs depended on theTas protein, which was either encoded in the vector genome (39,47) or provided for by cotransfection of replication-competenthelper virus, by a Tas expression plasmid (18, 45), or bya stable Tas-expressing cell line (5). To develop HFV vectorswhich are independent of Tas, we generated an expression plasmid(pMH4) (Fig. 1) in which gene expression of the provirus was regulatedby the strong CMV promoter. In this plasmid, the start of transcription,beginning with the R region of the LTR, was preserved (27, 34).The 3' region of the HFV genome with the accessory bel genes wasdeleted, and an expression cassette for GFP under the controlof the constitutively active SFFV U3 region was inserted. Transfectionof pMH4 gives rise to virus which is able to perform one roundof replication. Following integration into recipient cells, geneexpression from the HFV LTR is silent and the SFFV U3 promoterdirects the expression of GFP, which can easily be monitored.Transfection of an infectious genome under the control of theCMV promoter (pcHSRV2) into 293T cells has been reported to giverise to up to 10⁵ infectious viruses within 48 h (27). When pMH4 was transfectedinto 293T cells and hamster or human fibroblasts were exposedto the supernatant, transduction efficiencies were usually over50% under the assay conditions outlined above (Fig. 2). When thetransduced cells were reanalyzed following cultivation for severalweeks, the percentage of GFP-positive cells remained unchanged,indicating that the transduction was stable (data not shown).The transduction efficiency of recipient cells did not vary significantlywhen the env gene was deleted from the vector genome and Env wasprovided from a separate expression construct (pMH5 and pCenv-1)(Fig. 1). Neither did it vary when the pol gene ATG of pMH5 wasdown-mutated (pMH5/M54) and Env and Pol (pCgp-1) (Fig. 1) wereprovided in trans by triple plasmid cotransfection of 293T cells(see values in Fig. 2). Using this functional assay, we generateda set of deletion mutants of the vector to identify the regionsof the genome critical for vector transfer.

View larger version (16K):
[in this window]
[in a new window]

FIG. 1. HFV genome organization and basic HFV vectors and expression plasmids. The scale at the top is drawn with respect to the start of transcription (position 1 of R in the LTR). Vertical arrows above the pol gene of HFV indicate the location of purine-rich sequences which may serve as internal initiators of plus-strand synthesis during reverse transcription. The fourth central PPT has been characterized previously (25, 51). The arrow in the env gene indicates the FV-specific internal promoter (31). In pMH4, pMH5, and pCgp-1, the start of transcription of the CMV promoter, which drives the expression of HFV genes, is identical to that of HFV. In pMH4 and pMH5, an internal cassette made up of the SFFV U3 region that directs the expression of GFP (S65T) was inserted upstream of the 3' LTR (16). The 3' LTR was derived from the infectious clone pHSRV2 (47). This LTR is a deletion variant of the full-length LTR, and it occurred spontaneously in cell culture (46). pCpol-2 is a Pol expression plasmid. It contains the leader sequence of the spliced HFV pol mRNA (21). pA⁺ indicates the polyadenylation signal derived from bovine growth hormone and present in the pcDNA vector (Invitrogen).

View larger version (37K):
[in this window]
[in a new window]

FIG. 2. Two cis-acting elements are required to transfer HFV vectors. The vector plasmids (9 µg) together with pCgp-1 (9 µg) and pCenv-1 (9 µg), or adjusted with pcDNA (in the cases of pMH4 and pMH5) for a total amount of 27 µg of DNA, were transfected into 293T cells. The cell-free supernatant was used to transduce BHK-21 and KMST6 cells. The results are expressed as the percentages of GFP-positive cells relative to the total number of cells analyzed and represent the means and standard errors from four independent experiments. The locations of restriction enzyme sites used to construct the vectors are indicated with respect to the start of transcription. Deletions are marked as dotted lines. The scale is as in Fig. 1.

Two cis-acting elements are essential to transfer HFV vectors. The deletion of the 3' part of the pol region (pMH6) (Fig. 2) abrogated transduction by HFV vectors, while the 5' portionof pol was not required for efficient transfer (pMH12) (Fig. 2).This indicated that one essential CAS was located approximatelybetween positions 3870 and 5885 after the start of transcription(position 1 of the R region of the LTR).

Retroviral packaging sequences are usually located in the 5' region of the genome to avoid the packaging of subgenomic RNAs(4, 28). To determine whether a 5' CAS existed in the HFVgenome, we generated a series of deletion mutants extending intothe gag region with a plasmid which contained the element in polidentified in the previous experiments (pMH15). As shown in Fig.2, deletions were tolerated up to position 645 (pMH18), whilefurther deletions up to position 553 (pMH19) and 434 (pMH20) ledto modest or severe reductions in transfer efficiencies, respectively.Since the ATG start codon of the gag gene is located at position445 of the RNA (32), the 5' CAS of HFV extends into the gaggene. With pMH15, we observed a reduced transduction efficiencyrelative to that of pMH18, although the deletion in the latterwas greater (Fig. 2). This discrepancy is probably due to thefact that a relatively large aberrantly truncated Gag protein(approximately 200 amino acids) is expressed from pMH15, whichmay dominantly interfere with HFV particle assembly. With someother deletion constructs which could generate aberrant Gag-Polfusion proteins, such a dominant negative effect on the transferof pMH5 wild-type vector was observed (data not shown).

Taken together, the results presented in Fig. 2 indicate that two CASs are essential for the transfer of HFV-based vectors.One is located in the 5' leader region (CAS I) and one in the3' pol region (CAS II).

In the experiment whose results are presented in Fig. 2, all vector constructs except pMH4 and pMH5 were cotransfected withthe Gag-Pol and Env expression plasmids, pCgp-1 and pCenv-1. TheRU5 leader region and the gag and pol regions are contained inthe pCgp-1 plasmid (Fig. 1) because in FVs, Pol is expressed froma spliced mRNA, and the splice donor site is located in the Rregion at position 51 (35). Therefore, copackaging of the pCgp-1-derivedprimary transcript may take place, since it harbors CAS I andCAS II. RNase protection analysis revealed that pCgp-1 RNA wasindeed packaged into virions (data not shown). However, the pCgp-1transcript does not contain the U3-GFP cassette (Fig. 1), anda significant reduction in vector transfer efficiencies due tocopackaging of pCgp-1 RNA with the vector RNA was not observed(compare the transduction efficiencies obtained with pMH4 or pMH5with those obtained with pMH5/M54, pMH12, or pMH18, as shown inFig. 2).

