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1. Hepatitis C virus genotypes in multi-transfused individuals

Author

L M Jarvis, Peter Simmonds, and Christopher A. Ludlam

Subjects
business.industry, Hepatitis C virus, Genotype, medicine, Hematology, General Medicine, medicine.disease_cause, business, Virology, Genetics (clinical)
Published
2016

2. Seroprevalence of lyme borreliosis in Scottish blood donors

Author

H, Munro, S, Mavin, K, Duffy, R, Evans, and L M, Jarvis

Subjects
Adult, Male, Rural Population, Lyme Disease, Urban Population, Blood Safety, Middle Aged, Antibodies, Bacterial, Sampling Studies, Scotland, Seroepidemiologic Studies, Borrelia burgdorferi, Immunoglobulin G, Humans, Female, Disease Reservoirs
Published
2015

3. Prediction of cirrhosis in patients with chronic hepatitis C infection by artificial neural network analysis of virus and clinical factors

Author

P. C. Hayes, J. P. Hanley, C. A. Ludlum, L M Jarvis, Mika Ala-Korpela, Geoffrey Haydon, Yrjö Hiltunen, and R. Jalan

Subjects
Adult, Liver Cirrhosis, Male, medicine.medical_specialty, Cirrhosis, Hepatitis C virus, Logistic regression, medicine.disease_cause, Liver disease, Predictive Value of Tests, Virology, Internal medicine, medicine, Humans, Hepatology, medicine.diagnostic_test, business.industry, Hepatitis C, Hepatitis C, Chronic, equipment and supplies, medicine.disease, body regions, Logistic Models, Infectious Diseases, Hepatocellular carcinoma, Liver biopsy, Predictive value of tests, Immunology, Female, Neural Networks, Computer, business
Abstract

The diagnosis of cirrhosis in patients with hepatitis C virus (HCV) infection is currently made using a liver biopsy. In this study we have trained and validated artificial neural networks (ANN) with routine clinical host and viral parameters to predict the presence or absence of cirrhosis in patients with chronic HCV infection and assessed and interpreted the role of the different inputs on the ANN classification. Fifteen routine clinical and virological factors were collated from 112 patients who were HCV RNA positive by reverse transcriptase-polymerase chain reaction (RT-PCR). Standard and Ward-type feed-forward fully-connected ANN analyses were carried out both by training the networks with data from 82 patients and subsequently testing with data from 30 patients plus performing leave-one-out tests for the whole patient data set. The ANN results were also compared with those from multiple logistic regression. The performance of both ANN methods was superior compared with the logistic regression. The best performance was obtained with the Ward-type ANNs resulting in a sensitivity of 92% and a specificity of 98.9% together with a predictive value of a positive test of 95% and a predictive value of a negative test of 97% in the leave-one-out test. Hence, further validation of the ANN analysis is likely to provide a non-invasive test for diagnosing cirrhosis in HCV-infected patients.

Published
1998

4. Sexual transmission of GB virus C/hepatitis G virus

Author

L M Jarvis, Martina F. Scallan, Dan Clutterbuck, Peter Simmonds, and Gordon Scott

Subjects
Hepatitis, Sexually transmitted disease, education.field_of_study, Sexual transmission, Hepatitis C virus, Population, virus diseases, Viremia, Biology, medicine.disease, medicine.disease_cause, biology.organism_classification, GB virus C, Virology, Flaviviridae, Infectious Diseases, Immunology, medicine, education
Abstract

Although it is established that infection with GB virus C (GBV-C) or hepatitis G virus (HGV) can be transmitted parenterally, the prevalence of GBV-C/HGV viremia in the general population (2-5%) is relatively high compared with other parenterally borne viruses such as hepatitis C virus. To investigate the possibility of sexual transmission of GBV-C/HGV, we determined the frequency of viremia by the polymerase chain reaction and serological reactivity to the E2 protein by ELISA in samples collected from individuals at risk for sexually transmitted diseases attending a city genitourinary medicine clinic. GBV-C/HGV viremia was detected in 27 of 87 male homosexuals (31%) and 9 of 50 prostitutes (18%), frequencies significantly greater than those in matched controls (2/63) and local blood donors (2.3%). Among nonviremic individuals, a high frequency of serological reactivity to the E2 protein of GBV-C/HGV was also observed in the risk groups (male homosexuals: 14/60; prostitutes: 11/41), although these figures are likely to be underestimates of the frequency of past infection as detectable anti-E2 reactivity may attenuate rapidly over time following resolution of infection. Infection with GBV-C/HGV was more frequent among those coinfected with human immunodeficiency virus type 1. Among male homosexuals from whom retrospective samples were available, evidence for de novo infection was found in 9 of 22 individuals over a mean sampling time of 2.9 years, predicting an annualized incidence of GBV-C/HGV infection of approximately 11% in this group. The high prevalence and incidence of GBV-C/HGV infection in these individuals and prostitutes provides strong evidence for its spread by sexual contact. Further studies are required to investigate the mechanism of its transmission and the clinical significance of acute and persistent infection in these risk groups.

Published
1998

5. Transition-Metal Ethene Bonds: Thermochemistry of M+(C2H4)n (M = Ti−Cu, n = 1 and 2) Complexes

Author

M. R. Sievers, L. M. Jarvis, and P. B. Armentrout

Subjects
Ion beam, Chemistry, Analytical chemistry, General Chemistry, Mass spectrometry, Biochemistry, Catalysis, Dissociation (chemistry), Metal, Colloid and Surface Chemistry, Transition metal, Computational chemistry, visual_art, visual_art.visual_art_medium, Thermochemistry, Molecule, Bond energy
Abstract

Complexes of the first-row transition-metal cations (Ti+−Cu+) with one and two ethene molecules are studied by guided ion beam mass spectrometry. Thermalized complexes are formed in a flow tube source and examined by energy-resolved collision-induced dissociation with Xe. The energy dependence of the CID cross sections is analyzed with consideration of multiple collisions, internal energy of the reactants, and lifetime effects. First, D0(M+−C2H4), and second, D0(C2H4M+−C2H4), adiabatic metal ion ethene bond energies, in eV, obtained in this study are 1.51 ± 0.11 for Ti (first bond only), 1.29 ± 0.08 and 1.32 ± 0.14 for V, 0.99 ± 0.11 and 1.12 ± 0.11 for Cr, 0.94 ± 0.12 and 0.91 ± 0.15 for Mn, 1.50 ± 0.11 and 1.57 ± 0.16 for Fe, 1.93 ± 0.09 and 1.58 ± 0.14 for Co, 1.89 ± 0.11 and 1.79 ± 0.15 for Ni, and 1.82 ± 0.14 and 1.80 ± 0.13 for Cu, respectively. These values include corrections for diabatic dissociation in the cases of Fe+(C2H4) and Mn+(C2H4)2, a point that is discussed in detail. Previous work obta...

