ABSTRACT
As part of a biannual health examination, coprological samples from 3-mo-old Central American river turtles, Dermatemys mawii (Gray, 1847) in a breeding program in Belize, Central America, revealed a previously undescribed coccidian (Apicomplexa) in 17 of 46 (37%) samples. Of 3 positive fecal samples transported to the University of Florida, coccidian oocysts were observed in 1 sample. Sporulated oocysts were measured and described, and using polymerase chain reaction (PCR), an approximately 400–base pair (bp) region of both the small subunit (18S) ribosomal RNA gene and 1,200-bp region of the internal transcribed spacer (ITS) gene were amplified in all 3 samples and their products were sequenced. For comparative value, the same PCR reactions and amplifications were performed on a fecal sample containing oocysts of Eimeria mitraria obtained from a red-eared slider, Trachemys scripta elegans. Results indicated a new eimerian in D. mawii, Eimeria grayi n. sp.
The Central American river turtle (Dermatemys mawii Gray, 1847) (Fig. 1) is a large, aquatic freshwater turtle known locally in Belize as the “hicatee.” It is the single genus and species within the monotypic family Dermatemydidae. Once abundant, the hicatee has limited distribution along the coastal lowlands of southern Mexico, northern Guatemala, and Belize (Rhodin et al., 2017). It is a relatively large-bodied species, with historical records of 60 cm (24 in.) straight carapace length and weights of 22 kg (49 lb); however, more recent records have found few individuals over 14 kg (31 lb) in México or 11 kg (24 lb) in Guatemala (Vogt et al., 2011).
After decades of overexploitation for its meat and eggs, the hicatee has been virtually eliminated from much of its former range in México; its status in Guatemala is unknown. A countrywide survey conducted in 2010 by The Turtle Survival Alliance (TSA; https://turtlesurvival.org/history-mission/) indicated the hicatee was heavily depleted in most of Belize, with healthy populations remaining in a few remote areas. Classified as Critically Endangered (facing an extremely high risk of extinction) by the IUCN Red List, it is included as a priority species in each printing of Turtles in Trouble (Stanford et al., 2018). The hicatee is considered one of the 25 most endangered tortoises and freshwater turtles by the Turtle Conservation Coalition (Stanford et al., 2018).
The TSA began to collaborate with the Belize Foundation for Research and Environmental Education (BFREE), to launch a multiprong conservation effort to halt the decline of the hicatee, following a 2010 survey. BFREE consists of 1,153 acres of privately owned and protected forested land and a biological field station strategically located at the foothills of the Maya Mountains. Working with multiple stakeholders, BFREE developed a conservation strategy throughout Belize. In 2013, the Hicatee Conservation and Research Center (HCRC) was formed at the BFREE Field Station, with a breeding program to return captive-bred turtles to the wild as a major objective. In 2014, breeding stock was acquired from confiscations from the Belize Fisheries Department, collections from the wild, and rehabilitated individuals. That same year, the first clutch of 8 eggs was deposited and, in June of 2015, the first captive-born turtles hatched at the HCRC. In each consecutive year since, there has been successful egg production and hatching, with a significant increase in the number of clutches and hatchlings.
Beginning in 2014, biannual health assessments have been conducted annually at the HCRC. Fecal samples were obtained from those turtles that would defecate during manual restraint, and wet mounts were examined using a light microscope. In September 2018, eimerian oocysts were identified in the feces of 17 of 46 (37%) 3-mo-old turtles. Fecal samples from 3 turtles were subsequently submitted to the University of Florida for identification and sequencing of coccidia in the samples. Here we report our findings including the identification of the first eimerian oocysts observed in a fecal sample from D. mawii. According to Duszynski and Morrow (2014), no coccidian parasites have been described in D. mawii.
