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70. Parvovirus B19 infection and severe anaemia in Kenyan children: a retrospective case control study

Author

Tuju James, Gicheru Nimmo, Peshu Norbert, Cossart Yvonne, Wildig James, Williams Thomas N, and Newton Charles R

Subjects
Infectious and parasitic diseases, RC109-216
Abstract

Abstract Background During acute Human parvovirus B19 (B19) infection a transient reduction in blood haemoglobin concentration is induced, due to a 5-7 day cessation of red cell production. This can precipitate severe anaemia in subjects with a range of pre-existing conditions. Of the disease markers that occur during B19 infection, high IgM levels occur closest in time to the maximum reduction in haemoglobin concentration. Previous studies of the contribution of B19 to severe anaemia among young children in Africa have yielded varied results. This retrospective case/control study seeks to ascertain the proportion of severe anaemia cases precipitated by B19 among young children admitted to a Kenyan district hospital. Methods Archival blood samples from 264 children under 6 years with severe anaemia admitted to a Kenyan District Hospital, between 1999 and 2004, and 264 matched controls, were tested for B19 IgM by Enzyme Immunosorbent Assay and 198 of these pairs were tested for B19 DNA by PCR. 536 samples were also tested for the presence of B19 IgG. Results 7 (2.7%) cases and 0 (0%) controls had high B19 IgM levels (Optical Density > 5 × cut-off value) (McNemar's exact test p = 0.01563), indicating a significant association with severe anaemia. The majority of strongly IgM positive cases occurred in 2003. 10/264 (3.7%) cases compared to 5/264 (1.9%) controls tested positive for B19 IgM. This difference was not statistically significant, odds ratio (OR) = 2.00 (CI95 [0.62, 6.06], McNemar's exact test p = 0.3018. There was no significant difference between cases and controls in the B19 IgG (35 (14.8%) vs 32 (13.6%)), OR = 1.103 (CI95 [0.66, 1.89], McNemar's exact test, p = 0.7982), or the detection of the B19 DNA (6 (3.0%) vs 5 (2.5%)), OR = 1.2 (CI95 [0.33, 4.01], McNemar's exact test p = 1). Conclusions High B19 IgM levels were significantly associated with severe anaemia, being found only among the cases. This suggests that 7/264 (2.7%) of cases of severe anaemia in the population of children admitted to KDH were precipitated by B19. While this is a relatively small proportion, this has to be evaluated in the light of the IgG data that shows that less than 15% of children in the study were exposed to B19, a figure much lower than reported in other tropical areas.

Published
2010
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72. TTV a common virus, but pathogenic?

Author

Cossart, Yvonne and Cossart, Y

Subjects
*NOSOLOGY, *INFECTIOUS disease transmission, *BLOOD transfusion, *DNA viruses, *VIRAL hepatitis
Abstract

Commentary. Discusses a paper by Peter Simmonds, et al, which was published in the July 18, 1998 issue of `The Lancet.' Aspects of the transfusion-transmittable virus known as TTV; The pathogenic role of TTV; Suggestion that TTV may be a parvovirus; The strong circumstantial evidence of transmission of TTV by transfusion; Effects of the discovery of TTV.

Published
1998
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73. A STUDY OF HUMAN PAPILLOMAVIRUS TYPE 16 INVOLVEMENT IN CERVICAL CARCINOMAS 1920-1990.

Author

Rose, B., Thompson, C., Flampoulidou, M., Grace, J., and Cossart, Y.

Subjects
CERVICAL cancer
Abstract

Presents an abstract of the article "A Study of Human Papillomavirus Type 16 Involvement in Cervical Carcinomas 1920-1990," by B. Rose, C. Thompson, M. Flampoulidou, J. Grace and Y. Cossart, published in the December 2, 1990 issue of the journal "Immunology & Cell Biology."

Published
1990

79. Parvovirus B19 infection and severe anaemia in Kenyan children: a retrospective case control study.

Author

Wildig J, Cossart Y, Peshu N, Gicheru N, Tuju J, Williams TN, and Newton CR

Subjects
Antibodies, Viral blood, Case-Control Studies, Child, DNA, Viral blood, Enzyme-Linked Immunosorbent Assay, Humans, Immunoglobulin M blood, Kenya epidemiology, Retrospective Studies, Anemia epidemiology, Parvoviridae Infections complications, Parvoviridae Infections virology, Parvovirus B19, Human isolation & purification
Abstract

