Comparison of rapid detection methods for influenza A virus and their value in health-care management of institutionalized geriatric patients.

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J Clin Microbiol. 1994 January; 32(1): 70-74

Comparison of rapid detection methods for influenza A virus and their value in health-care management of institutionalized geriatric patients.

G P Leonardi, H Leib, G S Birkhead, C Smith, P Costello and W Conron

Department of Pathology, Nassau County Medical Center, East Meadow, New York 11554.

ABSTRACT

Respiratory specimens from 160 geriatric patients with suspectedinfluenza illness were used to evaluate the abilities of twoenzyme immunoassays (EIAs; Directigen FLU-A [Becton DickinsonMicrobiology Systems, Cockeysville, Md.] and Prima EIA [Baxter/BartelsDiagnostics, Inc., Issaquah, Wash.]) and direct immunofluorescencetesting (immunofluorescence assay [IFA]) to identify influenzaA virus. In comparison with culture isolation, the sensitivitiesand specificities of the IFA, Directigen FLU-A, and Prima EIAwere 92.5 and 97.2%, 86.8 and 99.1%, and 92.5 and 98.1%, respectively.In contrast to EIA, IFA was labor intensive and required a highdegree of technical expertise, and the results of IFA were difficultto interpret. These factors may preclude the use of IFA fortesting large numbers of specimens. A retrospective epidemiologicsurvey of influenza infection was done in six geriatric institutionswhich had used either rapid and culture testing or culture alone.Preventable cases of influenza A virus infection ranged from9 to 38% of all cases in facilities which used culture testingonly and which had not instituted amantadine prophylaxis. Theuse of direct specimen testing is recommended as an adjunctto culture isolation for the identification of influenza A virus.Use of a combination of these methods permits the timely administrationof appropriate antiviral therapy and infection control measures,while it also permits the antigenic surveillance of circulatinginfluenza strains, which is necessary for present vaccine efficacyevaluations and the creation of future effective vaccine formulations.

J Clin Microbiol. 1994 January; 32(1): 70-74

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