Your search keyword '"DNA, Helminth analysis"' showing total 790 results

1. Comparison of three LAMP protocols for the simultaneous detection of DNA from species that produce cystic echinococcosis.

Author

Avila HG and Periago MV

Subjects

Animals, Sensitivity and Specificity, Molecular Diagnostic Techniques methods, Molecular Diagnostic Techniques veterinary, Feces parasitology, Echinococcosis veterinary, Echinococcosis diagnosis, Echinococcosis parasitology, Nucleic Acid Amplification Techniques methods, Nucleic Acid Amplification Techniques veterinary, Echinococcus granulosus genetics, Echinococcus granulosus isolation & purification, DNA, Helminth analysis

Abstract

Cystic echinococcosis (CE) is a zoonotic parasitic disease caused by species of the Echinococcus granulosus sensu lato complex. Different types of canids may act as definitive hosts by eating raw viscera infected with fertile hydatid cysts. The intermediate host (mainly ungulates) and humans acquire the infection through the fecal oral route (i.e. egg ingestion). Globally, more than 1 million people are affected by CE, causing a loss of 1-3 million disability-adjusted life years (DALYs) and a financial burden of US$ 3 billion annually. Loop mediated isothermal amplification (LAMP) protocols promise to be a useful tool to detect DNA, providing a low cost and thermocycle-free methodology. Given that surveillance for CE can be performed in feces from canids or other environmental matrixes contaminated with eggs, the characteristics of a LAMP protocol would favor implementation in endemic areas with basic resources. Herein, we compared three LAMP protocols for the simultaneous detection of E. granulosus s.l. species that cause CE. This comparation was carried with DNA obtained from different stages of E. granulosus s.l. Two of these are newly developed protocols that showed good analytical sensitivity and specificity. In both cases, the use of malachite green dye to directly visualize the test result was possible. From these two new LAMP protocols, one had better values for the detection of DNA from different types of E. granulosus s.l. DNA samples. Therefore, through this study, we provide a low-cost new tool for DNA detection of E. granulosus s.l. in poorly equipped laboratories from endemic areas., Competing Interests: Declaration of Competing Interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper. Conflict of interest The authors declare that no conflict of interest exist., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

2. Paronatrema davidbowiei n. sp. (Trematoda: Syncoeliidae), a new parasite of the pelagic thresher (Alopias pelagicus) and its phylogenetic relationships within the suborder Hemiurata Skrjabin & Guschanskaja, 1954.

Author

Santoro M, Occhibove F, López-Verdejo A, Rojas A, and Solano-Barquero A

Subjects

Animals, RNA, Ribosomal, 28S genetics, RNA, Ribosomal, 28S analysis, Costa Rica, Gills parasitology, DNA, Ribosomal analysis, DNA, Helminth analysis, Perciformes parasitology, Bayes Theorem, Phylogeny, Trematoda classification, Trematoda genetics, Trematoda anatomy & histology, Trematode Infections veterinary, Trematode Infections parasitology, Fish Diseases parasitology, Microscopy, Electron, Scanning veterinary

Abstract

A new species of hemiurid trematode found on the gills and in the aorta of the pelagic thresher Alopias pelagicus from the eastern Pacific, off Costa Rica, is described based on an integrative taxonomic approach that includes the use of light and scanning electron microscopy, and 28S rDNA sequencing. Phylogenetic analysis was also performed to explore, for the first time, the relationships of a member of the subfamily Otiotrematinae within the suborder Hemiurata. Paronatrema davidbowiei n. sp. can be distinguished from the congeners by having tegumental spines on the dorsal surface of the forebody, papillae on the oral sucker, and different morphology or number of testicular follicles. BLAST analysis revealed that sequences of Paronatrema davidbowiei n. sp. had the highest degree of similarity with Hirudinella spp. (Hirudinellidae). Results from Maximum Likelihood and Bayesian phylogenetic analyses, returning trees with the exact same topology and strong branch support, distinguished between the two superfamilies included in the suborder Hemiurata: Azygioidea and Hemiuroidea. Our analysis placed the new species in a clade with Copiatestes filiferus, the only existing sequence of the family Syncoeliidae., Competing Interests: Declaration of competing interest The authors declare that there is no conflict of interest., (Copyright © 2024. Published by Elsevier B.V.)

Published

2024

3. An advance in the understanding the systematics of Echinochasmus Dietz, 1909 and Stephanoprora Odhner, 1902 (Digenea: Echinochasmidae), with the description of a new species of Echinochasmus from the Neotropical region of Mexico.

Author

Islas-Ortega AG, Aldama-Prieto Y, Sereno-Uribe AL, and García-Varela M

Subjects

Animals, Mexico, Trematoda classification, Trematoda anatomy & histology, Trematoda genetics, Trematoda isolation & purification, Birds parasitology, DNA, Ribosomal Spacer analysis, Bird Diseases parasitology, Argentina, DNA, Helminth analysis, RNA, Ribosomal, 28S analysis, RNA, Ribosomal, 28S genetics, Phylogeny, Trematode Infections parasitology, Trematode Infections veterinary

Abstract

Echinochasmids are a group of globally distributed digeneans, and the adults are found in the intestines of birds, mammals and reptiles. In the Neotropical region of Mexico, adult specimens were obtained from seven fish-eating bird species in six localities, whereas specimens of Stephanoprora aylacostoma were obtained experimentally in Argentina. Morphologically, the new specimens from the Neotropical region of Mexico were identified as Stephanoprora uruguayense and an undescribed species of Echinochasmus. Sequences for two nuclear (large subunit (28S) and internal transcribed spacer from DNA ribosomal (ITS1-5.8S-ITS2)) molecular markers were generated and analysed together with other sequences downloaded from GenBank. The phylogenies obtained with each molecular marker indicated that Echinochasmus is paraphyletic and agreed with previous phylogenetic studies. The first cluster included the type species (E. coaxatus, which has 24 head-collar spines) plus three congeneric species. The second cluster contained species of Echinochasmus plus Stephanoprora, including the species analysed herein, S. uruguayense, S. aylacostoma (with 22 head-collar spines) and Echinochasmus sp. (with 20 head-collar spines), which formed three independent subclades, allowing us to recognize a lineage that was described morphologically as a new species. Echinochasmus ostrowskiae n. sp. can be distinguished from its congeners by having a head collar with 20 spines in a single row, seven spines on each edge and three angle spines, and a pharynx with an irregular edge and by the body, egg and collar spine sizes. Additionally, new host and locality records for S. uruguayense are presented, expanding its geographical distribution range in the Americas., Competing Interests: Declaration of competing interest The authors declare there are no conflicts of interest., (Copyright © 2024 The Authors. Published by Elsevier B.V. All rights reserved.)

Published

2024

4. First report and molecular characterisation of an adult liver fluke (Fasciola hepatica) in a brown bear (Ursus arctos) in Türkiye.

Author

Gunyakti Kilinc S, Kesik HK, Celik F, and Simsek S

Subjects

Animals, Turkey, Electron Transport Complex IV analysis, Electron Transport Complex IV genetics, DNA, Helminth analysis, Phylogeny, Male, Polymerase Chain Reaction veterinary, Liver parasitology, Ursidae parasitology, Fasciola hepatica genetics, Fasciola hepatica isolation & purification, Fascioliasis veterinary, Fascioliasis parasitology

Abstract

Fascioliasis, caused by the parasite Fasciola hepatica, is a worldwide zoonotic disease that can have serious consequences for livestock, certain wild animals and humans. This study was conducted to morphologically and molecularly characterise a F. hepatica isolate from a brown bear. After examination of the internal organs, a Fasciola sp. isolate was obtained from the bile ducts of the liver. The adult parasite was morphologically analysed under a stereomicroscope and identified as F. hepatica. Measurements of body length, body width and ventral sucker area were then recorded. After isolation of the genomic DNA, a partial gene of the mitochondrial cytochrome oxidase subunit 1 (mt-CO1) was amplified by PCR. The amplified mt-CO1 PCR products were sequenced by one-way sequence analysis. According to the BLAST search results, the sequence of the isolate was identified as F. hepatica. In conclusion, this is the first report on the occurrence of F. hepatica in brown bears and the molecular characterisation of the isolate., Competing Interests: Declaration of competing interest The authors declare no conflict of interest., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

5. Gray foxes (Urocyon cinereoargenteus) as natural definitive hosts of Paragonimus mexicanus.

Author

Conejo-Chacón A, Robleto-Quesada J, Solano-Barquero A, and Rojas A

Subjects

Animals, Costa Rica, DNA, Helminth analysis, Disease Reservoirs parasitology, Disease Reservoirs veterinary, Bayes Theorem, Foxes parasitology, Paragonimiasis veterinary, Paragonimiasis parasitology, Paragonimiasis epidemiology, Phylogeny, Paragonimus isolation & purification, Paragonimus classification, Feces parasitology

