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2. Hepatitis C: looking at a virus that hasn't been seen.

Author

Overby LR

Subjects
Amino Acid Sequence, Hepacivirus immunology, Hepatitis Antibodies blood, Hepatitis C Antibodies, Humans, Molecular Sequence Data, RNA, Viral genetics, Genome, Viral, Hepacivirus genetics
Abstract

Hepatitis C (HCV) is the first virus to be discovered by molecular cloning without direct use of biological or biophysical methods. HCV was first recognised in 1974 as non-A, non-B (NANB) hepatitis resulting from blood transfusions. It took almost 15 years to identify it successfully--by detecting a clone in a library of cDNA prepared from the nucleic acids extracted from plasma known to be infectious for chimpanzees. The clone was derived from a positive-sense RNA of about 10,000 nucleotides, with a long open reading frame encoding for a polyprotein of about 3000 amino acids. The structure of the RNA and the encoded polyprotein had properties similar to known flaviviruses and pestiviruses. Functions of viral proteins produced by proteolytic cleavage of the polyprotein are estimated by analogy with known viruses of similar genomic organisation. Each of the HCV proteins has been produced in recombinant organisms and used as an antigen in immunoassays to investigate serological responses during the course of infection. Seroconversions to both structural and non-structural antigens are observed during the course of disease but typical diagnostic serological patterns have not yet evolved. Immunoassays for HCV antibodies reacting with recombinant antigens are used widely for screening blood donations and for studying the epidemiology of HCV infection. Comparisons of the nucleic acid sequences from different isolates of HCV have shown considerable variability throughout the genome. The importance of this genomic heterogeneity will be a challenging problem for the future.

Published
1993
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3. Hepatitis C virus: the major causative agent of viral non-A, non-B hepatitis.

Author

Choo QL, Weiner AJ, Overby LR, Kuo G, Houghton M, and Bradley DW

Subjects
Amino Acid Sequence, Animals, Antibodies, Viral analysis, Base Sequence, Hepatitis Viruses immunology, Humans, Molecular Sequence Data, Viral Proteins genetics, DNA, Viral genetics, Hepatitis C microbiology, Hepatitis Viruses genetics, Hepatitis, Viral, Human microbiology
Abstract

A 'blind' recombinant immunoscreening approach, of general application to studies of infectious diseases, was used to clone and identify the genome of the previously uncharacterized non-A, non-B hepatitis (NANB) virus. This agent is a positive-stranded RNA virus that appears to be distantly related to the flaviviridae family. A recombinant viral antigen (C100-3) was used to develop a capture assay for circulating antibody. Data obtained using this assay indicate that this agent, termed the hepatitis C virus (HCV), is the major cause of post-transfusion, community-acquired and cryptogenic, NANB. Anti-C100-3 antibody appears to be directed towards dominant, non-structural viral epitopes. It is a non-neutralising antibody that develops generally late in infection and is a particularly good marker of chronic, persistent viraemia. Many asymptomatic but infectious blood donors can now be detected using this antibody assay. HCV is associated with the development of hepatocellular carcinoma and possibly, other liver diseases.

Published
1990
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4. Properties of soluble DNA polymerase from sera of hepatitis B virus carriers.

Author

Mao JC, Otis ER, Mushahwar IK, and Overby LR

Subjects
DNA-Directed DNA Polymerase analysis, DNA-Directed DNA Polymerase isolation & purification, Hepatitis B immunology, Hepatitis B Surface Antigens analysis, Humans, Isoelectric Point, Molecular Weight, Solubility, Carrier State enzymology, DNA-Directed DNA Polymerase blood, Hepatitis B enzymology
Abstract

A soluble DNA polymerase was purified 8,000-fold from hepatitis B surface antigen positive serum. The molecular weight of the enzyme by gel filtration was about 1.60 X 10(5), the sedimentation coefficient was 5.5S, the apparent Km for dTTP was 4 micrometer, the optimum pH in the presence of Mg2+ was 9.2, and the pl was 4.7. The enzyme was found in HBsAg-positive sera and required an external primer for activity. The properties of the DNA polymerase were different from hepatitis B virus particle enzyme and from vertebrate and bacterial DNA polymerases. The prevalence of this enzyme did not correlate with HBeAg or particle DNA polymerase in HBsAg-positive sera.

Published
1981
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5. Diagnosis of acute hepatitis A by HAVAB-M, a direct radioimmunoassay for IgM anti-HAV.

Author

Decker RH, Kosakowski SM, Vanderbilt AS, Ling CM, Chairez R, and Overby LR

Subjects
Acute Disease, Animals, Antibodies, Viral biosynthesis, Antibody Specificity, Cross Reactions, Dose-Response Relationship, Immunologic, Goats, Humans, Liver immunology, Mercaptoethanol pharmacology, Quality Control, Radioimmunoassay, Rheumatoid Factor immunology, Antigens, Viral, Hepatitis A diagnosis, Hepatovirus immunology, Immunoglobulin M
Abstract

A three-step solid-phase radioimmunoassay, HAVAB-M, was developed for use in clinical labs as an aid to diagnosing hepatitis A. Polystyrene beads were coated with anti-human IgM (mu-chain specific) and were incubated successively with serum specimen, HAV, and anti-HAV 125I. HAVAB-M was used to assay sera from patients with hepatitis A and was found to have high sensitivity for the IgM antibody to HAV. The antibody was detectable within a few days of onset of symptoms of hepatitis, and it reached maximum concentrations within one to three weeks. The test was designed so that most patients' sera would become negative approximately three months after onset. HAVAB-M was shown to be specific for IgM antibody, with virtually no detection of IgG anti-HAV. The test showed no interference fro rheumatoid factor and no cross-reactivity with sera from patients with hepatitis B or other infectious diseases.

Published
1981
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6. Interpretation of various serological profiles of hepatitis B virus infection.

Author

Mushahwar IK, Dienstag JL, Polesky HF, McGrath LC, Decker RH, and Overby LR

Subjects
Hepatitis B classification, Hepatitis B Antibodies analysis, Hepatitis B Surface Antigens analysis, Hepatitis B e Antigens analysis, Humans, Time Factors, Hepatitis B immunology
Abstract

Serial serum specimens from 149 patients with clinically diagnosed hepatitis were tested for five hepatitis B serological markers: hepatitis B surface antigen and its antibody (anti-HBs); hepatitis B e-antigen and its antibody (anti-HBe); and antibody to hepatitis B core antigen (anti-HBc). The times of appearance, disappearance, and persistence of these markers were used to differentiate various serological profiles obtained from the study. Four distinctive profiles were found to be associated with acute hepatitis B followed by recovery, and three with chronic hepatitis. These serologic profiles were assessed as diagnostic and prognostic guides for clinical management of the disease.

