GB2228741A - Attenuated viruses. - Google Patents
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- C12N2770/32011—Picornaviridae
- C12N2770/32611—Poliovirus
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Abstract
An attenuated enterovirus or rhinovirus, suitable for use as a vaccine, has a reversed base pairing in the part, or in a part corresponding to the part, of the 5 min non-coding region of the genome of poliovirus type 3 Leon strain shown below: <IMAGE> A suitable attenuated poliovirus has the bases G and C at positions 469 and 534 respectively for a type 1 or type 2 poliovirus or at positions 472 and 537 respectively for a type 3 poliovirus.
Description
1, A - 1 ATTENUATED VIRUSES
This invention relates to the construction of vaccines agaidst rhinoviruses and enteroviruses, particularly polioviruses, by the introduction of defined mutations into their genomes. These mutations attenuate the virulence of wild type viruses and can further attenuate existing live attenuated vaccine virus strains, thereby making them less likely to revert to virulence.
At the present time, the only vaccines routinely used against enterovirus and rhinovirus infections are those against poliomyelitis. of these the live attenuated vaccines developed by Sabin in the 1950's have found greatest use throughout the world. Vaccine strains.derived from each of the three poliovirus serotypes (P1, P2 and P3) were prepared by passage of wild type viruses in cell cultures and whole animals until attenuated strains were obtained. These attenuated viruses are substantially less able to cause poliomyelitis in humans than the original wild type strains. They are administered orally and replicate in the gut to induce a protective immune response.
Although'these vaccines are generally regarded as safe, their use is associated with a low level of paralysis in vaccinees. This is most often associated with type 2 and type 3 serotypes and rarely, if ever, with type 1. There is therefore a requirement for improved type 2 and i type 3 vaccines which would be comparable in safety to the excellent type 1 strain. There is also a requirement for vaccines agairfst other enteroviruses, e.g. echo, coxsackie and hepatitis A, and against rhinoviruses.
The Sabin vaccine strains were developed by essentially empirical procedures. The genetic basis of their attenuation is not properly understood. over the past few years, however, scientists have employed a number of molecular biological techniques in an attempt to elucidate the mechanism by which the neurovirulence of these vaccine strains is reduced. Most of the work has concentrated on serotypes 1 and 3. For both of these the complete nucleotide sequences of the vaccine strains have been compared with those of their neurovirulent progenitors.
In the case of poliovirus type 1, the vaccine strain differs from its progenitor at 47 positions in the 7441 base genome (Nomoto et al, 1982, Proc Natl Acad SCi USA 79: 5793-5797). All of these are simple point mutations and 21 of them give rise to amino acid changes in virus coded proteins. Although several mutations are thought to contribute to the attenuation phenotype of the vaccine strain, direct evidence has been presented that the mutation of A to G at position 480 in the 51 noncoding region of the genome has a marked attenuating effect on the virus (Nomoto et al, 1987, UCLA Symp Mol Cell Biol, New 1 j ' - 3 Series, Vol 54 (Eds M A Brinton and R R Rueckert), 437-452, New York: Alan R Liss Inc).
Anal'ogous studies on poliovirus type 3 reveal just 10 nucleotide sequence differences in the 7432 base genome between the vaccine and its progenitor strain (Stanway et al, 1984, Proc Natl Acad Sci USA 81 1539- 1543). Just three of these give rise to amino acid substitutions in virus encoded proteins. The construction of defined recombinants between the vaccine and its progenitor strain has allowed the identification of the mutations which contribute to the attenuation phenotype. one of these is at position 2034 and causes a serine to phenylalanine change in virus protein VP3.
The other mutation of interest is C to U at position 472 in the 51 noncoding region of the genome. This latter mutation has been observed to rev.ert to the wild type C rapidly upon replication of the virus in the human gut (Evans et al, 1985, Nature 314: 548-550). This reversion is associated with an increase in neurovirulence. C at position 472 has also been shown to be essen Itial for' growth of a mouse/human polio recombinant virus in the mouse brain (La Monica et al, 1986, J Virol 57: 515-525). Recently, we have observed that at 481 in poliovirus type A changes to G in an analogous fashion upon replication of the type 2 vaccine in the gut of vaccinees.
in EP-A-0323900 attenuated enteroviruses in 2 - 4 particular polioviruses, and rhinoviruses are described which have an attenuating mutation at a position which is, or correspondswith, position 479 or 482 of poliovirus type 3 Leon strain. The attenuated viruses may also have an attenuating mutation at position 472.
