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Tsetse flies (Glossina spp.) can harbor up to three distinct species of endosymbiotic bacteria that exhibit unique modes of transmission and evolutionary histories with their host. Two mutualist enterics, Wigglesworthia and Sodalis, are transmitted maternally to tsetse flies' intrauterine larvae. The third symbiont, from the genus Wolbachia, parasitizes developing oocytes. In this study, we determined that Sodalis isolates from several tsetse fly species are virtually identical based on a phylogenetic analysis of their ftsZ gene sequences. Furthermore, restriction fragment-length polymorphism analysis revealed little variation in the genomes of Sodalis isolates from tsetse fly species within different subgenera (Glossina fuscipes fuscipes and Glossina morsitans morsitans). We also examined the impact on host fitness of transinfecting G. fuscipes fuscipes and G. morsitans morsitans flies with reciprocal Sodalis strains. Tsetse flies cleared of their native Sodalis symbionts were successfully repopulated with the Sodalis species isolated from a different tsetse fly species. These transinfected flies effectively transmitted the novel symbionts to their offspring and experienced no detrimental fitness effects compared to their wild-type counterparts, as measured by longevity and fecundity. Quantitative PCR analysis revealed that transinfected flies maintained their Sodalis populations at densities comparable to those in flies harboring native symbionts. Our ability to transinfect tsetse flies is indicative of Sodalis ' recent evolutionary history with its tsetse fly host and demonstrates that this procedure may be used as a means of streamlining future paratransgenesis experiments.
Trypanosomiasis in humans and nagana in other animals are highly debilitating diseases that are fatal if left untreated. According to the World Health Organization, at least 100,000 new cases of trypanosomiasis were reported each year over the past decade, and 60 million more people in 36 African nations are at risk of acquiring the disease.
Trypanosome transmission requires interaction between several organisms, including the pathogen, the insect vector, wild reservoirs, and the human host. While this interdependence can be complicated, it provides numerous opportunities for interfering with disease transmission. However, current solutions, which involve treating infected hosts chemotherapeutically and/or inhibiting further transmission by attempting to reduce the insect vector population with traps or insecticides, are impractical, are harmful to the environment and public health, and have had limited sustainability in the field (4, 12, 13). Recent advances in molecular biology provide opportunities to use transgenic technologies for the purpose of diminishing vectorial capacity via genetic manipulation (5).
Tsetse flies (Diptera: Glossinidae), which feed exclusively on vertebrate blood, harbor three distinct species of endosymbiotic bacteria that presumably play different roles in the flies. The obligate mutualist Wigglesworthia glossinidia is a member of the family Enterobacteriaceae. This bacterium resides mainly within the cells (bacteriocytes) of a specialized organ in the tsetse fly's anterior midgut called the “bacteriome” and has a highly streamlined 700-kb genome. A large proportion of its proteome encodes vitamin biosynthesis pathways that may help supplement the tsetse fly's vertebrate-blood-specific diet (2). This hypothesis is supported by the fact that tsetse flies become sterile in the absence of Wigglesworthia, but this reaction can be reversed by feeding the flies vitamin-supplemented blood (27, 28).
Tsetse flies harbor a second mutualistic symbiont, of the genus Sodalis, which is also a member of the family Enterobacteriaceae. This secondary symbiont has broad tissue tropism and can be found both inter- and intracellularly in the midgut, muscle, fat body, milk gland, and salivary glands of certain species (8). Analysis of the Sodalis genome sequence reveals that this organism is closely related, both in terms of genome size and chromosomal synteny, to several free-living pathogens, including Salmonella and Yersinia (35). However, the large number of pseudogenes (972) present on the Sodalis chromosome, in conjunction with an unusually low protein coding density (49.2%), may represent early genome erosion events during the course of symbiosis as the organism adapted to its host's physiological environment (1, 35). Using Escherichia coli macroarrays, Rio et al. (30) utilized a heterologous array hybridization approach to determine that significant differences exist between the genomes of Sodalis and another, closely related symbiotic bacterium (Sitophilus oryzae primary endosymbiont [SOPE]) from the rice weevil (18). These differences may account for the fact that each organism has adapted to the unique nutritional requirements of its host. These data suggest a specific, anchored relationship between symbiont and host and, furthermore, indicate an inability to readily undergo horizontal transmission and establishment in distinct insect taxa (30).