Fine mapping of CAS II. The second CAS was located in an approximately 2-kb fragment at the 3' end of the pol region and extending approximately 160nt into the env region (pMH12 in Fig. 2). To better understandthe function of CAS II in vector transfer and to optimize thecapacity of HFV vectors further, deletion mutants of the HpaI-EcoRVfragment (i.e., the fragment occupying positions 3146 to 5885of the viral RNA) of pMH18, a plasmid which already has 3' gagsequences downstream of position 645 deleted (Fig. 2), were constructed.Deletions introduced into the HpaI-EcoRV fragment in the 3' directionwere tolerated up to position 3871 (pMH25) (Fig. 3). Further deletionsup to position 4663 (pMH27) or 5216 (pMH30) resulted in significantlyreduced transfer efficiency (Fig. 3). Removal of approximately650 bp from the 3' region of the element (pMH26) led to a similarreduction. The transfer activity was restored when smaller deletionsfrom the 5' and 3' ends of the fragment were introduced (pMH32)or when only small internal fragments, i.e., of 550 or 220 bp,were removed from CAS II (pMH28 and pMH29 in Fig. 3, respectively).The experiments with the latter constructs suggest that CAS IIis bipartite.

View larger version (38K):
[in this window]
[in a new window]

FIG. 3. Fine mapping of CAS II. HFV vector deletion constructs were used to characterize the RNA element in the pol region more precisely. The experimental strategy described in the legend for Fig. 2 was used. The vertical arrows in pMH43 (bottom) indicate the location of purine-rich sequences, at least one of which probably functions as an internal PPT for the initiation of plus-strand synthesis (25, 51). Deletions are marked as dotted lines. The scale is as in Fig. 1.

It has been shown previously that HFV contains in the center of the genome (in the 3' pol region) a duplication of the PPT(25, 51). Such an internal PPT is also found in lentiviruses(9). For human immunodeficiency virus (HIV), the second PPTis involved in dual initiation of plus-strand synthesis (8).Furthermore, it has been reported that the central PPT is requiredfor optimal HIV replication in cell culture (8). We thereforewished to analyze whether the central PPT of HFV plays a majorrole in mediating transfer by CAS II. While efficient transferwas obtained with pMH32, a construct with a deletion in the PPT(pMH43) led to an approximately 50% reduction of transfer efficiency(Fig. 3). This indicated that the PPT may play some role in vectortransfer. Closer inspection of the genomic region in questionrevealed that not one but four potential central PPTs are presentin HFV (Fig. 1 and 3). It has not yet been determined which ofthese can be used by the virus and whether any of these is requiredfor efficient viral replication. However, pMH27, which containedall potential PPTs, was not transferred efficiently (Fig. 3).Furthermore, with pMH31, which contained the two centrally locatedpotential PPTs, transfer efficiency was reduced to the value ofthe negative control, pMH14, which lacked the complete CAS II(Fig. 3). The same holds true for a derivative of pMH14, pMH24,into which the fourth and originally reported PPT (25, 51)was introduced as an oligonucleotide (data not shown). These experimentsindicated that the functions of the internal PPT and CAS II aredifferent and required further analysis.

Effect of CAS II on gene expression and virion RNA content. The effect of CAS II on vector transfer led us to hypothesize that it has a function in either posttranscriptional regulationof gene expression or genome packaging. To investigate these topics,we used the three constructs, pMH5/M54, pM38, and pMH40, depictedin Fig. 4A. Common to the constructs is the presence of the completegag gene and the down-mutation of the pol gene ATG to CTG (14).While pMH5/M54 contained the complete pol region, pMH38 had the3' pol region (CAS II) deleted, and pMH40 lacked the 5' pol regionand contained CAS II. As expected from the results presented inFig. 3, cotransfection of pCpol-2 and pCenv-1 with the vectorDNAs affected transfer only with pMH5/M54 and pMH40 (Fig. 4A).

View larger version (28K):
[in this window]
[in a new window]

FIG. 4. Effect of CAS II on HFV protein expression and virion RNA content. The Gag-positive and Pol-negative vectors pMH5/M54, pMH38, and pMH40 were used to determine these effects. (A) The vector plasmids were cotransfected with pCpol-2 and pCenv-1 into 293T cells, and the transduction efficiencies of cell-free viruses were determined on BHK-21 cells. Results are expressed as described for Fig. 2. (B) The immunoblot analysis of 293T cells transfected with the vector constructs plus pCenv-1 revealed that all plasmids expressed similar amounts of Gag (pr74), thus ruling out an essential role for CAS II as an RNA transport element. A diluted lysate from BHK-21 cells infected with HSRV2, the virus derived from pHSRV2, was run as a control. (C) Gag content of cell-free particles following centrifugation through a sucrose cushion. Similar amounts of pr74^gag are present in the preparations of cells cotransfected with pCenv-1 plus either pMH5/M54, pMH38, or pMH40. Note that Env coexpression is required for cellular export of HFV capsids (16). (D) RNase protection analysis of virion RNA in the particulate material analyzed in Fig. 4C for Gag content. 5' (401-nt) and 3' (554-nt) fragments corresponding to the RU5 and U3R regions, respectively, of the viral RNA are specifically protected in pMH5/M54- and pMH40-derived virions. pMH38-derived virions showed an 80% reduced RNA content. The marker lane (M) contained in vitro-transcribed RNA from pSP/HFV-2 which was linearized with HindIII (777 nt), BsaAI (621 nt), and XbaI (429 nt).

Analysis of protein expression in cells transfected with the vector plasmids and pCenv-1 revealed that all three constructsexpressed pr74 Gag precursor protein to a similar extent (Fig.4B). Since the Gag protein could be expressed only from the vectorgenomes, it is very unlikely that CTE plays a role in CAS II-mediatedvector transfer.

We next investigated the virion RNA content of the three vector genomes. The replication strategy of HFV poses a problem inthis analysis, since reverse transcription of the RNA pregenomemost likely takes place as a late event in the viral replicationcycle before the budding of the virus (34). Although a definiteanswer to this question is not yet available, at the least, thepresence of large amounts of virion DNA (53) complicates thedetection and quantification of packaged virion RNA. To circumventthis problem, we analyzed the RNA content of extracellular virionsprepared following cotransfection of the vector plasmids (Fig.4A) with pCenv-1 alone. In this situation reverse transcriptioncannot occur. However, cleavage of the Gag precursor (pr74) togenerate the p70 molecule, which probably represents the finalcapsid-forming structure (16), also cannot occur (24). Theexpression of pr74 has been reported to result in a majority ofaberrantly formed capsid structures which are, however, envelopedupon coexpression of HFV Env (16, 24). Thus, we observed efficientcellular export of particulate material following cotransfectionof vector plasmids with the Env protein expression construct (Fig.4C). RNase protection analysis of similar amounts of virions,as judged by immunoblot analysis of Gag (Fig. 4C), revealed thatvector RNA was specifically protected in extracellular virionsprepared from cells cotransfected with pMH5/M54 plus pCenv-1 (Fig.4D). Specific bands of 401 and 554 nt, which corresponded to theprotection of 5' and 3' LTR regions (Fig. 4D), respectively, werealso detected in virions prepared from cells cotransfected withpMH40 plus pCenv-1 and, to a much lesser extent, in virions preparedfrom cells cotransfected with pMH38 plus pCenv-1 (Fig. 4D). Quantification(the mean of three assays) of the band corresponding to the protected5' RNA fragment revealed that in relation to the RNA content ofpMH5/MH54-derived virions (100%), the RNA content of pMH40-derivedvirions was approximately 90%, while the RNA content in pMH38-derivedvirions was reduced to approximately 20%. This suggests that CASII has a major effect on RNA pregenome packaging or virion RNAstability. Furthermore, unlike hepadnaviruses, HFV appeared notto require Pol for incorporation of virion RNA (38).