A new model for the secondary structure of the 51 non-coding RNA of poliovirus type 3 Leon strain has now been proposed by us (Skinner et al, 1989, J. Mol. Biol, 207, 379-392). in the model, bases in the region 470 to 540 are paired as follows:
471 477 483 .U C C.... C C A U G G A...
A G G.... G G U G C C U...
538 534 528 We have found that a poliovirus with the base pair 472-537 reversed, i.e. 472 G and 537 C, is attenuated. Further, this attenuated virus has a slightly lower LD.. value than the corresponding poliovirus which only has the mutation C to G at position 472 but which retains the wildtype G at position 537. There is no selective pressure on a poliovirus to mutate to a more attenuated poliovirus, so the attenuation in the double mutant poliovirus may be locked in.
The findings can be extrapolated to all polioviruses.
1 4 I- 1 1 - 5 Indeed, they may be extrapolated to other enteroviruses and rhinoviruses. Mutations resulting in the reversal of a base pair at sites c;f other enteroviruses and rhinoviruses corresponding to the positions shown above for poliovirus type 3 Leon strain can lead to attenuation. There is a relatively high degree of homology between the genome RNA of all enteroviruses and rhinoviruses. The positions of another strain of enterovirus or rhinovirus corresponding to the positions of poliovirus type 3 Leon strain (based on the numbering used in the Stanway ft l paper already referred to) can be determined by lining up the sequences of the genomic RNA of the strains.
Accordingly the invention relates to attenuated enteroviruses and rhinoviruses in which there is a reversal of a base pairing in the part, or in a part corresponding to the part, of the 51 non-coding region of the 9pnome of poliovirus type 3 Leon strain shown below:
471 477 483 U C C C C A U G G A A G G G G U G C C U 538 534 528 : 8 The accompanying Figure shows the relevant part of the 51 non-coding region of poliovirus type 3 Leon strain in more detail. In accordance with the present invention, one 1 A tf or more of the base pairs 471/538, 472/537, 473/536, 477/534, 478/533, 479/532, 480/531, 481/530, 482/529 and 483/528 or of the corresponding base pairs of rhinoviruses or of other enteroviruses may be reversed.
The present invention is particularly applicable to polioviruses. The invention is typically applied to a virus responsible for a disease or illness in humans. An attenuated poliovirus may be a type 1, type 2 or type 3 poliovirus, for example a Sabin strain with a reversed base pairing according to the invention. Types 2 and 3 are preferred. For types 1 and 2, positions 468, 474, 480, 525, 531 and 535 correspond to positions 471, 477, 483, 528, 534 and 538 respectively of poliovirus type 3.
Any base pair may be reversed to obtain an attenuated virus. More than one base pair, for example 2 or 3 base pairs, may be reversed. We have found in particular that the double mutation C to G at position 472 and G to C at position 537 in the 51 non-coding region of poliovirus type 3 Leon strain causes attenuation. A useful attenuated poliovirus therefore has the bases G and C at posi,tions 472 and 537 respectively in the case of type 3 polioviruses or at positions 469 and 534 respectively in the case of type 1 or 2 polioviruses. Indeed a useful attenuated enterovirus or rhinovirus generally may have a reversed base pairing at the paired positions corresponding to positions 472 and 537 of poliovirus type 3 Leon strain.
In a separate aspect of the invention, there are 1 z A - 7 provided attenuated enteroviruses, in'particular polioviruses, and rhinoviruses having an attenuating mutation at least at a position which is, or corresponds with, position 537 of the genome of poliovirus type 3 Leon strain. optionally there is also an attenuating mutation at position 472.