The tsetse fly's third symbiont (9), a member of the genus Wolbachia, is a rickettsia-like parasitic bacterium found only in certain populations of tsetse flies, as well as some other insects, mites, crustaceans, and filarial nematodes (29, 41). The role of Wolbachia in tsetse flies is unknown, although in other organisms it causes a variety of reproductive abnormalities, the most common of which is called “cytoplasmic incompatibility” (CI) (35). Recently, several groups have performed Wolbachia “transinfection” experiments, during which this bacterium was transferred between different hosts with the intention of determining the impact each organism exerts on the other. For example, McGraw et al. (24) transinfected Drosophila simulans with the overreplicating Wolbachia sp. strain popcorn, originally isolated from Drosophila melanogaster. Initially, high Wolbachia ovary densities likely caused a reduction in the reproductive fitness of the recipient flies. However, both conditions (high density and detrimental fitness costs) were rapidly reversed in subsequent generations, leading the authors to speculate that the host was intimately involved in regulating Wolbachia replication rates. In a different study, a Wolbachia strain (wKue) that induces CI in its native host (Ephestia kuehniella) was transferred to another moth host (Ostrinia scapulalis) that normally expresses Wolbachia-induced male killing (O. scapulalis was cleared of its native Wolbachia by tetracycline treatment). Thereafter, the recipient host expressed CI similar to that of the donor, thus demonstrating the crucial role of the Wolbachia genotype in determining the type of reproductive abnormality (34).
These symbioses are successful in large part because the above-mentioned bacteria have adapted to the tsetse fly's unique viviparous reproductive physiology. Adult females produce a single egg per gonotrophic cycle, which hatches in utero. The offspring completes its development through three larval instars in utero, during which time it acquires nutrients and both gut symbionts via milk gland secretions from the mother. Wolbachia bacteria, which reside primarily in reproductive tissue, are transmitted transovarially (29). Given the sterile nature of its vertebrate-blood-specific diet, the tsetse fly's resident microbial community is highly restricted in comparison to those of insects that feed on multiple diets throughout their development.
Sodalis is of great interest from the perspective of controlling trypanosomiasis. A procedure previously developed, called “paratransgenesis,” involves expressing a foreign protein in Sodalis (6). These recombinant Sodalis bacteria are then microinjected into the hemocoels of fertile female flies. The tsetse fly's unique viviparous reproductive biology (females use milk gland secretions to nourish three larval instars) ensures that recombinant symbionts are vertically transmitted to the progeny, where they inhabit the same body compartments as they do in their native host (8). Sodalis is ideally suited for use in paratransgenesis because it resides in the tsetse fly's midgut in close proximity to pathogenic trypanosomes, it can be cultured and genetically modified, and recombinant clones can be introduced into females, where they are vertically transmitted to the offspring (31). Furthermore, Sodalis' annotated genome indicates that the bacterium has reduced metabolic capabilities that would severely hinder (or most likely completely eliminate) survival outside of its normal host (36). In fact, attempts to colonize flies by including recombinant Sodalis in their blood meals have not been successful, in support of the maternal-transmission mode (unpublished data). Several antimicrobial peptides, which have little or no effect on Sodalis but are toxic to trypanosomes, have been identified for use in this system as transgene products (16, 21).
We conducted experiments to determine the level of biological integration shared by Sodalis and its tsetse fly host species, with the goal of streamlining the paratransgenesis approach for future field studies. Tsetse flies were chosen from distinct species groups (Glossina fuscipes fuscipes from the palpalis group and Glossina morsitans morsitans from the morsitans group) (7) with the intention of using individuals that were as distantly related as possible. Phylogenetic reconstruction analysis and restriction fragment length polymorphism (RFLP) analysis were performed to determine the relatedness of Sodalis strains from the aforementioned tsetse fly species. A transinfection procedure novel to this model system was developed to ascertain whether Sodalis from one tsetse fly species can successfully colonize another tsetse fly species and be vertically transmitted to the offspring without altering maternal fecundity. Finally, quantitative PCR (QT-PCR) analysis was initiated to investigate Sodalis symbiont densities in the progeny of wild-type (WT) and transinfected tsetse flies. We discuss the significance of our findings in the context of improving the application of tsetse fly paratransgenesis.