Effect of CAS II on virion protein content. We examined the protein composition of virions prepared from cells which were transfected with pCpol-2 and pCenv-1 plus thevector plasmids pMH5/M54, pMH38, or pMH40. As shown in Fig. 5,the p70-pr74 Gag doublet was detected in cellular lysates andextracellular virions following transfection of pMH5/M54 or pMH40together with pCpol-2 and pCenv. In sharp contrast to this, wenever observed cleavage of the pr74 Gag precursor protein in virionsprepared from the supernatant of cells transfected with pMH38plus pCpol-2 and pCenv-1. Immunoblotting with a Pol-specific antiserumdetected the precursor protein pr127 and the p80 reverse transcriptasein the lysates from cells transfected with the vector plasmids,which ruled out the possibility that the inability to cleave pr74^gag in pMH38-transfected cells was due to a lack of expression ofactive Pol (Fig. 5). When extracellular virions were probed forPol to determine whether it was incorporated into the virus particle,the assay sensitivity was at the margin of the detection level,yielding inconclusive results (data not shown).

View larger version (31K):
[in this window]
[in a new window]

FIG. 5. Effect of CAS II on Pol function. pMH5/M54, pMH38, and pMH40 were cotransfected into 293T cells together with pCpol-2 and pCenv-1. Forty-eight hours following transfection, Gag proteins were analyzed by immunoblotting in cellular lysates and in particulate material centrifuged through a sucrose cushion. A weak band which reacted with the Gag antibody and comigrated with the p70^gag band was often detected in cellular lysates of mock-transfected 293T cells. Therefore, this weak band in pMH38-transfected cells was regarded as being nonspecific. The cellular lysate blot reacted with Gag antibody was stripped and subsequently reacted with Pol antibody.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

The identification of cis-acting elements is a key step in the development of viral vectors. Using a sensitive indicator genesystem, which is based on efficient transient virus productionfollowing transfection of vector, and Gag-Pol and Env expressionplasmids (26, 48), we were able to identify CASs in the HFVgenome. One element was located in the 5' leader region of thepregenomic HFV transcript. In other retroviruses, the major RNApackaging sequence has been located in this region (4, 28,33), and it is likely that further studies will identify a similarfunction for the signal in question in HFV. This hypothesis issupported by the finding that the dimer linkage sequence of HFVis located in the 5' leader (15). In other retroviruses, thedimer linkage sequence and RNA packaging sequence usually overlap(4, 33).

By the same experimental strategy, we found another CAS in the 3' pol region of HFV, the presence of which was absolutelyrequired for vector transfer. This pointed to an essential roleof CAS II in viral replication. Further investigation of CAS IIrevealed that its function was independent of the additional PPTlocated in the central region of the HFV genome (25, 51).Although the presence of an internal PPT had some influence onvector transfer efficiency, the locations of CAS II and the PPTcould clearly be separated with appropriate vector constructs(Fig. 3). Similar findings have been made for HIV (42). Thepresence of the central PPT in the vector genome led only to amodest (twofold, as observed in the present study for HFV) increasein gene expression following transduction of recipient cells (42).In addition, currently used HIV vectors lack the central PPT (22,36).

Further, CAS II was found not to be required for efficient gene expression. CTEs have been identified in a variety of retrovirusesand in hepadnaviruses (7, 19, 20, 41, 49, 54). Infunctional terms, HFV belongs to the group of complex regulatedretroviruses (10, 43). However, in contrast to the lentivirusand the human T-cell leukemia and bovine leukemia groups of complexretroviruses, a posttranscriptionally acting regulatory proteinhas not been found for HFV, and structural gene expression appearedto be independent of RNA sequences outside the coding regions(3, 16). As deduced from the results shown in Fig. 4, thepresence or absence of CAS II had no major influence on the expressionof the HFV vectors used, and therefore, CAS II is unlikely toinfluence RNA transport. Since HFV makes extensive use of RNAsplicing (27, 30, 35), the identification of an FV-specificCTE is still awaited.

RNase protection analysis revealed the major influence of CAS II on virion RNA content. This can be interpreted as an indicationthat either CAS II is a genuine packaging sequence or its presenceis essential for stabilization of the RNA in the viral particle.Further experiments are required to clarify this question. Surprisingly,we found that the influence on viral RNA content was not the soleeffect of CAS II. The protein analysis of HFV virions showed that,in particles derived from a vector devoid of CAS II (pMH38), cleavageof the Gag precursor protein does not occur. The finding thatcleavage of pr74^gag is absolutely essential for HFV infectivity (13, 24) explainsthe very low transduction rate obtained with this vector. However,the reason for the lack of Gag cleavage is unclear at the moment.The protease of FVs is encoded in the pol reading frame (40,43), and HFV expresses Pol independently of Gag from a splicedmRNA (6, 14, 21, 29, 53). The mechanism by which HFVPol is incorporated into the viral particle is still unresolved.Our experiments suggest either that virion RNA may be a bridgingmolecule between Gag and Pol or that it may be required, not forPol incorporation per se, but for the functioning of the Pol precursorprotein. Furthermore, this may involve a complex interaction betweenviral RNA and Gag and Pol. More sensitive assays than those usedin this study are required to address this question.

The vectors resulting in the highest gene transfer efficiencies (pMH18, pMH25, pMH28, and pMH29) expressed RNA pregenomessmaller than 3.4 kb (without the inserted U3-GFP cassette). Giventhat the HFV wild-type pregenome is 11.7 kb in length (46),these still-preliminary vectors offer ample space for the insertionof foreign DNA without exceeding the viral packaging limit. Sincethe HFV LTR of these vectors is silent, they require the use ofan internal promoter to direct expression of the gene of interestfollowing transduction. This may turn out to be an advantage whentissue-specific or regulatable promoters can be used.

	ACKNOWLEDGMENTS

We thank Rolf Flügel for the generous gift of rabbit antiserum directed against HFV RNase H and Ian Johnston for criticalreview of the manuscript.

This work was supported by grants from the BMBF, Bayerische Forschungsstiftung, and EU (BMH4-CT97-2010).

	FOOTNOTES

^* Corresponding author. Mailing address: Institut für Virologie und Immunbiologie, Universität Würzburg, Versbacher Strasse7, 97078 Würzburg, Germany. Phone: (49) 931-201-3928. Fax: (49)931-201-3934. E-mail: rethwilm{at}vim.uni-wuerzburg.de.