Such an attenuated poliovirus may be a type 1, type 2 or type 3 poliovirus, for example a Sabin strain. Types 2 and 3 are preferred. For types 1 and 2, positions 469 and 534 correspond to positions 472 and 537 of poliovirus type 3 Leon strain. A useful attenuated poliovirus therefore has the base C at position 537 in the case of type 3 polioviruses or at position 534 in the case of types 1 and 2 polioviruses. Useful attenuated viruses with mutations at both positions 472 and 537 or at the corresponding positions are as described above.
An attenuated virus according to the invention is prepared by a process comprising: introducing the or each desired mutation by site-directed mutagenesis into a sub-cloned regi6rv, which includes the or each position it is wished to mutate, of a eDNA of an enterovirus or rhinovirus; (ii) reintroducing the thus modified region into a complete cDNA from which the region was derived; and (iii) obtaining live virus from the cDNA thus obtained.
A mutation can be introduced into a strain of an enterovirus or rhinovirub, for example wild-type virus, by - 8 site-directed mutagenesis of its genomic RNA. This may be achieved beginning with sub-cloning the appropriate region from an infectious DNA copy of the genome of any of the virus strain, for example a vaccine strain or its progenitor, into the single strand DNA of a bacteriophage such as M13. The virus strain may be a neurovirulent strain but is preferably a vaccine strain. For poliovirus it may be a Sabin, type 3 Leon or type 1 Mahoney strain. The or each desired mutation is then introduced into this sub-cloned cDNA using the technique of oligonucleotide directed mutagenesis.
After the introduction of mutations, the modified sub-cloned cDNAs are reintroduced into the complete cDNA from which they were derived and, for virulence testing in mice, into a cDNA derived from a murine poliovirus derivative known to cause a poliomyelitis type.disease in mice (La Monica et al, 1986). Live virus is recovered from the mutated full length cDNA by production of a positive sense RNA typically using a T7 promoter to direct transcription in vitro (van der Werf et alp 19869:1 Proc Natl Acad Sci, USA 83: 2330-2334). The recovered RNA may be applied to tissue cultures using standard techniques (Koch, 1973, Curr Top Microbiol Immunol 61: 89-138). After 4-6 days incubation virus can be recovered from the supernatant of the tissue culture. The level of neurovirulence of the modified virus may then be compared with that of the
1 j unmodified virus using a standard LDSO test in mice (La Monica et al, 1986) or the WHO approved vaccine safety test in monkeys (WHO Tech Rep Ser 687: 107-175, 1983).
The attenuated viruses can be used as vaccines. They may therefore be formulated as pharmaceutical compositions further comprising a pharmaceutically acceptable carrier or diluent. Any carrier or diluent conventionally used in vaccine preparations may be employed. For example, the presently used live attenuated poliovirus strains are stabilised in a solution of 1 molar MgCl 2 and administered as a mixture of the three serotypes.
The attenuated viruses can therefore be used to prevent an infection attributable to an enterovirus or rhinovirus in a human patient. For this purpose, they may be administered orally, as a nasal spray, or parenterally, for example by subcutaneous or intramuscular injection. A dose corresponding to the amount administered for a conventional live virus vaccine, such as up to 106 TCIDSO for a Sabin vaccine strain in the case of poliovirus, may be administered.
The following Examples illustrate the invention. EXAMPLE 1 Construction of in vitro mutants A synthetic T7 polymerase promoter was cloned into pBR322 in an EcoRI- Hind3 linker to give pBRT7. The linker 11' 11 - 10 included a Stul site 51 of the Hind3 site. The sequence fr'om the T7 polymerase promoter to the Stul site of the iesulting construct was: TTC GAA ATT AAT AW ACT CAC TAT AGG CCT.
This enabled sequences to be ligated to the T7 promoter so that only 2 extra Gs would be added to the 51 end of RNA transcripts. The extreme 51 end of p0LIO LEON (Stanway et al, 1984), which has a poly G tail and a Pstl site as a result of the cDNA cloning procedure, was replaced by a linker of the sequence:
TAT GAC GCG TGC GGC CGC AAG C= TAA A.AC7 (P01'o 51 non- coding region)... GGTAC...
