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. 2009 Dec 21;4(12):e8360. doi: 10.1371/journal.pone.0008360

A Real-Time PCR Array for Hierarchical Identification of Francisella Isolates

Kerstin Svensson 1,2,*, Malin Granberg 1, Linda Karlsson 1, Vera Neubauerova 3, Mats Forsman 1, Anders Johansson 1,2
Editor: Igor Mokrousov4
PMCID: PMC2793073  PMID: 20027310

Abstract

A robust, rapid and flexible real-time PCR assay for hierarchical genetic typing of clinical and environmental isolates of Francisella is presented. Typing markers were found by multiple genome and gene comparisons, from which 23 canonical single nucleotide polymorphisms (canSNPs) and 11 canonical insertion-deletion mutations (canINDELs) were selected to provide phylogenetic guidelines for classification from genus to isolate level. The specificity of the developed assay, which uses 68 wells of a 96-well real-time PCR format with a detection limit of 100 pg DNA, was assessed using 62 Francisella isolates of diverse genetic and geographical origins. It was then successfully used for typing 14 F. tularensis subsp. holarctica isolates obtained from tularemia patients in Sweden in 2008 and five more genetically diverse Francisella isolates of global origins. When applied to human ulcer specimens for direct pathogen detection the results were incomplete due to scarcity of DNA, but sufficient markers were identified to detect fine-resolution differences among F. tularensis subsp. holarctica isolates causing infection in the patients. In contrast to other real-time PCR assays for Francisella, which are typically designed for specific detection of a species, subspecies, or strain, this type of assay can be easily tailored to provide appropriate phylogenetic and/or geographical resolution to meet the objectives of the analysis.

Introduction

The genus Francisella consists of three species: F. philomiragia, F. novicida, and the etiological agent of the zoonosis tularemia, F. tularensis. In addition, there are several soil bacteria, tick endosymbionts and fish parasites that are genetically closely related to Francisella, but are not (yet at least) assigned to the genus (Figure 1). Three subspecies of F. tularensis are recognized, of which F. tularensis subspp. tularensis and holarctica cause severe, sometimes fatal, disease in humans. The third subspecies, mediasiatica, is rare and its virulence is described as moderate. F. tularensis subsp. holarctica has been isolated throughout the northern hemisphere, while F. tularensis subspp. tularensis and mediasiatica are geographically restricted to North America and Central Asia, respectively. The population structure of the two clinically relevant subspecies, F. tularensis subsp. tularensis (type A) and F. tularensis subsp. holarctica (type B), is highly clonal, a property that facilitates the design of genetic typing systems and deduction of evolutionary relationships among genetic subclades of Francisella, since mutations are mainly inherited vertically [1], [2].

Figure 1. Phylogenies of Francisella based on 16S rDNA and MLVA, respectively.

Figure 1

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A) Phylogeny of Francisella and representative relatives based on alignment of 1,070 bp of the 16S rDNA gene. Bootstrap values are indicated at the branching points. The scale bar indicates 0.02 nucleotide changes per site. Modified from [36]. B) Phylogeny of Francisella based on MLVA. Subspecies and major genetic branches (A1-A2, B1-B5) are indicated. Currently available genome sequences are in black boxes. Multiple strains are indicated by triangles at the branch edges. Modified from Johansson et al 2004 [26].

Tularemia is characterized by an acute course of infection, and mortality rates of F. tularensis subsp. tularensis infections historically reached 5 to 30% before effective antibiotic treatments were available. In contrast, F. tularensis subsp. holarctica infections are milder and may be fatal only to patients with an impaired immune system [3]. F. tularensis can infect humans, via aerosols or the skin, at doses as low as 10 cells [4], [5] and is listed by the CDC as a major potential bioterror agent [6]. Cultivation of F. tularensis is often avoided, since it poses considerable risks of laboratory-acquired infections via aerosolization. Laboratory culture work requires biosafety-level 3 (BSL-3) conditions and primary cultivation from a clinical specimen may require a seven-day incubation before colonies visible to the naked eye appear. To shorten the time required for clinical diagnosis, PCR assays targeting 16S rDNA [7] or specific genes encoding outer membrane proteins such as fopA [8] and lpnA [9][11] have been used to detect Francisella, and several real-time PCR assays have been developed recently that appear to be more sensitive than conventional PCR [12][17]. However, a serious drawback of PCR-detection is that cross-reactivity with environmental non-pathogenic Francisella bacteria may occur [18][20]. Therefore there is a need to develop PCRs for distinguishing clinically relevant Francisella species from closely related non-pathogenic Francisella present in environmental sources.

In research laboratories, isolates of F. tularensis have been identified and classified using a variety of molecular typing methods, including amplified fragment length polymorphism (AFLP) analysis [21], pulse-field gel electrophoresis (PFGE) [22], [23], insertion/deletion (INDEL) mutation analysis [24], multi-locus variable number of tandem repeats analysis (MLVA) [25], [26], multi-locus sequence typing (MLST) [2], and whole genome single-nucleotide polymorphism (SNP) analysis [1]. The highest typing resolution has been achieved by MLVA of rapidly mutating tandem repeats, but at a cost sometimes of incorrectly characterizing relationships among distantly related isolates.

In the present study, we developed a convenient real-time PCR assay based on robust genetic markers (SNPs and INDELs). A desired feature of the assay was that it should be able to distinguish between human pathogenic F.tularensis and the two genetically closely related species F. novicida and F. philomiragia which are of lower clinical relevance and often found in environmental sources. Moreover, the assay should be capable of identifying the subclades of F. tularensis (especially within F. tularensis subsp. holarctica, type B), and be compatible with standard real-time PCR machines that are now widely used in routine diagnostic laboratories. The developed assay meets all of these criteria, and can be tailored to match typing resolution requirements by adding or removing genetic markers as appropriate.

Materials and Methods

Ethics Statement

Ulcer specimens were collected as part of the routine clinical management of patients and the use of them for laboratory service improvement conducted in compliance with the regulation, policies and principles of the Swedish Public Health Service. Approval from an ethics committee was for that reason not sought after. The clinical routine for collecting specimens includes an open friendly verbal communication informing the patient that the sampling purpose is detecting the causative agent of tularemia. A verbal informed consent was required before submitting any sample to the laboratory. The specimens were de-identified and analyzed anonymously.

