Typing African relapsing fever spirochetes.Relapsing fever relapsing fever Infectious disease with recurring fever, caused by several spirochetes of the genus Borrelia, transmitted by lice, ticks, and bedbugs. Onset is sudden, with high fever, which breaks within a week with profuse sweating. Symptoms return about a week later. Borrelia Borrelia A genus of spirochetes that have a unique genome composed of a linear chromosome and numerous linear and circular plasmids. Borreliae are motile, helical organisms with 4–30 uneven, irregular coils, and are 5–25 micrometers long and 0. spp. challenge microbiologic typing because they possess segmented genomes that maintain essential genes on large linear plasmids. Antigenic variation Antigenic variation is the process by which an infectious organism alters its surface proteins in order to evade a host immune response. This change in antigenic profile may occur as the pathogen passes through a host population (also called "antigenic diversity") or may take place further complicates typing. Intergenic spacer (IGS IGS - Internet Go Server. , between 16S-23S genes) heterogeneity provides resolution among Lyrne disease-associated and some relapsing fever spirochetes. We used an IGS fragment for typing East African Adj. 1. East African - of or relating to or located in East Africa relapsing fever Borrelia spp. Borrelia recurrentis and their louse louse, common name for members of either of two distinct orders of wingless, parasitic, disease-carrying insects. Lice of both groups are small and flattened with short legs adapted for clinging to the host. vectors showed 2 sequence types, while 4 B. duttonii and their tick vectors had 4 types. IGS typing was unable to discriminate between the tick- and louseborne forms of disease. B. crocidurae, also present in Africa, was clearly resolved from the B. recurrentis/B. duttonii complex. IGS analysis of ticks showed relapsing fever Borrelia spp. and a unique clade clade Cladus, subtype Genetics A branch of biological taxa or species that share features inherited from a common ancestor; a single phylogenetic group or line. See Inheritance, Species. , distant from those associated with relapsing fever, possibly equivalent to a novel species in ticks from this region. Clinical significance of this spirochete spirochete Any of an order (Spirochaetales) of spiral-shaped bacteria. Some are serious pathogens for humans, causing such diseases as syphilis, yaws, and relapsing fever. Spirochetes are gram-negative (see gram stain) and motile. is undetermined. ********** Both tickborne and louseborne forms of relapsing fever, caused by borrelial spirochetes, are substantial causes of illness and death in regions of East Africa. In Tanzania and Ethiopia, for example, these infections are endemic, with much of the population living in close proximity with the disease vectors. Indeed, surveys of traditional Tanzanian "Tembe" dwellings have shown that up to 88% are infested in·fest tr.v. in·fest·ed, in·fest·ing, in·fests 1. To inhabit or overrun in numbers or quantities large enough to be harmful, threatening, or obnoxious: with ticks of the Ornithodoros moubata complex (1). These ticks are vectors for Borrelia duttonii, the cause of tickborne relapsing fever in East Africa. In disease-endemic regions, tickborne relapsing fever is one of the top 10 diseases associated with deaths in those <5 years of age. The louseborne form of the disease is caused by B. recurrentis and is transmitted by the human clothing louse, Pediculus humanus. In regions where louseborne relapsing fever is endemic, such as Ethiopia, this disease contributes substantially to human disease prevalence, particularly during the rainy season. Incidence data are largely lacking; the diagnosis typically relies on demonstration of spirochetes in blood films of samples taken from febrile febrile /feb·rile/ (feb´ril) pertaining to or characterized by fever. feb·rile adj. Of, relating to, or characterized by fever; feverish. patients. Clinical signs and symptoms overlap with those of other prevalent diseases such as malaria, which may lead to inaccurate diagnoses. Other Borrelia spp. have been associated with relapsing fever in Africa; for example, B. crocidurae is associated with this disease in West Africa West Africa A region of western Africa between the Sahara Desert and the Gulf of Guinea. It was largely controlled by colonial powers until the 20th century. West African adj. & n. (2). However, this spirochete has an established reservoir in rodent populations that also serve as hosts for the Ornithodoros erraticus ticks. Recent reports have also established additional spirochetes in tick vectors (3) and in human blood samples (4); however, their clinical relevance has yet to be defined. To determine the population structure within these spirochetes and to assess the role of newly described spirochetes, appropriate microbiologic tools must be used. Many widely used techniques for molecular typing have been applied to Borrelia with variable success (5,6). Of concem when these methods are used for characterizing these spirochetes is the organisms' ability to undergo multiphasic antigenic variation, which can be associated with large inter- or intraplasmidic recombinations/duplications (7,8). Indeed, this ability is a likely cause of the variability in genomic organization Organisms have a vast array of ways in which their respective genomes are organized. A comparison of the genomic organization of six major model organisms shows size expansion with the increase of complexity of the organism. of these spirochetes, which possess segmented genomes (9-11) composed of giant linear and circular plasmids. Although conventional approaches, such as sequencing of 16SRNA sRNA abbr. soluble RNA gene, have provided useful information on population structure among the Borrelia spp., this gene only provides low discriminatory resolution among African relapsing fever spirochetes (2,12). Others have used the flagellin flagellin /fla·gel·lin/ (flah-jel´in) a protein of bacterial flagella; it is composed of subunits in several-stranded helical arrangement. gene as a target for population structure (5,13); however, as with 16SRNA, these