Background: During acute Human parvovirus B19 (B19) infection a transient reduction in blood haemoglobin concentration is induced, due to a 5-7 day cessation of red cell production. This can precipitate severe anaemia in subjects with a range of pre-existing conditions. Of the disease markers that occur during B19 infection, high IgM levels occur closest in time to the maximum reduction in haemoglobin concentration. Previous studies of the contribution of B19 to severe anaemia among young children in Africa have yielded varied results. This retrospective case/control study seeks to ascertain the proportion of severe anaemia cases precipitated by B19 among young children admitted to a Kenyan district hospital., Methods: Archival blood samples from 264 children under 6 years with severe anaemia admitted to a Kenyan District Hospital, between 1999 and 2004, and 264 matched controls, were tested for B19 IgM by Enzyme Immunosorbent Assay and 198 of these pairs were tested for B19 DNA by PCR. 536 samples were also tested for the presence of B19 IgG., Results: 7 (2.7%) cases and 0 (0%) controls had high B19 IgM levels (Optical Density > 5 x cut-off value) (McNemar's exact test p = 0.01563), indicating a significant association with severe anaemia. The majority of strongly IgM positive cases occurred in 2003.10/264 (3.7%) cases compared to 5/264 (1.9%) controls tested positive for B19 IgM. This difference was not statistically significant, odds ratio (OR) = 2.00 (CI95 [0.62, 6.06], McNemar's exact test p = 0.3018. There was no significant difference between cases and controls in the B19 IgG (35 (14.8%) vs 32 (13.6%)), OR = 1.103 (CI95 [0.66, 1.89], McNemar's exact test, p = 0.7982), or the detection of the B19 DNA (6 (3.0%) vs 5 (2.5%)), OR = 1.2 (CI95 [0.33, 4.01], McNemar's exact test p = 1)., Conclusions: High B19 IgM levels were significantly associated with severe anaemia, being found only among the cases. This suggests that 7/264 (2.7%) of cases of severe anaemia in the population of children admitted to KDH were precipitated by B19. While this is a relatively small proportion, this has to be evaluated in the light of the IgG data that shows that less than 15% of children in the study were exposed to B19, a figure much lower than reported in other tropical areas.

Published
2010
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80. The early host innate immune response to duck hepatitis B virus infection.

Author

Tohidi-Esfahani R, Vickery K, and Cossart Y

Subjects
Age Factors, Animals, Apoptosis, Cells, Cultured, Female, Hepadnaviridae Infections immunology, Hepadnaviridae Infections physiopathology, Hepadnaviridae Infections virology, Hepatitis B Virus, Duck isolation & purification, Hepatitis, Viral, Animal physiopathology, Hepatitis, Viral, Animal virology, Hepatocytes cytology, Hepatocytes immunology, Immunity, Cellular, Immunity, Innate, Lymphocytes immunology, Male, Poultry Diseases physiopathology, Poultry Diseases virology, Ducks, Hepadnaviridae Infections veterinary, Hepatitis B Virus, Duck immunology, Hepatitis, Viral, Animal immunology, Poultry Diseases immunology
Abstract

The early phase after hepatitis B virus infection could play a crucial role in clearance and/or persistence of the virus, particularly in neonates. This work compared the early phase of duck hepatitis B virus infection in 1-day-old (D1) and 28-day-old (D28) ducks to determine whether differences in viral or host innate immune response can be related to the difference in outcome. In the first phase, almost immediately after inoculation, virus was taken up by components of the reticulo-endothelial systems, particularly liver-specific macrophages, Kupffer cells. Very early after infection, the induction of alpha interferon by infected hepatocytes occurred and was rapidly reinforced by recruitment of effector lymphocytes, which directly or indirectly caused apoptosis, eliminating infected hepatocytes, as was seen in mature birds. In addition, a lack of lymphocytic infiltration of the liver was found in D1 ducks, which supports the suggestion that the innate immune network is less effective in D1 ducks. Taken together, these results suggest that failure of the co-ordinated innate immune response rather than a defect in induced antiviral cell-mediated immunity may be the key factor which makes baby ducks vulnerable to persistence of hepadnavirus infection.

Published
2010
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81. Seroprevalence of antibodies to parvovirus B19 among children in Papua New Guinea.

Author

Wildig J, Mueller I, Kiniboro B, Maraga S, Siba P, and Cossart Y

Subjects
Antibodies, Viral blood, Child, Child, Preschool, Hemoglobins analysis, Humans, Immunoenzyme Techniques, Infant, Logistic Models, Multivariate Analysis, Papua New Guinea epidemiology, Parvoviridae Infections virology, Rural Population, Seroepidemiologic Studies, Surveys and Questionnaires, Parvoviridae Infections epidemiology, Parvovirus isolation & purification
Abstract

Parvovirus B19 (B19) is a common childhood infection that has recently been found to be associated with severe anemia in Papua New Guinean children. Population surveys were performed in 15 villages in Maprik district, East Sepik Province, Papua New Guinea in 2005. Plasma samples collected from children less than 10 years of age were tested for IgM and IgG antibodies to B19 by enzyme immunoassay. The prevalence of IgG antibody to B19 was 53.8% and ranged from 20% in those less than one year of age to 85.5% in those nine years of age. Considerable variation in IgG prevalence was observed between study areas, indicating complex patterns of transmission. Prevalence of IgM antibody to B19 was 1.5%. This study confirms that B19 infection is common among children in this tropical area. With 19.5% of children one year of age showing evidence of previous infection, any preventive measures should be targeted at the very young.