Published
1998

6. The Effect of Treatment with a-Interferon on Hepatitis G/GBV-C Viraemia

Author

L M Jarvis, Bjørn Myrvang, S Ritland, H Bell, Stig Harthug, Kjell Block Hellum, N. Raknerud, Peter Simmonds, B von der Lippe, Kjell Skaug, A Maeland, and A Hawkins

Subjects
Hepatitis, medicine.diagnostic_test, business.industry, Hepatitis C virus, Gastroenterology, virus diseases, Alpha interferon, Hepatitis C, medicine.disease, medicine.disease_cause, Virology, digestive system diseases, Liver biopsy, medicine, Liver function, business, Viral hepatitis, Interferon alfa, medicine.drug
Abstract

BACKGROUND: Hepatitis G virus (HGV) or GBV-C is frequently detected in patients co-infected with hepatitis C virus (HCV). This study investigated host and virologic factors influencing the response to HGV/GBV-C to alpha-interferon treatment. METHODS: HGV/GBV-C was detected and quantified by nested polymerase chain reaction. The influence of variables such as liver biopsy appearance, liver function abnormalities, and response of HCV to interferon treatment was monitored. RESULTS: Fourteen of the 25 HGV/GBV-C-infected patients treated with interferon (3-6 MIU three times a week for 6 months) became non-viraemic during treatment, although all relapsed after treatment withdrawal at 6 months, with no net change in virus load between 0 and 12 months. CONCLUSIONS: Predictive factors for clearance of HGV/GBV-C viraemia by interferon were pre-treatment severity of liver disease (median Knodell score of 4, compared with 7 for non-responders; P = 0.030) and alanine aminotransferase levels (median, 114, 182 for non-responders; P = 0.039). Clearance was associated with the treatment response of HCV. Nine of 13 who cleared HGV/GBV-C also cleared HCV, compared with 3 of 11 HGV/GBV-C non-responders; P = 0.05). The shared susceptibility of HGV/GBV-C and HCV to interferon treatment suggests a link between the mechanism of clearance of the two viruses.

Published
1998

7. Patterns of Hepatitis G Viraemia and Liver Disease in Haemophiliacs Previously Exposed to Non-virus Inactivated Coagulation Factor Concentrates

Author

Amanda J Lee, Christopher A. Ludlam, Peter Simmonds, Peter C. Hayes, John Hanley, and L M Jarvis

Subjects
Hepatitis, biology, business.industry, Hepatitis C virus, virus diseases, Hematology, medicine.disease_cause, medicine.disease, Haemophilia, Chronic liver disease, biology.organism_classification, Virology, digestive system diseases, Virus, Flaviviridae, Liver disease, medicine, Viral disease, business
Abstract

SummaryHepatitis G virus (HGV), a novel flavivirus, has been implicated as a cause of posttransfusion hepatitis. We have performed a longitudinal study in a cohort of haemophiliacs (n = 68) who previously received non-virus inactivated coagulation factor concentrates to assess both patterns of HGV viraemia and any associated liver disease. Hepatitis C virus (HCV) RNA was present in 58/68 and co-infection with human immunodeficiency virus (HIV) was present in 15/68.HGV RNA was detected in 17/68 (25%) samples from the mid-1980s. There was no association between either HIV infection (p = 0.74) or co-infection with a particular HCV genotype (p = 0.62). However, there was a relationship between HGV viraemia and the severity of haemophilia (p = 0.0004) with HGV RNA detected in 5/19, 9/16 and 3/32 patients with mild, moderate and severe haemophilia respectively.A longitudinal study was performed in 15/17 haemophiliacs with HGV viraemia using stored serum samples from the 1980s and 1990s. HGV viraemia persisted in 8/15 and cleared in 7/15 over a variable period of time. A Weibull model was constructed to estimate the duration of HGV viraemia in the study group. The 75th and 90th percentiles for the duration of HGV were estimated to be 8.7 years (95%, confidence interval 4.8-15.7) and 23.6 years (95% confidence interval 11.8-47.1) respectively. Laparoscopic liver inspection/biopsy was performed in 25/68. There was no association between severity of liver disease and HGV viraemia (p = 0.43). This study demonstrates considerable variation in patterns of HGV viraemia in haemophiliacs. We found little evidence to implicate HGV as a major cause of chronic liver disease in haemophiliacs.

Published
1998

8. Use of the quenching factor for predicting the properties of polymer quenching media

Author

C. Bates, George E. Totten, A. V. Sverdlin, and L. M. Jarvis

Subjects
chemistry.chemical_classification, Quenching, Materials science, Aqueous solution, High Energy Physics::Lattice, Metallurgy, Alloy, Metals and Alloys, Thermodynamics, chemistry.chemical_element, Polymer, engineering.material, Condensed Matter Physics, Decomposition, Condensed Matter::Materials Science, chemistry, Mechanics of Materials, Aluminium, Metallic materials, engineering, Solid solution
Abstract

The development of methods for evaluating and predicting the variation of the properties of polymer quenching media in operation requires an analysis of the quenching factor, which characterizes the degree of decomposition of the solid solution in quenching, which decreases the strength (hardness) of the alloy by a given value. In the present paper the quenching factorQ is used to compare the properties of aluminum alloys quenched in hot water and aqueous solutions of polymers.

Published
1996

9. Investigation of the relative infectivity and pathogenicity of different hepatitis C virus genotypes in hemophiliacs

Author

JA Ellender, A Chuansumrit, L M Jarvis, Christopher A. Ludlam, E Song, SP Field, Peter Simmonds, FE Preston, and L Nemes

Subjects
Infectivity, education.field_of_study, biology, business.industry, Hepatitis C virus, Hepacivirus, Immunology, Population, Cell Biology, Hematology, Hepatitis C, medicine.disease_cause, medicine.disease, biology.organism_classification, Biochemistry, Virology, Genotype frequency, Flaviviridae, Genotype, Medicine, business, education
Abstract

To assess the relative infectivity and pathogenicity of variants of hepatitis C virus (HCV) genotypes, the distribution of genotypes in hemophilic patients who had been treated with nonvirally inactivated factor concentrates or cryoprecipitates prepared from local blood donors was compared with those found in the respective blood donor populations. Genotype frequencies differed markedly in the four countries investigated (Scotland, Hungary, South Africa, and Thailand) but in each, the HCV genotype distributions in hemophiliacs and blood donors were similar. In addition, HCV genotypes in recipients of commercially manufactured concentrates were similar to those found in the US general population. These findings provide no evidence that HCV genotypes differ significantly from each other in replication rate, transmissibility, or infectivity.

Published
1996

10. Survey of type 6 group variants of hepatitis C virus in Southeast Asia by using a core-based genotyping assay

Author

J Mellor, L M Jarvis, Emily Walsh, Peter Simmonds, F Davidson, P L Yap, and L E Prescott

Subjects
Microbiology (medical), Genotype, Molecular Sequence Data, Hepacivirus, Flaviviridae, Polymorphism (computer science), Sequence Homology, Nucleic Acid, Humans, Coding region, Genotyping, Asia, Southeastern, Phylogeny, Genetics, Molecular Epidemiology, Base Sequence, Molecular epidemiology, Phylogenetic tree, biology, Data Collection, Genetic Variation, biology.organism_classification, Hepatitis C, Genetic Techniques, DNA, Viral, Restriction fragment length polymorphism, Polymorphism, Restriction Fragment Length, Research Article
Abstract

Previous surveys of the prevalences of genotypes of hepatitis C virus (HCV) in different populations have often used genotyping assays based upon analysis of amplified sequences from the 5' noncoding region (5'NCR), such as restriction fragment length polymorphism (RFLP) or hybridization with type-specific probes (e.g., InnoLipa). Although highly conserved, this region contains several type-specific nucleotide polymorphisms that allow major genotypes 1 to 6 to be reliably identified. Recently, however, novel HCV variants found in Vietnam and Thailand that are distantly related to the type 6a genotype (type 6 group) by phylogenetic analysis of coding regions of the genome often have sequences in the 5'NCR that are similar or identical to those of type 1 and could therefore not be identified by an assay of sequences in this region. We developed a new genotyping assay based upon RFLP of sequences amplified from the more variable core region to investigate their distribution elsewhere in southeast (SE) Asia. Among 108 samples from blood donors in seven areas that were identified as type 1 by RFLP in the 5'NCR, type 6 group variants were found in Thailand (7 from 28 samples originally identified as type 1) and Burma (Myanmar) (1 of 3) but were not found in Hong Kong (n = 43), Macau (n = 8), Taiwan (n = 6), Singapore (n = 2), or Malaysia (n = 18). Although this small survey suggests a relatively limited distribution for type 6 group variants in SE Asia, larger studies will be required to explore their distribution in other geographical regions and the extent to which their presence would limit the practical usefulness of 5'NCR-based genotyping assays for clinical or epidemiological purposes.

