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Novel Method for Processing Respiratory Specimens for Detection of Mycobacteria by Using C18-Carboxypropylbetaine: Blinded Study
Authors:Charles G. Thornton   Kerry M. MacLellan   Thomas L. Brink   Jr.   Denise E. Lockwood   Mark Romagnoli   June Turner   William G. Merz   Richard S. Schwalbe   Marcia Moody   Yvonne Lue     Selvin Passen
Affiliation:Department of Molecular Biology and Genetics1. and Department of Microbiology,2. Quest Diagnostics—Baltimore, Baltimore, Maryland 21227; Department of Pathology, Johns Hopkins Medical Institutes, Baltimore, Maryland 212873.; District of Columbia Department of Human Services Bureau of Laboratories, Washington, D.C. 200014.; Department of Pathology, University of Maryland at Baltimore, Baltimore, Maryland 212015.; and Quest Diagnostics—Teterboro, Teterboro, New Jersey 076086.
Abstract:A novel method for processing respiratory specimens to improve culture and acid-fast staining of mycobacteria is introduced. This new method utilized N,N-dimethyl-N-(n-octadecyl)-N-(3-carboxypropyl)ammonium inner salt (Chemical Abstract Service no. 78195-27-4), also known as C18-carboxypropylbetaine (CB-18). In a blinded, five-center study, CB-18-based processing was compared to the standard method combining NALC and NaOH (NALC/NaOH). A total of 573 respiratory specimens were tested. Individual specimens were split approximately equally; the host institutions processed half of each specimen by the NALC/NaOH method, while the other half was processed with CB-18 at Quest Diagnostics—Baltimore. A total of 106 specimens were culture positive for acid-fast bacilli (AFB). Replacement of the primary decontamination agent with CB-18 caused changes in all diagnostic parameters. Aggregate culture sensitivity improved by approximately 43% (P < 0.01), and smear sensitivity improved by approximately 58% (P < 0.01). The sensitivity of smear relative to that of M. tuberculosis isolates exceeded 93% (P < 0.01) when specimens were processed with CB-18. The average times to a positive result were reduced by 7.3 days in liquid culture (P < 0.01) and 5.3 days on solid media (P < 0.05); however, the CB-18 method had a 20.8% contamination rate in liquid culture versus a rate of approximately 7.5% with NALC/NaOH processing. There were also unusual reductions in liquid culture sensitivity and smear specificity among CB-18-processed specimens. The characteristics of the latter parameters suggested that refinement of the CB-18 processing method should allow further improvements in culture sensitivity. This study showed that the CB-18 method has the potential to improve both smear and culture detection for these important human pathogens.
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