Abstract

Paragonimus mexicanus is a trematode that causes pulmonary and extrapulmonary infections in humans, characterized by chest pain, dyspnea, fever, and weight loss. The detection of Paragonimus spp. is primarily achieved through the microscopic observation of eggs in feces, sputum, and pleural fluid. Paragonimus mexicanus has been found in various wild animals, including dogs, cats, raccoons, and opossums. Although the reservoirs of P. mexicanus in Costa Rica are unknown, this study analyzed fecal samples from gray foxes (Urocyon cinereoargenteus) using microscopic and molecular methods. In the morphological analysis, characteristic eggs of the genus Paragonimus were identified. DNA was extracted from fecal samples, and a fragment of the ITS2 loci of trematodes was amplified, which showed a 100 % similarity with P. mexicanus metacercariae from crabs in Ecuador. Then, a Bayesian inference phylogenetic analysis was performed with the obtained data and pre-existing sequences of P. mexicanus found in America, showing that our sequence clustered firstly with others from Colima and Veracruz (Mexico), and Ecuador, while a second cluster contained sequences from Chiapas (Mexico), Ecuador, and Guatemala. These results provide evidence of the presence of P. mexicanus in the gray fox and suggest its role as a possible new wild reservoir, which could have zoonotic implications for the infection of other animal species and humans. Additionally, our phylogenetic analysis reveals low genetic differentiation among the compared P. mexicanus populations and the possibility of additional Paragonimus species currently classified as P. mexicanus. The finding of this parasite in our country, together with comparisons with previous studies, highlights the complex evolutionary history and population dynamics of P. mexicanus., Competing Interests: Declaration of competing interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

6. Molecular characterization of Fasciola hepatica obtained from cattle and horse in Central Chile.

Author

Cabrera G, Cabezas C, Estay-Olea D, Stoore C, Baquedano MS, Paredes R, and Hidalgo C

Subjects

Animals, Cattle, Chile epidemiology, Horses parasitology, Phylogeny, DNA, Helminth analysis, DNA, Helminth genetics, Fasciola hepatica genetics, Fasciola hepatica isolation & purification, Cattle Diseases parasitology, Cattle Diseases epidemiology, Fascioliasis veterinary, Fascioliasis parasitology, Fascioliasis epidemiology, Horse Diseases parasitology, Horse Diseases epidemiology, Genetic Variation, Haplotypes

Abstract

Liver fluke infection, caused by the trematode Fasciola hepatica, is a parasitic zoonotic disease affecting various mammals, including humans, and has significant implications for public, animal, and ecosystem health. This study provides the first genetic characterization of F. hepatica in Chile, focusing on the complete mitochondrial gene cox1. Samples were collected from two different host species: cattle and horses. Our findings revealed that 70 % of detected haplotypes were found in either cattle or horses, which coincides with their geographical origin. Interestingly, the use of full-length sequences resulted in the identification of 80 % unique sequences, whereas this reduced to 45 % when analyzing the traditionally used short sequences. This underestimation of genetic diversity suggests that broader sequencing efforts might be essential for a more accurate understanding of F. hepatica genetic landscape. This research underscores the importance of understanding the genetic variability in parasites to improve strategies for disease control and treatment., Competing Interests: Declaration of competing interest The authors have no competing interests to declare that are relevant to the content of this article., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

7. Rapid on-site detection of echinococcosis and schistosomiasis based on RPA.

Author

Tian L, Shi Y, Yang Y, and Wang Y

Subjects

Humans, Animals, Schistosomiasis diagnosis, Nucleic Acid Amplification Techniques methods, Polymerase Chain Reaction, Sensitivity and Specificity, Recombinases, DNA, Helminth analysis, Echinococcosis diagnosis

Abstract

Background: Echinococcosis and schistosomiasis, caused by parasitic worms, pose significant threats to millions of people in the world. Rapid and effective pathogen detection and epidemic control by public health authorities are urgently needed., Objectives: In this study, we aimed to develop rapid on-site detection method to detect echinococcosis and schistosomiasis., Methods: Recombinase polymerase amplification (RPA) was utilised to examine its efficacy of detection of echinococcosis and schistosomiasis., Findings: The detection probes for RPA were created through comparing parasitic genomes from international genomic data and the sequences generated by our group. We established an optimised RPA on-site testing platform, which significantly reduces the detection time (less than 30 min) and simplifies the operation (free of expensive equipment) as compared to traditional polymerase chain reaction (PCR) method., Main Conclusions: This RPA detection platform in our study for identifying echinococcosis or schistosomiasis pathogens would be greatly applicable for epidemic investigation, border screening, and early clinical diagnosis.

Published

2024

8. Rapid and Direct Detection of the Stubby Root Nematode, Paratrichodorus allius, from Soil DNA Extracts Using Recombinase Polymerase Amplification Assay.

Author

Goraya M and Yan G

Subjects

Animals, Nucleic Acid Amplification Techniques methods, Recombinases metabolism, Recombinases genetics, Plant Roots parasitology, DNA, Helminth genetics, DNA, Helminth analysis, Plant Diseases parasitology, Nematoda genetics, Soil parasitology, Soil chemistry

Abstract

The stubby root nematode, Paratrichodorus allius, is one of the most important plant-parasitic nematodes. Besides root feeding, P. allius also transmits the Tobacco rattle virus in potatoes, which causes corky ringspot disease. Rapid detection of P. allius is key for efficient management. This study was conducted to develop a real-time recombinase polymerase amplification (RPA) assay that is capable of detecting P. allius directly in DNA extracts from soil using a simple portable device in real time. A fluorophore-attached probe was designed to target the internal transcribed spacer (ITS)-rDNA of P. allius and was used along with primers designed previously. The real-time RPA assay had the ability to detect P. allius DNA extracted directly from infested soil with a sensitivity of one-sixteenth portion of a single nematode. This RPA assay was specific, as it did not produce positive signals from non-target nematodes tested. The real-time RPA was found to be rapid as it could even detect P. allius in as little as 7 min. Testing with 15 field soil samples validated the RPA assay developed in this study. This is the first report of P. allius detection directly from soil DNA using real-time RPA and is the fastest method for P. allius detection in soil to date.

Published

2024

9. Soil surveillance for monitoring soil-transmitted helminths: Method development and field testing in three countries.

Author

Manuel M, Amato HK, Pilotte N, Chieng B, Araka SB, Siko JEE, Harris M, Nadimpalli ML, Janagaraj V, Houngbegnon P, Rajendiran R, Thamburaj J, Kaliappan SP, Sirois AR, Walch G, Oswald WE, Asbjornsdottir KH, Galagan SR, Walson JL, Williams SA, Luty AJF, Njenga SM, Ibikounlé M, Ajjampur SSR, and Pickering AJ

Subjects

Humans, Animals, Kenya epidemiology, DNA, Helminth genetics, DNA, Helminth analysis, India epidemiology, Helminths isolation & purification, Helminths genetics, Helminths classification, Male, Female, Child, Necator americanus isolation & purification, Necator americanus genetics, Prevalence, Adolescent, Child, Preschool, Ascariasis epidemiology, Ascariasis diagnosis, Ascariasis parasitology, Ancylostoma isolation & purification, Ancylostoma genetics, Trichuriasis epidemiology, Trichuriasis diagnosis, Trichuriasis parasitology, Adult, Epidemiological Monitoring, Sensitivity and Specificity, Trichuris isolation & purification, Trichuris genetics, Soil parasitology, Feces parasitology, Helminthiasis epidemiology, Helminthiasis diagnosis, Ascaris lumbricoides isolation & purification, Ascaris lumbricoides genetics

Abstract

Background: One-fifth of the global population is infected with soil-transmitted helminths (STH). Mass drug administration (MDA) with deworming medication is widely implemented to control morbidity associated with STH infections. However, surveillance of human infection prevalence by collecting individual stool samples is time-consuming, costly, often stigmatized, and logistically challenging. Current methods of STH detection are poorly sensitive, particularly in low-intensity and low-prevalence populations., Methodology/principal Findings: We aimed to develop a sensitive and specific molecular method for detecting STH DNA in large volumes of soil (20 g) by conducting laboratory and proof of concept studies across field sites in Kenya, Benin, and India. We collected human stool (n = 669) and soil (n = 478) from 322 households across the three study sites. We developed protocols for DNA extraction from 20 g of soil and qPCR to detect Ascaris lumbricoides, Trichuris trichiura, Necator americanus, and Ancylostoma duodenale. Agreement between detection of STH via qPCR, digital droplet PCR (ddPCR), and microscopy-based methods was assessed using the Cohen's Kappa statistic. Finally, we estimated associations between soil characteristics and detection of STH in soil by qPCR, as well as between STH detected in soil and STH detected in stool from matched households, adjusting for soil characteristics. The overall prevalence of STH in soil by qPCR was 31% for A. lumbricoides, 3% for T. trichiura, and 13% for any hookworm species. ddPCR and qPCR performed similarly. However, there was poor agreement between STH detected in soil by qPCR versus light microscopy. Microscopy underestimated the prevalence of A. lumbricoides and N. americanus and overestimated T. trichiura. Detection of an STH species in household soil was strongly associated with increased odds of a household member being infected with that same species., Conclusions/significance: Soil surveillance for STH has several benefits over stool-based surveillance, including lower cost and higher success rates for sample collection. Considering that delivery of MDA occurs at the community level, environmental surveillance using molecular methods could be a cost-effective alternate strategy for monitoring STH in these populations., Competing Interests: The authors have declared that no competing interests exist., (Copyright: © 2024 Manuel et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.)

