Showing total 9 results

1. Validation of an automated ELISA system for detection of antibodies to Aleutian mink disease virus using blood samples collected in filter paper strips

Author

Ian A. Gardner, Anna-Maija Virtala, Pirjo Aronen, Majvor Eerola, Olli Vapalahti, Anna Knuuttila, Haartman Institute (-2014), Veterinary Biosciences, Department of Virology, Departments of Faculty of Veterinary Medicine, Viral Zoonosis Research Unit, DAPHNE - Developing Assessment Practices in Higher Education, and Teachers' Academy

Subjects

Male, ERADICATION, ACCURACY, education, Bayesian analysis, Aleutian Mink Disease, Counter-current immunoelectrophoresis, Enzyme-Linked Immunosorbent Assay, Immunoelectrophoresis, Carnivore amdoparvovirus 1, 413 Veterinary science, Antibodies, Viral, Sensitivity and Specificity, Sensitivity, Seroepidemiologic Studies, COUNTERIMMUNOELECTROPHORESIS, Virology, biology.animal, INFECTION, COUNTER CURRENT IMMUNOELECTROPHORESIS, medicine, Aleutian Mink Disease Virus, Animals, Mink, Aleutian disease, LINKED-IMMUNOSORBENT-ASSAY, biology, medicine.diagnostic_test, Research, Reproducibility of Results, medicine.disease, 3. Good health, Infectious Diseases, biology.protein, Specificity, Female, Antibody, Counterimmunoelectrophoresis, Immune complex disease, Blood sampling

Abstract

Background: Aleutian mink disease virus (AMDV) is the cause of a chronic immune complex disease, Aleutian disease (AD), which is common in mink-producing countries. In 2005, implementation of an AMDV eradication programme in Finland created a need for an automated high-throughput assay. The aim of this study was to validate an AMDV-VP2 -recombinant antigen ELISA, which we developed earlier, in an automated assay format for the detection of anti-AMDV antibodies in mink blood and to determine the accuracy of this test compared with the reference standard (counter-current immunoelectrophoresis, CIEP). Methods: A blood sampling method based on filter paper 12-strips (blood combs) and a device to introduce these strips to an ELISA plate for elution of the samples were developed. Blood and serum samples were collected from 761 mink from two farms with low (2%) and high (81%) seroprevalences of AMDV infection in 2008. ELISA sensitivity and specificity were estimated with a Bayesian 2-test 2-population model that allowed for conditional dependence between CIEP and ELISA. Agreement between the two tests was assessed with kappa statistic and proportion agreement. Results: The sensitivity and specificity of the automated ELISA system were estimated to be 96.2% and 98.4%, respectively. Agreement between CIEP and ELISA was high, with a kappa value of 0.976 and overall proportion agreement of 98.8%. Conclusions: The automated ELISA system combined with blood comb sampling is an accurate test format for the detection of anti-AMDV antibodies in mink blood and offers several advantages, including improved blood sampling and data handling, fast sample throughput time, and reductions in costs and labour inputs.

Published

2014

2. The dose of HBV genome contained plasmid has a great impact on HBV persistence in hydrodynamic injection mouse model

Author

Jingjiao Song, Di Zhou, Lei Li, Lu Yang, Yun Zhou, Dongliang Yang, Sheng Li, Yan Yang, and Mengji Lu

Subjects

0301 basic medicine, Male, HBsAg, HBV persistence, Hepatitis B virus, Medizin, Genome, Viral, Biology, Hydrodynamic injection, medicine.disease_cause, lcsh:Infectious and parasitic diseases, 03 medical and health sciences, Mice, 0302 clinical medicine, Plasmid, Immune system, Liver Function Tests, In vivo, Virology, HBV mouse model, medicine, Animals, Humans, lcsh:RC109-216, The doses of HBV plasmid, Antigens, Viral, Research, virus diseases, Viral Load, Hepatitis B, Molecular biology, Immunohistochemistry, digestive system diseases, HBcAg, Disease Models, Animal, 030104 developmental biology, Infectious Diseases, HBeAg, DNA, Viral, 030211 gastroenterology & hepatology, Tumor necrosis factor alpha, Biomarkers, Plasmids

