Detection and Characterization of Genetic Recombination in Cytopathic Type 2 Bovine Viral Diarrhea Viruses

doi:10.1128/JVI.74.18.8771-8774.2000

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Journal of Virology, September 2000, p. 8771-8774, Vol. 74, No. 18
0022-538X/00/$04.00+0

Detection and Characterization of Genetic Recombination in Cytopathic Type 2 Bovine Viral Diarrhea Viruses

Julia F. Ridpath^* and John D. Neill

Virus and Prion Diseases of Livestock Research Unit, National Animal Disease Center, Agricultural Research Service-U.S. Department of Agriculture, Ames, Iowa 50010

Received 22 October 1999/Accepted 14 June 2000

	ABSTRACT

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In cytopathic bovine viral diarrhea virus genotype 1 (BVDV1) isolates, insertions are reported at position A (amino acid [aa]1535) and position B (aa 1589). Insertions at position B predominate.In this survey it was found that in BVDV2, insertions at positionA predominate. Possible reasons for this difference in relativefrequency arediscussed.

	TEXT

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Bovine viral diarrhea viruses (BVDV) are segregated into two genotypes, BVDV1 and BVDV2 (18, 26). Viruses from eithergenotype may be characterized as cytopathic or noncytopathic (6,11, 23) based on their activity in cell culture. NoncytopathicBVDV code for an NS2-3 protein that in cytopathic BVDV is processedto an NS3 protein (5). Processing of the NS2-3 protein in cytopathicBVDV1 occurs by several different strategies depending on theviral strain (3, 9, 10, 13, 15, 20, 21, 27,28). Most commonly it is associated with the insertion of sequencesinto the viral genome. In BVDV1, the amino acid sequences flankingthe carboxy-terminal end of inserted sequences correspond to eitheramino acid position 1535 or position 1589 (numbering is basedon BVDV-1 strain SD-1, GenBank accession number M96751), referredto as positions A and B, respectively (13). Most reported insertionsinto BVDV1 have been at position B and consist of duplicated viralgenomic sequences and/or ubiquitin coding sequences (8, 21),although insertions of other cellular coding sequences have beenreported (2, 13, 20). In contrast, limited informationis available on the molecular characterization of cytopathic BVDV2insertions.

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TABLE 1. PCR primers for detection and sequencing of insertions in NS2-3

In this study, nine cytopathic BVDV2 were examined for type and location of insertions. All viruses were isolated in NorthAmerica, between 1990 and 1998, from tissues submitted to diagnosticlaboratories. Isolation and propagation of viruses were performedas described earlier (25). All cytopathic viruses, except BVDV2-96B3491c,were coisolated with noncytopathic BVDV. Viruses were cloned atlimiting dilution and genotyped based on PCR amplification andcomparison of the 5' untranslated region (26). Biotype was determinedby activity in cell culture (6, 11) and production of NS3(5, 19), as determined by radioimmunoprecipitation usingbovine polyclonal antisera (25). Viruses were found to be freeof defective interfering particles by Northern blot analysis,which was performed as previously described (17) using a BVDV-specificprobe prepared from sequences from the NS3 coding region (datanotshown).

Total RNA was prepared from cultured cells 24 h after inoculation (24). Primer design and PCR amplification were performedas described previously (26). Three PCR products were generatedfor each virus using the primers listed in Table 1. Both strandsof each PCR product were sequenced in duplicate (22). Phylogeneticanalysis was performed using the Align Plus (Scientific and EducationalSoftware, State Line, Pa.), GeneWorks (Intelligenetics Inc., MountainView, Calif.), and DNASIS (Hitachi Software, San Bruno, Calif.)softwarepackages.