Published

2024

10. First molecular identification of Haemonchus contortus (Nematoda: Trichostrongylidae), a blood-sucking gastric nematode of artiodactyles, in the ground beetle Carabus granulatus (Coleoptera: Carabidae).

Author

Werszko J, Wilamowski K, Kraszewska O, Bakier S, and Pyziel AM

Subjects

Animals, Poland, DNA, Helminth analysis, Sequence Analysis, DNA, Phylogeny, Molecular Sequence Data, Base Sequence, Bison, Coleoptera parasitology, Haemonchus genetics, Haemonchus classification

Abstract

Among gastrointestinal nematodes, Haemonchus contortus (Rudolphi) Cobb (order Strongylidae; family Trichostrongylidae) is one of pathogenic and economic importance in domestic and wild ruminants, including the European bison, Bison bonasus Linnaeus (order Cetartiodactyla; family Bovidae); a species on the International Union for Conservation of Nature's Red List of Threatened Species. Carabus granulatus Linnaeus (order Coleoptera; family Carabidae) is one of the most prevalent species of ground beetle, inhabiting a wide range of terrestrial ecosystems in Poland. Twenty-six ground beetles of this species inhabiting the Białowieża Primeval Forest in eastern Poland were screened for the presence of DNA of pathogenic gastrointestinal nematodes of ruminants. Extracted DNA was sequenced and compared to reference sequences. In six insects, the presence of H. contortus DNA was detected. The obtained nucleotide sequences were homologous to each other and to the majority of the published DNA sequences of H. contortus isolates. The sequences were also identical to a sequence of H. contortus isolated from European bison in Poland. The study provides the first molecular evidence of the presence of H. contortus DNA in C. granulatus. The finding suggests that ground beetles may play a role in the transmission dynamics of this parasite., (© 2024 The Authors. Medical and Veterinary Entomology published by John Wiley & Sons Ltd on behalf of Royal Entomological Society.)

Published

2024

11. Description of three new species of Gyrodactylus von Nordmann, 1832 (Monogenea: Gyrodactylidae) on bitterling fishes (Acheilognathinae) from China.

Author

Jin X, Cheng H, Li M, Zou H, Cai J, Amoah K, Li W, and Wang G

Subjects

Animals, China, RNA, Ribosomal, 18S analysis, Cyprinidae parasitology, DNA, Ribosomal Spacer analysis, DNA, Helminth analysis, Lakes parasitology, Platyhelminths classification, Platyhelminths anatomy & histology, Platyhelminths isolation & purification, Platyhelminths genetics, Fish Diseases parasitology, Trematode Infections parasitology, Trematode Infections veterinary, Trematoda classification, Trematoda anatomy & histology, Trematoda genetics, Trematoda isolation & purification, Phylogeny

Abstract

Three new species of Gyrodactylus are described from three species of bitterling in Donghu Lake, China: Gyrodactylus ocellorhodei n. sp. from Rhodeus ocellatus; G. sinenorhodei n. sp. from Rhodeus sinensis; and G. acheilorhodei n. sp. from Acheilognathus macropterus. All the three new species showed similar opisthaptor morphology, especially the marginal hooks: all had a slender and perpendicular sickle shaft, and flat sickle base with distinct heel and inner arch which was different from the G. rhodei-group species parasitic on bitterling. Multivariate analyses based on hamulus and marginal hooks suggested that these three new species cannot be completely distinguished, despite some morphology divergence observed in certain less reliable morphometric features, such as hamulus root length, ventral bar total length and process shape. These three new species shared an identical 18S ribosomal RNA gene sequence, while the variation in the Internal Transcribed Spacers (ITS1-ITS2) sequence among them (8.4-11.2%, K2P) far exceeded the 1% ITS sequence difference that had been suggested as a threshold for species delimitation of Gyrodactylus. Phylogenetic analysis based on ITS1-ITS2 showed that all these sequenced Gyrodactylus spp. parasitic on the subfamily Acheilognathinae host formed a monophyletic group. However, a clear differentiation (18.9-20.9%, K2P of ITS1-ITS2) could be found between the subgroup from China (G. ocellorhodei n. sp., G. sinenorhodei n. sp. and G. acheilorhodei n. sp.) and that from Europe (G. rhodei)., Competing Interests: Declaration of competing interest The authors declare no conflict of interest., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

12. Comparison of different molecular protocols for the detection of Uncinaria stenocephala infection in dogs.

Author

Illiano S, Ciuca L, Bosco A, Rinaldi L, and Maurelli MP

Subjects

Animals, Dogs, DNA, Helminth isolation & purification, DNA, Helminth analysis, Parasite Egg Count veterinary, Parasite Egg Count methods, Larva, Sensitivity and Specificity, Dog Diseases parasitology, Dog Diseases diagnosis, Feces parasitology, Ancylostomatoidea isolation & purification, Ancylostomatoidea genetics, Hookworm Infections veterinary, Hookworm Infections diagnosis, Hookworm Infections parasitology, Polymerase Chain Reaction veterinary, Polymerase Chain Reaction methods

Abstract

The present study aims to assess the performance of different molecular targets using various matrices of samples for the detection of Uncinaria stenocephala (US) in hookworm infected dogs. To this end, the DNA extraction was performed on the following matrices of samples: (i) larvae of US obtained from experimentally infected dogs with US with different larvae counts per microliter (µl); (ii) pure US eggs suspension in distilled water with different egg counts per µl; (iii) spiked dog fecal samples with different US eggs per gram (EPG) of feces; (iv) feces from dogs naturally infected with hookworm eggs; (v) fecal suspension with hookworm eggs recovered from the FLOTAC apparatus. All the samples were tested with four different PCR protocols targeting specific regions for the detection of both hookworms US and AC as follows: Protocol A (ITS1, 5.8 S, ITS2) and Protocol B (18 S) for the detection of both species, Protocol C (ITS1) for the detection of AC and Protocol D (ITS1) for the detection of US. The best results were obtained with DNA extracted from US larvae matrix obtained from experimentally infected dogs, showing a detection limit of 3.5 larvae/ml for the protocols A, B and D. A moderate correlation was found between the FLOTAC technique and PCR protocols B and D with respect to fecal samples from dogs naturally infected with hookworms. Indeed, PCR protocols B (18 S) and D (ITS1) gave the best results for feces and fecal suspension from naturally infected dogs. However, all the PCR protocols used showed lower sensitivity than FLOTAC technique. Perhaps, isolating US eggs in advance could help to obtain better quality and quantity of DNA, avoiding some notable factors such as inhibitors present in faecal samples. However, a further study is needed to evaluate and standardise a protocol for the recovery of parasitic elements, that could be applied prior to DNA extraction. Therefore, this could lead to a better amplification of US eggs DNA. In conclusion, our results showed that the type of sample (sample-matrix) used for the DNA extraction samples is crucial, as this affects the diagnostic sensitivity of the technique., Competing Interests: Declaration of Competing Interest The authors declare the following financial interests/personal relationships which may be considered as potential competing interests: Lavinia Ciuca reports was provided by University of Naples Federico II. Lavinia Ciuca reports a relationship with University of Naples Federico II that includes: employment. If there are other authors, they declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper, (Copyright © 2024 The Authors. Published by Elsevier B.V. All rights reserved.)