Published
1996

11. Investigation of the pattern of hepatitis C virus sequence diversity in different geographical regions: implications for virus classification

Author

Edward C. Holmes, P L Yap, L M Jarvis, J Mellor, and Peter Simmonds

Subjects
Indian subcontinent, Phylogenetic tree, Phylogenetics, Virology, Hepatitis C virus, Genotype, Genetic variation, medicine, Biology, medicine.disease_cause, Virus classification, Sequence (medicine)
Abstract

Genotypes of hepatitis C virus (HCV) present within 104 samples from HCV-infected individuals from Africa, the Middle East, the Indian subcontinent and South-East Asia were identified by sequence comparisons in the core and NS-5 regions. Relatively short sequences (such as the 222 bp fragment of NS-5) provided effective discrimination of types, subtypes and isolates, and produced equivalent relationships between genotypes as were found upon comparison of longer sequences of NS-5, of the core region, and by comparison of the limited number of complete genomic sequences currently available. Measurement of evolutionary distances in the core and NS-5 regions allowed 79 of the 104 samples to be identified as examples of known genotypes, while 17 of the remainder could be provisionally classified as new subtypes of types 1 (Nigeria), 2 (Gambia), 3 (India, Pakistan and Bangladesh) and 4 (Middle East) on the basis of sequence comparison in core and NS-5 (n = 9) or provisionally using core alone (n = 8). The remaining sequences from Thailand made up two groups showing no close similarity to any of the six major genotypes classified to date, although one corresponded to an as yet unclassified variant of HCV also found in Thailand. However, phylogenetic analysis of the core and NS-5 regions indicated a distant relationship between these sequences with variants found in Vietnam and with type 6a, and collectively they formed a diverse single phylogenetic group. The existence of great diversity within a single genotype was also found amongst type 3 sequences in the Indian subcontinent, amongst type 4 variants in Central Africa and the Middle East, and amongst type variants in Nigeria. These findings may provide clues for understanding the origins and mechanisms of transmission of HCV.

Published
1995

12. Variation of the hepatitis C virus 5' non-coding region: implications for secondary structure, virus detection and typing

Author

J Mellor, Mickey S. Urdea, P L Yap, B. Douglas Smith, F Davidson, L M Jarvis, Janice A. Kolberg, and Peter Simmonds

Subjects
Genetics, viruses, Hepatitis C virus, virus diseases, Biology, medicine.disease_cause, Virology, Virus, Genetic variation, Genotype, medicine, Coding region, Typing, Restriction fragment length polymorphism, Genotyping
Abstract

Variation in the 5′ non-coding region (5′NCR) of hepatitis C virus (HCV) was investigated in detail by comparing 314 5′NCR sequences of viruses of genotypes 1 to 6. Evidence was obtained for the existence of associations between particular 5′NCR sequence motifs and virus types and subtypes. No recombination was observed between the 5′NCR and coding regions of different genotypes, implying that the sequence of subgenomic regions such as the 5′NCR can be used to deduce virus genotype. The distribution of polymorphic sites within the 5′NCR is used to propose improved oligonucleotide primers for virus detection and quantification that would be equally efficient in detecting RNA of different virus genotypes. The accuracy of two different genotyping methods (RFLP and the line probe assay) based on analysis of sequence polymorphisms in the 5′NCR is predicted from the sequences surveyed to be 97% and 83% respectively for types 1 to 6, with higher accuracies for distinguishing between subtypes 1a/1b, 2a/2b or 3a/3b. Several sites of genotype-specific polymorphism were covariant and maintained the base pairings required for a secondary structure model of the 5′NCR. Other sites of variation suggest minor modifications to this model and have implications for the probable functions of the 5′NCR

Published
1995

13. Heterogeneity of hepatitis C virus genotypes in hemophilia: relationship with chronic liver disease

Author

Michael Makris, J.C.E. Underwood, C. A. Ludlam, L. Philp, L. M. Jarvis, F. E. Preston, and Peter Simmonds

Subjects
Cirrhosis, medicine.diagnostic_test, business.industry, Hepatitis C virus, Immunology, virus diseases, Cell Biology, Hematology, Hepatitis C, medicine.disease, medicine.disease_cause, Chronic liver disease, Biochemistry, Virology, digestive system diseases, Liver disease, Liver biopsy, Genotype, medicine, Viral disease, business
Abstract

In this study we have determined the hepatitis C virus (HCV) serotype and genotype in a cohort of 96 HCV-infected hemophiliacs and have examined the relationship between HCV genotype and severity of chronic liver disease as determined by liver biopsy. HCV serotype was determined by specific enzyme-linked immunosorbent assays (ELISAs) and genotype by restriction fragment length polymorphism (RFLP) and HCV viral sequencing. The pattern of genotype distribution was quite unlike that of HCV-infected United Kingdom (UK) blood donors in that five of the six known HCV genotypes were represented, 50% were type 1, 13% type 2, and 18% type 3. An unexpected observation was the presence of HCV genotype 4 in four patients and type 5 in two patients. An additional feature was the presence of mixed infection, detected in 14% and 7% by serotype and genotype analysis, respectively. Liver biopsies were available from 51 patients. Cirrhosis was present in five of 27 (19%) of individuals with type 1, in 2 of 9 (22%) with type 2, and 5 of 8 (63%) of those with type 3. The heterogeneous pattern of HCV genotype distribution in this cohort of patients and the observed relationship between the severity of the related liver disease and specific HCV genotype may have important implications with respect to the natural history and treatment of HCV-related chronic liver disease in infected hemophiliacs worldwide.

Published
1995

14. Development of multiplexed nucleic acid testing for human immunodeficiency virus type 1 and hepatitis C virus

Author

A, Cleland, C, Davis, N, Adams, C, Lycett, L M, Jarvis, H, Holmes, and P, Simmonds

Subjects
HIV-1, Feasibility Studies, Humans, RNA, Viral, Hepacivirus, Polymerase Chain Reaction, Sensitivity and Specificity, Sequence Alignment, Conserved Sequence, DNA Primers, HIV Long Terminal Repeat
Abstract

In most Western countries, blood donations are routinely screened for hepatitis C virus (HCV) RNA by polymerase chain reaction (PCR) or other nucleic acid tests. We describe the development of a multiplexed assay for human immunodeficiency virus type 1 (HIV-1) and HCV in an internally controlled PCR suitable for large-scale blood donor screening.The HIV/HCV multiplexed PCR used primers from highly conserved regions in the long terminal repeat region. The National Institute for Biological Standards and Controls (NIBSC) International HIV-1 RNA standard, run control and HIV-1 subtype panel were used for assay evaluation.The HIV-1 PCR showed a sensitivity of 24 IU/ml for HIV-1 RNA (a dilution where 95% of replicate reactions were positive), which was at least five times more sensitive than the Roche Monitor version 1.5 (using the ultrasensitive extraction protocol) and Organon NASBA assays. The assay was capable of detecting all subtypes of HIV-1 (A to H), as well as the more divergent group N and O variants. The sensitivity of the PCR was unaffected by multiplexing with HCV primers and by the presence of a bovine viral diarrhoea virus (BVDV) internal control.We have developed a highly sensitive multiplexed PCR for HIV-1 and HCV RNA screening that can be introduced into current PCR-based blood donor screening at minimal cost and without significant operational changes.