The 51 end was therefore limited by a Hind3 site, whilst the Pstl site and the poly G tail were removed. A Kpnl site, at position 70 in Leon, was used as the 31 end of the linker. Using this construction, the 51 end of p0LIO LEON from the Hind3 to a BamHI site (674), was cloned into pBRT7 to give pBRT7SIL. The 51 non-coding region was brought under the control of the T7 promoter by digesting pBRT7SIL with Stul and Hind3, making the Hind3 site blunt-ended using mung bean nuclease and religating to give pl5 MBN. The resulting T7 promoter and 51 poliovirus sequence thus read: TTCGAAATTAATACGACTCACTATAGGTTAAAC-.
An Sst I site at the 31 end of the hybrid poliovirus type 3 Leon/type 2 lansing sequence in pVN23 (La Monica et 1 1 - 11 al, 1986) was removed by partial Sst I digestion, filling in by T4 polymerase and religation. Poliovirus sequences from this plasmid were then cloned into pl-5 MBN, following digestion of-both plasmids with M1ul and Sall, to give pT75PP. Infectious virus could be recovered by linearising pT75PP with Sall, synthesis of full length RNA using T7 polymerase and transfection of Hela cells with the RNA using the DEAE dextran method (van der Werf et al, 1986).
The template for in vitro mutagenesis was made by subcloning the 51 noncoding region of poliovirus type 3 Leon from pVN23 (La Monica et al, 1986) into the M13 derivative mICE 19 (Epernon, Nucl.Acids Res. 14, 2830, 1986), using the Hind3 and Sstl sites. A mutation was then introduced into this subcloned DNA fragment using the technique of oligonucleotide- directed mutagenesis (Zoller and Smith, Nucl. Acids Res. 10, 6487-6500, 198.2). The oligonucleotide used for construct MAS 27-7 was: CCA TGG TTA GCA TTA GCC GC.
Mutant 27-7 was constructed by hybridising this oligonucleotide to the single stranded cloned DNA fragment, in the M13 phage derivative. The oligonucleotide is complementary to the target region except at the position to be mutated, where the base complementary to the desired mutation is incorporated. The hybridised M13 and oligonucleotide DNA were incubated in a reaction mixture containing DNA precursors and the enzymes DNA polymerase and - 12 DNA ligase. After incubation for one hour at 37'C, closed circular DNA was isolated from this mixture by agarose gel e lectrophoresis'. This DNA was then used to transform E coli mutS or mutL-(deficient in DNA mismatch repair) which were then plated out on a lawn of E coli JM101.
M13 plaques which arose on this lawn of E coli were picked and propagated and single stranded M13 phage DNA isolated. The DNAS were then sequenced using the method of Sanger and those with the desired mutation were identified. From these, batches of replicative form double stranded DNA were prepared and the M1ul-Sstl fragment containing 471 base pairs of infectious poliovirus cDNA, which incorporates the mutation, was recovered The mutated cDNA fragment was then reintroduced into pT7SFP. Live virus was recovered from the mutated full length cDNA by the production of a positive sense RNA transcript from the T7 promoter in vitro (van der Werf et al, 1986) which was applied to Hela cells in tissue culture using standard techniques (Koch, 1973). After 4 to 6 days incubation a cytopathic effect was observed and vi,rus could be recovered from the supernatant.
Recovered mutant virus 27-7 with a G at position 472 was plaque purified and propagated in Hela cells. This virus pool was used for the preparation of RNA on which the sequence of the virus mutant was verified using primer extension nucleotide sequencing (Evans et al, 1985). A !f -f portion of the pool was also used to assay neurovirulence.
Assessment of vIrulence for mice Mutant virus 27-7 was grown in Hep2c cells, purified on sucrose gradie, nts (Evans et al, 1985) and pelleted twice through phosphate buffered saline (PBS) before resuspension in PBA at 109 pfu per ml. C57 black mice (obtained from OLAC), aged 21-28 days, were inoculated intracranially with 10-20pl of virus. Virus dilutions examined were from 101 to 10 7 pfu per mouse in tenfold steps, and five or ten mice were used per dilution. Animals were observed once or twice a day for a period of up to 40 days post inoculation. The endpoint of the experiment for the determination of the LDSO value was set at 21 days. The LDSO value of mutant 27-7 was >107 PfU.