Published

2024

13. The vicuna (Vicugna vicugna) as a natural host of Dictyocaulus filaria in Peru.

Author

Gomez-Puerta LA, Angulo-Tisoc JM, and Pacheco JI

Subjects

Animals, Peru, RNA, Ribosomal, 28S genetics, RNA, Ribosomal, 28S analysis, DNA, Helminth analysis, Phylogeny, Male, Female, Dictyocaulus isolation & purification, Dictyocaulus genetics, Camelids, New World parasitology, Dictyocaulus Infections parasitology

Abstract

Lungworm infection, or verminous pneumonia, is a parasitic disease that causes serious problems in small and large ruminants. Despite the fact that nematodes of the genus Dictyocaulus in cattle and sheep are the main cause of this disease, there are few studies on the natural infections of South American camelids. For this reason, this study aims to report the natural infection by Dictyocaulus filaria in vicunas (Vicugna vicugna) for the first time. During a shearing season (chaku) in Cuzco, Peru, two accidentally killed adult vicunas were submitted to the IVITA-Marangani research center in Cuzco for their respective necropsies. The tracheas of both vicunas had numerous nematodes, as seen during the necropsy. The nematodes were collected in 70% ethanol and were morphologically identified as D. filaria. Likewise, the DNA of six nematodes was extracted, and the ITS2 region and the 28S rRNA gene were amplified and sequenced. The nucleotide sequences of both genetic markers were up to 100% identical with previously reported D. filaria DNA sequences found in the goat yearlings from Turkey, sheep from Iran, Turkey, and India, and the argali from Uzbekistan, which confirmed the morphological diagnosis. This finding represents the first molecular confirmation of a natural D. filaria infection in a South American camelid. It will be necessary to carry out future studies to know the current situation of verminous pneumonia in domestic and wild South American camelids and to know the negative effects of the disease on them., Competing Interests: Declaration of competing interest Not applicable., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

14. Lepocreadiidae (Trematoda) associated with gelatinous zooplankton (Cnidaria and Ctenophora) and fishes in Australian and Japanese waters.

Author

Cribb TH, Cutmore SC, Wee NQ, Browne JG, Morales PD, and Pitt KA

Subjects

Animals, Australia, Cnidaria classification, DNA, Helminth analysis, DNA, Mitochondrial analysis, DNA, Ribosomal analysis, DNA, Ribosomal Spacer analysis, Fishes parasitology, Japan, Metacercariae isolation & purification, Phylogeny, Fish Diseases parasitology, Fish Diseases epidemiology, Trematoda classification, Trematoda genetics, Trematoda isolation & purification, Trematoda anatomy & histology, Trematode Infections veterinary, Trematode Infections parasitology, Trematode Infections epidemiology, Zooplankton

Abstract

We examined gelatinous zooplankton from off eastern Australia for lepocreadiid trematode metacercariae. From 221 specimens of 17 species of cnidarian medusae and 218 specimens of four species of ctenophores, infections were found in seven cnidarian and two ctenophore species. Metacercariae were distinguished using cox1 mtDNA, ITS2 rDNA and morphology. We identified three species of Prodistomum Linton, 1910 [P. keyam Bray & Cribb, 1996, P. orientale (Layman, 1930), and Prodistomum Type 3], two species of Opechona Looss, 1907 [O. kahawai Bray & Cribb, 2003 and O. cf. olssoni], and Cephalolepidapedon saba Yamaguti, 1970. Two species were found in cnidarians and ctenophores, three only in cnidarians, and one only in a ctenophore. Three Australian fishes were identified as definitive hosts; four species were collected from Scomber australasicus and one each from Arripis trutta and Monodactylus argenteus. Transmission of trematodes to these fishes by ingestion of gelatinous zooplankton is plausible given their mid-water feeding habits, although such predation is rarely reported. Combined morphological and molecular analyses of adult trematodes identified two cox1 types for C. saba, three cox1 types and species of Opechona, and six cox1 types and five species of Prodistomum of which only two are identified to species. All three genera are widely distributed geographically and have unresolved taxonomic issues. Levels of distinction between the recognised species varied dramatically for morphology, the three molecular markers, and host distribution. Phylogenetic analysis of 28S rDNA data extends previous findings that species of Opechona and Prodistomum do not form monophyletic clades., Competing Interests: Declaration of competing interest The authors declare that they have no conflict of interest., (Copyright © 2024 The Authors. Published by Elsevier B.V. All rights reserved.)

Published

2024

15. Detection of Wuchereria bancrofti infection in mosquitoes in areas co-endemic with Brugia malayi in Balasore district, Odisha, India.

Author

Abraham PR, Ramalingam B, Mohapatra P, Krishnamoorthy K, Hoti SL, and Kumar A

Subjects

Animals, India epidemiology, Humans, Mosquito Vectors parasitology, Culex parasitology, Endemic Diseases, Female, DNA, Helminth genetics, DNA, Helminth analysis, Filariasis epidemiology, Filariasis parasitology, Filariasis transmission, Wuchereria bancrofti isolation & purification, Wuchereria bancrofti genetics, Brugia malayi genetics, Brugia malayi isolation & purification, Elephantiasis, Filarial epidemiology, Elephantiasis, Filarial parasitology, Elephantiasis, Filarial transmission

Abstract

Lymphatic filariasis (LF) is a crippling and disfiguring parasitic condition. India accounts for 55% of the world's LF burden. The filarial parasite Wuchereria bancrofti is known to cause 99.4% of the cases while, Brugia malayi accounts for 0.6% of the issue occurring mainly in some pockets of Odisha and Kerala states. The Balasore (Baleswar) district of Odisha has been a known focus of B. malayi transmission. We employed molecular xenomonitoring to detect filarial parasite DNA in vectors. In six selected villages, Gravid traps were used to collect Culex mosquitoes and hand catch method using aspirators was followed for collection of mansonioides. A total of 2903 mosquitoes comprising of Cx. quinquefasciatus (n = 2611; 89.94%), Cx. tritaeniorhynchus (n = 100; 3.44%), Mansonia annuliferea (n = 139; 4.78%) and Mansonia uniformis (n = 53; 1.82%) were collected from six endemic villages. The species wise mosquitoes were made into 118 pools, each with a maximum of 25 mosquitoes, dried and transported to the laboratory at VCRC, Puducherry. The mosquito pools were subjected to parasite DNA extraction, followed by Real-time PCR using LDR and HhaI probes to detect W. bancrofti and B. malayi infections, respectively. Seven pools (6.66%) of Cx. quinquefasciatus, showed infection with only W. bancrofti while none of the pools of other mosquito species showed infection with either W. bancrofti or B. malayi. Although the study area is endemic to B. malayi, none of the vectors of B. malayi was found with parasite infection. This study highlights the ongoing transmission of bancroftian filariasis in the study villages of Balasore district of Odisha and its implications for evaluating LF elimination programme., (© 2024. The Author(s).)

Published

2024

16. Prevalence and molecular characterization of Hysterothylacium species infecting Pandora (Pagellus erythrinus) in the Mediterranean Sea of Egypt.

Author

Menshawy S, Essa B, Shaaban S, Zaid AA, AbouLaila M, and Wheeb H

Subjects

Animals, Egypt epidemiology, Prevalence, Mediterranean Sea epidemiology, Female, Male, Ascaridida Infections veterinary, Ascaridida Infections parasitology, Ascaridida Infections epidemiology, Phylogeny, Ascaridoidea isolation & purification, Ascaridoidea genetics, Ascaridoidea classification, Electron Transport Complex IV analysis, Electron Transport Complex IV genetics, DNA, Ribosomal Spacer analysis, DNA, Ribosomal Spacer genetics, DNA, Helminth analysis, Fish Diseases parasitology, Fish Diseases epidemiology

Abstract

Species of the genus Hysterothylacium are aquatic roundworms (nematodes) belonging to the family Raphidascarididae. Some species in this family are known to be associated with zoonotic diseases in humans after they consume their parasitic larvae in raw or undercooked fish. The aim of this research was to report the prevalence, morphology, and molecular characteristics of Hysterothylacium species in Pagellus erythrinus. A total of Two hundred fish were purchased from the fish market in Damanhour, Beheira Province, between December 2021 and November 2022 and subjected to examination. For molecular characterization, the internal transcribed spacer (ITS) region of nuclear ribosomal DNA and the mitochondrial cytochrome oxidase subunit 2 (COX-2) gene were used. Hysterothylacium species were morphologically described and identified from the intestine of Pagellus erythrinus in Beheira Province, Egypt. The PCR amplified 1087 bp and 629 bp of the target sequences of the ITS region and COX-2 gene, respectively. Sequence analysis revealed the Hysterothylacium thalassini species. The identified species provided novel biological data for the Hysterothylacium nematode in Pagellus erythrinus. The prevalence of Hysterothylacium species recovered from the intestine was 55%. The highest prevalence of 72% has been reported in summer compared to the lowest prevalence of 38% in the winter. Females had a higher prevalence of 61.8% than males, with 44.2%. The first detection, prevalence, and molecular characterization of H. thalassini in Pagellus erythrinus from Beheira Province, Egypt, was presented in this study., Competing Interests: Declaration of competing interest The authors declare that there are no conflicts of interest., (Copyright © 2024. Published by Elsevier B.V.)