Published
2001

15. Detection of enterovirus viraemia in blood donors

Author

J B, Welch, K, McGowan, B, Searle, J, Gillon, L M, Jarvis, and P, Simmonds

Subjects
Base Sequence, Molecular Sequence Data, Enterovirus Infections, Humans, Blood Donors, Viremia, Enterovirus
Abstract

The infrastructure established for screening blood donations for hepatitis C virus has enabled large-scale population testing for other viruses which are potentially transmissible by transfusion of blood components and plasma-derived blood products. We have measured the frequency of viraemia of enteroviruses and parechoviruses in 83 600 Scottish blood donors to allow an initial assessment of their risk to blood safety.Plasma samples collected from blood donors over 7 calendar months were tested anonymously in mini-pools of 95 donations, by polymerase chain reaction (PCR) for human enterovirus and parechovirus sequences.A total of 19 mini-pools, from the 880 that were tested, were PCR-positive for enterovirus RNA, predicting a donor prevalence of 0.023%. Enterovirus sequences were not detected in factor VIII or IX clotting factor concentrates. None of the 230 mini-pools or concentrates contained detectable parechovirus RNA.The prevalence of enterovirus viraemia detected in this study predicts that at least 1000 enterovirus-contaminated blood components are transfused per year in the UK. The frequency of transmission and clinical outcome after exposure to enterovirus-contaminated blood components in recipients is unknown.

Published
2001

17. Detection of GB virus C RNA by GBV-C LCx and two PCR assays with primers from the 5' non-coding and NS5B region

Author

H Bell, Peter Simmonds, L M Jarvis, E.S. Berg, and Kjell Skaug

Subjects
Hepatitis, Viral, Human, viruses, Genome, Viral, Viral Nonstructural Proteins, Sensitivity and Specificity, Virus, Serology, law.invention, chemistry.chemical_compound, Flaviviridae, law, Virology, Humans, NS5B, Polymerase chain reaction, DNA Primers, biology, Reverse Transcriptase Polymerase Chain Reaction, virus diseases, RNA, Hepatitis C, Chronic, biology.organism_classification, GB virus C, Molecular biology, Real-time polymerase chain reaction, chemistry, RNA, Viral, Reagent Kits, Diagnostic, 5' Untranslated Regions
Abstract

The objective of this study was to compare the sensitivity of three different reverse transcriptase-polymerase chain reaction (RT-PCR) based tests, for detection of GB virus C (GBV-C) RNA. One commercial and two 'in house' RT-PCR assays were employed in the testing of serum samples from 114 chronic hepatitis C infected individuals. A part of the 5' non-coding region (5'NCR) of the GBV-C genome was amplified by the GBV-C LCx assay (Abbott) and one of the 'in house' RT-PCR tests. In the other 'in house' RT-PCR a segment of the NS5B region was amplified. The 'in house' assays included the use of internal controls that were co-amplified with use of the same outer PCR primers as the virus targets. The GBV-C LCx from Abbott and 5'NCR 'in house' PCR tests detected 28 and 27 GBV-C positive individuals, respectively. The sample positive only in the LCx test was confirmed by the 'in house' 5'NCR RT PCR using an increased virus input. In comparison, the NS5B 'in house' PCR test detected 24 of the GBV-C positive samples. One sample showed no amplification of internal controls/virus target in the 5'NCR 'in house' PCR and another samples was amplification negative in the NS5B PCR. The PCR assays with primers from the 5'NCR of the virus genome e.g. the GBV-C LCx, were more sensitive compared with RT-PCR using primers from the NS5B region. The GBV-C LCx seemed to be the most sensitive and robust assay. Internal controls included in the 'in house' assays identified two samples with failure of the amplification.

Published
1999

18. Sexual transmission of GB virus C/hepatitis G virus

Author

M F, Scallan, D, Clutterbuck, L M, Jarvis, G R, Scott, and P, Simmonds

Subjects
Adult, Male, Adolescent, Hepatitis, Viral, Human, Incidence, Flaviviridae, Enzyme-Linked Immunosorbent Assay, HIV Infections, Sexually Transmitted Diseases, Viral, Middle Aged, Sex Work, Scotland, Viral Envelope Proteins, Prevalence, Humans, RNA, Viral, Female, Hepatitis Antibodies, Viremia, Homosexuality, Male, Retrospective Studies
Abstract

Although it is established that infection with GB virus C (GBV-C) or hepatitis G virus (HGV) can be transmitted parenterally, the prevalence of GBV-C/HGV viremia in the general population (2-5%) is relatively high compared with other parenterally borne viruses such as hepatitis C virus. To investigate the possibility of sexual transmission of GBV-C/HGV, we determined the frequency of viremia by the polymerase chain reaction and serological reactivity to the E2 protein by ELISA in samples collected from individuals at risk for sexually transmitted diseases attending a city genitourinary medicine clinic. GBV-C/HGV viremia was detected in 27 of 87 male homosexuals (31%) and 9 of 50 prostitutes (18%), frequencies significantly greater than those in matched controls (2/63) and local blood donors (2.3%). Among nonviremic individuals, a high frequency of serological reactivity to the E2 protein of GBV-C/HGV was also observed in the risk groups (male homosexuals: 14/60; prostitutes: 11/41), although these figures are likely to be underestimates of the frequency of past infection as detectable anti-E2 reactivity may attenuate rapidly over time following resolution of infection. Infection with GBV-C/HGV was more frequent among those coinfected with human immunodeficiency virus type 1. Among male homosexuals from whom retrospective samples were available, evidence for de novo infection was found in 9 of 22 individuals over a mean sampling time of 2.9 years, predicting an annualized incidence of GBV-C/HGV infection of approximately 11% in this group. The high prevalence and incidence of GBV-C/HGV infection in these individuals and prostitutes provides strong evidence for its spread by sexual contact. Further studies are required to investigate the mechanism of its transmission and the clinical significance of acute and persistent infection in these risk groups.

Published
1998

19. High prevalence of hepatitis G virus infection in multiply transfused children with thalassaemia

Author

Panya Seksarn, Yong Poovorawan, Voranaush Chongsrisawat, Apiradee Theamboonlers, Peter Simmonds, and L M Jarvis

Subjects
Male, Blood transfusion, Adolescent, Hepatitis, Viral, Human, medicine.medical_treatment, Hepatitis C virus, medicine.disease_cause, Polymerase Chain Reaction, medicine, Humans, Child, Hepatitis B virus, Hepatitis, Hepatology, biology, business.industry, Flaviviridae, Gastroenterology, virus diseases, Infant, Transfusion Reaction, Alanine Transaminase, Hepatitis C, Hepatitis B, medicine.disease, digestive system diseases, Alanine transaminase, Child, Preschool, Immunology, Coinfection, biology.protein, RNA, Viral, Thalassemia, Female, business
Abstract

We investigated the prevalence of hepatitis G virus (HGV) RNA in relation to the frequency of blood transfusions in thalassaemic children and in volunteer blood donors in Thailand. Furthermore, we studied the frequency of coinfection with hepatitis B virus (HBV) and/or hepatitis C virus (HCV) as well as a possible relationship to the alanine aminotransferase (ALT) status of the blood samples, taken at random from thalassaemic children who have received multiple blood transfusions and from volunteer blood donors. The results show detectable HGV-RNA in 32.6% of transfusion patients and in 5% of blood donors. The prevalence of HGV-RNA peaked between the 11th and 50th transfusion. The relationship between HGV infection and ALT status was not statistically relevant.The prevalence of hepatitis G virus (HGV) RNA was compared in a cohort of 89 thalassemic children (age range, 1-16 years) with a history of multiple blood transfusions, recruited from the hematology outpatient clinic at Thailand's Chulalongkorn Hospital and in specimens from 200 blood donors at the Red Cross in Bangkok. 29 specimens (32.6%) from thalassemic children, compared with 10 (5%) from blood donors, demonstrated detectable HGV RNA by reverse transcriptase analysis. 48% of the HGV-RNA-positive thalassemic children had elevated alanine aminotransferase levels, compared with 51.9% of the cohort without detectable HGV RNA; a finding that supports the assumption HGV infection does not cause detectable hepatitis. HGV RNA prevalence was 11.8% among children with 2-10 transfusions, 48.8% with 11-50 transfusions, 21.7% in those with 51-100 transfusions, and 16.7% among those with over 100 transfusions. This pattern suggests that at least some of the children recovered from HGV infection and may have developed immunity to reinfection. The clinical significance of HGV, as well as the apparent immunity acquired against reinfection, merit further investigation.