The viruses represented a genetically diverse sample, with derived NS2-3 amino acid sequence similarities ranging between81.3 and 98% (Fig. 1). No correlation was seen between amino acidsequence similarity and size and type of genomic insertion. Noinsertion was detected in BVDV2-96B3491c; the remaining eightviruses had insertions (Fig. 2). Only one virus, BVDV2-MsSt T4529c,had an insertion at position B. This insertion consisted of twofull-length ubiquitin genes and one partial ubiquitin gene (Fig.3A). The partial ubiquitin gene lacked 34 amino acid residuesfrom the amino terminus. Four viruses, BVDV2-ND 8799c, BVDV2-Galena16425c, BVDV2-Ok St 94-050-297c, and BVDV2-SD1630c, had insertionsat position A. Three viruses, BVDV2-296c, BVDV2-5912c, and BVDV2-6082c,had insertions within 10 amino acid positions of position A. Inall seven viruses the insertion contained a portion of cellularsequence coding for a DnaJ-like protein (J. D. Neill and J. F.Ridpath, Abstr. 17th Annu. Meet. Am. Soc. Virol. 1998, p. W3-W10,1998; unpublished data). This sequence had previously been identifiedin BVDV1-NADL (12) and in a cytopathic border disease isolate(1) (Fig. 3). For three of these viruses, BVDV2-Galena 16452c,BVDV2-OkSt 94-050-297c, and BVDV2-6082c, the DnaJ-like sequencewas preceded by 5, 22, and 28 amino acids residues, respectively;while in a fourth virus, BVDV2-ND 8799c, the DnaJ-like sequenceswere followed by a string of 10 amino acid residues. No significantsequence similarity was found between any of these flanking aminoacid sequences or the nucleotide sequence coding for them andsequences in the GenBank.

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FIG. 1. Phylogenetic analysis of deduced amino acid sequences flanking the NS2/NS3 junction. Consensus amino acid sequences of the NS2/NS3 junction region minus insertion sequences were deduced from sequences generated by using primers shown in Table 1. Sequences compared corresponded to amino acid residues 1290 to 1610 in BVDV1-SD-1. The dendrogram was produced by applying the unpaired geometric mean analysis method using the Higgins-Sharp algorithm (CLUSTAL4) supplied in the MacDNASIS software package (Hitachi Software). Calculated matching percentages are indicated at each branch point of the dendrogram.

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FIG. 2. Insertion sites in the NS2-3 coding region. (A) Arrows show the sites of reported insertions into cytopathic BVDV1. Position A corresponds to amino acid residue 1535 and position B corresponds to amino acid residue 1589 of BVDV-1 strain SD-1 (GenBank accession number M96751). (B) The NS2-3 coding regions derived from nine cytopathic BVDV2 minus inserted sequences are shown. One noncytopathic virus coisolated with a cytopathic virus (BVDV2-296nc) and one noncytopathic BVDV2 sequence from GenBank (BVDV2-890, GenBank accession number BVU18059) were included for comparison purposes. Arrows indicate sites of insertions. No arrow indicates that there was no insertion. Unlike their noncytopathic counterparts, eight of these viruses had genomic insertions. No insertion was detected in BVDV2-96B3491c. One virus, BVDV2-MsSt T4529c, had an insertion at position B. Four viruses, BVDV2-ND 8799c, BVDV2-Galena 16425c, BVDV2-Ok St 94-050-297c, and BVDV2-SD1630c, had insertions at position A. Three viruses, BVDV2-296c, BVDV2-5912c, and BVDV2-6082c, had insertions within 10 amino acid residues of position A.

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FIG. 3. Inserted sequences detected in cytopathic BVDV2. (A) The insertion in BVDV2-MsSt T4529c at position B consisted of two full-length ubiquitin genes and a partial ubiquitin gene (34 amino acid residues from the amino acid terminus are missing). (B) Seven viruses had insertions at or within 10 amino acid residues of position A. Each of these insertions contained a portion of a cellular gene that codes for a novel DnaJ-like protein (underlined sequences). For three of these viruses, BVDV2-Galena 16452c, BVDV2-OkSt 94-050-297c, and BVDV2-6082c, the DnaJ-like sequence was proceeded by 5, 22, and 28 amino acid residues, respectively. For virus BVDV2-ND 8799c, the DnaJ-like sequence was followed by a string of 10 amino acid residues.