Isolates and Clinical Specimens

A panel of 62 Francisella isolates (listed in Table 1), spanning as much as possible of the known genetic diversity within the genus, was used to determine the specificity of all of the tested markers (listed in Tables 2 and 3). The final one plate-assay, including 34 genetic markers, was applied to 14 isolates and six patient ulcer specimens obtained in 2008 at Umeå University Hospital, Sweden (Table 4), and also to five additional isolates of global origins (Table 1). The new assay was evaluated along with the standard PCR assay that is used for diagnosis of human ulceroglandular tularemia [27]. Plate design and interpretation of assay results are exemplified in Figure 2 by the analysis of the Live Vaccine Strain (LVS).

Table 1. Sixty-seven isolates of global origins used in this study.

Species (no. isolates) origin FSC no.a NAU IDb Alternative designations Vogler et al. 2009 subclade Johansson et al. 2004 groupc Table 5 geno-type Figure 3 subclade
F. philomiragia (5) Water, Bear River Refuge, UT 037 F0047 ATCC 25016 1 P.ATCC25017
Water, Bear River Refuge, UT 038 F0048 ATCC 25017 1 P.ATCC25017
Water, Odgen Bay Refuge, UT 039 F0049 ATCC 25018 1 P.ATCC25017
Moribund muskrat (Ondatra zibethicus), 1959, Brigham City, UT 144 F0045 ATCC 25015 1 P.ATCC25017
Atlantic cod (Gadus morhua), 2008, Norway 775d DSM18777 1 P.ATCC25017
F. novicida (5) Water, 1950, UT 040 F0050 ATCC 15482, U112 N N 2 N.U112
Human blood, 1991, Houston, TX 156e F0051 fx1 N N 3 N.FSC156
Human blood, 1991, Houston, TX 159 F0052 fx2 N N 3 N.FSC156
Human blood, 2003, Spain 454 FNSp1, F62 4 N.FSC454
Human, 2003, Brazil/UK/Germany 595 F58 5 N.Ftind44/[1], [2], [3]
F. tularensis subsp. mediasiatica (4) Experimental isolate, cap-, Rostov, Russia 122 F0004 (TTC-R)6-4-1 M.Br.FSC 147 M 6 M.FSC147
Midday gerbil (Meriones meridianus), 1965, Kazakhstan 147e F0011 GIEM 543 M.Br.FSC 147 M 6 M.FSC147
Hare, 1965, former USSR, Central Asia 149 F0013 120 M.Br.FSC 147 M 6 M.FSC147
Tick, 1982, former USSR, Central Asia 148 F0012 240 M.Br.FSC 147 M 6 M.FSC147
F. tularensis subsp. tularensis (11) 1960 (Eigelsbach) 013 F0006 FAM standard 7 A1.3/[4], [5]
Tick, 1935, British Columbia, Canada 041 F0005 Vavenby A.I.Br.001/002 A1 7 A1.3/[4], [5]
Squirrel, Georgia, USA 033e SnMF 8 A1.FSC033
Human pleural fluid, 1940, Fox Downs, Ohio, USA 046 F0008 A.I.Br.SCHU S4 A1 9 A1.SCHUS4
Human, 1941, Ohio, USA 237 F0567 Schu S4 A.I.Br.SCHU S4 9 A1.SCHUS4
Mites, 1988, Slovakia 199 F0007 SE-221/38 A.I.Br.SCHU S4 A1 9 A1.SCHUS4
Lab acquired when handling Nevada 14 053 F0009 F.tul AC A.II.Br.001/002 A2 10 A2
Hare, 1953, Nevada, USA 054 F0010 Nevada 14 A.II.Br.001/002 A2 10 A2
Hare, Canada 042 F0296 Utter A.II.Br.003/004 A2 10 A2
Human, 1920, Utah, USA 230 F0419 ATCC 6223 A.II.Br.ATCC 6223 A2 10 A2
1959, USA 604 RKI 03-1300, 8859 10 A2
F. tularensis subsp. holarctica (42) Human lymphnode, 1926, Japan 017 F0016 S-2 B.Br.001/002 B5 11 B5.FSC022
Hare, 1954, Oniwa, Japan 020 F0292 B5 11 B5.FSC022
Human, 1958, Tsuchiya, Japan 021 F0014 B.Br.001/002 B5 11 B5.FSC022
Human, 1950, Ebina, Japan 022 F0015 B.Br.001/002 B5 11 B5.FSC022
Tick, 1954, Fukushima, Japan 023 F0293 TH B5 11 B5.FSC022
Yerma, Japan 024 F0294 B5 11 B5.FSC022
Tick, 1957, Jama, Japan 075 F0017 B.Br.001/002 B5 11 B5.FSC022
Human blood, 1989, Norway 089 F0038 N1/89 (45F2) B.Br.OSU18 B2 12 B2.OSU18
Human blood, 1994, Bergen, Norway 158 F0301 CCUG 33391 B.Br.OSU18 B2 12 B2.OSU18
Beaver, 1976, Montana, USA 035 F0018 B423A B.Br.OSU18 B2 12 B2.OSU18
Hare, 1997, Austria 584 F30 12 B2.OSU18
Human ulcer, 2005, Ljusdal, Sweden 641e 05-32-85 12 B2.OSU18
Human, 2000, Örebro, Sweden 285 F0212 AO7346/00 B.Br.007/008 B4 13 B4.Ftind49/18
Tick, 1941, Montana, USA 012 F0291 425 F4G 13 B4.Ftind49/18
Human ulcer, 2004, Örebro, Sweden 519 04-32-23 13 B4.Ftind49/18
Human, 2004, Umeå, Sweden 663d 13 B4.Ftind49/18
Human, 2000, Uppsala, Sweden 274 F0228 R63/00 B.Br.010/011 Spain, France, & Sweden 13 B4.Ftind49/18
Human, 1993/94, Vosges, France 247 F0020 T 20 B.Br.FTNF002-00 Spain, France, & Sweden 14 B4.FTNF002-00
Hare, 1952, Chateauroux, France 025 F0295 061-1 B.Br.FTNF002-00 Spain, France, & Sweden 14 B4.FTNF002-00
Hare, Castilla y León, Spain 455 FT1 14 B4.FTNF002-00
Human skin lesion, Castilla y León, Spain 456 FT7 14 B4.FTNF002-00
Human, 1995, Ockelbo, Sweden 162 F0162 B.Br.012/013 B3 15 B3.19/[20], [23]
Human, 1995, Ockelbo, Sweden 178 F0044 B.Br.012/013 B3 15 B3.19/[20], [23]
Water, 1980, Crimea, Ukraine 115 F0021 B.Br.013/014 B3 15 B3.19/[20], [23]
Norwegian rat (Rattus norvegicus), 1988, Rostov, Russia 150 F0029 B3 15 B3.19/[20], [23]
Human blood, 1996, Raahe, Finland 250 F0164 B.Br.013/014 B3 16 B3.23/[24], [25]
Human lymph node, 2005, Summi Admin area, Ukraine FDC079d 16 B3.23/[24], [25]
Live vaccine strain, Russia 155 F0566 B.Br.LVS B3 17 B3.LVS
Tick (Dermacentor pictus), 1949, Moscov area, Russia 257e,f F0019 GIEM 503/840 B.Br.013/014 B3 18 B3.RC503
Tick (Dermacentor reticularis), 1995, Lanzhot, Czech Republic 184d F0191 T-35 B1 19 B1.20/21
Tick (Dermacentor reticularis), 1995, Lanzhot, Czech Republic 185 F0192 T-38 B.Br.013/014 B1 19 B1.20/21
Tick (Dermacentor reticularis), 1995, Lanzhot, Czech Republic 186 F0193 T-44 B.Br.013/014 B3 19 B1.20/21
Tick (Ixodes ricinus), 1995, Lanzhot, Czech Republic 187 F0194 T-60 B.Br.013/014 B1 19 B1.20/21
Bank vole (Clethrionomys glareolus), 1977, Seneca district, Slovakia FDC010 19 B1.20/21
Brown hare (Lepus europaeus), 1964, Vidiek district, Slovakia FDC014 19 B1.20/21
Water, 1985, Rostov region, Russia 121 F0025 12267 B.Br.013/014 B1 19 B1.20/21
Human, 1995, Äänekoski, Finland 249 F0163 1468 B.Br.013/014 B1 19 B1.20/21
Water, 1990, Odessa region, Ukraine 124 F0027 14588 B.Br.013/014 B1 20 B1.21/22
Water, 1990, Odessa region, Ukraine 119d 14592 B1 20 B1.21/22
Human, 2001, Oulu university hospital, Finland 293 F0178 T-10023 B.Br.013/014 20 B1.21/22
Human, 1998, Ljusdal, Sweden 200 F0134 3001MA B.Br.013/014 B1 21 B1.FSC200
Human ulcer, 1995, Ljusdal, Sweden 245 F0133 R42/95 B.Br.013/014 B1 21 B1.FSC200
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a