Phylogenetic studies were conducted on field-collected tsetse flies (Glossina austeni, Shimba Hills, Kenya; Glossina pallidipes, Arba Minsch, Ethiopia; Glossina brevipalpis, Shimba Hills, Kenya; Glossina morsitans submorsitans, Tanzania; and Glossina tachinoides and Glossina pallidipes gambiensis, Burkino Faso) and individuals colony-reared at Yale University. Rice weevils (Sitophilus oryzae) were reared in Villeurbanne (BF2I), France. Transinfection experiments were performed using G. fuscipes fuscipes and G. morsitans morsitans tsetse flies maintained in Yale's insectary at 24°C with 40 to 50% relative humidity. These flies received defibrinated bovine blood every 48 h through an artificial-membrane feeding system (26).
Sodalis glossinidius morsitans and Sodalis glossinidius fuscipes were isolated from surface-sterilized G. morsitans and G. fuscipes pupae and cultured on Aedes albopictus C6/36 cells as described previously (10). The cultures were subsequently maintained in vitro (in the absence of C6/36 cells) at 25°C in Mitsuhashi-Maramorosch (M-M) medium [1 mM CaCl2, 0.2 mM MgCl2, 2.7 mM KCl, 120 mM NaCl, 1.4 mM NaHCO3, 1.3 mM NaH2PO4, 22 mM d-(+) glucose, 6.5 g/liter lactalbumin hydrolysate, and 5.0 g/liter yeast extract] supplemented with 5% heat-inactivated fetal bovine serum (6).
The gene sequence encoding the cell division protein FtsZ was analyzed to phylogenetically compare different species of Sodalis and other closely related enterics. The gene fragment was PCR amplified using primers (F, 5′-GACGCGGTGATTAAAGTC-3′; R, 5′-CGATATCTCCAGCAACG-3′) designed on the basis of conserved regions (730 bp) of the ftsZ gene among eubacteria. All 50-μl PCR amplification reactions were performed in an MJ Research thermal cycler using the following procedure: 95°C for 5 min, followed by 35 cycles at 95°C, 55°C, and 72°C, each for 1 min, and a final 7-min elongation/extension. All PCR products were cloned into the pGEM-T vector (Promega) and sequenced using the T7 and SP6 primers. A minimum of three clones were sequenced from each amplification reaction. Symbiont genes were analyzed from a minimum of three flies for each Sodalis and Sitophilus species.
Comparative sequence analyses for FtsZ genes were conducted using the DNAStar software package (Lasergene, Madison, WI), and tree generation was performed using the algorithms in PAUP 4.0 (Swofford).
WT S. glossinidius morsitans and S. glossinidius fuscipes were embedded in 0.5% agarose plugs (~109 cells/plug) and subsequently treated with the following incubations: (i) 50°C and 37°C, each for 12 h, in 20 volumes of lysis solution (100 mM EDTA [pH 8.0], 10 mM Tris-HCl [pH 8.0], 1% N-lauroylsarcosine, 100 μg/ml proteinse K); (ii) three times for 1 h each time at room temperature in 10 volumes of storage buffer (100 mM EDTA [pH 8.0], 10 mM Tris-HCl [pH 8.0], 1 mM phenylmethylsulfonyl fluoride); and (iii) three times for 30 min each time at room temperature in 10 volumes of 10 mM Tris-HCl (pH 8.0). To remove plasmid and phage DNA, the plugs were subjected to contour-clamped homogeneous electric field (CHEF) gel electrophoresis at 14°C, with a ramping interval of 150 to 200 s, for 20 h at 200 V (1). The plugs were subsequently removed from the gel (1% agarose) and treated with PacI restriction endonuclease (TTAAT↓TAA [the arrow indicates the cut site]; New England Biolabs, Boston, MA) for 24 h at 37°C. The digested samples were again subjected to CHEF electrophoresis, this time using a 9.1- to 13.1-s ramping interval. Finally, the gel was stained with ethidium bromide, destained in double-distilled H2O, and viewed using a Kodak S2000 imaging system.
WT S. glossinidius morsitans and S. glossinidius fuscipes were genetically transformed using a modified version of a previously described protocol (11). In brief, 100 ml of log-phase cells (optical density at 600 nm, ~0.5; SmartSpec Plus spectrophotometer; Bio-Rad, Hercules, CA) were washed consecutively in 50 ml, 10 ml, and 2 ml of sterile 10% glycerol. The cell pellets were resuspended in 200 μl of sterile 10% glycerol, and 50-μl aliquots were mixed with ~50 ng of eGFPuv plasmid (BD Bioscience, Palo Alto, CA) and subjected to electroporation (voltage, 1.9 kV; capacitance, 25 μF; resistance, 200 Ω). Recombinant Sodalis (recSodalis) cells were immediately placed into 950 ml of M-M medium and allowed to recover for 24 h. Following this recovery, the Sodalis cells were placed onto a feeder layer of C6/36 cells, and transformants were selected with ampicillin (10 μg/ml) for another 24-h period. Finally, the cells were plated onto M-M agar (supplemented with antibiotics), and a single recSodalis colony was placed into liquid culture (37).
