Material examined

A total of 70 digestive tracts belonging to L. maximus (including stomach, small intestine, large intestine, pancreas and liver) were examined for parasites. Fifteen specimens belonging to the Mammals Collection of Museo Argentino de Ciencias Naturales Bernardino Rivadavia (MACN) from 4 provinces of Argentina: Buenos Aires: San Cayetano (SC, n = 6), Salta: Dragones (DR, n = 1), Córdoba: Bialet Massé (BM, n = 3) and Entre Ríos: La Elisa (LE, n = 5). Fifty-five specimens were collected between 2012 and 2021 from 10 sites that belong to 3 provinces of Argentina: Buenos Aires (n = 30): Campo La Costa (LC, n = 1), Bahía Blanca (BB, n = 2), Establecimiento La Merced (LM, n = 2), ECAS (n = 12), Punta Indio (PI, n = 1), Punta Rasa (PR, n = 1), Islote del Puerto (IP, n = 1), Campo La Bombilla (LB, n = 10); Entre Ríos: Estancia Palmira de Carpinchorí (ER, n = 12); and Santiago del Estero: Estancia Los Quebrachitos (SE, n = 13) (Table 1, Figure 1). Bahía Blanca, Islote del Puerto and Campo La Bombilla were brought together under the acronym Southwest of the Province of Buenos Aires (SOBA).

Figure 1. Map of Argentina with sites of origin of Lagostomus maximus specimens studied. See data of localities in Table 1.

Table 1. Detail of Lagostomus maximus specimens examined from Argentina and ecological data on Lagostonema specimens

^a MACN = Mammals Collection from Museo Argentino de Ciencias Naturales Bernardino Rivadavia.

^b Sites of southwest of Buenos Aires Province (SOBA).

The digestive tracts were fixed in 10% formalin or preserved in 96% ethanol, and nematodes were localized under a stereo-microscope (Olympus SZ61-TR), collected and preserved in 70% or 96% ethanol for morphological and molecular studies.

Morphological analysis

A total of 62 Lagostonema specimens from 13 sites (Table 1) were cleared in lactophenol and studied under light microscopy (Olympus BX51). Drawings were made with the aid of a drawing tube. Measurements were recorded in micrometres (μm) and expressed as mean, standard deviation and range between parentheses. These measurements were compared with those published by Sutton and Durette-Desset (Reference Sutton and Durette-Desset1987) (Table 2). On the other hand, transverse sections obtained along the body of 18 Lagostonema specimens were mounted to study the synlophe under light microscopy (Olympus BX51). Transverse body sections were illustrated with the dorsal side of the worm oriented to the top of the page. Voucher specimens were deposited in the Helminthological Collection of Museo de La Plata (MLP-He), La Plata, Buenos Aires, Argentina.

Table 2. Main morphological features and measurements of Lagostonema specimens; measurements are presented in micrometres as mean values and standard deviations followed by range values in parentheses

dfae: distance from anterior end; dfpe: distance from posterior end.

^a Width at midbody.

^b n = 20.

^c n = 19.

^d n = 17.

^e n = 16.

^f n = 18.

^g n = 13.

^h n = 11.

ⁱ n = 15.

^j n = 105.

^k n = 8.

^l n = 9.

^m n = 7.

ⁿ n = 5.

^o n = 50.

A principal component analysis (PCA) was performed to explore the morphometric characteristics of Lagostonema specimens from different host populations (SOBA, ER, ECAS and SE). The analysis was carried out using the ggplot2 package R (R Core Team, 2022). A total of 62 specimens (31 males and 31 females) and 22 morphometric variables (11 for males and 11 for females) were included.