Strain ID in the Francisella Strain Collection (FSC) and Francisella DNA Collection (FDC), Swedish Defense Research Agency, Umeå, Sweden.

b

Strain ID in the Northern Arizona University DNA collection.

c

MLVA-defined groups presented in Johansson et al. 2004. A1, F. tularensis subsp. tularensis subpopulation A1; A2, F. tularensis subsp. tularensis subpopulation A2; B, F. tularensis subsp. holarctica; M, F. tularensis subsp. mediasiatica; N, F. novicida.

d

The isolates FDC079, FSC119, FSC184, FSC663, and FSC775 (F. philomiragia subsp. noatunensis) were typed with the final one-plate assay and were not part of the set of 62 isolates used in the developing stage.

e

The isolates FSC017 (B5), FSC033 (A1), FSC147 (M), FSC156 (N), FSC257 (B3), and FSC641 (B2) were typed with the final one-plate assay, and were part of the set of 62 isolates used in the developing stage, to confirm the typing accuracy of the plate.

f

FSC257 is an alternative name for RC503.

Table 2. SNP markers, genes affected by the SNPs, and primers.

SNP SCHU S4a SNP position SCHU S4 locus ID SCHU S4 gene SNP state Primerb Primer sequencesc
F.1 1312210, FTTr04, 16S T D gcgggcCTATGGATCGTAGCCTTGGt
1379332, FTTr10, Gd A gcgggcagggcggcCTATGGATCGTAGCCTTGGg
1772676 FTTr07 C AGTTGGAAACGACTGTTAATACCGCA
T/N.1 83976 FTT0080 tpiA A D gcgggcAGAAACACATCAATTTATTCGTTCa
G A gcgggcagggcggcAGAAACACATCAATTTATTCGTTCg
C AGCATTTTCAGCTTTTAGGCTACCA
T.1 1165690 FTT1150c putA C D gcgggcagggcggcTGTTGAAAAAGCTCATATGTCAAGc
T A gcgggcTGTTGAAAAAGCTCATATGTCAAGt
C TCATACTCGATCATAAACGCATCA
N.1 83943 FTT0080 tpiA T D gcgggcACAGGAGTTGTGGCTTCACTAGAt
G A gcgggcagggcggcACAGGAGTTGTGGCTTCACTAGAg
C CATCAACTTTAGCTAACAATGAACGAAT
N.2 910194 FTT0901 lpnA A D gcgggcTGTAATCTTACACTTCCTTGTGGa
G A gcgggcagggcggcTGTAATCTTACACTTCCTTGTGGg
C GGCTCTGATGATGCAAAAGC
N.3 780 FTT0001 dnaA T D gcgggcGCAGATCTATAAACTCTTTGAAAt
C A gcgggcagggcggcGCAGATCTATAAACTCTTTGAAAc
C AATTTATTAAAGATTATGTAAATTCTATTCGT
M.2 84027 FTT0080 tpiA G D gcgggcagggcggcTCAGCTTTTAGGCTACCACCg
A A gcgggcTCAGCTTTTAGGCTACCACCa
C CAGGAGTTGTGGCTTCACTAGAGC
A.2 1199395 FTT1182c vacJ A D gcgggcGCATCAACACTATCACTAATCCCCTa
C A gcgggcagggcggcGCATCAACACTATCACTAATCCCCTc
C ATCACCAAGATTTTGCTGTGACATT
A.3 62997 FTT0062 atpA C D gcgggcagggcggcTGCTGTAGCTGCAACAATAATTGc
T A gcgggcTGCTGTAGCTGCAACAATAATTGt
C ATTGCAAACATTGTAAGACAGCTTGAAG
A.4 830716 FTT0810 ybaB T D gcgggcTCGGTAAGTATCGACAATTt
C A gcgggcagggcggcTCGGTAAGTATCGACAATTc
C AGCAGCTGCTATCAAATCTTC
A.5 350750 FTT0351 rplQ C D gcgggcagggcggcTAGAGGCTCAACGATTGc
T A gcgggcTAGAGGCTCAACGATTGt
C TGTCAGCTTCTTTGATTAATC
A.6 1806912 FTT1721 purF T D gcgggcTCGTACTCTTTAAAACCAAGCAt
C A gcgggcagggcggcTCGTACTCTTTAAAACCAAGCAc
C CTGAGGCTGTTTATAAAGCATGTAAAT
B.15 1113816 FTT1103 G D gcgggcagggcggcTCAACTTGGAATCCAAGGCg
A A gcgggcTCAACTTGGAATCCAAGGCa
C GCTTTGTTGATAGCTGCTTGGATACC
B.16 608246 FTT0588 aroA T D gcgggcATGCTAGCAAATTACCATCAAAAGt
G A gcgggcagggcggcATGCTAGCAAATTACCATCAAAAGg
C AACTCTTCTCGCCATCAACTTCTAT
B.17 1743251 FTT1673 ribA T D gcgggcCCAAGAGCTAAATTAGCTTCAAt
G A gcgggcagggcggcCCAAGAGCTAAATTAGCTTCAAg
C TGACCAAGAAGGTAGAGGTATTGGTT
B.18 1756146 FTT1686c T D gcgggcAGCAGCAGGACAAATAGt
C A gcgggcagggcggcAGCAGCAGGACAAATAGc
