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  • 1
    Electronic Resource
    Electronic Resource
    Springer
    Journal of molecular medicine 63 (1985), S. 241-251 
    ISSN: 1432-1440
    Keywords: HCMV isolation ; Antigen and nucleic acid detection ; Ig class-specific antibody determination ; Risk groups: pregnancy, blood transfusion, organ transplantation
    Source: Springer Online Journal Archives 1860-2000
    Topics: Medicine
    Notes: Summary Cytomegalic inclusion disease (CID) is caused by a horizontally or vertically transmitted human herpes virus infection and may persist for life without obvious clinical symptoms. A serious course of horizontal primary and recurrent infections, however, is often observed in immunocompromised persons such as recipients of organ transplants and patients receiving fresh blood transfusions. Vertical infection may cause fetopathies. The human cytomegalovirus (HCMV) is thought to inherit an oncogenic potential as lately discussed for AIDS and M. Kaposi. Laboratory diagnosis of HCMV infection is performed by light microscopy (inclusion bodies), electron microscopy, virus isolation in cell culture, demonstration of viral DNA and antigen in clinical specimens, by histochemical methods (e.g. immunoperoxidase technique) and by DNA and peptide analysis for identification of different isolates and viral finger prints. Evaluation of cell-mediated immunity in HCMV infection is performed quantitatively (assessment of Thelper/Tsuppressor ratios) or qualitatively (specific lymphocyte stimulation by the antigen). In most cases laboratory diagnosis is achieved by serological methods, i.e. demonstration and quantitation of HCMV-specific antibodies. In this context, a number of liquid- and solid-phase immunoassays have been developed, of which immunofluorescence and ELISA are most commonly used, besides complement fixation and passive haemaglutination. These procedures on the one hand allow the use of different antigen preparations as early and late viral proteins, and on the other hand permit a specific determination of different Ig classes and subclasses. A variety of assays has been established especially for determination of virus-specific IgM antibodies, which are predominantly found in active infection. These, however, at least in part may show non-specific results caused by interference of rheumatoid factor or IgG competition. Such problems have now been dealt with and are avoided by IgG precipitation or IgM immunosorption (“μ-capture” technique). These recent methods allow an exact epidemiological identification of risk groups for CMV infection. Results from our laboratory revealed 13% HCMV-IgM positive patients among pregnant women, 16% IgM positive patients among renal transplant recipients, 4% igM positive cases in patients after cardiosurgery and 1.7% IgM positives among prostitutes. The prevalence of HCMV infection as indicated by specific IgG antibodies was 56%, 90%, 83%, and 90%, respectively. No IgM antibodies were found in haemophiliacs and healthy blood donours, which showed a prevalence of HCMV infection in 69% and 47% of tested serum samples.
    Type of Medium: Electronic Resource
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  • 2
    ISSN: 1432-1831
    Source: Springer Online Journal Archives 1860-2000
    Topics: Medicine
    Notes: Abstract Sera of patients with acute (AH) and chronic active hepatitis (CAH) were tested for anti-hepatitis B virus (HBV) x-protein (HBx) by immunoblotting, using recombinant MS2- and βgal-HBx fusion proteins as substrate. Antibodies against HBx were detected in 5 out of 17 patients with AH at an early stage of infection, and in 13 out of 35 patients with CAH. Positive sera from AH patients showed a relatively weak anti-HBx reactivity when compared to sera from CAH patients. In follow up studies we tested serial serum samples from patients positive for anti-HBx. Patients with AH were observed for 3 to 6 weeks and CAH patients for up to 51 months. In general anti-HBx reactivities appeared to be stable although significant differences in apparent antibody levels were noted when sera from individual patients were compared. Our data further support an early expression of HBx-antigen in HBV-infected individuals. There was no correlation between HBe-antigen and anti-HBx in CAH.
