Your search keyword '"Mun H"' showing total 23 results

1. Evaluation of antibody-based and nucleic acid-based assays for diagnosis of hepatitis E virus infection in a rhesus monkey model

Author

Ying Gu, Shao W. Li, Guo Y. Huang, Ning S. Xia, Ying J. Zheng, Jun Zhang, Zhi Q. He, Sheng X. Ge, Mun H. Ng, and Ying B. Wang

Subjects

Time Factors, Genotype, medicine.disease_cause, Virus, Incubation period, Feces, Antigen, Hepatitis E virus, Virology, medicine, Animals, Seroprevalence, Hepatitis Antibodies, Hepatitis, Base Sequence, biology, medicine.disease, Macaca mulatta, Hepatitis E, Infectious Diseases, Immunoglobulin M, Immunoglobulin G, DNA, Viral, Immunology, biology.protein, RNA, Viral, Viral disease, Antibody

Abstract

We have evaluated four hepatitis E virus (HEV) specific antibody assays, using sequential samples taken from 86 rhesus monkeys at intervals for up to 86 weeks after they had been infected with different doses of HEV. The animals are a common experimental model of hepatitis E. The large collection of sequential samples used avoids uncertainties encountered in previous studies regarding the precise infection status of study subjects and minimizes bias due to the individuality of response to infection. One assay (YES IgG) was produced with synthetic peptides; the others (E2 IgM, E2 IgG, and GL IgG) were produced with recombinant antigens. The results were compared with the viral RNA contents of the serum and stool samples and the occurrence of these virological and immunological markers in the course of the infection was temporally related to the development of hepatitis. Diagnostic utility of the markers was assessed according to their response rates and prevalence at different times in the course of infection. All the animals produced E2 IgG and developed viremia and all but one also produced E2 IgM and excreted the virus in stool, whereas response rates for the other antibodies were lower and decreased with virus dose. Hepatitis occurred over a period of 4 weeks between 3 and 7 weeks after infection. Virological activity occurred mainly during the incubation period and the prevalence of viral markers declined rapidly after the onset of hepatitis. Production of the E2 antibodies immediately preceded the onset of hepatitis, and this was followed about one week later by production of the other antibodies. Seroprevalence E2 IgM reached a peak value 3 weeks after the onset of hepatitis, whereas seroprevalence of GL IgG and YES IgG peaked after the disease had subsided. E2 IgG persisted in all animals for the entire duration of the experiment of up to 86 weeks and possibly beyond and, thus, can serve as a useful epidemiological marker of HEV infection.

Published

2003

2. A bacterially expressed peptide prevents experimental infection of primates by the hepatitis E virus

Author

Kui Li, Xiao Y. Che, Mun H. Ng, Stanley W.K. Im, Ji Z. Zhang, Wan F. Zhu, Hui Zhuang, Guo M. Xu, and Ning S. Xia

Subjects

Recombinant Fusion Proteins, viruses, Peptide, medicine.disease_cause, Peripheral blood mononuclear cell, Virus, Microbiology, Viral Envelope Proteins, Hepatitis E virus, Escherichia coli, medicine, Animals, Seroconversion, Immunization Schedule, Glutathione Transferase, chemistry.chemical_classification, General Veterinary, General Immunology and Microbiology, biology, Public Health, Environmental and Occupational Health, virus diseases, biology.organism_classification, Macaca mulatta, Virology, digestive system diseases, Caliciviridae, Hepatitis E, Infectious Diseases, Immunization, chemistry, Molecular Medicine, Peptides

Abstract

A 23 kDa peptide of the major structural protein of the hepatitis E virus (HEV) expressed in E. coli was found to naturally interact with one another to form homodimers and the peptide was recognized strongly in its dimeric form by HEV reactive human sera. To determine if the peptide may confer protection against HEV infection, three monkeys were immunized with the purified peptide and three were given placebo. Both groups of animals were challenged with 10(5) genome equivalent dose of the homologous strain of HEV. All control animals excreted the virus for 10-12 days beginning 5 days after the infection. The viral genome was also present in the peripheral blood monocyte (PBMC) samples from two animals, but it was not detected in the plasma samples from any of the animals. The infection in two control animals was accompanied by HEV seroconversion. Immunization was found to abrogate HEV stool excretion in two animals and reduced the viral excretion to one day in the third. None of the immunized animals showed detectable HEV in plasma or PBMC samples nor did the animals showed evidence of HEV seroconversion. These results suggested that immunization with the bacterially expressed peptide may prevent experimental infection of primates with the homologous strain of HEV.

