Rapid determination of vapA/vapB genotype in Rhodococcus equi using a differential polymerase chain reaction method

Oldfield, Christopher J.; Bonella, Hal; Renwick, Lynne; Dodson, Hilary I.; Alderson, Grace; Goodfellow, Michael

doi:10.1023/b:anto.0000020383.66622.4d

Cited by 21 publications

(25 citation statements)

References 33 publications

Supporting

Mentioning

Contrasting

Unclassified

Order By: Relevance

“…Thus, vapA and vapB seem to be divergent allelic variants of the same ancestral vap gene, consistent with the observed mutual exclusivity of their corresponding PCR gene markers among R. equi isolates (38,39). Similarly, vapG and vapL, both of which are transcribed in the opposite direction relative to the other vap genes, appear to be derived from a common ancestral gene despite mapping to very different sites in their corresponding PAIs (Fig.…”

Section: Vol 190 2008 Sequence Of Rhodococcus Equi Vapb Virulence Psupporting

confidence: 77%

“…Six vap family genes were identified in the pVAPB1593 PAI: the previously described vapB (39,49), plus five new vap multigene family members, which we named vapJ, vapK1, vapK2, vapM, and vapL ( Fig. 1; also see Tables S1 and S2 in the supplemental material).…”

Section: Vol 190 2008 Sequence Of Rhodococcus Equi Vapb Virulence Pmentioning

confidence: 99%

“…Nonequine R. equi isolates often produce a larger (20-kDa) variant surface lipoprotein antigen, VapB (10,49), which is very similar in primary structure to VapA (78% amino acid sequence identity) (39). VapA and VapB (and corresponding genes) are mutually exclusive, i.e., they do not occur in the same isolate, suggesting that they are allelic variants of one locus that has divergently evolved in two different plasmid subpopulations (38).…”

mentioning

confidence: 99%

See 2 more Smart Citations

Evolution of theRhodococcus equi vapPathogenicity Island Seen through Comparison of Host-AssociatedvapAandvapBVirulence Plasmids

et al. 2008

View full text Add to dashboard Cite

The pathogenic actinomycete Rhodococcus equi harbors different types of virulence plasmids associated with specific nonhuman hosts. We determined the complete DNA sequence of a vapB ؉ plasmid, typically associated with pig isolates, and compared it with that of the horse-specific vapA ؉ plasmid type. pVAPB1593, a circular 79,251-bp element, had the same housekeeping backbone as the vapA ؉ plasmid but differed over an Ϸ22-kb region. This variable region encompassed the vap pathogenicity island (PAI), was clearly subject to selective pressures different from those affecting the backbone, and showed major genetic rearrangements involving the vap genes. The pVAPB1593 PAI harbored five different vap genes (vapB and vapJ to -M, with vapK present in two copies), which encoded products differing by 24 to 84% in amino acid sequence from the six full-length vapA ؉ plasmid-encoded Vap proteins, consistent with a role for the specific vap gene complement in R. equi host tropism. Sequence analyses, including interpolated variable-order motifs for detection of alien DNA and reconstruction of Vap family phylogenetic relationships, suggested that the vap PAI was acquired by an ancestor plasmid via lateral gene transfer, subsequently evolving by vap gene duplication and sequence diversification to give different (host-adapted) plasmids. The R. equi virulence plasmids belong to a new family of actinobacterial circular replicons characterized by an ancient conjugative backbone and a horizontally acquired niche-adaptive plasticity region.Rhodococcus equi is a member of the mycolic acid-containing group of actinobacteria, or mycolata, which also includes the Corynebacterium, Gordonia, Mycobacterium, and Nocardia genera (18). Like many other actinomycetes, R. equi is ubiquitous in nature and lives as a saprophyte in soil (25,35,41). The genus Rhodococcus is a genetically diverse taxon that may be empirically classified into two groups (4, 23): the nonpathogenic, or environmental, rhodococci, exemplified by Rhodococcus erythropolis, which includes metabolically versatile bacteria of industrial interest (32), and the pathogenic rhodococci, with two species, the plant pathogen Rhodococcus fascians (22) and the animal pathogen R. equi (25,35,41). All rhodococci typically harbor large conjugative plasmids encoding nicheadaptive functions, such as various primary and secondary metabolic processes in the environmental species and host colonization (virulence) factors in the pathogenic ones. Some of these extrachromosomal replicons are linear megaplasmids of up to 1 Mb in size, whereas others are circular plasmids of Ϸ100 kb (34, 55).R. equi can be isolated from pulmonary and extrapulmonary pyogranulomatous infections in various mammalian hosts. It causes equine purulent bronchopneumonia, or rattles, a severe respiratory disease of foals characterized by extensive abscessation of the lung parenchyma, lymphadenitis, and a high mortality rate. R. equi is also an opportunistic human pathogen associated with AIDS and immunosuppression. Human rho...