Published
1981
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8. Acute viral hepatitis in adults. Comparison of the radioimmunoassay and counterimmunoelectrophoresis methods of detecting HbsAg.

Author

Wenzel RP, Teates CD, Galapon Q, Barczak R, Ling CM, and Overby LR

Subjects
Acute Disease, Adult, Age Factors, Convalescence, Epitopes, False Positive Reactions, Humans, Immunoelectrophoresis instrumentation, Male, Radioimmunoassay, Hepatitis B immunology, Hepatitis B Antigens isolation & purification
Abstract

We compared the radioimmunoassay (RIA) and counterimmunoelectrophoretic (CIE) methods in detecting hepatitis B antigen (HBsAG) in 407 acute and 336 convalescent sera of adults with viral hepatitis. The CIE method demonstrated that 41% of acute and 28% of 14-to 17-day serum specimens were HBsAg-positive. The RIA method demonstrated seropositivity in 60% of acute and 56% of convalescent specimens (P less than .001). Eighty-four percent of coded specimens initially positive for HBsAg by RIA were found to have subtype antigenic determinants d or y; 92% of the HBsAg-negative controls were negative for subtype antigens, confirming the specificity of the RIA test. RIA subtyping data corroborated earlier work with immunodiffusion techniques.

Published
1975
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9. Viral hepatitis, type B. Studies on natural history and prevention re-examined.

Author

Krugman S, Overby LR, Mushahwar IK, Ling CM, Frösner GG, and Deinhardt F

Subjects
Aspartate Aminotransferases blood, Child, Hepatitis B immunology, Hepatitis B Antibodies analysis, Hepatitis B Antigens analysis, Hepatitis B Core Antigens immunology, Hepatitis B Surface Antigens analysis, Hepatitis B Surface Antigens immunology, Humans, Immunity, Active, Immunity, Maternally-Acquired, Immunization, Immunoglobulins, Hepatitis B prevention & control
Abstract

Frozen serial serum specimens obtained from past studies on the natural history and prevention of Type B hepatitis in children were retested by radioimmunoassay for the following markers of hepatitis B infection: hepatitis B surface antigen (HBsAg) and antibody (anti-HBs), hepatitis B e antigen (HBeAg) and antibody (anti-HBe), and antibody to hepatitis B core antigen (anti-HBc). The interval between exposure and evidence of viremia (HBsAg) was as short as six days. HBsAg and HBeAg persisted for two to five months and occasionally for more than one year after recovery. After the disappearance of their respective antigens, anti-HBc and anti-HBs persisted for more than seven years and anti-HBe for one to two years. Treatment with hepatitis B immune globulin after exposure induced complete or partial protection or prolongation of the incubation period. Administration of heat-inactivated hepatitis B virus, MS-2 strain, to 29 children induced an inapparent infection in three, characterized by a transient appearance of HBsAg and HBeAg, and the persistence of anti-HBc, anti-HBe and anti-HBs for more than two years.

Published
1979
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10. Hepatitis B infection in institutionalized Down's syndrome inmates: a longitudinal study with five hepatitis B virus markers.

Author

Hawkes RA, Boughton CR, Schroeter DR, Decker RH, and Overby LR

Subjects
Australia, Chronic Disease, Down Syndrome immunology, Female, Hepatitis B immunology, Hepatitis B Surface Antigens analysis, Humans, Institutionalization, Longitudinal Studies, Male, Antibodies, Viral analysis, Down Syndrome complications, Hepatitis B etiology, Hepatitis B Antibodies analysis, Hepatitis B Antigens analysis
Published
1980

11. Isolation of a cDNA clone derived from a blood-borne non-A, non-B viral hepatitis genome.

Author

Choo QL, Kuo G, Weiner AJ, Overby LR, Bradley DW, and Houghton M

Subjects
Animals, Bacteriophage lambda genetics, DNA isolation & purification, Hepatitis Antibodies analysis, Hepatitis C microbiology, Hepatitis Viruses immunology, Immunoblotting, Nucleic Acid Hybridization, Pan troglodytes, Protein Biosynthesis, RNA, Viral blood, Antigens, Viral genetics, DNA genetics, Hepatitis C immunology, Hepatitis Viruses genetics, Hepatitis, Viral, Human immunology, RNA, Viral genetics
Abstract

A random-primed complementary DNA library was constructed from plasma containing the uncharacterized non-A, non-B hepatitis (NANBH) agent and screened with serum from a patient diagnosed with NANBH. A complementary DNA clone was isolated that was shown to encode an antigen associated specifically with NANBH infections. This clone is not derived from host DNA but from an RNA molecule present in NANBH infections that consists of at least 10,000 nucleotides and that is positive-stranded with respect to the encoded NANBH antigen. These data indicate that this clone is derived from the genome of the NANBH agent and are consistent with the agent being similar to the togaviridae or flaviviridae. This molecular approach should be of great value in the isolation and characterization of other unidentified infectious agents.

Published
1989
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12. A specific immune response to purified HA antigen (HAAg) demonstrated by leukocyte migration inhibition in patients recovering from viral hepatitis A.

Author

Fasel-Folley J, Overby LR, and Frei PC

Subjects
Adult, Cell Movement, Female, Hepatitis A Antigens, Hepatitis B Surface Antigens analysis, Humans, Leukocytes immunology, Male, Reference Values, Antigens, Viral, Hepatitis A immunology, Hepatovirus immunology
Abstract

The mechanism responsible for liver cell necrosis in patients with hepatitis A is not known. Since the type of hepatic lesions and the clinical presentation of acute hepatitis B are similar and are probably related to the cell-mediated immune response to a viral antigen located in the liver cell, it is possible that a similar mechanism is involved in hepatitis A. In the present paper, immune reactivity to hepatitis A antigen (HAAg) was measured in 13 patients at the time of recovery from hepatitis A, by using the leukocyte migration inhibition test (LMIT) under agarose with purified HAAg as antigen. Eleven normal subjects without history of hepatitis and 4 patients convalescent from hepatitis B were used as controls. Inhibition of leukocyte migration by HAAg was found in 11 of the 13 patients, with an average migration index (MI) of 77.0% (SEM 3.5). No such inhibition was found in any of the controls: MI = 100.8% (SEM 1.0), P less than 0.0001. These findings show that, like for HBsAg in hepatitis B, an immune response specific for HAAg can be demonstrated by the LMIT after HAV infection. This response could perhaps be related to the liver injury associated to hepatitis A.