MATERIALS AND METHODS
Background, turtles, and samples:
Adult hicatees at HCRC (16°33.326′N, 88°42.423′W), Belize, Central America are kept in 2 outdoor fenced-in ponds; Pond 1 is 28.7 m long × 14 m wide × 3.2 m deep with 23 adult turtles and Pond 2 is 20.1 m long × 24.1 m wide × 3.2 m deep with 22 adults. In addition to hicatees, an adult Meso-American slider (Trachemys venusta), a native species, shares Pond 2. Juvenile turtles (<12 mo old) were housed in groups of 10 that were kept at the HCRC laboratory in plastic-lidded tanks that measured 97.1 cm × 50.8 cm × 17.8 cm. Well water was used and ambient water temperatures ranged between 22.2 and 25.6 C.
Hicatees are herbivores and were fed primarily Ficus spp. and Paspalum paniculatum (Russell River Grass) and to a much lesser degree Cecropia peltata (Trumpet Tree) and Inga spp. Seasonally, fruits such as fig and various Belizean apples are offered. Recently, the diet of hatchlings and yearlings has been supplemented with a commercially available aquatic turtle diet (Mazuri Aquatic Turtle Diet, St. Louis, Missouri) in an attempt to prevent a “softening” of the shell that appeared in the 2–3-yr-old turtles.
During biannual health examination of turtles at BFREE in 2017 and 2018, oocysts were identified in feces. In December 2018, previously collected fecal samples from 3 individuals of 3-mo-old hicatees of unknown sex, that were previously found positive for coccidia, were transported to the University of Florida, College of Veterinary Medicine (UFCVM), for specific identification. The turtles ranged in weight from 36 to 106 g, straight carapace length (SCL) from 64 to 90 mm, straight plastron length (SPL) from 44 to 71 mm, straight width (SW) from 54 to 78 mm, and straight depth or thickness (SD) from 26 to 38 mm. All 3 turtles were derived from captive-bred and hatched hicatees at BFREE, and were approximately 3 mo of age at the time feces were collected. In addition, for comparative purposes, feces from a red-eared slider, Trachemys scripta elegans, collected in June 2018 from Crooked Creek at Yellville, Marion County, Arkansas (36°13′22.134″N, −92°40′45.8292″W) was examined for coccidia.
Fecal sample analysis and oocyst morphometrics:
Upon arrival at UFCVM, the fecal samples were examined by centrifugal fecal flotation using Sheather's sugar solution (sp. gr. 1.25) (Zajac and Conboy, 2012). Flotation samples were examined at ×400 using a Zeiss Axio Scope A1 compound microscope and an Axiocam 506 color camera (Carl Zeiss Microscopy, LLC, White Plains, New York), and when present, up to 15 sporulated oocysts were measured in micrometers (μm) using a calibrated ocular micrometer. Size measurements are means followed by ranges in parentheses. Sporulated oocysts were up to 30 days old when measured and photographed. Measurements of oocysts and sporocysts are as follows: oocyst length (L) and width (W), their ranges and ratios (L/W), micropyle (M), oocyst residuum (OR), polar granule(s) (PG), sporocyst (SP) length (L) and width (W), their ranges and ratio (L/W), Stieda body (SB), sub-Stieda body (SSB), para-Stieda body (PSB), sporocyst residuum (SR), sporozoites (SZ), sporozoite refractile bodies (SRB), and nucleus (N). A photosyntype of a sporulated oocyst was accessioned into the Harold W. Manter Laboratory of Parasitology (HWML), University of Nebraska-Lincoln, as HWML 216401. Turtle taxonomy follows the reptile database (Uetz et al., 2020).