Abstract

Background Hydrodynamic injection (HI) of hepatitis B virus (HBV) mouse model is an useful tool for HBV related research in vivo. However, only 40% of C57/BL6 mice injected with 10 μg HBV genome contained plasmid (pAAV-HBV1.2), serum HBsAg more than 6 months and none of the BALB/c mice injected with 10 μg pAAV-HBV1.2 plasmid DNA, serum HBsAg positive more than 4 weeks in the previous study. Methods In this study, C57/BL6 and BALB/c mice were hydrodynamic injected with different doses of pAAV-HBV1.2 plasmid DNA. HBV related serum markers were detected by ELISA. ALT levels in the serum were measured using full automated biochemistry analyzer. HBcAg positive cells in the liver were detected by immunohistochemical staining. The mRNA levels of IRF3, ISGs including ISG15, OAS, PKR and immune factors including IFNγ, TNFα, TGFβ, IL-6, IL-10, PDL1 in liver of the mice were quantified by qRT-PCR. Results The results showed that the mice injected with 100 μg high-concentration or 1 μg low-concentration of pAAV-HBV1.2 plasmid DNA did not excert dominant influence on HBV persistence. In contrast, injection of 5 μg intermediate-dose of pAAV-HBV1.2 plasmid DNA led to significant prolonged HBsAg expression and HBV persistence in both C57/BL6 (80% of the mice with HBsAg positive more than 6 months) and BALB/c (60% of the mice with HBsAg positive more than 3 months) mice. IFNγ was significant up-regulated in liver of the mice injected with 1 μg or 100 μg pAAV-HBV1.2 plasmid DNA. TNFα was up-regulated significantly in liver of the mice injected with 100 μg pAAV-HBV1.2 plasmid DNA. Moreover, PDL1 was significant up-regulated in liver of the mice injected with 5 μg pAAV-HBV1.2 plasmid DNA. Conclusion In this paper we demonstrated that, in the HBV HI mouse model, the concentration of injected pAAV-HBV1.2 plasmid DNA contributes to the diverse kinetics of HBsAg and HBeAg in the serum as well as HBcAg expression level in the liver, which then determined the HBV persisternce, while the antiviral factors IFNγ, TNFα as well as immune negative regulatory factor PDL1 play important roles on HBV persistence.

Published

2017

3. The transcription map of HPV11 in U2OS cells adequately reflects the initial and stable replication phases of the viral genome

Author

Ene Ustav, Andres Männik, Helen Isok-Paas, and Mart Ustav

Subjects

DNA Replication, Gene Expression Regulation, Viral, HPV, Transcription, Genetic, Genome replication, Genome, Viral, Biology, Virus Replication, Genome, HPV11, Viral Proteins, Plasmid, Transcription (biology), Virology, Cell Line, Tumor, Gene expression, Coding region, Humans, Promoter Regions, Genetic, Genetics, Human papillomavirus 11, Research, Papillomavirus Infections, DNA replication, Promoter, Papillomavirus, Squamous carcinoma, Infectious Diseases, Transcriptome

Abstract

Background Although prophylactic vaccines have been developed against HPV6, HPV11, HPV16 and HPV18 there is the clear unmet medical need in order to justify the development of drugs targeting human papillomavirus replication. The native host cells of HPVs are human primary keratinocytes which can be cultivated in raft cultures. However, this method is difficult to use in high-throughput screening assays and the need for a cost-effective cellular system for screening potential anti-HPV drug candidates during all stages of HPV genome replication remains. Methods U2OS cells were transfected with HPV11 wt or E8- minicircle genomes and their gene expression was studied via 3′ RACE, 5′ RACE or via real time PCR methods. The DNA replication of these genomes was detected by Southern blot methods. Results The analysis of HPV11 transcripts in U2OS cells showed that the patterns of promoter use, splice sites and polyadenylation cleavage sites are identical to those previously characterized in human HPV-related lesions, human squamous carcinoma cell lines (e.g., SSC-4) and laryngeal papillomas. Transcriptional initiation from the three previously described HPV11 promoters in the E6 and E7 ORFs (P90, P264, and P674-714) were functional, and these promoters were used together with two promoter regions in the E1 ORF (P1092 and P1372). Mutating the E8 ORF ATG start codon to ACG eliminated the translation of fusion proteins from the E8 ORF coupled to E1 and E2 proteins C-terminal sequences, leading to the de-repression of gene expression (particularly from the P1092 promoter) and to the activation of genome replication. These data suggested that the expression of the functional E8^E2 protein is used to control viral gene expression and copy number of the HPV11 genome. The analysis of HPV11 E1 expression plasmids showed that the E6/E7 region, together with the E1 coding region, is crucial for the production of functionally active E1 protein. Conclusions The data presented in this paper suggest that in human osteosarcoma cell line U2OS the gene expression pattern of the HPV11 truly reflect the expression profile of the replicating HPV genome and therefore this cellular system is suitable for drug development program targeting HPV replication.

