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Identification and Population Structure of Burkholderia stabilis sp. nov. (formerly Burkholderia cepacia Genomovar IV)
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ABSTRACT
The
Burkholderia cepacia
complex currently comprises five genomic species, i.e.,
B. cepacia
genomovar I,
B. multivorans
(formerly known as
B. cepacia
genomovar II),
B. cepacia
genomovar III,
B. cepacia
genomovar IV, and
B. vietnamiensis
(also known as
B. cepacia
genomovar V). In the absence of straightforward diagnostic tests for the identification of
B. cepacia
genomovars I, III, and IV, the last two genomic species were not formally classified as novel
Burkholderia
species (genomovar I contains the type strain and therefore retains the name
B. cepacia
). In the present study, we describe differential biochemical tests and a
recA
gene-based PCR assay for the routine identification of strains currently known as
B. cepacia
genomovar IV and propose formal classification of this organism as
Burkholderia stabilis
sp. nov.
B. stabilis
can indeed be differentiated from all other
B. cepacia
complex strains by the absence of beta-galactosidase activity, from strains of
B. cepacia
genomovars I and III and
B. vietnamiensis
by the inability to oxidize sucrose, and from
B. multivorans
by the lack of growth at 42°C. In addition, analysis with the
recA
gene-derived primers BCRG41 (5′-ACCGGCGAGCAGGCGCTT-3′) and BCRG42 (5′-ACGCCATCGGGCATGGCA-3′) specifically allows the detection of
B. stabilis
strains in a conventional PCR assay. Examination of a set of 21
B. stabilis
strains by means of random amplified polymorphic DNA analysis and pulsed-field gel electrophoresis typing suggested that the genome of this organism is highly conserved, which is in sharp contrast to the generally accepted genomic diversity, variability, and plasticity among
B. cepacia
strains.
American Society for Microbiology
Title: Identification and Population Structure of
Burkholderia stabilis
sp. nov. (formerly
Burkholderia cepacia
Genomovar IV)
Description:
ABSTRACT
The
Burkholderia cepacia
complex currently comprises five genomic species, i.
e.
,
B.
cepacia
genomovar I,
B.
multivorans
(formerly known as
B.
cepacia
genomovar II),
B.
cepacia
genomovar III,
B.
cepacia
genomovar IV, and
B.
vietnamiensis
(also known as
B.
cepacia
genomovar V).
In the absence of straightforward diagnostic tests for the identification of
B.
cepacia
genomovars I, III, and IV, the last two genomic species were not formally classified as novel
Burkholderia
species (genomovar I contains the type strain and therefore retains the name
B.
cepacia
).
In the present study, we describe differential biochemical tests and a
recA
gene-based PCR assay for the routine identification of strains currently known as
B.
cepacia
genomovar IV and propose formal classification of this organism as
Burkholderia stabilis
sp.
nov.
B.
stabilis
can indeed be differentiated from all other
B.
cepacia
complex strains by the absence of beta-galactosidase activity, from strains of
B.
cepacia
genomovars I and III and
B.
vietnamiensis
by the inability to oxidize sucrose, and from
B.
multivorans
by the lack of growth at 42°C.
In addition, analysis with the
recA
gene-derived primers BCRG41 (5′-ACCGGCGAGCAGGCGCTT-3′) and BCRG42 (5′-ACGCCATCGGGCATGGCA-3′) specifically allows the detection of
B.
stabilis
strains in a conventional PCR assay.
Examination of a set of 21
B.
stabilis
strains by means of random amplified polymorphic DNA analysis and pulsed-field gel electrophoresis typing suggested that the genome of this organism is highly conserved, which is in sharp contrast to the generally accepted genomic diversity, variability, and plasticity among
B.
cepacia
strains.
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