Essential and Dispensable Virus-Encoded Replication Elements Revealed by Efforts To Develop Hypoviruses as Gene Expression Vectors

doi:10.1128/JVI.74.16.7568-7577.2000

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Journal of Virology, August 2000, p. 7568-7577, Vol. 74, No. 16
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Essential and Dispensable Virus-Encoded Replication Elements Revealed by Efforts To Develop Hypoviruses as Gene Expression Vectors

Nobuhiro Suzuki, Lynn M. Geletka, and Donald L. Nuss^*

Center for Agricultural Biotechnology, University of Maryland Biotechnology Institute, University of Maryland, College Park, Maryland 20742

Received 18 February 2000/Accepted 15 May 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

We have investigated whether hypoviruses, viral agents responsible for virulence attenuation (hypovirulence) of the chestnutblight fungus Cryphonectria parasitica, could serve as gene expressionvectors. The infectious cDNA clone of the prototypic hypovirusCHV1-EP713 was modified to generate 20 different vector candidates.Although transient expression was achieved for a subset of vectorsthat contained the green fluorescent protein gene from Aequoreavictoria, long-term expression (past day 8) was not observed forany vector construct. Analysis of viral RNAs recovered from transfectedfungal colonies revealed that the foreign genes were readily deletedfrom the replicating virus, although small portions of foreignsequences were retained by some vectors after months of replication.However, the results of vector viability and progeny characterizationprovided unexpected new insights into essential and dispensableelements of hypovirus replication. The N-terminal portion (codons1 to 24) of the 5'-proximal open reading frame (ORF), ORF A, wasfound to be required for virus replication, while the remaining598 codons of this ORF were completely dispensable. Substantialalterations were tolerated in the pentanucleotide UAAUG that containsthe ORF A termination codon and the overlapping putative initiationcodon of the second of the two hypovirus ORFs, ORF B. Replicationcompetence was maintained following either a frameshift mutationthat caused a two-codon extension of ORF A or a modification thatproduced a single-ORF genomic organization. These results arediscussed in terms of determinants of hypovirus replication, thepotential utility of hypoviruses as gene expression vectors, andpossible mechanisms by which hypoviruses recognize and deleteforeignsequences.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Fungi representing all major taxons have been reported to harbor viruses and related virus-like double-stranded (ds) RNA geneticelements (1, 17, 29). Similar to viruses of animals andplants, mycoviruses have potential utility for elucidating hostfunctions and manipulating host phenotype (see reference 41).Evidence of progress in developing this potential is providedby recent studies with members of the family Hypoviridae thatcause an attenuation of virulence (hypovirulence) and alter dependentdevelopmental process, e.g., asexual and sexual sporulation, oftheir host, the chestnut blight fungus Cryphonectria parasitica.For example, efforts to understand the molecular basis for hypovirulencerevealed a crucial role for G-protein signal transduction in awide range of vital fungal physiological processes that includedpathogenesis (4, 9, 15, 16, 23, 24, 40). In relatedstudies, Chen and Nuss (5) used full-length infectious cDNAclones of genomic RNAs derived from severe and mild hypovirusstrains to differentially influence the fungal phenotype and theinteraction between C. parasitica and its planthost.

The availability of a reverse genetics system for hypoviruses (3, 7) also provides opportunities to examine the consequencesof specific mutations of the viral genome and explore the potentialfor development of hypoviruses as fungal gene expression vectors.In this regard, deletion of 88% of the coding region for the papain-likeprotease p29 from the infectious cDNA clone of the prototypichypovirus CHV1-EP713 demonstrated that this viral protein wasdispensable for viral replication and revealed the extent of itscontribution to virus-mediated reduction in fungal pigmentationand asexual sporulation (10). This observation also impliedthat one could replace the deleted portion of the viral genomewith heterologous sequences, thus generating a hypovirus RNA cytoplasmicallyreplicating gene expression vector system. Additionally, sinceCHV1-EP713 RNA is not encapsidated, constraints on the size ofheterologous inserts, as are often encountered with many othervirus vector systems, were expected to beminimal.

Several potential applications can be envisioned for a cytoplasmically transmissible RNA-based hypovirus gene expression vector.The incorporation of a visual reporter gene could provide a convenientmeans for monitoring hypovirus movement from cell to cell duringanastomosis or long distance through a fungal colony or even afungal population. It might be possible to enhance ecologicalfitness of hypovirulent C. parasitica strains by expressing nucleargenes that are normally downregulated by hypovirus infection,e.g., viral expression of the mating pheromone gene Mat-2 (43)might relieve virus-mediated female infertility. Hypovirus hostrange might be extended to a number of pathogenic fungi by incorporatingC. parasitica host range determinants, once identified, withinrecombinant viral constructs. It is also conceivable that thephenotypic changes caused by hypovirus infection could be furthermodified by the incorporation of foreign genes that might alterspecific host metabolic or signaling pathways. Hypoviruses mayeven be exploited to deliver secretable gene products from infectedfungal cells to difficult to transform chestnut plant cells, e.g.,to enhance plant defenseresponses.

This study describes extensive efforts to modify the infectious CHV1-EP713 cDNA clone to express foreign genes. Although stableexpression constructs were not obtained, transient expressionof introduced foreign genes was confirmed. Moreover, significantnew insights into essential and dispensable virus-encoded elementsof replication were revealed by analysis of vector constructsand resulting progenyviruses.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Source of heterologous gene inserts. Four genes of nonhypovirus origin were selected for insertion into the full-length infectious cDNA clone of prototypic hypovirusCHV1-EP713. These included two reporter genes, the enhanced greenfluorescent protein gene (EGFP) from Aequorea victoria (30)and the Escherichia coli hygromycin B phosphotransferase gene(HYG) (11). The coding regions of these reporters were amplifiedfrom plasmids pEGFP (Clontech Laboratories, Inc., Palo Alto, Calif.)and pCPXHY1 (10), respectively, by PCR using primers that alsointroduced specific terminal restriction sites and cloned intopPCR-Script SK(+) (Stratagene, La Jolla, Calif.). Two nonreportergenes that included the foot-and-mouth disease virus 2A proteasegene (2A) (32) and the Mat-2 mating type pheromone gene (PH)of C. parasitica (43) were generated as synthetic oligonucleotides.The codon usage for the 2A gene, which encodes the 17-residuepeptide NFDLLKLAGDVESNPGP, was modified to match that of C. parasiticanuclear genes (AAA-TTT-GAC-TTG-CTC-AAG-TTG-GCC-GGT-GAC-GTC-GAG-TCC-AAC-CCG-GGT-CCC).

