Parasite collection and morphological identification

Sampling was conducted on hunter-killed bears processed at Wisconsin Department of Natural Resources check stations in Douglas, Bayfield, Ashland, Price, and Lincoln counties during the fall 2007 hunting season. Whole blood was aspirated from the body cavity of each bear into vacuum tubes containing EDTA to minimize clotting (Fisher Scientific, Pittsburgh, Pennsylvania). Blood smears were made in triplicate using 20 µl whole blood per slide, and air-dried, fixed in methanol for 5 min, then Giemsa stained for 1 hr (Harleco, Fisher Scientific, Waltham, Massachusetts). Whole blood was processed in this way because the degree of coagulation and field contamination of cavity-collected samples prevented centrifugation and filtration-based methods. Cover slips were mounted with Canada balsam and slides were microscopically examined for the presence of microfilariae (mf). Adult worms were field collected from the thoracic cavities of 2 bears in Bayfield County and stored in 70% ethanol for identification and DNA isolation. A representative pair of adults and a stained mf slide were submitted to the Museum of Natural History in Paris, France, for morphological study (MNHN no. 329JW). Adult worms were cleared in lactophenol, and transverse sections were made with a razor blade to observe the cuticular ornamentation, a diagnostic character of Dirofilaria spp.

Immunohistology

Midbody fragments of an adult female worm were fixed in 80% ethanol and embedded in paraffin using standard histological procedures. Adult D. immitis collected from naturally infected dogs were also embedded for comparison. Several different antibodies were used to screen D. ursi for the presence of Wolbachia endobacteria. First, polyclonal antibodies directed against the Wolbachia surface protein (WSP-1) of the endosymbiont of D. immitis (pab Di WSP,) or Brugia pahangi (pab Bp WSP) were used at dilutions of 1∶500 to 1∶1,000 (Kramer et al., 2003). Second, a monoclonal antibody raised against the B. malayi wsp (mab Bm WSP) was used at a dilution of 1∶100 (Punkosdy et al., 2003). For comparison, a commercial monoclonal antibody directed against the human heat shock protein 60 (mab HSP 60 LK2, Sigma, St. Louis, Missouri) was used, which cross-reacts with the bacterial hsp-1 ortholog. This antibody was used at a dilution of 1∶5.

For immunostaining, the alkaline phosphatase anti-alkaline phosphatase (APAAP) technique was applied according to the recommendations of the manufacturer (DakoCytomation, Hamburg, Germany) as described previously (Buttner et al., 2003). Following the primary antibody, a mouse anti-rabbit immunoglobulin G (IgG) (1∶25; DakoCytomation) was applied and this was followed by the application of a rabbit-anti mouse IgG (1∶25; DakoCytomation) that binds the APAAP complex (1∶50). As a substrate for the alkaline phosphatase, the chromogen Fast Red TR salt (Sigma) was used and hematoxylin (Merck, Darmstadt, Germany) served as the counter-stain. TBS with 1% albumin was used for a negative control instead of the primary antibody.

DNA isolation and sequence of filarial 5s rDNA intergenic region

Portions of a preserved adult female worm were excised using a razor blade and rinsed twice in 5-min changes of 1× phosphate-buffered saline, pH 7.2, at room temperature. Worm fragments were homogenized by vortexing with 2 zinc-coated BB shot pellets (Daisy, Rogers, Arkansas) in a 2-ml tube for 10 min at room temperature in tissue lysis solution (100 mM EDTA, 100 mM Tris, pH 7.5, 20 mM NaCl), and then were incubated at 65 C in the presence of 1% sodium dodecyl-sulfate, 2 µl 2-mercaptoethanol, and 2 mg/ml proteinase K for 1 hr, or until the samples were completely liquefied. Chromosomal DNA was purified by standard organic extraction and ethanol precipitation protocols (Sambrook and Russell, 2001). DNA was quantified using a NanoDrop Spectrophotometer (NanoDrop, Wilmington, Delaware) and integrity was verified by agarose gel electrophoresis (data not shown). Amplification of the 5s rDNA intergenic spacer region was performed as described (Xie et al., 1994), using D. immitis genomic DNA as a template for positive control, and substituting water for the template as a negative control. Amplicons from D. ursi and D. immitis templates were visualized by agarose gel electrophoresis (data not shown), cloned into the pCR4-TOPO vector, and transformed into OneShot Top 10 chemically competent cells following manufacturer's instructions (Invitrogen, Carlsbad, California). Recombinant plasmids were isolated from cultures of single-colony transformants using the QIAprep Spin Miniprep kit (Qiagen, Valencia, California), and DNA quantified as above. Plasmid inserts from 4 transformants for each species were sequenced from both sides using M13F and M13R primers at the University of Wisconsin Biotechnology Core DNA Sequence Laboratory (Madison, Wisconsin) using Big Dye Terminator chemistry (Applied Biosystems, Carlsbad, California). Forward and reverse sequences for each cloned fragment were aligned using ClustalW ( www.ebi.ac.uk/clustalw) to verify sequence accuracy.

