Utility of droplet digital PCR for the quantitative detection of polyomavirus JC in clinical samples

被引:13
作者
Giovannelli, Irene [1 ]
Ciccone, Nunziata [2 ]
Vaggelli, Guendalina [2 ]
Della Malva, Nunzia [2 ]
Torricelli, Francesca [3 ]
Rossolini, Gian Maria [1 ,2 ,4 ]
Giannecchini, Simone [1 ]
机构
[1] Univ Florence, Dept Expt & Clin Med, Viale Morgagni 48, I-50134 Florence, Italy
[2] Univ Florence, Careggi Univ Hosp, Clin Microbiol & Virol unit, Florence, Italy
[3] Careggi Univ Hosp, Genet Diagnost Unit, Florence, Italy
[4] Univ Siena, Dept Med Biotechnol, Siena, Italy
关键词
ddPCR; qPCR; Polyomavirus JC; PML diagnostics; PROGRESSIVE MULTIFOCAL LEUKOENCEPHALOPATHY; VIRUS; DNA; DISEASE; RISK;
D O I
10.1016/j.jcv.2016.07.008
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
Background: Quantitative PCR (qPCR) is the standard molecular method for detection of polyomavirus JC (JCPyV) DNA reactivation in serum and cerebrospinal fluid (CSF) in patients at risk of progressive multifocal leukoencephalopathy (PML). Recently, digital PCR has shown potential benefits over qPCR in viral diagnostics. Objective: To evaluate the performance of droplet digital PCR (ddPCR) assay in assessing JCPyV-DNA status in clinical samples of patients at risk for PML. Study design: JCPyV specific ddPCR was developed with primers/probes targeting Large T and the noncoding control region used in qPCR. The ddPCR accuracy of JCPyV-DNA quantification was investigated using serial dilutions of genomic JCPyV-DNA. The ddPCR JCPyV-DNA quantification and qPCR confirmation were performed on 150 CSF and 100 serum clinical samples. Results: Using genomic JCPyV-DNA, ddPCR was highly sensitive, repeatable and reproducible for both molecular targets. Using clinical samples, JCPyV-DNA was detected in 13% of CSF and in 50% of serum samples with limit of detection of 30 copies/ml. Among the 19 JCPyV-DNA-positive CSF detected using the ddPCR, 15 also tested positive with the qPCR. Among the 50 JCPyV-DNA-positive serum identified with ddPCR, 41 tested positive with qPCR. All the ddPCR-negative samples were negative when assessed using qPCR. Additionally, the mean JCPyV-DNA viral load obtained with ddPCR in all samples was not significantly different from that of qPCR. Conclusion: The results demonstrate that ddPCR is a highly sensitive alternative for measuring JCPyV-DNA that should be considered in clinical diagnostic testing of JCPyV-DNA in patients at risk of PML and other associated diseases. (C) 2016 Elsevier B.V. All rights reserved.
引用
收藏
页码:70 / 75
页数:6
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