C TTGTGTCGATTCAAAACCAGACTTA
B.19 1374034 FTT1343c A D gcgggcTTGCTACTGATGGTTTAACTa
C A gcgggcagggcggcTTGCTACTGATGGTTTAACTc
C CAATACGTCACTTATGCAGTGAT
B.20 1396117, FTT1354, pdpC G D gcgggcagggcggcTCTGATGAAGAATATCTTACAg
1789461 FTT1709 A A gcgggcTCTGATGAAGAATATCTTACAa
C ATTATGGCAAAACTATACCTT
B.21e 701320 FTT0684c sthA A D gcgggcACCAAGGTAGATTTGCAGCTACa
G A gcgggcagggcggcACCAAGGTAGATTTGCAGCTACg
C ATCCCTGTTGGGATATCCTCGACTAA
B.22e 1113320 FTT1103 A D gcgggcTGAATACTCTACGCGATAAGATa
G A gcgggcagggcggcTGAATACTCTACGCGATAAGATg
C ATCAGACTTAGGTGTTAGATCAGAGTT
B.23 253121 FTT0240 T D gcgggcTTACTACAAATTCGCCTCTAAt
G A gcgggcagggcggcTTACTACAAATTCGCCTCTAAg
C AGCAAAAGAGCTTACTAAACAATTTGA
B.24 1419996 FTT1373 fabH G D gcgggcagggcggcTATCGCCAGGTTTAATTTGATg
T A gcgggcTATCGCCAGGTTTAATTTGATt
C TCTGCAGCATCTATCCCATTAGCCTTA
B.25 1534495 FTT1484c aceF T D gcgggcTGTATCTAAGACAGCAGTGAAGt
C A gcgggcagggcggcTGTATCTAAGACAGCAGTGAAGc
C ATGGTAGCATAGTTCTAGGAATAAACT
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a

GenBank accession no. AJ749949.

b

D, Primer with derived SNP state; A, Primer with ancestral SNP state; C, Common primer.

c

Primer tails and 3′-end mismatch base are in lower case.

d

No sequences with a G found by BLAST search against the nt database 2009/22/04, among isolates of the family of Francisellacae, uncultured and environmental Francisella-like bacteria.

e

B.21 is identical to Ft-SNP1 and B.22 is identical to Ft-SNP2 in Svensson et al 2009 (submitted manuscript).

Table 3. INDEL markers, genes affected by the INDELs, and primers.

INDEL SCHU S4 INDEL position SCHU S4 locus ID SCHU S4 gene Primer Primer sequences
Ftind43 1541234..1541239 FTTt30, FTTt31 Arg-tRNA, Gly-tRNA IN GTTTCACAAATTTGCGGGAA
(intergenic) OUT AATCCCTTTGGGTGTGCCAT
CP TGGAGCGGGAAACGAGGC
Ftind44 895956..896021 FTT0886, FTT0887 recN, FTT0887 IN TCGACAAGTAGTTACTCAGCCTA
(intergenic) OUT TAAATCTAGTTGGCTGAGTAAT
CP ACTGTTGTCATTCCCACGTA
Ftind18b 439349..439371 FTT0425 asd IN AGACCCTCTAAATCACGATCA
OUT AGGTTTCTGGATAGACGCTGCA
CP ACTAACAGTACAATTACTACCGAT
Ftind45 725227..725228 FTT0706 glk2 IN ACCTAATATGACCATAGATGGAT
(pseudogene) OUT TCACCAATAGCTTCCATAACA
CP ACTCAGTGAAGCTATGGAATATCT
Ftind46 1830698..1830699 FTT1739 kdpA IN AGTTCTGTACTGCAAGAGCGA
(pseudogene) OUT GTAGCTGTTTCATGCCTTGCT
CP AGCACTTAATACAGCAGTTAGT
Ftind47 271674..271683 FTT0255 IN AGTAATACGCAAAGATTTTCTACA
OUT TCTTAACTGTATGCTAGTCTATGA
CP TAATAGAGCGGCTCTTCGAAT
Ftind48 960987..961011 FTT0948 IN ATCCTACTAATATCAATTCCAGT
OUT CCTTCAGCTTGAGTATTTTGACGT
CP ACTGTTATATTCAGTTATTTGCT
Ftind38 b 95661..95674 FTT0092 appC IN ACCCAATAAGCTCACCATCA
(pseudogene) OUT ATCTTTCTCAGGTACAGACTTTA
CP AGTACTATTTGCTTATCCAAGTGAA
Ftind49 834341..834349 FTT0816 IN AAGATTAAGTGGCAATTTAC
OUT TTCAACCTGGACAACCACTA
CP AGGATCCCAGTTAGGTTTAGTA
Ftind33b 512045..512063 FTT0492 lysR IN TCTAAATTTAAGCAATGTTTCTAACT
OUT ATCATCGTATAAGAAATCAACTT
CP TCAACCTTACAGAATAAGAATGT
Ftind50 88484..88576 FTT0086 IN CATCACTGCCACCAAGCATAT
OUT TGGGCACCATAAATAGCTAGT
CP CGATGCCATGGTCAGATGATCA
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a

GenBank accession no. AJ749949.

b

Ftind18, Ftind33 and Ftind38 were previously used in [24].