Present address: Molecular Hematology Branch, National Heart, Lung, and Blood Institute, National Institutes of Health, Bethesda,MD 20892-1654.

Present address: Laboratory of Neurovirology, University of California at Irvine, Irvine, CA 92697-4295.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Ausubel, F. M., R. Brent, R. E. Kingston, D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl. 1987. Current protocols in molecular biology. John Wiley & Sons, New York, N.Y.

2. Baum, C., K. Itoh, J. Meyer, C. Laker, Y. Ito, and W. Ostertag. 1997. The potent enhancer activity of the polycythemic strain of spleen focus-forming virus in hematopoietic cells is governed by a binding site for Sp1 in the upstream control region and by a unique enhancer core motif, creating an exclusive target for PEBP/CBF. J. Virol. 71:6323-6331[Abstract].

3. Baunach, G., B. Maurer, H. Hahn, M. Kranz, and A. Rethwilm. 1993. Functional analysis of human foamy virus accessory reading frames. J. Virol. 67:5411-5418[Abstract/Free Full Text].

4. Berkowitz, R., J. Fischer, and S. P. Goff. 1996. RNA packaging. Curr. Top. Microbiol. Immunol. 214:177-218[Medline].

5. Bieniasz, P. D., O. Erlwein, A. Aguzzi, A. Rethwilm, and M. O. McClure. 1997. Gene transfer using replication-defective human foamy virus vectors. Virology 235:65-72[Medline].

6. Bodem, J., M. Löchelt, I. Winkler, R. P. Flower, H. Delius, and R. M. Flügel. 1996. Characterization of the spliced pol transcript of feline foamy virus: the splice acceptor site of the pol transcript is located in gag of foamy viruses. J. Virol. 70:9024-9027[Abstract].

7. Bray, M., S. Prasad, J. W. Dubay, E. Hunter, K.-T. Jeang, D. Rekosh, and M.-L. Hammarskjold. 1994. A small element from Mason-Pfizer monkey virus genome makes human immunodeficiency virus type 1 expression and replication rev-independent. Proc. Natl. Acad. Sci. USA 91:1256-1260[Abstract/Free Full Text].

8. Charneau, P., M. Alizon, and F. Clavel. 1992. A second origin of DNA plus-strand synthesis is required for optimal human immunodeficiency virus replication. J. Virol. 66:2814-2820[Abstract/Free Full Text].

9. Charneau, P., and F. Clavel. 1991. A single-stranded gap in human immunodeficiency virus unintegrated linear DNA defined by a central copy of the polypurine tract. J. Virol. 65:2415-2421[Abstract/Free Full Text].

10. Cullen, B. R. 1991. Human immunodeficiency virus as a prototypic complex retrovirus. J. Virol. 65:1053-1056[Free Full Text].

11. Cullen, B. R. 1994. RNA-sequence-mediated gene regulation in HIV-1. Infect. Agents Dis. 3:68-76[Medline].

12. DuBridge, R. B., P. Tang, H. C. Hsia, P.-M. Leong, J. H. Miller, and M. P. Calos. 1987. Analysis of mutation in human cells by using Epstein-Barr virus shuttle system. Mol. Cell. Biol. 7:379-387[Abstract/Free Full Text].

13. Enssle, J., N. Fischer, A. Moebes, B. Mauer, U. Smola, and A. Rethwilm. 1997. Carboxy-terminal cleavage of the human foamy virus Gag precursor molecule is an essential step in the viral life cycle. J. Virol. 71:7312-7317[Abstract].

14. Enssle, J., I. Jordan, B. Mauer, and A. Rethwilm. 1996. Foamy virus reverse transcriptase is expressed independently from the gag protein. Proc. Natl. Acad. Sci. USA 93:4137-4141[Abstract/Free Full Text].

15. Erlwein, O., D. Cain, N. Fischer, A. Rethwilm, and M. O. McClure. 1997. Identification of sites that act together to direct dimerization of human foamy virus RNA in vitro. Virology 229:251-258[Medline].

16. Fischer, N., M. Heinkelein, D. Lindemann, J. Enssle, C. Baum, E. Werder, H. Zentgraf, J. G. Müller, and A. Rethwilm. 1998. Foamy virus particle formation. J. Virol. 72:1610-1615[Abstract/Free Full Text].

17. Hahn, H., G. Baunach, S. Bräutigam, A. Mergia, D. Neumann-Haefelin, M. D. Daniel, M. O. McClure, and A. Rethwilm. 1994. Reactivity of primate sera to foamy virus gag and bet proteins. J. Gen. Virol. 75:2635-2644[Abstract/Free Full Text].

18. Hirata, R. K., A. D. Miller, R. G. Andrews, and D. W. Russel. 1996. Transduction of hematopoietic cells by foamy virus vectors. Blood 88:3654-3661[Abstract/Free Full Text].

19. Huang, J., and T. J. Liang. 1993. A novel hepatitis B virus (HBV) genetic element with Rev response element-like properties that is essential for expression of HBV gene products. Mol. Cell. Biol. 13:7476-7486[Abstract/Free Full Text].

20. Huang, Z.-M., and T. S. B. Yen. 1994. Hepatitis B virus RNA element that facilitates accumulation of surface gene transcripts in the cytoplasm. J. Virol. 68:3193-3199[Abstract/Free Full Text].

21. Jordan, I., J. Enssle, E. Güttler, B. Mauer, and A. Rethwilm. 1996. Expression of human foamy virus reverse transcriptase involves a spliced pol mRNA. Virology 224:314-319[Medline].

22. Kim, V. N., K. Mitrophanous, S. M. Kingsman, and A. J. Kingsman. 1998. Minimal requirement for a lentivirus vector based on human immunodeficiency virus type 1. J. Virol. 72:811-816[Abstract/Free Full Text].

23. Kögel, D., M. Aboud, and R. M. Flügel. 1995. Molecular biological characterization of the human foamy virus reverse transcriptase and ribonuclease H domains. Virology 213:97-108[Medline].

24. Konvalinka, J., M. Löchelt, H. Zentgraf, R. M. Flügel, and H.-G. Kräusslich. 1995. Active foamy virus proteinase is essential for virus infectivity but not for formation of a Pol polyprotein. J. Virol. 69:7264-7268[Abstract].

25. Kupiec, J. J., J. Tobaly-Tapiero, M. Canivet, M. Santillana-Hayat, R. M. Flügel, J. Peries, and R. Emanoil-Ravier. 1988. Evidence for a gapped linear duplex DNA intermediate in the replicative cycle of human and simian spumaviruses. Nucleic Acids Res. 16:9557-9565[Abstract/Free Full Text].

26. Lindemann, D., M. Bock, M. Schweizer, and A. Rethwilm. 1997. Efficient pseudotyping of murine leukemia virus particles with chimeric human foamy virus envelope proteins. J. Virol. 71:4815-4820[Abstract].