Regardless of the existence, identity, or position of insertion, all cytopathic viruses produced an NS3 with the same molecularweight based on mobility in polyacrylamide gel electrophoresis(data not shown). It is theorized that insertions at positionB result in processing of NS2-3 by introducing either a new cleavagesite at the carboxy terminus of the insertion or by introducingsequences with autocatalytic activity that act at the carboxyterminus of the insertion (for a review, see reference 16).The result of either mechanism is cleavage at position B, makingGly₁₅₉₀ the N-terminal amino acid of NS3. The amino acid sequencesflanking the 3' end of the insertions in the vicinity of positionA were approximately 50 amino acid residues upstream of Gly₁₅₉₀and were not highly conserved. However, as stated above, the NS3proteins produced by each of the cytopathic BVDV2 were the samesize, regardless of the insertion position. This suggests thatprocessing of the NS2-3 by cytopathic viruses with insertionsupstream from position B occurs by a different mechanism. It hasbeen proposed that insertions upstream of position B induce aconformational change that allows cleavage via a cryptic mechanismat Gly₁₅₉₀ (16), but no experimental data areavailable.

Previously, BVDV2 cytopathology has been associated with recombination between a noncytopathic BVDV2 and a cytopathic BVDV1at position A (23) or the presence of viral subgenomic RNAswith ubiquitin inserts at position B (2). In this study weshow that cytopathic BVDV2, like cytopathic BVDV1, may have insertionsat positions A or B or may have no insertions at all. Unlike cytopathicBVDV1, in which insertions are most often seen at position B andcontain ubiquitin coding sequences, insertions in BVDV2 were mostfrequently observed in the vicinity of position A and containedportions of a gene coding for a DnaJ-like protein (Neill et al.,Abstr. 17th Annu. Meet. Am. Soc. Virol. 1998). Three possibleexplanations for the differences in relative frequency of positionand type of insertion are (i) differences in recombination frequenciesdue to sequence variation, (ii) differences in the stability ofrecombinations, or (iii) differences in the relative amounts ofmRNA coding for ubiquitin and DnaJ-like protein in BVDV1- andBVDV2-infectedcells.

Nucleotide sequence accession numbers. GenBank accession numbers for sequences derived in this study are AF268171 through AF268180.

	ACKNOWLEDGMENTS

We thank Margaret Walker, Tracy Waltz, Becky Zaworski, Sharon Stark, and Bernadette Hackbart for excellent technical supporton thisproject.

	FOOTNOTES

^* Corresponding author. Mailing address: National Animal Disease Center, USDA-ARS, 2300 Dayton Ave., Ames, IA 50010. Phone:(515) 663-7586. Fax: (515) 663-7458. E-mail: jridpath{at}nadc.ars.usda.gov.

REFERENCES

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Abstract
Text
References

1. Becher, P., G. Meyers, A. D. Shannon, and H. J. Thiel. 1996. Cytopathogenicity of border disease virus is correlated with integration of cellular sequences into the viral genome. J. Virol. 70:2992-2998[Abstract].

2. Becher, P., M. Orlich, M. König, and H. J. Thiel. 1999. Nonhomologous RNA recombination in bovine viral diarrhea virus: molecular characterization of a variety of subgenomic RNAs isolated during an outbreak of fatal mucosal disease. J. Virol. 73:5646-5653[Abstract/Free Full Text].

3. Becher, P., M. Orlich, and H. J. Thiel. 1998. Ribosomal S27a coding sequences upstream of ubiquitin coding sequences in the genome of a pestivirus. J. Virol. 72:8697-8704[Abstract/Free Full Text].

4. Collett, M. S., R. Larson, S. K. Belzer, and E. Retzel. 1988. Proteins encoded by bovine viral diarrhea virus: the genomic organization of a pestivirus. Virology 165:200-208[CrossRef][Medline].

5. Donis, R. O., and E. J. Dubovi. 1987. Differences in virus-induced polypeptides in cells infected by cytopathic and noncytopathic biotypes of bovine virus diarrhea-mucosal disease virus. Virology 158:168-173[CrossRef][Medline].

6. Gillespie, J., J. Baker, and K. McEntee. 1960. A cytopathogenic strain of virus diarrhea virus. Cornell Vet. 50:73-79[Medline].

7. Greiser-Wilke, I., K. E. Dittmar, B. Liess, and V. Moennig. 1992. Heterogeneous expression of the non-structural protein p80/p125 in cells infected with different pestiviruses. J. Gen. Virol. 73:47-52[Abstract/Free Full Text].