Table 4. Fourteen isolates and six ulcer specimens from tularemia patients in Sweden 2008 characterized by the developed hierarchical real-time PCR array.

Category FSC no.a Sample IDb Location of the receiving hospital Table 5 genotype Figure 3 subclade
Isolates 792 32–92 Säffle 13 B4.Ftind49/18
844 32–280 Uddevalla 13 B4.Ftind49/18
780 32–51 Luleå 16 B3.23/[24], [25]
785 32–75 Falun 16 B3.23/[24], [25]
812 32–123 Sunderbyn 16 B3.23/[24], [25]
816 32–142 Boden 16 B3.23/[24], [25]
823 32–155 Lövånger 16 B3.23/[24], [25]
831 32–173 Skellefteå 16 B3.23/[24], [25]
794 24–95 Östersund 19 B1.20/21
777 32–38c Örebro 19 B1.21/22
787 32–79 Umeå 20d B1.21/22
778 32–47c Ljusdal 20d B1.21/22
783 32–69 Färila 21 B1.FSC200
817 32–145 Bollnäs 21 B1.FSC200
Ulcer specimens 32–151e Jönköpingf 16, 17 or 18g B3.23/[24], [25]
32–300e Gävle 16, 17 or 18g B3.23/[24], [25]
32–87e Umeå 16, 17 or 18g B3.23/[24], [25]
32–215 e Uddevalla 19h B1.20/21
32–38c Örebro 20h B1.21/22
32–47c Ljusdal 20h B1.21/22
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a

Strain ID in the Francisella Strain Collection, Swedish Defense Research Agency, Umeå, Sweden.

b

Sample ID at the Department of Clinical Bacteriology, Umeå University, Umeå, Sweden.

c

Isolate FSC777 and ulcer specimens 32–38 are from the same patient. Isolate FSC778 and ulcer specimens 32–47 are from the same patient.

d

The exact genotype could not be determined due to detection failure of marker B.22 (the difference in time of appearance between the two PCR products was less than one cycle).

e

F. tularensis cultures were negative.

f

The patient reported probable acquisition of tularemia when visiting the county of Jämtland, where the regional center is Östersund.

g

The genotype and subclade were assigned based on marker B.20, which exhibited an A for all three specimens, and on marker B.23, which exhibited a T. No other markers were screened due to scarcity of DNA.

h

The genotype and subclade were assigned based on: marker B.20, which exhibited a G for all three specimens; on marker B.21, which exhibited a G for specimens 32–215, and an A for specimens 32–38 and 32–47; and on marker B.22, which exhibited a G for specimens 32–38 and 32–47. No other markers were screened due to scarcity of DNA.

Figure 2. Example of plate design and interpretation of results for the genetic classification of F. tularensis strain LVS.

Figure 2

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A) The allelic state of each marker in the LVS strain is indicated in boldface. A colored well corresponds to a phylogenetically determining (canonical) marker for a specific genetic subclade. B) A phylogenetic tree is generated from hierarchical analysis of the typing results. Thick lines indicate the inferred evolutionary history of strain LVS. D = derived state, A = ancestral state.

DNA Preparation

F. tularensis isolates were re-cultured and a loopful of each isolate was suspended in phosphate buffered saline, heat-killed and DNA was prepared by phenol/chloroform extraction using Phase Lock Gel Light tubes (Eppendorf, Hamburg, Germany) or by a chaotropic salt method [27]. The latter was also used to prepare DNA from the clinical specimens. The concentration of DNA in each sample was determined using a BioPhotometer (Eppendorf, Hamburg, Germany) or NanoDrop spectrophotometer (Thermo Scientific, Wilmington, DE, USA), then adjusted to 2.5 ng/µl.

Genetic Markers and Primers

Phylogenetically informative SNPs and INDELs were identified by BLAST searches of available Francisella genomes and DNA sequences at the National Centre for Biotechnology Information (NCBI). In addition, two INDELs and 12 SNPsC previously shown to discriminate between isolates of Francisella were selected and tested for specificity [2], [24], [28][30].

For each SNP marker, two forward allele-specific primers with different 3′ bases, each matching one of the SNP allele states, and a reverse common primer, were designed using Primer3 [31] (Table 2). The primers were designed according to a SNP discrimination assay described by Germer and Higuchi [32], [33], in which GC-rich tails of different lengths are added to each of the two allele-specific primers: a 14 bp (GCGGGCAGGGCGGC) tail was attached to the primer with G or C at the 3′-end, and a six bp (GCGGGC) tail was attached to the primer with A or T at the 3′-end. The GC-tails were in the original publication added primary to obtain a difference in the melting temperature, but a larger difference in the time of appearance between the two PCR-products was also obtained. For each INDEL marker, one common primer (CP) and two forward primers were designed: one inside (IN) and one outside (OUT) the deletion (Table 3). The CP-OUT primer pair was used as a positive control.

All primers were obtained (from Eurofins MWG, Ebersberg, Germany) and matched regions with an identical nucleic acid sequence in compared genomes and DNA sequences of the genus Francisella to minimize amplification failure of screened isolates.