Published
1986
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13. Science and technology in mitigating AIDS.

Author

Overby LR and Allain JP

Subjects
Antigens, Viral immunology, DNA, Viral blood, Flow Cytometry, HIV genetics, HIV immunology, HIV Antibodies blood, Humans, Immunoblotting, Immunoenzyme Techniques, Polymerase Chain Reaction, Recombinant Proteins immunology, Viral Proteins immunology, Acquired Immunodeficiency Syndrome diagnosis
Abstract

The workshop emphasized contributions of genetic engineering in providing reagents and techniques for diagnosing and monitoring HIV infections. Despite a variety of tests for specific antibodies, virus antigens and nucleic acids no consistent serum profile has emerged that correlates well with virus life cycle or clinical course. HIV infections are a great deal more complex than hepatitis B infections where diagnosis and prognosis are very accurately based on serologic profiles. HIV generates at least 15 virus proteins all of which are immunogenic. The workshop emphasized studies on immunogenicity of the proteins. Full understanding of the virus life cycle and the clinical course of disease may require in-depth studies of the production and immunogenicity of the virus-directed catalytic and regulatory gene products. Fortunately, all of these reagents can be produced through biotechnology. The new techniques described in the workshop will allow expanded studies to proceed rapidly.

Published
1988
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14. Hepatits A virus infection in fulminant hepatitis and chronic active hepatitis.

Author

Rakela J, Redeker AG, Edwards VM, Decker R, Overby LR, and Mosley JW

Subjects
Adolescent, Adult, Antibodies, Viral analysis, Chronic Disease, Feces microbiology, Female, Hemagglutination Tests, Hepatitis A diagnosis, Hepatitis B Surface Antigens, Hepatitis, Viral, Human diagnosis, Humans, Immune Adherence Reaction, Male, Microscopy, Electron, Radioimmunoassay, Hepatitis microbiology, Hepatitis A microbiology, Hepatovirus isolation & purification
Published
1978

15. Characteristics of herpes simplex virus resistance to disodium phosphonoacetate.

Author

Duff RG, Robishaw EE, Mao JC, and Overby LR

Subjects
DNA Replication drug effects, DNA, Viral biosynthesis, DNA-Directed DNA Polymerase metabolism, Drug Resistance, Microbial, Simplexvirus enzymology, Simplexvirus metabolism, Organophosphorus Compounds pharmacology, Phosphonoacetic Acid pharmacology, Simplexvirus drug effects
Abstract

Herpes simplex virus (HSV), which was partially resistant to the inhibitory effect of disodium phosphonoacetate (PAA), could be recovered following four virus passages in the presence of 100 microgram/ml PAA. Resistant strains were isolated from both HSV type 1 and HSV type 2. Virus resistance to PAA was not complete, and in most isolations a significant proportion of the virus stock remained susceptible to the drug. Resistance was shown to be heritable and persisted through virus passage and cloning experiments. PAA inhibited the replication of virus-specific DNA in sensitive strains of HSV but not in resistant strains of HSV. In vitro experiments directly demonstrated that PAA inhibited the activity of the virus-specific DNA polymerase 10 times more effectively in PAA-susceptible HSV than in PAA-resistant HSV. The treatment of HSV-infected mice with high levels of PAA did not induce the formation of resistant virus strains.

Published
1978
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16. Comparison of confirmation methods for hepatitis-B antigen and the nature of false-positives detected by 125I-immunoglobulins.

Author

Ling CM, Decker RH, Foemmel RS, and Overby LR

Subjects
Animals, Antibodies, Antibody Specificity, Blood Donors, Cross Reactions, False Positive Reactions, Guinea Pigs immunology, Humans, Immunoglobulins, Iodine Radioisotopes, Neutralization Tests, Hepatitis B Antigens analysis, Radioimmunoassay methods
Abstract

Immunologic specificity associated with solid-phase direct radioimmunoassay (RIA) using guinea pig antibodies for HBsAg detection (Ausria-125TM) was examined further with physicochemical techniques. The RIA reactivities which could not be neutralized by wide-spectrum human anti-HBs serum appeared to be physically distinct from true HBsAg particles; hence, they were truly false-positive, resulting from immunologic cross-reactions. In order to ensure the full advantages of using this highly sensitive RIA test, a confirmatory test using specific human anti-HBs for neutralization is therefore required to distinguish the true- and false-positives. The basic RIA technique is a two-step procedure. Two basic confirmation procedures, namely, a first-step neutralization and a second-step neutralization, were investigated in depth to assess their efficacy and practicality for confirmation. Both procedures were effective for confirmation purposes; however, the first-step neutralization procedure failed to confirm some high-titered HBsAg samples unless these samples were appropriately diluted. The second-step neutralization method did not require dilutions of any test samples.

Published
1975

17. Non-A/non-B hepatitis in experimentally infected chimpanzees: cross-challenge and electron microscopic studies.

Author

Bradley DW, Maynard JE, Cook EH, Ebert JW, Gravelle CR, Tsiquaye KN, Kessler H, Zuckerman AJ, Miller MF, Ling C, and Overby LR

Subjects
Animals, Factor IX administration & dosage, Factor IX adverse effects, Factor VIII administration & dosage, Factor VIII adverse effects, Hepatitis C etiology, Hepatitis C pathology, Pan troglodytes, Transfusion Reaction, Hepatitis C immunology, Hepatitis, Viral, Human immunology, Immunity, Liver ultrastructure
Abstract

Inoculation of eight chimpanzees with factor VIII, factor IX, or "H" strain plasma resulted in enzymatic and histopathologic evidence of non-A/non-B hepatitis in all eight animals. Challenge of two chimpanzees convalescent from factor VIII-induced disease with either factor IX or "H" strain plasma resulted in non-A/non-B hepatitis only in the animal inoculated with factor IX materials. Reciprocal cross-challenge of a chimpanzee convalescent from factor IX-induced disease with factor VIII also produced unequivocal enzymatic and histopathologic evidence of non-A/non-B hepatitis. Cross-challenge of a chimpanzee convalescent from "H" strain-induced non-A/non-B hepatitis with factor VII did not cause a second bout of non-A/non-B hepatitis. These findings suggest the factor VIII materials and "H" strain plasma used in these studies share a common etiologic agent (or agents), but that factor VIII and factor IX may contain two distinct agents. Electron microscopic (EM) examination of thin-sectioned, acute-phase liver biopsies from all but one of the chimpanzees receiving the primary inocula revealed the presence of abnormal hepatocyte cytoplasmic structures previously shown to be associated with non-A/non-B hepatitis. Crystalline structure containing 25 to 30 nm particles were visualized by EM in the cytoplasm of endothelial or Kupffer cells in acute-phase liver biopsies obtained from three chimpanzees inoculated with either factor VIII materials or "H" strain plasma.