Sequencing of Wolbachia MLST and wsp loci

Genomic DNA was examined for the presence of Wolbachia by polymerase chain reaction (PCR). Amplification used standard primers developed for a multilocus sequence typing system (MLST) for Wolbachia (Baldo, Dunning Hotop et al., 2006) and contained M13 forward and reverse sequencing tags at the 5′ ends to serve as anchors for the degenerate primers during amplification ( http://pubmlst.org/wolbachia/). PCR was performed essentially as described (Baldo et al., 2006a) by using Quick-Load Taq 2× Master Mix (New England Biolabs, Ipswich, Massachusetts), 1 µM of each primer, and 1 µl (∼20 ng) DNA in 20-µl reactions. Additional degenerate primers, WSPintF and WSPintR (Bazzocchi et al., 2000), were used to amplify a fragment of the gene encoding Wolbachia surface protein (WSP-1). PCR was performed using Quick-Load Taq 2× Master Mix adjusted to 2.0 mM Mg²⁺, 1 µM of each primer and 1 µl (∼20 ng) of DNA in a 25-µl reaction. The thermal profile was 94 C for 4 min followed by 35 cycles at 94 C for 45 sec, 50 C for 45 sec, and 72 C for 1.5 min, followed by a final extension of 72 C for 10 min.

Products of the Wolbachia MLST primer pairs were verified by agarose gel electrophoresis, purified using a QIAquick PCR Purification Kit (Qiagen), then cloned. Plasmid DNA was isolated using the GenElute Plasmid Miniprep kit (Sigma) and inserts sequenced on both strands. The ftsZ amplicon was cloned into the PsiI site within the BamHI restriction endonuclease gene of the positive selection vector, pPSV, and the construct was transformed into NEB 5-alpha F′I^q chemically competent Escherichia coli (New England Biolabs). Inserts were sequenced with the M13R primer and a vector-specific primer: 5′ CAGATCGGAGAACATATAGACGTC. PCR products for all other MLST primer pairs were cloned into pCR2.1-TOPO and transformed into One Shot Top 10 competent cells (Invitrogen). Insert sequencing was with the M13F and M13R primers. For each gene fragment, a minimum of 6 independent clones were sequenced and an individual sequence matching the consensus sequence was analyzed further. The amplified wsp fragment was similarly purified, then sequenced bidirectionally, using the primers used for PCR. The sequences obtained were compared to sequences in NCBI databases using BLAST programs (Altschul et al., 1990). The ftsZ fragment was selected for multiple sequence alignment and phylogenetic analysis.