Molecular and phylogenetic analysis

Fourteen Lagostonema specimens stored in 96% ethanol and previously identified on morphological traits were used for the polymerase chain reaction (PCR) and sequencing. Genomic DNA from individual worms was extracted and purified using a commercial DNA extraction kit (Wizard® Genomic DNA Purification Kit, Promega, Madison, WI, USA) according to the manufacturer’s protocol for tissues, to 2 genomic fragments: ITS1 (to 9 specimens from ECAS, SOBA, ER and SE) and cox1 (to 5 specimens from ECAS, SOBA and SE). All the amplifications were performed in a Multigene Labnet International, Inc. thermocycler and the following mix: each 50 μL PCR contained 1× GoTaq Green Master Mix (Promega, Madison, WI), 0.4 μM of each primer and 1 μL of the extracted DNA. Fragments of ITS1 were amplified using the primers AngioF1674 (forward) and 58SR4 (reverse) described by Qvarnstrom et al. (Reference Qvarnstrom, Silva, Teem, Hollingsworth, Bishop, Graeff-Teixeira and Silva2010), with the following conditions: initial denaturation at 94°C for 5 min, 35 cycles of 94°C for 30 s, 54°C for 30 s and 72°C for 1 min, and final extension at 72°C for 3 min. Regarding cox1 gene marker fragments were amplified using the primers LCO 1490 (forward) and HCO 2198 (reverse) described by Sharma and Kobayashi (Reference Sharma and Kobayashi2014), with the following conditions: initial denaturation at 94°C for 5 min, 35 cycles of 94°C for 30 s, 46°C for 40 s and 72°C for 1 min, and final extension at 72°C for 10 min. The PCR products were checked on ethidium bromide-stained 1.5% Tris-Borate-EDTA using 0.8% agarose gels electrophoresis and examined by UV transillumination. All PCR products were purified and sequenced in both directions with amplifying primers (Macrogen, Seoul, Korea).

Consensus sequences were constructed and compared using the algorithm BLASTn to known sequences from GenBank, the National Center for Biotechnology Information database (https://www.ncbi.nlm.nih.gov). To obtain aligned sequences, the MUSCLE alignment method (Edgar, Reference Edgar2004) was used by MEGA 5 version 5.2 program (Tamura et al., Reference Tamura, Peterson, Peterson, Stecher, Nei and Kumar2011). To evaluate the similarity between different species obtained from GenBank, the number of differences between bases was analysed using the MEGA 5 version 5.2 program (Tamura et al., Reference Tamura, Peterson, Peterson, Stecher, Nei and Kumar2011). Phylogenetic trees were generated with 2 methods: Maximum Likelihood (ML) and Bayesian Inference (BI), using the PhyML package (Guindon and Gascuel, Reference Guindon and Gascuel2003), MEGA 5 program (Tamura et al., Reference Tamura, Peterson, Peterson, Stecher, Nei and Kumar2011) and MrBayes version 3.1.2 (Ronquist and Huelsenbeck, Reference Ronquist and Huelsenbeck2003), respectively. Species of Molineinae and other Molineidae available in GenBank were used as outgroups (Table 3).

Table 3. Sequences of Lagostonema specimens and other Molineinae/Molineidae species used for phylogenetic analyses (GenBank accession numbers)

Data analysis

Ecological parameters including prevalence (P), mean intensity (MI) and mean abundance (MA) were calculated for hosts and provinces (specimens housed at MACN were excluded) according to Bush et al. (Reference Bush, Lafferty, Lotz and Shostak1997).

Lagostonema ecasiense Sutton and Durette-Desset, Reference Sutton and Durette-Desset1987

General diagnosis: Small nematodes with body slightly coiled or not coiled. Cephalic vesicle present. In apical view: lips absent, buccal aperture rounded, 2 amphids, 4 external labial papillae and 4 cephalic papillae observed (Figure 2B). Excretory pore and deirids situated at approximately the same level, slightly in front of the end of the oesophagus (Figure 4E).

Figure 2. Light microscope photographs and drawings of Lagostonema ecasiense. Male. (A) Whole specimen with indications of the apical view (B) and the transverse sections made to study the synlophe (C–F). (B) Anterior end, apical view. (C–F) Cross sections of the synlophe in different regions of the body: (C) at oesophagus level, (D) at oesophago–intestinal junction, (E) at midbody, (F) in front of caudal bursa.

