Avian influenza virus (AIV) infection,
caused by influenza virus
type A, is an infectious, acute respiratory disease of birds related
to influenza outbreaks worldwide. The highly pathogenic AIV subtype
H5N1 has crossed species barriers to infect mammals, including humans,
with fatal outcomes and has received attention as a potential pandemic
threat. A rapid and timely detection in poultry is vitally important
to prevent the virus spread. Despite their great sensitivity, conventional
detection methods such as real-time reverse transcription-polymerase
chain reaction and the agar gel precipitation test are time-consuming
and labor-intensive and require special training. In this work, an
immunowall device was evaluated as an easier and faster way for detecting
AIV H5-hemagglutinin (AIV H5-HA). For detection, fluorescence-labeled
or enzyme-labeled antibody was employed as a labeling antibody in
a sandwich immunoassay. Both were shown in this paper to be easier
and faster assays for detection compared with the conventional enzyme-linked
immunosorbent assay (ELISA) kit. In addition, high selectivity was
achieved for AIV H5-HA detection after the evaluation of other different
HA virus subtypes. The limit of detection was 0.23 ng/mL for the enzyme-labeled
antibody. This value was equivalent to that of the conventional ELISA
kit but 8 times faster (31 min compared to 260 min). The detection
range was 0.23–100 ng/mL. The immunowall device with the enzyme-labeled
antibody offers a rapid, sensitive, selective, and simple immunoassay
system for future H5 AIV real sample detection.
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