Published
1998

20. Clinical significance of intrahepatic hepatitis C virus levels in patients with chronic HCV infection

Author

P. C. Hayes, David J. Harrison, Geoffrey Haydon, L M Jarvis, C S Blair, Kenneth J. Simpson, and Peter Simmonds

Subjects
Adult, Male, Cirrhosis, Genotype, Hepacivirus, Hepatitis C virus, medicine.disease_cause, Virus Replication, Polymerase Chain Reaction, Sensitivity and Specificity, Statistics, Nonparametric, Virus, Flaviviridae, medicine, Humans, Transaminases, medicine.diagnostic_test, biology, Gastroenterology, virus diseases, Hepatitis C, Hepatitis C, Chronic, biology.organism_classification, medicine.disease, digestive system diseases, Liver, Liver biopsy, Immunology, RNA, Viral, Female, Polymorphism, Restriction Fragment Length
Abstract

Background —The clinical significance of a single assessment of circulating hepatitis C virus (HCV) RNA and its relation to the level of intrahepatic HCV RNA remains unclear. Aims —To investigate the relation between intrahepatic HCV levels and clinicopathological characteristics of chronic HCV infection. Patients —Ninety eight consecutive patients with chronic HCV infection were studied; none had received α interferon therapy. Of these, 12 patients were repeatedly negative for HCV RNA in serum by reverse transcriptase polymerase chain reaction (RT-PCR). Methods —After diagnostic laparoscopy and liver biopsy, semiquantitative analysis of intrahepatic HCV RNA levels was carried out by limiting dilution of HCV cDNA. HCV genotypes were assessed in 96 patients by restriction fragment length polymorphism analysis of HCV cDNA. Results —Ten out of 12 patients who were RT-PCR negative for HCV RNA in serum were RT-PCR positive in liver; however, this group had a significantly lower intrahepatic HCV level and serum aminotransferase level than the remaining 86 patients. Histological severity (cirrhosis: n=10); histological activity index; HCV genotype (genotype 1: n=41; genotype 2: n=12; genotype 3: n=36; genotype 4: n=7); mode of infection (intravenous drug abuse: n=58; post-transfusion: n=10; haemophiliac: n=4; sporadic: n=26) and alcohol abuse did not affect the intrahepatic virus level. There was no correlation between patient age, duration of infection, and intrahepatic HCV level. Conclusions —Intrahepatic virus levels were not determined by host factors (age of patient, mode or duration of infection) or by virus factors (HCV genotype). Repeatedly negative RT-PCR for HCV RNA in serum does not indicate absence of HCV from the liver.

Published
1998

21. The effect of treatment with alpha-interferon on hepatitis G/GBV-C viraemia. The CONSTRUCT Group

Author

L M, Jarvis, H, Bell, P, Simmonds, A, Hawkins, K, Hellum, S, Harthug, A, Maeland, S, Ritland, B, Myrvang, B, von der Lippe, N, Raknerud, and K, Skaug

Subjects
Adult, Male, Hepatitis, Viral, Human, Flaviviridae, Interferon-alpha, Alanine Transaminase, Middle Aged, Viral Load, Hepatitis C, Polymerase Chain Reaction, Treatment Outcome, Humans, RNA, Viral, Female, Viremia, Aged
Abstract

Hepatitis G virus (HGV) or GBV-C is frequently detected in patients co-infected with hepatitis C virus (HCV). This study investigated host and virologic factors influencing the response to HGV/GBV-C to alpha-interferon treatment.HGV/GBV-C was detected and quantified by nested polymerase chain reaction. The influence of variables such as liver biopsy appearance, liver function abnormalities, and response of HCV to interferon treatment was monitored.Fourteen of the 25 HGV/GBV-C-infected patients treated with interferon (3-6 MIU three times a week for 6 months) became non-viraemic during treatment, although all relapsed after treatment withdrawal at 6 months, with no net change in virus load between 0 and 12 months.Predictive factors for clearance of HGV/GBV-C viraemia by interferon were pre-treatment severity of liver disease (median Knodell score of 4, compared with 7 for non-responders; P = 0.030) and alanine aminotransferase levels (median, 114, 182 for non-responders; P = 0.039). Clearance was associated with the treatment response of HCV. Nine of 13 who cleared HGV/GBV-C also cleared HCV, compared with 3 of 11 HGV/GBV-C non-responders; P = 0.05). The shared susceptibility of HGV/GBV-C and HCV to interferon treatment suggests a link between the mechanism of clearance of the two viruses.

Published
1998

22. Patterns of hepatitis G viraemia and liver disease in haemophiliacs previously exposed to non-virus inactivated coagulation factor concentrates

Author

J P, Hanley, L M, Jarvis, P C, Hayes, A J, Lee, P, Simmonds, and C A, Ludlam

Subjects
Adult, Adolescent, Hepatitis, Viral, Human, Flaviviridae, Middle Aged, Hemophilia A, Hemophilia B, Blood Coagulation Factors, von Willebrand Diseases, Child, Preschool, Humans, Viremia, Child, Drug Contamination
Abstract

Hepatitis G virus (HGV), a novel flavivirus, has been implicated as a cause of posttransfusion hepatitis. We have performed a longitudinal study in a cohort of haemophiliacs (n = 68) who previously received non-virus inactivated coagulation factor concentrates to assess both patterns of HGV viraemia and any associated liver disease. Hepatitis C virus (HCV) RNA was present in 58/68 and co-infection with human immunodeficiency virus (HIV) was present in 15/68. HGV RNA was detected in 17/68 (25%) samples from the mid-1980s. There was no association between either HIV infection (p = 0.74) or co-infection with a particular HCV genotype (p = 0.62). However, there was a relationship between HGV viraemia and the severity of haemophilia (p = 0.0004) with HGV RNA detected in 5/19, 9/16 and 3/32 patients with mild, moderate and severe haemophilia respectively. A longitudinal study was performed in 15/17 haemophiliacs with HGV viraemia using stored serum samples from the 1980s and 1990s. HGV viraemia persisted in 8/15 and cleared in 7/15 over a variable period of time. A Weibull model was constructed to estimate the duration of HGV viraemia in the study group. The 75th and 90th percentiles for the duration of HGV were estimated to be 8.7 years (95%, confidence interval 4.8-15.7) and 23.6 years (95% confidence interval 11.8-47.1) respectively. Laparoscopic liver inspection/biopsy was performed in 25/68. There was no association between severity of liver disease and HGV viraemia (p = 0.43). This study demonstrates considerable variation in patterns of HGV viraemia in haemophiliacs. We found little evidence to implicate HGV as a major cause of chronic liver disease in haemophiliacs.