Published
1980
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18. Hepatitis B surface antigen (HBsAg) subtype-specific antibodies in persons vaccinated against hepatitis B.

Author

Jilg W, Delhoune C, Deinhardt F, Roumeliotou-Karayannis AJ, Papaevangelou GJ, Mushahwar IK, and Overby LR

Subjects
Adolescent, Adult, Antibody Specificity, Epitopes immunology, Female, Hepatitis B Antibodies immunology, Hepatitis B Surface Antigens classification, Hepatitis B Vaccines, Humans, Male, Middle Aged, Hepatitis B Antibodies analysis, Hepatitis B Surface Antigens immunology, Vaccination, Viral Vaccines immunology
Abstract

One hundred sixty-three persons immunised against hepatitis B with a vaccine containing HBsAg either of adw or ayw subtype were examined for antibodies against the a, d, and y determinants of HBsAg. Sera were tested for antibodies against HBsAg adw and HBsAg ayw separately by a solid-phase radioimmunoassay using polystyrene beads coated with HBsAg of either adw or ayw subtype, and the relative amounts of antibodies against the single determinants were calculated. After the third immunisation, all vaccinees had antibodies against the common determinant a. A quantitative evaluation showed that on average about 50% of HBsAg-specific antibodies were directed against the a determinant, and about 50% against d or y, respectively. However, as only anti-a is protective against cross-infection with other HBsAg subtypes, the degree of immunity of a person vaccinated against hepatitis B should be evaluated by the determination of antibodies to a rather than antibodies against total HBsAg.

Published
1984
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19. Serologic studies of transmission of hepatitis A in humans.

Author

Decker RH, Overby LR, Ling CM, Frösner G, Deinhardt F, and Boggs J

Subjects
Disease Outbreaks, Female, Hepatitis A immunology, Hepatovirus ultrastructure, Humans, Immunoglobulin G isolation & purification, Male, Radioimmunoassay, Retrospective Studies, Antibodies, Viral analysis, Hepatitis A transmission, Hepatovirus immunology
Abstract

In 1968, studies of infectious hepatitis in volunteers were reported. Immunologic procedures for serologic study of the hepatitis A virus were not available at that time, and only the clinical and biochemical parameters of the disease were reported. Serial serum specimens from the participants in the study were retained; these specimens had been taken before inoculation and up to more than 100 days after inoculation. When a radioimmune assay for antibody to hepatitis A virus was developed, the series of sera was analyzed retrospectively. Forty-four male volunteers were involved in a series of three studies. Twenty (46%) of the volunteers were found to be initially immune to hepatitis A virus. Eighteen susceptible volunteers (with no preexisting antibody) were challenged with infectious virus. Eight of these volunteers developed clinical hepatitis and seroconverted; one seroconverted without evidence of clinical disease; and nine neither seroconverted nor had evidence of clinical disease. The radioimmune assay provided a method for diagnosis of immune status and of the acute disease caused by hepatitis A virus.

Published
1979
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20. An enzyme immunoassay for hepatitis B e-antigen and antibody.

Author

Mushahwar IK and Overby LR

Subjects
Blood Donors, Electrophoresis, Humans, Immunoenzyme Techniques, Radioimmunoassay, Antibodies, Viral analysis, Hepatitis B Antibodies analysis, Hepatitis B Antigens analysis, Hepatitis B e Antigens analysis
Abstract

A solid-phase enzyme-linked immunoassay for the detection of hepatitis B e-antigen (HBeAg) and antibody (anti-HBe) was developed and compared with rheophoresis and radioimmunoassay (RIA). The enzyme-immunoassay (EIA) was similar to RIA in sensitivity and was approximately 1000-fold more sensitive than rheophoresis for HBeAg, and approximately 6000-fold more sensitive than rheophoresis for anti-HBe.

Published
1981
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21. Serodiagnosis of viral hepatitis A by a modified competitive binding radioimmunoassay for immunoglobulin M anti-hepatitis A virus.

Author

Bradley DW, Fields HA, McCaustland KA, Maynard JE, Decker RH, Whittington R, and Overby LR

Subjects
Acute Disease, Animals, Antibody Specificity, Convalescence, Humans, Immunoglobulin G analysis, Antibodies, Viral analysis, Hepatitis A diagnosis, Hepatovirus immunology, Immunoglobulin M analysis, Radioimmunoassay methods
Abstract

A competitive binding radioimmunoassay (CBA) for antibody to hepatitis A virus (HAV) was evaluated and compared with a standard solid-phase radioimmunoassay for anti-HAV, CBA was found to be sensitive and specific for the detection of anti-HAV, as demonstrated by the 98% concordance of CBA and solid-phase radioimmunoassay test results. The standard CBA test was modified for the differential detection of acute (immunoglobulin M) and convalescent (immunoglobulin G) anti-HAV by incorporation of a step in which immunoglobulin G anti-HAV was preferentially absorbed with S. aureus cells (protein A). The modified CBA test was shown to be capable of differentiating between acute- and convalescent-phase sera. The modified CBAM test was able to detect immunoglobulin M anti-HAV up to approximately 4 weeks after the onset of illness.

Published
1979
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22. Reexamination of hepatitis B virus subtypes and e-antigen expression by radioimmunoassays.