Published

2024

17. TREMATODE SPECIES DETECTION AND QUANTIFICATION BY ENVIRONMENTAL DNA-qPCR ASSAY IN LAKE CHANY, RUSSIA.

Author

Gacad JLJ, Yurlova NI, Tanabe-Hosoi S, and Urabe M

Subjects

Animals, Russia, Species Specificity, Trematode Infections parasitology, Trematode Infections diagnosis, Trematode Infections veterinary, Sensitivity and Specificity, DNA Primers, Snails parasitology, Lakes parasitology, Real-Time Polymerase Chain Reaction standards, Trematoda genetics, Trematoda classification, Trematoda isolation & purification, DNA, Helminth isolation & purification, DNA, Helminth analysis, DNA, Environmental isolation & purification, DNA, Environmental analysis

Abstract

Environmental DNA (eDNA) surveys promise to be a sensitive and powerful tool for the detection of trematodes. This can contribute to the limited studies on trematode ecology, specifically in aquatic ecosystems. Here, we developed species-specific primer and probe sets for Moliniella anceps, Opisthioglyphe ranae, and Plagiorchis multiglandularis cercariae and applied a novel eDNA qPCR assay to detect larval trematodes quantitatively. We evaluated the effectiveness of the assays using filtered lake water samples collected from different sites of Lake Fadikha and Kargat River Estuary in Lake Chany, Russia, showing high species specificity and sensitivity in all 3 assays. Further, all 3 assays had high efficiencies ranging from 94.9 to 105.8%. Moliniella anceps, O. ranae, and P. multiglandularis were detected in the environmental water samples through real-time PCR. Thus, we anticipate that our approach will be beneficial for biomonitoring, measuring, and managing ecological systems., (© American Society of Parasitologists 2024.)

Published

2024

18. Identification of third stage larvae of strongyles and molecular diagnosis of Strongylus vulgaris in the feces of Thoroughbred horses kept in training centers in Rio de Janeiro, Brazil.

Author

Martins AV, Corrêa LL, Ribeiro MS, de Lima Coelho A, Lobão LF, Palmer JPS, Knackfuss FB, Molento MB, and da Silva Barbosa A

Subjects

Animals, Horses, Brazil, Male, Female, Horse Diseases diagnosis, Horse Diseases parasitology, Parasite Egg Count veterinary, Polymerase Chain Reaction veterinary, DNA, Helminth analysis, Anthelmintics therapeutic use, Feces parasitology, Strongylus isolation & purification, Larva, Strongyle Infections, Equine diagnosis, Strongyle Infections, Equine parasitology

Abstract

The aims of the present study were to identify strongyles in the feces of Thoroughbred horses based on larval morphology; to detect Strongylus vulgaris using molecular diagnosis and compare results to those of feces culture; and to determine the association between the presence of S. vulgaris with corresponding animal information (age range, gender, and anthelmintic use). Feces of horses kept in six Training Centers in Rio de Janeiro State, that showed the presence of ≥500 eggs per gram of feces (EPG) were subjected to strongyle identification. Of the 520 fecal samples collected, 35 had an EPG ≥ 500. After fecal culture for L3 larvae identification, DNA was extracted, subjected to PCR to amplify the ITS2 region DNA fragment of S. vulgaris, and sequenced. A total of 3500 larvae were analyzed. Most were classified as small strong (99.7%), with an emphasis on the type A subfamily of Cyathostominae. Forms of S. vulgaris only corresponded to 0.2%. In all, 25 samples showed amplified S. vulgaris DNA products and 11 showed nucleotide sequences with high sequence identity. Fecal culture and PCR results showed poor agreement (kappa = 0.105) for S. vulgaris diagnosis. Age, gender, anthelmintic use, and anthelmintic administration interval were not statistically significant. The present study showed the presence of S. vulgaris in the feces of horses kept in Rio de Janeiro Training Centers, mainly seen via PCR, which has emerged as the most effective tool for diagnosis. This study made it possible to identify strongyles that infect horses in the region, emphasizing upon the necessity for constant monitoring of the animals., Competing Interests: Declaration of competing interest The authors declare that they have no conflict of interest., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

19. Estimating Prevalence and Infection Intensity of Soil-Transmitted Helminths Using Quantitative Polymerase Chain Reaction and Kato-Katz in School-Age Children in Angola.

Author

Soultani M, Bartlett AW, Mendes EP, Hii SF, Traub R, Palmeirim MS, Lufunda LMM, Colella V, Lopes S, and Vaz Nery S

Subjects

Humans, Child, Angola epidemiology, Animals, Prevalence, Male, Female, Helminthiasis epidemiology, Helminthiasis diagnosis, Helminthiasis parasitology, Real-Time Polymerase Chain Reaction methods, Adolescent, Ascaris lumbricoides isolation & purification, Ascaris lumbricoides genetics, Strongyloidiasis epidemiology, Strongyloidiasis diagnosis, Strongyloidiasis parasitology, DNA, Helminth analysis, DNA, Helminth genetics, Helminths isolation & purification, Helminths genetics, Parasite Egg Count, Trichuris isolation & purification, Trichuris genetics, Feces parasitology, Soil parasitology, Strongyloides stercoralis isolation & purification, Strongyloides stercoralis genetics

Abstract

Quantitative polymerase chain reaction (qPCR) is gaining recognition in soil-transmitted helminth (STH) diagnostics, especially for Strongyloides stercoralis and differentiating hookworm species. However, sample preservation and DNA extraction may influence qPCR performance. We estimated STH prevalence and infection intensity by using qPCR in schoolchildren from Huambo, Uige, and Zaire, Angola, and compared its performance with that of the Kato-Katz technique (here termed Kato-Katz). Stool samples from 3,063 children (219 schools) were preserved in 96% ethanol and analyzed by qPCR, of which 2,974 children (215 schools) had corresponding Kato-Katz results. Cluster-adjusted prevalence and infection intensity estimates were calculated by qPCR and Kato-Katz, with cycle threshold values converted to eggs per gram for qPCR. Cohen's kappa statistic evaluated agreement between qPCR and Kato-Katz. DNA extraction and qPCR were repeated on 191 (of 278) samples that were initially qPCR negative but Kato-Katz positive, of which 112 (58.6%) became positive. Similar prevalence for Ascaris lumbricoides (37.5% versus 34.6%) and Trichuris trichiura (6.5% versus 6.1%) were found by qPCR and Kato-Katz, respectively, while qPCR detected a higher hookworm prevalence (11.9% versus 2.9%). The prevalence of moderate- or high-intensity infections was higher by Kato-Katz than by qPCR. Agreement between qPCR and Kato-Katz was very good for A. lumbricoides, moderate for T. trichiura, and fair for hookworm. Strongyloides stercoralis prevalence was 4.7% (municipality range, 0-14.3%), and no Ancylostoma ceylanicum was detected by qPCR. Despite suboptimal performance, presumably due to fixative choice, qPCR was fundamental in detecting S. stercoralis and excluding zoonotic A. ceylanicum. Further evaluations on sample fixatives and DNA extraction methods are needed to optimize and standardize the performance of qPCR.

Published

2024

20. Molecular and morphological evidence suggests the reallocation from Parastrigea brasiliana (Szidat, 1928) Dubois, 1964 to Apharyngostrigea Ciurea, 1927 (Digenea: Strigeidae), a parasite of boat-billed heron (Cochlearius cochlearius) from the Neotropical region.

Author

López-Jiménez A, González-García MT, and García-Varela M

Subjects

Animals, DNA, Helminth analysis, DNA, Mitochondrial analysis, Helminth Proteins analysis, Mexico, Microscopy, Electron, Scanning veterinary, Trematode Infections parasitology, Bird Diseases parasitology, Birds, Trematoda anatomy & histology, Trematoda classification, Trematoda genetics, Trematoda ultrastructure, Trematode Infections veterinary

Abstract

Parastrigea brasiliana (Szidat, 1928) Dubois, 1964, was described from (Cochlearius cochlearius) in South America. The taxonomy of this species has been unstable due that it was described as a member of Strigea Abildgaard, 1790. However, the same author one year later transferred it to Apharyngostrigea Ciurea, 1927 and since then, it has been alternatively placed in the genus Apharyngostrigea or Parastrigea Szidat, 1928 from Strigeidae. In the current research, specimens identified as P. brasiliana were collected from type host in southeastern Mexico. We sequenced three molecular markers: the internal transcribed spacers ITS1 and ITS2 including the 5.8S gene (ITS region), the D1-D3 domains of the large subunit (LSU) from nuclear DNA and cytochrome c oxidase subunit I (cox 1) from mitochondrial DNA. These sequences were aligned with other sequences available in the GenBank dataset from Strigeidae. Maximum likelihood and Bayesian analyses inferred with three molecular markers consistently showed that P. brasiliana is not closely related to other members of the genus Parastrigea and are placed in a reciprocal monophyletic clade inside Apharyngostrigea, with very low genetic divergence, varying from 0 to 0.09% for the ITS, from 0 to 0.08% for the LSU and from 0.21 to 0.43% for cox 1. Consequently, we proposed to reallocate it to A. brasiliana. The phylogenetic analyses obtained are key and very useful for re-evaluate the morphology of A. brasiliana because this species share morphological characters with the genera Parastrigea (concentration of vitelline follicles distributed in two lateral expansions on the forebody) and Apharyngostrigea (absence of pharynx). Finally, the current record of A. brasiliana expands its distribution range in four countries, namely, the USA, Mexico, Venezuela and Brazil, in the Neotropical region., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2022

21. Integrative taxonomy of Mesocriconema onoense (Tylenchida: Criconematidae) from Vietnam highly suggests the synonymization of Mesocriconema brevistylus and related species.