Construction of virus expression vectors. Modification of and gene insertion into the full-length hypovirus cDNA was facilitated by the development of a mutation/modificationcassette system. The foundation plasmid pTRN was generated byPCR-mediated replacement (21) of the original multiple cloningsite of the commercially available plasmid pTZ19R (U.S. Biochemicals,Cleveland, Ohio) with oligonucleotides specifying a multiple cloningsite (NotI, SacII, AscI, XbaI, NheI, KpnI, RsrII, and SpeI) thatcontained combinations of the unique restriction sites found inthe plasmid harboring the full-length CHV1-EP713 viral cDNA, pLDST.Construction of the pTRN-based cassette used in this study, pTNR4,involved insertion of the 5'-terminal 3.7-kb XbaI-NheI CHV1-EP713cDNA fragment derived from pLDST (7), followed by modificationsof the multiple cloning site for applications not described inthis study that included destruction of the XbaI site and introductionof an additional NotI site following the SpeI site. Followingappropriate alterations of, or insertion of foreign gene sequencesinto, the viral cDNA fragment in pTRN4, modified full-length CHV1-EP713viral cDNAs were reconstituted by insertion of the 3'-terminal8.9-kb NheI-SpeI CHV1-EP713 cDNA fragment, also derived from pLDST.The resulting plasmids were linearized at the SpeI site and usedas a template for in vitro synthesis of viral vector transcriptsfrom the T7 polymerase promoter present in the pLDST-derived XbaI-NheIfragment. All synthetic viral-vector transcripts contained thewild-type CHV1-EP713 5'- and 3'-noncoding terminal sequences withthe exception of the group II vectors, which contained a two-nucleotidechange immediately upstream of the open reading frame (ORF) Ainitiator codon from taATGg to ccATGg. Transfection of C. parasiticaspheroplasts and recovery of infected fungal colonies was performedas described by Suzuki et al. (38). The integrity of each vectorconstruct was verified by sequence analysis at insert junctionsand modification sites. Detailed descriptions of cloning stepsare available from the authors uponrequest.

GFP visualization. Sterile glass coverslips (22 by 22 mm) were placed on cellophane overlaying potato dextrose agar (PDA) and hyphae of transfectedfungal colonies were allowed to grow as a thin layer between thecellophane and coverslip from a small agar inoculation plug placedat the edge of the coverslip. Coverslips with attached hyphaewere transferred to a glass slide, mounted with distilled water,and observed with a Leica fluorescence stereomicroscope modelMZ FLIII (Leica Microscopy Systems, Heerbrugg, Switzerland). Emissionof green fluorescence was observed with a GFP plant fluorescentfilter set (GFP3; Leica Microscopy Systems) and photographed witha Spot 1.3.0 charge-coupled device digital camera (DiagnosticInstruments, Inc., Sterling Heights, Mich.). A C. parasitica transformant(strain EGFP-CP) in which EGFP gene expression was driven by theC. parasitica glyceraldehyde-3-phosphate dehydrogenase (GPD) genepromoter (Pgpd) was used as a positivecontrol.

dsRNA isolation and ClampR analysis. dsRNA was isolated from fungal colonies transfected with transcripts of each of the vector constructs and subjected to agarosegel electrophoretic analysis as described by Suzuki et al. (38).A single-tube, reverse transcriptase PCR protocol, ClampR (25),was performed on isolated dsRNA preparations as described previously(38). The 25-µl reaction mixture contained 10 mM Tris-HCl (pH8.3), 50 mM KCl, 1.5 mM MgCl₂, appropriate primer sets (10 pmoleach) annealed to dsRNA (100 ng) after a previous denaturationand annealing step, 1 U of avian myeloblastosis virus reversetranscriptase (Life Technologies, Gaithersburg, Md.), and 1 Uof AmpliTaq DNA polymerase (Perkin-Elmer, Branchburg, N.J.). Thereaction mixtures were incubated at 42°C for 30 min, followedby 30 PCR cycles of 94°C for 1 min, 45°C for 1.5 min, and 72°Cfor 2 min. Amplified PCR products were subcloned into pPCRScriptand subjected to sequenceanalysis.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Strategies for design of hypovirus expression vectors. As indicated in Fig. 1, hypovirus CHV1-EP713 contains two large ORFs designated ORF A and ORF B (34). ORF A encodes twopolypeptides, p29 and p40, that are released from polyproteinp69 by an autocatalytic event mediated by the papain-like proteasedomain within p29 (6). Expression of ORF B also involves anautoproteolytic event in which p48, also a papain-like protease,is released from the N-terminal portion of the encoded polyprotein.The junction between ORFs A and B consists of the sequence 5'-UAAUG-3',where the UAA portion serves as the termination codon of ORF Aand the AUG portion is the 5'-proximal translation initiationcodon of ORF B.