Real-time PCR

In the final assay, real-time PCR amplifications of 34 genetic markers were performed using an iCycler (BioRad) with 5 ng DNA, or a Mastercycler instrument (Eppendorf) with 2 ng DNA, in both cases in 25 µl reaction mixtures in 68 wells of a 96-well plate (one primer pair per well was used). The reaction mixture for SNP detection consisted of 5 pmol of each primer (MWG-Biotech), 3U of AmpliTaq DNA Polymerase Stoffel Fragment, 2 mM MgClB2B, 50 µM dNTP, 20x SYBR Green I, 4% dimethyl sulfoxide (DMSO), and 2% glycerol. Two master mixes were prepared in which each of the allele-specific primers were added. The amplification conditions were: 50°C for 2 min, 95°C for 10 min, followed by 40 cycles at 95°C for 15 sec and 60°C for 1 min. The SNP in each sample was determined by inspecting the amplification curves. Amplification appeared earlier in reaction mixtures containing the forward primers with a matching 3′-base. A positive result was assigned when there was a one cycle or more difference between the time of appearance of PCR-products, and the number of cycles did not exceed 35. For INDEL analysis, Power SYBR Green PCR Mastermix was used with the same cycling conditions as for SNPs. The presence of a deletion was detected by failure of the reaction mixture with one primer in the deleted sequence to yield a detectable amplification product, while the control reaction with primer pairs surrounding the deletion succeeded. For cases where one primer overlapped a small deletion a minimum detection threshold of a five-cycle difference in time of appearance between the control and test reactions was set.

Quality Controls

The final 68-well assay included one PCR reaction per well (no multiplexing). To evaluate the typing accuracy of the assay, a test blinded to the investigator was performed on a subset of six isolates previously used in the development stage and representing the MLVA genetic groups F. novicida (N), F. t. mediasiatica (M), A1, B2, B3, and B5 of Francisella. Genetic group designations are found in Figure 1 and Table 1. The detection limit of the final assay was tested with serial logarithmic dilutions of F. tularensis subsp. holarctica Live Vaccine Strain (LVS) DNA, starting at one ng. The detection limit was set at the lowest amount of DNA with which PCR amplification of all 34 markers occurred. The reproducibility of the assay was assessed using one ng DNA of LVS tested in three replicate runs.

MLVA

To assign MLVA clusters for isolates that had not been previously characterized in [26], MLVA was performed using a CEQ 8800 instrument (Beckman Coulters, Fullerton, CA), as previously described [26].

Accession Numbers

Completed genomic sequences (with GenBank accession numbers in parenthesis) used in this work were: U112 (CP000439), ATCC25017 (CP000937), WY96-3418 (CP000608), FSC147 (CP000915), FTNF002-00/FTA (CP000803), OSU18 (CP000437), LVS (AM233362) and SCHUS4 (AJ749949).

Draft genome sequences (with GenBank accession numbers in parenthesis) used in this work were: ATCC25015 (ABYY00000000), FSC200 (AASP00000000), FTE (ABSS00000000) and FTG (ABXZ00000000).

Preliminary sequence data were obtained from the MIT Broad Institute website at www.broad.mit.edu for the following Francisella strains: GA99-3549, GA99-3548, FSC033, FSC022, and FSC257/RC503.

The following Francisella genomes from Baylor College of Medicine Human Genome Sequencing Center website at www.hgsc.bcm.tmc.edu were not available at the time of the study, but are mentioned here: ATCC6223, KO97-1026, MI00-1730 and OR96-0246/BSA; The OR96-0463 genome was sequenced by the Joint Genome Institute and Lawrence Livermore National Laboratory, and is available from http://genome.ornl.gov.

The following previously published genes found to discriminate between isolates of Francisella, were used: dnaA (AM261088 to AM261101) [29]; tpiA (AM261102 to AM261115 [29], AY794514 to AY794528 and AY794497 [2]); lpnA/tul4/17kD (AM261150 to AM261161 and AM261164) [29]; putA (AM261165 to AM261178) [29]; aroA (AY794435 to AY794449 and AY794495) [2]; atpA (AY794498 to AY794513) [2]; vacJ (DQ451123 to DQ451126) [28]; fabH (DQ863407 to DQ863420) [30]; FTT0086 (DQ863472 to DQ863483) [30]; asd/FTT0425 (Ftind18) and lysR/FTT0492 (Ftind33) [24]; appC/FTT0092 (Ftind38) [24], and aceF, RD17 (AY794422) [2].

Results

Selection of Genetic Markers

We identified 49 SNPs and 15 INDELs with potential canonical properties by analyzing various available DNA sequences. Strain polymorphism was verified using a pair of isolates showing the two possible allelic states. Twenty-four SNPs and three INDELs were not used in further analyses because of amplification failure, or (in SNP analysis) because there was a less than one cycle difference in the time of appearance of different PCR products. In evaluation of the remaining SNPs and INDELs in a panel of 62 Francisella isolates of diverse genetic and geographical origins, two SNPs and one INDEL were found to be incongruent with the phylogenetic structure of F. tularensis determined by Vogler et al [1], and were therefore also discarded. The final set of markers comprised 23 SNPs and 11 INDELs, which were arrayed in a hierarchical assay structure in 68 wells of a 96-well plate (one primer pair per well was used) (Figure 2).

Detection Level and Typing Resolution

The limit of detection of our assay was found to be 100 pg DNA. Three replicate runs using F. tularensis strain LVS showed identical results. An indefinite typing result occurred on average in 0.3 to one marker per plate. However, unambiguous strain classification was still possible using the information obtained from the other markers. The assay successfully detected and discriminated among the three species of Francisella, the five major genetic clades of F. tularensis, and the subclades of F. tularensis subsp. holarctica. A comparison with a set of recently published canonical SNPs [1] showed perfect correlation with the results obtained in our assay (as shown in the Francisella phylogeny depicted in Figure 3, which indicates names of markers and subclades from both research groups). Our markers B.20 to B.23 and B.25, B.16 and A.4 added typing resolution to the genetic branches B.Br.013/014, B.Br.002/003, and A.I.001/002 previously defined by Vogler et al [1] (Figure 3, Table 5). In addition, the use of INDELs Ftind44, Ftind48 and Ftind49 provided resolution at phylogenetic nodes where no corresponding SNP was identified by Vogler et al. (Figure 3). Our markers T.1 and Ftind44 also conveniently discriminated all F. tularensis strains from F. novicida, F. philomiragia and F. noatunensis isolates (Figure 3, Table 5).

Figure 3. Schematic SNP and INDEL phylogeny, indicating genetic markers and Francisella subclades.

Figure 3

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Markers presented in this study are indicated in black and, for comparison, SNP markers developed in a recent study by Vogler et al 2009 [1] are indicated in gray. The branch names of Vogler et al. have been abbreviated to simplify the nomenclature. Stars indicate terminal subclades defined by Francisella genomes and circles represent collapsed branch points along the genetic lineages that contain isolates of a particular genotype (a subclade). The subclades are named for the flanking SNPs and INDELs. The branch lengths do not represent true phylogenetic distances. The position of B.15/Ftind47 (marked by the asterisk in the figure) could not be definitively determined; it could be either where shown, or be descendant from B.1/2.