Molecular biology:
Nucleic acids were extracted from feces of 3 hicatees found at BFREE to possess coccidian oocysts and from a fecal sample of a T. s. elegans containing oocysts of Eimeria mitraria using a DNeasy blood and tissue kit (Qiagen, Germantown, Maryland) following the manufacturer's instructions. An approximately 400-bp region of the small subunit (18S) ribosomal RNA gene was amplified as previously described (Garner et al., 2006). Briefly, 15 μl of a commercial master mix (Invitrogen, Waltham, Massachusetts), 1 μl each of 20 μM forward primer 1,135 (ACYATAAACTATGCCRACTAGA) and reverse primer 1,503 (CYTCCYTRCRTTARACACGCAA), and 3 μl of the extracted DNA were mixed and amplification reactions as follows were completed in a thermal cycler (Bio Rad T100; Bio Rad, Hercules, California): 94 C for 5 min, followed by 40 cycles of 94 C for 30 sec, annealing at 48 C for 1 min, 72 C for 1 min and then a final 7-min extension at 72 C. An approximately 1,200-bp region of the internal transcribed spacer (ITS)-1 gene, the 5.8S gene, and a portion of the ITS-2 region were amplified using a heminested reaction. The forward primer, EITSF (GATCGGAGGGTCCTGTGAA) was used with reverse primer EITSR1 (CCTCTCGAGGCTACAAYTCG) in the first-round PCR reaction, and then forward primer EITSF was used with reverse primer EITSR2 (GGACACGCGATTTTCACTTT) in the second round PCR reaction (Stoneburg et al., 2018). PCR reactions were mixed as above, and cycling conditions were as follows: 95 C for 2 min, followed by 40 cycles of 95 C for 30 sec, annealing at 53 C for 30 sec, 72 C for 1 min, and then a final 5-min extension at 72 C. PCR products, including a negative and previously identified positive control, were run on a 1.5% agarose gel with ethidium bromide and were visualized under ultraviolet light. Successfully amplified products of the expected length were excised and purified using the QIAquick® Gel Extraction kit (Qiagen) following the manufacturer's instructions and submitted to a commercial facility (Genewiz, South Plainfield, New Jersey) for sequencing. Final products were edited to remove primer sequences using commercial software (Geneious, Auckland, New Zealand), and analyzed using the nucleotide Basic Local Alignment Search Tool (BLASTn; https://blast.ncbi.nlm.nih.gov). Bayesian phylogenetic analysis was performed using the Mr. Bayes 3.2.6 plugin for Geneious with an HKY85 substitution model, gamma-distributed rate variation, and 4 chains of 2 × 106 generations with 25% burn-in (Huelsenbeck and Ronquist, 2001); Toxoplasma gondii (EF472967) was selected as an outgroup.
RESULTS
At the September 2018 BFREE health examination, coccidia were identified in feces of 17 of 46 (37%) 3-mo-old hicatees. Of the 3 fecal samples from this age group that were examined at the University of Florida, a uniform population of oocysts was identified in 1 sample that we describe herein as new.
DESCRIPTION
Eimeria grayi n. sp. (Figs. 2–5)
Description of sporulated oocyst:
Oocyst shape (n = 15): ellipsoidal; smooth, thin-walled; L × W: 30.4 (26–35) × 15.2 (13–17), L/W: 2.0 (1.7–2.5); M, OR, PG: all absent. Distinctive feature of oocyst: 3 conical projections (2.1–3.5 long) present on 1 end, with the oocyst wall forming a broadly pointed end on the opposite pole.
Description of sporocyst and sporozoites:
SP: (n = 4); shape: elongate–ellipsoidal, with a smooth single-layered wall; L × W: 13.7 × 7.5 (12–19 × 6–12), L/W 1.8 (1.7–2.2); SR: sporocyst residuum, coarsely granular, and scattered; SZ: banana-shaped, 14.2 × 3.6 (14–15 × 3–4) in situ; N visible, slightly posterior to midpoint of SZ. Distinctive feature of SP: slightly pointed at 1 end with a distinct SB, SR of only a few globules, and a SRB in each SZ.
Taxonomic summary
Type host:
Central American river turtle, Dermatemys mawii Gray, 1847 (Testudines: Dermatemydidae). Collected 11 August and 11 November 2018. Host photovouchers: University of Florida (UF) 191862-191866.
Type and only locality:
Belize Foundation for Research and Environmental Education, Mile Marker 58, Southern Highway, Belize, Central America (16°33.326′N, 88°42.423′W).
Prevalence:
1/3 (33%) based on oocyst identification in samples; 3/3 (100%) based on PCR and sequencing of the 18S rRNA and ITS genes.
Materials deposited:
Photosyntype of a sporulated oocyst is deposited in the Harold W. Manter Laboratory of Parasitology (HWML), University of Nebraska, as HWML 206401.
