Pseudorabies virus vaccine
The present invention is concerned with a pseudorabies virus (PrV) mutant, a recombinant DNA molecule comprising PrV DNA, a host cell transformed with said recombinant DNA molecule, a cell culture infected with the mutant, a vaccine derived from the PrV mutant as well as a method to distinguish whether an animal has been vaccinated or is infected with naturally-occurring Pseudorabies virus.
Pseudorabies virus is a member of the herpes virus group. It is the causative agent of Aujeszky's disease which induces serious economic losses especially among piglets in swine breeding farms and leads to latent infection in older animals. The predominant visible feature of PrV infection is intense pruritus generally resulting in host mutilation of the involved area. Violent excitement, fits and paralysis, all symptoms of encephalomyelitis, precede death which usually occurs within a few days following onset of clinical signs.
The research and development trend among traditional vaccine manufacturers has generally emphasized research leading to vaccines that are based upon virus subunits rather than live viruses. This departure from modified live virus vaccines is partly due to the recognized safety of such subunit vaccines because their unlikelihood to contain infectious live viruses. Another reason for developing a subunit vaccine has been to allow for the development of a diagnostic test that would accompany the vaccine and would differentiate vaccinated from infected animals.
Subunit vaccines have also their limitations. They contain a limited number of viral antigens compared to those produced by live viruses. This paucity of antigens produces a weak immune response of short duration in the vaccinated animal. This, however, is partly advantageous because it allows to discern vaccinated animals from infected animals. Vaccination only will stimulate production of antibodies to the limited spectrum of antigens present in the vaccine. By sampling the serum of the animal, it is possible to show that the vaccinated animal has antibodies only to the antigens contained in the vaccine while an animal infected with the wild-type virus would have antibodies against a wider range of antigens.
Live modified virus vaccines have the advantage that they comprise more antigens and that thus a stronger immune response can be obtained. The chances are that uncontrolled mutations occur during passaging, resulting in populations of virus particles which are heterogeneous in virulence and immunizing properties. More important it is well known that such traditional attenuated viruses can revert to virulence resulting in disease of the vaccinated animals and the possible spread of the pathogen to other animals.
The approach of deleting a gene to attenuate a virus coupled with a diagnostic tool for that gene, provides a vaccine that can be differentiated from any of the currently used PrV vaccines and from naturally- occurring PrV.
Herpes viruses of the PrV type contain in their core a double-stranded DNA molecule with a molecular weight of about 90 x 106 daltons (D) , separated by inverted repeats into a long and a short unique region UL and US, respectively (Sheldric, P. and N. Berthelot, 1975. Inverted repetitions in the chromosome of herpes simplex virus. Cold Spring Harbor Symp. Quant. Biol. 39:667-678).
Sequencing, mapping of mRNA, and analyses of mutants have shown that the herpes virus genome encodes a minimum of 75 open reading frames (ORFs), of which 69 map in the UL and US sequences (McGeoch, D.J. , M.A. Dalrymple, A.J. Davison, A. Dolan, M.C. Frame, D. McNab, L.J. Perry, J.E. Scott and P. Taylor, 1988. The complete DNA sequence of the long unique region in the genome of herpes simplex virus type l. J. Gen. Virol. 69:1531-1574; Wagner, E.K., 1984. Individual HSV transcripts. Characterization of specific genes, p. 45-104. In: B. Roizman (ed.), The Herpesviruses, vol. 3, Plenum Press, New York.).
The genome of the herpes viruses is commonly referred to in terms of restriction enzyme fragments. For pseudorabies virus recently the sequence of the Bam HI fragments 11 and 16 has been published (Klupp, B.G. and T.C. Mettenleiter, 1991. Sequence and expression of the glycoprotein gH gene of Pseudorabies Virus. Virology 182:732-741).
Recently a US patent has been issued (US 5,037,742) which discloses the use of PrV as a vector for foreign genes. The gill-region is specifically used for this purpose. In US 5 047 237 a virus vaccine has been disclosed which contains a mutation in the gpX-sequence. In EP 0 141 458 gl~ mutants have been described.
The object of the invention is to provide a PrV mutant which can be used for the preparation of a modified live vaccine, which can be given without the risk of inoculating animals with inadequately attenuated pathogenic micro-organisms. In addition, also the risk that attenuated pathogens may revert to a virulent state resulting in disease of the inoculated animals and the possible spread of pathogen to other animals, can be reduced by use of a mutant virus.
Furthermore, the PrV mutant offers the possibility of a multivalent vaccine without the risk of adverse mutual interference of different antigenic components.
An other object of the present invention is to provide a PrV vaccine virus which is distinguishable from any field strain. It is important to discriminate between animals vaccinated with a PrV vaccine and those infected with a wild type virus so as to be able to take appropriate measures to reduce spreading of a virulent virus.