Published
2007

82. Human papillomavirus in the oral cavity of patients with and without renal transplantation.

Author

Rose B, Wilkins D, Li W, Tran N, Thompson C, Cossart Y, McGeechan K, O'Brien C, and Eris J

Subjects
Adult, Aged, Aged, 80 and over, DNA, Viral analysis, Female, Humans, Male, Middle Aged, Papillomavirus Infections etiology, Risk Factors, Kidney Transplantation, Mouth virology, Papillomaviridae isolation & purification
Abstract

This study investigates human papillomavirus (HPV) infection in the oral cavities of 88 Australian renal transplant recipients and 88 immunocompetent controls. Oral cavities were examined for lesions and brushings collected for HPV analysis by consensus PCR. No warts were identified; HPV DNA was detected in 18% of transplant versus 1% control samples (P<0.001). Cutaneous HPVs predominated. One patient had HPV16 in samples taken four years apart without evidence of associated lesions or malignancy. Transplant recipients were more likely than controls to have current cutaneous warts (P<0.001), fewer sexual partners (P=0.001), and to have never consumed alcohol (P=0.01). Among the transplant group, the risk of an HPV-positive sample was higher among older patients (P=0.05), and those with past cutaneous warts (P=0.04). This study extends previous surveys by encompassing overt and asymptomatic infection, a broad spectrum of cutaneous and genital HPVs, and by providing new data on risk factors for oral HPV infection.

Published
2006
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83. Parvovirus B19 infection contributes to severe anemia in young children in Papua New Guinea.

Author

Wildig J, Michon P, Siba P, Mellombo M, Ura A, Mueller I, and Cossart Y

Subjects
Aging, Antibodies, Viral blood, Case-Control Studies, Child, Preschool, Female, Humans, Immunoglobulin M blood, Infant, Malaria, Falciparum complications, Male, Odds Ratio, Papua New Guinea, Parvoviridae Infections virology, Anemia complications, Parvoviridae Infections complications, Parvovirus B19, Human
Abstract

Background: Severe anemia (hemoglobin level, <50 g/L) is a major cause of death among young children, and it arises from multiple factors, including malaria and iron deficiency. We sought to determine whether infection with parvovirus B19 (B19), which causes the cessation of erythropoiesis for 3-7 days, might precipitate some cases of severe anemia., Methods: Archival blood samples collected in the Wosera District of Papua New Guinea, from 169 children 6 months-5 years old with severe anemia and from 169 control subjects matched for age, sex, and time were tested for B19 immunoglobulin M (IgM) by enzyme immunoassay and for B19 DNA by nested polymerase chain reaction (PCR). A total of 168 separate samples from children in the Wosera District were tested for B19 IgG., Results: A strong association between acute B19 infection (positive by both IgM and PCR) and severe anemia was found (adjusted odds ratio, 5.61 [95% confidence interval, 1.93-16.3]). The prevalence of parvovirus B19 IgG reached >90% in 6-year-olds., Conclusions: B19 infections play a significant role in the etiology of severe anemia in this area of malarial endemicity. Given the high levels of morbidity and mortality associated with severe anemia in such regions, the prevention of B19 infection with a vaccine might be a highly effective public health intervention.

Published
2006
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84. Removal of biofilm from endoscopes: evaluation of detergent efficiency.

Author

Vickery K, Pajkos A, and Cossart Y

Subjects
Biofilms, Colony Count, Microbial, Equipment Contamination prevention & control, Equipment Reuse, Humans, Infection Control methods, Cross Infection prevention & control, Detergents, Disinfection methods, Endoscopes microbiology, Escherichia coli isolation & purification
Abstract

Background: Biofilm consisting of bacteria enclosed in a matrix of exopolysaccharide (EPS) forms on many medical devices such as catheters and implants. Nosocomial infection is, thus, a newly recognized scenario of biofilm development. Biofilm removal by physical methods such as ultrasound and mechanical cleaning is reasonably effective but difficult to supervise in practice. Chemical methods are often ineffective because of biofilm resistance to biocides. In this study, we compared the efficiency of different detergents used in endoscope reprocessing., Methods: Escherichia coli biofilm was generated on Teflon and medical grade PVC tubing under low flow conditions. Sections of biofilm covered tubing were washed using test detergents and biofilm removal was assessed by counting remaining adherent bacteria after washing and by scanning electron microscopy to qualitatively assess the amount and nature of the remaining biofilm., Results: Control tubing developed a multilayered biofilm consisting of >10(5) bacterial cells/cm(2). Only Matrix (Whiteley Medical, Sydney, Australia) produced >4 log reduction in viable bacterial numbers. Matrix and Epizyme Rapid (3M Australia, Pymble, Australia) were able to remove up to 75% and 60% of the biofilm, respectively., Conclusions: Many commonly used enzymatic cleaners fail to reduce the viable bacterial load or remove the bacterial EPS. Cleaners with high enzyme activity, Epizyme Rapid, removed more biofilm but failed to reduce bacterial numbers more than 2 logs. The only cleaner containing no enzymes, Matrix, significantly reduced bacterial viability and residual bacterial EPS.

Published
2004
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85. Plantar warts of defined aetiology in adults and unresponsiveness to low dose cimetidine.