Animals were sacrificed when full flaccid paralysis of one or more limbs was evident, and stored at -20'C until the brain was removed for virus isolation. The brain was homogenised in 10m1 PBS, clarified by low speed centrifugation and filtered through a 0.22pm filter before inoculation of' 4m1 onto 108 Hep2c cells. Five viruses were recovered. The recovered viruses were designated 27 plaque 1A, 27 plague 2A, 27.7A, 27.7B and 27. 7C. Virus isolates were grown up, sequenced (Evans et al, 1985) and reinoculated into mice to determine their LD.. values.
The WM values and sequences are shown in Table 1 k ' - 14 below, together with those for the original mutant 27-7 and for type 3 Leon. Differences between the base sequence for type 3 Leon and that for the other viruses are underlined.
TABLE 1
Virus LD..(pgu) Sequence (470-475... 535-539) Leon 101 A U C C U A C G G A A 27-7 >10 7 A U G C U A C G G A A 27 plaque 1A 4x10 A U G C U A C G G A A 27 plaque 2A 103 27-7A 10' A U C C U A C G G A A 27-7B 10 1 A U C C U A C G G A A 27-7C 10' A U G C U A C G C A A These results show that mutant 27-7 is not a stable attenuated virus because viruses 27-7A and 27-7B, derived from 27-7, have back-mutated at position 472 to become neurovirulent viruses having LD.. values in the re, gion of 101-101 pfu. However, virus 27-7C has an LD.. value of 106 pfu and shows a compensating stabilising mutation at position 537. AS can be seen from the accompanying Figure, bases 472 and 537 are paired. Virus 27- 7C was deposited at the European Collection of Animal Cell Cultures, Porton Down, GB on 16 January 1990 under accession number ECACC 90011604.
1 1 1 EXAMPLE 2
In an attempt to identify more 27.7c type viruses, arental virus 27.7 was again intracranially injected into mice. Viruses were recovered from animals displaying paralysis. The results are shown in Table 2.
1 TABLE 2 virus Base at position: 472 537 MAS 27.7 27.7 pl A G G 27.7 A c G.
27.7 B c G 27.7 C G c 27.7 p 2A c G 27.7 p 2A/1A c G 27.7 p 2A/2A c G 27.7 p 2A/3A c G 27.7 p 2A/4A c G 27.7 p 2A/4B c G 27.7 D C T T A A G 489 492 494 498 27.7 E c G 27.7 F c G One 27.7C type virus was isolated from a group of 13 such recovered viruses. in a further attempt to identify more 27.7C typeviruses, virus 27 plaque 1A (same sequence of 51 non-coding region as the parental 27.7 virus) was injected intracranially into mice. Viruses were recovered from animals displaying paralysis. The results are shown in Table 3.
TABLE 3
Virus Base at position: 472 537 27 pl 1A G G 27 pl IA/1C c G 27 pl 1A/IB c G 27 pl IA/2B G P 27 pl 1A/2C c G 27 pl 1A/3A G c 27 pl 1A/3B c G 27 pl 1A/4A c G 27 pl 1A/5B G c 27 pl 1A/6A c G 27 pl 1A/7B c G 27 pl IA/7C c G A further three 27.7C type viruses were isolated from J - 17 a group of 12 recovered viruses. These 27.7C type viruses have been designated 27 pl 1A/2B, 27 plaque 1A/3A and 27 pl 1A/5B.
It was hoped that when this virus 27.7C was passaged many times through mice that the LD.. value of this virus woul be maintain ed at 106 _ 107 p. f.u. Indeed, it is shown in Table 4 below that when 27.7C virus was passaged for a further generation in mice (27.7C/2A-7D) that all 9 recovered viruses from mice displaying paralysis were base paired attenuating polioviruses (G at 472 and C at 537).