Table 5. Francisella genotypes in this study.

Genotype F.1 Ftind 43 T/N.1 T.1 Ftind 44 N.1 N.2 N.3 Ftind 18a M.2 Ftind 45 A.2 Ftind 46 A.3 A.4 A.5 A.6 Ftind 47 B.15 Ftind 48 B.16 Ftind 38a B.17 Ftind 49 B.18 Ftind 33 B.19 B.20 B.21 B.22 B.23 Ftind 50 B.24 B.25
1. P.ATCC25017 T b DEL c G T NDd ND ND ND ND ND ND ND ND ND ND ND ND ND ND ND ND ND ND ND ND ND ND ND ND ND ND ND ND ND
2. N.U112 T INe A T DEL T G C IN A IN C IN T C T C IN A IN G IN G IN C IN C A G G G IN T C
3. N.FSC156 T IN A T DEL G A C IN A IN C IN T C T C IN A IN G IN G IN C IN C A G G G IN T C
4. N.FSC454 T IN A T ND G G T IN A ND C ND T C T C IN A IN ND ND G ND C ND ND A G G G ND T T
5. N.Ftind44/ [1], [2], [3] T IN A T DEL G G C IN A IN C IN T C T C IN A IN G IN G IN C IN C A G G G IN T C
6. M.FSC147 T IN A C IN G G C DEL G IN C IN T C T C IN A IN G IN G IN C IN C A G G G IN T C
7. A1.3/ [4], [5] T IN A C IN G G C IN A DEL A DEL C C T C IN A IN G IN G IN C IN C A G G G IN T C
8. A1.FSC033 T IN A C IN G G C IN A DEL A DEL C T T C IN A IN G IN G IN C IN C A G G G IN T C
9. A1.SCHUS4 T IN A C IN G G C IN A DEL A DEL C C C C IN A IN G IN G IN C IN C A G G G IN T C
10. A2.1/2 T IN A C IN G G C IN A DEL A IN T C T T IN A IN G IN G IN C IN C A G G G IN T C
11. B5.FSC022 T IN A C IN G G C IN A IN C IN T C T C DEL G IN T IN G IN C IN C A G G G IN T C
12. B2.OSU18 T IN A C IN G G C IN A IN C IN T C T C DEL G DEL G DEL T IN C IN C A G G G IN T C
13. B4.Ftind49/18 T IN A C IN G G C IN A IN C IN T C T C DEL G DEL G IN G DEL C IN C A G G G IN T C
14. B4.FTNF002-00 T IN A C IN G G C IN A IN C IN T C T C DEL G DEL G IN G DEL T IN C A G G G IN T C
15. B3.19/ [20], [23] T IN A C IN G G C IN A IN C IN T C T C DEL G DEL G IN G IN C DEL A A G G G IN T C
16. B3.23/ [24], [25] T IN A C IN G G C IN A IN C IN T C T C DEL G DEL G IN G IN C DEL A A G G T IN T C
17. B3.LVS T IN A C IN G G C IN A IN C IN T C T C DEL G DEL G IN G IN C DEL A A G G T DEL G C
18. B3.RC530 T IN A C IN G G C IN A IN C IN T C T C DEL G DEL G IN G IN C DEL A A G G T IN T T
19. B1.20/21 T IN A C IN G G C IN A IN C IN T C T C DEL G DEL G IN G IN C DEL A G G G G IN T C
20. B1.21/22 T IN A C IN G G C IN A IN C IN T C T C DEL G DEL G IN G IN C DEL A G A G G IN T C
21. B1.FSC200 T IN A C IN G G C IN A IN C IN T C T C DEL G DEL G IN G IN C DEL A G A A G IN T C
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a

Ftind18, Ftind33 and Ftind38 were previously used in [24].

b

A boldfaced marker corresponds to a phylogenetically determining (canonical) marker for a specific genetic subclade.

c

DEL = derived deletion.

d

ND = not detected.

e

IN = ancestral state.

Concordance to MLVA

The categorization of F. tularensis isolates based on 23 SNPs and 11 INDELs was consistent with the MLVA-groupings presented by Johansson et al in 2004 [26] (Table 1, Figure 1) with one exception. In our SNP/INDEL analysis, strain FSC186 was classified as belonging to B1, while it was classified as B3 by MLVA [26]. An analysis of MLVA data showed that the inconsistency was likely caused by homoplasy (characters shared by a set of strains but not present in their common ancestor) at the highly variable MLVA markers Ft-M3 and Ft-M6 (Table 6).

Table 6. Repeat numbers for isolates within subclades B1 and B3 of F. tularensis subsp. holarctica at four MLVA-loci.

Isolate ID Johansson et al. 2004 group In this study Ft-M3 Ft-M6 Ft-M20 Ft-M21
FSC162 B3 B3 17 4 3 2
FSC178 B3 B3 17 4 3 2
FSC115 B3 B3 13 4 3 3
FSC150 B3 B3 14 4 3 2
FSC250 B3 B3 21 4 3 2
FSC155 B3 B3 16 4 4 2
FSC257 B3 B3 17 4 3 4
FSC185 B1 B1 11 5 3 2
FSC186 B3 B1 12 4 3 2
FSC187 B1 B1 12 6 3 2
FDC010 B1 10 4 3 2
FDC014 B1 10 6 3 2
FSC121 B1 B1 9 6 3 2
FSC249 B1 B1 9 6 4 2
FSC124 B1 B1 17 6 3 2
FSC293 B1 17 5 3 2
FSC200 B1 B1 10 5 3 2
FSC245 B1 B1 10 5 3 2
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Categorization of Francisella Strains by the Real-time PCR array

Twenty-one genotypes were detected by the hierarchical array (Table 5). The typing accuracy of the final one-plate assay was assessed in a blind test, in which we correctly categorized six isolates previously tested individually for each marker. We further used the assay to categorize 14 isolates obtained from patients with tularemia in Sweden in 2008 (Figure 4, Table 4), and five isolates that were not included in the development of the assay (Table 1). We characterized six human tularemia ulcer specimens that were positive by the standard PCR for diagnosis of ulceroglandular tularemia [27] by amplifying the four selected markers B.20 to B.23 (Figure 4, Table 4), since we could not apply the new assay with all 34 markers due to scarcity of DNA.