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FIG. 1. Schematic representation of vector constructs. The genetic organization of the infectious cDNA clone of wild-type hypovirus CHV1-EP713 in plasmid pLDST (7) is shown at the top. The coding strand is 12,712 nucleotides in length, excluding the poly(A) tract, and contains two ORFs, A and B (34). ORF A encodes two polypeptides, p29 and p40, that are released from polyprotein p69 by an autocatalytic event mediated by the papain-like protease domain within p29 (6). Expression of ORF B also involves an autoproteolytic event in which p48, also a papain-like protease, is released from the N-terminal portion of the encoded polyprotein. The junction between ORFs A and B consists of the sequence 5'-UAAUG-3' (map positions 2362 to 2366) where the UAA portion serves as the termination codon of ORF A and the AUG portion is the 5'-proximal translation initiation codon of ORF B. Diagrams of 20 CHV1-EP713-based gene expression vector candidates, organized within four groups (I to IV) on the basis of four design strategies, are shown below the wild-type CHV1-EP713 cDNA. Four foreign genes (indicated by shaded boxes) were incorporated into the vectors: the enhanced A. victoria green fluorescent protein gene (EGFP), the E. coli hygromycin B phosphotransferase gene (HYG), the foot-and-mouth disease virus 2A protease gene (2A), and the Mat-2 mating type pheromone gene (PH) of C. parasitica. The dashed lines shown in vector constructs NtNcoIEGFPp29 $Delta$ 25-243 and Ct2APHp29 $Delta$ 25-243 indicate the deletion of the BamHI fragment (bases 562 to 1218) of the p29 coding domain leading to the fusion of p29 proline residue 24 with p29 leucine residue 244. The cloning operations used to construct individual expression vector candidates are described in detail in Methods and Materials and in Results.

Four basic strategies were explored to construct a total of 20 hypovirus expression vector candidates. The observation that88% of the p29 papain-like protease coding domain of ORF A wasdispensable for viral replication (10) provided the basis forthe first group of vectors, targeting the p29 coding region asa candidate for insertion of foreign gene sequences. Two foreigngenes previously demonstrated to express efficiently in transformedC. parasitica were utilized for these initial studies. The E.coli hygromycin phosphotransferase gene (HYG) is the basic selectionmarker used in a large number of C. parasitica transformationvectors (2, 8, 10, 16). The enhanced mutant form ofthe GFP (EGFP) gene from Aequorea victoria (30) is expressedefficiently under the control of the C. parasitica GPD promoterafter ectopic chromosomal integration (see Fig. 3).

For group I vectors, the reporter genes were inserted in frame into previously characterized p29 deletion mutant infectiouscDNAs. The first of these mutants, originally described by Cravenet al. (10) and designated $Delta$ p29 (referred to here as p29 $Delta$ 25-243),contained a deletion of the BamHI fragment spanning map positions562 to 1218, thereby fusing codon Pro24 with codon Leu244 (seereference 34 for the CHV1-EP713 sequence map coordinates). Thesecond mutant, designated p29 $Delta$ 25-109, contained a smaller deletionextending from map position 562 to 822, fusing Pro24 with Glu110(38). Since the active p29 protease domain (amino acid [aa]residues 135 to 248) and cleavage site (Gly248-Gly249) remainedintact in the latter mutant (6), the p29-reporter fusion proteinencoded in vectors p29 $Delta$ 25-109EGFP and p29 $Delta$ 25-109HYG was predictedto be cleaved from the polyprotein at the normal p29 cleavagesite. In contrast, the p29-reporter fusion protein produced bythe $Delta$ p29-based constructs p29 $Delta$ 25-243EGFP and p29 $Delta$ 25-243HYG, whichlacked the p29 protease domain, was predicted to be further fusedto p40. Two additional group I vectors (p29 $Delta$ 25-109EGFP2A and p29 $Delta$ 25-243EGFP2A)were engineered to incorporate the foot-and-mouth disease virus2A protease (2A) (32) with the intention of liberating an N-terminalp29-reporter fusionprotein.

Vectors in group II contained modifications or gene insertions at the precise N terminus (designated Nt in vector constructs)of ORF A. This was accomplished by first using PCR mutagenesisto modify the ORF A translation initiation codon from TAATGG (mappositions 494 to 499) to CCATGG, thus creating an NcoI restrictionsite in the foundation vector construct NtNcoI. Other constructsin this group were then generated by insertions of reporter genesinto the NcoI site. Vector NtNcoIEGFP was predicted to produceEGFP fused to p29, while deletion of the p29 BamHI fragment (mappositions 562 to 1218) in vector NtNcoIEGFPp29 $Delta$ 25-243 was predictedto produce EGFP flanked by p29 aa residues 1 to 24 at the N terminusand by p29 aa residues 244 to 248 at the C terminus all fusedto p40. The 2A protease domain was introduced into the 3'-flankingregion of the EGFP in vector NtNcoIEGFP2A $Delta$ p29 with the intentionof liberating the EGFP-2A fusion protein from p29. An NcoI-modifiedtranslation initiation codon was also engineered at the N terminusof a vector in which the entire p29 coding domain was deletedand a 2A gene was fused to the p40 coding domain. The NcoI sitein this vector, NtNcoI2A $Delta$ p29, was then used to introduce the EGFPsequence to form vector NtNcoIEGFP2A $Delta$ p29.

Vectors in group III contained gene inserts in the 3'-terminal portion of the p40 coding domain near or adjacent to the pentanucleotideUAAUG that separates ORF A from ORF B, i.e., in the C terminus(designated Ct in vector constructs) of the ORF A-encoded polyprotein.Vectors Ct2A and Ct2APH contained, respectively, the 2A domainand the 2A domain fused to the C. parasitica Mat-2 pheromone gene(PH) inserted immediately upstream of the pentanucleotide. Thelatter construct was predicted to produce an unfused pheromoneprotein. Vector Ct2APHp29 $Delta$ 25-243 was similar to Ct2APH but wasin the background of the original $Delta$ p29 $Delta$ 25-243 recombinant virus.In vector Ctp40[2A], the 3'-terminal sequence of the p40 codingdomain (map positions 2,318 to 2,361) was duplicated to form anintermediate construct that contained an SbfI site for subsequentinsertion of the EGFP and HYG genes to produce vectors Ctp40[2AEGFP]and Ctp40[2AHYG], respectively. These last two vectors were predictedto produce reporter proteins fused at the C terminus with p40amino acid residues 361 to374.

The final group of vectors, group IV, consisted of two constructs in which the EGFP gene was inserted in place of most ofORF A (the p69 polyprotein coding domain). Vectors $Delta$ p69bEGFP and $Delta$ p69bEGFP2A contained the EGFP and EGFP-C-terminal 2A fusion genesinserted between the BamHI site at position 562 and a new BamHIsite engineered precisely at the pentanucleotide in such a waythat the stop codon was destroyed (UAAUG to CCAUG) while retainingthe AUG initiator codon in frame with the upstream region. Thatis, these vectors have a single large ORF that is predicted toproduce the EGFP fused at the N terminus with p29 aa 1 to 24 andat the C terminus with p48 of ORF B or unfused at the C terminusdue to 2A protease activity,respectively.