Published
1998

23. The clinical significance of the detection of hepatitis GBV-C RNA in the serum of patients with fulminant, presumed viral, hepatitis

Author

L M Jarvis, Geoffrey Haydon, P. C. Hayes, Kenneth J. Simpson, and Peter Simmonds

Subjects
Adult, Male, medicine.medical_specialty, Blood transfusion, Adolescent, Hepatitis, Viral, Human, Transcription, Genetic, Fulminant, medicine.medical_treatment, Gastroenterology, Polymerase Chain Reaction, Flaviviridae, Virology, Internal medicine, medicine, Humans, Clinical significance, Blood Transfusion, Fulminant hepatitis, Child, Hepatitis, Hepatology, biology, business.industry, Transfusion History, biology.organism_classification, medicine.disease, Infectious Diseases, Hepatic Encephalopathy, Immunology, RNA, Viral, Female, business, Viral hepatitis
Abstract

In a significant number of cases of fulminant (presumed viral) hepatitis worldwide, no aetiological agent has been identified. Recently, it has been suggested that a newly described flavivirus, GBV-C, is responsible for some of these cases. This study aimed to assess the clinical significance of GBV-C RNA, demonstrated by reverse transcriptase-polymerase chain reaction (RT-PCR), in the serum of patients with fulminant non-A to E hepatitis. Twenty-three consecutive cases of non-A to E fulminant hepatitis were included in the study. GBV-C RNA was reverse transcribed and amplified using two RT-PCR based detection methods. Medical records were examined to assess clinical history, duration and mode of infection, transfusion history, liver histology and clinical outcome. Five (three female, two male; mean age 21.2 years) of 23 patients had GBV-C RNA detected in their serum by RT-PCR: all five patients were RT-PCR positive following amplification by primers specific for the 5' non-coding region (NCR), whilst four were positive by primers for the NS3 region. Prior to the onset of illness, two patients had risk factors for transmission of an infectious agent; however, all five patients had been transfused during their illness, prior to testing for GBV-C. Of these, two (of two in whom serum was available) were negative for GBV-C after the onset of fulminant hepatitis but before their first transfusion. This study does not support the hypothesis that the detection of hepatitis G virus (HGV)/GBV-C RNA in the serum of patients with fulminant hepatitis indicates a causal association. However, it does demonstrate that a careful transfusion history and screening of blood products is vital before the importance of GBV-C in the aetiology of fulminant hepatitis can be established.

Published
1997

24. Infection with hepatitis G virus among recipients of plasma products

Author

Peter Simmonds, J. P. Hanley, F Davidson, L M Jarvis, Christopher A. Ludlam, and P L Yap

Subjects
Male, Hepatitis, Viral, Human, Hepatitis C virus, Population, Immunoglobulins, Blood Donors, medicine.disease_cause, Hemophilia A, Virus, Factor IX, Flaviviridae, Agammaglobulinemia, Prevalence, Medicine, Humans, education, education.field_of_study, Factor VIII, biology, business.industry, virus diseases, General Medicine, Hepatitis C, biology.organism_classification, medicine.disease, GB virus C, Virology, digestive system diseases, Scotland, Immunology, Female, Viral disease, business, Viral hepatitis, Drug Contamination
Abstract

Summary Background Hepatitis G virus (HGV or GBV-C) is a newly discovered human flavivirus distantly related to hepatitis C virus (HCV). Little information is available on its natural history or routes of transmission, although it can be transmitted parenterally. We investigated the prevalence of persistent infection of HGV and HCV in patients exposed to non-virus-inactivated pooled blood products associated with transmission of HCV. Methods RNA was extracted from the plasma of 112 patients with haemophilia and 57 with hypogamma-globulinaemia, as well as from 64 different batches of archived coagulation-factor concentrates and immuno-globulins. RNA was reverse transcribed and amplified with primers from the 5' non-coding region of HCV and HGV by a nested polymerase chain reaction (PCR). Viral RNA was quantified by titration of complementary DNA before amplification. Findings Among non-remunerated UK blood donors HGV infection (detected by PCR) was more common than HCV infection (four [32%] of 125 compared with 137 [0076%] of 180 658 in southeast Scotland). Testing of batches of factor VIII and factor IX concentrates prepared without viral inactivation procedures showed high frequencies of contamination with HGV (16 of 17 factor VIII batches positive; six of six factor IX batches positive), with no difference between remunerated and non-renumerated donors. However, among 95 haemophiliacs who had received non-virus-inactivated concentrates, 13 (14%) were positive for HGV compared with 79 (83%) who were positive for HCV. Two of 37 recipients of long-term immunoglobulin replacement therapy were positive for HGV. Virus inactivation of blood products substantially reduced or eliminated contamination by HGV RNA sequences. Interpretation Despite the extremely high level of HGV contamination of non-virus-inactivated blood products, their use was not associated with high rates of persistent infection in recipients. The infectivity of HGV in blood products may be lower than that of HCV, or the virus may be less able to establish persistent infection in humans. Whatever the case, the high prevalence of active HGV infection in the general population remains difficult to explain.

Published
1996

25. A combined management protocol for patients with coagulation disorders infected with hepatitis C virus

Author

Elwyn Elias, J. Linin, M. M. Ahmed, L M Jarvis, David Mutimer, Stefan G. Hubscher, M. Garrido, Jonathan T. Wilde, and Peter Simmonds

Subjects
Adult, Male, Viral Hepatitis Vaccines, medicine.medical_specialty, Hepatitis C virus, Blood Component Transfusion, Haemophilia, medicine.disease_cause, Clinical Protocols, Internal medicine, Biopsy, medicine, Humans, Retrospective Studies, medicine.diagnostic_test, business.industry, Biopsy, Needle, virus diseases, Retrospective cohort study, Hematology, Hepatitis C, Blood Coagulation Disorders, medicine.disease, Liver biopsy, Cryoprecipitate, Immunology, Female, Complication, business
Abstract

The case notes of 394 adults with bleeding disorders registered at our centre together with those of the 72 patients who had died since 1971 were reviewed. 36/72 deceased patients had evidence of HCV infection. Liver decompensation was present at time of death in six. 274 (70%) of the currently registered patients had received factor concentrate or cryoprecipitate and 174 of these were screened for HCV infection. 76% of tested patients were RIBA positive. 87% of RIBA-positive patients were RT-PCR positive. 50 RIBA-positive patients, including nine who were HIV infected, have undergone percutaneous liver biopsy following appropriate factor infusion with no complication. The biopsy was assessed using a Histological Activity Index (HAI) ranging from 0 to 13. Patients with HAIor = 6 were offered treatment with interferon. Patients with HAI6 were followed up with a view to re-biopsy in 2-3 years to assess progression. The median HAI was 4.5 (range 0-10) with HAIor = 6 in 13 cases (27%). HAI was not correlated with duration of infection. haemophilia severity. RT-PCR status. HIV status or HCV genotype. Liver biopsy, a safe procedure in our hands, is an important investigation in HCV-infected patients to assess suitability for interferon therapy.

