Estimation of Performance Characteristics of Analytical Methods for Mycobacterium avium subsp. paratuberculosis Detection in Dairy Products

Butot, Sophie; Ricchi, M.; Sevilla, Iker A.; Michot, Lise; Molina, Elena; Tello, Maitane; Russo, Simone; Arrigoni, N.; Garrido, Joseba M.; Tomás, David

doi:10.3389/fmicb.2019.00509

Cited by 21 publications

(10 citation statements)

References 44 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…However, when researchers in other laboratories have attempted to adopt the optimised phage assay or the PMS-phage assay, technology transfer has generally not been a smooth process (e.g. Butot et al 2019 ), and considerable training and troubleshooting has been needed from QUB researchers. We acknowledged some time ago (Foddai and Grant 2017 ) that the PMS-phage assay has a complex, multi-step protocol that does not lend itself well to high-throughput testing of milk samples.…”

Section: Introductionmentioning

confidence: 99%

A novel one-day phage-based test for rapid detection and enumeration of viable Mycobacterium avium subsp. paratuberculosis in cows’ milk

Foddai

Grant

2020

Appl Microbiol Biotechnol

View full text Add to dashboard Cite

Bacteriophage-based methods for the rapid detection of viable Mycobacterium avium subsp. paratuberculosis (MAP) in veterinary specimens are a recent addition to the Johne’s disease diagnostic toolbox. Here, we report the use of D29 mycobacteriophage-coated tosylactivated paramagnetic beads to capture and concentrate MAP cells from samples (termed phagomagnetic separation, PhMS) and then naturally lyse viable MAP cells (from the inside out) to provide DNA for IS900 qPCR purposes. Transmission electron microscopy confirmed that D29 phages had bound to beads in the correct orientation and that the phage-coated beads captured MAP cells from a suspension. During test optimization, conventional IS900 PCR results were used to subjectively assess the effect of different phage:bead coating ratios, differing amounts of coated beads during PhMS, optimal incubation time post-PhMS to obtain maximal MAP DNA, and the potential benefit of a brief heat shock (55 °C/1 min) prior to IS900 TaqMan qPCR. The limit of detection 50% (LOD50%) of the optimised PhMS-qPCR assay was 10.00 MAP cells/50 ml milk (95% CI 1.20–82.83). Finally, in order to demonstrate the new assay’s ability to detect viable MAP in naturally contaminated milk, bulk tank milk samples from 100 dairy farms were tested. Forty-nine (49%) of these tested PhMS-qPCR-positive, with viable MAP numbers detected ranging from 3–126 MAP/50 ml. The novel PhMS-qPCR assay is a sensitive, specific and easy-to-apply phage-based assay for viable MAP, with potential application for milk surveillance or diagnosis of Johne’s disease. Key points • Phage-coated magnetic beads could capture, concentrate and lyse MAP cells from milk. • PhMS-qPCR assay proved to be a rapid, sensitive and specific test for viable MAP. • A potential application of PhMS-qPCR assay for milk surveillance was demonstrated.

show abstract

Section: Introductionmentioning

confidence: 99%

A novel one-day phage-based test for rapid detection and enumeration of viable Mycobacterium avium subsp. paratuberculosis in cows’ milk

Foddai

Grant

2020

Appl Microbiol Biotechnol

View full text Add to dashboard Cite

show abstract

“…For the usage of PMS-PA for milk, it is crucial to know that: (i) maximal numbers of MAP cells were found to sediment in the pellet fraction upon centrifugation at 2500 g for 15 min at ambient temperature; (ii) milk specimens should be refrigerated at 4 °C after collection and MAP testing should commence within 24 h, or, when not possible, specimens can be frozen at −70 °C for up to one month without significant loss of MAP viability [ 92 ]. However, the PMS-PA performance characteristics obtained by Butot et al [ 94 ] were inconsistent with those published by Foddai and Grant [ 43 ]. Using the most probable number enumeration technique to determine the reference value, the LOD 50 of PMS-PA was assessed to be 3.7 log 10 CFU/50 mL of both raw and heat-treated milk.…”

Section: Combination Of Phage Amplification Assay With Peptide-medmentioning

confidence: 80%

“…Different paramagnetic beads coated with antibodies and/or peptides were evaluated with the aim of determining the capture efficiency and specificity for MAP cells [ 91 , 94 ]. The most common beads for MAP capture are MyOne Tosylactivated Dynabeads, which were used in all studies summarized in Table 5 and Table 6 .…”