Replication competence of expression vector constructs. The replication competence of each vector construct was examined by transfecting spheroplasts prepared from virus-free C.parasitica EP155 and scoring for the recovery of viral dsRNA fromregenerated mycelial cultures (results are summarized in Table1). Although the HYG gene is efficiently expressed in C. parasiticafrom integrated plasmid vectors (7, 8), neither of the groupI vectors that contained HYG as the foreign gene (p29 $Delta$ 25-243HYGand p29 $Delta$ 25-109HYG) were found to be replication competent (Fig.2, lanes 2 and 5). In contrast, transcripts derived from all EGFP-containingvectors were able to readily establish productive infections (Fig.2, lanes 1, 3, 4, and 6).

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TABLE 1. Properties of vector constructs

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FIG. 2. Agarose gel electrophoretic analysis of viral dsRNAs recovered from transfected C. parasitica colonies 3 weeks posttransfection. Transfected fungal colonies were transferred from regeneration media to PDA plates 7 days posttransfection, cultured for 1 week, transferred to liquid growth media for an additional week of culturing, harvested, and processed to recover dsRNA according to the protocol of Hillman et al. (19). Partially purified viral dsRNA preparations were treated with S1 nuclease (5 U) to digest single-stranded RNA (3) and examined by agarose (0.7%) gel electrophoresis. Full-length viral dsRNAs are the slowest-migrating bands in each lane. The faster-migrating species observed in lanes 7, 15, 17, and 21 correspond to internally deleted defective viral dsRNAs previously identified in hypovirus-infected isolates (2, 35). Lanes marked with an M contain 200 ng of 1-kb DNA ladder (Life Technologies) as relative size markers, with arrows indicating the positions of the 5.1-, 2.0-, and 1.0-kb bands. Lane 1, p29 $Delta$ 25-243EGFP; lane 2, p29 $Delta$ 25-243HYG; lane 3, p29 $Delta$ 25-243EGFP2A; lane 4, p29 $Delta$ 25-109EGFP; lane 5, p29 $Delta$ 25-109HYG; lane 6, p29 $Delta$ 25-109EGFP2A; lane 7, NtNcoI; lane 8, NtNcoIEGFP; lane 9, NtNcoIEGFPp29 $Delta$ 25-243; lane 10, NtNcoIEGFP2A; lane 11, NtNcoI2A $Delta$ p29; lane 12, NtNcoIEGFP2A $Delta$ p29; lane 13, Ct2A; lane 14, Ct2APH; lane 15, Ct2APHp29 $Delta$ 25-243; lane 16, Ctp40[2A]; lane 17, Ctp40[2AEGFP]; lane 18, Ctp40[2AHYG]; lane 19, $Delta$ p69bEGFP; lane 20, $Delta$ p69bEGFP2A; lane 21, wild-type virus cDNA pLDST.

The group II foundation vector, NtNcoI, readily established an infection upon transfection (Fig. 2, lane 7) and stably retainedthe altered sequence (TAATGG to CCATGG) adjacent to the ORF Ainitiation codon (data not shown), indicating that the mutationrequired to introduce the NcoI site had no gross negative effecton virus replication. Interestingly, the introduction of foreigngene sequences into this NcoI site resulted in loss of replicationcompetency (Fig. 2, lanes 8 to 12). Moreover, transcripts derivedfrom vectors NtNcoI2A $Delta$ p29 and NtNcoIEGFP2A $Delta$ p29, both of whichlacked any of the p29 coding domain, also failed to initiate productiveinfections. The potential role for the 5' proximal portion ofthe p29 coding domain in CHV1-EP713 replication will be addressedin a subsequentsection.

Insertion of foreign sequences adjacent to the UAAUG pentanucleotide separating ORFs A and B in the group III vectors hadmixed consequences for virus replication. Vector Ct2A, in whichthe 2A protease gene was inserted immediately upstream of theUAAUG pentanucleotide, was replication incompetent (Fig. 2, lane13). However, insertion of the C. parasitica Mat-2 pheromone gene(43) preceded by the 2A gene into the same position, eitherin the context of the full-length CHV1-EP713 sequence (Ct2APH)or the $Delta$ p29 background (Ct2APHp29 $Delta$ 25-243), was tolerated and yieldedinfectious transcripts (Fig. 2, lanes 14 and 15). Similarly, transcriptsderived from vectors Ctp40[2A] and Ctp40[2AEGFP], in which the3'-terminal sequence of the p40 coding domain (nucleotides 2,318to 2,361) was duplicated to form an SbfI site for insertion offoreign genes, were infectious (Fig. 2, lanes 16 and 17). Finally,as was observed for group I vectors containing the HYG gene, vectorCtp40[2AHYG] was not replicationcompetent.

Group IV expression vectors were constructed with the anticipation that they might be replication incompetent. Although itwas clearly established that 88% of the p29 coding domain couldbe deleted without abolishing CHV1-EP713 replication (10), therewas no evidence to suggest that the p40 coding domain would alsobe dispensable. Additionally, the pentanucleotide separating ORFsA and B was mutated to remove the ORF A translation stop codon,creating an in-frame single ORF genome organization. Surprisingly,transcripts derived from both vectors, $Delta$ p69bEGFP and $Delta$ p69bEGFP2A,readily initiated infections (Fig. 2, lanes 19 and 20). Thus,p40, like most of p29, is dispensable for CHV1-EP713 replication.The role of the UAAUG pentanucleotide will be considered in moredetail in a latersection.