The growth rates of recSodalis cultures were established by measuring the optical densities at 600 nm of two clonal populations of each species over two 1-week periods.
Newly eclosed adult female G. morsitans morsitans and G. fuscipes fuscipes flies were given a blood meal supplemented with 30 μg/ml ampicillin prior to injection. Each fly species was then divided into two groups. One group from each fly species received an injection of ~1.5 × 104 recSodalis bacteria originally isolated from its own species, and the other group received an injection of recSodalis bacteria originally isolated from the other species. Hereafter, the treated fly groups will be referred to as follows: tsetse species/Sodalis species (e.g., G. morsitans morsitans/S. glossinidius morsitans).
All injections were performed on flies anesthetized with CO2, using glass needles and a Narashige IM300 microinjector. Following injection, all groups of flies (n = 20 for each group) were mated (n = 10 males) and subsequently maintained on their designated diets. Two other groups, both of which received no injection, were fed either normal blood (G. fuscipes fuscipesREG and G. morsitans morsitansREG) or blood supplemented with ampicillin (G. fuscipes fuscipesAMP and G. morsitans morsitansAMP). All groups were subsequently maintained in separate cages and received the appropriate diet (as indicated in Table Table1)1) every 48 h throughout the course of the experiment.
The number of pupae and the number of deceased mothers from each group were recorded following each of four 15-day larval-deposition cycles. Total DNA was extracted from mothers and offspring at designated times using the method of Holmes and Bonner (19). The presence of recSodalis in treated females was determined by using a PCR amplification assay. The primers used (F, 5′-AGTGGAGAGGGTGAAGGTGA-3′; R, 5′-ATCCCAGCAGCAGTTACAAA-3′) targeted a 600-bp fragment of the gene encoding the enhanced green fluorescent protein (eGFP) from the eGFPuv transformation plasmid (BD Biosciences, Palo Alto, CA). To confirm vertical transmission of recSodalis, fly DNA from 14-day-old adult progeny from each group of treated mothers was PCR amplified (F, 5′-ACCGACTGGGGACAGTACGATG-3′; R, 5′-CAAAGAAGTCATAGGTCATAAC-3′) using primers specific for the Sodalis chromosomal exochitinase gene (849-bp amplicon; GenBank accession no. BSPY11391). PCR amplification, using an MJ Research (PTC-200) thermal cycler, consisted of a 2-min hot start at 94°C, followed by 30 cycles at 94°C for 30 s, 54°C for 40 s, and 72°C for 1 min and a final elongation/extension at 72°C for 7 min. The amplified products were verified by agarose gel electrophoresis.
Total DNA was extracted from (i) in vitro cultures of S. glossinidius fuscipes and S. glossinidius morsitans, (ii) 2-week-old adult offspring of WT mothers, (iii) 2- and 60-day-old mothers treated with recSodalis harboring the eGFPuv plasmid, and (iv) 2-week-old adult offspring of aposymbiotic WT flies (these individuals were fed an antibiotic-supplemented diet and served as a background control). The Holmes and Bonner (19) method of DNA extraction was used in all cases.
QT-PCR was performed with an icycler iQ real-time PCR detection system (Bio-Rad, Hercules, CA). A 117-bp region of the single-copy Sodalis exochitinase gene was amplified with the following primers: F, 5′-TTATACCGACTGGGGACAGT-3′, and R, 5′-ATAGGCGGTCGGGGATAATT-3′. A specific fluorescent beacon designed for the central portion of the amplicon (Sgchi probe, 5′-FAM-CCGCCGCGTTGATGTCGGGAGTCGTGGCCGGCGG-DABCYL-3′) was utilized for chitinase quantification. PCR reagents included PLATINUM Quantitative PCR SuperMIX-UDG (Invitrogen, Carlsbad, CA; catalog no. 11730-017) and the addition of 1.7 μl of template, specific primers, and beacon (1.5 U PLATINUM Taq DNA polymerase, 20 mM Tris-HCl, pH 8.4, 50 mM KCl, 3 mM MgCl2, 200 μM dATP, 200 μM dGTP, 200 μM dCTP, 400 μM dUTP, 1 U UDG, 0.2 μM of each primer, and 0.2 μM beacon) in a final reaction volume of 50 μl. The amount of fluorescence generated was measured during each amplification cycle (8 min and 30 seconds at 95°C, followed by 40 cycles at 95°C for 15 seconds and 1 min at 56°C). Optical-density readings were used to normalize the amount of individual DNA (μg) analyzed so that Sodalis density would be represented as the chitinase copy number per tsetse fly). Symbiont density estimates were obtained by comparison to a standard curve using Bio-Rad icycler iQ Multi-Color Real Time PCR data analysis software. All assays were carried out in 96-well format plates in duplicate and were averaged for each sample. Negative controls were included in all amplification reactions.