Both objects are met by providing a PrV mutant comprising a mutation obtained by recombinant DNA techniques in a part of the PrV genome which spans the region comprising the DNA sequences of the open reading frame (ORF) encoding the polypeptide as shown in SEQ ID NO:2.
The term recombinant DNA techniques used herein refers to in vitro techniques to produce DNA molecules containing novel combinations of (coding) sequences or altered sequences, and the insertion of these into vectors that can be used for their incorporation into host organisms or cells in which they are capable of continued propagation of the modified sequences.
The term "polypeptide" refers to a molecular chain of amino acids, does not refer to a specific length of the product and if required can be modified in vivo or in vitro, for example by glycosylation, amidation, carboxylation or phosphorylation; thu& inter alia peptides, oligopeptides and proteins are included within the definition of polypeptide.
A mutation is understood to be a change of the genetic information by recombinant DNA techniques in the above-mentioned region with respect to the genetic information present in this region of the genome of naturally occurring PrV.
The mutation is in particular, a nucleic acid substitution, deletion, insertion or inversion, or a combination thereof resulting in a PrV mutant which fails to produce the antigenic or functional polypeptide, shown in SEQ ID NO:2, or in a PrV mutant which contains an inserted heterologous nucleic sequence. The mutation may result also in the production of a polypeptide deviating from the above- mentioned polypeptide of SEQ ID NO:2 displaying altered antigenic or functional properties.
Most preferably the mutation is a deletion and/or an insertion and/or one or more nucleotide substitutions.
The preferred substitution herein is a combination of substitutions such that the codon encoding His at position 37 is changed to a codon encoding Arg, the codon encoding Glu at position 355 is changed to a codon encoding Asp, and the codon encoding Val at position 375 is changed to a codon encoding Ala.
Also a mutation can occur in the control elements for the ORF localized in the intergenic sequence, which may result in a failure of the expression of the polypeptide.
The deletion in the genome of the PrV mutant may comprise a whole ORF.
PrV mutants according to the invention can also be obtained by inserting a nucleic acid sequence into the genome thereby preventing or altering the expression of the polypeptide shown in SEQ ID NO:2.
The BamHI 4 fragment of the PrV virus comprises the nucleic acid sequence spanning 9382 nucleotide base pairs (GenBank Data Library Accession No. L00676). This sequence comprises inter alia two open reading frames: a. ORF-1 localized between basepair no. 760 and basepair no. 2333, which in opposite direction codes for the polypeptide shown in SEQ ID NO:2, having 525 amino acids; b. ORF-2 localized between basepair no. 2440 and basepair no. 2921, which in this direction codes for a polypeptide, having 161 amino acids.
The (insertion-)region referred to in the present invention (SEQ ID NO:l) has not been identified previously within the PRV genome. Surprisingly, it has been found that a mutation is allowable in this region without disrupting essential functions of the PrV.
In particular it has been found herein that nucleotide substitution A110 to Gilθ' A1065 ^° c1065 and T11 4 to c ll24 resulting in a change of the respective codons results in the expression of a polypeptide having functional characteristics deviating from those of the polypeptide shown in SEQ ID NO:2 such that the PrV mutant thus obtained is less virulent than the parent virus.
The above-mentioned nucleotide substitution results in 3 amino acid exchanges in the deduced ORF gene product: His at position 37 is substituted by Arg, Glu at position 355 is substituted by Asp and Val at position 375 is substituted by Ala.
Unexpectedly, it has been found that the introduction of a mutation into the region defined above in particular the substitution outlined above significantly reduces the virulence of the live PrV mutant without affecting the protective properties of the PrV mutant. This finding has offered the possibility to obtain an attenuated PrV mutant, e.g. by introducing a deletion or insertion or substitution into the region defined above.
In a preferred embodiment of the invention a PrV mutant has a mutation in the part of the PrV genome having the nucleic acid sequence as shown in SEQ ID NO:l.
It will be understood that for the DNA sequence coding for the polypeptide of SEQ ID Nϋ:2 natural variations can exist between individual Pseudorabies viruses. These variations may result in a change in one or more nucleotides in the ORF which, however, still will encode functional polypeptides.
Moreover, the possibility exists to use genetic engineering technology to bring about above-mentioned variations resulting in a DNA sequence related to the sequence shown in SEQ ID NO:l which still encodes functional polypeptide. It is clear that PrV mutants comprising a mutation in such a corresponding nucleic acid sequence are also included within the scope of the invention.
Although the PrV mutant according to the invention is derived from the strain Ka, any PrV strain can be used to prepare the PrV mutant, such as NIA-3, RICE, 75V19 or Phylaxia.
PrV mutants can be provided with an insertion in the DNA sequence defined herein.
In one aspect of the invention such an insert is merely meant to prohibit or alter the expression of the polypeptide shown in SEQ ID NO:2. This can for instance be done by insertion of a number of basepairs which is not divisable by three, thereby shifting the reading frame, or by inserting a sequence containing a stop codon, or by inserting a non-sense sequence.
