Author: Lin, Yong; Fu, Yongfeng; Xu, Menghua; Su, Liyun; Cao, Lingfeng; Xu, Jin; Cheng, Xunjia
Title: Evaluation of a PCR/ESIâ€MS platform to identify respiratory viruses from nasopharyngeal aspirates Cord-id: 4qop47fs Document date: 2015_5_20
ID: 4qop47fs
Snippet: Acute respiratory tract infection is a major cause of morbidity and mortality worldwide, particularly in infants and young children. Highâ€throughput, accurate, broadâ€range tools for etiologic diagnosis are critical for effective epidemic control. In this study, the diagnostic capacities of an Ibis platform based on the PCR/ESIâ€MS assay were evaluated using clinical samples. Nasopharyngeal aspirates (NPAs) were collected from 120 children (<5 years old) who were hospitalized with lower resp
Document: Acute respiratory tract infection is a major cause of morbidity and mortality worldwide, particularly in infants and young children. Highâ€throughput, accurate, broadâ€range tools for etiologic diagnosis are critical for effective epidemic control. In this study, the diagnostic capacities of an Ibis platform based on the PCR/ESIâ€MS assay were evaluated using clinical samples. Nasopharyngeal aspirates (NPAs) were collected from 120 children (<5 years old) who were hospitalized with lower respiratory tract infections between November 2010 and October 2011. The respiratory virus detection assay was performed using the PCR/ESIâ€MS assay and the DFA. The discordant PCR/ESIâ€MS and DFA results were resolved with RTâ€PCR plus sequencing. The overall agreement for PCR/ESIâ€MS and DFA was 98.3% (118/120). Compared with the results from DFA, the sensitivity and specificity of the PCR/ESIâ€MS assay were 100% and 97.5%, respectively. The PCR/ESIâ€MS assay also detected more multiple virus infections and revealed more detailed subtype information than DFA. Among the 12 original specimens with discordant results between PCR/ESIâ€MS and DFA, 11 had confirmed PCR/ESIâ€MS results. Thus, the PCR/ESIâ€MS assay is a highâ€throughput, sensitive, specific and promising method to detect and subtype conventional viruses in respiratory tract infections and allows rapid identification of mixed pathogens. J. Med. Virol. 87:1867–1871, 2015. © 2015 Wiley Periodicals, Inc.
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