Author

Lee SH, Rose B, Thompson CH, and Cossart Y

Subjects
Adult, Dose-Response Relationship, Drug, Female, Humans, Male, Middle Aged, Pilot Projects, Polymerase Chain Reaction, Warts virology, Adjuvants, Immunologic administration & dosage, Cimetidine administration & dosage, Foot Diseases drug therapy, Foot Diseases virology, Papillomaviridae isolation & purification, Warts drug therapy
Published
2001

86. Variable oncogene promoter activity of human papillomavirus type 16 cervical cancer isolates from Australia.

Author

Watts KJ, Thompson CH, Cossart YE, and Rose BR

Subjects
Australia, Female, HeLa Cells, Humans, Mutagenesis, Site-Directed, Oncogene Proteins, Viral metabolism, Papillomaviridae isolation & purification, Papillomavirus E7 Proteins, Papillomavirus Infections virology, Polymerase Chain Reaction, Tumor Virus Infections virology, Genetic Variation genetics, Oncogene Proteins, Viral genetics, Papillomaviridae genetics, Promoter Regions, Genetic genetics, Repressor Proteins, Uterine Cervical Neoplasms virology
Abstract

The functional significance of sequence variation within the upstream regulatory region (URR) of six human papillomavirus type 16 (HPV16) cervical cancer isolates from Australia was investigated. Specific changes in transcription factor binding sites leading to increased promoter activity may explain the transforming ability of some episomal HPV16 isolates.

Published
2001
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87. Squamous carcinoma of the head and neck: molecular mechanisms and potential biomarkers.

Author

Rose BR, Thompson CH, Tattersall MH, O'Brien CJ, and Cossart YE

Subjects
Biomarkers, Tumor, Carcinoma, Squamous Cell pathology, Carcinoma, Squamous Cell virology, Gene Deletion, Gene Expression Regulation, Neoplastic genetics, Head and Neck Neoplasms pathology, Head and Neck Neoplasms virology, Humans, Microsatellite Repeats genetics, Models, Genetic, Oncogenes genetics, Polymorphism, Genetic, Risk Factors, Carcinoma, Squamous Cell genetics, Head and Neck Neoplasms genetics, Molecular Biology, Mutation genetics
Abstract

Squamous cell carcinoma (SCC) of the head and neck remains a major health problem worldwide. Recent advances in cell biology suggest that cancer results from the accumulation of specific genetic mutations, many of which have now been identified. These mutations can cause the activation of genes that promote cellular proliferation or inhibit cell death (oncogenes), or they may inactivate genes that inhibit proliferation or promote cell death (tumour suppressor genes). Although there is no known set sequence of events leading to the formation of SCC of the head and neck, there is evidence that many of the genomic mutations implicated in other forms of cancer have an aetiological role in these tumours. Certain viruses, notably Epstein-Barr virus and some types of human papillomaviruses, are causally related to some head and neck cancers. There is now the prospect of using molecular markers to achieve earlier diagnosis and to aid in the prediction of both tumour behaviour and likely responses to particular treatment modalities.

Published
2000
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88. Analysis of mutations in the URR and E6/E7 oncogenes of HPV 16 cervical cancer isolates from central China.

Author

Stephen AL, Thompson CH, Tattersall MH, Cossart YE, and Rose BR

Subjects
China epidemiology, DNA, Viral analysis, Female, Humans, Mutation, Open Reading Frames, Papillomaviridae genetics, Papillomavirus E7 Proteins, Prevalence, Uterine Cervical Neoplasms epidemiology, Uterine Cervical Neoplasms virology, Oncogene Proteins, Viral genetics, Regulatory Sequences, Nucleic Acid genetics, Repressor Proteins, Uterine Cervical Neoplasms genetics
Abstract

High rates of cervical cancer have been reported from parts of China and this may reflect a predominance of cervical infection with particularly aggressive human papillomavirus (HPV) variants. This PCR-based investigation of cervical tumours from Sichuan province in central China demonstrated an HPV positivity rate of 88%. HPV 16 was most common (21/34, 61%), followed by HPV 18 (3/34, 9%), while types 33, 45, 58 and 59 were each identified in one specimen. Sequencing of up to 1349 bases of the 21 HPV 16-positive isolates, encompassing the enhancer/promoter of the upstream regulatory region (URR) and the E6 and E7 genes, revealed distinct patterns of genomic stability and variability. An overall mutation rate of 5% was seen in the URR. One isolate had a large deletion of 436 bases in the enhancer; while varying combinations of 21 point mutations were identified in the remainder, impacting several YY1, NF1, TEF-1 and Oct-1 sites. More sequence variations were found in E6 compared to E7 (81% vs. 52% of isolates showing at least one mutation), some of which resulted in changes to the translated amino acids. Since the E6/E7 genes encode the oncogenic proteins essential for malignant transformation, and as their expression is controlled by the URR, it is possible that some of the identified mutations altered the oncogenicity of the virus: either directly by changing amino acid sequences of the E6 or E7 oncoproteins, or indirectly through alterations to transcription factor binding sites in the URR., (Copyright 2000 Wiley-Liss, Inc.)

Published
2000
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89. Hepatitis C in injecting drug-using women during and after pregnancy.