Fitness and QT-PCR data are all presented as the mean ± standard error of the mean (SEM). Statistical analysis was performed using SAS system v9.1 for Windows. The specific statistical test used to analyze each data set is indicated where appropriate in Results. Where densities appeared skewed, the data were log transformed to satisfy normality. Differences were considered significant at a P value of ≤0.05.
A phylogenetic tree was generated based on the FtsZ gene sequences of different Sodalis species. This gene has been used successfully for the same purpose with different Wolbachia strains (41). Our results indicated that all mutations observed in the ftsZ locus were synonymous and that the insect symbionts Sodalis and SOPE form a clade related to the other enterics examined. However, the FtsZ gene sequence did not demonstrate enough variability to determine the ancestral relationships among the Sodalis species, although the Sodalis and SOPE could be described as sister taxa (Fig. (Fig.1A1A).
RFLP analysis was used as a means of identifying large-scale divergence between the S. glossinidius fuscipes and S. glossinidius morsitans genomes. Prior to enzymatic treatment of agarose plugs containing total bacterial DNA, the Sodalis multicopy extrachromosomal elements were run out of the samples via CHEF electrophoresis (Fig. (Fig.1B).1B). The remaining intact chromosomal DNA was then treated with PacI restriction endonuclease, which was chosen because of its low cutting frequency (76 cut sites within the 4.2-Mb chromosome). Analysis of the banding patterns of the digested chromosomal DNAs from the two species revealed few polymorphisms: only two over the range of DNA fragments visible on the gel (Fig. (Fig.1B).1B). Furthermore, RFLP analysis using the PmeI restriction endonuclease (which cuts the chromosome 52 times) revealed no visible polymorphisms (data not shown). These results, in conjunction with the phylogenetic analysis of ftsZ, provided preliminary evidence leading us to conclude that S. glossinidius fuscipes and S. glossinidius morsitans represent closely related organisms symbolic of a recent symbiotic association with their host taxa.
Prior to transinfecting female flies, the in vitro growth rates of recSodalis glossinidius fuscipes and recSodalis glossinidius morsitans were established. As indicated in Fig. Fig.2,2, clonal populations of both bacterial strains grew at virtually identical rates following their initial passage.
We next set out to determine whether recSodalis was able to successfully colonize transinfected females and be subsequently transmitted to their offspring. To achieve this goal, a PCR amplification approach was used to detect the Sodalis chromosomal exochitinase gene in female flies and offspring harboring WT Sodalis, and recSodalis. PCR was also used to detect the eGFPuv plasmid in mothers treated with recSodalis. All groups of treated mothers and their offspring retained the introduced recSodalis throughout the course of these experiments (Fig. (Fig.3A3A).
Of note is our inability to detect the GFP gene in the offspring of transinfected mothers. This phenomenon was unlikely to have resulted from loss of the eGFPuv plasmid during the 30-day pupal stage (on the contrary, unpublished data from our laboratory indicated that recSodalis bacteria grown in vitro retained their plasmids in the absence of antibiotic selection over a 3-month test period). Oxygen deprivation in the sealed environment of the tsetse fly's pupal case more likely accounted for our inability to consistently detect this gene (although very faint bands were present in some samples), as the replication and stability of plasmids carrying ColE1 replication origins (i.e., pGFPuv) can be severely impeded under such conditions (15, 20). We are currently developing a method of inserting exogenous DNA directly into the Sodalis chromosome via homologous recombination.
