Publication | Open Access
Primer-mediated enzymatic amplification of cytomegalovirus (CMV) DNA. Application to the early diagnosis of CMV infection in marrow transplant recipients.
106
Citations
32
References
1989
Year
Viral ReplicationViral DiagnosticsImmunologyPathologyPrimer-mediated Enzymatic AmplificationNucleic Acid Amplification TestViral PersistenceCmv InfectionHematologyMarrow Transplant RecipientsCell TransplantationDiagnostic VirologyTransplantationVirologyChronic Viral InfectionCmv CultureHivDna ReactivityCmv Antibody StatusNucleic Acid AmplificationMedicine
A nucleic acid amplification procedure, the polymerase chain reaction (PCR), has been used to establish a diagnostic assay for the identification of cytomegalovirus (CMV) immediate-early sequences in clinical specimens. Preliminary testing against virus-infected cell cultures indicated that the PCR assay was highly CMV-specific, recognizing both wild-type and laboratory strains of CMV. There was no cross-reactivity with human DNA or with DNA from other herpes viruses. The sensitivity of the assay, using cloned CMV AD169 Eco RI fragment-J as template, was 1 viral genome per 40,000 cells. In a prospective study of CMV infection in bone marrow transplant recipients, the PCR assay correctly identified four patients with confirmed CMV infection. In three of these patients who were followed longitudinally, correlation of DNA reactivity with CMV culture and CMV antibody status over time indicated that DNA was the most sensitive marker for the diagnosis of CMV infection.
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