Author

Latt NC, Spencer JD, Beeby PJ, McCaughan GW, Saunders JB, Collins E, and Cossart YE

Subjects
Adult, Case-Control Studies, Female, Hepatitis C diagnosis, Hepatitis C transmission, Humans, Liver Function Tests, Pregnancy, Pregnancy Outcome epidemiology, Prospective Studies, Risk Factors, Viremia epidemiology, Viremia virology, Hepatitis C epidemiology, Pregnancy Complications, Infectious virology, Substance Abuse, Intravenous
Abstract

Background: A high proportion of female injecting drug users (IDU) have evidence of hepatitis C virus (HCV) infection. We undertook a prospective study of patients attending a clinic for pregnant IDU to determine the impact of pregnancy on the course of HCV infection and whether pregnancy is affected by HCV infection., Methods: One hundred and thirty-one IDU were recruited and followed up with liver function tests, HCV serology and HCV-RNA tests., Results: Of 131 patients, 125 had HCV antibodies (anti-HCV positive) at delivery, and of these 62% were HCV-RNA positive. The anti-HCV-negative women were younger and had a shorter duration of drug use than the anti-HCV-positive women. There were no differences between viraemic and non-viraemic women with respect to age, ethnicity, duration of injecting drug use, methadone maintenance dose, hepatitis B exposure or reported high-risk behaviour. Alanine aminotransferase (ALT) levels were higher and the proportion with ALT > 55 IU/L higher in viraemic women. Viraemia persisted in all 55 women who were viraemic at term. Eleven had an ALT flare post-partum that was unrelated to viral load and was clinically unsuspected. Four had concurrent elevated gamma-glutamyltranspeptidase and were considered to be drinking alcohol at hazardous levels. Four of 23 women who were HCV-RNA negative at term became positive during follow up., Conclusions: Pregnancy does not adversely affect the course of hepatitis C. A modest rebound in ALT levels, but not HCV-RNA, occurs after delivery in some viraemic women. This supports the theory that immune mechanisms rather than direct viral cytopathology are involved in hepatocyte injury during HCV infection. Hepatitis C infection did not influence pregnancy complications and outcomes.

Published
2000
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90. Evaluation of disinfection and sterilization of reusable angioscopes with the duck hepatitis B model.

Author

Chaufour X, Deva AK, Vickery K, Zou J, Kumaradeva P, White GH, and Cossart YE

Subjects
Animals, Cross Infection prevention & control, DNA, Viral analysis, Disease Models, Animal, Ducks, Jugular Veins virology, Sterilization, Angioscopes, Angioscopy adverse effects, Disinfection, Hepatitis B Virus, Duck isolation & purification, Liver virology
Abstract

Purpose: Nosocomial transmission of viral hepatitis and retrovirus infection has been reported. The expected risk is greatest for the hepatitis B virus (HBV). The duck HBV (DHBV) has similar biologic and structural characteristics to HBV and has been adopted as a suitable model for disinfectant testing., Methods: Angioscopic examination of the external jugular vein was performed on DHBV-infected ducks. After use, the instrument was air dried for 3 minutes. Samples were obtained by flushing the channel with 5 mL of phosphate buffered saline solution. The samples were collected immediately after drying (control), after flushing with 5 mL of water, after glutaraldehyde disinfection for 5, 10, and 20 minutes, and after ethylene oxide gas sterilization. Angioscopes were either precleaned or uncleaned before disinfection/sterilization. Residual infectivity was assessed with inoculation of samples into the peritoneal cavity of day-old ducks (n = 231)., Results: DNA analysis results of liver samples showed that all 38 control ducks became infected. The frequency of DHBV infection was reduced to 93% (14 of 15) by flushing the angioscope with 5 mL of sterile water. No transmission occurred after the use of any of the properly precleaned and disinfected/sterilized angioscopes. However, after the use of the uncleaned angioscopes, the transmission rate was 90% (9 of 10) and 70% (7 of 10) after 5 and 10 minutes of contact time, respectively, in 2% glutaraldehyde. Even after the recommended 20 minutes of contact time, there was still 6% (2 of 35) transmission. After ethylene oxide sterilization, two of the recipient ducklings (2 of 35) were infected with DHBV., Conclusion: There was no disease transmission after reuse of disposable angioscopes adequately cleaned before disinfection or sterilization. However, if the angioscopes are inadequately cleaned, DHBV can survive despite glutaraldehyde disinfection or ethylene oxide sterilization. This contrasts with previous in vitro and in vivo data with solid surgical instruments. It is postulated that the presence of a narrow lumen or residual protein shielding within the lumen may compromise effective inactivation of hepadnaviruses on angioscopes, with the potential risk for patient-to-patient transmission.

Published
1999
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91. A novel human papillomavirus DNA sequence related to epidermodysplasia verruciformis-associated types isolated from recurrent scar carcinoma.

Author

Lee SH, Rose BR, Thompson CH, and Cossart YE

Subjects
Amino Acid Sequence, Base Sequence, Humans, Male, Middle Aged, Molecular Sequence Data, Carcinoma genetics, Cicatrix genetics, DNA Probes, HPV, DNA, Viral analysis, Epidermodysplasia Verruciformis genetics, Papillomaviridae genetics, Skin Neoplasms genetics
Published
1999
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92. Broadsheet. Number 49: Laboratory investigation of hepatitis C: a review.

Author

Cossart YE

Subjects
False Negative Reactions, False Positive Reactions, Genotype, Hepacivirus isolation & purification, Hepatitis C immunology, Hepatitis C Antibodies blood, Humans, Polymerase Chain Reaction, Predictive Value of Tests, Prognosis, RNA, Viral blood, Reagent Kits, Diagnostic, Sensitivity and Specificity, Hepatitis C diagnosis
Published
1999
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93. Cellular immune response of ducks to duck hepatitis B virus infection.