27. Lindemann, D., and A. Rethwilm. 1998. Characterization of a human foamy virus 170-kilodalton Env-Bet fusion protein generated by alternative splicing. J. Virol. 72:4088-4094[Abstract/Free Full Text].

28. Linial, M. L., and A. D. Miller. 1990. Retroviral RNA packaging: sequence requirements and implications. Curr. Top. Microbiol. Immunol. 157:125-152[Medline].

29. Löchelt, M., and R. M. Flügel. 1996. The human foamy virus pol gene is expressed as a Pro-Pol polyprotein and not as a Gag-Pol fusion protein. J. Virol. 70:1033-1040[Abstract].

30. Löchelt, M., R. M. Flügel, and M. Aboud. 1994. The human foamy virus internal promoter directs the expression of the functional Bel 1 transactivator and Bet protein early after infection. J. Virol. 68:638-645[Abstract/Free Full Text].

31. Löchelt, M., W. Muranyi, and R. M. Flügel. 1993. Human foamy virus genome possesses an internal, Bel-1-dependent and functional promoter. Proc. Natl. Acad. Sci. USA 90:7317-7321[Abstract/Free Full Text].

32. Maurer, B., H. Bannert, G. Darai, and R. M. Flügel. 1988. Analysis of the primary structure of the long terminal repeat and the gag and pol genes of the human spumaretrovirus. J. Virol. 62:1590-1597[Abstract/Free Full Text].

33. Miller, A. D. 1997. Development and applications of retroviral vectors, p. 437-473. In J. M. Coffin, S. H. Hughes, and H. E. Varmus (ed.), Retroviruses. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

34. Moebes, A., J. Enssle, P. D. Bieniasz, M. Heinkelein, D. Lindemann, M. Bock, M. O. McClure, and A. Rethwilm. 1997. Human foamy virus reverse transcription that occurs late in the viral replication cycle. J. Virol. 71:7305-7311[Abstract].

35. Muranyi, W., and R. M. Flügel. 1991. Analysis of splicing patterns of human spumaretrovirus by polymerase chain reaction reveals complex RNA structures. J. Virol. 65:727-735[Abstract/Free Full Text].

36. Naldini, L., U. Blömer, P. Gallay, D. Ory, R. Mulligan, F. H. Gage, I. M. Verma, and D. Trono. 1996. In vivo gene delivery and stable transduction of nondividing cells by a lentiviral vector. Science 272:263-267[Abstract].

37. Namba, M., K. Nishitani, F. Hyodoh, F. Fukushima, and T. Kimoto. 1985. Neoplastic transformation of human diploid fibroblasts (KMST-6) by treatment with ⁶⁰Co gamma rays. Int. J. Cancer 35:275-280[Medline].

38. Nassal, M., and H. Schaller. 1993. Hepatitis B virus replication. Trends Microbiol. 1:221-228[Medline].

39. Nestler, U., M. Heinkelein, M. Lücke, J. Meixensberger, W. Scheurlen, A. Kretschmer, and A. Rethwilm. 1997. Foamy virus vectors for suicide gene therapy. Gene Ther. 4:1270-1277[Medline].

40. Netzer, K. O., A. Schliephake, B. Maurer, R. Watanabe, A. Aguzzi, and A. Rethwilm. 1993. Identification of pol-related gene products of human foamy virus. Virology 192:336-338[Medline].

41. Ogert, R. A., L. H. Lee, and K. L. Beemon. 1996. Avian retroviral RNA element promotes unspliced RNA accumulation in the cytoplasm. J. Virol. 70:3834-3843[Abstract].

42. Parolin, C., B. Taddeo, G. Palu, and J. Sodroski. 1996. Use of cis- and trans-acting regulatory sequences to improve expression of human immunodeficiency virus vectors in human lymphocytes. Virology 222:415-422[Medline].

43. Rethwilm, A. 1995. Regulation of foamy virus gene expression. Curr. Top. Microbiol. Immunol. 193:1-23[Medline].

44. Rethwilm, A. 1996. Unexpected replication pathways of foamy viruses. J. Acquir. Immune Defic. Syndr. Hum. Retrovirol. 13(Suppl. 1):S248-S253.

45. Russell, D. W., and A. D. Miller. 1996. Foamy virus vectors. J. Virol. 70:217-222[Abstract].

46. Schmidt, M., O. Herchenröder, J. Heeney, and A. Rethwilm. 1997. Long terminal repeat U3 length polymorphism of human foamy virus. Virology 230:167-178[Medline].

47. Schmidt, M., and A. Rethwilm. 1995. Replicating foamy virus-based vectors directing high level expression of foreign genes. Virology 210:167-178[Medline].

48. Soneoka, Y., P. M. Cannon, E. E. Ramsdale, J. C. Griffith, G. Romano, S. M. Kingsman, and A. J. Kingsman. 1995. A transient three-plasmid expression system for the production of high titer retroviral vectors. Nucleic Acids Res. 23:628-633[Abstract/Free Full Text].

49. Tabernero, C., A. S. Zolotukhin, J. Bear, R. Schneider, G. Karsenty, and B. K. Felber. 1997. Identification of an RNA sequence within an intracisternal-A particle element able to replace Rev-mediated posttranscriptional regulation of human immunodeficiency virus type 1. J. Virol. 71:95-101[Abstract].

50. Telenitzky, A., and S. P. Goff. 1997. Reverse transcriptase and the generation of retroviral DNA, p. 121-160. In J. M. Coffin, S. H. Hughes, and H. E. Varmus (ed.), Retroviruses. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

51. Tobaly-Tapiero, J., J. J. Kupiec, M. Santillana-Hayat, M. Canicet, J. Peries, and R. Emanoil-Ravier. 1991. Further characterization of the gapped DNA intermediates of human spumavirus: evidence for a dual initiation of plus-strand DNA synthesis. J. Gen. Virol. 72:605-608[Abstract/Free Full Text].

52. Weiss, R. A. 1996. Foamy viruses bubble on. Nature 380:201[Medline].

53. Yu, S. F., D. N. Baldwin, S. R. Gwynn, S. Yendapalli, and M. L. Linial. 1996. Human foamy virus replication: a pathway distinct from that of retroviruses and hepadnaviruses. Science 271:1579-1582[Abstract].

54. Zolotukhin, A. S., A. Valentin, G. N. Pavlakis, and B. K. Felber. 1994. Continuous propagation of RRE( $-$ ) and Rev( $-$ )RRE( $-$ ) human immunodeficiency virus type 1 molecular clones containing a cis-acting element of simian retrovirus type 1 in human peripheral blood lymphocytes. J. Virol. 68:7944-7952[Abstract/Free Full Text].