methods, although useful for interspecies comparisons, are of limited value for discrimination of African relapsing fever spirochetes and for intraspecies in·tra·spe·cif·ic also in·tra·spe·cies adj. Arising or occurring within a species: intraspecific competition. Adj. 1. analysis. A partial intergenic spacer region (IGS; rrs [16S rRNA]-ileT [tRNA]) has recently been used for typing Lyme-associated Borrelia spp., together with other genetic loci loci [L.] plural of locus. loci Plural of locus, see there (14). Additionally, IGS fragment typing proved valuable for differentiating relapsing fever spirochetes (15). However, these researchers only applied this typing to US strains and to nonpathogenic relapsing fever spirochetes from Sweden. We applied this method to isolates, blood samples, ticks, and lice collected in Tanzania and Ethiopia. Materials and Methods Blood Samples Blood samples from Tanzania were collected into glass capillary tubes after fingerprick of spirochetemic patients attending Mvumi Hospital, Dodoma, Tanzania. In Ethiopia, samples were collected from persons who were hospitalized with louseborne relapsing fever at the Black Lion Black Lion was an anti-fascist resistance movement in Ethiopia during the Italian occupation. The movement was founded in western Ethiopia, and included fighters such as the Shoan Ras Abebe Aregay. Dr. Hospital in Addis Ababa Addis Ababa (ăd`ĭs ăb`əbə) [Amharic,=new flower], city (1994 pop. 2,112,737), capital of Ethiopia. It is situated at c.8,000 ft (2,440 m) on a well-watered plateau surrounded by hills and mountains. . Total DNA DNA: see nucleic acid. DNA or deoxyribonucleic acid One of two types of nucleic acid (the other is RNA); a complex organic compound found in all living cells and many viruses. It is the chemical substance of genes. was extracted from these samples by using a QIAamp DNA blood mini kit (Qiagen, Crawley, UK). Isolates Borrelial isolates were obtained from blood samples drawn from patients with clinical cases of relapsing fever as previously described (16-18). Borrelia spp. were grown in Barbour-Stoenner-Kelly medium (BSKII) (19) incubated at 33[degrees]C to stationary phase The term stationary phase may refer to
A mechanical method of separating immiscible liquids or solids from liquids by the application of centrifugal force. This force can be very great, and separations which proceed slowly by gravity can be speeded up enormously in centrifugal , washed with 0.1 mmol phosphate-buffered saline, and DNA was prepared by using phenolchloroform extraction. A total of 6 cultivated B. duttonii isolates (Ly, La, Lw, Ma, Ku, and Wi) and 18 B. recurrentis isolates (A1-A18) were investigated. Cultures were diluted in BSKII medium, and the one with the lowest growth was added to media from which DNA was extracted. Because these spirochetes are fastidious fas·tid·i·ous adj. 1. Possessing or displaying careful, meticulous attention to detail. 2. Difficult to please; exacting. 3. Having complex nutritional requirements. Used of microorganisms. , recovery from a single cell cannot be guaranteed. For comparison, other Borrelia spp. analyzed included Nearctic relapsing fever strains B. hermsii (HS1), B. turicatae, and B. parkeri; West African West Africa A region of western Africa between the Sahara Desert and the Gulf of Guinea. It was largely controlled by colonial powers until the 20th century. West African adj. & n. B. crocidurae; and Lyme borreliosis Lyme borreliosis Another name for Lyme disease. Mentioned in: Lyme Disease strain B. burgdorferi sensu stricto (B31). Lice Lice were collected from the clothing of patients with louseborne relapsing fever, kept in 70% ethanol, and transported to the United Kingdom (import license not required). Total DNA was extracted by using a DNeasy Tissue kit (Qiagen) from pools of 4 to 6 lice. Ticks Ticks were collected from traditional dwellings in 4 villages, Mvumi Makulu (MK), Iringa Mvumi (IM), Ikombolinga (IK), and Mkang'wa (MA), in the Dodoma Rural Dodoma Rural is one of the 5 districts of the Dodoma Region of Tanzania. It is bordered to the North by the Kondoa District, to the East by the Kongwa District, to the South by the Dodoma Urban District and to the West by the Singida Region. District, central Tanzania. Scoops of earth were collected and passed through a sieve, and ticks were collected into containers containing 70% ethanol. Dead ticks were imported under license (AHZ/2074A/2001/13) and heat inactivated inactivated rendered inactive; the activity is destroyed. inactivated viruses treated so that they are no longer able to produce evidence of growth or damaging effect on tissue. (>80[degrees]C for 30 min) before DNA extraction DNA extraction is a routine procedure to collect DNA for subsequent molecular or forensic analysis. Outline of a DNA extraction There are three basic steps in a DNA extraction, the details of which may vary depending on the type of sample and any substances that may . After manual homogenization homogenization (həmŏj'ənəzā`shən), process in which a mixture is made uniform throughout. Generally this procedure involves reducing the size of the particles of one component of the mixture and dispersing them evenly of 1 to 6 ticks with a sterile pestle pestle /pes·tle/ (pes´'l) an implement for pounding drugs in a mortar. pes·tle n. A club-shaped, hand-held tool for grinding or mashing substances in a mortar. , samples were digested overnight in SNET n. 1. The fat of a deer. v. t. 1. The clear of mucus; to blow. lysis buffer A lysis buffer is used for the purpose of lysing cells for use in experiments that analyze the compounds of the cells (e.g. western blot). There are many different kind of lysis buffers that one can apply, depending on what analysis the cell lysate will be used for. (20 mmol/L Tris-HCl pH 8.0, 5 mmol/L EDTA EDTA: see chelating agents. , 400 mmol/L NaCl, 1% sodium dodecyl sulfate Sodium dodecyl sulfate (or sulphate) (SDS or NaDS) (C12H25NaO4S),is an anionic surfactant that is used in household products such as toothpastes, shampoos, shaving foams and bubble baths for its thickening effect and its ability to , 55[degrees]C), supplemented with proteinase proteinase /pro·tein·ase/ (pro´ten-as?) endopeptidase. pro·tein·ase n. A protease that begins the hydrolytic breakdown of proteins usually by splitting them into polypeptide chains. K (400 [micro]g/mL final concentration). Debris was pelleted, lysate ly·sate n. The cellular debris and fluid produced by lysis. was transferred to a fresh tube, and total DNA extracted by using standard phenolchloroform extraction or the automated MagnaPure DNA extraction robot with the LC DNA isolation kit II for tissues (Roche, Lewes, UK). DNA extracted from 2 purification rounds was pooled, concentrated, and resuspended in sterile distilled water Noun 1. distilled water - water that has been purified by distillation H2O, water - binary compound that occurs at room temperature as a clear colorless odorless tasteless liquid; freezes into ice below 0 degrees centigrade and boils above 100 degrees centigrade; . PCR PCR polymerase chain reaction. PCR abbr. polymerase chain reaction Polymerase chain reaction (PCR) A Borrelia-specific nested polymerase chain reaction Nested polymerase chain reaction is a modification of polymerase chain reaction intended to reduce the contaminations in products due to the amplification of unexpected primer binding sites. (PCR) designed to amplify the 16S-23S IGS region was used (14). The outer primers were anchored in the 3' end of the rrs gene and the ileT genes, respectively (5'-GTATGTTTAGTGAGGGGGGTG-3' and 5'-GGATCATAGCTCAGGTGGTTAG-3' for forward and reverse, respectively, while the inner nested primers were 5'-AGGGGGGTGAAGTCGTAACAAG-3' and 5'-GTCTGATAAACCTGAGGTCGGA-3', again for forward and reverse). Amplicons were resolved with 1% agarose agarose more highly purified form of agar with similar uses to agar and widely used in the separation of nucleic acid fragments. gels, bands were excised, and DNA was purified by using a Wizard SV gel and PCR clean-up system (Promega, Southhampton, UK). DNA Sequencing DNA sequencing The determination of the sequence of nucleotides in a sample of DNA. Purified DNA was sequenced directly or cloned into pGEMT-easy (Promega) and sequenced. Sequencing reactions were performed according to according to prep. 1. As stated or indicated by; on the authority of: according to historians. 2. In keeping with: according to instructions. 3. manufacturer's recommendations by using BigDye terminator v3.1 cycle sequencing kit (Applied Biosystems Applied Biosystems, Inc. (formerly NASDAQ: ABIO) is the original name of a pioneer biotechnology company founded in 1981 in Foster City, California, among the Silicon Valley cities of the southern San Francisco Bay Area. , Warrington, UK) and analyzed on an Applied Biosystems Genetic Analyzer (Applied Biosystems, Foster City, CA, USA). Data Analysis Nucleotide sequences were analyzed by using Chromas (version 1.45) and DNA Star software (Lasergene 6). Multiple alignments were performed by using ClustalW. Results produced by IGS fragment typing were compared with those obtained using the rrs gene with sequences held in GenBank. Phylogenetic Trees The phylogenetic phy·lo·ge·net·ic adj. 1. Of or relating to phylogeny or phylogenetics. 2. Relating to or based on evolutionary development or history. relationships of sequence data were compared by using Mega software (version 3) and neighbor-joining methods for compilation of the tree. A bootstrap See boot. (operating system, compiler) bootstrap - To load and initialise the operating system on a computer. Normally abbreviated to "boot". From the curious expression "to pull oneself up by one's bootstraps", one of the legendary feats of Baron von Munchhausen. value of 250 was used to determine confidence in tree-drawing parameters. Results Clinical Isolates Cultivable isolates of B. duttonii were identical over the 587-bp portion of the IGS sequenced and, consequently, the Ly strain was selected to represent these isolates. This isolate has been used by others as representative for B. duttoni (2,20). When applied to B. recurrentis, IGS fragment sequencing was able to group these isolates into 2 types that differed by 2 nucleotides (nt). Of the 18 isolates A1-A10, A17, and A18 comprised type I, while isolates A11-A16 gave a second type II profile. When the 2 B. recurrentis types were compared with B. duttonii types I-IV, differences appeared negligible (Table 1, Figure 1). The IGS fragment sequences of B. duttonii type II and B. recurrentis type I were identical. [FIGURE 1 OMITTED] A comparison of rrs gene sequences confirmed the difference between the 2 groups of B. recurrentis, in this case, with only a single nucleotide difference (Table 2, Figure 2). Whereas the IGS fragment analysis produced different profiles within species, analysis of the rrs gene sequences, with the exception of the B. recurrentis types, produced single clusters for each relapsing fever species (Table 2, Figure 2). Differences between species were small, with a 4-nt difference between B. recurrentis and B. duttonii; a 6-nt difference between B. recurrentis and B. crocidurae; and only 2 nt differentiating B. duttonii and B. crocidurae (Table 2). [FIGURE 2 OMITTED] Lice Clothing lice collected from 21 febrile, spirochetemic louseborne relapsing fever patients from Ethiopia produced amplicons from 20 samples. Of these, 18 were identified as the B. recurrentis type I, and 2 represented type II. Thus, sequence types detected among clinical isolates mirrored those found in the lice. Ticks Tick infestation infestation /in·fes·ta·tion/ (-fes-ta´shun) parasitic attack or subsistence on the skin and/or its appendages, as by insects, mites, or ticks; sometimes used to denote parasitic invasion of the organs and tissues, as by helminths. rates in traditional Tembe huts approached that previously described (1), with ticks found in an average of 61% of the 150 huts tested (range 49%-69%). Ten of 14 Makulu village huts contained ticks positive by partial IGS PCR (71.4%), and all were identical to B. duttonii Ly strain. Ten of 11 Makang'wa village huts (91%) were similarly positive for IGS DNA. Greater heterogeneity was observed with 3 IGS types detected. The first, type I, was identical to the Ly strain and was found in 8 of the tick extracts (80%). Ticks from hut MA/15 gave a different sequence, diverging by 7 nt from the Ly strain (type II). Notably, the IGS fragment produced from these ticks was identical to that seen in B. recurrentis type I. A further profile, type III Type III may stand for:
Nine of 12 Iringa Mvumi village tick extracts (75%) yielded borrelial IGS fragment amplicons; 1 (IM/36) produced 2 different-sized bands (sequence types I and an IGS sequence showing greatest homology homology (hōmŏl`əjē), in biology, the correspondence between structures of different species that is attributable to their evolutionary descent from a common ancestor. with B. crocidurae). Sequence analysis showed 4 IGS types. B. duttonii type I (Ly strain) was again predominant, identified in 7 (70%) of the 10 sequences, with the smaller (568 bp) detected as a mixed infection in 1 tick extract (IM/36, 10%). The sequence for this smaller band fell outside the B. duttonii/B, recurrentis cluster and showed greatest homology with an isolate of B. crocidurae. However, this band was surprisingly distant from the IGS B. crocidurae sequence held in GenBank AF884004. Because of its highly divergent nature, this latter sequence was excluded from further analysis. Two additional single tick extracts (each representing 10%), yielded larger amplicons of 757 bp and 759 bp, respectively (IM/16 and IM/19). Substantial differences between these sequences and those of B. duttonii were evident, and these sequences were assigned Borrelia spp. types 1 and 2, respectively (Table 3). Ticks from 9 (75%) of 12 huts from Ikombolinga amplified, yielding 2 distinct IGS fragment types. Ly strain type I was found in most (8 [89%]/9), and a larger amplicon of 762 bp was sequenced from IK/23, which shared little sequence homology with the Ly strain. As a result of this divergence with known B. duttonii, this amplicon was assigned Borrelia spp. type 3 (Table 3). Clinical Tickborne Relapsing Fever Patients DNA was extracted from 6 partially purified blood cultures from tickborne relapsing fever patients and amplified by using IGS fragment primers. Of these, 5 (83%) were identical to those of the Ly strain (type I), and 1 was 568 bp, identical to strains found in ticks (IM/36) and showing greatest homology with B. crocidurae. An additional 6 blood samples from spirochetemic tickborne relapsing fever patients yielded amplicons, 5 of which were identical to the Ly strain, while the remainder, B. duttonii type IV (patient WM) showed 10-12 nt differences and 1 nt deletion when compared with other sequence types (Table 1). In summary, B. duttonii type I was predominant, found in isolates from patient isolates and blood from patients with clinical cases of tickborne relapsing fever and O. moubata ticks. In fact, this was the only type represented among cultivable isolates. Three variants, types II, III, and IV, were occasionally found in both clinical patients (type IV) and ticks (types II, III). A further, smaller, amplicon showed greatest homology with B. crocidurae and fell outside the cluster of B. recurrentis and B. duttonii sequences and was found in both a tick and a patient. Although these variants are an apparent minority, they have been found in conjunction with type I in ticks (B. crocidurae-like) and as the only Borrelia type found in patients with clinical cases (1 patient with B. duttonii type IV and 1 with a B. crocidurae-like spirochete). Whether these strains can be cultivated remains unresolved. Novel partial IGS sequence types were found in ticks from huts IM/16 and IM/19, which clustered together with those found in IK/23 and were assigned Borrelia spp. types 1, 2, and 3, respectively. Each of these Borrelia types showed slight variability in their IGS fragment sequence (Table 3); however, they formed a distinct cluster away from other borrelial species. Insufficient material remained to undertake further PCR assays with other targets such as the flaB or rrs genes. Greatest homology was with Nearctic species B. hermsii and B. turicatae. All differ substantially from the Ly B. duttonii strain, except over the primer regions, and consequently cannot be considered as belonging to this species. Accession Numbers B. recurrentis types I and II were assigned GenBank accession numbers DQ000277 and DQ000278, respectively. B. duttonii groups I-IV were assigned DQ000279-DQ000282, respectively. The B. crocidurae--like sequence was given DQ000283. Borrelia spp. IGS sequences types 1-3 were assigned DQ000284-DQ000286, respectively, while the B. crocidurae IGS sequence determined in this study was given DQ000287. Discussion Application of gene sequence-based approaches has provided useful information regarding population structure and possible phylogenetic associations among Borreliae spp. (21). Of particular value has been sequence-based comparisons of the rrs-rrlA IGS region, which (because noncoding DNA Noun 1. noncoding DNA - sequence of a eukaryotic gene's DNA that is not translated into a protein intron deoxyribonucleic acid, desoxyribonucleic acid, DNA - (biochemistry) a long linear polymer found in the nucleus of a cell and formed from nucleotides and shows greater variability than would be expected for coding sequences) is sufficiently conserved to permit phylogenetic conclusions (22,23). Our results demonstrated that the differences between B. duttonii and B. recurrentis were as great as those within species, raising the question of whether these spirochetes are indeed a different species. This difference is exemplified by the identical IGS fragment sequence shared between B. recurrentis and B. duttonii type II. Whether these data suggest a common ancestral lineage for these relapsing fever spirochetes can only be fully resolved through sequence analysis of the whole genome. An analogous situation was found when IGS typing was used to characterize other microbes such as Fusobacterium spp.; in that situation, good resolution of strains was provided; however, with IGS typing, 2 species appeared to be identical (23). Analysis of rrs phylogeny, in contrast, showed distinct clusters for B. duttonii, B. recurrentis, and B. crocidurae; however, a small number of nucleotides differentiated these clusters. Some Old World relapsing fever spirochetes show a high degree of similarity, both in