    Type of Medium: Electronic Resource
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  • 3
    Electronic Resource
    Electronic Resource
    Springer
    European journal of clinical microbiology & infectious diseases 4 (1985), S. 41-45 
    ISSN: 1435-4373
    Source: Springer Online Journal Archives 1860-2000
    Topics: Medicine
    Notes: Abstract The results of RNA analysis for the detection of rotavirus were compared with those of a standard enzyme-linked immunsorbent assay (ELISA) and electron microscopy using 212 faecal specimens obtained from 200 children with gastroenteritis. Rotavirus was extracted directly from faecal specimens and RNA segments were made visible by polyacrylamide gel electrophoresis using a silver staining technique. Of the 212 faecal specimens 137 were found to be positive in ELISA, 125 in RNA analysis and 121 in both methods. Forty-nine of the 212 specimens were also investigated by electron microscopy. Thirty-five were positive when examined by electron microscopy, 37 were positive in ELISA and 33 in RNA analysis. RNA analysis of 119 faecal samples in outbreaks and sporadic cases of rotavirus infection yielded 42 different rotavirus electrophoretypes. The results indicated that no one method was sufficient to detect all positive specimens and that RNA analysis is useful in epidemiological studies.
    Type of Medium: Electronic Resource
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  • 4
    ISSN: 1439-0973
    Source: Springer Online Journal Archives 1860-2000
    Topics: Medicine
    Description / Table of Contents: Zusammenfassung Mit einem schnellen, zuverlässigen und empfindlichen CMV-Antigentest konnten bei 24 Patienten Zytomegalieviren nachgewiesen werden. Das Kollektiv setzt sich aus HIV-infizierten Patienten, Nierentransplantierten und Frühgeborenen zusammen. Der Antigennachweis wurde mit einem Schnelltest durchgeführt, der auf dem Nachweis CMV-spezifischer Kernproteine mittels monoklonalem Antikörper in der Zellkultur beruht. Die beschriebene Methode wurde mit dem herkömmlichen Nachweis von CMV-Antigen in der Zellkultur verglichen. Bei Patienten, die aufgrund ihrer beeinträchtigten Immunitätslage keine eindeutige serologische Reaktion auf eine CMV-Infektion zeigten, konnte das Virus in der Bronchiallavage oder im Urin nachgewiesen werden. Der Test dauert nicht länger als 24 Stunden. Die Brauchbarkeit und Zuverlässigkeit dieses Antigen-Schnelltests für die Diagnose einer CMV-Infektion bei abwehrgeschwächten Patienten konnten belegt werden. Neueste medikamentöse Behandlungsmöglichkeiten der CMV-Infektion und die Risiken von Folgeschäden fordern den verstärkten Einsatz routinemäßiger Antigenuntersuchungen bei unterschiedlichen Probenmaterialien.
    Notes: Summary Laboratory diagnosis of 24 cases of human cytomegalovirus (HCMV) infection in patients with the acquired immunodeficiency syndrome, renal transplant recipients and premature infants was achieved. These results were obtained by a rapid, sensitive and versatile HCMV-antigen detection method, which combined cell culture and immunoperoxidase staining with a monoclonal antibody to an HCMV “early” nuclear protein. The results were compared with HCMV isolation by the conventional cell culture method. While some of these immunocompromised patients lacked a significant antibody response, infective HCMV could be detected in the patients' urine and bronchial lavage fluid. The diagnostic procedure took no longer than 24 h. The usefulness of this antigen test for an effective diagnosis in immunocompromised individuals was demonstrated. We recommend routine analysis of various specimens, since recent developments in chemotherapy of HCMV infection and the risks of long-term damage demand immediate management of the patients concerned.
