Comparison of Three Commercially Available Dengue NS1 Antigen Capture Assays for Acute Diagnosis of Dengue in Brazil

被引:108
作者
Queiroz Lima, Monique da Rocha [1 ]
Ribeiro Nogueira, Rita Maria [1 ]
Schatzmayr, Hermann Goncalves [1 ]
dos Santos, Flavia Barreto [1 ]
机构
[1] Fiocruz MS, Inst Oswaldo Cruz, Flavivirus Lab, BR-21045900 Rio De Janeiro, Brazil
来源
PLOS NEGLECTED TROPICAL DISEASES | 2010年 / 4卷 / 07期
关键词
LINKED-IMMUNOSORBENT-ASSAY; NONSTRUCTURAL PROTEIN NS1; VIRUS-INFECTION; LABORATORY DIAGNOSIS; CELLS; IMMUNOASSAY; CIRCULATION; EXPRESSION; ANTIBODIES; MEMBRANE;
D O I
10.1371/journal.pntd.0000738
中图分类号
R51 [传染病];
学科分类号
100401 ;
摘要
Background: Dengue is associated with explosive urban epidemics and has become a major public health problem in many tropical developing countries, including Brazil. The laboratory diagnosis of dengue can be carried out using several approaches, however sensitive and specific assays useful to diagnose in the early stage of fever are desirable. The flavivirus non-structural protein NS1, a highly conserved and secreted glycoprotein, is a candidate protein for rapid diagnosis of dengue in endemic countries. Methodology/Principal Findings: We aimed to evaluate the potential use of 3 commercial kits in a panel of 450 serum samples for early diagnosis of dengue in Brazil. The PanBio Early ELISA (PanBio Diagnostics) showed a sensitivity of 72.3% (159/220) and a specificity of 100%, while the sensitivity of the Platelia (TM) NS1 assay (Biorad Laboratories) was 83.6% (184/ 220). However, the highest sensitivity (89.6%; 197/220) was obtained by using the NS1 Ag Strip (Biorad Laboratories). A lower sensitivity was observed in DENV-3 cases by all 3 kits. Serum positive by virus isolation were more often positive than cases positive by RT-PCR by all three assays and a higher detection rate was observed during the first four days after the onset of the symptoms. The presence or absence of IgM showed no influence in the confirmation by the pan-E Early ELISA (P = 0,6159). However, a higher confirmation by both Platelia (TM) NS1 (Biorad) and Dengue NS1 Ag Strip (Biorad) in the absence of IgM was statistically significant (P < 0,0001 and P = 0,0008, respectively). Only the Platelia (R) NS1 test showed a higher sensitivity in confirming primary infections than secondary ones. Conclusions/Significance: The results indicate that commercial kits of dengue NS1 antigen are useful for the laboratory diagnosis of acute primary and secondary dengue. It can be used in combination with the MAC-ELISA for case detection and as screening test to complement viral isolation.
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