Pervasive Recombination and Sympatric Genome Diversification Driven by Frequency-Dependent Selection in <i>Borrelia burgdorferi</i>, the Lyme Disease Bacterium

Haven, James; Vargas, Levy C.; Mongodin, Emmanuel F.; Xue, Vincent; Hernández, Yözen; Pagan, Pedro; Fraser, Claire M.; Schutzer, Steven E.; Luft, Benjamin J.; Casjens, Sherwood; Qiu, Wei

doi:10.1534/genetics.111.130773

Cited by 68 publications

(128 citation statements)

References 89 publications

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“…This is similar to the finding that the locations of important virulence factor-encoding genes, such as dbpA-dbpB, ospA-ospB, and ospC, are conserved in particular genome segments, even though sizes may be somewhat different due to genetic rearrangements, especially on the outer edges of the linear plasmids. Gene duplication followed by rearrangement and mutations appear to have resulted in the evolution and antigenic variation of a number of B. burgdorferi virulence factors and other proteins (4,28,43,62,82,97,109,110). Often, duplicated genes that encode functionally redundant proteins that exhibit overlapping roles are present in the same operon, with each protein demonstrating altered specificities for host cell factors.…”

Section: Discussionmentioning

confidence: 99%

Detection of Established Virulence Genes and Plasmids To Differentiate Borrelia burgdorferi Strains

2012

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ABSTRACTBorrelia burgdorferisensu stricto is the major causative agent of Lyme disease in the United States, whileB. gariniiandB. afzeliiare more prevalent in Europe. The highly complex genome ofB. burgdorferiis comprised of a linear chromosome and a large number of variably sized linear and circular plasmids. Many plasmids of this spirochete are unstable during its culturein vitro. Given that many of theB. burgdorferivirulence factors identified to date are plasmid encoded, spirochetal plasmid content determination is essential for genetic analysis of Lyme pathogenesis. Although PCR-based assays facilitate plasmid profiling of sequencedB. burgdorferistrains, a rapid genetic content determination strategy for nonsequenced strains has not yet been described. In this study, we combined pulsed-field gel electrophoresis (PFGE) and Southern hybridization for detection of genes encoding known virulence factors,ribosomal RNA genespacer restriction fragment length polymorphismtypes (RSTs),ospCgroup determination, and sequencing of the variabledbpAandospCgenes. We show that two strains isolated from the same tick and both originally named N40 are in fact very distinct. Furthermore, we failed to detectbbk32, which encodes a fibronectin-binding adhesin, in one “N40” strain. Thus, two distinct strains that show different plasmid profiles, as determined by PFGE and PCR, were isolated from the same tick and vary in theirospCanddbpAsequences. However, both belong to group RST3B.

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Section: Discussionmentioning

confidence: 99%

Detection of Established Virulence Genes and Plasmids To Differentiate Borrelia burgdorferi Strains

2012

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“…Recombination is known to maintain sequence polymorphisms within B. burgdorferi s.l. populations (Haven et al, 2011) and the high number of STs can impede the identification of associations with clinical manifestations of LB. The test for recombination (not shown) indicated that this is a frequent event even for chromosomal housekeeping genes, as other studies (Haven et al, 2011) have also revealed.…”

Section: Association With Disseminated/persistent Forms Of Lyme Borrementioning

confidence: 99%

Imbalanced presence of Borrelia burgdorferi s.l. multilocus sequence types in clinical manifestations of Lyme borreliosis

Coipan

Jahfari

Fonville

et al. 2016

Infection, Genetics and Evolution

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In this study we used typing based on the eight multilocus sequence typing scheme housekeeping genes (MLST) and 5S-23S rDNA intergenic spacer (IGS) to explore the population structure of Borrelia burgdorferi sensu lato isolates from patients with Lyme borreliosis (LB) and to test the association between the B. burgdorferi s.l. sequence types (ST) and the clinical manifestations they cause in humans. Isolates of B. burgdorferi from 183 LB cases across Europe, with distinct clinical manifestations, and 257 Ixodes ricinus lysates from The Netherlands, were analyzed for this study alone. For completeness, we incorporated in our analysis also 335 European B. burgdorferi s.l. MLST profiles retrieved from literature. Borrelia afzelii and Borrelia bavariensis were associated with human cases of LB while Borrelia garinii, Borrelia lusitaniae and Borrelia valaisiana were associated with questing I. ricinus ticks. B. afzelii was associated with acrodermatitis chronica atrophicans, while B. garinii and B. bavariensis were associated with neuroborreliosis. The samples in our study belonged to 251 different STs, of which 94 are newly described, adding to the overall picture of the genetic diversity of Borrelia genospecies. The fraction of STs that were isolated from human samples was significantly higher for the genospecies that are known to be maintained in enzootic cycles by mammals (B. afzelii, B. bavariensis, and Borrelia spielmanii) than for genospecies that are maintained by birds (B. garinii and B. valaisiana) or lizards (B. lusitaniae). We found six multilocus sequence types that were significantly associated to clinical manifestations in humans and five IGS haplotypes that were associated with the human LB cases. While IGS could perform just as well as the housekeeping genes in the MLST scheme for predicting the infectivity of B. burgdorferi s.l., the advantage of MLST is that it can also capture the differential invasiveness of the various STs.

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“…The 5S (rrf)-23S (rrl) intergenic spacer region is a tandemly repeated sequence that is unique to B. burgdorferi sensu lato and has been used to differentiate and identify different isolates of Borrelia spirochetes in many different sample types including ticks (Postic et al, 1994;Humphrey et al, 2010), blood meal hosts (Chu et al, 2008) and patients (Postic et al, 1998;Rijpkema et al, 2009). This is in contrast with other markers such as the ospA or ospC genes are not ideal for phylogenetic analyses of inferences because of frequent recombination events (Haven et al, 2011). Previous studies from the northeastern or midwestern US have examined the genetic structure of B. burgdorferi with other genes and found limited genetic structure at a local scale but evidence of regional barriers to gene flow (Qiu et al, 2002;Humphrey et al, 2010).…”

Section: Introductionmentioning

confidence: 99%

Comparative genetic diversity of Lyme disease bacteria in Northern Californian ticks and their vertebrate hosts

Swei

Bowie

2015

Ticks and Tick-borne Diseases

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Pervasive Recombination and Sympatric Genome Diversification Driven by Frequency-Dependent Selection in Borrelia burgdorferi, the Lyme Disease Bacterium

Cited by 68 publications

References 89 publications

Detection of Established Virulence Genes and Plasmids To Differentiate Borrelia burgdorferi Strains

Detection of Established Virulence Genes and Plasmids To Differentiate Borrelia burgdorferi Strains

Imbalanced presence of Borrelia burgdorferi s.l. multilocus sequence types in clinical manifestations of Lyme borreliosis

Comparative genetic diversity of Lyme disease bacteria in Northern Californian ticks and their vertebrate hosts

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