Alternatively, the insert comprises a heterologous nucleic acid sequence encoding a polypeptide.
The prerequisite for such a useful recombinant PrV mutant is that the heterologous nucleic acid sequence is incorporated in a permissive position or region of the genomic PrV sequence, i.e. a position or region which can be used for the incorporation of a heterologous sequence without disrupting essential functions of PrV such as those necessary for infection or replication. Such a region is called an insertion-region.
The term "recombinant PrV mutant" as used herein denotes infective virus which has been genetically modified by incorporation into the virus genome of a heterologous nucleic acid sequence, i.e. DNA which comprises a nucleic acid sequence not identical to the nucleic acid sequence of a gene naturally present in PrV.
On infection of a cell by the recombinant PrV mutant, it may express the heterologous gene in the form of a heterologous polypeptide.
The insertion-region referred to in the present invention has not been identified previously within the PrV genome. Surprisingly, it has been found that a mutation such as the incorporation of heterologous DNA is allowable in this region without disrupting essential functions of the PrV.
In summary, the insertion-region essentially defined above characterizes the localization of a region within the PrV genome which can be used to introduce a deletion or to incorporate a heterologous nucleic acid sequence, if desired after deleting DNA sequences from this region, or can be used to introduce other mutations in said region.
The heterologous nucleic acid sequence to be incorporated into the PRV genome according to the present invention can be derived from any source, e.g. viral, prokaryotic, eukaryotic or synthetic. Said heterologous nucleic acid sequence can be derived from a pathogen, preferably a porcine pathogen, which after insertion into the PrV genome can be applied to induce immunity against disease.
Preferably nucleic acid sequences encoding a polypeptide of parvovirus, enteropathogenic Escherichia coli, foot and mouth disease virus, Bordetella bronchiseptica, Mycoplasma hyopneumoniae, Pasteurella multocida or Streptococcus suis are contemplated for incorporation into the insertion- region of the PRV genome.
Furthermore, heteronucleic acid sequences encoding polypeptides for pharmaceutical or diagnostic applications, in particular immuno-modulators such as lymphokines, interferons or cytokines, or marker enzymes as β-galactosidase or superoxidedismutase may be incorporated into said insertion-region.
An essential requirement for the expression of the heterologous nucleic acid sequence in a recombinant PrV mutant is an adequate promoter operably linked to the heterologous nucleic acid sequence. It is obvious to those skilled in the art that the choice of a promoter extends to any eukaryotic, prokaryotic or viral promoter capable of directing gene transcription in cells infected by the recombinant PrV, e.g. promoters of the retroviral long terminal repeat (Gorman et al., Proc. Natl. Acad. Sci. USA 79, 6777-6781, 1982), the SV40 promoter (Mulligan and Berg, Science 209, 1422-1427, 1980) or the cytomegalovirus immediate early promoter (Schaffner et al., Cell 41, 521-530, 1985).
The technique of in vivo homologous recombination can be used to introduce a nucleic acid sequence carrying the mutated sequence into the PrV genome.
The first step of this technique includes the construction of a recombinant DNA molecule for recombination with PrV genomic DNA. Such a recombinant DNA molecule may be derived from any suitable plasmid, cosmid or phage, plasraids being most preferred, and comprises a fragment of PrV DNA containing DNA of the part of the PrV genome as defined above.
A mutation can be introduced in this fragment by deletion or by insertion of a heterologous nucleic acid sequence, optionally in combination with controlling sequences.
The DNA sequence of the part of the PrV genome as defined above preferably is flanked by PrV nucleic acid sequences which should be of appropriate length, e.g. 50-3000 bp, as to allow in vivo homologous recombination with the viral PrV genome to occur.
The recombinant DNA molecule obtained in this way is suitable for introducing the mutation into the PrV genome.
If desired, a recombinant DNA molecule can be made which contains two or more different heterologous nucleic acid sequences derived from the same or different pathogens, said sequences being incorporated into insertion-region sequences which are flanked by PrV nucleic acid sequences. Such a recombinant DNA molecule can be employed to produce recombinant PrV which expresses two or more different antigenic polypeptides to provide a multivalent vaccine.
Next, cells, e.g. swine kidney cells or VERO cells can be transfected with PrV DNA or infected with a wild type PrV in the presence of the recombinant DNA molecule as described above whereby recombination occurs between the sequences in the recombinant DNA molecule and the corresponding sequences in the PrV genome.
Recombination can also be brought about by co- transfecting the cells with a nucleic acid sequence containing the mutation sequence flanked by appropriate flanking PrV sequences without plasmid sequences. Recombinant viral progeny is thereafter produced in cell culture and can be selected for example genotypically or phenotypically, e.g. by hybridization or by detecting enzyme activity encoded by a gene co-integrated along with nucleic acid sequence comprising the mutation. Another possibility is the detection of the absence of the polypeptide for which the nucleic acid sequence in which the mutation was localized was coding. In the same way the presence of the polypeptide coded for by an inserted heterologous nucleic acid sequence can be detected.