Published

2015

4. Development of a reverse genetics system for respiratory syncytial virus long strain and an immunogenicity study of the recombinant virus

Author

Zhizheng Fang, Xuhua Guan, Bing Hu, Jianbo Zhan, Jiawei Jiang, Yongzhong Jiang, Guoming Li, and Yuanding Chen

Subjects

Genetic Vectors, Gene Expression, Respiratory Syncytial Virus Infections, Viral Plaque Assay, CD8-Positive T-Lymphocytes, Recombinant virus, Antibodies, Viral, Virus Replication, Virus, Microbiology, Mice, Immune system, Attenuated vaccine candidates, Genes, Reporter, T-Lymphocyte Subsets, Virology, Respiratory Syncytial Virus Vaccines, Animals, Humans, Neutralizing antibody, Immunity, Cellular, Mice, Inbred BALB C, Protection, biology, Immunogenicity, Research, Hep G2 Cells, Reverse Genetics, Disease Models, Animal, Infectious Diseases, Viral replication, Immunoglobulin G, Respiratory Syncytial Virus, Human, biology.protein, Antibody, Genetic Engineering, Respiratory syncytial virus (RSV) Long strain

Abstract

Background Respiratory Syncytial Virus (RSV) is an important human respiratory pathogen, particularly of infants and older adults, and despite several decades of research and development, no licensed vaccine is available. Studies have confirmed that enhancement of RSV disease does not occur after inoculation with RSV live-attenuated vaccine candidates, making such vaccines preferable. In this paper, reverse genetics was used to construct two recombinant viruses, a recombinant Long strain (rLong) and rLong-∆G-EGFP; rLong-∆G-EGFP is a recombinant mutant in which G was replaced with the EGFP gene, based on the Long strain of RSV. Results Both rLong and rLong-∆G-EGFP were constructed successfully and recovered in Hep-2 cells, and autofluorescence was observed in rLong-∆G-EGFP-infected cells during consecutive passages. Titers of rLong and rLong-∆G-EGFP were ~100-fold lower than the parental strain. Although virulence was attenuated, high titers of neutralizing antibodies were induced in BALB/c mice after being inoculated with recombinant viruses in a three-dose schedule. Unexpectedly, the neutralizing antibody titer in rLong-∆G-EGFP-immunized recipients did not decline significantly compared with the rLong strain. Protective efficacy of recombinant viruses in lung tissue was up to 100%, and the serum neutralizing antibody levels could stabilize at 21 days with no significant fall post-challenge. Enzyme-linked immunospot (ELISPOT) assays showed that both recombinant viruses were capable of inducing CD8+ T cell immune responses, which are crucial for virus clearance, and that rLong stimulated a higher level of IFN-γ production by comparison. In terms of inducing a balanced immune response, rLong-∆G-EGFP elicited slightly higher levels of IgG2a antibodies and lower levels of IgG1/IgG2a than the rLong virus. Conclusions This study suggested that immunization with rLong and rLong-∆G-EGFP were immunogenic and protected against RSV infection in the lower respiratory tract of BALB/c mice better than in the nose. Because of a relative low IgG1/IgG2a ratio, rLong-∆G-EGFP was more inclined to make CD4+ T cells, shifting toward a Th1-type response, indicating that the generation of a more balanced Th1/Th2 response was desirable. This explorative study on the recombinant Long viruses also contributed to obtaining more RSV attenuated candidates by a reverse genetics approach.

Published

2014

5. Serosurvey of veterinary conference participants for evidence of zoonotic exposure to canine norovirus – study protocol

Author

João R. Mesquita and Maria São José Nascimento

Subjects

Veterinary medicine, Canine norovirus, viruses, medicine.disease_cause, Antibodies, Viral, Study Protocol, Zoonosis, fluids and secretions, Clinical Protocols, Seroepidemiologic Studies, Surveys and Questionnaires, Zoonoses, Dog Diseases, Caliciviridae Infections, 0303 health sciences, education.field_of_study, Transmission (medicine), virus diseases, Occupational exposure, 3. Good health, Infectious Diseases, Public Health, medicine.medical_specialty, Population, Enzyme-Linked Immunosorbent Assay, lcsh:Infectious and parasitic diseases, Veterinarians, 03 medical and health sciences, Dogs, Virology, medicine, Animals, Humans, lcsh:RC109-216, education, Close contact, 030304 developmental biology, Portugal, 030306 microbiology, business.industry, Public health, Norovirus, Outbreak, Congresses as Topic, medicine.disease, digestive system diseases, Risk factors, Case-Control Studies, business