This article has been cited by other articles:

Wiktorowicz, T., Peters, K., Armbruster, N., Steinert, A. F., Rethwilm, A. (2009). Generation of an improved foamy virus vector by dissection of cis-acting sequences. J. Gen. Virol. 90: 481-487 [Abstract] [Full Text]
Roy, J., Linial, M. L. (2007). Role of the Foamy Virus Pol Cleavage Site in Viral Replication. J. Virol. 81: 4956-4962 [Abstract] [Full Text]
Trobridge, G. D., Miller, D. G., Jacobs, M. A., Allen, J. M., Kiem, H.-P., Kaul, R., Russell, D. W. (2006). Foamy virus vector integration sites in normal human cells. Proc. Natl. Acad. Sci. USA 103: 1498-1503 [Abstract] [Full Text]
Peters, K., Wiktorowicz, T., Heinkelein, M., Rethwilm, A. (2005). RNA and Protein Requirements for Incorporation of the Pol Protein into Foamy Virus Particles. J. Virol. 79: 7005-7013 [Abstract] [Full Text]
Patton, G. S., Erlwein, O., McClure, M. O. (2004). Cell-cycle dependence of foamy virus vectors. J. Gen. Virol. 85: 2925-2930 [Abstract] [Full Text]
Stenbak, C. R., Linial, M. L. (2004). Role of the C Terminus of Foamy Virus Gag in RNA Packaging and Pol Expression. J. Virol. 78: 9423-9430 [Abstract] [Full Text]
Boyer, P. L., Stenbak, C. R., Clark, P. K., Linial, M. L., Hughes, S. H. (2004). Characterization of the Polymerase and RNase H Activities of Human Foamy Virus Reverse Transcriptase. J. Virol. 78: 6112-6121 [Abstract] [Full Text]
Heinkelein, M., Rammling, M., Juretzek, T., Lindemann, D., Rethwilm, A. (2003). Retrotransposition and Cell-to-Cell Transfer of Foamy Viruses. J. Virol. 77: 11855-11858 [Abstract] [Full Text]
Heinkelein, M., Leurs, C., Rammling, M., Peters, K., Hanenberg, H., Rethwilm, A. (2002). Pregenomic RNA Is Required for Efficient Incorporation of Pol Polyprotein into Foamy Virus Capsids. J. Virol. 76: 10069-10073 [Abstract] [Full Text]
Heinkelein, M., Dressler, M., Jarmy, G., Rammling, M., Imrich, H., Thurow, J., Lindemann, D., Rethwilm, A. (2002). Improved Primate Foamy Virus Vectors and Packaging Constructs. J. Virol. 76: 3774-3783 [Abstract] [Full Text]
Wodrich, H., Bohne, J., Gumz, E., Welker, R., Krausslich, H.-G. (2001). A New RNA Element Located in the Coding Region of a Murine Endogenous Retrovirus Can Functionally Replace the Rev/Rev-Responsive Element System in Human Immunodeficiency Virus Type 1 Gag Expression. J. Virol. 75: 10670-10682 [Abstract] [Full Text]
Russell, R. A., Zeng, Y., Erlwein, O., Cullen, B. R., McClure, M. O. (2001). The R Region Found in the Human Foamy Virus Long Terminal Repeat Is Critical for both Gag and Pol Protein Expression. J. Virol. 75: 6817-6824 [Abstract] [Full Text]
Vassilopoulos, G., Trobridge, G., Josephson, N. C., Russell, D. W. (2001). Gene transfer into murine hematopoietic stem cells with helper-free foamy virus vectors. Blood 98: 604-609 [Abstract] [Full Text]
Lindemann, D., Pietschmann, T., Picard-Maureau, M., Berg, A., Heinkelein, M., Thurow, J., Knaus, P., Zentgraf, H., Rethwilm, A. (2001). A Particle-Associated Glycoprotein Signal Peptide Essential for Virus Maturation and Infectivity. J. Virol. 75: 5762-5771 [Abstract] [Full Text]
Cain, D., Erlwein, O., Grigg, A., Russell, R. A., McClure, M. O. (2001). Palindromic Sequence Plays a Critical Role in Human Foamy Virus Dimerization. J. Virol. 75: 3731-3739 [Abstract] [Full Text]
Meiering, C. D., Maxine L. Linial, (2001). Historical Perspective of Foamy Virus Epidemiology and Infection. Clin. Microbiol. Rev. 14: 165-176 [Abstract] [Full Text]
Imrich, H., Heinkelein, M., Herchenröder, O., Rethwilm, A. (2000). Primate foamy virus Pol proteins are imported into the nucleus. J. Gen. Virol. 81: 2941-2947 [Abstract] [Full Text]
Hu, W.-S., Pathak, V. K. (2000). Design of Retroviral Vectors and Helper Cells for Gene Therapy. Pharmacol. Rev. 52: 493-512 [Abstract] [Full Text]
Jewell, N. A., Mansky, L. M. (2000). In the beginning: genome recognition, RNA encapsidation and the initiation of complex retrovirus assembly. J. Gen. Virol. 81: 1889-1899 [Full Text]
Pietschmann, T., Zentgraf, H., Rethwilm, A., Lindemann, D. (2000). An Evolutionarily Conserved Positively Charged Amino Acid in the Putative Membrane-Spanning Domain of the Foamy Virus Envelope Protein Controls Fusion Activity. J. Virol. 74: 4474-4482 [Abstract] [Full Text]
Heinkelein, M., Thurow, J., Dressler, M., Imrich, H., Neumann-Haefelin, D., McClure, M. O., Rethwilm, A. (2000). Complex Effects of Deletions in the 5' Untranslated Region of Primate Foamy Virus on Viral Gene Expression and RNA Packaging. J. Virol. 74: 3141-3148 [Abstract] [Full Text]
Callahan, M. E., Switzer, W. M., Matthews, A. L., Roberts, B. D., Heneine, W., Folks, T. M., Sandstrom, P. A. (1999). Persistent Zoonotic Infection of a Human with Simian Foamy Virus in the Absence of an Intact orf-2 Accessory Gene. J. Virol. 73: 9619-9624 [Abstract] [Full Text]
Baldwin, D. N., Linial, M. L. (1999). Proteolytic Activity, the Carboxy Terminus of Gag, and the Primer Binding Site Are Not Required for Pol Incorporation into Foamy Virus Particles. J. Virol. 73: 6387-6393 [Abstract] [Full Text]
Enssle, J, Moebes, A, Heinkelein, M, Panhuysen, M, Mauer, B, Schweizer, M, Neumann-Haefelin, D, Rethwilm, A (1999). An active foamy virus integrase is required for virus replication. J. Gen. Virol. 80: 1445-1452 [Abstract]
Wu, M., Mergia, A. (1999). Packaging Cell Lines for Simian Foamy Virus Type 1�Vectors. J. Virol. 73: 4498-4501 [Abstract] [Full Text]
Pietschmann, T., Heinkelein, M., Heldmann, M., Zentgraf, H., Rethwilm, A., Lindemann, D. (1999). Foamy Virus Capsids Require the Cognate Envelope Protein for Particle Export. J. Virol. 73: 2613-2621 [Abstract] [Full Text]
Linial, M. L. (1999). Foamy Viruses Are Unconventional Retroviruses. J. Virol. 73: 1747-1755 [Full Text]

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Heinkelein, M.
	Articles by Rethwilm, A.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Heinkelein, M.
	Articles by Rethwilm, A.