TABLE 4
Virus MAS 27.7 27.7 27.7 27.7 27.7 27.7 27.7 27.7 27.7 27.7 27.7 27.7 C/2A C/2B C/4A C/SA C/5B C/6A C/7A C/7 C C/7D C/2A/7A C/2A/7 C Base at position: 472 G G G G G G G G G G G G ALL G 1 537 G C C C C C C C ALL C i k - These 27.7C type viruses have now been passaged for a further three generations in mice. All polioviruses recovered from paralysed animals were base paired attenuating (LD... > 106 p.f.u.) polioviruses (G at 472 and C at 537). Some of our most recent data on the passage of these 27.7C polioviruses in mice is summarised in Table 5 below.
TABLE 5
Vi rus Base at position: LDSO 472 537 27.7 Parental Virus G G 8.25 x 10 6 27.7C G C 2.63 X 106 (3 Viruses) 27.7C/2A-7D G C 2.57 X 106 (9 Viruses) 1 27.7C/2A/3A-7B G C 5.43 X 106 (4 Viruses) EXAMPLE 3: Protective Immunity Elicited by 27.7C Type Virus In a series of experiments groups of C57BL/6 mice 1 1 - 19 were injected intracranially with 101_107 p.f.u. of a 27.7C virus. Animals were then observed daily for paralysis up to Day 50. SurvivIng non-paralysed mice were then bled out and sera assayed-for levels of neutralising antibody to Lansing poliovirus. The results for three attenuated stable base paired 27.7C type viruses are shown in Tables 6 to 8.
TABLE 6: Neutralising antibody elicited by 27.7C/2A/5B virus Day Number Virus Titre- Antibody Titre Paralysed or Injected to Lansing Non-Paralysed 10 7 32 Non-Paralysed 10 7 64 NonParalysed 26 10 6 >256 No.p-Paralysed 26 10 6 16 Non-Paralysed 27 10 5 128 Non-Paralysed 28 10 5 16 Non-Paralysed 28 10 5 < Non-Pa,ralysed 29 10 5 < Non-Paralysed 29 10 5 8 Non-Paralysed 37 10 4 < Non-Paralysed 37 10 4 < Non-Paralysed 38 10 4 < Non-Paralysed i TABLE 7: Neutralising Antibody Elicited by 27.7C/2A/7C Virus Day Number Virus Titre- Antibody Titre Paralysed or injected to Lansing Non-Paralysed 27 10 7 128 Non-Paralysed 10 6 8 Non-Paralysed 31 10 6 32 Non-Paralysed 32 10 6 64 Non-Paralysed 32 10 6 128 Non-Paralysed 33 105 >256 Non-Paralysed 33 105 8 Non-Paralysed 34 10 5 2 Non-Paralysed 34 10 5 4 Non-Paralysed 10 4 < NoP-Paralysed TABLE 8: Neutralising Antibody Elicited by 27.7C/2A/7D Virus Day Number Virus Titre Antibody Titre Paralysed or injected to Lansing Non-Paralysed 39 10 7 128 Non-Paralysed 39 10 7 64 Non-Paralysed 10 7 64 Non-Paralysed 10 7 64 Non-Paralysed 41 10 6 16 Non-Paralysed 41 10 6 64 Non-Paralysed 43 10 5 < Non-Paralysed 43 10 5 128 Non-Paralysed 44 105 2 Non-Paralysed 10 4 < Non-Paralysed 10 4 < Non-Paralysed 46 10 4 < Non-Paralysed EXAMPLE 4: Multiple copies of 27.7C virus genome obtained by polymerase chain reaction (PCR) p27.7C PCR was constructed using DNA obtained from the 27.7C virus using polymerase chain reaction. An oligonucleotide complimentary to the nucleotides 761-783 of poliovirus type 3 was used to reverse transcribe RNA extracted from purified 27.7C virus. A second 1 l( t - 22 oligonucleotide homologous to nucleotides 36-60 was then used to amplify the region of 27.7C between nucleotides 96-783 which cohtains the CG to GC mutation responsible for the attenuation of revertant 27.7C. This PCR amplified DNA was digested with M1ul and Sstl and cloned into pt7SFP (Skinner et al J. Mol. Biol. 207, 379-392, 1989), following digestion of the plasmid with M1ul and Sstl, to give p27.7C PCR.