Abstract

Background Noroviruses have emerged as the leading cause of outbreaks and sporadic cases of acute gastroenteritis in humans worldwide. Person-to-person contact and consumption of contaminated food are considered the most important ways of transmission of noroviruses however zoonotic transmission has been suggested. Recently, noroviruses have been found in dogs which, unlike bovine and swine noroviruses, may present a higher risk of zoonotic transfer, given to the often close contacts between humans and pet dogs in many societies across the world. The present paper describes a seroepidemiologic study aiming to provide information on the exposure level of humans to canine norovirus. Methods/Design A case–control study was designed to address the potential exposure to canine norovirus based on the presence of antibodies against canine norovirus. Sera from veterinarians (a population repeatedly in close contact with dogs) will be collected in an annual Veterinary Sciences Congress in Portugal. In addition, sera from general population will be obtained and used as controls for comparative purposes. All sera will be tested for the presence of canine norovirus antibodies using a virus-like particle-based enzyme immune assay. Risk factors for canine norovirus antibodies presence in veterinarians will be investigated through the delivery of an anonymized questionnaire to the participants. Discussion The present study aims to identify seropositive individuals to canine norovirus and to assess risk profiles among veterinary professionals with occupational exposure to dogs. To our knowledge this is the first study providing information on the potential zoonotic risk of canine norovirus, thus allowing the development of preventive measures and ascertaining potential risks for Public Health resulting from contact to dogs.

Published

2012

6. Establishment of real-time quantitative reverse transcription polymerase chain reaction assay for transcriptional analysis of duck enteritis virus UL55 gene

Author

Shunchuan Zhang, Dekang Zhu, Xiaoyue Chen, Ying Wu, Renyong Jia, Mingshu Wang, Zhengli Chen, Qihui Luo, and Anchun Cheng

Subjects

Molecular Sequence Data, Biology, Melting curve analysis, law.invention, lcsh:Infectious and parasitic diseases, chemistry.chemical_compound, Viral Proteins, law, Transcription (biology), Virology, Animals, lcsh:RC109-216, Gene, Cells, Cultured, DNA Primers, Reverse Transcriptase Polymerase Chain Reaction, Research, Gene Expression Profiling, Sequence Analysis, DNA, Fibroblasts, Reference Standards, Molecular biology, Actins, Reverse transcription polymerase chain reaction, Gene expression profiling, Mardivirus, Infectious Diseases, Ducks, chemistry, Agarose gel electrophoresis, DNA, Viral, Recombinant DNA, DNA

Abstract

Background Real-time quantitative reverse transcription polymerase chain reaction assay (qRT-PCR) has become the benchmark for detection and quantification of target gene expression level and been utilized increasingly in detection of viral load and therapy monitoring. The dynamic transcription variation of duck enteritis virus UL55 gene during the life cycle of duck enteritis virus in infected cells has not been reported yet. Results The newly identified duck enteritis virus UL55 gene was amplified and cloned into pMD18-T vector after digestion to generate a recombinant plasmid pMD18-T/UL55 for the establishment of qRT-PCR as standard DNA. The results of agarose gel electrophoresis and melting curve analysis demonstrated the primers we designed for qRT-PCR were specific and available. We used β-actin as a reference gene for normalization and established two standard curves based on pMD18-T/UL55 and pMD18-T/β-actin successfully. Based on that, the transcriptional analysis of DEV UL55 gene was performed, and the result suggested the expression of UL55 mRNA was at a low level from 0 to 8 h post-infection(p.i.), then accumulated quickly since 12 h p.i. and peaked at 36 h p.i., it can be detected till 60 h p.i.. Nucleic acid inhibition test was carried out for analyzing a temporal regulation condition of DEV UL55 gene, result revealed that it was sensitive to ganciclovir. Synthesis procedures of DEV UL55 gene can be inhibited by ganciclovir. Conclusions The method we established in this paper can provide quantitative values reflecting the amounts of measured mRNA in samples. It's available for detection and quantification, also can be used in DEV diagnosis. The DEV UL55 gene was produced most abundantly during the late phase of replication in DEV-infected cells and the transcription of it depended on the synthesized DNA. DEV UL55 gene is a γ2 gene which occurs last and have a strict requirement for viral DNA synthesis.