Author

Nguyen HT, Nguyen TD, Le TML, and Trinh QP

Subjects

Animals, DNA, Helminth analysis, Female, Phylogeny, RNA, Helminth analysis, Tylenchida anatomy & histology, Tylenchida genetics, Vietnam, DNA, Intergenic analysis, RNA, Ribosomal, 18S analysis, RNA, Ribosomal, 28S analysis, Tylenchida classification

Abstract

The genus Mesocriconema is one of the most diverse genera within the family Criconematidae, known as ring nematodes, with more than 90 species. Although species in this genus usually show distinct morphological characterizations, the identification based only on morphology can lead to misidentification in many studies resulted in a number of synonymizations in the genus over time. In this study, an integrated approach has been applied in characterizing Mesocriconema onoense from Vietnam. The molecular data of 28S rRNA, ITS, 18S rRNA regions were analyzed and discussed to confirm the correct names on GenBank. Besides, phylogenetic analyses of 28S rRNA, ITS, and 18S rRNA regions of Mesocriconema species revealed that Mesocriconema brevistylus should be considered as a junior synonym of M. onoense. Consequently, M. helicus, M. onostris, and M. paronostris should also be considered as the synonyms of M. onoense., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2021

22. First demonstration of Strongyloides parasite from an imported pet meerkat - Possibly a novel species in the stercoralis/procyonis group.

Author

Takaki Y, Kadekaru S, Takami Y, Yoshida A, Maruyama H, Une Y, and Nagayasu E

Subjects

Animals, Base Sequence, DNA, Helminth analysis, Male, Pets, Strongyloides genetics, Strongyloides isolation & purification, Strongyloidiasis diagnosis, Strongyloidiasis parasitology, Herpestidae, Strongyloides classification, Strongyloidiasis veterinary

Abstract

Strongyloides is a genus of parasitic nematodes of vertebrates that contains over 50 species, each with a variable host range. A recent molecular phylogenetic analysis on this genus showed that Strongyloides spp. from various carnivore hosts form a strongly supported clade together with Strongyloides stercoralis, a major pathogen of humans and dogs (named the "stercoralis/procyonis group"). In the present study, we obtained DNA sequencing data of Strongyloides sp. isolated from an imported meerkat (Suricata suricatta). Based on the phylogenetic analysis, we considered this a new member of the stercoralis/procyonis group. This study represents the first isolation and molecular characterization of a Strongyloides species from hosts belonging to the family Herpestidae (mongooses and meerkat). However, whether the meerkat serves as a natural host of this Strongyloides species remains to be investigated., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2021

23. First report of fatal baylisascariasis-induced acute pancreatitis in a giant panda.

Author

Qin Z, Liu S, Bai M, Geng Y, Miller DL, Zhao R, Hou R, Huang W, Zhang D, and Su X

Subjects

Acute Disease, Animals, Animals, Zoo, Ascaridida Infections parasitology, Ascaridida Infections pathology, Blood Chemical Analysis veterinary, China, DNA, Helminth analysis, Fatal Outcome, Hematologic Tests veterinary, Male, Pancreatitis parasitology, Pancreatitis pathology, Sequence Analysis, DNA veterinary, Ascaridida Infections veterinary, Ascaridoidea isolation & purification, Pancreatitis veterinary, Ursidae

Abstract

A wild adult male giant panda that was rescued from a nature reserve in Sichuan Province, China, has died. The panda had been in poor physical condition: it was wheezing and had increased serum amylase. A pathological examination was performed in order to determine the cause of death. Gross examination revealed 1380 mL of yellowish fluid in the abdominal cavity, 356 nematodes in the digestive tract and one filling the pancreatic duct, contractions and variably-sized dark purple areas in the spleen, a collapsed right lung and consolidation of the left lung. Acute pancreatitis was confirmed histopathologically via edema, focal necrosis and hemorrhage with inflammatory cell infiltration. Other major histopathological changes included serous-hemorrhagic pneumonia, lymphocytic necrosis and depletion in the spleen, and degeneration and necrosis of renal tubular epithelial cells. The nematodes were identified as Baylisascaris schroederi via molecular assays. In conclusion, the cause of death of the giant panda was determined to be multiple organ dysfunction syndrome caused by baylisascariasis-induced acute pancreatitis. To our knowledge, this is the first report of fatal baylisascariasis-induced acute pancreatitis in the giant panda., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2021

24. High-throughput sequencing of Fasciola spp. shows co-infection and intermediate forms in Balochistan, but only Fasciola gigantica in the Punjab province of Pakistan.

Author

Rehman ZU, Martin K, Zahid O, Ali Q, Rashid I, Hafeez MA, Ahmad N, Ashraf K, Betson M, Sargison ND, and Chaudhry U

Subjects

Animals, Buffaloes, Cattle, Cattle Diseases parasitology, Coinfection epidemiology, Coinfection parasitology, DNA, Helminth analysis, DNA, Mitochondrial analysis, DNA, Ribosomal analysis, Fascioliasis epidemiology, Fascioliasis parasitology, Goat Diseases parasitology, Goats, High-Throughput Nucleotide Sequencing veterinary, Pakistan epidemiology, Prevalence, Sheep, Sheep Diseases parasitology, Sheep, Domestic, Species Specificity, Cattle Diseases epidemiology, Coinfection veterinary, Fasciola isolation & purification, Fascioliasis veterinary, Goat Diseases epidemiology, Sheep Diseases epidemiology

Abstract

Fasciola gigantica and Fasciola hepatica are digenetic trematodes causing fasciolosis in ruminants. The host and geographical distribution of both Fasciola species are influenced by environmental and climatic conditions favouring survival and development of free-living stages and intermediate hosts, and livestock management practices. The aim of the present study was to describe the host distribution of the two Fasciola species in buffalo, cattle, goats, and sheep in the Balochistan and Punjab provinces of Pakistan. 359 flukes were collected from a total of 32 livers from the four livestock species. Deep amplicon sequencing of the internal transcribed spacer region 2 of ribosomal DNA (rDNA ITS-2) and mitochondrial nicotinamide adenine dinucleotide dehydrogenase 1 (mtDNA ND-1) loci confirmed co-infection of F. hepatica and F. gigantica in Balochistan and single species F. gigantica infection in Punjab. In Balochistan, co-infections and hybrids of both Fasciola species were identified in cattle, with more F. hepatica detected than F. gigantica. However, F. hepatica was the only species identified in goats, and F. gigantica was the only species identified in buffalo. In Punjab, all flukes were confirmed as F. gigantica in each of the four livestock species. Overall, the results indicate differences in the host and geographical distribution of F. gigantica and F. hepatica, and provide useful knowledge for the development of control strategies for livestock and humans., (Copyright © 2021. Published by Elsevier B.V.)

Published

2021

25. Redescription of Paradiplozoon opsariichthydis (Jiang, Wu et Wang 1984) Jiang, Wu et Wang, 1989 (Monogenea, Diplozoidae).

Author

Jirsová D, Koubková B, Jirounková E, Vorel J, Zhou X, Ding X, Gelnar M, and Kašný M

Subjects

Animals, Cytochromes b analysis, DNA, Helminth analysis, DNA, Ribosomal Spacer analysis, Female, Fish Diseases parasitology, Fish Proteins analysis, Male, Trematoda classification, Trematoda genetics, Trematode Infections parasitology, Cyprinidae, Host-Parasite Interactions, Phylogeny, Trematoda anatomy & histology

Abstract

Paradiplozoon opsariichthydis (Jiang, Wu et Wang, 1984) Jiang, Wu et Wang, 1989 (Platyhelminthes, Monogenea, Diplozoidae) is blood-feeding parasite from the gills of Asian cyprinid fish Opsariichthys bidens Günther, 1873. In this study, we present a morphological redescription of P. opsariichthydis neotype main morphological features e.g. size of body and clamps due to the fact that the type material is missing. We decided to supplement morphological descriptions by the relevant molecular data (internal transcribed spacer - ITS2) related to P. opsariichthydis adult worm isolates and other representatives of genus Paradiplozoon to cross verify our findings. In addition to that, this study also brings an attention to the host identification. Thus, parasite data were complemented by the determinant cytochrome oxidase b (cytb) sequences of its hosts. All novel sequences are deposited in GenBank. This combination of the morphological and molecular data related to both the parasite and its host seems to be the optimal approach to the general process of (re)description of highly host-specific parasitic organisms, which can then lead to a meaningful phylogenetic analysis., (Copyright © 2021 The Authors. Published by Elsevier B.V. All rights reserved.)