Published

2001

3. Human herpesvirus-6 and human herpesvirus-7 infections in bone marrow transplant recipients

Author

Paul K.S. Chan, S. K. F. Lo, T. K. Chan, Yu-Lung Lau, Mun H. Ng, F. E. Chen, Raymond Liang, C. Y. Cheung, Joseph S. M. Peiris, and Kwok-Yung Yuen

Subjects

Human cytomegalovirus, Neutrophil Engraftment, biology, viruses, virus diseases, biochemical phenomena, metabolism, and nutrition, biology.organism_classification, medicine.disease, medicine.disease_cause, Virology, Herpesviridae, law.invention, Infectious Diseases, medicine.anatomical_structure, law, Betaherpesvirinae, Immunology, medicine, Human herpesvirus 6, Bone marrow, Nested polymerase chain reaction, Polymerase chain reaction

Abstract

Human cytomegalovirus (HCMV), human herpesvirus-6 (HHV-6), and human herpesvirus-7 (HHV-7) DNA in peripheral blood leukocytes (PBL) of 61 bone marrow transplant recipients was monitored weekly during the first 12 weeks post-transplantation by a nested polymerase chain reaction (PCR). Thirty-seven (61%), 17 (28%), and 32 (53%) of patients had one or more PBL specimens positive for HCMV, HHV-6 or HHV-7 DNA, respectively. HHV-7 DNA in PBL during the early post-transplant period was associated with a longer time to neutrophil engraftment (mean 28.8 days vs 19.8 days; P = 0.01). In two patients who failed to engraft, HHV-6 DNA and HHV-7 DNA was detected in plasma and PBL, respectively, early in their post-transplant period. Patients with HCMV disease were more likely to have concurrent HHV-7 DNA in PBL prior to onset of disease than were patients with asymptomatic HCMV infection, suggesting that HHV-7 may be a cofactor in the progression from HCMV infection to HCMV disease. In the 17 patients (179 specimens) in whom viral DNA in plasma was studied (in addition to PBL), a positive result was found only in 3. In each, viral DNA in plasma appeared to correlate with clinically significant disease. HHV-7 DNA in plasma was associated with encephalitis in an allograft recipient.

Published

1997

4. Purified recombinant EBV desoxyribonuclease in serological diagnosis of nasopharyngeal carcinoma

Author

KH Chan, Samira Debouze, Marie Claude Stolzenberg, Jonathan S.T. Sham, Abdelmadjid Bouguermouh, Mun H. Ng, D. Choy, and Tadamasa Ooka

Subjects

Cancer Research, medicine.diagnostic_test, biology, Immunofluorescence, medicine.disease_cause, medicine.disease, Epstein–Barr virus, Virology, Virus, Serology, law.invention, Oncology, Antigen, Nasopharyngeal carcinoma, law, hemic and lymphatic diseases, medicine, Recombinant DNA, biology.protein, Antibody

Abstract

To evaluate applications of highly purified recombinant EBV DNAase in the diagnosis and prognosis of NPC, we tested sera from patients with NPC, other EBV-associated diseases and EBV-seropositive and -seronegative healthy subjects by immunoblotting and DNAase inhibitory assay. The results were compared with those obtained by the conventional immunofluorescence assays against the EBV-specified early antigens and capsid antigens. The antigenic specificity of the immunoblotting assay for IgG antibody against the viral enzyme, but not that for the IgA antibody, was correlated with DNAase-inhibitory activity of the sera and their titers of IgG antibodies against the viral early antigens. Purified IgA as well as IgG from NPC sera inhibited enzyme activity with similar efficiency. The use of highly purified viral DNase has increased the sensitivity of detection of the corresponding antibodies by immunoblotting, with the IgG antibody being detected in all but one, and IgA antibody in all but 2, of the 174 NPC sera tested. The IgG antibody was also commonly detected in the other groups of control sera, while the IgA antibody was detected in about 10% of African Burkitt's lymphoma and Algerian Hodgkin's lymphoma patients and less than 3% of the other control subjects. These results suggest that IgA antibody against recombinant EBV DNAase may be useful in the diagnosis of NPC, but the level of this antibody did not appear to be related to clinical stages of this cancer.

Published

1996

5. Follow-up study of acute hepatitis C

Author

Stanley W.K. Im, Mun H. Ng, W. W. Peng, and D. Tan

Subjects

Adult, Male, China, medicine.medical_specialty, Blood transfusion, medicine.medical_treatment, Hepatitis C virus, Molecular Sequence Data, Disease, medicine.disease_cause, Polymerase Chain Reaction, Serology, Immunoenzyme Techniques, Medical microbiology, Virology, medicine, Humans, Hepatitis Antibodies, Seroconversion, Base Sequence, biology, Patient Selection, virus diseases, Alanine Transaminase, General Medicine, Middle Aged, Hepatitis C, digestive system diseases, Acute Disease, biology.protein, RNA, Viral, Female, Viral disease, Antibody, Biomarkers, Follow-Up Studies

Abstract

An extended follow-up study of hepatitis C virus (HVC) infection was conducted in Guangzhou and its nearby regions on patients hospitalized with acute hepatitis. Routine screening of blood donors for HCV was not yet instituted at the time of this study. HCV was found to be a common cause of the disease, and the infection had a close association with recent histories of blood transfusion. Sequential sera obtained from patients during hospitalization and after discharge were tested for the presence of HCV antibodies by the first and the second generation of commercial test kits, for levels of alanine aminotransferase (ALT), and for the presence of HCV-RNA. The development of HCV antibodies in some of the patients may be delayed for protracted period following clinical onset. HCV-RNA was only intermittently detectable both before and after seroconversion. Six of 33 patients studied showed seroreversion and 5 of them were accompanied by loss of HCV-RNA and serum ALT returned to normal levels. The disease persisted in 24 of 27 patients without seroreversion, accompanied by intermittent detection of HCV-RNA throughout the protracted course of the infection. Our results indicate that both EIA for detection of HCV antibodies and PCR for serum HCV-RNA should be used in combination for reliable diagnosis of HCV infection and screening of blood for transfusion.