1.	Ausubel, F. M., R. Brent, R. E. Kingston, D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl. 1987. Current protocols in molecular biology. John Wiley & Sons, New York, N.Y.
2.	Baum, C., K. Itoh, J. Meyer, C. Laker, Y. Ito, and W. Ostertag. 1997. The potent enhancer activity of the polycythemic strain of spleen focus-forming virus in hematopoietic cells is governed by a binding site for Sp1 in the upstream control region and by a unique enhancer core motif, creating an exclusive target for PEBP/CBF. J. Virol. 71:6323-6331[Abstract].
3.	Baunach, G., B. Maurer, H. Hahn, M. Kranz, and A. Rethwilm. 1993. Functional analysis of human foamy virus accessory reading frames. J. Virol. 67:5411-5418[Abstract/Free Full Text].
4.	Berkowitz, R., J. Fischer, and S. P. Goff. 1996. RNA packaging. Curr. Top. Microbiol. Immunol. 214:177-218[Medline].
5.	Bieniasz, P. D., O. Erlwein, A. Aguzzi, A. Rethwilm, and M. O. McClure. 1997. Gene transfer using replication-defective human foamy virus vectors. Virology 235:65-72[Medline].
6.	Bodem, J., M. Löchelt, I. Winkler, R. P. Flower, H. Delius, and R. M. Flügel. 1996. Characterization of the spliced pol transcript of feline foamy virus: the splice acceptor site of the pol transcript is located in gag of foamy viruses. J. Virol. 70:9024-9027[Abstract].
7.	Bray, M., S. Prasad, J. W. Dubay, E. Hunter, K.-T. Jeang, D. Rekosh, and M.-L. Hammarskjold. 1994. A small element from Mason-Pfizer monkey virus genome makes human immunodeficiency virus type 1 expression and replication rev-independent. Proc. Natl. Acad. Sci. USA 91:1256-1260[Abstract/Free Full Text].
8.	Charneau, P., M. Alizon, and F. Clavel. 1992. A second origin of DNA plus-strand synthesis is required for optimal human immunodeficiency virus replication. J. Virol. 66:2814-2820[Abstract/Free Full Text].
9.	Charneau, P., and F. Clavel. 1991. A single-stranded gap in human immunodeficiency virus unintegrated linear DNA defined by a central copy of the polypurine tract. J. Virol. 65:2415-2421[Abstract/Free Full Text].
10.	Cullen, B. R. 1991. Human immunodeficiency virus as a prototypic complex retrovirus. J. Virol. 65:1053-1056[Free Full Text].
11.	Cullen, B. R. 1994. RNA-sequence-mediated gene regulation in HIV-1. Infect. Agents Dis. 3:68-76[Medline].
12.	DuBridge, R. B., P. Tang, H. C. Hsia, P.-M. Leong, J. H. Miller, and M. P. Calos. 1987. Analysis of mutation in human cells by using Epstein-Barr virus shuttle system. Mol. Cell. Biol. 7:379-387[Abstract/Free Full Text].
13.	Enssle, J., N. Fischer, A. Moebes, B. Mauer, U. Smola, and A. Rethwilm. 1997. Carboxy-terminal cleavage of the human foamy virus Gag precursor molecule is an essential step in the viral life cycle. J. Virol. 71:7312-7317[Abstract].
14.	Enssle, J., I. Jordan, B. Mauer, and A. Rethwilm. 1996. Foamy virus reverse transcriptase is expressed independently from the gag protein. Proc. Natl. Acad. Sci. USA 93:4137-4141[Abstract/Free Full Text].
15.	Erlwein, O., D. Cain, N. Fischer, A. Rethwilm, and M. O. McClure. 1997. Identification of sites that act together to direct dimerization of human foamy virus RNA in vitro. Virology 229:251-258[Medline].
16.	Fischer, N., M. Heinkelein, D. Lindemann, J. Enssle, C. Baum, E. Werder, H. Zentgraf, J. G. Müller, and A. Rethwilm. 1998. Foamy virus particle formation. J. Virol. 72:1610-1615[Abstract/Free Full Text].
17.	Hahn, H., G. Baunach, S. Bräutigam, A. Mergia, D. Neumann-Haefelin, M. D. Daniel, M. O. McClure, and A. Rethwilm. 1994. Reactivity of primate sera to foamy virus gag and bet proteins. J. Gen. Virol. 75:2635-2644[Abstract/Free Full Text].
18.	Hirata, R. K., A. D. Miller, R. G. Andrews, and D. W. Russel. 1996. Transduction of hematopoietic cells by foamy virus vectors. Blood 88:3654-3661[Abstract/Free Full Text].
19.	Huang, J., and T. J. Liang. 1993. A novel hepatitis B virus (HBV) genetic element with Rev response element-like properties that is essential for expression of HBV gene products. Mol. Cell. Biol. 13:7476-7486[Abstract/Free Full Text].
20.	Huang, Z.-M., and T. S. B. Yen. 1994. Hepatitis B virus RNA element that facilitates accumulation of surface gene transcripts in the cytoplasm. J. Virol. 68:3193-3199[Abstract/Free Full Text].
21.	Jordan, I., J. Enssle, E. Güttler, B. Mauer, and A. Rethwilm. 1996. Expression of human foamy virus reverse transcriptase involves a spliced pol mRNA. Virology 224:314-319[Medline].
22.	Kim, V. N., K. Mitrophanous, S. M. Kingsman, and A. J. Kingsman. 1998. Minimal requirement for a lentivirus vector based on human immunodeficiency virus type 1. J. Virol. 72:811-816[Abstract/Free Full Text].
23.	Kögel, D., M. Aboud, and R. M. Flügel. 1995. Molecular biological characterization of the human foamy virus reverse transcriptase and ribonuclease H domains. Virology 213:97-108[Medline].
24.	Konvalinka, J., M. Löchelt, H. Zentgraf, R. M. Flügel, and H.-G. Kräusslich. 1995. Active foamy virus proteinase is essential for virus infectivity but not for formation of a Pol polyprotein. J. Virol. 69:7264-7268[Abstract].
25.	Kupiec, J. J., J. Tobaly-Tapiero, M. Canivet, M. Santillana-Hayat, R. M. Flügel, J. Peries, and R. Emanoil-Ravier. 1988. Evidence for a gapped linear duplex DNA intermediate in the replicative cycle of human and simian spumaviruses. Nucleic Acids Res. 16:9557-9565[Abstract/Free Full Text].
26.	Lindemann, D., M. Bock, M. Schweizer, and A. Rethwilm. 1997. Efficient pseudotyping of murine leukemia virus particles with chimeric human foamy virus envelope proteins. J. Virol. 71:4815-4820[Abstract].