Author

Vickery K, Cossart Y, and Dixon R

Subjects
Acute Disease, Animals, Chronic Disease, Ducks, Female, Hepadnaviridae Infections pathology, Hepatitis B Antibodies blood, Immunity, Cellular, Leukocytes, Mononuclear virology, Liver immunology, Liver pathology, Liver virology, Lymphocyte Activation, Male, Spleen cytology, Hepadnaviridae Infections immunology, Hepatitis B Virus, Duck immunology, Leukocytes, Mononuclear immunology
Abstract

Duck hepatitis B virus (DHBV) has been a useful model for hepadnavirus infection. There have been few studies on immunity to DHBV and none describing the cell-mediated immune response by acute and chronically infected ducks. A duck hepatitis B antigen-specific blastogenesis assay was used to measure DHBV antigen-specific responses of duck peripheral blood (PBMC) and splenic mononuclear cells (SMCs) from uninfected control ducks, ducks acutely or chronically infected with DHBV, and ducks immune to DHBV. A comparison of the group mean responses by PBMC to DHBV surface antigen (DHBsAg) found that the immune group was significantly different to the other three groups (controls or unexposed, P < 0.0001; acutely infected, P< 0.01; chronically infected, P < 0.01). The responses to DHBsAg by PBMC of the acute group (P< 0.01) were significantly different also to that of the unexposed group. For DHBV core antigen (DHBcAg), significant differences in the responses were found between immune ducks and unexposed (P < 0.0005) and acutely infected (P < 0.05) groups. The SMC showed a significant difference between unexposed ducks and immune ducks (P< 0.05) in the group mean responses to DHBsAg. The responses to DHBcAg were significantly different between the immune group and the acute (P < 0.01) and unexposed (P < 0.01) groups. The group mean of unexposed ducks was also significantly different to that of acutely infected ducks (P < 0.01). This study indicates that the cellular immune response in immune animals differs from acutely and chronically infected ducks. Further studies of these differences may provide some explanations for the differing outcomes of DHBV infection.

Published
1999

94. Inactivation of duck hepatitis B virus by a hydrogen peroxide gas plasma sterilization system: laboratory and 'in use' testing.

Author

Vickery K, Deva AK, Zou J, Kumaradeva P, Bissett L, and Cossart YE

Subjects
Animals, Ducks, Equipment Contamination, Hepadnaviridae Infections transmission, Hepatitis B Virus, Duck isolation & purification, Cross Infection prevention & control, Disinfectants, Hepadnaviridae Infections prevention & control, Hepatitis B Virus, Duck physiology, Hydrogen Peroxide, Sterilization methods
Abstract

Human hepatitis B virus (HBV) is an important cause of nosocomial infections and can be transmitted by contaminated instruments. However, tests of the efficacy of sterilization of materials and equipment contaminated by HBV are difficult to perform because the virus cannot be cultured in the laboratory. In this study, we aimed to evaluate the capability of a low temperature, hydrogen peroxide gas plasma sterilizer (Sterrad, Advanced Sterilization Products, Irvine California,) to inactivate duck hepatitis B virus (DHBV). In laboratory efficacy studies using DHBV dried on to glass filter carriers and exposed to one-half of the hydrogen peroxide gas plasma sterilization process, there was a 10(7) or greater decrease in the viral titer, with no infectivity detected on the carriers after treatment. In-use studies were performed using a laparoscope that was experimentally contaminated with DHBV to mimic the possible transmission of infection between successive patients. Following exposure to the hydrogen peroxide gas plasma sterilization process no transmission of DHBV infection from the laparoscope occurred despite obvious visual soiling with blood (N = 8) while the transmission rate for the unprocessed laparoscope (positive control) was 100% (26/26), and that for instruments after a water wash was 63% (7/11). In conclusion the hydrogen gas plasma sterilization process completely inactivates DHBV a representative of the hepadna group of viruses.

Published
1999
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95. Varicella vaccination of health-care workers.

Author

Burgess MA, Cossart YE, Wilkins TD, Botham S, Fearns G, and Chitour K

Subjects
Adolescent, Adult, Antibodies, Viral blood, Chickenpox blood, Chickenpox immunology, Chickenpox Vaccine adverse effects, Female, Humans, Male, Middle Aged, Risk Factors, Vaccines, Attenuated adverse effects, Vaccines, Attenuated immunology, Vaccines, Attenuated therapeutic use, Chickenpox prevention & control, Chickenpox Vaccine immunology, Chickenpox Vaccine therapeutic use, Health Personnel
Abstract