The p27.7C PCR sequence was checked between the M1ul and Sstl cloning sites by double stranded DNA sequencing. Infectious virus was recovered by linearising p27.7C PCR with Sall, synthesising full length RNA by T7 polymerase and transfection of HeLa cells with RNA using the DEAE dextran method (van der Werf et al, 1986). The sequence of the recovered virus was determined through the inserted region, and the non-plaque purified preparation had an.LD50 of greater than 106 when tested in mice.
1 k V 1k
Claims (12)
- An attenuated enterovirus or rhinovirus in which there is a reversal of a base pairing in the part, or in a part corresponding to the part, of the 51 non-coding region of the genome of poliovirus type 3 Leon strain shown below:471 477 483 U C C.... C C A U G G A....A G G.... G G U G C C U....538 534 528
- 2. An attenuated virus according to claim 1, which is a poliovirus.
- 3. An attenuated virus according to claim 2, which is a type 1 poliovirus.
- 4. An attenuated virus according to claim 2, which is a type 2 poliovirus.
- 5. An attenuated virus according to claim 2, which is a type 3 poliovirus.
- 6. An attenuated virus according to claim 3 or 4, which has the bases G and C at positions 469 and:534 respectively.
- 7. An attenuated virus according to claim 5, which has the bases Gand C at positions 472 and 537 respectively.
- 8. A process for the preparation of an attenuated enterovirus or rhinovirus as defined in claim 1, which process comprises:i.4 k - (i) introducing the or each clesired mutation by site-directed mutagenesis into a sub-cloned region, which i ncludes the oreach position it is wished to mutate, of a CDNA of an enterovirus or rhinovirus; (ii) reintroducing the thus modified region into th complete cDNA from which the region was derived; and (M) obtaining live virus from the cDNA thus obtained.
- 9. An attenuated virus according to claim 1, which is poliovirus 27.7C or a 27.7C type poliovirus hereinbefore described in the Examples.
- 10. A pharmaceutical composition comprising a pharmaceutically acceptable carrier or diluent and an attenuated virus as claimed in any one of claims 1 to 7 and 9.
- 11. An attenuated virus as claimed in.any one of claims 1 to 7 and 9 for use as a vaccine.
- 12. An attenuated enterovirus or rhinovirus having an attenuating mutation at least at a position which is., or corresponds with, position 537 of the genoffie of Po,liovirus' type 3 Leon strain.8 Pued 1990atThe Patent Oflice,State House.6671 Mghlinlb,)rn.londonWC1R4TP. Purther copies maybe obtalnedfrom The Patent Office. Mes Branch. St Mary - ,ray. Orpingtor, Kent BR5 3RD. Prir ted by MWtiplex techniques ltd. St Mary Cray. Kent. Con 1'87 1
Applications Claiming Priority (1)
Application Number | Priority Date | Filing Date | Title |
---|---|---|---|
GB898901094A GB8901094D0 (en) | 1989-01-18 | 1989-01-18 | Attenuated viruses |
Publications (3)
Publication Number | Publication Date |
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GB9001111D0 GB9001111D0 (en) | 1990-03-21 |
GB2228741A true GB2228741A (en) | 1990-09-05 |
GB2228741B GB2228741B (en) | 1992-07-22 |
Family
ID=10650230
Family Applications (2)
Application Number | Title | Priority Date | Filing Date |
---|---|---|---|
GB898901094A Pending GB8901094D0 (en) | 1989-01-18 | 1989-01-18 | Attenuated viruses |
GB9001111A Expired - Lifetime GB2228741B (en) | 1989-01-18 | 1990-01-18 | Attenuated viruses |
Family Applications Before (1)
Application Number | Title | Priority Date | Filing Date |
---|---|---|---|