EGFP expression in fungal cells infected with expression vector constructs. Replication-competent EGFP constructs p29 $Delta$ 25-243EGFP, p29 $Delta$ 25-243EGFP2A, p29 $Delta$ 25-109EGFP, p29 $Delta$ 25-109EGFP2A, Ctp40[2AEGFP], $Delta$ p69bEGFP,and $Delta$ p69bEGFP2A were examined for green fluorescence on day 6posttransfection (results are summarized in Table 1). The highestlevel of fluorescence was observed for mycelia infected with vectorCtp40[2AEGFP] (Fig. 3). However, the level of fluorescence wasconsiderably lower than that exhibited by mycelia stably transformedwith the EGFP gene under the control of the C. parasitica GPDpromoter, pEGFP-CP (Fig. 3). Fluorescence was also detected atvery low levels in mycelia transfected with vectors p29 $Delta$ 25-243EGFP2A,p29 $Delta$ 25-109EGFP, and p29 $Delta$ 25-109EGFP2A (Fig. 3). Importantly, greenfluorescence was lost for each of the EGFP-positive transfectantswithin several weeks of culturing following transfer of a portionof the mature colony to new PDA plates. No fluorescence was observedat any time posttransfection for mycelia infected with transcriptsderived from vectors p29 $Delta$ 25-243EGFP, $Delta$ p69bEGFP, and $Delta$ p69bEGFP2Aor for colonies transfected with wild-type CHV1-713 transcripts(pLDST) (Fig. 3).

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FIG. 3. Micrographs of EGFP-expressing C. parasitica strains. Agar plugs containing transfected fungal mycelia were transferred from regeneration plates to cellophane-overlaid PDA plates on day 4 posttransfection and placed at the edge of a glass coverslip. The mycelia were allowed to grow between the coverslip and the cellophane for 2 days and then transferred to a glass slide for observation (see Materials and Methods). Mycelia attached to the coverglass were observed under a fluorescent microscope at ×100 magnification. Vector constructs used for transfection are indicated at the bottom of each panel and include p29 $Delta$ 25-243EGFP, p29 $Delta$ 25-243EGFP2A, p29 $Delta$ 25-109EGFP, p29 $Delta$ 25-109EGFP2A, Ctp40[2AEGFP], $Delta$ p69bEGFP, and $Delta$ p69bEGFP2A. A colony transfected with synthetic transcripts derived from wild-type virus cDNA, pLDST, served as a negative control, while a transformant in which the EGFP gene (pEGFP-CP) is expressed from the C. parasitica GPD gene promoter (Pgpd) was used as a positive control.

Stability of expression vectors after transfection. The transient nature of GFP fluorescence expression suggested either a significant reduction in vector replication or in thestability of the foreign gene within the replicating vector RNA.Since dsRNA was found to be present in infected mycelia even monthsafter transfection (data not shown), a single-tube reverse transcriptionPCR analysis, ClampR (25), was performed on dsRNAs recoveredfrom infected mycelium at 3 and 9 weeks posttransfection in aneffort to examine foreign gene stability. As indicated in Fig.4, the foreign gene sequences were partially or completely deletedfrom all group I vector RNAs by 3 weeks posttransfection. In contrast,foreign genes were retained in three of the four infectious groupIII vectors, Ct2A40, Ct2APH, and Ct2APHp29 $Delta$ 25-243, at week 3.Similar results were observed for the two infectious group IVvectors. However, foreign genes appeared to be deleted from replicatingvector RNAs in all groups by week 9.

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FIG. 4. ClampR analysis of dsRNA recovered from fungal colonies transfected with candidate expression vectors. For each replication-competent vector (shown at the top) ClampR was performed on the full-length cDNA clone (lane 1 in each set) and on dsRNA isolated 3 weeks (lane 2 of each set) and 9 weeks (lane 3 of each set) posttransfection. Transfected hyphae were transferred from regeneration plates to PDA plates at 7 days posttransfection. After incubation for 7 days, the cultures were transferred to liquid medium for an additional week of culturing and then harvested for recovery of dsRNA (3-week samples) or transferred weekly to new PDA plates for 6 weeks (9-week samples) before transfer to liquid medium. Primer sets were chosen to amplify fragments spanning the foreign gene insert as follows: NS7 and BR54 (nucleotide map positions 476 to 493 and 1386 to 1402, respectively) for vectors p29 $Delta$ 25-243EGFP, p29 $Delta$ 25-243EGFP2A, p29 $Delta$ 25-109EGFP, and p29 $Delta$ 25-109EGFP2A; NS21 and NS22 (nucleotide map positions 2240 to 2259 and 2382 to 2401, respectively) for Ctp40[2A], Ct2APH, Ct2APHp29 $Delta$ 25-243, and Ctp40[2AEGFP]; and BR16 and NS22 (nucleotide map positions 364 to 382 and 2382 to 2401, respectively) for $Delta$ p69bEGFP and $Delta$ p69bEGFP2A. Amplified fragments were electrophoresed in a 2.0% agarose gel in 1× Tris-borate-EDTA. M refers to the 100-bp DNA ladder size markers (Life Technologies). Arrows indicate the migration positions of the 2.1-, 0.6-, and 0.1-kbp size standards.

To gain further insight into the deletion process, ClampR fragments generated from 9-week-old colonies (Fig. 4) were clonedand sequenced. With the exception of p29 $Delta$ 25-109EGFP2A, a singledeletion breakpoint was observed for five individual subclonedClampR fragments generated from the progeny RNA of each vector,suggesting that a population consisting of a major deletion specieswas stabilized by 9 weeks posttransfection. As indicated in Fig.5, progeny of all replication-competent vector constructs in groupI retained the 5'-proximal p29 coding region upstream of the BamHIsite at position 562 used for foreign gene insertion and a shortsequence encoding from 1 (p29 $Delta$ 25-109EGFP2A) to 19 (p29 $Delta$ 25-243EGFP2A)aa residues of the foreign EGFP sequence. The position of the3'-terminal deletion breakpoints varied considerably for the differentvectors. For example, the deletion progeny generated from vectorp29 $Delta$ 25-243EGFP retained 10 codons from the C terminus of the EGFPprotein, while the 3'-deletion breakpoints for progeny derivedfrom vectors p29 $Delta$ 25-243EGFP2A, p29 $Delta$ 25-109EGFP, and p29 $Delta$ 25-109EGFP2Aextended to different regions of the p29 or p40 coding domains.In the case of progeny of vector p29 $Delta$ 25-109EGFP2A, three of thefive ClampR clones retained a portion of the FMDV 2A proteasesequence, whereas the other two did not. Thus, although entireforeign genes were unstable, portions of foreign sequences wereretained in some hypovirus vector progeny for long periods ofculturing.