The objective of this open study was to evaluate the response of non-immune health-care workers to two doses of live attenuated varicella vaccine given two months apart. One hundred subjects (58 females; aged 17-49 yr, mean 22.8 yr) received two doses of varicella vaccine. Blood samples for antibody estimation were taken before vaccination, 2 months after the first dose and 6 weeks after the second dose. Reactions were recorded daily in diaries by the vaccinees and controlled by telephone contacts by the investigators. Ninety-four of 99 vaccinees (94.9%, 95% CL 88.6, 98.3) had detectable antibodies after the first dose [titers 4-1024, geometric mean titer (GMT): 53.2 (95% CL 42.4, 66.8)]. After the second dose, all vaccinees had antibodies (100%, 95% CL 96.6, 100.0) [titers 32-2048, GMT: 235.6 (95% CL 199.0, 278.8)]. Mild reactions limited to the injection site occurred in 1 in 4 subjects after each dose. Vesicular rashes occurred in one subject after the 1st dose and in 3 subjects after the 2nd dose, 1 subject was febrile (38.2 degrees C) after the 1st dose. Eighty-one subjects were retested 12 months after the second vaccination. Three had become seronegative (one developed mild varicella 2 months later). Two had boosted their titers (one after mild clinical varicella 1 month earlier, the other after close contact with clinical cases). The GMT of the group had fallen to 83.6 (95% CL 65.4, 106.8). The identification and vaccination of seronegative health-care workers is safe and efficient, and will benefit the workers themselves and the communities in which they work.

Published
1999
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96. Detection of persistent vegetative bacteria and amplified viral nucleic acid from in-use testing of gastrointestinal endoscopes.

Author

Deva AK, Vickery K, Zou J, West RH, Selby W, Benn RA, Harris JP, and Cossart YE

Subjects
Decontamination, Endoscopy, Gastrointestinal, Equipment Contamination, HIV isolation & purification, Hepacivirus isolation & purification, Hepatitis B virus isolation & purification, Humans, RNA, Viral analysis, Bacteria isolation & purification, Cross Infection etiology, DNA, Viral analysis, Endoscopes microbiology, Viruses isolation & purification
Abstract

Hospital-acquired infection attributed to inadequate decontamination of gastrointestinal endoscopes prompted an in use evaluation of recommended procedures. Specimens were obtained from the internal channels of 123 endoscopes before, during and after decontamination by flushing with saline and brushing with a sterile brush, and examined for vegetative bacteria by broth and plate culture. Four endoscopy units were tested; the chemical disinfectants used were: 2% glutaraldehyde in Centres 1 and 2 (automated) and Centre 3 (manual); peracetic acid in Centre 4 (automated). Samples from patients in Centre 1 with known chronic hepatitis B virus (HBV), hepatitis C virus (HCV) and human immunodeficiency virus (HIV-1) infection were also examined for viral nucleic acid by ultracentrifugation, nucleic acid extraction, reverse transcription (for RNA) and polymerase chain reaction (PCR). No persistent vegetative bacteria were found following standard manual cleaning and disinfection for 20 min in 2% glutaraldehyde in Centres 2 and 3 (N = 37). At Centre 1, while plate culture yielded no growth, 34% of samples (10/29) grew vegetative bacteria in broth culture after cleaning and disinfection for 20 min in 2% glutaraldehyde. Investigation revealed an error in manual cleaning; no bacteria were detected in 37 samples taken after this was corrected. At Centre 4, despite the use of peracetic acid as a sterilant, three out of 20 (15%) of post decontamination samples grew bacteria; one contained persistent bacteria. HBV and HCV PCR analysis detected viral nucleic acid in three out of four and four out of six samples from viraemic patients undergoing endoscopy in Centre 1 during the period of improper manual washing. After proper cleaning was instituted, samples from nine out of nine HCV viraemic patients were negative. HIV RNA was detected in five of 14 samples taken from endoscopes after use on HIV positive patients but all post decontamination samples were negative. Detection of bacteria in washes from endoscope channels is a useful warning of a breakdown in decontamination practice. Inadequate brushing of internal channels may result in persistent HCV and HBV viral nucleic acid, the significance of which is not clear. These results reinforce the importance of adequate manual cleaning of endoscopes before chemical disinfection.

Published
1998
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97. Cholestatic hepatitis after liver transplantation is associated with persistently high serum hepatitis C virus RNA levels.

Author

Doughty AL, Spencer JD, Cossart YE, and McCaughan GW

Subjects
Adult, Cholestasis complications, Diagnosis, Differential, Female, Hepatitis C complications, Humans, Male, Middle Aged, RNA, Viral blood, Recurrence, Viral Load, Cholestasis diagnosis, Graft Rejection diagnosis, Hepacivirus genetics, Hepatitis C diagnosis, Liver Transplantation
Abstract

Viral recurrence is universal after transplantation for hepatitis C infection. This may lead to difficulties in differentiating allograft dysfunction caused by chronic rejection from hepatitis C virus (HCV) recurrence. Cases of severe cholestatic hepatitis have also been reported in conjunction with reinfection of the graft with HCV. Patients receiving transplants for HCV-related liver disease were studied before and after transplantation by HCV RNA quantitation of serial serum samples. Four major clinical patterns of HCV recurrence could be distinguished posttransplantation: group 1, asymptomatic hepatitis with no significant symptoms; group 2, cholestatic hepatitis with centrilobular ballooning; group 3, hepatitis leading to chronic allograft rejection; and group 4, persistently normal serum aminotransferase levels. Pretransplantation viral load was shown to be an important indicator of disease severity because the group 2 patients had significantly higher pretransplantation viral loads than patients in group 1 (P = 0.01) and group 4 (P = 0.005). The group 2 patients also had persistently significantly higher posttransplantation viral loads than the patients in group 1 (P = 0.01) and group 4 (P = 0.02), whereas patients who developed chronic allograft rejection showed marked decreases in serum HCV RNA before retransplantation. Patients from group 4 had the lowest viral loads after transplantation. These results show that persisting graft cholestasis due to HCV is associated with persistently high HCV RNA levels compared with other etiologies of graft dysfunction. Prospective studies are needed to determine whether such quantitation may be diagnostically helpful in distinguishing the different patterns of HCV-related graft dysfunction observed after liver transplantation.