using 16S RNA RNA: see nucleic acid. RNA in full ribonucleic acid One of the two main types of nucleic acid (the other being DNA), which functions in cellular protein synthesis in all living cells and replaces DNA as the carrier of genetic gene sequences (12) and in flagellin (20,24). Using the 16S RNA gene, we found that only 4 bases differed over the rrs gene between B. duttonii and B. recurrentis; this finding was also reported previously (12). Ras et al. concluded that this small difference did not support these being single species but instead postulated that B. recurrentis could be a clone derived from the B. crocidurae--B, hispanica--B. duttonii cluster (12). Although our results would support the concept that B. recurrentis, B. duttonii, and B. crocidurae are clonal variants, IGS fragment typing suggested a substantially greater distance between the B. duttonii/B. recurrentis complex and B. crocidurae. More B. crocidurae isolates were not available to further verify phylogenetic inference by using partial IGS sequencing. A further bias within this comparison is that the rrs phylogeny presented here used cultivable isolates. Since only B. duttonii type I was represented among these isolates, the rrs gene phylogeny may not truly represent the diversity found among these spirochetes. Despite these apparently conflicting datasets, resolution of the IGS fragment typing was clearly greater, enabling a more detailed analysis of clinical or host associations. Failure to discriminate between the B. duttonii/B, recurrentis complex, however, would require the use of alternative targets, if they are indeed different species. This apparent paradox may reflect that these are clones derived from a common ancestral origin (12). This hypothesis is strengthened by the finding of a partial IGS sequence (B. duttonii type II) in O. moubata complex ticks from a disease-endemic area for tickborne relapsing fever, which showed total homology with the predominant sequence type identified among B. recurrentis. Further investigation of ticks from this area should be conducted. To overcome problems associated with use of single gene targets for addressing population structure among microorganisms, multilocus sequence typing Multilocus sequence typing (MLST) is a technique in molecular biology for the typing of multiple loci. The procedure characterizes isolates of bacterial species using the DNA sequences of internal fragments of multiple (usually seven) housekeeping genes. (MLST MLST Multi Locus Sequence Typing MLST Medical Logistics Support Team MLST Mini Losi Super Truck (1/18th scale radio control vehicle) ), which is less likely to show linkage disequilibrium linkage disequilibrium n. The nonrandom association between two or more alleles such that certain combinations of alleles are more likely to occur together on a chromosome than other combinations of alleles. than many surface markers, is commonly used to investigate more conserved housekeeping genes. However, a few housekeeping genes possessed by Borrelia spp. are located on plasmids, which raises a question about the validity of this approach (25). Others have used surface exposed proteins as targets for MLST (14). More recently, an MLST study focused on 18 different, highly polymorphic polymorphic - polymorphism loci to show the role of recombination recombination, process of "shuffling" of genes by which new combinations can be generated. In recombination through sexual reproduction, the offspring's complete set of genes differs from that of either parent, being rather a combination of genes from both parents. in creation of diversity among Lyme disease--associated spirochetes and their correlation with outer surface protein C alleles (25). Despite extensive application of these methods to Lyme Disease--associated Borrelia spp., the relapsing fever spirochetes have been largely neglected. However, recently a MLST-based approach, in which rrs, flaB, gyrB, and glpQ chromosomal genes were used to examine the phylogenetic relationship among B. parkeri and B. turicatae, confirmed their species status and demonstrated that the Florida canine Borrelia isolate clustered among B. turicatae (26). Investigations have been limited by the lack of available strains for assessing and identifying suitable markers. Cultivating these fastidious microbes is challenging, with some, until recently, considered noncultivable (16-18). Furthermore, the complexity of coexistent mechanisms for antigenic variation with associated potential for major genomic reorganization presents a problem for many microbiologic typing approaches. Isolates that are homogeneous by gene sequence-based approaches may present vastly different pulsed-field electrophoretic profiles (16,17,26), possibly through extensive genetic duplication associated with antigenic variation of major outer membrane The outer membrane refers to the outside membranes of Gram-negative bacteria, the chloroplast, or the mitochondria. It is used to maintain the shape of the organelle contained within its structure, and it acts as a barrier against certain dangers. proteins, whose genes are carried on large linear plasmids (7,11). Although using the more variable IGS region for molecular typing of relapsing fever spirochetes has been reported as valuable (15), only a limited selection of relapsing fever species, B. miyamotoi and B. lonestari, have been assessed. When we used this approach to characterize clinical isolates from patients with tickborne relapsing fever and louseborne relapsing fever, blood samples from patients, and ticks and lice collected in East Africa, we demonstrated that this method could successfully be applied to all sample types. We also demonstrated 3 distinct groups: a) 1 comprising cultivable strains of B. duttonii/B, recurrentis and amplicons from tick, lice, and human blood samples; b) 1 from both a patient and a tick showing greatest homology with B. crocidurae; and c) a further group containing unique amplicons from ticks collected in Tanzania. This last group was distinct in its IGS sequence and is likely compatible with the novel Borrelia species from this region (3,4,20). Three sequence types were identified that clustered within this