Recombinant virus can also be selected positively based on resistance to compounds such as neomycine, gentamycine or mycophenolic acid. The selected recombinant PrV can be cultured on a large scale in cell culture after which recombinant PrV containing material or heterologous polypeptides expressed by said PrV can be collected thereof.
Host cells transformed with a recombinant DNA molecule as defined above also form part of the invention.
Also another part of the invention is formed by cell cultures infected with PrV mutants according to the invention.
A live PrV mutant according to the present invention can be used to vaccinate animals, particularly pigs. When vaccination with a PrV mutant in which the mutation is a deletion, preferably no expression of the PrV polypeptide as shown in SEQ ID NO:2 is established while still replication of the PrV mutant in the inoculated host takes place.
When vaccination is accomplished with a PrV mutant expressing one or more different heterologous polypeptides of specific pathogens it is preferably followed by replication of the recombinant PrV within the inoculated host, expressing in vivo the heterologous polypeptide along with the PrV polypeptides. The polypeptides expressed in the inoculated host will then elicit an immune response against both PrV and the specific pathogen. If the heterologous polypeptide derived from the specific pathogen can stimulate a protective immune response, then the animal inoculated with a recombinant PrV mutant according to the invention will be immune to subsequent infection by that pathogen as well as to infection by PrV. Thus, a heterologous nucleic acid sequence incorporated into the insertion-region of the PrV genome according to the invention may be
continuously expressed in vivo, providing a solid, safe and long-lasting immunity to a pathogen.
A PrV mutant according to the invention containing and expressing one or more different heterologous polypeptides can serve as a monovalent 01 multivalent vaccine.
For the preparation of a live vaccine the PrV mutant according to the present invention can be grown on a cell culture of porcine origin or on VERO cells. The viruses thus grown can be harvested by collecting the tissue cell culture fluids and/or cells. The live vaccine may be prepared in the form of a suspension or may be lyophilized.
In addition to an immunogenically effective amount of the PrV mutant the vaccine may contain a pharmaceutically acceptable carrier or diluent.
Examples of pharmaceutically acceptable carriers or diluents useful in the present invention include stabilizers such as SPGA, carbohydrates (e.g. sorbitol, mannitol, starch, sucrose, glucose, dextran), proteins such as albumin or casein, protein containing agents such as bovine serum or skimmed milk and buffers (e.g. phosphate buffer).
Optionally, one or more compounds having adjuvant activity may be added to the vaccine. Suitable adjuvants are for example aluminium hydroxide, phosphate or oxide, oil-emulsions (e.g. of Bayol F(R) or Marcol 52(R), saponins or vitamin-E solubilisate.
The useful dosage to be administered will vary depending on the age, weight and mode of administration. A suitable dosage can be for example about 102-107 pfu/animal.
An PrV mutant according to the invention can also be used to prepare an inactivated vaccine.
For administration to animals, the PrV mutant according to the presentation can be given inter alia intranasally, intradermally, subcutaneously or intramuscularly.
It is a further object of the present invention to produce subunit vaccines, pharmaceutical and diagnostic preparations comprising a heterologous polypeptide expressed by the PrV mutant according to the invention. This can be achieved by culturing cells infected with said PrV mutant under conditions that promote expression of the heterologous polypeptide. The heterologous polypeptide may then be purified with conventional techniques to a certain extent depending on its intended use and processed further into a preparation with immunizing, therapeutic or diagnostic activity.
The above described active immunization against specific pathogens will be applied as a protective treatment in healthy animals. It goes without saying that animals already infected with a specific pathogen can be treated with antiserum comprising antibodies evoked by a PrV mutant according to the invention comprising a heterologous gene derived from the specific pathogen encoding an antigenic polypeptide. Antiserum directed against a PrV mutant according to the invention can be prepared by immunizing animals, for example pigs, with an effective amount of said PrV mutant in order to elicit an appropriate immune response. Thereafter the animals are bled and antiserum can be prepared.
The invention also provides a method for distinguishing an animal vaccinated with a vaccine of the present invention from an animal infected with naturally occurring PrV. This method comprises analyzing a body fluid of the animal for the presence of antigens normally expressed in and circulating in the body fluid of an animal infected with a naturally- occurring PrV, identifying antigens which are present in the body fluid and correlating said antigens with antigens expressed in and circulating in the body fluid of an animal infected with a pseudorabies virus mutant of the invention. The presence of antigens which are normally expressed in the animal by a naturally-occurring PrV is indicative for infection with PrV, while the presence of the same antigens with the exception of those no longer included in the PrV mutant of the invention is indicative of an animal vaccinated with the vaccine of the invention and not infected with a naturally-occurring pseudorabies virus.
Determining the presence and identification of the antigens can be done directly by the detection of the antigens in the body fluid or indirectly by the detection of antibodies in the body fluid which are specific for the antigens.
