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Epstein-Barr virus load in transplant patients: Early detection of post-transplant lymphoproliferative disorders
被引:14
|作者:
Dolores Fellner, Maria
[1
]
Durand, Karina A.
[1
]
Solernou, Veronica
[2
]
Bosaleh, Andrea
[2
]
Balbarrey, Ziomara
[2
]
Garcia de Davila, Maria T.
[2
]
Rodriguez, Marcelo
[3
]
Irazu, Lucia
[3
]
Alonio, Lidia V.
[1
]
Picconi, Maria A.
[1
]
机构:
[1] Carlos G Malbran Natl Inst Infect Dis, Dept Virol, Oncogen Viruses Serv, Av Velez Sarsfield 563,C1282AFF, Buenos Aires, DF, Argentina
[2] Prof Dr Juan P Garrahan Natl Pediat Hosp, Pathol Serv, Pichincha 1890,C1249ABP, Buenos Aires, DF, Argentina
[3] Carlos G Malbran Natl Inst Infect Dis, Dept Parasitol, Operat Team Qual Management, Av Velez Sarsfield 563,C1282AFF, Buenos Aires, DF, Argentina
来源:
关键词:
Epstein-Barr virus;
Early PTLD detection;
Lymphoma;
Real-time PCR;
Transplant patients;
Viral load;
STEM-CELL TRANSPLANTATION;
VIRAL LOAD;
PCR METHOD;
EBV LOAD;
DISEASE;
QUANTIFICATION;
RECIPIENTS;
DIAGNOSIS;
BLOOD;
D O I:
10.1016/j.ram.2016.02.006
中图分类号:
Q93 [微生物学];
学科分类号:
071005 ;
100705 ;
摘要:
High levels of circulating EBV load are used as a marker of post-transplant lymphoproliferative disorders (PTLD). There is no consensus regarding the threshold level indicative of an increase in peripheral EBV DNA. The aim of the study was to clinically validate a developed EBV quantification assay for early PTLD detection. Transversal study: paired peripheral blood mononuclear cells (PBMC), plasma and oropharyngeal lymphoid tissue (OLT) from children undergoing a solid organ transplant with (n = 58) and without (n = 47) PTLD. Retrospective follow-up: 71 paired PBMC and plasma from recipients with (n = 6) and without (n = 6) PTLD history. EBV load was determined by real-time PCR. The diagnostic ability to detect all PTLD (categories 1-4), advanced PTLD (categories 2-4) or neoplastic PTLD (categories 3 and 4) was estimated by analyzing the test performance at different cut-off values or with a load variation greater than 0.5 log units. The higher diagnostic performance for identifying all, advanced or neoplastic PTLD, was achieved with cut-off values of 1.08; 1.60 and 2.47 log EBV gEq/10(5) PBMC or 2.30; 2.60; 4.47 log gEq/10(5) OLT cells, respectively. EBV DNA detection in plasma showed high specificity but low (all categories) or high (advanced/neoplastic categories) sensitivity for PTLD identification. Diagnostic performance was greater when: (1) a load variation in PBMC or plasma was identified; (2) combining the measure of EBV load in PBMC and plasma. The best diagnostic ability to identify early PTLD stages was achieved by monitoring EBV load in PBMC and plasma simultaneously; an algorithm was proposed. (C) 2016 Asociacion Argentina de Microbiologia. Published by Elsevier Espana, S.L.U.
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页码:110 / 118
页数:9
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