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FIG. 5. Illustration of deletion breakpoints in progeny RNA recovered from mycelia transfected with hypovirus vector constructs. DNA fragments amplified by ClampR for genomic dsRNA templates recovered from infected mycelia at 9 weeks posttransfection (Fig. 4) were cloned into the SrfI site of pPCRScript (Stratagene Systems), and five independent clones were subsequently sequenced. The breakpoints for each deletion progeny are indicated by arrowheads. Nucleotide and amino acid sequences are shown below the schematic representations for some of the more informative deletion breakpoints. Map positions are indicated at each end of the sequence information. Arrows show the amino acid sequence for viral proteins p29, p40, and p48. The symbols =, $-$ , and -//- are used to indicate sequences not shown due to space limitations, the same sequence as found in the original parental vector shown in the top row, and deleted sequences, respectively.

Foreign gene sequences were completely deleted from each of the group III replication-competent vector genomes, as diagrammedin Fig. 5. Vectors Ctp40[2A] and Ctp40[2AEGFP] reverted preciselyto their parental virus, CHV1-EP713, suggesting a homologous recombinationmediated by the duplicated p40 coding sequence of the vector constructs.The deletion events that led to removal of foreign sequences fromvector Ct2APH included the additional deletion of a viral U residueimmediately 5' of the ORF A translation stop codon, causing aframeshift and a resulting two-codon extension of ORF A relativeto that present in CHV1-EP713 (Fig. 5 and 6) (AUUUUAAUGUAUAAto AUUUAAUGUAUAA, the pentanucleotide within bases 2358to 2371 is shown in boldface). A similar frameshifted deletionproduct was generated for Ct2APHp29 $Delta$ 25-243. However, the eventsleading to the formation of this progeny must have involved deletionof two viral U residues since the G residue present at the thirdposition of the C-terminal Met codon of the PH gene was retained(Fig. 5 and 6).

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FIG. 6. Sequences in the pentanucleotide region of vector construct progeny. ClampR fragments were obtained with primer set NS21 and NS22 (map positions 2240 to 2259 and 2382 to 2401, respectively) for progeny dsRNAs of vectors Ct2APH, Ct2APHp29 $Delta$ 25-243, and $Delta$ p69bEGFP2A 9 weeks after transfection and sequenced. Nucleotide sequences and deduced amino acid sequences for the ORF A-ORF B junction of CHV1-EP713 are shown for reference. Asterisks indicate termination codons of ORF A, and the underlined sequence refers to the pentanucleotide. Nonviral nucleotides are shown in lowercase letters.

Different deletion patterns were observed for the two group IV vectors that were distinguished by the presence of a singleORF rather than the prototypical two-ORF organization. Vector $Delta$ p69bEGFP underwent complete deletion of the EGFP gene to revertto its progenitor, $Delta$ p69b, indicating that the progeny of thisvector were able to replicate with the UAAUG pentanucleotide modifiedso as to fuse p29 codons 1 to 24 with the N terminus of ORF Bin a single-ORF configuration. In contrast, the single-ORF vector $Delta$ p69bEGFP2A was converted to a deletion product containing twoORFs with a junction similar to that seen for the deletion productsof group II vectors Ct2APH and Ct2APHp29 $Delta$ 25-243, i.e., the equivalentof deleting a U residue just prior to the ORF A stop codon causinga two-codon extension into the p48 coding region and reconstructionof the ORF B codingdomain.

The recovery of multiple independent viable deletion progeny that contained a two-codon extension of the 5'-proximal ORF wassurprising (Fig. 6), given the prediction (34) that the UAAUGpentanucleotide junction separating ORFs A and B is likely toregulate the termination of ORF A translation and reinitiationof ribosomes for subsequent translation of ORF B. To reduce thepossibility that the viability of these deletion mutants is dependenton compensatory mutations, a mutated virus cDNA, designated FS1,was constructed in which the first residue of the pentanucleotide,U 2362, was deleted within the context of the infectious viruscDNA. FS1 transcript derived from the reconstituted virus cDNAwas able to replicate and to induce the same set of phenotypicchanges caused by wild-type CHV1-EP713 (data not shown). The sequenceintegrity of the mutated region was confirmed by ClampR and sequenceanalyses, indicating that the mutant virus is viable and stable.We conclude that the single frameshift deletion of U 2362 andthe resulting two codon extension of ORF A is tolerated withoutobservable changes in virus replication or virus-mediated alterationsof fungalphenotype.

Deletion mutation of the 5' portion of the p29 coding domain abolishes replication competency. With the exception of the foundation vector NtNcoI, all group II vectors were replication incompetent. Comparison of thesevectors with those that could initiate an infection revealed oneobvious distinguishing feature: all replication-competent vectorscontained at least 66 nucleotides (map positions 496 to 561, Met1through Pro24) of the 5' portion of the p29 coding domain. Thepossibility that the 5'-proximal portion of the p29 coding domainplays a role in virus replication was investigated by furtherdeletion from the Pro24 codon toward the N terminus of the p29coding region within the context of the replication-competent,foreign-gene-free p29 $Delta$ 25-243 and $Delta$ p69b mutants. In one set ofdeletion mutants, p29 codon Val12 was fused with Asp242 of p29( $Delta$ p29-based mutant NS36a) or with Met1 of p48 ( $Delta$ p69b-based mutantNS36b). In the second set of mutants, the deletion was extendedto p29 translation initiation codon Met1, completely eliminatingthe p29 N-terminal coding domain. Both sets of deletions resultedin loss of replication competency when tested repeatedly undertransfection conditions in which transcripts from the originalp29 $Delta$ 25-243 and $Delta$ p69b vectors consistently initiated productiveinfections.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Animal viruses have been modified for delivery of foreign genes of potential therapeutic value, while plant viruses are beingharnessed for large scale in planta production of protein products.The availability of infectious full-length hypovirus cDNA clones(3, 5, 7), the only viral reverse genetics system currentlyavailable for the kingdom Fungi, provides the platform for manipulatinga fungal virus for analogous applications. A potential for engineeringhypoviruses as gene expression vectors was suggested by the observationthat 88% of the p29 coding domain was dispensable for virus replication(10) and by the absence of a virus-encoded coat protein (34)that might place packaging constraints on insert size. Moreover,transcripts generated from chimeric cDNA clones derived from asevere and a mild strain were recently shown to be fully infectiousand genetically stable (5). However, the performance of the20 independent hypovirus vector candidates described in this reporthas failed to meet initialexpectations.