8. Greiser-Wilke, I., L. Haas, K. Dittmar, B. Liess, and V. Moennig. 1993. RNA insertions and gene duplications in the nonstructural protein p125 region of pestivirus strains and isolates in vitro and in vivo. Virology 193:977-980[CrossRef][Medline].

9. Kümmerer, B. M., D. Stoll, and G. Meyers. 1998. Bovine viral diarrhea virus strain Oregon: a novel mechanism for processing of NS2-3 based on point mutations. J. Virol. 72:4127-4138[Abstract/Free Full Text].

10. Kupfermann, H., H. J. Thiel, E. J. Dubovi, and G. Meyers. 1996. Bovine viral diarrhea virus: characterization of a cytopathogenic defective interfering particle with two internal deletions. J. Virol. 70:8175-8181[Abstract].

11. Lee, K., and J. Gillespie. 1957. Propagation of virus diarrhea virus of cattle in tissue culture. Am. J. Vet. Res. 18:952-955[Medline].

12. Meyers, G., T. Rumenapf, N. Tautz, E. J. Dubovi, and H. J. Thiel. 1991. Insertion of cellular sequences in the genome of bovine viral diarrhea virus. Arch. Virol. Suppl. 3:133-142[Medline].

13. Meyers, G., D. Stoll, and M. Gunn. 1998. Insertion of a sequence encoding light chain 3 of microtubule-associated proteins 1A and 1B in a pestivirus genome: connection with virus cytopathogenicity and induction of lethal disease in cattle. J. Virol. 72:4139-4148[Abstract/Free Full Text].

14. Meyers, G., N. Tautz, E. J. Dubovi, and H. J. Thiel. 1991. Viral cytopathogenicity correlated with integration of ubiquitin-coding sequences. Virology 180:602-616[CrossRef][Medline].

15. Meyers, G., and H. J. Thiel. 1995. Cytopathogenicity of classical swine fever virus caused by defective interfering particles. J. Virol. 69:3683-3689[Abstract].

16. Meyers, G., and H. J. Thiel. 1996. Molecular characterization of pestiviruses. Adv. Virus Res. 47:53-118[Medline].

17. Neill, J. D., and W. L. Mengeling. 1988. Further characterization of the virus-specific RNAs in feline calicivirus infected cells. Virus Res. 11:59-72[Medline].

18. Pellerin, C., J. van den Hurk, J. Lecomte, and P. Tussen. 1994. Identification of a new group of bovine viral diarrhea virus strains associated with severe outbreaks and high mortalities. Virology 203:260-268[CrossRef][Medline].

19. Pocock, D. H., C. J. Howard, M. C. Clarke, and J. Brownlie. 1987. Variation in the intracellular polypeptide profiles from different isolates of bovine virus diarrhoea virus. Arch. Virol. 94:43-53[CrossRef][Medline].

20. Qi, F., J. F. Ridpath, and E. S. Berry. 1998. Insertion of a bovine SMT3B gene in NS4B and duplication of NS3 in a bovine viral diarrhea virus genome correlate with the cytopathogenicity of the virus. Virus Res. 57:1-9[CrossRef][Medline].

21. Qi, F., J. F. Ridpath, T. Lewis, S. R. Bolin, and E. S. Berry. 1992. Analysis of the bovine viral diarrhea virus genome for possible cellular insertions. Virology 189:285-292[CrossRef][Medline].

22. Ridpath, J. F., and S. R. Bolin. 1997. Comparison of the complete genomic sequence of the border disease virus, BD31, to other pestiviruses. Virus Res. 50:237-243[CrossRef][Medline].

23. Ridpath, J. F., and S. R. Bolin. 1995. Delayed onset postvaccinal mucosal disease as a result of genetic recombination between genotype 1 and genotype 2 BVDV. Virology 212:259-262[CrossRef][Medline].

24. Ridpath, J. F., and S. R. Bolin. 1998. Differentiation of types 1a, 1b and 2 bovine viral diarrhoea virus (BVDV) by PCR. Mol. Cell Probes 12:101-106[CrossRef][Medline].

