Performance of an antigen assay for diagnosing acute hepatitis E virus genotype 3 infection

被引:41
|
作者
Tremeaux, Pauline [1 ]
Lhomme, Sebastien [1 ,2 ]
Chapuy-Regaud, Sabine [1 ,2 ]
Peron, Jean-Marie [3 ]
Alric, Laurent [4 ]
Kamar, Nassim [1 ,5 ]
Izopet, Jacques [1 ,2 ]
Abravanel, Florence [1 ,2 ]
机构
[1] CHU Toulouse, Hop Purpan, Natl Reference Ctr Hepatitis E, Virol Lab, F-31300 Toulouse, France
[2] Ctr Physiopathol Toulouse Purpan, INSERM, U1043, F-31300 Toulouse, France
[3] CHU Toulouse, Hop Purpan, Dept Gastroenterol, F-31300 Toulouse, France
[4] CHU Toulouse, Hop Purpan, Serv Med Interne, F-31300 Toulouse, France
[5] CHU Toulouse, Hop Rangueil, Dept Nephrol Dialyse & Transplantat Multiorgane, F-31300 Toulouse, France
关键词
Hepatitis E virus; HEV-antigen; Immunocompromised patients; Immunocompetent patients; ORGAN-TRANSPLANT RECIPIENTS; IMMUNOCOMPROMISED PATIENTS; DEVELOPED-COUNTRIES; DIVERSITY; IMMUNOCOMPETENT; FRANCE; IGG;
D O I
10.1016/j.jcv.2016.03.019
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
Background: Hepatitis E virus (HEV) is a major cause of hepatitis worldwide. Its diagnosis is based on the detection of anti-HEV IgM and/or HEV-RNA. Objective: To evaluate the performance of the Wantai HEV-antigen (Ag) ELISA(Plus) assay for diagnosing acute HEV infections. Study design: Specificity was assessed using 100 blood samples containing no anti-HEV IgM, anti-HEV IgG, or HEV-RNA. Cross reactivity was assessed using samples positive for hepatitis C virus RNA (n = 10), Epstein-Barr virus DNA (n = 10) and cytomegalovirus DNA (n = 10). Serial dilutions of 4 HEV RNA positive samples were used to estimate the corresponding viremia detected with the Ag assay. Blood samples from 33 immunocompetent and 31 immunocompromised patients with an acute HEV genotype 3 infection, HEV-RNA positive, were tested to assess diagnostic sensitivity. Results: The HEV-Ag assay was 100% specific, with no cross-reactivity. The lower viremias detected ranged from 10(3) copies/ml to 10(5) copies/ml (800-80,000 UI/ml). Diagnostic sensitivity for an acute HEV infection was 91%, with no significant difference between immunocompetent (88%) and immunocompromised (94%) patients. The HEV-Ag assay was more frequently positive in immunocompromised patients at the acute phase (94%) than was the anti-HEV IgM test (71%; p = 0.04). The HEV-Ag assay ratio was correlated with HEV-RNA viral load ( p = 0.54; p < 0.0001). Conclusion: The HEV-Ag assay performed well and could be suitable for laboratories with no molecular diagnosic facilities. (C) 2016 Elsevier B.V. All rights reserved.
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页码:1 / 5
页数:5
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