It was possible to demonstrate that the CHV1-EP713 infectious transcript could maintain replication competence while accommodatingthe insertion of foreign genes at several different sites withinORF A. Moreover, transient expression of the inserted foreigngene was achieved for several of the vector candidates. However,long-term expression was compromised by the ability of the viralreplication machinery to recognize and delete all or most of theforeign sequences within a few weeks posttransfection. In thisregard, it is noteworthy that some vector progeny did retain asmany as 60 nucleotides of foreign sequence for an extended timeperiod. Efforts to find a correlation between sequence instabilityand differences in codon usage between viral ORFs and foreigngene sequences were not successful. The ill-defined and generallyunpredictable nature of foreign gene instability in RNA virusvectors has been reviewed in detail by Scholthof et al. (33).As noted by these authors, several RNA virus vectors have foundconsiderable utility in spite of the problem of long-term foreigngeneinstability.

In related studies, functionally conserved coding domains derived from hypovirus CHV1-Euro7 that differed as much as 13% atthe nucleotide level from that of the corresponding CHV1-EP713domain were stably maintained in CHV1-EP713/CHV1-Euro7 chimericviruses (reference 5 and data not shown). Now that hypovirusesbelonging to three distinct species have been sequenced in full(5, 20, 34, 36), it will be of considerable interestto determine whether genes derived from more distantly relatedhypoviruses will be stably retained in CHV1-EP713 chimeric virusesor recognized as foreign anddeleted.

Although only transient expression of foreign genes was achieved in this study, the possibility that hypoviruses can be developedas vectors for stable gene expression is not excluded. Insertionswere restricted in this study to ORF A. It is quite conceivablethat regions within ORF B are more tolerant of gene insertion.An alternative vector strategy was also suggested by the observationthat the 5'-terminal portion of the p29 coding domain was requiredfor vector RNA replication. Shapira et al. (35) previously characterizedinternally deleted dsRNAs recovered from CHV1-EP713 infected coloniesthat retained only the terminal noncoding regions: ~150 bp fromthe terminus corresponding to the 5' end of the coding strandand ~450 bp from the other terminus. Although these small dsRNAsreplicated in the presence of the full-length viral RNA, effortsto use these terminal sequences to construct a helper virus-dependentreplicon as a gene expression vector were unsuccessful (B. Chenand D. L. Nuss, unpublished results). The absence of a N-terminalp29 coding domain in those constructs may have been responsiblefor the failure to observe expression of inserted genes, a possibilitycurrently underinvestigation.

The fact that defective RNAs lacking the N-terminal portion of p29 can replicate in the presence of the full-length hypovirusRNA suggests that this element does not play a direct role inthe replication process. Could the N-terminal portion of p29 playa role in facilitating translation of the CHV1-EP713 coding domains?In this context, it is intriguing to consider that the long CHV1-EP7135'-noncoding region contains seven mini-ORFs and has been shownto inhibit in vitro translation (31), properties often associatedwith internal ribosome entry sites (IRES) (28, 42). This raisesthe possibility that the 5'-terminal noncoding region and theN-terminal portion of p29 might function coordinately to facilitatean IRES-guided translation mechanism. Certainly, precedents existfor the involvement of coding domain elements in facilitatingboth viral RNA amplification (e.g., references 18 and 27)and cap-dependent or cap-independent translation (14, 26,39). The role of the N-terminal portion of p29 in hypovirusreplication and gene expression clearly warrants further detailedinvestigation.

Analyses of viable vectors and recovered progeny also provided unexpected revelations concerning the UAAUG pentanucleotidethat separates ORFs A and B. As indicated by Hillman et al. (20),this pentanucleotide is conserved in the prototype members oftwo of the three recognized species within the genus Hypovirus,CHV1-EP713 and CHV2-NB58, that share only 60% overall nucleotidesequence identity. These authors further reported the presenceof an A/U string immediately preceding the pentanucleotide forboth hypovirus species: the sequences 5'-AAAAUAAAAUUUUAAUG-3'for CHV1-EP713 (pentanucleotide in boldface) and 5'-AAAAUUUUAAUUAAUUAAUG-3'for CHV2-NB58. Interestingly, insertion of the 2A domain immediatelypreceding the pentanucleotide resulted in a replication-incompetentvector, Ct2A, even though this domain was tolerated at severalother sites within ORF A. In contrast, insertion of the C. parasiticapheromone gene at this site resulted in viable vectors, Ct2APHand Ct2APHp29 $Delta$ 25-243. The potential secondary structure for thetwo sequences 5'-UCCAACCCGGGUUAAUG-3' for the 2A gene and5'-UGCGUUGUCAUGUAAUG-3' for the pheromone gene, may providea clue for the observed differences; the 2A sequence has the potentialfor forming a 10-residue hairpin structure that involves the firstU of the pentanucleotide, U2362.