27.	Lindemann, D., and A. Rethwilm. 1998. Characterization of a human foamy virus 170-kilodalton Env-Bet fusion protein generated by alternative splicing. J. Virol. 72:4088-4094[Abstract/Free Full Text].
28.	Linial, M. L., and A. D. Miller. 1990. Retroviral RNA packaging: sequence requirements and implications. Curr. Top. Microbiol. Immunol. 157:125-152[Medline].
29.	Löchelt, M., and R. M. Flügel. 1996. The human foamy virus pol gene is expressed as a Pro-Pol polyprotein and not as a Gag-Pol fusion protein. J. Virol. 70:1033-1040[Abstract].
30.	Löchelt, M., R. M. Flügel, and M. Aboud. 1994. The human foamy virus internal promoter directs the expression of the functional Bel 1 transactivator and Bet protein early after infection. J. Virol. 68:638-645[Abstract/Free Full Text].
31.	Löchelt, M., W. Muranyi, and R. M. Flügel. 1993. Human foamy virus genome possesses an internal, Bel-1-dependent and functional promoter. Proc. Natl. Acad. Sci. USA 90:7317-7321[Abstract/Free Full Text].
32.	Maurer, B., H. Bannert, G. Darai, and R. M. Flügel. 1988. Analysis of the primary structure of the long terminal repeat and the gag and pol genes of the human spumaretrovirus. J. Virol. 62:1590-1597[Abstract/Free Full Text].
33.	Miller, A. D. 1997. Development and applications of retroviral vectors, p. 437-473. In J. M. Coffin, S. H. Hughes, and H. E. Varmus (ed.), Retroviruses. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
34.	Moebes, A., J. Enssle, P. D. Bieniasz, M. Heinkelein, D. Lindemann, M. Bock, M. O. McClure, and A. Rethwilm. 1997. Human foamy virus reverse transcription that occurs late in the viral replication cycle. J. Virol. 71:7305-7311[Abstract].
35.	Muranyi, W., and R. M. Flügel. 1991. Analysis of splicing patterns of human spumaretrovirus by polymerase chain reaction reveals complex RNA structures. J. Virol. 65:727-735[Abstract/Free Full Text].
36.	Naldini, L., U. Blömer, P. Gallay, D. Ory, R. Mulligan, F. H. Gage, I. M. Verma, and D. Trono. 1996. In vivo gene delivery and stable transduction of nondividing cells by a lentiviral vector. Science 272:263-267[Abstract].
37.	Namba, M., K. Nishitani, F. Hyodoh, F. Fukushima, and T. Kimoto. 1985. Neoplastic transformation of human diploid fibroblasts (KMST-6) by treatment with ⁶⁰Co gamma rays. Int. J. Cancer 35:275-280[Medline].
38.	Nassal, M., and H. Schaller. 1993. Hepatitis B virus replication. Trends Microbiol. 1:221-228[Medline].
39.	Nestler, U., M. Heinkelein, M. Lücke, J. Meixensberger, W. Scheurlen, A. Kretschmer, and A. Rethwilm. 1997. Foamy virus vectors for suicide gene therapy. Gene Ther. 4:1270-1277[Medline].
40.	Netzer, K. O., A. Schliephake, B. Maurer, R. Watanabe, A. Aguzzi, and A. Rethwilm. 1993. Identification of pol-related gene products of human foamy virus. Virology 192:336-338[Medline].
41.	Ogert, R. A., L. H. Lee, and K. L. Beemon. 1996. Avian retroviral RNA element promotes unspliced RNA accumulation in the cytoplasm. J. Virol. 70:3834-3843[Abstract].
42.	Parolin, C., B. Taddeo, G. Palu, and J. Sodroski. 1996. Use of cis- and trans-acting regulatory sequences to improve expression of human immunodeficiency virus vectors in human lymphocytes. Virology 222:415-422[Medline].
43.	Rethwilm, A. 1995. Regulation of foamy virus gene expression. Curr. Top. Microbiol. Immunol. 193:1-23[Medline].
44.	Rethwilm, A. 1996. Unexpected replication pathways of foamy viruses. J. Acquir. Immune Defic. Syndr. Hum. Retrovirol. 13(Suppl. 1):S248-S253.
45.	Russell, D. W., and A. D. Miller. 1996. Foamy virus vectors. J. Virol. 70:217-222[Abstract].
46.	Schmidt, M., O. Herchenröder, J. Heeney, and A. Rethwilm. 1997. Long terminal repeat U3 length polymorphism of human foamy virus. Virology 230:167-178[Medline].
47.	Schmidt, M., and A. Rethwilm. 1995. Replicating foamy virus-based vectors directing high level expression of foreign genes. Virology 210:167-178[Medline].
48.	Soneoka, Y., P. M. Cannon, E. E. Ramsdale, J. C. Griffith, G. Romano, S. M. Kingsman, and A. J. Kingsman. 1995. A transient three-plasmid expression system for the production of high titer retroviral vectors. Nucleic Acids Res. 23:628-633[Abstract/Free Full Text].
49.	Tabernero, C., A. S. Zolotukhin, J. Bear, R. Schneider, G. Karsenty, and B. K. Felber. 1997. Identification of an RNA sequence within an intracisternal-A particle element able to replace Rev-mediated posttranscriptional regulation of human immunodeficiency virus type 1. J. Virol. 71:95-101[Abstract].
50.	Telenitzky, A., and S. P. Goff. 1997. Reverse transcriptase and the generation of retroviral DNA, p. 121-160. In J. M. Coffin, S. H. Hughes, and H. E. Varmus (ed.), Retroviruses. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
51.	Tobaly-Tapiero, J., J. J. Kupiec, M. Santillana-Hayat, M. Canicet, J. Peries, and R. Emanoil-Ravier. 1991. Further characterization of the gapped DNA intermediates of human spumavirus: evidence for a dual initiation of plus-strand DNA synthesis. J. Gen. Virol. 72:605-608[Abstract/Free Full Text].
52.	Weiss, R. A. 1996. Foamy viruses bubble on. Nature 380:201[Medline].
53.	Yu, S. F., D. N. Baldwin, S. R. Gwynn, S. Yendapalli, and M. L. Linial. 1996. Human foamy virus replication: a pathway distinct from that of retroviruses and hepadnaviruses. Science 271:1579-1582[Abstract].
54.	Zolotukhin, A. S., A. Valentin, G. N. Pavlakis, and B. K. Felber. 1994. Continuous propagation of RRE( $-$ ) and Rev( $-$ )RRE( $-$ ) human immunodeficiency virus type 1 molecular clones containing a cis-acting element of simian retrovirus type 1 in human peripheral blood lymphocytes. J. Virol. 68:7944-7952[Abstract/Free Full Text].