More specifically the discrimination between animals vaccinated with a vaccine which comprises the PrV mutant of the invention and animals infected by naturally occurring viruses can be accomplished by analyzing a body fluid for the presence of the polypeptide shown in SEQ ID "TO:2 and at least one other antigen normally expressed in an animal both by the PrV mutant and by a naturally-occurring PrV.
Antigens or antibodies which are present in the body fluid are identified and the presence or absence of said antigens or polypeptides is determined. The presence of antigens which are normally expressed in an animal infected by a naturally-occurring virus or antibodies against such antigens and the absence of the polypeptide shown in SEQ ID NO:2 or antibodies against such polypeptides would be indicative of an animal vaccinated with the vaccine of the invention and not infected with naturally-occurring PrV.
Another aspect of the invention is a testkit for distuinguishing the PrV mutant of the invention from naturally-occurring PrV mutants in the body fluid of an animal. Such a testkit comprises a compound suitable for the detection of the polypeptide shown in SLQ ID NO:2, or antibodies against it, and a compound suitable for the detection of an antigen expressed by both the PrV mutant accoording to the invention and naturally-occurring PrV strains, or antibodies against said antigen.
Another test can be performed to determine if an animal is infected by a naturally-occurring PrV. In this case only a test on the presence of antigens from or antibodies against the polypeptide shown in SEQ ID NO:2 can show if an animal has been infected by a naturally-occurring PrV.
Accordingly a teskit comprising only the test on the presence of antigens from or antibodies against the polypeptide shown in SEQ ID NO:2 forms part of the invention.
EXAMPLES
1. Virus and cell culture
The virulent PRV strain Ka and mutant PRV strains were propagated and plaque-ourified in Madin Darby bovine kidney cells (MDBK, ATCC CCL 221) or in SK-6 porcine kidney cells.
The cells were maintained in Eagle minimal essential medium (MEM) with 10% newborn calf serum (Boehringer, Mannheim, FRG) and 100 units/ml penicillin and 100 μg/ml streptomycin. For growth of virus also BHK (baby hamster kidney) cells were used in Dulbecco modified minimal essential medium (DMEM). Virions were purified from the supernatant of infected cells (ca. 5 pfu/cell) by differential centrifugation and velocity sedimentation through 12 to 52% (w/v) sucrose gradient as recently described (Lukacs et al., 1985).
The virion band was aspirated, diluted with 0.2 M Tris- HC1, 5 mM EDTA, 0.15 M NaCl, and concentrated by pelleting in a SW27 rotor (Beckman) at 25.000 RPM, 4°C for one hour.
2. Subcloning and sequence analysis
Bam HI fragment 4 of the wildtype pseudorabies virus strain Ka was subcloned as a 3.8 kb Bam Hi/Sal I fragment, a 2.7 kb Sal I fragment and a 2.9 kb Sal I fragment into a pBR322 derivative into which a multiple cloning site originating from bacteriophage M13mpl8 had been introduced. The extreme left and right termini of the whole Bam HI-4 fragment were sequenced. For further sequencing a nested set of overlapping deletion subclones were prepared by exonuclease III/nuclease SI digestion (Henikoff, S., 1986. Unidirectional digestion with exonuclease III created targeted breakpoints for DNA sequencing. Gene 28:351-359) using a commercially available kit (Pharmacia, Freiburg, Germany). DNA sequence analysis was performed by the dideoxy chain
termination method (Sanger, F., Nicklen, S. and Coulson, A.R., 1977. DNA sequencing with chain terminating inhibitors. Proc. Natl. Acad. Sci. USA 74:5463-5467) on double-strand plasmid DNA (Hattori, M. and Sakaki, Y., 1986. Dideoxy sequencing method using denatured plasmid templates. Anal. Biochem. 152:232-238) using pBR322- specific oligonucleotides as primers (New England Biolabs). 7-deaza-2 -deoxy-GTP was used in stead of dGTP in sequencing reactions to minimize band compression (Mizusawa S., Nishimura, S. and Seela, F., 1986. Improvement of dideoxy chain termination method of DNA sequencing by use of deoxy-7-deazaguanosine triphosphate in place of dGTP. Nucleic Acids Res. 14, 1319-1324) resulting from the high G+C content of pseudorabies virus DNA. Sequencing products were labelled with 35S- dATP (Amersham-Buchler, Braunschweig, Germany) and electrophoretically separated fragments were visualized by autoradiography. Sequences of both strands of the viral DNA were determined at least twice on independent clones. Orientation of Bam HI fragment 4 relative to Bam HI-15 was determined by partial sequencing of a Sal I- fragment containing the Bam HI-15 junction. Sequences obtained were compiled using the University of Wisconsin Genetics Computer Group software package (Devereux, J. , Haeberli, P. and Smithies, O. , 1984. A comprehensive set of sequence analysis for the VAX. Nucleic Acids Res. 12:387-395) in VAX/VMS version 7.1. It was found that the sequence contained two open reading frames.