GB898901094A Pending GB8901094D0 (en) | 1989-01-18 | 1989-01-18 | Attenuated viruses |
Country Status (12)
Country | Link |
---|---|
EP (1) | EP0383433B1 (en) |
JP (1) | JPH04502705A (en) |
AT (1) | ATE89860T1 (en) |
AU (1) | AU649376B2 (en) |
CA (1) | CA2045649C (en) |
DE (1) | DE69001689T2 (en) |
DK (1) | DK0383433T3 (en) |
ES (1) | ES2058777T3 (en) |
GB (2) | GB8901094D0 (en) |
NZ (1) | NZ232152A (en) |
WO (1) | WO1990008189A1 (en) |
ZA (1) | ZA90324B (en) |
Families Citing this family (8)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
US5286640A (en) * | 1988-01-05 | 1994-02-15 | Almond Jeffrey W | Attenuated polioviruses |
GB8901093D0 (en) * | 1989-01-18 | 1989-03-15 | Almond Jeffrey W | Attenuated viruses |
EP0401421B1 (en) * | 1989-06-08 | 1996-01-03 | American Cyanamid Company | Non-reverting RNA viruses |
GB9107563D0 (en) * | 1991-04-10 | 1991-05-29 | Macadam Andrew J | Thermostable viruses |
GB9107552D0 (en) * | 1991-04-10 | 1991-05-29 | Macadam Andrew J | Attenuated viruses |
GB9323819D0 (en) * | 1993-11-19 | 1994-01-05 | Smithkline Beecham Biolog | Anlytical method |
GB0615933D0 (en) | 2006-08-10 | 2006-09-20 | Nat Inst Biological Standards & Control | Attenuated polioviruses |
GB201022077D0 (en) | 2010-12-29 | 2011-02-02 | Health Prot Agency | Inactivated poliovaccine |
Family Cites Families (2)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
GB8800100D0 (en) * | 1988-01-05 | 1988-02-10 | Almond J W | Attenuated viruses |
GB8901093D0 (en) * | 1989-01-18 | 1989-03-15 | Almond Jeffrey W | Attenuated viruses |
-
1989
- 1989-01-18 GB GB898901094A patent/GB8901094D0/en active Pending
-
1990
- 1990-01-17 ZA ZA90324A patent/ZA90324B/en unknown
- 1990-01-18 AU AU49479/90A patent/AU649376B2/en not_active Ceased
- 1990-01-18 DE DE9090300500T patent/DE69001689T2/en not_active Expired - Fee Related
- 1990-01-18 NZ NZ232152A patent/NZ232152A/en unknown
- 1990-01-18 EP EP90300500A patent/EP0383433B1/en not_active Expired - Lifetime
- 1990-01-18 JP JP2502364A patent/JPH04502705A/en active Pending
- 1990-01-18 CA CA002045649A patent/CA2045649C/en not_active Expired - Fee Related
- 1990-01-18 GB GB9001111A patent/GB2228741B/en not_active Expired - Lifetime
- 1990-01-18 WO PCT/GB1990/000074 patent/WO1990008189A1/en active Application Filing
- 1990-01-18 AT AT90300500T patent/ATE89860T1/en not_active IP Right Cessation
- 1990-01-18 ES ES90300500T patent/ES2058777T3/en not_active Expired - Lifetime
- 1990-01-18 DK DK90300500.7T patent/DK0383433T3/en active
Non-Patent Citations (1)
Title |
---|
J. Mol. Biol., vol.207, pages 379-392 (1989) * |
Also Published As
Publication number | Publication date |
---|---|
WO1990008189A1 (en) | 1990-07-26 |
ZA90324B (en) | 1990-10-31 |
ES2058777T3 (en) | 1994-11-01 |
EP0383433B1 (en) | 1993-05-26 |
GB8901094D0 (en) | 1989-03-15 |
ATE89860T1 (en) | 1993-06-15 |
GB2228741B (en) | 1992-07-22 |
DE69001689T2 (en) | 1993-09-02 |
CA2045649A1 (en) | 1990-07-19 |
AU4947990A (en) | 1990-08-13 |
DK0383433T3 (en) | 1993-06-21 |
AU649376B2 (en) | 1994-05-19 |
DE69001689D1 (en) | 1993-07-01 |
EP0383433A1 (en) | 1990-08-22 |
GB9001111D0 (en) | 1990-03-21 |
CA2045649C (en) | 1998-11-10 |
NZ232152A (en) | 1992-11-25 |
JPH04502705A (en) | 1992-05-21 |
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Legal Events
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732 | Registration of transactions, instruments or events in the register (sect. 32/1977) | ||
PCNP | Patent ceased through non-payment of renewal fee |
Effective date: 20000118 |