Literature DB >> 12409382

Human cytomegalovirus DNA in plasma and serum specimens of renal transplant recipients is highly fragmented.

René Boom1, Cees J A Sol, Tim Schuurman, Alex Van Breda, Jan F L Weel, Marcel Beld, Ineke J M Ten Berge, Pauline M E Wertheim-Van Dillen, Menno D De Jong.   

Abstract

Quantitation of cytomegalovirus (CMV) DNA in plasma and serum by PCR is increasingly used to identify patients at risk for developing CMV disease and to monitor the efficacy of antiviral therapy. Although CMV DNA levels are generally interpreted as viral loads, the exact nature of the viral DNA in these specimens is unknown. We studied the state of CMV DNA in plasma and serum specimens obtained from three renal transplant recipients at peak viral DNA levels during primary CMV infection. For this purpose, DNA isolated from these specimens was fractionated by size, and CMV DNA levels in the resulting DNA fractions were measured by quantitative PCR targeted at large (578-bp) and small (134-bp) amplicons. These experiments showed that the molecular sizes of DNA fragments from which CMV DNA is amplified were small (<2,000 bp), indicating that CMV DNA in plasma and serum is highly fragmented. Furthermore, CMV DNA levels were consistently higher when targeted at the smaller amplicon, providing additional evidence for the fragmentation of viral DNA. In conclusion, the first results with three patients have shown that CMV DNA in plasma and serum is highly fragmented and does not necessarily reflect the amount of infectious virus. These observations have potential consequences for understanding CMV pathogenesis and interpreting CMV DNA levels in individual patient management.

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Year:  2002        PMID: 12409382      PMCID: PMC139725          DOI: 10.1128/JCM.40.11.4105-4113.2002

Source DB:  PubMed          Journal:  J Clin Microbiol        ISSN: 0095-1137            Impact factor:   5.948


  32 in total

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  20 in total

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2.  Optimization of quantitative detection of cytomegalovirus DNA in plasma by real-time PCR.

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3.  Cytomegalovirus quantitation by real-time PCR is unaffected by delayed separation of plasma from whole blood.

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5.  Evaluation of the Epstein-Barr virus R-gene quantification kit in whole blood with different extraction methods and PCR platforms.

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6.  Does Size Matter? Comparison of Extraction Yields for Different-Sized DNA Fragments by Seven Different Routine and Four New Circulating Cell-Free Extraction Methods.

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7.  Diagnostic value of measuring Epstein-Barr virus (EBV) DNA load and carcinoma-specific viral mRNA in relation to anti-EBV immunoglobulin A (IgA) and IgG antibody levels in blood of nasopharyngeal carcinoma patients from Indonesia.

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8.  Monitoring cytomegalovirus infection in adult and pediatric bone marrow transplant recipients by a real-time PCR assay performed with blood plasma.

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9.  Validation of clinical application of cytomegalovirus plasma DNA load measurement and definition of treatment criteria by analysis of correlation to antigen detection.

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Journal:  J Clin Microbiol       Date:  2004-04       Impact factor: 5.948

10.  Optimized quantification of fragmented, free circulating DNA in human blood plasma using a calibrated duplex real-time PCR.

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