novel IGS sequence clade, separate from the B. duttonii-B, recurrentis complex. This clade fell among those containing B. hermsii and B. turicatae (Figure 1), thus supporting earlier reports of a new Borrelia spp. characterized by using flagellin and 16S RNA sequences (Borrelia species ABl13315 [3], Figure 2), and reported to show greater resemblance to Nearctic isolates such as B. hermsii and B. turicatae, rather than Old World tickborne relapsing fever and louseborne relapsing fever isolates (3,4,20). Insufficient material remained to allow repeat analysis for either flaB or rrs genes to confirm that Borrelia species types 1-3 were indeed the same spirochete described above. These Borreliae spp. were not detected in any relapsing fever patient samples; consequently, their clinical significance has yet to be established. Of further interest was the identification of a B. crocidurae--like sequence in a patient and O. moubata tick. B. crocidurae is not believed to be present in East Africa but is endemic to the West African coast. Although the patient may have traveled from the west coast, finding this sequence type in a tick that was co-infected with the local endemic B. duttonii suggests that this spirochete may coexist in this area and may have extended vector compatibility. These findings were facilitated by methods able to give substantial resolution between strains, such as partial IGS typing, and would not have been possible by using clinical criteria or customary diagnostic approaches. Traditionally, relapsing fever nomenclature was assigned according to the spirochete's arthropod arthropod Any member of the largest phylum, Arthropoda, in the animal kingdom. Arthropoda consists of more than one million known invertebrate species in four subphyla: Uniramia (five classes, including insects), Chelicerata (three classes, including arachnids and horseshoe vector and the host species susceptibility. Clinical differences have also been documented: the louseborne form of the disease has been considered the most severe (27,28), although more frequent relapses are associated with the tickborne form. Such differences have lately been questioned because more recent studies of louseborne relapsing fever suggest less severe outcomes (29). B. duttonii has been correlated with higher perinatal death rates (30-32), while B. recurrentis is associated with a higher incidence of epistaxis epistaxis /ep·i·stax·is/ (-stak´sis) nosebleed; hemorrhage from the nose, usually due to rupture of small vessels overlying the anterior part of the cartilaginous nasal septum. ep·i·stax·is n. (28). These differences suggest that the diseases are associated with different clinical etiologic agents; however, these differences may actually be associated with differences in transmission or even in host response. Alternatively, different clinical symptoms may be serotype serotype /se·ro·type/ (ser´o-tip) the type of a microorganism determined by its constituent antigens; a taxonomic subdivision based thereon. se·ro·type n. See serovar. v. associated. Indeed, serotype switching has been associated with different clinical symptoms in rodent models infected with the American relapsing fever spirochete, B. turicatae (33). The lack of animal models for East African isolates precludes similar studies among these spirochetes. However, different isolates of the same species (B. recurrentis, which express different variable membrane proteins, have been shown to induce tumor necrosis factor tumor necrosis factor n. Abbr. TNF A protein that is produced in the presence of an endotoxin, especially by monocytes and macrophages, is able to attack and destroy tumor cells, and exacerbates chronic inflammatory diseases. release to different degrees (34). Unlike many relapsing fever spirochetes, B. duttonii and B. recurrentis infections are believed to be diseases of humans with as yet unidentified animal reservoirs. This restricted host range may impose constraints on these species compared with their less host-specific relatives. Indeed, this could account for greater diversity among other tickborne Borrelia spp. than among B. duttonii and the louseborne B. recurrentis. In summary, 38 B. recurrentis sequences and 47 B. duttonii IGS fragments were studied, showing 2 sequence types differing by 2 nt in the former and 4 types differing in from 1 to 12 nt (and a further deletion in 1 type) in the latter. These observations suggest more recent evolution of B. recurrentis, if one assumes that both spirochetes acquired changes in their IGS region at the same rate. IGS fragment sequencing proved to be a valuable typing tool for these spirochetes, allowing discrimination between relapsing fever and other borrelial species carried by ticks and lice prevalent in the same geographic region. However, this method was unable to separate B. duttonii and B. recurrentis. This typing approach appeared sufficiently robust to work on multiple sample types, including isolated strains, patient blood samples, and ticks and lice, thus negating the requirement for cultivation. Acknowledgments We thank Alison Talbert for local organization in Tanzania and Stafford Sanya, Salomie Bitia, Asha Abdi, Ezekiel Enoch, and Vendelino Raymond for assistance with field collection of materials in Tanzania. We also thank David Warrell and colleagues for collaboration with collection of material from Ethiopia. Isolates of B. hermsii (HS1), B. turicatae, and B. parkeri were kindly provided by A. Livesley, while DNA from B. crocidurae was provided by S. Bergstrom. This study was funded by The Royal Society and Wellcome Trust The Wellcome Trust is a United Kingdom-based charity established in 1936 to administer the fortune of the American-born pharmaceutical magnate Sir Henry Wellcome. Its income was derived from what was originally called Burroughs Wellcome & Co, later renamed in the UK as the . Dr Scott's research has been supported by The Wellcome Trust. Ethical approval was granted by Hammersmith Hospitals NHS Trust and COSTECH COSTECH Commission on Science and Technology in Dar es Salaam Dar es Salaam Largest city (pop., 1995 est.: 1,747,000), capital, and major port of Tanzania. Founded in 1862 by the sultan of Zanzibar, it came under the German East Africa Co. in 1887. . References (1.) Talbert A, Nyange A, Molteni F. Spraying tick-infested houses with lambda-cyhalothrin reduces the incidence of tick-borne relapsing fever in children under five years old. Trans R Soc Trop Med Hyg. 1998;92:251-3. (2.) Brahim H. Identifying relapsing fever borrelia, Senegal. Emerg Infect Dis. 2005; 11:474-5. (3.) Mitani H, Talbert A, Fukunaga M, New World relapsing fever Borrelia found in Ornithodoros porcinus ticks in central Tanzania. Microbiol Immunol. 