show abstract

Section: Vol 190 2008 Sequence Of Rhodococcus Equi Vapb Virulence Psupporting

confidence: 77%

Section: Vol 190 2008 Sequence Of Rhodococcus Equi Vapb Virulence Pmentioning

confidence: 99%

mentioning

confidence: 99%

See 1 more Smart Citation

Evolution of theRhodococcus equi vapPathogenicity Island Seen through Comparison of Host-AssociatedvapAandvapBVirulence Plasmids

et al. 2008

View full text Add to dashboard Cite

show abstract

“…Early studies showed that VapA-encoding virulence plasmids were typical of equine strains (28,29), while a second plasmid type, encoding VapB, a VapA variant (24), was common among nonequine (pig and human) isolates (10,(30)(31)(32)(33). Recently, the existence of a third type of R. equi virulence plasmid was identified in bovine and human isolates that were initially deemed to be "plasmidless" (because vapA and vapB negative) but that tested positive for a traA plasmid conjugal transfer gene marker (34).…”

mentioning

confidence: 99%

An Invertron-Like Linear Plasmid Mediates Intracellular Survival and Virulence in Bovine Isolates of Rhodococcus equi

et al. 2015

View full text Add to dashboard Cite

dWe report a novel host-associated virulence plasmid in Rhodococcus equi, pVAPN, carried by bovine isolates of this facultative intracellular pathogenic actinomycete. Surprisingly, pVAPN is a 120-kb invertron-like linear replicon unrelated to the circular virulence plasmids associated with equine (pVAPA) and porcine (pVAPB variant) R. equi isolates. pVAPN is similar to the linear plasmid pNSL1 from Rhodococcus sp. NS1 and harbors six new vap multigene family members (vapN to vapS) in a vap pathogenicity locus presumably acquired via en bloc mobilization from a direct predecessor of equine pVAPA. Loss of pVAPN rendered R. equi avirulent in macrophages and mice. Mating experiments using an in vivo transconjugant selection strategy demonstrated that pVAPN transfer is sufficient to confer virulence to a plasmid-cured R. equi recipient. Phylogenetic analyses assigned the vap multigene family complement from pVAPN, pVAPA, and pVAPB to seven monophyletic clades, each containing plasmid type-specific allelic variants of a precursor vap gene carried by the nearest vap island ancestor. Deletion of vapN, the predicted "bovine-type" allelic counterpart of vapA, essential for virulence in pVAPA, abrogated pVAPN-mediated intramacrophage proliferation and virulence in mice. Our findings support a model in which R. equi virulence is conferred by host-adapted plasmids. Their central role is mediating intracellular proliferation in macrophages, promoted by a key vap determinant present in the common ancestor of the plasmid-specific vap islands, with host tropism as a secondary trait selected during coevolution with specific animal species.

show abstract

“…It can also be used for detection of many equine diseases (Oldfield et al, 2004;Ocampo-Sosa et al, 2007;Pusterla et al, 2007;Letek et al, 2008;Monego et al, 2009). Polymerase chain reaction (PCR)-based diagnostic tests can allow rapid and sensitive detection of equine infectious pathogen (Paxson, 2008).…”

Section: Polymerase Chain Reaction (Pcr)mentioning

confidence: 99%

Biotechnological tools for diagnosis of equine infectious diseases

Prasad¹,

Brar²,

Ikbal³

et al. 2016

JEBAS

View full text Add to dashboard Cite

Rapid diagnosis of infectious diseases and appropriate treatment with in time are important steps that promote optimal clinical outcomes and general public health. Today there is large number of new technologies such as nanotechnology, biosensors, and microarray techniques, are being developed and used as diagnostic tools for equine infectious diseases. Nucleic acid based techniques such as polymerase chain reaction (PCR) have become conventional tools in veterinary research and plays an important role in specific typing determinations as well as for rapid screening of ample numbers of samples at the time of equine disease outbreaks. Other biotechnological techniques are populous to be used in the coming times as they can enhance diagnostic efficacy in less time and cost as compared to conventional techniques. This review focuses on biotechnological tools available for equine diseases diagnosis and its applications hold great promise for improving the speed and accuracy of diagnostics for equine infectious diseases.

show abstract

Rapid determination of vapA/vapB genotype in Rhodococcus equi using a differential polymerase chain reaction method

Cited by 21 publications

References 33 publications

Evolution of theRhodococcus equi vapPathogenicity Island Seen through Comparison of Host-AssociatedvapAandvapBVirulence Plasmids

Evolution of theRhodococcus equi vapPathogenicity Island Seen through Comparison of Host-AssociatedvapAandvapBVirulence Plasmids

An Invertron-Like Linear Plasmid Mediates Intracellular Survival and Virulence in Bovine Isolates of Rhodococcus equi

Biotechnological tools for diagnosis of equine infectious diseases

Contact Info

Product

Resources

About