In the case of untreated mothers, all groups contained WT Sodalis flora at day 2. However, by day 60, WT Sodalis had been eliminated from those mothers fed an ampicillin-supplemented diet, and it was not present in any subsequent offspring. In contrast, when the flies were fed normal blood, WT Sodalis bacteria were present in all mothers and their offspring (Fig. (Fig.3B).3B). These results demonstrate that female flies are able to reproduce when maintained on ampicillin (which does not affect the intracellular primary symbiont, Wigglesworthia) and that experimentally introduced Sodalis bacteria are efficiently transmitted to offspring.
The fitness effects of transferring recSodalis between tsetse fly species are shown in Fig. 4A to D. Over the course of the 60-day observation period, no significant difference in mortality was observed within the G. fuscipes fuscipes (P = 0.9629; Wilcoxon test) and the G. morsitans morsitans (P = 0.7326; log rank test) groups (Fig. 4A and B).
Fecundity, as measured by the total number of larvae deposited per group over the course of four deposition cycles, was the second parameter measured as a means of determining the fitness cost associated with interspecific symbiont-host interactions. No significant difference in numbers of larvae produced was observed within any of the G. fuscipes fuscipes and G. morsitans morsitans groups (Fig. 4C and D) (P = 0.2492 and 0.3269, respectively; nested two-factor analysis of variance [ANOVA]).
When comparisons were made between all of the G. fuscipes fuscipes groups combined and all of the G. morsitans morsitans groups combined, some significant differences were observed. For example, significantly fewer (P < 0.0001; log rank test) G. fuscipes fuscipes mothers survived (51% ± 10.2%) the 60-day observation period than G. morsitans morsitans mothers (90% ± 3%) (Fig. 4A and B). Also, a significant difference (P< 0.05; nested two-factor ANOVA) in the cumulative number of larvae (the total over 60 days) was observed between the G. fuscipes fuscipes (n = 143 pupae) and G. morsitans morsitans (n = 226 pupae) groups.
QT-PCR was used to determine the number of genomes per Sodalis cell grown in vitro. Both strains maintained multiple chromosomes, with S. glossinidius fuscipes ranging from 19 (±6.2) to 28 (±4.3) and S. glossinidius morsitans ranging from 23 (±3.1) to 31 (±2.4) (Table (Table2).2). This range is not significantly different between Sodalis species (experiment 1, P = 0.11; experiment 2, P = 0.16; Students' t test). Because both strains harbor several chromosomes, all ensuing mention of Sodalis density is a reflection of the genome copy number rather than absolute Sodalis cell numbers.
A similar approach was utilized to determine if WT G. fuscipes fuscipes (G. fuscipes fuscipesWT) and WT G. morsitans morsitans (G. morsitans morsitansWT) maintained similar Sodalis densities and if transinfected flies maintained their novel symbionts at titers similar to those of their WT counterparts. With these goals in mind, we used genomic DNA (extracted from treated and control flies) as a template to perform QT-PCR with primers that amplify a region of the Sodalis single-copy chitinase gene. The results, which are shown in Fig. Fig.5,5, are presented as the number of Sodalis exochitinase gene copies per tsetse fly (and thus represent the number of Sodalis genomes per fly).
Two-week-old adult female progeny of flies from both WT species maintained their symbionts at virtually identical levels (G. fuscipes fuscipesWT, 1.33 × 107 ± 4.3 × 105; G. morsitans morsitansWT, 1.57 × 107 ± 5 × 106; P = 0.9459) (Fig. (Fig.5)5) (Nested two-factor weighted ANOVAs were used for all statistical comparisons in this section). Furthermore, no significant difference was observed between G. fuscipes fuscipesWT and G. fuscipes fuscipes/S. glossinidius fuscipes (P = 0.0731) and G. fuscipes fuscipesWT and G. fuscipes fuscipes/S. glossinidius morsitans (P = 0.1096). However, this was not the case with the G. morsitans morsitans groups. Offspring of G. morsitans morsitans/S. glossinidius morsitans and G. morsitans morsitans/S. glossinidius fuscipes mothers exhibited bacterial densities significantly lower than those of their G. morsitans morsitansWT counterparts (G. morsitans morsitans/S. glossinidius morsitans versus G. morsitans morsitansWT, P = 0.0219; G. morsitans morsitans/S. glossinidius fuscipes versus G. morsitans morsitansWT, P = 0.0003) (Fig. (Fig.5).5). When both treated groups within G. fuscipes fuscipes (G. fuscipes fuscipes/S. glossinidius fuscipes plus G. fuscipes fuscipes/S. glossinidius morsitans) were compared to both treated groups within G. morsitans morsitans (G. morsitans morsitans/S. glossinidius morsitans plus G. morsitans morsitans/S. glossinidius fuscipes), no significant difference was observed (P = 0.0911). Furthermore, no significant difference was observed when the treated groups within each species were compared (G. fuscipes fuscipes/S. glossinidius fuscipes versus G. fuscipes fuscipes/S. glossinidius morsitans, P = 0.8348; G. morsitans morsitans/S. glossinidius morsitans versus G. morsitans morsitans/S. glossinidius fuscipes, P = 0.1430). Thus, transinfection does not compromise the tsetse fly's ability to maintain natural Sodalis densities.