Published

1994

6. Development and Evaluation of an Epstein-Barr Virus (EBV) Immunoglobulin M Enzyme-Linked Immunosorbent Assay Based on the 18-Kilodalton Matrix Protein for Diagnosis of Primary EBV Infection

Author

Honglin Chen, Kwok-Hung Chan, Mun H. Ng, R. X. Luo, Joseph S. M. Peiris, and Wing-Hong Seto

Subjects

Microbiology (medical), Epstein-Barr Virus Infections, Herpesvirus 4, Human, Recombinant Fusion Proteins, Enzyme-Linked Immunosorbent Assay, Antibodies, Viral, medicine.disease_cause, Sensitivity and Specificity, Herpesviridae, Virus, Serology, Viral Matrix Proteins, Virology, hemic and lymphatic diseases, medicine, Humans, Gammaherpesvirinae, Antigens, Viral, Epstein–Barr virus infection, DNA Primers, Base Sequence, biology, medicine.disease, biology.organism_classification, Epstein–Barr virus, Molecular biology, Molecular Weight, Immunoglobulin M, Evaluation Studies as Topic, biology.protein, Capsid Proteins, Antibody

Abstract

A new immunoglobulin M (IgM) enzyme-linked immunosorbent assay (ELISA) based on the recombinant Epstein-Barr virus (EBV) matrix protein was developed. Compared to indirect immunofluorescence for the detection of IgM antibody to the EBV capsid antigen on clinical specimens, the sensitivity and specificity of the new IgM ELISA were 96 and 96%, respectively.

Published

1998

7. A bacterially expressed particulate hepatitis E vaccine: antigenicity, immunogenicity and protectivity on primates

Author

Jun Zhang, Shao W. Li, Sheng X. Ge, Shu Q. Pang, Guo Y. Huang, Yang L. Xian, Ning S. Xia, Mun H. Ng, Yi M. Li, Zhi Q. He, and Shan H. Ou

Subjects

Viral Hepatitis Vaccines, Antigenicity, medicine.drug_class, medicine.medical_treatment, Biology, Monoclonal antibody, medicine.disease_cause, Virus, Microbiology, Hepatitis E virus, medicine, Animals, Hepatitis, General Veterinary, General Immunology and Microbiology, Immunogenicity, Public Health, Environmental and Occupational Health, medicine.disease, Virology, Macaca mulatta, Hepatitis E, Infectious Diseases, Capsid, Molecular Medicine, Electrophoresis, Polyacrylamide Gel, Adjuvant

Abstract

It was evaluated its antigenicity, immunogenicity and efficacy of a candidate recombinant hepatitis E virus (HEV) vaccine, referred hitherto as HEV 239 vaccine. The vaccine peptide has a 26 amino acids extension from the N terminal of another peptide, E2, of the HEV capsid protein, which has been shown to protect monkeys against HEV infection previously. The vaccine peptide is similar as E2 in that: first, the vaccine peptide migrates predominantly as dimer in SDS-PAGE and it is dissociated into monomers by heating; second, its dimeric form of which predominantly recognized by HEV reactive human serum; and third, it shows the same pattern of reaction as E2 with a panel of eight monoclonal antibodies that had been raised against E2. In contrast to E2, the vaccine peptide aggregates to form particles of 13 nm mean radius, and consequently, it is more than 240 times more immunogenic than E2. Using alum as adjuvant, immunizing dose determined in mice was 80-250 ng for the vaccine and >60 microg for E2. Rhesus monkeys twice vaccinated with a 10 microg or a 20 microg formulation of this vaccine showed essentially the same antibody response, whereas the response to a 5 microg formulation was delayed but reached similar antibody levels. All the three vaccine formulations afford complete protection against infection with 10(4) genome equivalent dose of the homologous genotype 1 virus. At higher virus dose of 10(7), the same vaccine formulation partially protected against the infection and completely protected against hepatitis. The efficacy of the vaccine was essentially the same for the homologous genotype 1 virus and heterologous genotype 4 virus.