Synlophes (based on 10 males and 8 females): body with continuous cuticular ridges without struts, extending along the entire body with an axis of orientation coincident with the sagittal axis and directed from ventral to dorsal (Figures 2, 3).

Figure 3. Light microscope photographs and drawings of Lagostonema ecasiense. Female. (A) Whole specimen with indications of level of transverse sections made to study the synlophe. (B–I) Cross sections of the synlophe in different regions of the body: (B) at oesophagus level, (C) at oesophago–intestinal junction, (D) at midbody, (E) before vulva (anterior infundibulum), (F) behind vulva (posterior uterine branch), (G) distal part of intestine, (H–I) tail.

In both sexes, synlophe bears 9 ridges at level of muscular oesophagus, and 10 ridges both at level of oesophago–intestinal junction and at midbody, with 3 dorsal ridges, 5 ventral ridges and 2 lateral ridges (associated to the 2 lateral hypodermal cords) more developed (Figures 2C–E, 3B–D). In males, number of ridges increases progressively until reaching 15 (range: 12–15) in front of the caudal bursa (Figure 2F). In females, number of ridges increases progressively until reaching 14 at level of vulva; then progressively decreases to 5 ridges at level of tail (Figure 3E–I). In both sexes, behind midbody, lateral ridges decrease in size (Figures 2F, 3E–I).

Males (based on 31 specimens): The measurements are shown in Table 2. Caudal bursa subsymmetrical of type 2-1-2 with small dorsal lobe. Rays 2 the longest. Rays 4 very short. Rays 8 not reaching the extremities of the dorsal ray and arising from the base of this latter (Figure 4A). Dorsal ray divided into 2 sub-branches at its extremity, each sub-branch bearing 3 papillae: papilla 9 (external), papilla 10 (internal) and phasmid (middle). Subequal alate spicules divided into 3 points at their distal end, the latero-dorsal point being the longest (Figure 4B). Gubernaculum enlarged at its distal end and curved ventrally (Figure 4C). Genital cone bearing on its ventral lip the papilla zero and on its dorsal lip 2 rod-like papillae 7 (Figure 4D).

Figure 4. Lagostonema ecasiense. Male. (A) Caudal bursa, ventral view, the arrow indicates one phasmid (ph). (B) Spicules. (C) Gubernaculum. (D) Genital cone, ventral view. Female. (E) Anterior end, left lateral view, the arrow indicates the deirid (d). (F) Ovejector, right lateral view. (G) Posterior end, left lateral view. (H) egg.

Females (based on 31 specimens): The measurements are shown in Table 2. Didelphic (Figure 4F). Vulva in the posterior quarter of the body. Ovejector symmetrical (Figure 4F). Tail with distal spine and 2 sublateral tubercles (Figure 4G). Eggs oval, with thin shell, some morulated and other in gastrulation stage (Figure 4H).

Host:

Lagostomus maximus (Desmarest, 1817): Localities: specimens measured were from ECAS, SOBA, ER and SE (Table 2, the specimens from SE are refered as Lagostonema sp. in the table). Other specimens studied were from Buenos Aires Province: SC, LC, LM, PI and PR; Córdoba Province: BM; and Entre Ríos Province: LE.

Site of infection: small intestine and, secondarily, stomach.

Specimens deposited: MLP-He 8073, MLP-He 8074, MLP-He 8075, MLP-He 8076, MLP-He 8077, MLP-He 8078, MLP-He 8079 and MLP-He 8080.

Ecological data: The highest values of total P were registered for ER and SE. The highest values of MI and MA were registered for SE (Table 1).

Morphometric analysis

The PCA conducted to explore the morphometric characteristics between the Lagostonema specimens did not reveal groupings among the host populations studied (SOBA, ER, ECAS and SE), although a slight tendency towards separation of the SE specimens can be interpreted. In this sense, the ranges of most diagnostic characters (e.g., ratios such as BW/BL, EP/BL, SL/BL, Vulva/BL and TL/BL) are overlapped (Table 2, Supplementary Fig. S1).