A first ORF (SEQ ID NO:l), ORF-1, can be found from basepair no. 760 to basepair no. 2333. The start codon is localized at basepair 2333, indicating a transcription direction opposite to the second ORF, ORF- 2, which can be found from basepair no. 2440 to basepair no. 2921.
The intergenic sequence between the two ORF's comprises an AT-rich sequence, which probably functions as a control element.
3. Determination of virulence marker. The non virulent PRV Bartha strain has 3 different lesions in its genome. Firstly a deletion in the US region influencing the expression of the glycoproteins gl and gp63 (Lo niczi et al. J.Virol. 49, 970-979 (1984)). Secondly a mutation in the nonessential gill glycoprotein (Mettenleiter et al. J.Virol. 62, 2712-2717 (1988)). Thirdly an effect in the BamHI-4 fragment that was not defined yet (Lominiczi et al., J.Virol. 61, 796-801 (1987)). To define the exact nature of this defect the BamHI-4 fragment of both the Bartha and the wildtype Kaplan strain were sequenced. A 3.8 kb BamHI/sall, a 2.7 kb Sail/Sail, and a 2.9 Sail/Sail subfragment of the BamHI-4 fragment were subcloned in pBR322. Firstly the left and the right termini of the BamHI-4 fragment were sequenced. Secondly a overlapping nested set of deletion subclones was prepared by exonucleaselll/nuclease SI digestion using a commercially available kit (Pharmacia, Freiburg, Germany) . Then both strands of the viral DNA were sequenced twice on independent clones. The sequences overlapping the Sail sites were determined by using nested deletion subclones from the complete BamHI-4 fragment. DNA sequence analyses was performed by the dideoxy chain termination method using pBR322 specific oligonucleotides as primers. Sequence comparison of the 3.8 BamHI/Sall subfragment of the Bartha strain and the wildtype Kaplan strain revealed 7 nucleotide changes in the region of the ORF (SEQ ID NO:l), 3 of which resulted into an amino acid change in the ORF (Table 1).
Table 1
No amino acid changes could be found in the ORF-2, the N-terminal part of the subsequent ORF or in the ori consensus. To determine if the reduced virulence of the Bartha strain is caused by these amino acid sequence changes, the ORF of the Bartha strain corresponding to the ORF defined herein was replaced by this ORF (SEQ ID NO:l) of the Kaplan strain. In this marker rescue experiment a Bartha strain was used were the gill as well as the gl/gp63- defects had already been restored. The complete 3.8 kb BamHI/Sall fragment of the Kaplan strain (without the 7 mutations) was subcloned in pBR322. This fragment was exchanged with the BamHI/Sall fragment of the Bartha strain by cotransfection of the 3.8 kb fragment with the glll-gl/gp63 restored Bartha mutant. Bartha clones with the 3.8 kb Kaplan fragment were selected and further purified by three rounds of plaque purification.
An animal experiment with the Bartha strain, the Bartha strain with the restored gill and gl/gp63 defects and the Bartha strain with the restored gill, gl/gp63 and ORF defects was performed to determine the contribution of these defects to the virulence of PRV in pigs. In this experiment the Bartha strain proved to be non virulent, the Bartha strain with the restored gill and gl/gp63 defects proved to be very mildly virulent. The restoration of the ORF resulted in a full virulent PRV strain. Restoration of the other parts of the BamHI-4 fragment did not had any influence on the virulence (Figure 1) .
4. Construction of a deletion and insertion in the open reading frame.
To construct an ORF PRV Kaplan mutant, the left 3.8 kb BamHI/Sall fragment of the BamHI-4 was cloned into the multiple cloning site of pBR322. Then the left BamHI site was deleted by cleavage with BamHI, Klenow fill up and religation. Cleavage with Bst-XI/StuI resulted in a 126 bp deletion within the ORF. In this deletion an unique BamHI site was created by linker insertion. In this new BamHI site, a gX-BGal expression cassette (Mettenleiter et al., J of Virol Meth. , 30, 55-66 (1990)) was inserted. The ORF with the BGal cassette was then used for cotransfection with the PRV Kaplan strain. All blue staining plaques were isolated, checked by restriction analyses and souther blotting, and further purified by three rounds of plaque purification.
LEGEND TO THE FIGURE.
Marker rescue experiments with subfragments of BamHI-4 using SalI-subfragments of 2.7 kbp, 2.9 kbp and BamHI/Sall-subfragment of 3.8 kbp. Location of the BamHI restriction sites is indicated in the middle part of the figure.
The location of the ORFs within the BamHI-4 fragment is indicated by the open bars. Results (+ or -) of the marker rescue experiments are summarized in the lower part of the figure.
SEQUENCE LISTING
(1) GENERAL INFORMATION:
(i) APPLICANT:
(A) NAME: AKZO N.V.