Published
1996

26. Assessment of liver histology in patients with hepatitis C and normal transaminase levels

Author

A J, Stanley, G H, Haydon, J, Piris, L M, Jarvis, and P C, Hayes

Subjects
Adult, Male, Genotype, Biopsy, Humans, RNA, Viral, Alanine Transaminase, Female, Hepacivirus, Prognosis, Hepatitis C
Abstract

To compare liver histology in patients with hepatitis C infection (HCV) between patients with normal and abnormal alanine aminotransferase (ALT) and examine its relationship with HCV genotype and route of infection.One hundred consecutive patients with known HCV presenting for diagnostic laparoscopy and liver biopsy were studied. Route of infection was noted and ALT measured on the day of biopsy and HCV genotype determined. Hepatic pathology was analysed using the Edinburgh scoring system (ESS).Fifteen patients had normal ALT, of whom three (20%) had cirrhosis and 10 (66.7%) fibrosis. Of patients with raised ALT, cirrhosis and fibrosis were similarly found in 14 (16.5%) and 62 (72.9%) respectively. Severe, moderate and mild inflammation occurred in one (6.7%), four (26.7%) and 10 (66.6%) patients with normal ALT compared with 17 (20%), 50 (58.8%) and 18 (21.2%) of those with raised ALT (P0.01). There was no significant difference in age, route of infection or genotype between those with normal and raised ALT levels.Of patients with normal ALT at time of liver biopsy, a significant minority have cirrhosis or significant hepatic inflammation. Liver biopsy is essential in HCV infection as a guide to both therapy and prognosis.

Published
1996

27. Development of anti-interferon antibodies and breakthrough hepatitis during treatment for HCV infection in haemophiliacs

Author

Peter Simmonds, John Hanley, Christopher A. Ludlam, and L M Jarvis

Subjects
Adult, Male, Adolescent, Hepatitis C virus, Alpha interferon, Interferon alpha-2, medicine.disease_cause, Hemophilia A, Virus, Antibodies, Flaviviridae, medicine, Humans, Interferon alfa, Aged, biology, business.industry, Interferon-alpha, Hematology, Hepatitis C, Middle Aged, medicine.disease, biology.organism_classification, Virology, Recombinant Proteins, Immunology, biology.protein, Female, Viral disease, Antibody, business, medicine.drug
Abstract

The development of anti-interferon antibodies may lead to treatment failure during interferon therapy. We have studied the development of such antibodies in a group of 39 haemophiliacs receiving interferon-alpha 2a for chronic hepatitis C virus (HCV) infection. Anti-interferon antibodies developed in five (13%) patients and were associated with "breakthrough hepatitis' in three cases. There was an association between the development of anti-interferon antibodies and infection with HCV genotype 3a (P = 0.01). This study suggests that the development of anti-interferon antibodies may lead to treatment failure in a proportion of haemophiliacs with HCV infection. The association with genotype 3a has not previously been reported. Monitoring for the development of breakthrough hepatitis due to anti-interferon antibodies may provide the opportunity to develop strategies to overcome their effects.

Published
1996

28. Investigation of chronic hepatitis C infection in individuals with haemophilia: assessment of invasive and non-invasive methods

Author

L M Jarvis, Peter C. Hayes, Christopher A. Ludlam, Janet Andrews, Juan Piris, Robert Lee, John Hanley, Peter Simmonds, and Rosemary Dennis

Subjects
Adult, Male, medicine.medical_specialty, Cirrhosis, Adolescent, Genotype, Hepatitis C virus, Biopsy, HIV Infections, Chronic liver disease, Haemophilia, medicine.disease_cause, Hemophilia A, Gastroenterology, Cohort Studies, Liver disease, Predictive Value of Tests, Internal medicine, medicine, Humans, Child, Aged, Ultrasonography, Hepatitis, Laparotomy, medicine.diagnostic_test, business.industry, Endoscopy, Hematology, Hepatitis C, Middle Aged, medicine.disease, Evaluation Studies as Topic, Liver biopsy, Chronic Disease, Female, business
Abstract

Hepatitis C virus (HCV) infection is the major cause of chronic liver disease in individuals with haemophilia. A wide spectrum of disease severity is found in this group, ranging from mild hepatitis to cirrhosis. We have studied a cohort of 87 anti-HCV positive haemophiliacs who have been infected with HCV for 10-25 years and assessed the relative value of invasive and non-invasive methods of evaluating liver disease. The severity of liver disease was assessed using ultrasound scan (n = 77), upper GI endoscopy (n = 50), laparoscopic liver inspection (n = 33) and liver biopsy (n = 22). Invasive investigations were performed without any significant bleeding complications. Evidence of severe liver disease was found in approximately 25% of patients. There was agreement between the severity of liver histology and the information derived from the laparoscopic liver inspection, endoscopy and ultrasound in 86%. Co-infection with HIV was significantly associated with more severe liver disease (P = 0.006). This study provides further evidence that liver disease is emerging as a major complication in haemophiliacs and severe liver disease is more common in those co-infected with HIV. We have shown the potential value of laparoscopic liver inspection, in combination with endoscopy and ultrasound, in staging the extent of liver disease, and suggest that most patients may be managed without resorting to liver biopsy.

Published
1996

29. Investigation of the relative infectivity and pathogenicity of different hepatitis C virus genotypes in hemophiliacs

Author

L M, Jarvis, C A, Ludlam, J A, Ellender, L, Nemes, S P, Field, E, Song, A, Chuansumrit, F E, Preston, and P, Simmonds

Subjects
Humans, Hepacivirus, Hemophilia A, Hepatitis C
Abstract

To assess the relative infectivity and pathogenicity of variants of hepatitis C virus (HCV) genotypes, the distribution of genotypes in hemophilic patients who had been treated with nonvirally inactivated factor concentrates or cryoprecipitates prepared from local blood donors was compared with those found in the respective blood donor populations. Genotype frequencies differed markedly in the four countries investigated (Scotland, Hungary, South Africa, and Thailand) but in each, the HCV genotype distributions in hemophiliacs and blood donors were similar. In addition, HCV genotypes in recipients of commercially manufactured concentrates were similar to those found in the US general population. These findings provide no evidence that HCV genotypes differ significantly from each other in replication rate, transmissibility, or infectivity.

Published
1996

30. Investigation of the pattern of hepatitis C virus sequence diversity in different geographical regions: implications for virus classification. The International HCV Collaborative Study Group

Author

J, Mellor, E C, Holmes, L M, Jarvis, P L, Yap, and P, Simmonds

Subjects
Asia, Base Sequence, Genes, Viral, Genotype, Viral Core Proteins, Molecular Sequence Data, Genetic Variation, Genome, Viral, Hepacivirus, Sequence Analysis, DNA, Viral Nonstructural Proteins, Europe, Terminology as Topic, Africa, Humans, RNA, Viral, Phylogeny
Abstract

Genotypes of hepatitis C virus (HCV) present within 104 samples from HCV-infected individuals from Africa, the Middle East, the Indian subcontinent and South-East Asia were identified by sequence comparisons in the core and NS-5 regions. Relatively short sequences (such as the 222 bp fragment of NS-5) provided effective discrimination of types, subtypes and isolates, and produced equivalent relationships between genotypes as were found upon comparison of longer sequences of NS-5, of the core region, and by comparison of the limited number of complete genomic sequences currently available. Measurement of evolutionary distances in the core and NS-5 regions allowed 79 of the 104 samples to be identified as examples of known genotypes, while 17 of the remainder could be provisionally classified as new subtypes of types 1 (Nigeria), 2 (Gambia), 3 (India, Pakistan and Bangladesh) and 4 (Middle East) on the basis of sequence comparison in core and NS-5 (n = 9) or provisionally using core alone (n = 8). The remaining sequences from Thailand made up two groups showing no close similarity to any of the six major genotypes classified to date, although one corresponded to an as yet unclassified variant of HCV also found in Thailand. However, phylogenetic analysis of the core and NS-5 regions indicated a distant relationship between these sequences with variants found in Vietnam and with type 6a, and collectively they formed a diverse single phylogenetic group. The existence of great diversity within a single genotype was also found amongst type 3 sequences in the Indian subcontinent, amongst type 4 variants in Central Africa and the Middle East, and amongst type variants in Nigeria. These findings may provide clues for understanding the origins and mechanisms of transmission of HCV.