Published

2021

26. The phylogeographic puzzle of Pseudoacanthocephalus toshimai, an amphibian acanthocephalan in northern Japan.

Author

Nakao M and Ishigoka C

Subjects

Acanthocephala classification, Acanthocephala genetics, Animals, DNA, Helminth analysis, DNA, Mitochondrial analysis, Japan, Phylogeography, Acanthocephala physiology, Animal Distribution, Bufonidae parasitology, Host-Parasite Interactions, Ranidae parasitology

Abstract

The amphibian acanthocephalan, Pseudoacanthocephalus toshimai, was considered to be an island-endemic species in Hokkaido, Japan. However, the parasite was found from Rana ornativentris, Rana tagoi, Zhangixalus arboreus, and Bufo japonicus formosus in northern Honshu (Aomori and Iwate Prefectures), which is separated from Hokkaido by the Tsugaru Strait. The mitochondrial DNA-based phylogenetic and population genetic analyses of P. toshimai showed that the northern Honshu isolates are far distantly related to the Hokkaido isolates, and that a demographic population expansion occurred in Hokkaido during the recent geological past. The rich genetic diversity of P. toshimai in northern Honshu suggests a scenario that anuran hosts invaded Hokkaido together with P. toshimai via the land bridge of the Tsugaru Strait. However, the evolutionary history of Rana pirica, a main definitive host for P. toshimai in Hokkaido, is contradictory to the introduction scenario inferred from the parasite. The finding of several geographically mismatched isolates of P. toshimai from both northern Honshu and Hokkaido suggests a possibility that the migration of the parasite infrequently occurred between the two areas even after the land bridge disappeared. More detailed information on the evolutionary history of anurans is needed to resolve the biogeographical enigma of P. toshimai., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2021

27. Morphological and molecular data of new species of Characithecium and Diaphorocleidus (Monogenea: Dactylogyridae) from Neotropical characid fishes.

Author

Zago AC, Franceschini L, Abdallah VD, Müller MI, Azevedo RK, and da Silva RJ

Subjects

Animals, Brazil epidemiology, DNA, Helminth analysis, DNA, Ribosomal analysis, Electron Transport Complex IV analysis, Helminth Proteins analysis, Male, Mitochondrial Proteins analysis, Prevalence, Trematoda anatomy & histology, Trematoda cytology, Trematoda genetics, Trematode Infections parasitology, Characidae, Fish Diseases parasitology, Trematoda classification, Trematode Infections veterinary

Abstract

The present study describes three new species of monogenean parasites of characid fishes from the Upper Paraná River basin, Brazil: Characithecium paranapanemense n. sp. on Psalidodon paranae and Psalidodon bockmanni, Diaphorocleidus magnus n. sp. on Astyanax lacustris and Psalidodon fasciatus, and Diaphorocleidus neotropicalis n. sp. on Astyanax lacustris and P. bockmanni. An amendment for Diaphorocleidus is proposed, since additional characters observed in the new species required to extend the generic diagnostic features mainly to include: articulation process connecting the base of the MCO with accessory piece present or absent, and accessory piece with variable shapes (plate-like, pincer-shaped, wrench-shaped, sheath-shaped), divided or not into subunits. Characithecium paranapanemense n. sp. can be distinguished from other congeners by the morphology of its MCO and accessory piece. Diaphorocleidus magnus n. sp. differs from most of its congeners by the morphology of its accessory piece, the presence of articulation process connecting the base of the MCO with accessory piece, and the morphology of the sclerotized structures of the haptor. Diaphorocleidus neotropicalis n. sp. can be easily distinguished from its congeners by the morphology of the accessory piece, the sclerotized structures of the haptor and the morphology of the vagina. Molecular data of the new species (partial 28S rDNA and mitochondrial cytochrome oxidase I) were obtained and the first phylogenetic analysis based on 28S rDNA gene sequences for species of Characithecium and Diaphorocleidus are provided. Although Diaphorocleidus and Characithecium share some morphological similarities, phylogenetic analysis indicates that species of these two genera are not closely related., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2021

28. Systematics of Crepidostomum species from the Russian Far East and northern Japan, with description of a new species and validation of the genus Stephanophiala.

Author

Vainutis KS, Voronova AN, and Urabe M

Subjects

Animals, DNA, Helminth analysis, DNA, Mitochondrial analysis, Electron Transport Complex IV analysis, Helminth Proteins analysis, Japan, RNA, Helminth analysis, RNA, Ribosomal, 28S analysis, Siberia, Trematoda anatomy & histology, Trematoda genetics, Host-Parasite Interactions, Phylogeny, Trematoda classification

Abstract

Current article touched upon the issue of the complicated taxonomic status of some species from the genus Crepidostomum collected from the freshwater fish in the rivers of Primorsky region, Sakhalin, and Hokkaido Islands. Primary morphological analyses showed affiliation of the worms to the species C. farionis (Müller, 1784) Lühe, 1909; C. metoecus Braun, 1900b; C. chaenogobii Yamaguti and Matsumura, 1942; C. nemachilus Krotov, 1959. We described the new species Crepidostomum achmerovi sp. nov. that is a sibling species of C. nemachilus. Molecular-genetic investigation have shown that C. nemachilus and C. achmerovi sp. nov. are closely related to C. metoecus in both 28S rDNA and cox1 mtDNA markers. Crepidostomum nemachilus forms a separate branch within the C. metoecus clade on the 28S BI tree with strong statistical support and separate clade in relation to C. metoecus clade on the cox1 BI tree. Values of p-distances between Crepidostomum species were at intergeneric level. Crepidostomum metoecus species complex including five species (C. metoecus, C. nemachilus, C. oschmarini, C. brinkmanni, and C. achmerovi sp. nov.) was reconsidered as independent genus Crepidostomum sensu stricto. Minimum Spanning Network showed that C. nemachilus, C. metoecus and C. achmerovi sp. nov. were separated by large number of mutational events and represent independent phyletic lines. An amended diagnosis is provided for the subfamily Crepidostomatinae, the genera Crepidostomum s. str. and Stephanophiala Nicoll, 1909, along with keys to species of both genera., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2021

29. Detection of six soil-transmitted helminths in human stool by qPCR- a systematic workflow.

Author

Azzopardi KI, Hardy M, Baker C, Bonnici R, Llewellyn S, McCarthy JS, Traub RJ, and Steer AC

Subjects

Animals, DNA, Helminth analysis, Fiji, Humans, Workflow, Feces parasitology, Helminths isolation & purification, Multiplex Polymerase Chain Reaction methods

Abstract

Soil-transmitted helminths (STH) infect up to one-quarter of the global population, with a significant associated disease burden. The main human STH are: Ancylostoma spp. and Necator americanus (hookworms); Ascaris lumbricoides, Trichuris trichiura, and Strongyloides stercoralis. The aim of this study was to establish a scalable system for stool STH multiplex quantitative real-time polymerase chain reactions (qPCR). Stool samples collected in Fiji and preserved in potassium dichromate were transferred to Melbourne at ambient temperature. Samples were washed to remove potassium dichromate and DNA was extracted with the Mini-Beadbeater-24 and a column-based kit. A SYBR green qPCR to detect the vertebrate mitochondrial gene was used as a DNA extraction control. Samples were tested using a probe-based multiplex qPCR targeting A. lumbricoides, T. trichiura and S. stercoralis, and in a second multiplex reaction to detect hookworms to the species level (A. duodenale, A. ceylanicum, N. americanus). An internal amplification control in both multiplex assays was included to prevent false-negative results due to PCR inhibitors. Samples were homogenised for a single cycle of 40 seconds to release STH DNA and washed stool was stored for up to 15 weeks at -30°C without compromising DNA. Our multiplex qPCR detected multiple species of STH without reduced sensitivity compared to singleplex. qPCR data from 40 stools was validated against STH-positive stools determined by microscopy. We have developed and validated an efficient and staged system for detecting six clinically important STH affecting humans that could be easily implemented without advanced automation in any qPCR-capable laboratory., Competing Interests: The authors have declared that no competing interests exist.

Published

2021

30. Detection and molecular characteristics of Rhytidodoides sp. (Digenea: Rhytidodidae) from the gall bladder of green sea turtles (Chelonia mydas) in the Ogasawara Islands, Japan.