In this study, we examined the efficacy of transinfecting female tsetse flies with nonnative symbiotic flora and whether any fitness costs are associated with this procedure. Because endogenous WT bacteria could have a competitive advantage over recombinant native and nonnative bacteria, effective removal of WT symbionts from experimental flies was imperative for the study. Our results indicate that both G. morsitans morsitans and G. fuscipes fuscipes female flies were transiently cured (via treatment with ampicillin) of their native Sodalis symbionts during the course of these experiments. Sodalis bacteria genetically modified in vitro were then able to successfully colonize their antibiotic-treated native hosts. Furthermore, Sodalis-free flies were effectively transinfected with recSodalis originally isolated from a different host species, and the recombinant symbiotic flora was maintained at densities similar to those in WT individuals.
Several studies, which were based on genomics information, have been performed to determine the phylogenetic positioning and species relatedness of tsetse fly symbionts. For example, Aksoy et al. (3) determined that the 16S rRNA gene sequences of Sodalis bacteria from five distinct tsetse fly species were practically identical (only 2 out of 1,100 bp were different between Sodalis isolates from the most divergent tsetse fly species examined), arguing for a recent association with their tsetse fly hosts. In contrast, a similar analysis of Wigglesworthia from the same tsetse fly species revealed significant differences in 16S rRNA genes from this bacterium. Furthermore, analysis of 28S rRNA gene spacer (internal transcribed spacer 2) sequences from corresponding tsetse flies indicated concordant evolution with Wigglesworthia, implying that a tsetse fly ancestor had been infected with this bacterium some 50 to 100 million years ago. Then, from this ancestral pair, extant species of tsetse flies and associated Wigglesworthia strains radiated without horizontal-transfer events between species (3). This long association is also reflected in the drastically reduced genome size of the Wigglesworthia bacterium (2).
Our phylogenetic analysis of ftsZ genes from different Sodalis species also supports the concept of a recent symbiotic association between this bacterium and its tsetse fly host. Accordingly, distinct Sodalis strains and their respective hosts have evidently undergone little cospeciation to date. Our RFLP analysis, which was performed to determine whether divergence has occurred on a larger, whole-genome scale, also did not reveal extensive genomic polymorphisms. However, the genome sequence of Sodalis does show a significantly reduced coding capacity and extreme genome erosion (35), both phenomena indicative of a transitioning process from a free-living to a symbiotic state. Arguing against horizontal transfer between species, O'Neill et al. (29) subjected the extrachromosomal DNAs of Sodalis bacteria from five tsetse fly species to RFLP analysis and determined that each one represented a unique isolate. More recently, Sodalis cultured from the hemolymph of G. palpalis gambiensis and G. morsitans morsitans were shown to be genetically distinct when examined by amplified fragment length polymorphism analysis (14). The exact extent of cospeciation between Sodalis and tsetse flies thus needs to be further examined, possibly by performing a more comprehensive RFLP analysis of the chromosomes of distinct Sodalis species or by utilizing loci that are under more relaxed selection for phylogenetic analysis. Our ability to transinfect tsetse flies with heterologous species of this bacterium, without apparently inflicting detrimental fitness costs, further supports a lack of extensive host-symbiont coevolution that would result in species-specific functional adaptations.
Of crucial importance for a successful paratransgenic strategy is the question of whether transinfected females exhibit a fitness cost compared to their WT counterparts. In the field, such an occurrence would give WT flies an advantage over paratransgenic flies, and the latter group would likely die off. We observed no major inhibitory effects on the fecundity or longevity of transinfected females compared to their WT counterparts. Russell and Moran (33) observed a similar response when performing transinfection experiments in the pea aphid, Acyrthosiphon pisum. Clonal strains of A. pisum naturally free of secondary symbionts exhibited no apparent reduction in fitness (as determined by measuring the “mean relative growth rate”) when transinfected with three different native symbionts from infected donor strains. Interestingly, when the experiment was repeated with a novel symbiont (isolated from the aphid Aphis craccivora), donor A. pisum exhibited elevated fitness effects. Further experiments are necessary to better determine the functional role of secondary symbionts with regard to host physiology.