Published
1995

31. Variation of the hepatitis C virus 5' non-coding region: implications for secondary structure, virus detection and typing. The International HCV Collaborative Study Group

Author

D B, Smith, J, Mellor, L M, Jarvis, F, Davidson, J, Kolberg, M, Urdea, P L, Yap, and P, Simmonds

Subjects
Recombination, Genetic, Base Composition, Polymorphism, Genetic, Base Sequence, Genotype, Molecular Sequence Data, Genetic Variation, Humans, Nucleic Acid Conformation, RNA, Viral, Hepacivirus, Codon
Abstract

Variation in the 5' non-coding region (5'NCR) of hepatitis C virus (HCV) was investigated in detail by comparing 314 5'NCR sequences of viruses of genotypes 1 to 6. Evidence was obtained for the existence of associations between particular 5'NCR sequence motifs and virus types and subtypes. No recombination was observed between the 5'NCR and coding regions of different genotypes, implying that the sequence of subgenomic regions such as the 5'NCR can be used to deduce virus genotype. The distribution of polymorphic sites within the 5'NCR is used to propose improved oligonucleotide primers for virus detection and quantification that would be equally efficient in detecting RNA of different virus genotypes. The accuracy of two different genotyping methods (RFLP and the line probe assay) based on analysis of sequence polymorphisms in the 5'NCR is predicted from the sequences surveyed to be 97% and 83% respectively for types 1 to 6, with higher accuracies for distinguishing between subtypes 1a/1b, 2a/2b or 3a/3b. Several sites of genotype-specific polymorphism were covariant and maintained the base pairings required for a secondary structure model of the 5'NCR. Other sites of variation suggest minor modifications to this model and have implications for the probable functions of the 5'NCR.

Published
1995

32. Survey of major genotypes and subtypes of hepatitis C virus using RFLP of sequences amplified from the 5' non-coding region

Author

F. Davidson, P. Simmonds, J. C. Ferguson, L. M. Jarvis, B. C. Dow, E. A. C. Follett, C. R. G. Seed, T. Krusius, C. Lin, G. A. Medgyesi, H. Kiyokawa, G. Olim, G. Duraisamy, T. Cuypers, A. A. Saeed, D. Teo, J. Conradie, M. C. Kew, M. Lin, C. Nuchaprayoon, O. K. Ndimbie, and P. L. Yap

Subjects
Genetics, biology, Genotype, Hepatitis C virus, Hepacivirus, Hcv transmission, Blood Donors, medicine.disease_cause, biology.organism_classification, Virology, Polymerase Chain Reaction, law.invention, Restriction enzyme, law, medicine, Coding region, Humans, Restriction fragment length polymorphism, Polymerase chain reaction, Polymorphism, Restriction Fragment Length
Abstract

A method is described for identifying different genotypes of hepatitis C virus (HCV) by restriction endonuclease cleavage of sequences amplified by PCR from the 5′ non-coding region. Using the enzymes HaeIII-RsaI and HinfI-MvaI, followed by cleavage with BstU1 or ScrFI, it was possible to identify and distinguish HCV genotypes 1a, 1b, 2a, 2b, 3a, 3b, 4, 5 and 6. The method was used to investigate the prevalence of these genotypes in 723 blood donors in 15 countries, the largest survey to date, and one which covered a wide range of geographical regions (Europe, America, Africa and Asia). These results, combined with a review of the existing literature, indicate the existence of several distinct regional patterns of HCV genotype distribution, and provide the framework for future detailed epidemiological investigations of HCV transmission.

Published
1995

33. Heterogeneity of hepatitis C virus genotypes in hemophilia: relationship with chronic liver disease

Author

F E, Preston, L M, Jarvis, M, Makris, L, Philp, J C, Underwood, C A, Ludlam, and P, Simmonds

Subjects
Liver Cirrhosis, Virulence, Biopsy, Genetic Variation, Alanine Transaminase, Genome, Viral, Hepacivirus, Hemophilia A, Hepatitis C, Severity of Illness Index, Blood Coagulation Factors, Cohort Studies, England, Liver, RNA, Viral, Serotyping, Drug Contamination, Polymorphism, Restriction Fragment Length
Abstract

In this study we have determined the hepatitis C virus (HCV) serotype and genotype in a cohort of 96 HCV-infected hemophiliacs and have examined the relationship between HCV genotype and severity of chronic liver disease as determined by liver biopsy. HCV serotype was determined by specific enzyme-linked immunosorbent assays (ELISAs) and genotype by restriction fragment length polymorphism (RFLP) and HCV viral sequencing. The pattern of genotype distribution was quite unlike that of HCV-infected United Kingdom (UK) blood donors in that five of the six known HCV genotypes were represented, 50% were type 1, 13% type 2, and 18% type 3. An unexpected observation was the presence of HCV genotype 4 in four patients and type 5 in two patients. An additional feature was the presence of mixed infection, detected in 14% and 7% by serotype and genotype analysis, respectively. Liver biopsies were available from 51 patients. Cirrhosis was present in five of 27 (19%) of individuals with type 1, in 2 of 9 (22%) with type 2, and 5 of 8 (63%) of those with type 3. The heterogeneous pattern of HCV genotype distribution in this cohort of patients and the observed relationship between the severity of the related liver disease and specific HCV genotype may have important implications with respect to the natural history and treatment of HCV-related chronic liver disease in infected hemophiliacs worldwide.

Published
1995

34. Frequent reinfection and reactivation of hepatitis C virus genotypes in multitransfused hemophiliacs

Author

F. McOmish, L M Jarvis, Christopher A. Ludlam, Henry G. Watson, John F. Peutherer, and Peter Simmonds

Subjects
Serotype, Blood transfusion, Genotype, Hepacivirus, medicine.medical_treatment, Hepatitis C virus, Restriction Mapping, Blood Donors, Enzyme-Linked Immunosorbent Assay, medicine.disease_cause, Hemophilia A, Hemophilia B, Polymerase Chain Reaction, law.invention, law, Recurrence, medicine, Immunology and Allergy, Humans, Blood Transfusion, Polymerase chain reaction, Clotting factor, biology, business.industry, Hepatitis C, biology.organism_classification, medicine.disease, Virology, Infectious Diseases, Immunology, RNA, Viral, Virus Activation, business
Abstract

The frequency and dynamics of infection with different genotypes of hepatitis C virus were investigated in a cohort of hemophiliacs repeatedly exposed to non-virus-inactivated clotting factor. Among 63 infected hemophiliacs, genotype 1 (n = 38, subtypes 1a [27] and 1b [11]) was predominant; genotypes 2a (n = 1), 2b (n = 3), 3a (n = 20), and 5a (n = 1) accounted for the remainder. This distribution was similar to that found in Scottish blood donors from whom the infected blood products were manufactured. Hemophiliacs with severe disease were more likely to be polymerase chain reaction-positive than those with moderate or mild disease. Over 10 years, changes in the circulating major genotype and serotype were observed in 9 of 29 hemophiliacs and from one subtype to another in 3, although there was no clear trend toward replacement with any particular variant. Replacement occurred after the introduction of inactivated clotting factor in 4 subjects, implicating reactivation rather than reinfection. Those coinfected with human immunodeficiency virus were more likely to show a change in genotype.

Published
1994

35. Transfusion transmitted virus

Author

L M Jarvis, Peter Simmonds, and F Davidson

Subjects
biology, business.industry, Medicine, General Medicine, biology.organism_classification, business, Virology, Transfusion transmitted virus
Published
1998

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