Author

Shorey J, Mushahwar IK, Shorey J, and Overby LR

Subjects
Adult, Age Factors, Blood Donors, Carrier State immunology, Female, Hepatitis B immunology, Humans, Male, Radioimmunoassay, Antibodies, Viral analysis, Carrier State microbiology, Hepatitis B microbiology, Hepatitis B Antibodies analysis, Hepatitis B Antigens analysis, Hepatitis B e Antigens analysis, Hepatitis B virus classification
Abstract

Radioimmunoassay methods were used to determine both the hepatitis B virus (HBV) subtype and hepatitis B e antigen (HBeAg) and antibody (anti-HBe) status of a group of hepatitis B surface antigen (HBsAg)-positive blood donors. The study involved sera containing HBV of the three major occidental subtypes, adw2, ayw3, and ayw2. The previously reported association of the y-type virus with HBeAg and the d types with anti-HBe was again observed. However, when the two y subgroups, ayw2 and ayw3, were considered individually, it was evident that the ayw3 specimens alone accounted for the association with HBeAg while the ayw2 sera were strongly associated with anti-HBe. The study also indicated that the prevalence of HBeAg declined and that of anti-HBe increased progressively with advancing age. On the average, ayw2 donors were significantly older than the adw2 donors, and donors from both of these groups were older than the ayw3 donors. It is postulated that the observed age differences account, at least in part, for the differing prevalence of e markers in the three HBV subtype groups, and that these age differences, in turn, may reflect a tendency for infections with the ayw2 viral strain to persist longer than adw2 infections, and both of these longer than ayw3 infections. Alternately, the three subtypes may represent epidemiologic shifts from remote ayw2 and adw2 infections to more recent ayw3 infections.

Published
1982
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23. Post-transfusion hepatitis: the role of hepatitis B antibody.

Author

Koretz RL, Overby LR, and Gitnick GL

Subjects
Blood Donors, Hepatitis B prevention & control, Humans, Time Factors, Transfusion Reaction, gamma-Globulins therapeutic use, Antibodies, Hepatitis B epidemiology
Abstract

Aliquots from units of blood previously transfused as part of a prospective post-transfusion hepatitis (PTH) study were rescreened for the presence of hepatitis B antibody (anti-HBS) to determine the effect of transfusion of such material. Anti-HBS was more commin in commercial blood. Infusion of anti-HBS was not associated with an increased or decreased risk of PTH, hepatitis B, or hepatitis B (HB) exposure. Receipt of anti-HBS did not modify the hepatitis which occurred. Receipt of large amounts of anti-HBS may be associated with an increased incidence of HB events. Preexisting anti-HBS was not only not protective against PTH, but more PTH (67% versus 40%) and hepatitis B (47% versus 12%) were seen in those patients with it.

Published
1976

24. Inhibition of DNA polymerase from herpes simplex virus-infected wi-38 cells by phosphonoacetic Acid.

Author

Mao JC, Robishaw EE, and Overby LR

Abstract

Infection of Wi-38 cells with herpes simplex virus induced an elevated DNA polymerase activity which had many biochemical properties different from normal cell DNA polymerase. Phosphonoacetic acid specifically inhibited the virus-induced DNA polymerase as compared to the normal WI-38 cell DNA polymerase. The compound did not appear to inhibit enzyme activity by interacting with the DNA primer.

Published
1975
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26. Detection of HBeAg and anti-HBe in acute hepatitis B by a sensitive radioimmunoassay.

Author

Frösner GG, Brodersen M, Papaevangelou G, Sugg U, Haas H, Mushahwar IK, Ling CM, Overby LR, and Deinhardt F

Subjects
Acute Disease, Germany, West, Greece, Humans, Antibodies, Viral analysis, Hepatitis B immunology, Hepatitis B Antibodies analysis, Hepatitis B Antigens analysis, Radioimmunoassay methods
Abstract

A solid-phase radioimmunoassay using anti-HBe-coated polysterence beads and iodine-125-labeled anti-HBe of human origin was developed for the detection of HBeAg. Anti-HBe could be determined by a blocking test. Both assays were about 500-fold more sensitive than immunodiffusion. Few nonspecific positive results for HBeAg could be recognized in the anti-HBe test by increase in cpm over that of the negative control. HBeAg was not found in acute hepatitis A and non A-non B hepatitis or in a control group of accident patients. On admission to the hospital 12 of 48 (25%) acute hepatitis B patients from Greece and 17 of 20 (85%) acute hepatitis B patients from Germany were HBeAg-positive. All 39 initially HBeAg negative sera were already anti-HBe positive. Tests of the acute stage and follow-up sera of the 20 German patients indicated that HBeAg is regularly present in the incubation period and early acute phase of hepatitis B. After onset of disease the antigen is cleared from the serum very rapidly in uncomplicated cases and is usually followed by the appearance of anti-HBe. Like anti-HBc, anti-HBe can serve as a tool for the diagnosis of hepatitis B after the disappearance of HBsAg.

Published
1978
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27. Inhibition of herpes simplex virus replication by phosphonoacetic acid.

Author

Overby LR, Robishaw EE, Schleicher JB, Rueter A, Shipkowitz NL, and Mao JC

Subjects
Fibroblasts virology, Humans, Simplexvirus physiology, Antiviral Agents pharmacology, Phosphonoacetic Acid pharmacology, Simplexvirus drug effects, Virus Replication drug effects
Abstract

Replication of herpes simplex virus in WI-38 cells was inhibited by phosphonoacetic acid, as measured by decreased virus cytopathogenic effect and incorporation of radiolabeled thymidine in virus-infected cells. The drug appeared to have no effect on adsorption, penetration, or release of the virus nor on the synthesis of ribonucleic acid or protein. It appeared to inhibit virus deoxyribonucleic acid synthesis.

Published
1974
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29. Seroepidemiological investigation of patients and family contacts in an epidemic of hepatitis A.

Author

Frösner GG, Overby LR, Flehmig B, Gerth HJ, Haas H, Decker RH, Ling CM, Zuckerman AJ, and Frösner HR

Subjects
Adolescent, Adult, Age Factors, Child, Child, Preschool, Feces immunology, Germany, West, Hepatitis A transmission, Humans, Infant, Middle Aged, Radioimmunoassay, Rural Population, Antibodies, Viral analysis, Antigens, Viral analysis, Disease Outbreaks, Hepatitis A immunology, Hepatovirus immunology
Abstract

Serial blood and faecal samples were collected from patients and family contacts during an outbreak of hepatitis A in a village and tested by a solid-phase competitive type radioimmunoassay for hepatitis A antigen and hepatitis A antibody. The amount and duration of excretion of hepatitis A antigen was correlated with the severity of the illness. In 2 severe clinical cases, hepatitis A antigen was demonstrated in faecal extracts 11 days before the onset of jaundice and continuing for 10 days thereafter, with maximum shedding during the late incubation period. Faecal antigen was demonstrated in low concentrations for only 2 days in a patient with mild disease and in a person with subclinical infection. There was an inverse correlation between the incidence of infection and prevalence of hepatitis A antibody and age. Of 24 infections, 19 (79%) occurred in persons in the age group 0 to 20 years, a group in which only 6% of individuals had pre-existing antibody. Hepatitis A antibody was present in the serum of 3 persons in low titres of 1:20 to 1:40 on the day jaundice developed. The antibody titres increased very rapidly during the following 2 weeks of illness and slowly during the following months, reaching titres of 1:900 to 1:3500. In a separate study, a mean antibody titre of 1:591 was found in 13 patients, 12 years after clinical hepatitis A with jaundice.