    Type of Medium: Electronic Resource
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  • 5
    ISSN: 1439-0973
    Source: Springer Online Journal Archives 1860-2000
    Topics: Medicine
    Description / Table of Contents: Zusammenfassung 24 männliche, homosexuelle Personen, die an dem Lymphadenopathie- oder erworbenen Immundefektsyndrom erkrankt sind, wurden mit indirektem ELISA und Western blot unter Verwendung monoklonaler „Tracer“ auf HIV-Antikörper in den Immunglobulinklassen A, G, M und den Immunglobulinsubklassen G 1–4 untersucht. Alle untersuchten Patienten wiesen HIV-spezifische Serum-Antikörper in der Immunglobulinsubklasse G1 auf, etwa die Hälfte im IgG3, nur zwei bzw. einer im IgG2 und IgG4. IgM-Antikörper gegen HIV waren nur bei einem Patienten nachweisbar, bei dem eine Serokonversion bei Verlaufsuntersuchungen mit mehreren Blutproben festgestellt wurde. Von 12 Patienten mit Zeichen einer beginnenden Enzephalitis wurden auch Liquorproben getestet. Während die liquorständigen Antikörper gegen HIV im allgemeinen auf die IgG-Subklasse 1 beschränkt sind, ließen sich in zwei Fällen zusätzlich in den Blutproben nicht vorhandene IgM-Antikörper finden. Die intrathekale, pathognomonische Antikörperproduktion bei HIV-Infektion, im wesentlichen gegen die Strukturproteine gp120, gp41 und p24 gerichtet, kann durch die vergleichende Messung von Antikörpern gegen das Herpes simplex-Virus in Blut- und Liquorproben abgesichert werden.
    Notes: Summary Twenty-four homosexual adult patients suffering from LAS or AIDS were investigated for immunoglobulin class- and IgG subclass-specific antibodies to human immunodeficiency virus (HIV) by the indirect ELISA and Western blot using monoclonal tracer antibodies. All patients revealed HIV-specific serum antibodies of IgG subclass 1, and half of them IgG3. Only two had IgG2 and one IgG4 antibodies. IgM-anti-HIV was present in a person who presented a seroconversion in subsequent blood specimens. In twelve patients who developed signs of an ongoing encephalitis, cerebrospinal fluid specimens were also tested. HIV-specific IgG antibodies were usually restricted to the subclass 1. In two cases specific IgM was found to be present, although lacking in the blood specimens. By comparison with HSV antibody detection in blood and CSF, an intrathecal, possibly pathognomonic antibody formation to HIV could be confirmed, mainly directed to gp120, gp41 and p24.
    Type of Medium: Electronic Resource
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  • 6
    ISSN: 1439-0973
    Source: Springer Online Journal Archives 1860-2000
    Topics: Medicine
    Description / Table of Contents: Zusammenfassung In 175 Seren von gesunden und an primären oder sekundären Herpesvirusinfektionen erkrankten Personen wurden mit einem indirekten ELISA unter Verwendung von trägergebundenem Antigen (CMV, VZV, HSV) und monoklonalen Zweitantikörpern Subklassen-spezifische Immunglobuline in den Klassen A, G und M sowie in den IgG-Subklassen 1 bis 4 bestimmt. Auf ähnliche Weise wurden mit einem indirekten IFT EBV-spezifische Viruskapsid-Antikörper untersucht. Nur IgG1 Antikörper waren bei nahezu allen untersuchten Personen nachzuweisen. Die Bestimmung des virusspezifischen IgA und IgG1/IgG3 kann die konventionelle Serodiagnostik (IgM, IgG) von frischen Infektionen oder Reaktivierungen mit VZV, EBV und möglicherweise CMV ergänzen. Weiterhin wird die Differenzierung zwischen Primär- und Sekundärinfektionen mit CMV und VZV in einigen Fällen dadurch möglich, daß in aufeinanderfolgenden Serumproben IgG3 früher als IgG1 nachzuweisen ist. Rekurrente Herpesinfektionen können nicht serologisch diagnostiziert werden.
    Notes: Summary In 175 sera from healthy persons as well as those suffering from primary or secondary herpes virus infections/reactivations, serum antibodies were assessed by an indirect ELISA in the immunoglobulin classes A, G and M and the subclasses G1-4, using carrier-fixed antigens (CMV, VZV, HSV) and monoclonal tracer antibodies. In a similar way EBV-specific antibodies were tested by an indirect IFT. Only IgG1 antibodies were detectable in nearly all persons. Virusspecific IgA and IgG3 may support conventional serological methods (IgM, IgG) indicating recent infection/reactivation with VZV, EBV and possibly CMV. Furthermore, differentiation of primary and secondary CMV and VZV infection was possible in some cases, when IgG3 was detectable before IgG1 in subsequent blood specimens. Recurrent herpes lesions could not be diagnosed serologically.
    Type of Medium: Electronic Resource
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