Sequence alignments and tree construction

Sequences were aligned using Muscle v3.6 (Edgar, 2004) with the ‘-noanchors’ option (Supplements 1 and 2). Aligned sequences were trimmed at their termini to remove unaligned or ambiguously aligned regions using Jalview 9.5 (Waterhouse et al., 2009). The new D. ursi 5S rDNA (GenBank accessions GQ241942–GQ241945; and Wolbachia ftsZ (GenBank accession GQ217523) sequences were aligned with the following filarial 5S rDNA sequences and Wolbachia ftsZ sequences, respectively, as designated by NCBI gi and GenBank accession numbers. 5S rDNA: Litomosoides sigmodontis (975832, U31639.1), Acanthocheilonema viteae (975826, U31646.1), Brugia timori (975829, U31636.1), Brugia malayi (533165, L36060.1), Wuchereria bancrofti (975837, U31644.1), Loa loa (975831, U31638.1), Mansonella perstans (975833, U31640.1), Onchocerca volvulus (13661788, AF325539.1), O. ochengi (104345435, DQ523781.1), O. cervicalis (535354), D. repens (6006475, AJ242967.1), D. immitis (169641052, EU360965.1), and Ascaris lumbricoides (159683, M27961.1) (outgroup). Wolbachia ftsZ: D. immitis (44894817, AY523519.1), D. repens (4090332, AJ010273.1), O. ochengi (4090322, AJ010268.1), O. volvulus (9857237, AJ276501.1), O. gutturosa (4090318, AJ010266.1), O. gibsoni (4090320, AJ010267.1), O. lupi (23504732, AJ415416.1), Brugia malayi (113707539, DQ842341.1), B. pahangi (48476367, AY583315.1), Wuchereria bancrofti (70610294, DQ093835.1), Litomosoides sigmodontis (4090328, AJ010271.1), Mansonella perstans (60098023, AJ628414.1), Kalotermes flavicollis (18996128, AJ292345.2), Falsomia candida (19572717, AJ344216.1), Drosophila melanogaster (113707537, DQ842340.1), Dr. simulans (225591853, CP001391.1), Tribolium confusum (113707531, DQ842337.1), and Armadilidium vulgare (113707475, DQ842309.1). No outgroup was included in the Wolbachia ftsZ alignment and tree because recent data suggest that the standard outgroups from the Anaplasmataceae lead to erroneous reconstructions (Bordenstein et al., 2009). For the filarial sequence set, the total alignment length was 171 sites; of these, 60 were parsimony informative; for the Wolbachia ftsZ sequences, the total alignment length was 435 sites, with 115 sites being parsimony informative (data not shown). Trees were generated using Mega4 (Tamura et al., 2007) using the Minimum Evolution (ME) method (Rzhetsky and Nei, 1992) with the parameters listed below or by Maximum Parsimony (data not shown). Bootstrap confidence values, reported as percentages, were calculated based on 1,000 replicates (Felsenstein, 1985). Distances (base substitutions per site) were computed using the Kimura 2-parameter method (Kimura, 1980). The pairwise deletion option was used to eliminate positions containing alignment gaps and missing data. The ME tree was searched using the Close-Neighbor-Interchange (CNI) algorithm (Nei and Kumar, 2000) at a search level of 1.

Parasite prevalence and morphological analysis

Unsheathed mf were observed in the blood of 10 of 47 (21%) bears from 5 counties. Ten mf were examined morphologically (Fig. 1F–H) and measured (in μ) 198–242 long, 4–5.5 wide; head attenuated or not, depending on orientation; 1 or 2 first nuclei isolated in the cephalic space; nuclei tightly packed except in some regions; nerve ring, identified in all specimens; excretory pore and cell, identified in half of the specimens; anus identified once; R2–R4 nuclei identified in half of the specimens; R1 identified once. A very thin anucleated caudal filament 20–40 long was noted. With respect to the adult worm cuticle (Fig. 1A,B,E), females and males have the typical ornamentation marking of the subgenus Nochtiella Faust, 1937, made of successive longitudinal crests (Wong and Brummer, 1978). In the posterior ventral region of the male, this ornamentation (Fig. 1E) has a particular aspect and forms the area rugosa (antislip apparatus for mating) (Bain and Chabaud, 1988). Other characters are those of Dirofilaria Railliet & Henry, 1910 (see Anderson and Bain, 1976), i.e., stout worms with a blunt anterior extremity, no buccal capsule; in females, tail short and caudal extremity with rugosities (Fig. 1C), vulva post-esophageal, relatively small vagina with 2 anterior bents and a posterior chamber (Fig. 1D); in males, caudal alae present, numerous bulky pedunculated precloacal papillae, spicules markedly dissimilar (data not shown). The female posterior region of this specimen is spirally coiled (4 coils), making the length measurement approximate. Measurements of female (in μ unless otherwise stated): about 150 mm long (not precisely measurable because it is coiled); 600 wide; esophagus 1,225 long and relatively thin; tail 65 long; vulva 1,825 from head, vagina 170 long, 100 wide. Male: 50.65 mm long, 440 wide; esophagus 980; tail 75; left spicule 450 (handle 190); right spicule 165; area rugosa 2,000 long, extended from 3,400 to 1,300 from tail extremity.