Published
1977
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30. Antigenic subgroups of hepatitis B (surface) antigen in Berlin (West) and their epidemiological aspects.

Author

Lange W, Overby LR, Werner J, Köhler H, and Apodaca J

Subjects
Adolescent, Adult, Berlin, Child, Child, Preschool, Germany, West, Humans, Infant, Renal Dialysis, Substance-Related Disorders, Carrier State immunology, Epitopes, Hepatitis B immunology, Hepatitis B Antigens analysis
Abstract

Sera of 334 hepatitis B patients and 118 sera of HBsAg carriers were tested for the distribution of the subgroups ad and ay by means of rheophoresis technique or solid phase radiommunoassay. The distribution of subgroups revealed a typical pattern. The ad-antigen determinant was more frequent in hepatitis B patients, blood donors and hemodialysis patients whereas the ay determinant was detected in drug users, guest workers and juveniles at a considerably higher percentage. The difference in distribution is discussed as an epidemiological phenomenon of hepatitis B virus, dependent on environmental factors characteristic for certain groups of the population. The routine testing for HGsAg subgroups is recommended as a valuable epidemiologic tool.

Published
1975

31. Antiviral potential of phosphonoacetic acid.

Author

Overby LR, Duff RG, and Mao JC

Subjects
Animals, Cell-Free System, Cells, Cultured, Cricetinae, DNA-Directed DNA Polymerase metabolism, Drug Resistance, Microbial, Herpesviridae drug effects, Herpesviridae enzymology, Herpesviridae Infections drug therapy, Macromolecular Substances, Mesocricetus, Microbial Sensitivity Tests, Phosphonoacetic Acid therapeutic use, Simplexvirus drug effects, Species Specificity, Antiviral Agents, Organophosphorus Compounds pharmacology, Phosphonoacetic Acid pharmacology
Abstract

Phosphonoacetate has been found to inhibit specifically the replication of herpes-viruses. A partial inhibition of vaccinia virus represents the only activity outside the herpesvirus class. The drug was found to be a specific inhibitor of the virus-induced DNA polymerases. Normal cellular polymerases were relatively insensitive to phosphonoacetate, resulting in low cellular toxicity. Our working hypothesis is that the drug binds to the enzyme and that initiation of polynucleotide synthesis occurs in the presence of the drug and the required template, substrates, and cations. However, addition of deoxynucleosides to the elongating nascent chain is prevented by the enzyme-bound drug. Kinetic analyses indicated that phosphonoacetate did not interfere with the binding of DNA template to polymerase; and it did not compete with nucleotide substrate binding. The highly specific inhibitory effects of phosphonoacetate allowed for the selection of partially resistant strains of HSV. Resistance of virus to the drug in cell culture was directly correlated with the same relative resistance of the corresponding cell-free DNA polymerases. Phosphonoacetate was also effective therapeutically in herpesvirus skin and ocular infections in animals. Intraperitoneal administration of the drug reduced death and severity of disease in experimental encephalitis in hamsters. High specificity, low toxicity, and reproducible efficacy in lower animals suggested that phosphonoacetate could be a useful new antiviral drug. Sensitivity to phosphonoacetate also is a useful research tool as a genetic marker for herpesviruses.

Published
1977
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33. Serodiagnosis of recent hepatitis B infection by IgM class anti-HBc.

Author

Chau KH, Hargie MP, Decker RH, Mushahwar IK, and Overby LR

Subjects
Antibody Specificity, Hepatitis B Core Antigens immunology, Humans, Neutralization Tests, Radioimmunoassay, Serologic Tests, Time Factors, Antibodies, Viral analysis, Hepatitis B immunology, Hepatitis B Antibodies analysis, Immunoglobulin M analysis
Abstract

The time sequence, relative reactivity, and persistence of anti-HBc IgM were assessed in patients with HBsAg-positive viral hepatitis. A solid-phase immunoassay was developed using the IgM capture procedure with anti-mu-coated polystyrene beads. HBcAg was purified from serum Dane particles and used as a probe with 125I-labeled anti-HBc IgG. This immunoassay exhibited a pronounced prozoning phenomenon, and relative titers of sera differed widely depending upon the dilution of serum tested. When all sera were tested at 1:5,000 dilution, results were comparable in different patient groups. Anti-HBc IgM persisted at detectable levels for up to 2 years, and it was necessary to establish relative titers to discriminate current from remote infections. A cut-off assay value was established, and in 12 cases of acute hepatitis B virus (HBV) infection, antibody exceeded this value for about 6 months after onset of HBs antigenemia. A similar profile of anti-HBc IgM persistence was observed in seven patients who developed an HBsAg chronic carrier state. Long-term viral replication did not sustain elevated IgM class-specific antibody levels. The studies suggest that anti-HBc IgM analyses may be useful for differentiating recent and current HBV infections from remote infections, eliminating HBV as the agent for non-A, non-B hepatitis in asymptomatic HBsAg carriers, and detecting HBV as the etiologic agent during silent (HBsAg negative) infections.

Published
1983
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34. Anti-hepatitis B core immunoglobulin M in the serologic evaluation of hepatitis B virus infection and simultaneous infection with type B, delta agent, and non-A, non-B viruses.

Author

Perrillo RP, Chau KH, Overby LR, and Decker RH

Subjects
Carrier State, Diagnosis, Differential, Enzyme-Linked Immunosorbent Assay, Hepatitis B diagnosis, Hepatitis B Surface Antigens analysis, Hepatitis C diagnosis, Hepatitis delta Antigens, Humans, Antibodies, Viral analysis, Hepatitis B immunology, Hepatitis B Antibodies analysis, Hepatitis B Antigens, Hepatitis B Core Antigens immunology, Hepatitis C immunology, Hepatitis, Viral, Human immunology, Immunoglobulin M analysis
Abstract