ZooBank registration:
urn:lsid:zoobank.org:act:B7C62C80-DF94-49F0-A73F-586C1FB2B578.
Etymology:
The specific epithet is named in honor of the British naturalist, John Edward Gray (1800–1875), who described the host in 1847.
Molecular biology:
All 3 fecal samples had similar content of the 18S rRNA and ITS genes. After primer editing, a 347-bp segment of the 18S rRNA gene was determined for the hicatee coccidian (GenBank accession MW538581). BLASTn results identified 99.4% sequence identity to several apicomplexan organisms, including Caryospora-like sp. US3 (MN450817) from a green sea turtle (Chelonia mydas), Caryospora cheloniae genotype 1 (KT361639) from Ch. mydas, and multiple lizard Schellackia spp. The hicatee coccidian was 99.7% identical to a 347-bp segment of the 18S rRNA gene of the reference sample of E. mitraria (GenBank accession MW538549). An 841-bp segment of the ITS region was determined for the hicatee coccidian and reference sample of E. mitraria (GenBank accessions MW538550 and MW538533, respectively), with 75.2% sequence identity to each other. Bayesian phylogenetic analysis placed the hicatee coccidian in a clade with Eimeria collieie, E. mitraria, Eimeria arnyi, and 2 coccidians of green sea turtles (Ca. cheloniae and Caryospora-like sp. US3) with a posterior probability of 0.89 (Fig. 6).
Remarks
The oocysts being passed by the hicatee possessed multiple conical projections with 3 projecting from 1 pole and a broader-based projection from the opposite pole (Figs. 2–5). To date, the 7 previously described oocysts of Testudines having mitra-like conical projections or irregular surfaces from at least 1 end of their oocyst are (1) Eimeria amazonensis from the red-footed tortoise, Chelonoidis (formerly Geochelone) carbonaria from Brazil (Lainson et al., 2008); (2) Eimeria hynekprokopi from the Indochinese box turtle, Cuora galbinifrons from Vietnam (Široký and Modrý, 2010); (3) Eimeria iversoni from a captive Galapagos tortoise, Chelonoidis sp. (McAllister et al., 2014); (4) Eimeria jirkamoraveci in the Neotropical chelid turtle Mesoclemmys (previously Batrachemys) heliostemma (Široký et al., 2006); (5) E. mitraria originally described from the Asian Chinese three-keeled pond turtle, Mauremys (formerly Chinemys) reevesii and subsequently described in multiple species of aquatic turtles on 3 continents (Laveran and Mesnil, 1902; Duszynski and Morrow, 2014); (6) Eimeria motelo from the yellow-footed tortoise, Chelonoidis (formerly Geochelone) denticulata, from Peru (Hurková et al., 2000); and (7) Eimeria stylosa in the red-eared slider from Texas (McAllister and Upton, 1989). Overall, oocysts of E. grayi are considerably larger than other coccidians with surface projections (Table I).
DISCUSSION
McAllister and Upton (1989) were the first to present a summation of the coccidian parasites of the Order Testudines; they reported over 30 species of Eimeria and a single species of Isospora. More recently, Duszynski and Morrow (2014) summarized the coccidian parasites of turtles of the world. They listed 66 species of Eimeria, 3 species of Isospora, and a single species each of Caryospora and Sarcocystis. However, to date, there are no coccidians known from the only extant member of the family Dermatemydidae, D. mawii. In addition, the only coccidian known from any turtle in Belize is Eimeria pseudemydis (Lainson, 1968), originally described from the emydid ornate slider, Trachemys ornata. Because D. mawii is severely threatened across its range and is listed as Critically Endangered by the IUCN Red List (Vogt et al., 2006) based on widespread, dramatic, and ongoing population declines, it is important to gain knowledge about its parasites to help mitigate these negative concerns.
