Low correlation of human cytomegalovirus DNA amplification by polymerase chain reaction with cytomegalovirus disease in organ transplant recipients

Weber, Bernard; Nestler, Ulf; Ernst, Wolfgang; Rabenau, Holger F.; Braner, J.; Birkenbach, A.; Scheuermann, Ernst; Schoeppe, W; Doerr, Hans Wilhelm

doi:10.1002/jmv.1890430217

Cited by 38 publications

(23 citation statements)

References 25 publications

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“…Furthermore, samples with low levels of antigenemia and a large number of copies of CMV DNA were observed. Similar differences between the results of an antigenemia assay and quantitative PCR have been reported by others (5,14,21), but the clinical significance of large CMV DNA copy numbers with a low or a negative antigenemia assay result remains to be elucidated.…”

Section: Discussionsupporting

confidence: 70%

Quantification of Human Cytomegalovirus DNA in Bone Marrow Transplant Recipients by Real-Time PCR

Griscelli¹,

Barrois²,

Chauvin³

et al. 2001

J Clin Microbiol

110

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A real-time PCR assay was developed to quantify human cytomegalovirus (CMV) DNA in peripheral blood leukocytes (PBLs) of bone marrow transplantation patients. Unlike other teams, we quantified CMV and the glyceraldehyde-3-phosphate dehydrogenase (GAPDH) gene using a plasmid containing both sequences as an external standard. Tenfold serial dilutions of this plasmid yielded overlapping standard curves that allowed the quantification of CMV and GAPDH gene copies in an efficient and accurate manner. Sequential blood samples (164 specimens) were collected from 16 patients. PBLs were tested by the pp65 antigenemia assay and quantitative CMV and GAPDH gene PCRs. CMV DNA was detected by PCR in 13 patients a mean of 15 days prior to the appearance of antigenemia. The administration of anti-CMV drugs led to a rapid decrease in the numbers of viral copies and positive nuclei. Real-time PCR assay results correlated with those of the CMV pp65 antigenemia assay (P < 0.00001). The TaqMan assay may be a useful tool for rapid quantification of CMV infection and for monitoring of CMV reactivation in bone marrow transplantation recipients.Human cytomegalovirus (CMV) is a well-known cause of mortality in blood and bone marrow transplantation (BMT) patients. Monitoring of CMV reactivation from latency is critical for these patients. Prophylaxis against CMV disease with ganciclovir (8, 9) or foscarnet (16) in asymptomatic BMT recipients has been shown to dramatically reduce the incidence of CMV disease (8, 17). As ganciclovir and foscarnet are myelotoxic and nephrotoxic, respectively, full treatment is often started at the time of documented CMV reactivation. The key to efficient and effective management of CMV infection in these patients is a test capable of rapidly monitoring and quantifying the presence of CMV in the blood. This is particularly essential for the identification of subjects at high risk of developing CMV disease, e.g., patients receiving steroid or immunosuppressive compounds for accelerated graft-versus-host disease and also for the application and monitoring of preemptive antiviral therapeutic strategies. The CMV assays presently available and frequently used in this setting include shell vial culture (7), the CMV antigenemia assay (2), PCR for CMV DNA (3), hybrid capture assay for quantitation of CMV DNA (10), and detection of CMV RNA by nucleic acid sequencebased amplification (1).Among white blood cells, peripheral blood leukocytes (PBLs) are the main CMV carriers during active CMV infection. The detection of CMV antigenemia in PBLs has been shown to be an early marker of CMV infection. A monoclonal antibody is used to detect pp65, the CMV lower matrix phosphoprotein in PBLs, and this test is widely used to monitor BMT recipients. Although a correlation was found between the number of pp65-positive PBLs and the development of clinical symptoms, this method (6, 20) poses a number of problems. It is difficult to perform before engraftment because the number of leukocytes is limited and false-negative results are ...

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Section: Discussionsupporting

confidence: 70%

Quantification of Human Cytomegalovirus DNA in Bone Marrow Transplant Recipients by Real-Time PCR

Griscelli¹,

Barrois²,

Chauvin³

et al. 2001

J Clin Microbiol

110

View full text Add to dashboard Cite

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“…Therefore, qualitative PCR-based assays are probably too sensitive for clinical purposes. The plus-minus answer they supply is overly simplistic for clinical purposes, as it only allows for a single threshold to initiate therapy and provides limited feedback on response to therapy (21,28,35).…”

Section: Discussionmentioning

confidence: 99%

Measurement of Human Cytomegalovirus Loads by Quantitative Real-Time PCR for Monitoring Clinical Intervention in Transplant Recipients