The clinical value of an enzyme-linked immunosorbent assay for the detection of immunoglobulin M (IgM) antibody to hepatitis B core antigen (anti-HBc IgM) was evaluated by testing serum samples from the following groups of patients: (a) 27 individuals who had been diagnosed as having acute hepatitis B virus (HBV) infection, (b) 29 hepatitis B surface antigen (HBsAg) carriers, (c) 6 subjects with acute non-B hepatitis, and (d) 10 HBsAg-negative but anti-HBc-positive subjects who were suspected of being index cases for the intimate transmission of HBV. Whereas 24 of the 27 individuals with presumed acute HBV infection exhibited anti-HBc IgM, only 2 of 29 HBsAg carriers were found to be positive. Hepatitis B surface antigen persisted during an 8-mo observation period in 3 anti-HBc IgM-negative subjects with acute HBsAg-positive hepatitis. Before anti-HBc IgM testing, it was considered that these cases had evolved to the HBsAg carrier state. However, the regular demonstration of anti-HBc IgM in acute type B hepatitis, as well as the failure to detect this antibody in the majority of HBsAg carriers, led to reclassification of these cases as probable instances of acute non-A, non-B or delta-agent hepatitis superimposed on the HBsAg carrier state. Through additional testing, the diagnosis of non-A, non-B (NANB) infection was confirmed in 2 of these cases, and delta-agent infection was identified in the third. None of the non-B hepatitis cases exhibited anti-HBc IgM. However, 5 of the 10 suspected type B index cases were anti-HBc IgM-positive, indicating that they were very recently infected and most likely had infected their cohabiting sexual partners. The results from this study indicate that testing for anti-HBc IgM may improve serodiagnostic accuracy when acute NANB and delta-agent hepatitis occur in previously unrecognized HBsAg carriers. Moreover, it may be a useful test in defining potential high risk sources of exposure to HBV.

Published
1983

35. Challenges and opportunities in biotechnology.

Author

Overby LR

Subjects
Acquired Immunodeficiency Syndrome prevention & control, Drug Industry, Factor VIII chemical synthesis, Factor VIII therapeutic use, Genetic Engineering methods, Hepatitis B Vaccines, Hepatitis C prevention & control, Humans, Plasminogen Activators chemical synthesis, Plasminogen Activators therapeutic use, Protein Processing, Post-Translational, Retroviridae immunology, Simplexvirus immunology, Viral Hepatitis Vaccines chemical synthesis, Viral Hepatitis Vaccines therapeutic use, Viral Vaccines chemical synthesis, Viral Vaccines classification, Viral Vaccines therapeutic use, Cloning, Molecular, DNA, Recombinant, Medical Laboratory Science
Abstract

The biotechnology industry is thriving, and many predicted accomplishments have actually occurred during the last decade. Cloning and expression of genetic information is now simple and routine. Initial commercial products have been realized, but there is much yet to be accomplished in evaluating the clinical significance of many other gene products made available by biotechnology resources. During the next decade, human health care and the pharmaceutical industry should be affected substantially by first- and second-generation recombinant DNA products. Recombinant vaccines, blood coagulation factors, and known biological modulators produced by rDNA technologies should be widely used. Further opportunities will be realized with increasing discoveries of new bioactive molecules and identification of NANB hepatitis and AIDS infectious agents. Full exploitation of health care products will depend on innovative new delivery systems or the ability to reconstruct mammalian and plant genes, providing for in-situ delivery of the necessary gene products.

Published
1985

36. Radioimmunoassay for detection of hepatitis B e antigen and its antibody. Results of clinical evaluation.

Author

Mushahwar IK, McGrath LC, Drnec J, and Overby LR

Subjects
Epitopes, Female, Hepatitis B Surface Antigens, Humans, Infant, Quality Control, Radioimmunoassay, Antibodies, Viral, Hepatitis B diagnosis, Hepatitis B Antibodies, Hepatitis B Antigens, Hepatitis B e Antigens standards
Abstract

The performance of a solid phase radioimmunoassay (ABBOTT-HBe) for the detection of hepatitis B e antigen (HBeAg) and its antibody anti-HBe was evaluated in clinical studies. The reagents and procedure were found to be reproducible by seven investigators, and lab-to-lab variations were minimal. In HBsAg positive sera, ABBOTT-HBe detected HBeAg or anti-HBe in 90% of the specimens compared to 50% tested by immunodiffusion. During the early acute stage of viral infection, serum HBeAg coincided with the rise and decline of HBsAg and seroconversion to anti-HBe occurred most often prior to loss of HBsAg. Patients with clinical evidence of chronic liver disease showed persistence of HBsAg and HBeAg. Vertical transmission studies of hepatitis B virus infection from mother to newborns, showed that mothers whose sera were positive for both HBsAg and HBeAg resulted in a greater incidence of transmission of hepatitis B virus to their offspring than mothers whose sera were HBsAg positive but HBeAg negative.

Published
1981
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37. Letter: Cytomegalovirus in non-B post-transfusion hepatitis.

Author

Fiala M, Nelson RJ, Myhre BA, Guze LB, Overby LR, and Ling CM

Subjects
Adenoviridae immunology, Antibodies isolation & purification, Complement Fixation Tests, Fluorescent Antibody Technique, Hepatitis immunology, Hepatitis microbiology, Hepatitis B Antibodies isolation & purification, Hepatitis B Antigens isolation & purification, Herpesvirus 4, Human immunology, Humans, Immunization, Passive, Measles virus immunology, Prospective Studies, Radioimmunoassay, Simplexvirus immunology, Cytomegalovirus immunology, Hepatitis etiology, Transfusion Reaction
Published
1974
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38. Cryptic association of e antigen with different morphologic forms of hepatitis B surface antigen.

Author

Vnek J, Prince AM, Trepo C, Williams AE, Mushahwar IK, Ling CM, and Overby LR

Subjects
Animals, Carrier State immunology, Hepatitis B immunology, Hepatitis B Antigens analysis, Hepatitis B Surface Antigens isolation & purification, Isoelectric Focusing, Molecular Weight, Pan troglodytes, Peptides analysis, Polysorbates, Hepatitis B Antigens isolation & purification, Hepatitis B Surface Antigens analysis
Abstract

When highly purified HBsAg particles, separated by rate zonal centrifugation into populations differing in predominant size, were tested for HBeAg, the e1 specificity was detected preferentially in association with particle fractions containing large filaments and Dane particles. These results were obtained both by agar gel diffusion and by radioimmunoassay for e antigen. The e antigen activity present in these fractions was potentiated by prior treatment of particles with Tween 80, suggesting cryptic localization of e1 specificity within or under the outer membrane. The HBeAg released by detergent treatment from a purified preparation composed predominantly of small-particle forms of HBsAg was separated by electrofocusing into a peak of nonparticulate e antigen in the pH range of 5.7--6.0. Sodium dodecyl sulfate-polyacrylamide gel electrophoresis showed three major polypeptides in this preparation with approximate molecular weights of 25,000, 55,000, and 70,000. Furthermore, two additional peaks of e antigen activity were detected which migrated in association with HBsAg particles at isoelectric points of 4.4 and 5.5--5.6. The major portion of e antigen remained in association with particles after further purification by rate zonal centrifugation.