25. Ridpath, J. F., and S. R. Bolin. 1990. Viral protein production in homogeneous and mixed infections of cytopathic and noncytopathic BVD virus. Arch. Virol. 111:247-256[Medline].

26. Ridpath, J. F., S. R. Bolin, and E. J. Dubovi. 1994. Segregation of bovine viral diarrhea virus into genotypes. Virology 205:66-74[CrossRef][Medline].

27. Tautz, N., G. Meyers, R. Stark, E. J. Dubovi, and H. J. Thiel. 1996. Cytopathogenicity of a pestivirus correlates with a 27-nucleotide insertion. J. Virol. 70:7851-7858[Abstract].

28. Tautz, N., G. Meyers, and H. J. Thiel. 1993. Processing of poly-ubiquitin in the polyprotein of an RNA virus. Virology 197:74-85[CrossRef][Medline].

29. Wengler, G., D. Bradley, and M. Collett. 1995. Family Flaviviridae, p. 415-427. In F. Murphy, C. Fauquet, and D. Bishop (ed.), Virus taxonomy, 6th ed. Springer-Verlag, New York, N.Y.

Journal of Virology, September 2000, p. 8771-8774, Vol. 74, No. 18
0022-538X/00/$04.00+0

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1.	Becher, P., G. Meyers, A. D. Shannon, and H. J. Thiel. 1996. Cytopathogenicity of border disease virus is correlated with integration of cellular sequences into the viral genome. J. Virol. 70:2992-2998[Abstract].
2.	Becher, P., M. Orlich, M. König, and H. J. Thiel. 1999. Nonhomologous RNA recombination in bovine viral diarrhea virus: molecular characterization of a variety of subgenomic RNAs isolated during an outbreak of fatal mucosal disease. J. Virol. 73:5646-5653[Abstract/Free Full Text].
3.	Becher, P., M. Orlich, and H. J. Thiel. 1998. Ribosomal S27a coding sequences upstream of ubiquitin coding sequences in the genome of a pestivirus. J. Virol. 72:8697-8704[Abstract/Free Full Text].
4.	Collett, M. S., R. Larson, S. K. Belzer, and E. Retzel. 1988. Proteins encoded by bovine viral diarrhea virus: the genomic organization of a pestivirus. Virology 165:200-208[CrossRef][Medline].
5.	Donis, R. O., and E. J. Dubovi. 1987. Differences in virus-induced polypeptides in cells infected by cytopathic and noncytopathic biotypes of bovine virus diarrhea-mucosal disease virus. Virology 158:168-173[CrossRef][Medline].
6.	Gillespie, J., J. Baker, and K. McEntee. 1960. A cytopathogenic strain of virus diarrhea virus. Cornell Vet. 50:73-79[Medline].
7.	Greiser-Wilke, I., K. E. Dittmar, B. Liess, and V. Moennig. 1992. Heterogeneous expression of the non-structural protein p80/p125 in cells infected with different pestiviruses. J. Gen. Virol. 73:47-52[Abstract/Free Full Text].
8.	Greiser-Wilke, I., L. Haas, K. Dittmar, B. Liess, and V. Moennig. 1993. RNA insertions and gene duplications in the nonstructural protein p125 region of pestivirus strains and isolates in vitro and in vivo. Virology 193:977-980[CrossRef][Medline].
9.	Kümmerer, B. M., D. Stoll, and G. Meyers. 1998. Bovine viral diarrhea virus strain Oregon: a novel mechanism for processing of NS2-3 based on point mutations. J. Virol. 72:4127-4138[Abstract/Free Full Text].
10.	Kupfermann, H., H. J. Thiel, E. J. Dubovi, and G. Meyers. 1996. Bovine viral diarrhea virus: characterization of a cytopathogenic defective interfering particle with two internal deletions. J. Virol. 70:8175-8181[Abstract].
11.	Lee, K., and J. Gillespie. 1957. Propagation of virus diarrhea virus of cattle in tissue culture. Am. J. Vet. Res. 18:952-955[Medline].