Of note is the significant difference in both cumulative mortality and fecundity between the G. fuscipes fuscipes and G. morsitans morsitans groups examined. Fundamental differences in the habitat preferences of these flies could account for this discrepancy. G. fuscipes fuscipes is a member of the palpalis group, which inhabits humid riparian/dense-forest environments, while G. morsitans morsitans (a member of the morsitans group) resides mainly in the drier open-savannah zone (22). All flies used in these studies were reared in an insectary environment favorable to G. morsitans morsitans, which may have resulted in a cumulative fitness disadvantage for G. fuscipes fuscipes.
Prior studies of symbiont density dynamics in G. morsitans morsitans indicated tight regulation of the mutualistic partners through host development and during potentially disruptive events, including host immune challenge, parasite infections, and environmental perturbations (32). Furthermore, different tsetse fly species can harbor different Sodalis loads. Cheng and Aksoy (8) reported high Sodalis levels in midgut tissues from G. morsitans morsitans and Glossina palpalis palpalis and lower levels in G. austeni and G. brevipalpis. QT-PCR experiments performed in this study indicate similar Sodalis densities in G. morsitans morsitans and G. fuscipes fuscipes. However, symbiont-cured G. morsitans morsitans flies repopulated with recombinant native and nonnative Sodalis maintained these bacteria at densities significantly lower than those in their WT counterparts. It should be noted, however, that the P values for the G. morsitans morsitans groups are just below the cutoff delineating significance from nonsignificance. We speculate that had we given the G. morsitans morsitans progeny carrying recSodalis more than 2 weeks prior to harvesting them for assay, their Sodalis densities may have increased to levels comparable to those in WT individuals. In contrast, all of the G. fuscipes fuscipes groups examined exhibited similar Sodalis densities.
Our QT-PCR data are also interesting when considered in the context of tsetse fly-trypanosome interactions. We demonstrated that WT and transinfected individuals of both tsetse fly species maintain similar Sodalis densities. Previous experiments indicated that a positive correlation might exist between high Sodalis densities and trypanosome infection rates (23, 39). This hypothesis is based on the fact that lectins, which exhibit potent trypanocidal activity (38), are inhibited by sugars (i.e., N-acetylglucosamine) produced as by-products of the Sodalis-mediated metabolism of tsetse fly chitin (25, 40). Our findings of similar symbiont densities is somewhat surprising considering that palpalis group flies (G. fuscipes fuscipes) are more refractory to trypanosome infection than flies belonging to the morsitans group (17). Contrary to the above-mentioned hypothesis, our results imply that the degree of susceptibility to infection may not correlate solely with the Sodalis density. The effect of Sodalis transinfection on the tsetse fly's capacity to vector trypanosomes will be the target of future research.
Tsetse flies are the sole vector of African trypanosomes, the causative agent of sleeping sickness in humans and nagana in animals. One potential component of an integrated tsetse fly control strategy is called paratransgenesis, a process whereby flies are made resistant to trypanosome infection by populating them with genetically modified Sodalis bacteria that produce a trypanocidal compound (5). For paratransgenesis to be an effective component of a field-based trypanosomiasis control program, all tsetse fly species that vector the causative agent would theoretically need to be manipulated. The results of this study provide preliminary experimental evidence indicating that Sodalis strains from two distinct host species are similar enough to interspecifically colonize tsetse flies and have little subsequent impact on host fitness under the conditions tested.
This work was generously funded by grants to S.A. from the NIH (AI51584) and GM (069449) and the Robert Leet and Clara Guthrie Patterson Trust. R.V.M.R. was the recipient of an NIH training grant (T32AI07404), a CDC fellowship for training in vector-borne diseases (T01-CCT122306), and a Sigma Xi grant-in-training award. B.L.W. is the recipient of a Kirschstein-NRSA training fellowship (F32AI062680).
We thank Douglas Smith for help with tsetse fly injections, Agnès Vallier for Sitophilus DNA preparations, and members of the Aksoy laboratory for critical review of the manuscript.
Published ahead of print on 1 September 2006.