Published

2004

8. Analysis of hepatitis E virus neutralization sites using monoclonal antibodies directed against a virus capsid protein

Author

Hui Zhuang, Shao W. Li, Ying Gu, Jun Zhang, Zhi Q. He, Guo Y. Huang, Sheng X. Ge, Ning S. Xia, and Mun H. Ng

Subjects

medicine.drug_class, viruses, Blotting, Western, Enzyme-Linked Immunosorbent Assay, Biosensing Techniques, Biology, Monoclonal antibody, medicine.disease_cause, Virus, Neutralization, Epitope, Epitopes, Mice, Hepatitis E virus, Neutralization Tests, medicine, Animals, DNA Primers, Infectivity, Mice, Inbred BALB C, General Veterinary, General Immunology and Microbiology, Base Sequence, Public Health, Environmental and Occupational Health, Antibodies, Monoclonal, Virology, Molecular biology, Infectious Diseases, Capsid, biology.protein, Molecular Medicine, Capsid Proteins, Antibody

Abstract

The dimeric form of the recombinant peptide (E2), comprising amino acid 394-606 of the capsid protein of hepatitis E virus (HEV), is strongly recognized by HEV reactive human serum, and when used as a vaccine, it protects rhesus monkeys against experimental HEV infection. In this work, the relationship of E2 to HEV has been probed using three murine monoclonal antibodies, 8C11, 13D8 and 8H3, all of which react predominantly against the E2 dimer, and can effect immune capture of the virus as well. 8C11 and 8H3 were further found to neutralize HEV infectivity in animals. Cross-blocking patterns between these antibodies discerned two spatially separate antigenic domains, one identified by 8C11 and 13D8, and the other, by 8H3. Kinetic studies using BIAcore biosensor suggest that the epitope to which 8H3 is directed is partially masked, and thus has limited access by the native antibody. However, this is not the case with the smaller Fab. Access to the 8H3 epitope was enhanced by the binding of 8C11, and inhibited by the binding of 13D8 to a distal site on the peptide. Similar to the effects of binding 8H3 to E2, 8C11 was found to enhance immune capture by 8H3, while 13D8 was inhibitory. Moreover, 8C11 and 8H3 act synergistically to neutralize HEV infectivity. The parallel cross-reaction patterns that these antibodies exhibit against the peptide and the virus, respectively, implicate two interacting conformationally dependent neutralization sites on the HEV particle. These sites might cooperate in the adsorption and penetration of the HEV virus.

Published

2004

9. Selection pressure-driven evolution of the Epstein-Barr virus-encoded oncogene LMP1 in virus isolates from southeast Asia

Author

Geoff Connolly, Scott R. Burrows, Jacqueline M. Burrows, Denis J. Moss, Judy Tellam, Megan Woolfit, Leanne Cooper, Sofia Mubarika Haryana, Lindell Bromham, Gwenael Piganeau, Mun H. Ng, Natasha Webb, John M. Nicholls, L M Poulsen, and Rajiv Khanna

Subjects

Mitochondrial DNA, Epstein-Barr Virus Infections, Herpesvirus 4, Human, Immunology, Molecular Sequence Data, Viral Oncogene, Biology, Southeast asian, Viral Matrix Proteins - genetics, Microbiology, Genetic analysis, Virus, Transformation and Oncogenesis, Cell Line, Viral Matrix Proteins, Evolution, Molecular, Virology, medicine, otorhinolaryngologic diseases, Humans, Herpesvirus 4, Human - genetics - isolation & purification, Amino Acid Sequence, Lymphocytes, Selection, Genetic, Gene, Asia, Southeastern, Phylogeny, Genetics, Phylogenetic tree, Nasopharyngeal Neoplasms - virology, Nasopharyngeal Neoplasms, medicine.disease, Selection (Genetics), stomatognathic diseases, Nasopharyngeal carcinoma, Insect Science

Abstract

The geographically constrained distribution of Epstein-Barr virus (EBV)-associated nasopharyngeal carcinoma (NPC) in southeast Asian populations suggests that both viral and host genetics may influence disease risk. Although susceptibility loci have been mapped within the human genome, the role of viral genetics in the focal distribution of NPC remains an enigma. Here we report a molecular phylogenetic analysis of an NPC-associated viral oncogene, LMP1, in a large panel of EBV isolates from southeast Asia and from Papua New Guinea, Africa, and Australia, regions of the world where NPC is and is not endemic, respectively. This analysis revealed that LMP1 sequences show a distinct geographic structure, indicating that the southeast Asian isolates have evolved as a lineage distinct from those of Papua New Guinea, African, and Australian isolates. Furthermore, a likelihood ratio test revealed that the C termini of the LMP1 sequences of the southeast Asian lineage are under significant positive selection pressure, particularly at some sites within the C-terminal activator regions. We also present evidence that although the N terminus and transmembrane region of LMP1 have undergone recombination, the C-terminal region of the gene has evolved without any history of recombination. Based on these observations, we speculate that selection pressure may be driving the LMP1 sequences in virus isolates from southeast Asia towards a more malignant phenotype, thereby influencing the endemic distribution of NPC in this region., published_or_final_version

Published

2004

10. Molecular diversity of Epstein-Barr virus IgG and IgA antibody responses in nasopharyngeal carcinoma: a comparison of Indonesian, Chinese, and European subjects

Author

Dewi Kartikawati Paramita, Mun H. Ng, Bambang Hariwiyanto, Jaap M. Middeldorp, Sofia Mubarika Haryana, Tabitha Schouten, Jajah Fachiroh, Ahmad Harijadi, Pathology, CCA - Cancer immunology, CCA - Target Discovery & Preclinial Therapy Development, CCA - Biomarkers, CCA - Evaluation of Cancer Care, AII - Infectious diseases, and AII - Cancer immunology