Published

2011

7. Identification of the 3' and 5' terminal sequences of the 8 rna genome segments of european and north american genotypes of infectious salmon anemia virus (an orthomyxovirus) and evidence for quasispecies based on the non-coding sequences of transcripts

Author

Kira Salonius, Angela Riveroll, Frederick S. B. Kibenge, Molly J. T. Kibenge, Nathalie Simard, and Vikas Kulshreshtha

Subjects

Untranslated region, Polyadenylation, Genotype, Sequence analysis, Isavirus, Salmo salar, Viral quasispecies, Biology, lcsh:Infectious and parasitic diseases, Cell Line, Rapid amplification of cDNA ends, Virology, Consensus sequence, Animals, Cluster Analysis, lcsh:RC109-216, Gene, 3' Untranslated Regions, Phylogeny, Genetics, Polymorphism, Genetic, Research, RNA, Sequence Analysis, DNA, Europe, Infectious Diseases, North America, Nucleic Acid Conformation, RNA, Viral, 5' Untranslated Regions

Abstract

Background Infectious salmon anemia (ISA) virus (ISAV) is a pathogen of marine-farmed Atlantic salmon (Salmo salar); a disease first diagnosed in Norway in 1984. This virus, which was first characterized following its isolation in cell culture in 1995, belongs to the family Orthomyxoviridae, genus, Isavirus. The Isavirus genome consists of eight single-stranded RNA segments of negative sense, each with one to three open reading frames flanked by 3' and 5' non-coding regions (NCRs). Although the terminal sequences of other members of the family Orthomyxoviridae such as Influenzavirus A have been extensively analyzed, those of Isavirus remain largely unknown, and the few reported are from different ISAV strains and on different ends of the different RNA segments. This paper describes a comprehensive analysis of the 3' and 5' end sequences of the eight RNA segments of ISAV of both European and North American genotypes, and evidence of quasispecies of ISAV based on sequence variation in the untranslated regions (UTRs) of transcripts. Results Two different ISAV strains and two different RNA preparations were used in this study. ISAV strain ADL-PM 3205 ISAV-07 (ADL-ISAV-07) of European genotype was the source of total RNA extracted from ISAV-infected TO cells, which contained both viral mRNA and cRNA. ISAV strain NBISA01 of North American genotype was the source of vRNA extracted from purified virus. The NCRs of each segment were identified by sequencing cDNA prepared by three different methods, 5' RACE (Rapid amplification of cDNA ends), 3' RACE, and RNA ligation mediated PCR. Sequence analysis of five clones each derived from one RT-PCR product from each NCR of ISAV transcripts of segments 1 to 8 revealed significant heterogeneity among the clones of the same segment end, providing unequivocal evidence for presence of intra-segment ISAV quasispecies. Both RNA preparations (mRNA/cRNA and vRNA) yielded complementary sequence information, allowing the simultaneous identification and confirmation of the 3' and 5' NCR sequences of the 8 RNA genome segments of both genotypes of ISAV. The 3' sequences of the mRNA transcripts of ADL-ISAV-07 terminated 13-18 nucleotides from the full 3' terminus of cRNA, continuing as a poly(A) tail, which corresponded with the location of the polyadenylation signal. The lengths of the 3' and 5' NCRs of the vRNA were variable in the different genome segments, but the terminal 7 and 11 nucleotides of the 3' and 5' ends, respectively, were highly conserved among the eight genomic segments of ISAV. The first three nucleotides at the 3' end are GCU-3' (except in segment 5 with ACU-3'), whereas at the 5' end are 5'-AGU with the polyadenylation signal of 3-5 uridines 13-15 nucleotides downstream of the 5' end terminus of the vRNA. Exactly the same features were found in the respective complementary 5' and 3' end NCR sequences of the cRNA transcripts of ADL-ISAV-07, indicating that the terminal sequences of the 8 RNA genome segments are highly conserved among the two ISAV genotypes. The 5' NCR sequences of segments 1, 2, 3, 5, and 7, and the 3' NCR sequences of segments 3 and 4 cRNA were 100% identical in the two genotypes, and the 3' NCR sequences of segment 5 cRNA was the most divergent, with a sequence identity of 77.2%. Conclusions We report for the first time, the presence of intra-segment ISAV quasispecies, based on sequence variation in the NCR sequences of transcripts. In addition, this is the first report of a comprehensive unambiguous analysis of the 3' and 5' NCR sequences of all 8 RNA genome segments from two strains of ISAV representing the two genotypes of ISAV. Because most ISAV sequences are of cDNA to mRNA, they do not contain the 3' end sequences, which are removed during polyadenylation of the mRNA transcripts. We report for the first time the ISAV consensus sequence CAT/ATTTTTACT-3' (in the message sense 5'-3') in all segments of both ISAV genotypes.

