A rapid phage assay for detection of viable Mycobacterium avium subsp. paratuberculosis in milk

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作者
Sepideh Hosseiniporgham
Lucio Rebechesu
Pierangela Pintore
Stefano Lollai
Maria Dattena
Simone Russo
Angelo Ruiu
Leonardo A. Sechi
机构
[1] Università di Sassari,Dipartimento di Scienze Biomediche
[2] Istituto Zooprofilattico della Sardegna,National Reference Centre for Paratuberculosis, Sede Territoriale di Piacenza
[3] Agenzia Regionale Ricerca in Agricoltura (AGRIS),undefined
[4] Istituto Zooprofilattico Sperimentale della Lombardia e dell’Emilia Romagna (IZSLER),undefined
[5] Istituto Zooprofilattico della Sardegna,undefined
[6] Azienda Ospedaliera Universitaria,undefined
[7] Mediterranean Center for Disease Control,undefined
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摘要
Paratuberculosis is an incurable gastroenteritis among ruminants that is promoted by Mycobacterium avium subsp. paratuberculosis (MAP), an acid-fast mycobacterium. To accelerate the detection of viable pathogen, a conventional (peptide mediated magnetic separation: PMS) and novel (phage-bead qPCR: PBQ) phage based assay was optimized. A superior limit of detection (LOD) of 10 MAP per 10 mL milk was suggested for PBQ compared to 100 cells/10 mL for PMS-phage assay. Via PBQ, viable MAP was found in 48.78% out 41 unpasteurized sheep and goat milk samples. Sheep milk samples (n = 29) that were tested by PMS-phage assay contained no viable MAP. The absence of viable MAP in milk collected from 21 of the recent sheep animals was also confirmed by PBQ after a 2-week gap. Although, the two phage assays comparably detected no viable MAP in the milk samples, MAP DNA and antibodies against MAP were recognized in milk and sera of some of these animals within two instances of sampling representing that some sheep animals were MAP shedders. In conclusion, PBQ and PMS-phage could be promising methods for the assessment of MAP viability in milk samples. However, PBQ was privileged over the PMS-phage assay due to the lower LOD, rapidity, higher sensitivity, lack of need to M. smegmatis and consequent virucidal treatment that are essential in PMS-phage assay for making lawn and inactivation of exogenous mycobacteriophages respectively.
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