2004;48:501-5. (4.) Kisinza W, McCall P, Mitani H, Talbert A, Fukunaga M. A newly identified tick-borne Borrelia species and relapsing fever in Tanzania. Lancet. 2003;362:1283-4. (5.) Fukunaga M, Okada K, Nakao M, Konishi T, Sato Y. Phylogenetic analysis of Borrelia species based on flagellin gene sequences and its application for molecular typing of Lyme disease Lyme disease, a nonfatal bacterial infection that causes symptoms ranging from fever and headache to a painful swelling of the joints. The first American case of Lyme's characteristic rash was documented in 1970 and the disease was first identified in a cluster at borreliae. Int J Syst Bacteriol. 1996;46:898-905. (6.) Godfroid E, Min Hu C, Humair P-F P-F Power-Fusion (Flash website) , Bollen A, Gern L, PCR-reverse line blot typing method underscores the genomic heterogeneity of Borrelia valaisiana species and suggests its potential involvement in Lyme disease. J Clin Microbiol. 2003;41:3690-8. (7.) Penningon P, Cadavid D, Bunikis J, Norris S, Barbour A. Extensive interplasmidic duplications change the virulence phenotype of the relapsing fever agent Borrelia turicatae. Mol Microbiol. 1999;34:1120-32. (8.) Kitten T, Barbour AG, The relapsing fever agent Borrelia hermsii has multiple copies of its chromosome and linear plasmids. Genetics. 1992;132:311-24. (9.) Ras NM, Postic D, Ave P, Huerre M, Baranton G. Antigenic variation Of Borrelia turicatae Vsp surface lipoproteins Lipoproteins The packages in which cholesterol and triglycerides travel throughout the body. Mentioned in: Lipoproteins Test lipoproteins (lip´ōprō´tēns), n. occurs in vitro in vitro /in vi·tro/ (in ve´tro) [L.] within a glass; observable in a test tube; in an artificial environment. in vi·tro adj. In an artificial environment outside a living organism. and generates novel serotypes. Res Microbiol. 2000;151:5-12. (10.) Hayes L, Wright D, Archard L. Segmented arrangement of Borrelia duttonii DNA and location of variant surface antigen genes. J Gen Microbiol. 1988;134(Pt 7):1785-93. (11.) Takahashi Y, Cutler S, Fukunaga M. Size conversion of a linear plasmid in the relapsing fever agent Borrelia duttonii. Microbiol Immunol. 2000;44:1071-4. (12.) Ras NM, Lascola B, Postic D, Cutler SJ, Rodhain F, Baranton G, et al. Phylogenesis phy·lo·gen·e·sis n. See phylogeny. of relapsing fever Borrelia spp. Int J Syst Bacteriol. 1996;46:859-65. (13.) Fukunaga M, Ushijima Y, Aoki LY, Talbert A. Detection of Borrelia duttonii, a tick-borne relapsing fever agent in central Tanzania, within ticks by flagellin gene-based nested polymerase chain reaction. Vector Borne Zoonotic Zoonotic A disease which can be spread from animals to humans. Mentioned in: Zoonosis Dis. 2001;1:331-8. (14.) Bunikis J, Garpmo U, Tsao J, Berglund J, Fish D, Barbour AG. Sequence typing reveals extensive strain diversity of the Lyme borreliosis agents Borrelia burgdorferi Borrelia burg·dor·fe·ri n. A spirochete causing Lyme disease in humans. Borrelia burgdorferi The spirochete agent of Lyme disease, which contains several outer membrane proteins and a highly immunogenic flagellar in North America and Borrelia afzelii in Europe. Microbiology. 2004;150:1741-55. (15.) Bunikis J, Tsao J, Garpmo U, Berglund J, Fish D, Barbour A. Typing of Borrelia relapsing fever group strains. Emerg Infect Dis. 2004;10:1661-4. (16.) Cutler SJ, Akintunde C, Moss J, Fukunaga M, Kurtenbach K, Talbert A, et al. Successful in vitro cultivation of Borrelia duttonii and its comparison with Borrelia recurrentis. Int J Syst Bacteriol. 1999;49:1793-9. (17.) Cutler SJ, Moss J, Fukunaga M, Wright D, Fekade D, Warrell D. Borrelia recurrentis characterization and comparison with relapsing-fever, Lyme-associated, and other Borrelia spp. Int J Syst Bacteriol. 1997;47:958-68. (18.) Cutler SJ, Fekade D, Hussein K, Knox KA, Melka A, Cann K, et al. Successful in-vitro cultivation of Borrelia recurrentis. Lancet. 1994;343:242. (19.) Barbour A. Isolation and cultivation of Lyme disease spirochetes. Yale J Biol Med. 1984;57:521-5. (20.) Fukunaga M, Ushijima Y, Aoki L, Talbert A. Detection of Borrelia duttonii, a tick-borne relapsing fever agent in central Tanzania, within ticks by flagellin gene-based nested polymerase chain reaction. Vector Borne Zoonotic Dis. 2001;1:331-8. (21.) Wang G; van Dam AP, Schwartz I, Dankert J, Molecular typing of Borrelia burgdorferi sensu lato: taxonomic, epidemiological, and clinical implications. Clin Microbiol Rev. 1999;12:633-53. (22.) Liveris D, Varde S, Iyer R, Koenig S, Bittker S, Cooper D, et al. Genetic diversity of Borrelia burgdorferi in Lyme disease patients as determined by culture versus direct PCR with clinical specimens. J Clin Microbiol. 1999;37:565-9. (23.) Conrads G, Claros MC, Citron citron (sĭt`rən), name for a tree (Citrus medica) of the family Rutaceae (orange family), and for its fruit, the earliest of the citrus fruits to be introduced to Europe from Asia. DM, Tyrrell KL, Merriam V, Goldstein E, 16S-23S rDNA internal transcribed spacer ITS (for internal transcribed spacer) refers to a piece of non-functional RNA situated between structural ribosomal RNAs (rRNA) on a common precursor transcript. Read from 5' to 3', this polycistronic rRNA precursor transcript contains the 5' external transcribed sequence (5' ETS), sequences for analysis of the phylogenetic relationships among species of the genus Fusobacterium. Int J Syst Evol Microbiol. 