Published
1998
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98. Horizontal transmission of hepatitis B in a children's day-care centre: a preventable event.

Author

McIntosh ED, Bek MD, Cardona M, Goldston K, Isaacs D, Burgess MA, and Cossart YE

Subjects
Australia, Child, Child, Preschool, DNA Fingerprinting, Hepatitis B Antigens blood, Humans, Infant, Male, Serologic Tests, Carrier State diagnosis, Child Day Care Centers, Disease Transmission, Infectious prevention & control, Hepatitis B prevention & control, Hepatitis B transmission, Hepatitis B Vaccines administration & dosage, Vaccination
Abstract

Using molecular finger-printing, we provided evidence that, in a children's day-care centre, a known hepatitis B virus (HBV) hepatitis B e antigen (HBeAg) carrier transmitted HBV to another child (the index case). The chronic HBV carrier had an exudative skin lesion and a history of biting. We sought to identify other at-risk children and prevent further transmission. Blood samples were collected and tested serologically for HBV. Of the 90 other children, 78 (87 per cent) were tested and none had serological evidence of HBV infection; 73 (81 per cent) were of Caucasian background; 38 (49 per cent) had a history of HBV immunisation with serological confirmation. Therefore, 1 (2.4 per cent, 95 per cent confidence interval 1.0 to 12.8 per cent) of the 41 known susceptible contacts became infected. The risk of horizontal HBV transmission in a children's day-care centre is low but not negligible. Staff and children should be vaccinated when a child in a day-care centre is a known HBV carrier.

Published
1997
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99. The removal of model viruses, poliovirus type 1 and canine parvovirus, during the purification of human albumin using ion-exchange chromatographic procedures.

Author

Cameron R, Davies J, Adcock W, MacGregor A, Barford JP, Cossart Y, and Harbour C

Subjects
Animals, Dogs, HeLa Cells, Humans, Isoelectric Point, Chromatography, Ion Exchange methods, Drug Contamination prevention & control, Parvovirus isolation & purification, Poliovirus isolation & purification, Serum Albumin isolation & purification
Abstract

The manufacturing process for albumin in Australia is based primarily on ion-exchange chromatography. The capacity of ion-exchange matrices to remove non-enveloped viruses (canine parvovirus and poliovirus type 1) was assessed using a scaled-down chromatographic process which was shown to yield product meeting purity criteria set for the manufacturing process. Poliovirus type 1 and canine parvovirus were added at one tenth the volume of desalted and delipidated Supernatant II + III produced by traditional Cohn Fractionation from human plasma before the material was applied to DEAE and CM ion-exchangers connected in series. Samples were taken at equilibration, wash, elution and regeneration steps and the log clearance and reduction of the viruses calculated. The mean clearance and reduction factors for viral load of poliovirus type 1 were 5.3 logs and 3.2 logs, respectively and 1.8 logs and 1.8 logs for canine parvovirus.

Published
1997
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100. Sequence variation in the upstream regulatory region of HPV 18 isolates from cervical cancers.

Author

Rose BR, Thompson CH, Zhang J, Stoeter M, Stephen A, Pfister H, Tattersall MH, and Cossart YE

Subjects
Female, Humans, Mutation, Regulatory Sequences, Nucleic Acid, DNA, Viral genetics, Papillomaviridae genetics, Uterine Cervical Neoplasms virology
Abstract

This study describes sequence variation in both the enhancer and promoter segments of the upstream regulatory region (URR) of 28 human papillomavirus (HPV) type 18 isolates from cervical cancers, 25 from women treated at an Australian center and three from overseas included for comparison. No large-scale changes were found in either region. Fourteen substitutions were identified in the enhancer region with the number in individual isolates ranging from one to eight. Four substitutions impacted cellular transcription factor binding sites but there were no obvious associations with clinicopathological variables. The promoter segment was found to be more highly conserved than the enhancer, but four of the five point mutations identified involved cellular transcription factor binding motifs including a substitution of C for T at nt 104 which affected 21 samples. This change was found to impact upon a previously unrecognized Yin Yang (YY1) binding site. Electrophoretic mobility shift assays (EMSA) showed that this substitution significantly reduced protein-DNA binding and evidence was sought for its possible clinical implications. Of the 24 women with less than Stage III disease and known clinical outcome, tumor recurrence was observed in all of the 6 women whose isolates had the "prototype" T at nt 104, whereas only 8 of the 18 cancers with the mutation at this YY1 site recurred. This is the first report on URR variation in HPV 18 isolates from the South Pacific region. The study also provides initial data on diversity in the promoter region and preliminary evidence suggesting that a specific point mutation in this region may be clinically significant.

Published
1997
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