2013
DOI: 10.1128/jcm.03201-12
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Comparison of Typing Methods with a New Procedure Based on Sequence Characterization for Salmonella Serovar Prediction

Abstract: bAs the development of molecular serotyping approaches is critical for Salmonella spp., which include >2,600 serovars, we performed an initial evaluation of the ability to identify Salmonella serovars using (i) different molecular subtyping methods and (ii) a newly implemented combined PCR-and sequencing-based approach that directly targets O-and H-antigen-encoding genes. Initial testing was performed using 46 isolates that represent the top 40 Salmonella serovars isolated from human and nonhuman sources, as r… Show more

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Cited by 96 publications
(79 citation statements)
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“…enterica isolates (n ϭ 754 tested) were incorrectly serotyped by traditional serotyping, and thus molecular serotyping may aid in identification (37). Serovar was confirmed by PCR detection of the Salmonella O serogroup genes by a multiplex PCR assay that simultaneously targets genes for five Salmonella O antigens (B, C1, C2-C3, D1, and E1), as described by Ranieri et al (35) and Herrera-Léon et al (38); in addition, PCR amplification and sequencing of the genes encoding the H1 and H2 antigens were performed. Primer sets, DNA amplification, and PCR conditions for fliC (encodes H1 antigen) and fljB (encodes H2 antigen) have been previously described by Imre et al (39) and Mortimer et al (40).…”
Section: Methodsmentioning
confidence: 99%
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“…enterica isolates (n ϭ 754 tested) were incorrectly serotyped by traditional serotyping, and thus molecular serotyping may aid in identification (37). Serovar was confirmed by PCR detection of the Salmonella O serogroup genes by a multiplex PCR assay that simultaneously targets genes for five Salmonella O antigens (B, C1, C2-C3, D1, and E1), as described by Ranieri et al (35) and Herrera-Léon et al (38); in addition, PCR amplification and sequencing of the genes encoding the H1 and H2 antigens were performed. Primer sets, DNA amplification, and PCR conditions for fliC (encodes H1 antigen) and fljB (encodes H2 antigen) have been previously described by Imre et al (39) and Mortimer et al (40).…”
Section: Methodsmentioning
confidence: 99%
“…Primer sets, DNA amplification, and PCR conditions for fliC (encodes H1 antigen) and fljB (encodes H2 antigen) have been previously described by Imre et al (39) and Mortimer et al (40). DNA sequence data were compared to sequences in an internal database (CUFSL) of H1 and H2 sequences, as previously described (35). Molecular serotyping results were able to resolve serovar conflicts for the 12 isolates with different serovars identified by traditional serotyping and PFGE.…”
Section: Methodsmentioning
confidence: 99%
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“…array technology , PCR (Paddock et al, 2012), real-time PCR (Anklam et al, 2012;Fratamico et al, 2011). For a more in depth study of molecular serotyping approaches for Salmonella see Ranieri et al, 2013; for E. coli see DebRoy et al, 2011; for L. monocytogenes see Doumith et al, 2005, Kérouanton et al, 2010and Vitullo et al, 2013; and for Campylobacter see Poly et al, 2011. For the four pathogens considered in this Opinion molecular serotyping is considered to provide a low to moderate discriminatory capability. This is normally similar or marginally higher than traditional serotyping as sub-types can often be recognised within serotypes.…”
Section: Molecular Serotypingmentioning
confidence: 99%
“…Sin embargo, el poder de discriminación del PFGE, es decir, su capacidad de diferenciar entre cepas, es limitada si se compara con la secuenciación de genomas completos. De hecho, se estima que sólo 1% del genoma es analizado cuando se observa el patrón de bandas generadas por el PFGE 10,11 . En varios estudios e investigaciones epidemiológicas ha quedado de manifiesto la limitación del PFGE, sobre todo en casos donde las cepas involucradas son de tipo monomórficas o clonales.…”
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