Section: Combination Of Phage Amplification Assay With Peptide-medmentioning

confidence: 99%

Phage Amplification Assay for Detection of Mycobacterial Infection: A Review

Beinhauerová

Slaná

2021

Microorganisms

View full text Add to dashboard Cite

An important prerequisite for the effective control, timely diagnosis, and successful treatment of mycobacterial infections in both humans and animals is a rapid, specific, and sensitive detection technique. Culture is still considered the gold standard in the detection of viable mycobacteria; however, mycobacteria are extremely fastidious and slow-growing microorganisms, and therefore cultivation requires a very long incubation period to obtain results. Polymerase Chain Reaction (PCR) methods are also frequently used in the diagnosis of mycobacterial infections, providing faster and more accurate results, but are unable to distinguish between a viable and non-viable microorganism, which results in an inability to determine the success of tuberculosis patient treatment or to differentiate between an active and passive infection of animals. One suitable technique that overcomes these shortcomings mentioned is the phage amplification assay (PA). PA specifically detects viable mycobacteria present in a sample within 48 h using a lytic bacteriophage isolated from the environment. Nowadays, an alternative approach to PA, a commercial kit called Actiphage™, is also employed, providing the result within 6–8 h. In this approach, the bacteriophage is used to lyse mycobacterial cells present in the sample, and the released DNA is subsequently detected by PCR. The objective of this review is to summarize information based on the PA used for detection of mycobacteria significant in both human and veterinary medicine from various kinds of matrices.

show abstract

“…In practice, potential false positive results may arise with plaque-based phage assays due to ineffective viricide treatment, meaning that some plaques would be due to non-inactivated D29 phages, or some cells bursting before plating in agar happens, also releasing D29 phages that will interact with M. smegmatis lawn to form plaques. Early adopters of the phage-PCR assay or PMS-phage assay have run into such issues, and have found the multiple steps and transfers involved, the timed incubation steps, the need for molten agar and an M. smegmatis culture, and one or two overnight incubations tedious ( 32 ). In my experience of transferring our optimized Phage assay or PMS-phage assays to a number of other laboratories, this has rarely proved to be a straightforward process and a lot of follow-up troubleshooting activity has ensued.…”

Section: What Does a Phage Assay Positive Results Mean?mentioning

confidence: 99%

Bacteriophage-Based Methods for Detection of Viable Mycobacterium avium subsp. paratuberculosis and Their Potential for Diagnosis of Johne's Disease

Grant

2021

Front. Vet. Sci.

View full text Add to dashboard Cite

Bacteriophage-based methods for detecting Mycobacterium avium subsp. paratuberculosis (MAP) are a potential new approach for diagnosis of Johne's disease (JD). The basis of these tests is a mycobacteriophage (D29) with a lytic lifecycle that is able to infect a range of Mycobacterium spp., not just MAP. When added to a test sample, the phages will bind to and infect mycobacterial cells present. If the host mycobacterial cells are viable, the phages will take over the metabolic machinery of the cells to replicate and produce multiple copies of themselves (phage amplification), before weakening the host cell walls by enzyme action and causing cell lysis. Cell lysis releases the host cell contents, which will include ATP, various enzymes, mycobacterial host DNA and progeny D29 phages; all of which can become the target of subsequent endpoint detection methods. For MAP detection the released host DNA and progeny phages have principally been targeted. As only viable mycobacterial cells will support phage amplification, if progeny phages or host DNA are detected in the test sample (by plaque assay/phage ELISA or qPCR, respectively) then viable mycobacteria were present. This mini-review will seek to: clearly explain the basis of the phage-based tests in order to aid understanding; catalog modifications made to the original plaque assay-based phage amplification assay (FASTPlaqueTB™) over the years; and summarize the available evidence pertaining to the performance of the various phage assays for testing veterinary specimens (bovine milk, blood and feces), relative to current JD diagnostic methods (culture, fecal PCR, and blood-ELISA).

show abstract

Estimation of Performance Characteristics of Analytical Methods for Mycobacterium avium subsp. paratuberculosis Detection in Dairy Products

Cited by 21 publications

References 44 publications

A novel one-day phage-based test for rapid detection and enumeration of viable Mycobacterium avium subsp. paratuberculosis in cows’ milk

A novel one-day phage-based test for rapid detection and enumeration of viable Mycobacterium avium subsp. paratuberculosis in cows’ milk

Phage Amplification Assay for Detection of Mycobacterial Infection: A Review

Bacteriophage-Based Methods for Detection of Viable Mycobacterium avium subsp. paratuberculosis and Their Potential for Diagnosis of Johne's Disease

Contact Info

Product

Resources

About