During 2017–2018 there was a die-off of 3-mo-old hicatees at BFREE. Although no specific cause could be determined, in examinations, coccidia were identified in their feces. In these examinations, 17 of 46 (37%) 3-mo-old turtles were positive for coccidia. Several coccidia in aquatic turtles are known to result in severe clinical disease and pathology. For example, sporulated oocysts were identified in captive Indo-Gangetic flap shelled turtle (Lissemys andersonii) that had disseminated visceral coccidiosis; 2 distinct Eimeria spp. were identified in 1 case (Helke et al., 2006). In addition, Caryospora-like coccidia were associated with an epizootic of green turtles off the coast of the southeastern United States (Stacy et al., 2019), and 2 distinct coccidian genotypes were associated with mass mortalities in green turtles off the coast of southeast Queensland, Australia (Chapman et al., 2016). Unfortunately, with the 2017–2018 die-off of hicatees at BFREE, although 22 turtles in various states of postmortem change were necropsied in Belize, tissues were not found to be suitable for histopathology. It is currently unknown whether the coccidia identified in these turtles were responsible for the mortality event seen at BFREE.
Historically, identification of Eimeria spp. has been based largely on host species, oocyst morphological features, pathological changes in the host, and geographic distribution (Duszynski and Wilber, 1997; Tenter et al., 2002). Although eimerian parasites were generally considered to be highly host specific (Duszynski, 1986), strict host specificity in reptiles has been questioned (McAllister and Upton, 1989) and exceptions to host specificity have been reported in mammals (Zhao and Duszynski, 2001; Zhao et al., 2001). In 1 of the ponds with adult hicatees is a Meso-American slider. Multiple attempts at capturing this turtle for fecal analysis were unsuccessful and we do not know if it shares coccidia with hicatees. Additionally, fecal samples need to be collected from wild hicatees to determine if they are the primary host of E. grayi.
Because some species of Eimeria are morphologically identical and cannot be distinguished using microscopy, molecular tools are needed to identify and establish phylogenetic relationships of Eimeria spp. accurately (Tenter et al., 2002). Yang et al. (2015) conducted molecular analysis at 3 loci: the 18S and 28S rRNA, and the mitochondrial cytochrome oxidase gene (COI) in reporting a new eimerian, E. collieie in the Western long-necked turtle (Chelodina colliei), a species native to Australia. At the 18S rRNA locus, E. collieie shared 96.4% and 98.3% genetic similarity to Eimeria ranae (GenBank accession number: EU717219) and E. arnyi (AY613853), respectively. At the 28S rRNA locus, E. collieie shared the highest (91.6%) genetic similarity to Eimeria papillata (GenBank accession number: GU593706) from chickens, and phylogenetic analysis at this locus placed E. collieie in a separate clade. Additional sequence data at these and other gene loci are needed to better understand the phylogenetic relationships of the Eimeria species of Testudines. Because the hicatee is the only member of its family, sequence data from proposed E. grayi n. sp. should provide important information about an eimerian in isolated populations in its limited range in Central America.
ACKNOWLEDGMENTS
The authors assert all applicable international, national, and/or institutional guidelines for the care and use of animals were followed. The Arkansas Game and Fish Commission issued a Scientific Collecting Permit to CTM. The authors thank Dr. Ellis C. Greiner for technical help and critical evaluation of this manuscript. Thanks also to Dr. Gabor Racz and Dr. Scott L. Gardner (HWML) for expert curatorial assistance. We also thank Thomas Pop and staff at BFREE, Belize, Central America, Nichole D. Bishop, Department of Wildlife Conservation and Ecology, University of Florida, for help in collecting and transporting fecal samples from hicatees and Dr. Coleman Sheehy and Kathryn Daly, Florida Museum of Natural History, for providing accession numbers (UF 191862-191866) for images of hicatees at BFREE. Research was conducted with the approval of the Belize Ministry of Fisheries, Forestry, the Environment, and Sustainable Development, under the Belize Fisheries Department (permit 00026-18), entitled, “Investigations into the Captive Management and Reproductive Biology of the Central American River Turtle, Dermatemys mawii, in Belize.”
LITERATURE CITED
Author notes
Version of Record, first published online with fixed content and layout, in compliance with ICZN Arts. 8.1.3.2, 8.5, and 21.8.2 as amended, 2012. ZooBank publication registration: urn:lsid:zoobank.org:pub:0AE4E6E3-3799-4FAC-8501-3AD2F969E369.