Figure 1

Dirofilaria ursi from Ursus americanus. (A–D) Female. (A) Transverse section at midbody, part of worm showing a lateral hypodermal chord, submedian muscles, and cuticular longitudinal crests. (B) Detail of 4 crests, longitudinal view. (C) Posterior region, tail with terminal rugosities, right lateral chord. (D) Vulva, ventral view, and vagina with 2 bends and chamber containing a few microfilariae in transverse sections. (E) Male, cuticular crests and area rugosa, right lateral view (pointed area is the lateral chord). (F–H) Blood microfilariae. (F) Anterior region, with nerve ring, orientation different from that of H. (G) Posterior region and anucleated filament; the R2, R3, and R4 are identified. (H) General morphology; nerve ring and excretory pore are identified. Scale bars in μ: A, C, D, 100; B, 30; E, 50; F, G, H, 20.

Immunohistology

Polyclonal and monoclonal anti-wsp antibodies and a commercially available anti-hsp 60 antibody were used to examine D. ursi for Wolbachia. Histologically, D. ursi presented very similarly to D. immitis, with a broad hypodermis and thick musculature (Fig. 2A). Only unfertilized eggs and early embryos were observed in the uterine branches of the examined mid-body fragments of D. ursi. Numerous Wolbachia endobacteria were detected in the hypodermis and the lateral chords. No staining was observed in the uterus or the musculature (Fig. 2B–F). Wolbachia were labeled by all antibodies used, with differing levels of background labeling. The same was observed for D. immitis (Fig. 2G–I). The highest background was detected with the mab HSP 60 antibody (Fig. 2G), while the antibodies directed against wsp were more specific. Reactivity of all anti-Wolbachia antibodies tested indicated that D. ursi contains Wolbachia endobacteria that can be labeled by immunohistology with the same antibodies used to detect Wolbachia in D. immitis.

Figure 2

Immunohistological detection of Wolbachia endobacteria in the hypodermis of Dirofilaria ursi (A–F) from American black bear and in Dirofilaria immitis (G–I) for comparison. (A) Transversal section showing multiple uterus sections, hypodermis, and a thick musculature; negative control, no primary antibody. (B) Granular staining of Wolbachia in the hypodermis using polyclonal antibodies directed against the Wolbachia surface protein of the endosymbiont of D. immitis (pab Di WSP). (C) Strong labeling of Wolbachia in the hypodermis using a monoclonal antibody raised against the Brugia malayi wsp (mab Bm WSP). (D–F) Consecutive cross-sections showing Wolbachia in the hypoderms stained with different antibodies. (D) polyclonal antibodies directed against the Wolbachia surface protein of the endosymbiont of Brugia pahangi (pab Bp WSP); (E) pab Di WSP; (F) mab Bm WSP. (G–I) Consecutive longitudinal sections showing muscles and Wolbachia in the lateral chords using various antibodies. (G) mab HSP 60; (H) pab Di WSP; (I) mab Bm WSP. Arrow, cuticle; arrowhead, Wolbachia; hy, hypodermis; ut, uterus; mu, musculature.