Molecular and phylogenetic studies

Nucleotide sequence data of the rDNA (ITS1) and mtDNA (cox1) are reported and are available in GenBank (GenBank accession number, Table 3). The rDNA (ITS1) revealed 9 haplotypes, and their sequences were 528–534 base pairs (bp) (exclusive of the primers); G + C content ranged between 44% and 45%, while A + T content ranged between 29.9% and 31.5%. Multiple alignments of 12 ITS1 sequences from species in the subfamily Molineinae produced a data set of 549 characters. The maximum and minimum values of similarity among studied populations were observed between the isolates from ECAS and ER (98.36–99.45%), and ER/SOBA and SE (79.78–83.78% and 79.60–84.69%), respectively. The minimum and maximum values between the Lagostonema studied populations and the other 3 species studied were 63.20% concerning Durettenema spp. and 82.51% concerning Oswaldocruzia filiformis (Table 5).

Table 5. Intra- and inter-specific similarity percentage observed with ITS1 rDNA between Lagostonema specimens from different Lagostomus maximus populations and other species of Molineinae

^a Maximum value of similarity among Lagostonema studied populations.

^b Minimum value of similarity among Lagostonema studied populations.

^c Minimum value between Lagostonema studied populations and other Molineinae species.

^d Maximum value between Lagostonema studied populations and other Molineinae species.

The consensus tree showed 2 phylogenetic groups corresponding to genus Lagostonema and the 3 species of the Molineinae analysed, with good resolution (95 BI/90 ML). Considering the analysed populations of Lagostonema specimens, the formation of at least 2 robust clades was observed, corresponding to the haplotypes of ECAS (94 BI/95 ML) and ER (96 BI/100 ML). The position of the haplotypes from the southwest of Buenos Aires Province (SOBA) was unclear, but they were separated from the other subclades. In contrast, SE specimens formed a separate clade, clearly distinct from the other populations with high resolution (100 BI/100 ML) (Figure 5).

Figure 5. Phylogenetic tree of Molineinae species based on ITS1 rDNA region obtained with Maximum Likelihood (ML) and Bayesian Inference (BI).

The mtDNA (cox1) encoding gene revealed 5 haplotypes and their sequences were of 337 bp (exclusive of the primers); G + C content ranged between 29.9% and 31.5%, while the A + T content ranged between 67.9% and 70.1%. Multiple alignments of 11 cox1 sequences from species in the family Molineidae produced a data set of 337 characters. The maximum and minimum values of similarity between populations were observed between the isolates from SOBA and SE (98.51%), and SOBA and ECAS (88.72%–89.31%), respectively. The minimum and maximum values between Lagostonema specimens and the studied species belonging to other genera were 45.40% concerning Oswaldocruzia filiformis and 89.91% concerning Oswaldocruzia belenensis, respectively (Table 6).

Table 6. Intra- and inter-specific similarity percentage observed with cox1 mtDNA between Lagostonema specimens from different Lagostomus maximus populations and other species of Molineidae

^a Minimum values of similarity among Lagostonema studied populations.

^b Maximum value of similarity among Lagostonema studied populations.

^c Maximum value between Lagostonema studied populations and other Molineidae species.

^d Minimum value between Lagostonema studied populations and other Molineidae species.

The consensus tree showed that the haplotypes corresponding to Lagostonema specimens formed a clade with good resolution (97 BI/90 ML), being Oswaldocruzia belenensis the sister species. Considering the analysed populations of Lagostonema, a high genetic similarity was observed between the haplotypes of SE forming a separate subclade, following those of SOBA and ECAS (Figure 6).

Figure 6. Phylogenetic tree of Molineidae species based on cox1 mtDNA region obtained with Maximum Likelihood (ML) and Bayesian Inference (BI).