Published
1979
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39. Hepatitis B e-antigen and its correlation with other serological markers in chimpanzees.

Author

Ling CM, Mushahwar IK, Overby LR, Berquist KR, and Maynard JE

Subjects
Animals, Carrier State, Hepatitis B Antibodies analysis, Hepatitis B Surface Antigens analysis, Pan troglodytes, Time Factors, Hepatitis B immunology, Hepatitis B Antigens analysis
Abstract

Three chimpanzees experimentally infected with hepatitis B virus, and another three chimpanzees that were hepatitis surface antigen carriers, were studied for the presence of viral antigens and humoral immune responses. Quantitative analyses of hepatitis B surface and e-antigens in sequential serum samples at early acute stages revealed cyclic oscillations of these two antigens following a synchronous pattern. Similar analyses of anti-e-antigen and anti-hepatitis B core antigen antibodies from the three experimentally infected primates indicated that peak titers of these two antibodies occurred as surface antigen decreased to undetectable levels. Of the three surface-antigen carriers, two were positive for e-antigen and one was positive for e-antigen antibody for the entire course of surveillance (8, 9, and 22 months, respectively).

Published
1979
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40. Non-A, non-B hepatitis: a prospective study of a hemodialysis outbreak with evaluation of a serologic marker in patients and staff.

Author

Gitnick G, Weiss S, Overby LR, Ling CM, Chairez R, and Parsa K

Subjects
Adult, Aged, Alanine Transaminase blood, Aspartate Aminotransferases blood, Clinical Enzyme Tests, Female, Hemodialysis Units, Hospital, Hepatitis C epidemiology, Hepatitis C immunology, Humans, Immunodiffusion, Male, Middle Aged, Personnel, Hospital, Prospective Studies, Antigens, Viral analysis, Disease Outbreaks epidemiology, Hepatitis C diagnosis, Hepatitis Viruses immunology, Hepatitis, Viral, Human diagnosis, Renal Dialysis adverse effects
Abstract

An outbreak of non-A, non-B hepatitis (NANBH) in a hemodialysis unit was prospectively studied and the clinical, biochemical, and serologic events were correlated with an experimental immunodiffusion assay for serum antigen and antibody. One hundred sixteen subjects (76 dialysis patients and 40 staff members) were studied over an 8-month period. Hepatitis was defined as two consecutive SGPT levels greater than two times the upper limit of normal occurring in two separate samples drawn greater than 7 days apart in the absence of other likely causes of liver disease. Weekly serum specimens were obtained and tested for SGPT, SGOT, alkaline phosphatase, bilirubin HBsAg, anti-HBc, anti-HBs, total anti-HAV, and anti-HAV IgM by commercial reagents, and for antigen and antibody by agar gel diffusion using reference reagents previously obtained from well-documented posttransfusion NANBH patients. Clinical evaluations were performed three times per week. Thirty patients and none of the staff developed NANBH. The NANBH patients were asymptomatic, except for two patients with jaundice. Fifteen of the 30 patients were positive for antigen which was detectable in at least one serum collected during the acute phase. Six patients and 10 staff without clinical NANBH or abnormal serology had antigen. Antigenemia was also observed in three patients with acute hepatitis B, with chronic hepatitis B in one patient and with alcoholic hepatitis in one patient. Thus, an antigen was detected in a high proportion of patients during the acute phase of NANBH, and it was also found in exposed patients who had other liver diseases.(ABSTRACT TRUNCATED AT 250 WORDS)

Published
1983
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41. Prevalence of hepatitis B e antigen and its antibody as detected by radioimmunoassays.

Author

Mushahwar IK, Overby LR, Frosner G, Deinhardt F, and Ling CM

Subjects
Carrier State immunology, Counterimmunoelectrophoresis, Hepatitis B immunology, Hepatitis B Core Antigens analysis, Hepatitis B Surface Antigens analysis, Humans, Immunoelectrophoresis, Neutralization Tests, Antibodies, Viral analysis, Hepatitis B Antibodies analysis, Hepatitis B Antigens analysis, Radioimmunoassay
Abstract

A solid-phase radioimmunoassay (RIA) for the detection of hepatitis B e antigen (HBeAg) and antibody (anti-HBe) was developed. The RIA was approximately 1,000-fold more sensitive than rheophoresis for HBeAg, and approximately 6,000-fold more sensitive than rheophoresis for anti-HBe. Generally, less than one-fifth of hepatitis B antigen (HBsAg)-positive sera from blood donors were positive for either HBeAg or anti-HBe by rheophoresis; in contrast, more than 90% of the samples were positive by the RIA method. The ratio of HBeAg to anti-HBe among HBsAg carriers varied in different geographic localities. Also, the presence of HBeAg correlated directly with the titer of HBsAg and the presence of Dane core particles. Anti-HBe was associated with lower titers of serum HBsAg.

Published
1978
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44. The significance of IgM antibodies to hepatitis B core antigen in hepatitis B carriers and hepatitis B-associated chronic liver disease.

Author

Feinman SV, Overby LR, Berris B, Chau K, Schable CA, and Maynard JE

Subjects
Alanine Transaminase blood, Biopsy, Carrier State, Chronic Disease, Diagnosis, Differential, Hepatitis B diagnosis, Humans, Liver pathology, Antibodies, Viral immunology, Hepatitis B immunology, Hepatitis B Antibodies immunology, Hepatitis B Core Antigens immunology, Immunoglobulin M immunology
Published
1982
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49. Prevention of endemic HAA-positive hepatitis with gamma globulin. Use of a simple radioimmune assay to detect HAA.

Author

Ginsberg AL, Conrad ME, Bancroft WH, Ling CM, and Overby LR

Subjects
Blood Donors, Clinical Trials as Topic, Complement Fixation Tests, Hemagglutination Inhibition Tests, Hepatitis A diagnosis, Hepatitis A immunology, Hepatitis B immunology, Hepatitis B Antigens, Humans, Immunodiffusion, Immunoelectrophoresis, Male, Military Medicine, Placebos, Time Factors, United States, Hepatitis A prevention & control, Hepatitis B prevention & control, Hepatitis B virus immunology, Radioimmunoassay, gamma-Globulins therapeutic use
Published
1972
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