Sequence analysis and phylogenetic tree construction

Four 5s rDNA sequences amplified from D. ursi had 97–100% similarity and were distinguished by single nucleotide differences, mainly within the intergenic regions (data not shown), confirming previous observations of intergenic sequence variation within filarial species (Xie et al., 1994). Each sequence was most similar to orthologous sequences from D. immitis (E value <6e⁻⁷⁵) by sequence comparison using nucleotide level BLAST comparison ( http://www.ncbi.nlm.nih.gov/). The experiment was controlled by amplification and sequencing of D. immitis 5s rDNA, which was confirmed to be identical to D. immitis 5s rDNA sequences present in GenBank (data not shown). We carried out a phylogenetic analysis using 1 of the D. ursi 5s rDNA sequences with orthologous sequences from other filarial genera, including Dirofilaria, Onchocerca, Brugia, Wuchereria, Mansonella, Loa, and Litomosoides, with the intestinal roundworm Ascaris as an outgroup. The minimum evolution tree generated shows strong support for placement of the filarial worms collected from Wisconsin black bears into Dirofilaria (Fig. 3). A bootstrap consensus tree generated using maximum parsimony also grouped the D. ursi sequence with other Dirofilaria sequences (data not shown). As would be expected from their high sequence identity, the choice of D. ursi sequence did not alter the placement within the tree (data not shown). The D. ursi 5s rDNA sequences were deposited in GenBank, accessions GQ241942–GQ241945.

Figure 3

Minimum evolution tree based on an alignment of 5s rDNA intergenic sequences. Bootstrap confidence values (1,000 replicates) are shown as percentages. Values less than 50% are omitted. The units for the scale bar are substitutions per site. NCBI GI numbers are included after each species name. The Dirofilaria ursi sequence, with taxon name shown in bold font, was generated as part of this study. This analysis places D. ursi in the branching of D. (D.) immitis.

Gene fragments were successfully amplified using 4 of the 5 Wolbachia MLST primer pairs (gatB, coxA, fbpA, and ftsZ; GenBank accessions GQ217524, GQ217525, GQ217526, and GQ217523, respectively). No product was obtained with the standard hcpA primers or with alternative hcpA primers provided at the Wolbachia MLST website ( http://pubmlst.org/wolbachia/). A fragment of the wsp gene was also amplified (GenBank accession GQ217527). In all cases, sequences matching the consensus of the individually sequenced clones gave greater BLAST similarity to Wolbachia sequences in GenBank than the variant sequences that deviated from the consensus. The ftsZ sequence from this filarial endosymbiont groups with Wolbachia ftsZ sequences from D. immitis and D. repens, with high bootstrap values in a minimum evolution tree (Fig. 4). Similar results were obtained using maximum parsimony (data not shown). With the exception of ftsZ, there are very few Wolbachia sequences from filarial nematodes in GenBank that correspond to the genes comprising the MLST set. This is particularly true for supergroup C, where sequences exist solely for Wolbachia coxA from D. immitis and O. volvulus and Wolbachia fbpA from O. volvulus. In contrast, the MLST primers have been used extensively on Wolbachia from arthropods (Baldo, Dunning Hotop et al., 2006). For this reason, the top BLAST hits for gatB, coxA, and fbpA were to supergroup C sequences where available, but otherwise to Wolbachia from Brugia malayi (supergroup D) and from arthropods. Nonetheless, the sequences that we obtained are clearly from Wolbachia. The wsp gene has been sequenced from Wolbachia that infect a large number of diverse arthropod and filarial nematode hosts (Bazzocchi et al., 2000; Jeyaprakash and Hoy, 2000; Baldo, Dunning Hotop et al., 2006; Baldo and Werren, 2007). The Wisconsin D. ursi Wolbachia wsp sequence had the greatest similarity to wsp orthologs from other supergroup C Wolbachia and clearly grouped with those from D. immitis and D. repens in neighbor joining phylogenetic trees generated as part of the BLAST result page (data not shown).

Figure 4

Minimum evolution tree based on an alignment of Wolbachia ftsZ nucleic acid sequences. Bootstrap confidence values (1,000 replicates) are shown as percentages. Values less than 50% are omitted. The units for the scale bar are substitutions per site. NCBI GI numbers are included after each species name. The ftsZ sequence from Wolbachia of Dirofilaria ursi, with taxon name shown in bold font, was generated as part of this study. Letters to the right of the bracketed branches denote the Wolbachia supergroup. Branches are color-coded to match the color of the supergroup letters. This analysis places D. ursi in the branching of D. (N.) repens.