Subjects

Immunoglobulin A, Epstein-Barr Virus Infections, Herpesvirus 4, Human, Nasopharyngeal neoplasm, Enzyme-Linked Immunosorbent Assay, medicine.disease_cause, Immunofluorescence, Antibodies, Viral, Immunoglobulin G, White People, Antigen, Asian People, hemic and lymphatic diseases, medicine, otorhinolaryngologic diseases, Immunology and Allergy, Humans, Antigens, Viral, biology, medicine.diagnostic_test, Carcinoma, Genetic Variation, Nasopharyngeal Neoplasms, medicine.disease, Virology, Epstein–Barr virus, Europe, stomatognathic diseases, Infectious Diseases, Nasopharyngeal carcinoma, Epstein-Barr Virus Nuclear Antigens, Indonesia, Immunology, biology.protein, Hong Kong, Capsid Proteins, Antibody

Abstract

Epstein-Barr virus (EBV)-specific immunoblot analysis was used to reveal the molecular diversity of immunoglobulin (Ig) G and IgA antibody responses against Epstein-Barr nuclear antigen (EBNA), early antigen (EA), and viral capsid antigen (VCA) in serum samples from patients with nasopharyngeal carcinoma (NPC) and control subjects, by use of immunofluorescence assay (IFA). Control donors (n=150) showed IgG responses to few EBV proteins--VCA-p18, VCA-p40, EBNA1, and Zebra--and sporadically weak IgA reactivity to EBNA1 and VCA-p18. Patients with NPC stage 1 (n=6) had similar response patterns. Patients with NPC stage 2-4 (n=132) showed significantly more diverse IgG and IgA responses to EA and VCA proteins--VCA-p18/-p40, EBNA1, Z-encoded broadly reactive activator, and EAd-p47/54, -DNAse, -thymidine kinase, and -p138. No correlation was found between IFA titers and the number of EBV proteins recognized by IgG or IgA. Our results reveal dissimilarity between EBV polypeptides recognized by IgG and IgA antibodies, which suggests independent B cell triggering events.

Published

2003

11. Epstein-Barr Virus (EBV) DNA in Sera of Patients with Primary EBV Infection

Author

Kwok-Hung Chan, Wing-Hong Seto, Mun H. Ng, and Joseph S. M. Peiris

Subjects

Microbiology (medical), Epstein-Barr Virus Infections, Herpesvirus 4, Human, medicine.disease_cause, Polymerase Chain Reaction, Sensitivity and Specificity, Herpesviridae, Virus, chemistry.chemical_compound, Predictive Value of Tests, Positive predicative value, hemic and lymphatic diseases, Virology, Medicine, Gammaherpesvirinae, Humans, Epstein-Barr Virus Infections - diagnosis - virology, Herpesvirus 4, Human - genetics - isolation & purification, Polymerase Chain Reaction - methods, biology, business.industry, biology.organism_classification, Ebv infection, Epstein–Barr virus, chemistry, Immunology, DNA, Viral, business, DNA, DNA, Viral - blood

Abstract

Detection of Epstein-Barr Virus (EBV) DNA by PCR in serum had a sensitivity of 80%, a specificity of 94%, and positive and negative predictive values of 95 and 79%, respectively, for the diagnosis of primary EBV infection. We suggest that this is a useful addition to the panel of tests used for this purpose., published_or_final_version

Published

2001

12. Conformational antigenic determinants generated by interactions between a bacterially expressed recombinant peptide of the hepatitis E virus structural protein

Author

Ningshao Xia, Mun H. Ng, Ji-Zhong Zhang, Stanley W.K. Im, X. Y. Che, Sik To Lai, S. H. Lau, and Tai Nin Chau

Subjects

viruses, Blotting, Western, Peptide, Molecular cloning, Biology, medicine.disease_cause, Epitope, Virus, law.invention, Epitopes, Open Reading Frames, Antigen, Hepatitis E virus, law, Virology, medicine, Escherichia coli, Animals, Humans, Hepatitis Antibodies, chemistry.chemical_classification, Viral Structural Proteins, Immune Sera, Hepatitis Antigens, Recombinant Proteins, Hepatitis E, Infectious Diseases, Biochemistry, Capsid, chemistry, Recombinant DNA, Rabbits

Abstract

A 23 kDa peptide locating to amino acid residues 394 to 604 of the major Hepatitis E Virus (HEV) structural protein was expressed in E. coli. This peptide was found to interact naturally with one another to form homodimers and it was recognized strongly and commonly in its dimeric form by HEV reactive human sera. The antigenic activity associated with the dimeric form was abrogated when the dimer was dissociated into monomer and the activity was reconstituted after the monomer was re-associated into dimer again. The dimeric form of the peptide elicited a vigorous antibody response in experimental animals and the resulting antisera were found to cross-react against HEV, effecting an efficient immune capture of the virus. These results attributed the antigenic activity associated with the dimeric form of the peptide to conformational antigenic determinants generated as a result of interaction between the peptide molecules. It is suggested that some of these antigenic determinants may be expressed by the HEV capsid and raised the possibility of this bacterially expressed peptide as an HEV vaccine candidate.