Figure 4. Example of use.

Figure 4

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The subclade names for 14 isolates and six ulcer specimens from tularemia patients in Sweden 2008 (Table 4) genotyped by the developed hierarchical real-time PCR array, and the location of the receiving hospitals.

Discussion

In the present study we combined analysis of INDELs and SNPs in a real-time PCR array for robust, rapid and flexible hierarchical identification of F. novicida and F. philomiragia, and typing of human pathogenic members of the genus Francisella. In contrast to previously published real-time PCR assays, our assay was designed to cover the full currently known phylogenetic range of Francisella. The assay was also tailored to provide high typing resolution for F. tularensis subsp. holarctica isolates originating from Scandinavia, where our laboratory is located. Hierarchical typing based on cultivation and bacterial phenotypes has long been a fundamental element of the characterization of bacteria in diagnostic microbiology laboratories. Hierarchical typing based on genetic characters has only recently been applied, for classification of Bacillus anthracis and Francisella tularensis strains [1], [24], [34], [35]. This work demonstrates that a genetic hierarchical approach, based on carefully selected markers with canonical properties, can be used across an extensive phylogenetic typing range in the genus Francisella.

We have identified 34 genomic markers serving as phylogenetic guides, which can be added to or excluded from an assay depending on the testing objectives, i.e. according to the taxonomic and geographical resolution required. For example, in diagnostics, where the purpose is to verify the presence or absence of F. tularensis specimens, including canonical markers for species and subspecies levels in the assay may be sufficient. In contrast, in epidemiological investigations, where the aim is to track disease-transmission paths and/or sources, higher typing resolution might be desired, and thus markers that characterize the complete phylogeny, or alternatively only a selected subset with high resolution, should be included in the assay. In forensic investigations, complete characterization of isolates is needed to provide statistical and unambiguous evidence to infer relationships between isolates, and thus all canonical markers may be included in the assay. Geographical aspects could also be taken into consideration when selecting markers to be included. For example, in clinical laboratories located in Scandinavia it is not expected to find F. tularensis subsp. tularensis isolates in clinical samples tested, since this subspecies is confined to North America. Thus, only one canonical marker specific for the subspecies tularensis may be included and not all markers characterizing subclades of the subspecies. Instead, a very high discriminatory power for all the F. tularensis subsp. holarctica genetic groups that are known to be present in Sweden would be desired, i.e., groups B1 to B4 in Figure 1. Therefore, all canonical markers defining these subclades may be included. Finally, since we have included genomic markers for discriminating human pathogenic F. tularensis isolates from F. philomiragia and F. novicida which are of less clinical relevance and often present in environmental sources, the assay could potentially be used to monitor environmental Francisella.

A comparison of results obtained from SNP and INDEL markers shows good agreement. Both marker types apparently provide similar and stable phylogenetic information. Further, INDELs and SNPs are slowly mutating markers that provide very similar typing resolution. The lower typing resolution of INDELs in our assay was probably due to marker discovery bias: INDELs were easier to identify in the relatively few and genetically diverse available genome sequences than in the many available short sequence stretches from closely related isolates. In contrast, SNPs could be readily identified in both kinds of DNA sequences. We note that INDEL markers in the real-time PCR assay strengthen the SNP marker information at the main phylogenetic nodes (Figure 3). Deletion events should be evolutionarily unidirectional [2], while SNPs may revert. Thus, SNPs may (at least theoretically) display homoplastic patterns, while INDELs should not do so in a clonally structured bacterial population. We found that use of INDELs made the assay more robust and provided additional resolution at nodes where no corresponding SNP was identified.

The limit of detection of our assay was 100 pg of DNA, based on the lowest amount of DNA from which all 34 markers included in a single plate were amplified; a higher quantity than minimum amounts reported for other real-time PCR assays with fewer targets. This is a limitation that should be addressed in future work. Possibly, adaptation to a real-time PCR system including probes such as TaqMan SNP Genotyping Assay or the SNaPshot (Single Nucleotide Primer Extension) Assay (Applied Biosystems), could provide higher sensitivity. However, the reproducibility of the results was good and the failure of classification low, indicating that the assay was technically robust. The applicability of our assay to clinical isolates was also demonstrated, since we were able to characterize F. tularensis subsp. holarctica isolates obtained from patients in Sweden 2008, and bacterial DNA in ulcer specimens from tularemia patients.

We observed that the isolate FSC186 was classified as belonging to MLVA group B3 by Johansson et al 2004, but our data based on slowly mutating canonical SNPs and INDELs indicate that the isolate belongs to group B1. This finding illustrates the risk of homoplastic effects when using very rapidly mutating genetic markers in the MLVA for F. tularensis (Table 6). A detailed analysis showed that the MLVA markers Ft-M3 and Ft-M6 were the causes of the homoplasy effect. Accordingly, a genetic analysis of F. tularensis isolates including Ft-M3 and Ft-M6 should be complemented with analysis of more robust markers, such as SNPs and/or INDELs to ensure correct phylogenetic classification.

In summary, real-time PCR assays based on a hierarchical classification concept, as exemplified in this work, are flexible typing tools for phylogenetic and geographical resolution of Francisella. The level of discrimination can be easily adjusted by adding or removing genetic markers, a property which is not generally provided by conventional PCR methods or by previously developed real-time PCR assays. The presented hierarchical real-time PCR array could be used in public health laboratories as well as in research laboratories for a wide range of Francisella identification and typing purposes.

Acknowledgments

We thank Helen Edebro and Anders Sjöstedt for providing clinical samples and Ulla Eriksson for maintaining the Francisella Strain Collection (FSC) in Umeå, Sweden. We also thank Pär Larsson for helpful discussions and providing information about INDELs. We are indebted also to numerous colleagues for kindly providing strains to the FSC.

Footnotes

Competing Interests: The authors have declared that no competing interests exist.

Funding: This study was supported by the Swedish Ministry of Foreign Affairs (FOI project No. A4942 and A4952) www.ud.se and the Medical Faculty, Umeå University, Umeå, www.umu.se/medfak. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript. This work was part of the European biodefence laboratory network (EDA B-0060-ESM4-GC) coordination work on dangerous pathogens.

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