Nucleotides immediately upstream of position 2362 are also notable in a second interesting observation regarding the pentanucleotide.Viral uracil residues were deleted in the progeny RNA recoveredfrom mycelia transfected with two independent vector constructs(vectors Ct2APH and Ct2APHp29 $Delta$ 25-243), resulting in a two-codonextension of ORF A. Additionally, a similar dicistronic genomestructure was generated in the progeny of virus $Delta$ p69bEGFP2A thatwas engineered to have a monocistronic genome. Based on evidencefrom mutational analysis of an identical pentanucleotide in thedicistronic influenza virus RNA7 (22), it was suggested thatthe hypovirus pentanucleotide facilitated a ribosome terminationand reinitiation mechanism that might, in turn, regulate the relativetranslation of the two ORFs (34). This would be functionallyanalogous to the $-$ 1 ribosomal frameshift in the yeast killer virusthat regulates the relative production of the Gag and Gag-Polfusion proteins (12) or the $-$ 1 termination-reinitiation proposedfor the production of coat protein and RDRP protein by the Helminthsporiumvictoriae 190S totivirus (37). Even a twofold change in theefficiency of frameshifting from the normal 1.9% can have a significanteffect on killer virus RNA replication (13). Thus, it was surprisingthat specific alteration of the pentanucleotide in mutant FS1that extended ORF A by two codons did not cause any detectablechange in viral RNA accumulation or infected host symptomexpression.

An even more surprising result regarding the UAAUG pentanucleotide was the stable replication of the progeny derived fromexpression vector $Delta$ p69bEGFP2A, in which the two-ORF genetic configurationwas abolished by a modification of the ORF A termination codonthat fused Pro24 of p29 directly in frame with Met1 of p48. Thisresult suggests that the UAAUG pentanucleotide is altogether dispensablefor virus replication. In this regard, Smart et al. (36) recentlyreported a single-ORF configuration for hypovirus GH2, a proposedmember of a third hypovirus species very distantly related toCHV1-EP713.

An additional unexpected revelation from this study was that p40 is not required for CHV1-EP713 replication. Although no functionhas previously been assigned to p40, computer-assisted analysisof the deduced p40 amino acid sequence indicated a very high pKavalue, suggesting a possible role as a basic RNA binding protein.However, the ability to retain replication competence in the absenceof any portion of the p40 coding domain (vectors $Delta$ p69bEGFP and $Delta$ p69bEGFP2A) eliminates this virus-encoded protein as playingan essential role in either viral transcription orreplication.

The apparent dispensability of the pentanucleotide, most of p29 and all of p40 for virus replication, raises the questionof why they are retained in the wild-type virus. The most obviousexplanation is that these elements in some way contribute to viralfitness under natural field conditions. p29 has been shown tocontribute to virus-mediated reductions in host pigment production,asexual sporulation, and laccase production (8, 10), andthe symptom determinant has been mapped to a region extendingfrom Phe25 through Gln73 (38). However, it is unclear just howthese traits benefit virus reproduction. In this regard, preliminarystudies suggest that portions of ORF A do influence the efficiencyof virus transmission to asexual progeny (N. Suzuki et al., unpublishedresults). Fortunately, the C. parasitica-hypovirus experimentalsystem lends itself to detailed studies of molecular host-pathogeninteractions. The vector progeny recovered in this study providethe basis for future mutagenesis studies to determine the contributionof p40 to virus-mediated alteration of fungal phenotype, includinghypovirulence, and the role of the pentanucleotide in regulatingthe relative expression of viral gene products and the role ofthe N terminus of p29 in translation initiation. It is anticipatedthat continued efforts to develop hypovirus expression vectorsby gene insertions in ORF B or the use of defective RNA platformswill lead to additional revelations about hypovirus molecularbiology.

	ACKNOWLEDGMENTS

This work was supported in part by National Institutes of Health grant GM55981 to D.L.N.

We are grateful to Todd Parsley, Angus Dawe, and Gert Segers for helpfuldiscussions.

	FOOTNOTES

^* Corresponding author. Mailing address: Center for Agricultural Biotechnology, University of Maryland Biotechnology Institute,Plant Sciences Bldg., Rm. 5115, College Park, MD 20742-4450. Phone:(301) 405-0334. Fax: (301) 314-9075. E-mail: nuss{at}umbi.umd.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Buck, K. W. 1986. Fungal virology $---$ an overview, p. 2-84. In K. W. Buck (ed.), Fungal virology. CRC Press, Boca Raton, Fla.
2.	Chen, B., G. H. Choi, and D. L. Nuss. 1993. Mitotic stability and nuclear inheritance of integrated viral cDNA in engineered hypovirulent strains of the chestnut blight fungus. EMBO J. 12:2991-2998[Medline].
3.	Chen, B., G. H. Choi, and D. L. Nuss. 1994. Attenuation of fungal virulence by synthetic infectious hypovirus transcripts. Science 264:1762-1764[Abstract/Free Full Text].
4.	Chen, B., S. Gao, G. H. Choi, and D. L. Nuss. 1996. Extensive alteration of fungal gene transcript accumulation and elevation of G-protein-regulated cAMP levels by a virulence-attenuating hypovirus. Proc. Natl. Acad. Sci. USA 93:7996-8000[Abstract/Free Full Text].
5.	Chen, B., and D. L. Nuss. 1999. Infectious cDNA clone of hypovirus CHV1-Euro7: a comparative virology approach to investigate virus-mediated hypovirulence of the chestnut blight fungus Cryphonectria parasitica. J. Virol. 73:985-992[Abstract/Free Full Text].
6.	Choi, G. H., R. Shapira, and D. L. Nuss. 1991. Cotranslational autoproteolysis involved in gene expression from a double-stranded RNA genetic element associated with hypovirulence of the chestnut blight fungus. Proc. Natl. Acad. Sci. USA 88:1167-1171[Abstract/Free Full Text].
7.	Choi, G. H., and D. L. Nuss. 1992. Hypovirulence of chestnut blight fungus conferred by an infectious viral cDNA. Science 257:800-803[Abstract/Free Full Text].
8.	Choi, G. H., and D. L. Nuss. 1992. A viral gene confers hypovirulence-associated traits to the chestnut blight fungus. EMBO J. 11:473-477[Medline].
9.	Choi, G. H., B. Chen, and D. L. Nuss. 1995. Virus-mediated or transgenic suppression of a G protein $alpha$ subunit and attenuation of fungal virulence. Proc. Natl. Acad. Sci. USA 92:305-309[Abstract/Free Full Text].
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