Published

2001

13. Epstein-Barr virus (EBV) infection in infancy

Author

Joseph S. M. Peiris, W.H Seto, John S. Tam, Kwok-Hung Chan, and Mun H. Ng

Subjects

Male, Epstein-Barr Virus Infections, Herpesvirus 4, Human, Mononucleosis, medicine.disease_cause, Antibodies, Viral, Herpesviridae, Serology, Capsid, Seroepidemiologic Studies, Virology, medicine, Gammaherpesvirinae, Humans, Longitudinal Studies, Seroconversion, Subclinical infection, biology, business.industry, Infant, Newborn, biology.organism_classification, medicine.disease, Fetal Blood, Epstein–Barr virus, Infectious Diseases, Epstein-Barr Virus Nuclear Antigens, Immunology, Hong Kong, Female, Viral disease, business

Abstract

Background: Epstein–Barr virus (EBV) has been shown to be the cause of infectious mononucleosis (IM) and has more complicated associations with several malignant diseases. These EBV associated diseases provide a strong incentive for the development of an EBV vaccine. Most primary EBV infection during infancy and early childhood is mild or subclinical. Little is known about its infection in infancy. The pattern of EBV serological response during infancy may be important for vaccine management. Objectives: this study has served to clarify the epidemiology and serology of primary EBV infection during early infancy. Study design: longitudinal serum samples from 66 Hong Kong infants were tested for EBV antibodies by immunofluorescence. Cord blood and sequential serum samples from these infants were taken at birth and then at 4-month intervals up to 2 years of age. Results: maternal antibodies were present at different levels in all cord blood specimens and in serum samples of 8 infants at 4-month of age. Evidenced by VCA-IgG seroconversion, 60.6% (40/66) infants were infected during the first 2 years of life. One episode occurred before 8 months of age but, thereafter and for the remaining 16 months of follow-up until the infants were 2 years of age, the infection occurred at essentially a constant rate affecting about 20% of the remaining seronegative infants every 4 months. Conclusions: the abrupt onset of the infection after a delay of 8 months is a remarkable feature of primary EBV infection during infancy, which implicates a protective role for maternal antibodies. Persisting maternal antibodies may additionally serve to contain the infection once it occurred. This may partly explain why, unlike during adolescence, primary EBV infection early in life is usually asymtomatic.

Published

2001

14. Seroprevalence of antibodies to human herpesviruses in England and Hong Kong

Author

Yu-Lung Lau, R. B. Heath, Mun H. Ng, C. Y. Yeung, H. K. Osman, and Hillar O. Kangro

Subjects

Human cytomegalovirus, Adult, Herpesvirus 3, Human, Herpesvirus 4, Human, Adolescent, viruses, Herpesvirus 6, Human, Cytomegalovirus, medicine.disease_cause, Antibodies, Viral, Herpesviridae, Serology, Virology, Medicine, Gammaherpesvirinae, Seroprevalence, Humans, Simplexvirus, Child, biology, business.industry, Varicella zoster virus, Age Factors, Infant, Newborn, virus diseases, Infant, medicine.disease, biology.organism_classification, Infectious Diseases, England, Child, Preschool, Immunology, Hong Kong, Human herpesvirus 6, business

Abstract

The age-related prevalence of antibodies to herpesviruses was compared in England and Hong Kong. Altogether 327 sera from England and 266 sera from Hong Kong were tested for antibodies to herpes simplex virus (HSV), varicella-zoster virus (VZV), Epstein-Barr virus (EBV), cytomegalovirus (CMV), and human herpesvirus 6 (HHV-6). Herpesvirus infections were common in both countries but generally were acquired earlier and were more prevalent in Hong Kong. Over 90% of children in Hong Kong were infected with VZV, EBV, and HHV-6 by 8 years of age. HSV and CMV were the least prevalent childhood infections in both countries, although, 30–40% of babies in Hong Kong became infected during the first year of life. CMV infections were rare throughout childhood in the English cohort. Overcrowding and early attendance at kindergarten may aid more efficient and earlier transmission of herpesvirus in Hong Kong. The high prevalence of CMV in particular may have implications for the management of young pregnant women and organ transplant recipients in Hong. © 1994 Wiley-Liss, Inc.

Published

1994

15. P.336 Hepatitis E virus infection in rural communities of southern China

Author

Q.S. Guo, Jun Zhang, Y.P. Li, Y. Nong, Shengxiang Ge, R.C. Li, Mun H. Ng, Ningshao Xia, and Y.J. Zheng

Subjects

Infectious Diseases, Southern china, Virology, Biology, Hepatitis E virus infection

Published

2006

16. A study on Epstein Barr Virus receptor activity in cell free extracts of human lymphoblastoid cells

Author

Sylvia W. L. Lui, K. H. Chan, and Mun H. Ng

Subjects

Herpesvirus 4, Human, Binding Sites, Cell-Free System, Lymphoblast, Sonication, General Medicine, Biology, medicine.disease_cause, Trypsin, Burkitt Lymphoma, Epstein–Barr virus, Virology, DNA-binding protein, Cell Line, Neoplasm Proteins, Raji cell, hemic and lymphatic diseases, medicine, Humans, Adsorption, Ploidy, Receptor, Antigens, Viral, medicine.drug

