Ganzenmueller, Tina, Kaiser, Rolf, Baier, Claas, Wehrhane, Marlies, Hilfrich, Brigitta, Witthuhn, Jenny, Flucht, Sandra and Heim, Albert (2020). Comparison of the performance of the Panther Fusion respiratory virus panel to R-Gene and laboratory developed tests for diagnostic and hygiene screening specimens from the upper and lower respiratory tract. J. Med. Microbiol., 69 (3). S. 427 - 436. LONDON: MICROBIOLOGY SOC. ISSN 1473-5644

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Abstract

Introduction. Diagnosis of acute respiratory infections (ARIs) can be facilitated by the Panther Fusion (PF) automatic, random access PCR system for the detection of influenzavirus A (Flu A) and B (Flu B), parainfluenzavirus (Paraflu), respiratory syncytial virus (RSV), human metapneumovirus (hMPV), rhinovirus (RV) and human adenovirus (AdV) in nasopharyngeal swabs. Aim. To evaluate the performance of PF in comparison with established methods, including subsets of (1) lower respiratory tract (LRT) specimens and (2) upper respiratory tract (URT) hygiene screening specimens of patients without ARI symptoms. Methodology. The performance characteristics of PF were compared with bioMerieux R-Gene and laboratory-developed PCR tests (LDTs). Overall, 1544 specimens with 6658 individual diagnostic requests were analysed. Results. The overall concordances of PF and LDTs for Flu A, Flu B and AdV were 98.4, 99.9 and 96.1%, respectively; by re-testing of discrepant specimens concordances increased to 99.4, 99.9 and 98.0%, respectively. Initial concordances of PF and R--Gene assays for RSV, Paraflu, hMPV and RV were 98.4, 96.3, 99.3 and 96.0%, respectively, and retest concordances were 99.7, 97.9, 99.9 and 98.9%, respectively. No differences to the overall performance were found for the subgroups of LRT and hygiene screening specimens. PCR cycle threshold (Ct) values correlated very well between methods, indicating that a semi-quantitative diagnostic approach using Ct values (e.g. highly vs. weakly positive) could augment the diagnostic information. Conclusion. PF performed similar to R-Gene and LDTs not only for its intended use but also for LRT and hygiene screening specimens with shorter hands-on and turnaround times.

Item Type: Journal Article
Creators:
CreatorsEmailORCIDORCID Put Code
Ganzenmueller, TinaUNSPECIFIEDUNSPECIFIEDUNSPECIFIED
Kaiser, RolfUNSPECIFIEDUNSPECIFIEDUNSPECIFIED
Baier, ClaasUNSPECIFIEDUNSPECIFIEDUNSPECIFIED
Wehrhane, MarliesUNSPECIFIEDUNSPECIFIEDUNSPECIFIED
Hilfrich, BrigittaUNSPECIFIEDUNSPECIFIEDUNSPECIFIED
Witthuhn, JennyUNSPECIFIEDUNSPECIFIEDUNSPECIFIED
Flucht, SandraUNSPECIFIEDUNSPECIFIEDUNSPECIFIED
Heim, AlbertUNSPECIFIEDUNSPECIFIEDUNSPECIFIED
URN: urn:nbn:de:hbz:38-351137
DOI: 10.1099/jmm.0.001133
Journal or Publication Title: J. Med. Microbiol.
Volume: 69
Number: 3
Page Range: S. 427 - 436
Date: 2020
Publisher: MICROBIOLOGY SOC
Place of Publication: LONDON
ISSN: 1473-5644
Language: English
Faculty: Unspecified
Divisions: Unspecified
Subjects: no entry
Uncontrolled Keywords:
KeywordsLanguage
INFLUENZA-A; DISEASE SEVERITY; ADENOVIRUS DNA; VIRAL LOAD; PCR; BURDEN; IMPACT; INFECTIONS; CHILDREN; ASSAYMultiple languages
MicrobiologyMultiple languages
URI: http://kups.ub.uni-koeln.de/id/eprint/35113

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