12.	Meyers, G., T. Rumenapf, N. Tautz, E. J. Dubovi, and H. J. Thiel. 1991. Insertion of cellular sequences in the genome of bovine viral diarrhea virus. Arch. Virol. Suppl. 3:133-142[Medline].
13.	Meyers, G., D. Stoll, and M. Gunn. 1998. Insertion of a sequence encoding light chain 3 of microtubule-associated proteins 1A and 1B in a pestivirus genome: connection with virus cytopathogenicity and induction of lethal disease in cattle. J. Virol. 72:4139-4148[Abstract/Free Full Text].
14.	Meyers, G., N. Tautz, E. J. Dubovi, and H. J. Thiel. 1991. Viral cytopathogenicity correlated with integration of ubiquitin-coding sequences. Virology 180:602-616[CrossRef][Medline].
15.	Meyers, G., and H. J. Thiel. 1995. Cytopathogenicity of classical swine fever virus caused by defective interfering particles. J. Virol. 69:3683-3689[Abstract].
16.	Meyers, G., and H. J. Thiel. 1996. Molecular characterization of pestiviruses. Adv. Virus Res. 47:53-118[Medline].
17.	Neill, J. D., and W. L. Mengeling. 1988. Further characterization of the virus-specific RNAs in feline calicivirus infected cells. Virus Res. 11:59-72[Medline].
18.	Pellerin, C., J. van den Hurk, J. Lecomte, and P. Tussen. 1994. Identification of a new group of bovine viral diarrhea virus strains associated with severe outbreaks and high mortalities. Virology 203:260-268[CrossRef][Medline].
19.	Pocock, D. H., C. J. Howard, M. C. Clarke, and J. Brownlie. 1987. Variation in the intracellular polypeptide profiles from different isolates of bovine virus diarrhoea virus. Arch. Virol. 94:43-53[CrossRef][Medline].
20.	Qi, F., J. F. Ridpath, and E. S. Berry. 1998. Insertion of a bovine SMT3B gene in NS4B and duplication of NS3 in a bovine viral diarrhea virus genome correlate with the cytopathogenicity of the virus. Virus Res. 57:1-9[CrossRef][Medline].
21.	Qi, F., J. F. Ridpath, T. Lewis, S. R. Bolin, and E. S. Berry. 1992. Analysis of the bovine viral diarrhea virus genome for possible cellular insertions. Virology 189:285-292[CrossRef][Medline].
22.	Ridpath, J. F., and S. R. Bolin. 1997. Comparison of the complete genomic sequence of the border disease virus, BD31, to other pestiviruses. Virus Res. 50:237-243[CrossRef][Medline].
23.	Ridpath, J. F., and S. R. Bolin. 1995. Delayed onset postvaccinal mucosal disease as a result of genetic recombination between genotype 1 and genotype 2 BVDV. Virology 212:259-262[CrossRef][Medline].
24.	Ridpath, J. F., and S. R. Bolin. 1998. Differentiation of types 1a, 1b and 2 bovine viral diarrhoea virus (BVDV) by PCR. Mol. Cell Probes 12:101-106[CrossRef][Medline].
25.	Ridpath, J. F., and S. R. Bolin. 1990. Viral protein production in homogeneous and mixed infections of cytopathic and noncytopathic BVD virus. Arch. Virol. 111:247-256[Medline].
26.	Ridpath, J. F., S. R. Bolin, and E. J. Dubovi. 1994. Segregation of bovine viral diarrhea virus into genotypes. Virology 205:66-74[CrossRef][Medline].
27.	Tautz, N., G. Meyers, R. Stark, E. J. Dubovi, and H. J. Thiel. 1996. Cytopathogenicity of a pestivirus correlates with a 27-nucleotide insertion. J. Virol. 70:7851-7858[Abstract].
28.	Tautz, N., G. Meyers, and H. J. Thiel. 1993. Processing of poly-ubiquitin in the polyprotein of an RNA virus. Virology 197:74-85[CrossRef][Medline].
29.	Wengler, G., D. Bradley, and M. Collett. 1995. Family Flaviviridae, p. 415-427. In F. Murphy, C. Fauquet, and D. Bishop (ed.), Virus taxonomy, 6th ed. Springer-Verlag, New York, N.Y.