Multiplex lateral flow test sensitivity and specificity in detecting influenza A, B and SARS-CoV-2 in adult patients in a UK emergency department

被引:0
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作者
Batra, Rahul [1 ]
Blandford, Edward [2 ]
Kulasegaran-Shylini, Raghavendran [2 ]
Futschik, Matthias E. [2 ,3 ]
Bown, Abbie [4 ]
Catton, Matthew [4 ]
Conti-Frith, Hermione [4 ]
Alexandridou, Alexandra [4 ]
Gill, Rebecca [4 ]
Milroy, Clara [4 ]
Harper, Sean [2 ]
Gettings, Holly [5 ]
Noronha, Maryann [5 ]
Harrison, Hooi-Ling [5 ]
Douthwaite, Sam [6 ]
Nebbia, Gaia [6 ]
Klapper, Paul E. [2 ,7 ]
Tunkel, Sarah [2 ]
Vipond, Richard [4 ]
Hopkins, Susan [2 ]
Fowler, Tom [2 ,8 ]
机构
[1] St Thomas Hosp, Dept Infect Dis, London, England
[2] UK Hlth Secur Agcy, London, England
[3] Univ Plymouth, Fac Hlth, Sch Biomed Sci, Plymouth, England
[4] UK Hlth Secur Agcy, Salisbury, England
[5] Guys & St Thomas NHS Fdn Trust, Emergency Dept, London, England
[6] Guys & St Thomas NHS Fdn Trust, Dept Infect, London, England
[7] Univ Manchester, Manchester, England
[8] Queen Mary Univ London, William Harvey Res Inst, London, England
关键词
COVID-19; emergency department; respiratory; Diagnostic Tests;
D O I
10.1136/emermed-2024-214177
中图分类号
R4 [临床医学];
学科分类号
1002 ; 100602 ;
摘要
Background Rapid identification of individuals with acute respiratory infections is crucial for preventing nosocomial infections. For rapid diagnosis, especially in EDs, lateral flow devices (LFDs) are a convenient, inexpensive option with a rapid turnaround. Several 'multiplex' LFDs (M-LFDs) now exist, testing for multiple pathogens from a single swab sample. We evaluated the real-world performance of M-LFD versus PCR testing in detecting influenza A, B and SARS-CoV-2) in the ED setting. Methods After preliminary evaluation of an M-LFD (SureScreen) with laboratory-grown virus and PCR-negative clinical samples, it was evaluated in a real-world setting at the ED of St Thomas' Hospital (London, UK) from 1 December 2022 to 21 April 2023. Eligible participants were >= 18 years of age, admitted with respiratory symptoms and received concurrent M-LFD and PCR tests. Main endpoints were sensitivity to detect influenza A/B (primary) and SARS-CoV-2 (secondary) versus PCR. The probability of a true positive in relation to viral concentration (expressed as PCR cycle threshold (Ct)) was analysed using logistic regression. Results In total, 808 symptomatic participants were included (49.8% female; mean age 46.9 years). Test sensitivity (95% CI) was 67.0% (56.9% to 76.1%) for influenza A (n=100), 94.1% (71.3% to 99.9%) for influenza B (n=17) and 48.2% (39.7% to 56.8%) for SARS-CoV-2 (n=141). Sensitivity for SARS-CoV-2 was significantly lower than that for influenza A and B (p=0.0057 and p=0.00088, respectively). The probability of a true positive was 98% for Ct<25 for influenza A and SARS-CoV-2 (influenza B non-evaluable). No co-infections were identified by PCR or M-LFD. Conclusion The real-world performance of SureScreen M-LFD was consistent with laboratory evaluation and achieved a high sensitivity for individuals with high viral concentration, most likely to be infectious. Given the representative UK population sample, results could be generalised for use in other settings.
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