Abstract

Epstein Barr Virus (EBV) receptor activity in cell free extracts is operationally defined as one which causes a reduction in the effective concentration of the early antigen inducing particles of an EBV preparation when the latter is preincubated with the extract before infection. Such activity was detected in the surface extract of Raji cells and to a lesser extent in that of BJAB cells, both of which are B lymphoblastoid cells that are susceptible to infection with EBV. Receptor activity was not detected in similar extracts of P3HR-1 cells and human diploid fibroblasts neither of which are known to be susceptible to EBV infection. Receptor activity in the Raji cell extract was found to be associated with membranous structures. This may have rendered the activity resistant to treatment with trypsin and sonication. The activity was however abrogated if the extract was exposed to neutral detergent. Binding of receptor activity was observed when Raji cell extract was chromatographed on a column of immobilized EBV. Subsequent electrophoretic analysis showed however that this procedure did not result in an appreciable purification of the receptor activity. Neutral detergent treated extract was similarly chromatographed. The resulting eluates did not contain detectable receptor activity but were less heterogeneous in protein content as compared with that of the original extract. It is not certain at present if these EBV binding proteins are involved in the receptor activity of the extract.

Published

1978

17. Glycoproteins and sialyl transferase of human B lymphoblastoid cell lines

Author

Mun H. Ng and Sylvia W. L. Lui

Subjects

Herpesvirus 4, Human, Neuraminidase, Biology, Galactose Oxidase, Cell Line, Viral Proteins, chemistry.chemical_compound, Transferases, Virology, Neuraminic acid, Humans, Transferase, Glycoproteins, chemistry.chemical_classification, B-Lymphocytes, Lymphoblast, Periodic Acid, General Medicine, Burkitt Lymphoma, Molecular biology, Sialyltransferases, Neoplasm Proteins, Molecular Weight, chemistry, Biochemistry, Lymphoblastoid cell, Galactose oxidase, Neuraminic Acids, Cell Surface Glycoproteins, Glycoprotein

Abstract

We used two radiolabeling methods to study glycoproteins on the surface of lymphoblastoid cells. One of the methods affects tritiation of residues which are oxidized with galactose oxidase and the other causes tritiation of neuraminic acid residues. This approach was shown to allow a better resolution of cell surface glycoproteins than if either method were used alone. Glycoproteins of B1--19 cells which harbor the Epstein-Barr virus genomes were compared with those of its parental cell line, BJAB, which does not harbor the viral genomes. These studies did not reveal a unique viral protein. A 28,000 mol. wt. glycoprotein was found to be the most prominent neuraminic acid-labeled product of B1--19 cells and also of the two other cell lines, Raji and Ly38, which harbor the EBV genomes. A similar molecular weight species from BJAB cells identified by galactose oxidase labeling might be deficient in neuraminic acid residues as it was poorly labeled by the periodate oxidation method. The neuraminic acid content and level of sialyl transferase of BJAB cells were found to be lower than those of the other cell lines studied.

Published

1980

18. Post-Transcriptional Control of Interferon Synthesis

Author

Mun H. Ng and Jan Vilcek

Subjects

Time Factors, Polynucleotides, Immunology, Stimulation, Cycloheximide, Biology, Kidney, Microbiology, Vesicular stomatitis Indiana virus, chemistry.chemical_compound, Leucine, Interferon, Culture Techniques, Virology, Genes, Regulator, Animal Viruses, medicine, Protein biosynthesis, Animals, RNA, Messenger, Molecular Biology, Carbon Isotopes, Messenger RNA, Dactinomycin, Protein synthesis inhibitor, Staining and Labeling, Translation (biology), Molecular biology, Stimulation, Chemical, Culture Media, Poly I-C, chemistry, Genetic Code, Protein Biosynthesis, Insect Science, Interferons, Rabbits, medicine.drug

Abstract

Low to moderate doses of cycloheximide had a stimulatory effect on interferon production in rabbit kidney cell cultures treated with double-stranded polyinosinate-polycytidylate (poly I:poly C). A very marked stimulation occurred in the presence of a dose of cycloheximide inhibiting amino acid incorporation into total cellular protein by about 75%. Higher doses of cycloheximide caused a shift in interferon release towards later intervals and a gradual decrease in the overall degree of stimulation. An even greater increase in the amount of interferon produced was observed if cells were treated with cycloheximide for only 3 to 4 hr immediately after their exposure to poly I:poly C. Under the latter conditions, a rapid burst of interferon production occurred after the reversal of cycloheximide action. Treatment with a high dose of actinomycin D before the reversal of cycloheximide action caused a further increase and a marked prolongation of interferon production. It is postulated that inhibitors of protein synthesis suppress the accumulation of a cellular regulatory protein (repressor) which interacts with the interferon messenger ribonucleic acid mRNA and thereby prevents its translation. Therefore, active interferon mRNA can apparently accumulate in rabbit kidney cells which, after exposure to poly I:poly C, are kept in the presence of an inhibitor of protein synthesis. Some of this accumulated interferon mRNA can be translated during a partial block of cellular protein synthesis, but its most efficient translation occurs after the reversal of the action of the protein synthesis inhibitor.