(B) STREET: Velperweg 76
(C) CITY: Arnhem
(E) COUNTRY: The Netherlands
(F) POSTAL CODE (ZIP): NL-6824 BM
(ii) TITLE OF INVENTION: Pseudorabies virus vaccine (iii) NUMBER OF SEQUENCES: 2
(iv) COMPUTER READABLE FORM:
(A) MEDIUM TYPE: Floppy disk
(B) COMPUTER: IBM PC compatible
(C) OPERATING SYSTEM: PC-DOS/MS-DOS
(D) SOFTWARE: Patentln Release #1.0, Version #1.25 (EPO)
(vi) PRIOR APPLICATION DATA:
(A) APPLICATION NUMBER: EP 92.203.079.6
(B) FILING DATE: 06-OCT-1992
(2) INFORMATION FOR SEQ ID NO:l:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 1578 base pairs
(B) TYPE: nucleic acid
(C) STRANDEDNESS: double
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: DNA (genomic)
( i) ORIGINAL SOURCE:
(A) ORGANISM: Pseudorabies virus
(B) STRAIN: Kaplan
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:l:
ATGGAGTTTG AGTACCAGAG CACGATCGTG CACCAGGGGG TGCTGTTCTA CGTCGCCGAC 60
GGCGGGGACC GCGCGTACTT TGTGCACGGG GGCTGCATCG TGTCCGTGCA CCGGCGCTCG 120
CGGGAGATCG GCAAGTTCGG GCTCACGCTG CGCGGGAACG CGCCCGGGAA CCGCGTCGTC 180
GCCAACTACG TGCGCACGGA GCTGGCGCGC CTCGGCCGCG CGTGGGCCGC CCCGCAGGGG 240
AGCGACGACG TCTTCGTGGA CGCCCTGGGG CTGCTGCTGC CGCTGACGGA GCTGGACCTC 300
TGCGGCCGCG CGGAGCTGGA CGTGTACGAC CCCTACCTCG TCGAGTGCAT GGTCTCGCTG 360
CCGGCGTCGG CGCTCTCGCT GACGCTCGTG CACGACCGCC AGCAGGACCG CGTCCTGGAG 420
SUBSTITUTESHEET
CTCCTGGCCG AGCCCGCCAT CGTGCACCCC TCCTCGGGCT TCGTGTACGC CGTGAACGAG 48 GCCTGCTTCG CGCTGGTGCA GGCGTACCTC TCCGAGCTGC CCAGCTCGCT GCAGGTGCTG 54 ACGGAGGGGC TCTTTGACGG CATCCCCGGC GTGCGCCCCC CGCTCAGCGG CGAGACGCGG 60 CCCACGGCCG TGGTGGTGAA GGGCGGGCGC GCGGCCCCCA CGCTGAGCGT GCGCCCGCGC 66 CGGTACGCCG AGCGCGCGCT GCGCGCGACG GTGGTCAGCG ACTTTGTGCA GGTGCGCTAC 72 ATCCCGGCGA CGCGGCGCAT CTGGGCGACG CGCGGCGGGA GCCTGTCCCT GCAGATGCTC 78 TGCGACCTCG TGGCCGGGGC GGACGCCATC CTGCGGCGGG CCGCGGGCGC CTCGGACGAC 84 GCCTCGGCCG CCGTGGTCGA GGCCGTGTCC GCCGTCGCGG CGGACCCCTT CTTCGGGACG 90 GGCTCCACGT CGCTCACGGG CGCGCAGCGG TTCGCGCTGT ACCAGTTCAT CCTGGCCCGC 96 TGGCACCTGC CGAGCTGCTA CGCCGCGCTG GAGGGCATGC TCGACAGGCT GGACGAGCGC 102 CCCGGGGCGG GCGCGGGCGA CGACGACGAC GACGACGGAG GAGAAGGGGG AGGAGGGGGC 108 GGCCACGGCG GCTCTCGGGC CGCGAGCGCC GTGGCCCACG CCGTCAACCG CGTGCTGCGC 1140 GAGGCGACCG TCTTCGGCGA GGTGATGCGG ATGCTCGTGA ACGCCGCCGT GGTGCACGCC 1200 CCCGCGATCG CGGACCCGGC GGGGGCCTCG CCGCCGACGA CGAAGCACGC CCGGGAGGAC 1260 GCGGCGACGG GCCTGGAGCT GGCGGTCATG ATGAGCGACG CGGAGACGAA CGCGCCGGAC 1320 GCCGACGCGT GCGAGCTGGT GGAGGCGGCC GGGGCGCGGG TGCTGGACGG GCTCTACGCC 1380 GGCCGGGGCC TCGTCGCCGC GACGGCGCCC GTGGGGCGCG CGCTGCGGCC CACGTCCGCC 144 GTCTGCGCCG AGGCGGCGCT CCTGACCGCC TTCGGCGACT CGCCCGCGGC CCTCCGCGGG 1500 GCCCAGTACC TGTTTCAGCT GTTTCGGGCG CGCCTGACCC GCGCCAACAT CTCCATCGTC 1560 CTCAATAAAA ACCGTTAA 1578
SUBSTITUTE SHEET
(2) INFORMATION FOR SEQ ID NO:2:
(i) SEQUENCE CHARACTERISTICS:
(A) LENGTH: 525 amino acids
(B) TYPE: amino acid
(C) STRANDEDNESS: single
(D) TOPOLOGY: linear
(ii) MOLECULE TYPE: protein
(vi) ORIGINAL SOURCE:
(A) ORGANISM: Pseudorabies virus
(B) STRAIN: Kaplan
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:2:
Met Glu Phe Glu Tyr Gin Ser Thr He Val His Gin Gly Val Leu Phe 1 5 10 15
Tyr Val Ala Asp Gly Gly Asp Arg Ala Tyr Phe Val His Gly Gly Cys
20 25 30
He Val Ser Val His Arg Arg Ser Arg Glu He Gly Lys Phe Gly Leu 35 40 45
Thr Leu Arg Gly Asn Ala Pro Gly Asn Arg Val Val Ala Asn Tyr Val 50 55 60
Arg Thr Glu Leu Ala Arg Leu Gly Arg Ala Trp Ala Ala Pro Gin Gly 65 70 75 80
Ser Asp Asp Val Phe Val Asp Ala Leu Gly Leu Leu Leu Pro Leu Thr
85 90 95
Glu Leu Asp Leu Cys Gly Arg Ala Glu Leu Asp Val Tyr Asp Pro Tyr 100 105 110
Leu Val Glu Cys Met Val Ser Leu Pro Ala Ser Ala Leu Ser Leu Thr 115 120 125
Leu Val His Asp Arg Gin Gin Asp Arg Val Leu Glu Leu Leu Ala Glu 130 135 140
Pro Ala He Val His Pro Ser Ser Gly Phe Val Tyr Ala Val Asn Glu 145 150 155 160
Ala Cys Phe Ala Leu Val Gin Ala Tyr Leu Ser Glu Leu Pro Ser Ser
165 170 175
Leu Gin Val Leu Thr Glu Gly Leu Phe Asp Gly He Pro Gly Val Arg 180 185 190
Pro Pro Leu Ser Gly Glu Thr Arg Pro Thr Ala Val Val Val Lys Gly 195 200 205
Gly Arg Ala Ala Pro Thr Leu Ser Val Arg Pro Arg Arg Tyr Ala Glu 210 215 220
Arg Ala Leu Arg Ala Thr Val Val Ser Asp Phe Val Gin Val Arg Tyr 225 230 235 240
He Pro Ala Thr Arg Arg He Trp Ala Thr Arg Gly Gly Ser Leu Ser 245 250 255
Leu Gin Met Leu Cys Asp Leu Val Ala Gly Ala Asp Ala He Leu Arg 260 265 270
Arg Ala Ala Gly Ala Ser Asp Asp Ala Ser Ala Ala Val Val Glu Ala 275 280 285
Val Ser Ala Val Ala Ala Asp Pro Phe Phe Gly Thr Gly Ser Thr Ser 290 295 300
Leu Thr Gly Ala Gin Arg Phe Ala Leu Tyr Gin Phe He Leu Ala Arg 305 310 315 320
Trp His Leu Pro Ser Cys Tyr Ala Ala Leu Glu Gly Met Leu Asp Arg 325 330 335
Leu Asp Glu Arg Pro Gly Ala Gly Ala Gly Asp Asp Asp Asp Asp Asp 340 345 350
Gly Gly Glu Gly Gly Gly Gly Gly Gly His Gly Gly Ser Arg Ala Ala 355 360 365
Ser Ala Val Ala His Ala Val Asn Arg Val Leu Arg Glu Ala Thr Val 370 375 380
Phe Gly Glu Val Met Arg Met Leu Val Asn Ala Ala Val Val His Ala 385 390 395 400
Pro Ala He Ala Asp Pro Ala Gly Ala Ser Pro Pro Thr Thr Lys His 405 410 415
Ala Arg Glu Asp Ala Ala Thr Gly Leu Glu Leu Ala Val Met Met Ser 420 425 430
Asp Ala Glu Thr Asn Ala Pro Asp Ala Asp Ala Cys Glu Leu Val Glu 435 440 445
Ala Ala Gly Ala Arg Val Leu Asp Gly Leu Tyr Ala Gly Arg Gly Leu 450 455 460
Val Ala Ala Thr Ala Pro Val Gly Arg Ala Leu Arg Pro Thr Ser Ala 465 470 475 480
Val Cys Ala Glu Ala Ala Leu Leu Thr Ala Phe Gly Asp Ser Pro Ala 485 490 495
Ala Leu Arg Gly Ala Gin Tyr Leu Phe Gin Leu Phe Arg Ala Arg Leu 500 505 510
Thr Arg Ala Asn He Ser He Val Leu Asn Lys Asn Arg 515 520 525