Published

2010

8. What happened after the initial global spread of pandemic human influenza virus A (H1N1)? A population genetics approach

Author

Gilberto Vaughan, Diego Emiliano Jimenez-Gonzalez, Ana Flisser, Fernando Martínez-Hernández, Arony Martinez-Flores, Guiehdani Villalobos-Castillejos, Pablo Maravilla, Simon Kawa-Karasik, and Mirza Romero-Valdovinos

Subjects

Short Report, Hemagglutinins, Viral, Neuraminidase, medicine.disease_cause, H5N1 genetic structure, Virus, lcsh:Infectious and parasitic diseases, Evolution, Molecular, Viral Proteins, Influenza A Virus, H1N1 Subtype, Virology, Pandemic, Influenza, Human, medicine, Humans, lcsh:RC109-216, Genetic variability, Pandemics, Molecular Epidemiology, biology, Population size, Computational Biology, Influenza A virus subtype H5N1, Infectious Diseases, Communicable Disease Control, biology.protein, Human mortality from H5N1, Databases, Nucleic Acid

Abstract

Viral population evolution dynamics of influenza A is crucial for surveillance and control. In this paper we analyzed viral genetic features during the recent pandemic caused by the new influenza human virus A H1N1, using a conventional population genetics approach based on 4689 hemagglutinin (HA) and neuraminidase (NA) sequences available in GenBank submitted between March and December of 2009. This analysis showed several relevant aspects: a) a scarce initial genetic variability within the viral isolates from some countries that increased along 2009 when influenza was dispersed around the world; b) a worldwide virus polarized behavior identified when comparing paired countries, low differentiation and high gene flow were found in some pairs and high differentiation and moderate or scarce gene flow in others, independently of their geographical closeness, c) lack of positive selection in HA and NA due to increase of the population size of virus variants, d) HA and NA variants spread in a few months all over the world being identified in the same countries in different months along 2009, and e) containment of viral variants in Mexico at the beginning of the outbreak, probably due to the control measures applied by the government.

Published

2010

9. The biennial cycle of respiratory syncytial virus outbreaks in Croatia

Author

Vlatka Tomić, Ivana Galinović, Vladimir Drazenovic, Robert C. Welliver, Sunčanica Ljubin-Sternak, Tatjana Vilibić-Čavlek, and Gordana Mlinarić-Galinović

Subjects

Urban Population, Croatia, Virus isolation, viruses, Short Report, Viral antigen, Respiratory Syncytial Virus Infections, Biology, Virus, lcsh:Infectious and parasitic diseases, Disease Outbreaks, Virology, Nasopharynx, Humans, lcsh:RC109-216, Respiratory system, Child, Acute respiratory tract infection, Antigens, Viral, Respiratory tract infections, Outbreak, Infant, Infectious Diseases, Child, Preschool, Respiratory Syncytial Virus, Human, Immunology, Seasons, respiratory syncytial virus, biennial cycle, Nasopharyngeal secretion

Abstract

The paper analyses the epidemic pattern of respiratory syncytial virus (RSV) outbreaks in children in Croatia. Over a period of 11 consecutive winter seasons (1994–2005) 3,435 inpatients from Zagreb County aged from infancy to 10 years who were hospitalised with acute respiratory tract infections were tested for RSV-infection. RSV was identified in nasopharyngeal secretions of patients by virus isolation in cell culture and by detection of viral antigen with monoclonal antibodies. In the Zagreb area, RSV outbreaks were proven to vary in a two-year cycle, which was repeated every 23–25 months. This biennial cycle comprised one larger and one smaller season. Climate factors correlated significantly with the number of RSV cases identified only in the large seasons, which suggests that the biennial cycle is likely to continue regardless of meteorological conditions. Knowledge of this biennial pattern should be useful in predicting the onset of RSV outbreaks in Croatia, and would facilitate planning for the prevention and control of RSV infections in the region.

Published

2008