Published

1971

19. Heterocomplexes of human interferon and immunoglobulins: formation and properties

Author

K. P. Fung and Mun H. Ng

Subjects

Immunoglobulins, Cell Line, chemistry.chemical_compound, Mice, Cytopathogenic Effect, Viral, Interferon, Virology, medicine, Animals, Humans, Sodium dodecyl sulfate, Gel electrophoresis, Dactinomycin, biology, Molecular mass, General Medicine, Molecular biology, Molecular Weight, Biochemistry, chemistry, Cell culture, Glutaral, biology.protein, Glutaraldehyde, Interferons, Antibody, medicine.drug

Abstract

To form heterocomplexes, human diploid fibroblast interferon was reacted with an excess of human immunoglobulin in the presence of an optimal concentration of glutaraldehyde. There was virtually no loss of interferon activity due to this treatment and the resulting heterocomplexes possessed the biological properties of both native interferon and immunoglobulin molecules. The apparent molecular weights determined by gel electrophoresis in the presence of sodium dodecyl sulfate were 20,000 for native interferon and 0.5 to 1 X 10(6) for the heterocomplex. Native interferon injected into mice intramuscularly had a serum half life of about 5 hours. However, serum interferon was not detected in mice receiving a similar dose of the heterocomplex.

Published

1978

20. Antigenic content of an in vitro cellular immunity reactive cell surface extract of Raji cells

Author

Mun H. Ng, H. C. Ho, and W.S. Ng

Subjects

Cellular immunity, Herpesvirus 4, Human, Cell, Fluorescent Antibody Technique, Cell Line, HeLa, Antigen, Immunity, Antigens, Neoplasm, hemic and lymphatic diseases, Virology, medicine, Leukocytes, Humans, Antigens, Viral, Immunity, Cellular, Blood Cells, biology, General Medicine, Fibroblasts, biology.organism_classification, Burkitt Lymphoma, In vitro, Cell biology, Raji cell, medicine.anatomical_structure, Antigens, Surface, Clone (B-cell biology), Subcellular Fractions

Abstract

Antigenic content of a Raji cell surface extract (TS) was studied by sequential abosrption of rabbit antiserum to this extract with different cells. Anti-TS was first allowed to react exhaustively with human blood cells followed by HeLa cells and human diploid fibroblasts. The residual reactivity was studied by stepwise absorption with an EBV-negative B lymphoblastoid cell line, BJAB, and then with B1--19, a clone derived from EBV transformed BJAB cells. These processes delineated three kinds of reactivities in anti-TS having specificities for antigens on B blasts, EBV-determined cell surface antigen(s) and antigens that are exclusive to Raji cells, respectively. These results are compatible with the heterogeneous protein content of TS and with the results of our earlier in vitro cell-mediated immunity studies using a similar preparation of Raji cell TS.

Published

1978

21. Interferons: Physicochemical Properties and Control of Cellular Synthesis

Author

Mun H. Ng and Jan Vilcek

Subjects

Interferon production, Interferon inducer, Viral replication, Biochemistry, Cellular synthesis, Interferon, medicine, Biology, Virology, medicine.drug

Abstract

Publisher Summary Interferons are a class of protein capable of suppressing viral replication in competent animal cells. They are produced by a variety of animal cells in response to stimulation with a fairly wide range of materials. This characteristic cell-mediated antiviral action of interferons has proved to be the most useful parameter for the definition of interferons. This chapter reviews information on the general aspects of interferon production and action. It also focuses on the known physicochemical properties of interferons and control of the cellular synthesis of interferons. The chapter also discusses interferon induction by viruses and other agents. Although interferons had once been considered specific products of cell-virus interaction, more recent evidence shows that interferon production by animal cells can also be stimulated by a number of other agents. The still growing list of nonviral interferon inducers includes complex infectious agents, as well as relatively simple chemicals. The relationship between the structure and activity of polynucleotide interferon inducers is also discussed in the chapter.

Published

1972

22. Membrane-bound intracellular interferon in rabbit kidney cell cultures

Author

Brian Berman, Mun H. Ng, and Jan Vilcek

Subjects

Cytoplasm, Time Factors, Membrane bound, Biology, Cell Fractionation, Kidney, Tritium, Vibration, Cell Line, Choline, Interferon, Virology, Rabbit kidney, medicine, Centrifugation, Density Gradient, Animals, Trypsin, Cycloheximide, Uridine, Carbon Isotopes, Cell Membrane, Cell biology, Poly I-C, Cell culture, Interferons, Rabbits, Ribosomes, Intracellular, medicine.drug

Published

1972

23. Potentiation of the action of interferon by extracts of Escherichia coli

Author

Mun H. Ng and Jan Vilcek

Subjects

Dactinomycin, Plant Extracts, Long-term potentiation, Biology, Vesicular stomatitis Indiana virus, medicine.disease_cause, Microbiology, Interferon, Virology, Viral Interference, medicine, Escherichia coli, Interferons, medicine.drug

Published

1967