Li¹,

Dummer²,

Estes³

et al. 2003

J Clin Microbiol

141

104

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“…Others have reported a similar difference between antigenemia and quantitative PCR results (10,16), but the clinical significance of a high HCMV DNA load associated with a low antigenemia remains to be established.…”

mentioning

confidence: 82%

“…The detection of the pp65 antigen in leukocytes is a sensitive method widely used for the early diagnosis of HCMV infection, but it is laborintensive, requires immediate processing, and relies on a subjective interpretation of the slides (1, 7). Qualitative PCR detection of HCMV DNA in leukocytes or plasma is considered the most sensitive method, but it lacks specificity for the diagnosis of HCMV disease (2,6,16). Quantification of HCMV DNA has been proposed to be more specifically associated with the disease (1,18).…”

mentioning

confidence: 99%

Quantification of Human Cytomegalovirus DNA by Real-Time PCR

et al. 2001

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A quantitative real-time PCR assay was developed to measure human cytomegalovirus (HCMV) DNA load in peripheral blood leukocytes (PBLs). The HCMV DNA load in PBLs was normalized by means of the quantification of a cellular gene (albumin). The results of the real-time PCR assay correlated with those of the HCMV pp65-antigenemia assay (P < 0.0001).Human cytomegalovirus (HCMV) infection is characterized by a primary infection leading to a lifelong persistence of the viral genome. Periodically, the virus reactivates from latency and recovers its ability to multiply. HCMV is a major cause of morbidity and mortality in bone marrow or solid-organ transplant recipients and in AIDS patients. Early diagnosis of HCMV infection in high-risk patients is essential in order to start preemptive treatments (3,13,15). The detection of the pp65 antigen in leukocytes is a sensitive method widely used for the early diagnosis of HCMV infection, but it is laborintensive, requires immediate processing, and relies on a subjective interpretation of the slides (1, 7). Qualitative PCR detection of HCMV DNA in leukocytes or plasma is considered the most sensitive method, but it lacks specificity for the diagnosis of HCMV disease (2, 6, 16). Quantification of HCMV DNA has been proposed to be more specifically associated with the disease (1, 18). Real-time PCR based on the TaqMan technology (4, 5) provides an accurate means to quantify viral DNA with the major advantage of avoiding post-PCR handling that can be the source of DNA carryover. Recent studies report the utility of real-time PCR for the quantification of HCMV DNA (9,11,12,14,17). In these studies, the primers used for PCR were located in the major immediate-early gene (12,14,17), the US17 gene (9), or the glycoprotein B gene (17). As suggested by Yun et al., the sensitivity of quantitative PCR may be dependent on the viral target gene (17); however, the most appropriate region for amplification has not been established, as the sequence diversity of clinical isolates remains to be characterized. In the present study, a real-time PCR assay was developed to quantify HCMV DNA in peripheral blood leukocytes (PBLs) using a target sequence located in the UL83 gene which codes for the lower matrix protein detected in the pp65 antigenemia test. The HCMV DNA load in PBLs was normalized by means of the quantification of a cellular gene (albumin) and the results were compared to those of the pp65 antigenemia assay.DNA extractions were performed in all experiments using the QIAamp blood kit (QIAGEN S. A., Courtaboeuf, France) according to the manufacturer's recommendations, except that DNA was eluted in 200 l of distilled water. To amplify HCMV DNA, primers and probe were defined in the UL83 region as follows: pp549s (direct primer), 5Ј-GTCAGCGTTC GTGTTTCCCA-3Ј; pp812as (reverse primer), 5Ј-GGGACAC AACACCGTAAAGC-3Ј; and pp770s (fluorogenic probe), 5ЈFAM-CCCGCAACCCGCAACCCTTCATG-3ЈTAMRA. No cross-reactivity was observed when the specificity of the primers and probe was tested for other human herp...

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Low correlation of human cytomegalovirus DNA amplification by polymerase chain reaction with cytomegalovirus disease in organ transplant recipients

Cited by 38 publications

References 25 publications

Quantification of Human Cytomegalovirus DNA in Bone Marrow Transplant Recipients by Real-Time PCR

Quantification of Human Cytomegalovirus DNA in Bone Marrow Transplant Recipients by Real-Time PCR

Measurement of Human Cytomegalovirus Loads by Quantitative Real-Time PCR for Monitoring Clinical Intervention in Transplant Recipients

Quantification of Human Cytomegalovirus DNA by Real-Time PCR

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