2002;52:493-9. (24.) Fukunaga M, Koreki Y. The flagellin gene of Borrelia miyamotoi sp. nov. and its phylogenetic relationship among Borrelia species. FEMS FEMS Federation of European Microbiological Societies FEMS Federation of European Materials Societies FEMS Fabrication Engineering Management System FEMS Facility Equipment Maintenance System (PMEL/TMDE) Microbiol Lett. 1995;134:255-8. (25.) Qiu W-G, Schutzer SE, Bruno JF, Attic O, Xu Y, Dunn JJ, et al. Genetic exchange and plasmid transfers in Borrelia burgdorferi sensu stricto revealed by three-way genome comparisons and multilocus sequence typing. Proc Natl Acad Sci U S A. 2004;101:14150-5. (26.) Schwan TG, Raffel SJ, Schrumpf ME, Policastro PF, Rawlings JA, Lane RS, et al. Phylogenetic analysis of the spirochetes Borrelia parkeri and Borrelia turicatae and the potential for tick-borne relapsing fever in Florida. J Clin Microbiol. 2005;43:3851-9. (27.) Borgnolo G, Denku B, Chiabrera F, Hailu B. Louse-borne relapsing fever in Ethiopian children: a clinical study. Ann Trop Paediatr. 1993;13:165-71. (28.) Ramos J, Malmierca E, Reyes F, Wolde W, Galata A, Tesfamariam A, et al., Characteristics of louse-borne relapsing fever in Ethiopian children and adults. Ann Trop Med Parasitol. 2004;98:191-6. (29.) Brown V, Larouze B, Desve G, Rousset J, Thibon M, Fourrier A, et al. Clinical presentation of louse-borne relapsing fever among Ethiopian refugees in northern Somalia. Ann Trop Med Parasitol. 1988;82:499-502. (30.) Jongen VH, van Roosmalen J, Tiems J, Van Holten J, Wetsteyn JC. Tick-borne relapsing fever and pregnancy outcome in rural Tanzania. Acta Obstet Gynecol Scand. 1997;76:834-8. (31.) Barclay A, Coulter J. Tick-borne relapsing fever in central Tanzania. Trans R Soc Trop Med Hyg. 1990;84:852-6. (32.) Melkert P, Mortality in high risk patients with tick-borne relapsing fever analysed by the Borrelia-index. East Afr Med J. 1991;68:875-9. (33.) Cadavid D, Pachner AR, Estanislao L, Patalapati R, Barbour AG. Isogenic isogenic /iso·gen·ic/ (-jen´ik) syngeneic. isogenic (ī´sōjen´ik), adj originating from a common source; possessing the same genetic composition. serotypes of Borrelia turicatae show different localization Customizing software and documentation for a particular country. It includes the translation of menus and messages into the native spoken language as well as changes in the user interface to accommodate different alphabets and culture. See internationalization and l10n. in the brain and skin of mice. Infect Immun. 2001;69:3389-97. (34.) Vidal V, Scragg I, Cutler S, Rockett K, Fekade D, Warrell D, et al. Variable major lipoprotein lipoprotein (lĭp'əprō`tēn), any organic compound that is composed of both protein and the various fatty substances classed as lipids, including fatty acids and steroids such as cholesterol. is a principal TNF-inducing factor of louse-borne relapsing fever. Nat Med. 1998;4:1416-20. Dr Scott is a researcher in the Department of Cellular and Molecular Biology molecular biology, scientific study of the molecular basis of life processes, including cellular respiration, excretion, and reproduction. The term molecular biology was coined in 1938 by Warren Weaver, then director of the natural sciences program at the Rockefeller , Imperial College of Science, Technology and Medicine (education) Imperial College of Science, Technology and Medicine - (IC, ICST&M) One of the colleges of London University. The Department of Computing is the home of FOLDOC. IC Home. , London. She has worked with relapsing fever spirochetes for 2 years, primarily characterizing variable membrane proteins. Address for correspondence: Sally Cutler, Bacterial Zoonoses Zoonoses Infections of humans caused by the transmission of disease agents that naturally live in animals. People become infected when they unwittingly intrude into the life cycle of the disease agent and become unnatural hosts. , Department of. Statutory and Exotic Bacterial Diseases, Veterinary Laboratories Agency The Veterinary Laboratories Agency (VLA) is an executive agency of the UK government department, the Department for Environment, Food and Rural Affairs(Defra). It carries out animal disease surveillance, diagnostic services and veterinary scientific research for government and , Woodham Lane, New Haw haw, common name for several plants, e.g., the hawthorn and the black haw (see honeysuckle). , Addlestone, Surrey, KT15 3NB, United Kingdom; fax: 44-1932-357-423; email: s.cutler@ vla.defra.gsi.gov.uk Julie Christine Scott, * David Julian Maurice Wright, * and Sally Jane Cutler ([dagger]) * Imperial College of Science, Technology and Medicine, South Kensington, London, United Kingdom; and ([dagger]) Veterinary Laboratories Agency, Weybridge, Surrey, United Kingdom
Table 1. Sequence heterogeneity among the 568- to 587-bp intergenic
spacer sequence of the Borrelia duttoniil B. recurrentis group *
Position
Strain 108 129 187 215 304 325/326
B. recurrentis A T T C T GT
type I
B. recurrentis A T C T T GT
type II
B. duttonii G T C C C GT
type I
B. duttonii A T T C T GT
type II
B. duttonii A C T C T GT
type III
B. duttonii G T C C T AC
type IV
Consensus A T T/C C T GT
sequence
Position
Strain 379 402 438 441 456 467
B. recurrentis T A T G T T
type I
B. recurrentis T A T G T T
type II
B. duttonii T A C T T T
type I
B. duttonii T A T G T T
type II
B. duttonii T A T G T T
type III
B. duttonii G -- T T C C
type IV
Consensus T A T G T T
sequence
Position
Strain 474 491 525 532
B. recurrentis A G G C
type I
B. recurrentis A G G C
type II
B. duttonii A G A G
type I
B. duttonii A G G C
type II
B. duttonii A G G C
type III
B. duttonii G A G G
type IV
Consensus A G G G/C
sequence
* Only exemplar sequences are included. GenBank accession nos. for
B. recurrentis are DQ000277-8; those for B. duttonii types I-IV are
DQ000279-DQ000282.
Table 2. Sequence heterogeneity within and between Borellia spp.
using the rrs gene
Position
Type or species 57 206 373 488 917 1013 1429
B. recurrentis type I A T C T T G T
B. recurrentis type II A T C T T A T
B. duttonii A C C C C G C
B. crocidurae G C -- C C G C
Table 3. Intergenic spacer sequence diversity among 757-762 by
Borrelia spp., DQ000284-DQ000286
Location
Strain 133 224 255 290 336 337
Type 1 (IM/16) C G G A -- --
Type 2 (IM/19) T A A G T A
Type 3 (IK/23) C A G G T G
Consensus C A G G T X
sequence
Location
Strain 347 402-5 424 512 520
Type 1 (IM/16) T -- C A C
Type 2 (IM/19) T -- C G T
Type 3 (IK/23) -- TAGA T G T
Consensus T -- C G T
sequence
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