Author

Kitayama C, Hayashi K, Hayashi K, Igarashi H, Kondo S, Ogawa R, Hashimoto T, Okubo S, Takashima Y, Itagaki T, Kuroki T, and Shibahara T

Subjects

Animals, DNA, Helminth analysis, DNA, Ribosomal analysis, Gallbladder Diseases parasitology, Japan epidemiology, Phylogeny, Prevalence, Trematoda anatomy & histology, Trematoda genetics, Trematode Infections parasitology, Gallbladder Diseases veterinary, Trematoda isolation & purification, Trematode Infections veterinary, Turtles

Abstract

Trematodes of the genus Rhytidodoides are parasitic in marine turtles. Of the already known species, Rhytidodoides similis Price, 1939, occurs especially in the gall bladder. In this study, we surveyed 73 green sea turtles (Chelonia mydas) in the Ogasawara Islands, Japan, and detected Rhytidodoides sp. from the gall bladders of 18 turtles. A detailed morphological analysis revealed that the forebody of Rhytidodoides sp. differed slightly in shape from that of R. similis. There has been no information on DNA sequences of the family Rhytidodidae. A molecular phylogeny based on 28S rDNA sequences of Rhytidodoides sp. and related taxa suggested that the Rhytidodidae is sister to the other families of Echinostomatoidea. The intraspecific diversity of Rhytidodoides sp. was examined by using DNA sequences of mitochondrial cytochrome c oxidase subunit 1 gene (COI). The population genetic features of the COI haplotypes demonstrated that Rhytidodoides sp. is highly diverse in the Ogasawara Islands. The DNA sequences determined in this study will contribute to the species identification of congeners and the taxonomic reconsideration of the Echinostomatoidea., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2021

31. Morphological and genetic characterization of Porrocaecum angusticolle (Molin, 1860) (Nematoda: Ascaridomorpha) from the common buzzard Buteo buteo (Linnaeus) (Accipitriformes: Accipitridae) in Czech Republic.

Author

Guo N, Sitko J, Chen HX, and Li L

Subjects

Animals, Ascaridida Infections parasitology, Ascaridoidea anatomy & histology, Ascaridoidea genetics, Ascaridoidea ultrastructure, Czech Republic, DNA, Helminth analysis, DNA, Ribosomal analysis, Electron Transport Complex IV analysis, Female, Helminth Proteins analysis, Male, Microscopy veterinary, Microscopy, Electron, Scanning veterinary, Ascaridida Infections veterinary, Ascaridoidea isolation & purification, Bird Diseases parasitology, Hawks

Abstract

Porrocaecum angusticolle is a nematode species mainly parasitic in the birds of Accipitriformes and Strigiformes. However, some aspects of the morphology of P. angusticolle remain insufficiently known. In the present study, the detailed morphology of P. angusticolle was studied using light and, for the first time, scanning electron microscopy, based on newly collected specimens from the common buzzard Buteo buteo (Linnaeus) (Accipitriformes: Accipitridae) in Czech Republic. Some previously unreported morphological features of taxonomic significance were observed. The nuclear and mitochondrial DNA markers, including partial large ribosomal DNA (28S), complete internal transcribed spacer (ITS-1 + 5.8S + ITS-2), cytochrome c oxidase subunit 1 (cox1) and subunit 2 (cox2) of P. angusticolle were sequenced for molecular identification of this species. There was no intraspecific genetic variation detected in the 28S and ITS regions among different individuals of P. angusticolle, but low level of intraspecific nucleotide divergence was found in the cox1 (0.26-0.78%) and cox2 regions (1.0%). The 28S and cox2 of P. angusticolle were sequenced for the first time. Our molecular evidence supported the validity of both P. angusticolle and P. depressum. The newly obtained genetic data are helpful for further studies of DNA-based taxonomy, population genetics and phylogeny of the genus of Porrocaecum., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2021

32. Gastric ulceration caused by genetically identified Anisakis simplex sensu stricto in a harbor porpoise from the Western Pacific stock.

Author

Katahira H, Matsuda A, Banzai A, Eguchi Y, and Matsuishi TF

Subjects

Animals, Anisakiasis parasitology, Anisakiasis pathology, DNA, Helminth analysis, DNA, Ribosomal analysis, Female, Japan, Stomach Ulcer parasitology, Anisakiasis veterinary, Anisakis physiology, Phocoena, Stomach Ulcer pathology

Abstract

The genus Anisakis is a well-known group of nematodes that parasitize cetaceans as the final host and cause mucosal damage to their stomach. However, little has been done to precisely identify the nematodes recovered from the final hosts, especially in the Western Pacific, because of taxonomic confusion about the discrimination of sibling species and the difficulties of obtaining specimens from cetaceans. We describe the results of genetic identification and histopathological observations of specimens recovered from an ulcerated lesion and stomach contents in the forestomach of a female harbor porpoise accidentally caught by a set net fishery in Usujiri, southern Hokkaido, Japan. All the specimens arbitrarily collected from the lesion and stomach contents were identified as Anisakis simplex sensu stricto according to their ITS rDNA sequences. The size of the ulcer was approximately 6.3 mm in diameter and it was infected with 119 individual nematodes, mostly consisting of L3 and L4 stage larvae (95.0%). Histological sections were characterized by a locally extensive ulcer with the parasites penetrating into the muscularis externa that caused a thickening of the surrounding mucosa., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2021

33. A review of molecular identification tools for the opisthorchioidea.

Author

Duflot M, Setbon T, Midelet G, Brauge T, and Gay M

Subjects

Animals, DNA Primers, DNA, Helminth analysis, DNA, Mitochondrial genetics, DNA, Ribosomal genetics, DNA, Ribosomal Spacer analysis, Electron Transport Complex IV genetics, Genes, Helminth, Heterophyidae classification, Heterophyidae genetics, Heterophyidae isolation & purification, Molecular Diagnostic Techniques, Nucleic Acid Amplification Techniques, Opisthorchidae classification, Opisthorchidae genetics, Opisthorchidae isolation & purification, Phylogeny, Polymerase Chain Reaction, Polymorphism, Restriction Fragment Length, Random Amplified Polymorphic DNA Technique, Trematoda genetics, Trematoda isolation & purification, DNA, Helminth genetics, Parasitology methods, Trematoda classification

Abstract

The superfamily Opisthorchioidea encompasses the families Cryptogonimidae, Opisthorchiidae and Heterophyidae. These parasites depend on the aquatic environment and include marine and freshwater species. Some species, such as Clonorchis sinensis and Opisthorchis viverrini, have a high impact on public health with millions of infected people worldwide and have thus been the object of many studies and tool developments. However, for many species, tools for identification and detection are scarce. Although morphological descriptions have been used and are still important, they are often not efficient on the immature stages of these parasites. Thus, during the past few decades, molecular approaches for parasite identification have become commonplace. These approaches are efficient, quick and reliable. Nonetheless, for some parasites of the superfamily Opisthorchioidea, reference genomic data are limited. This study reviews available genetic data and molecular tools for the identification and/or the detection of this superfamily. Molecular data on this superfamily are mostly based on mitochondrial and ribosomal gene sequence analyses, especially on the cytochrome c oxidase subunit 1 gene and internal transcribed spacer regions respectively., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2021

34. Accurate and rapid detection of Fasciola hepatica copro-DNA in sheep using loop-mediated isothermal amplification (LAMP) technique.

Author

Amiri S, Shemshadi B, Shirali S, Kheirandish F, and Fallahi S

Subjects

Animals, Cross-Sectional Studies, DNA, Helminth analysis, Diagnostic Tests, Routine veterinary, Fascioliasis diagnosis, Fascioliasis epidemiology, Feces parasitology, Iran epidemiology, Prevalence, Sheep, Sheep Diseases epidemiology, Sheep, Domestic, Fasciola hepatica isolation & purification, Fascioliasis veterinary, Molecular Diagnostic Techniques veterinary, Nucleic Acid Amplification Techniques veterinary, Sheep Diseases diagnosis

Abstract

Fascioliasis is a parasitic infection caused by Fasciola spp. in humans and animals. Despite significant advances in vaccination and new therapeutic agents, little attention has been paid to validate methods for the diagnosis of fascioliasis in animals. This study aimed to compare the loop-mediated isothermal amplification (LAMP) technique with PCR assay for the diagnosis of F. hepatica in sheep. In this cross-sectional study, 195 stool samples were collected from sheep for 3 months in Lorestan province, West of Iran. Specimens' parasitological examination was performed by using the direct wet mount and formalin-ether concentration method. After DNA extraction from the samples, molecular analysis was done using PCR and LAMP techniques based on the Fasciola ribosomal intergenic spacer (IGS) sequence. Of 195 specimens of sheep, 11 specimens were identified as F. hepatica-positive infection by using microscopic, PCR and LAMP assays. Kappa agreement test results showed that there was a significant agreement between the results of microscopic examination diagnostic tests, PCR and LAMP (Kappa = 0.51-0.72 and p < .001). According to the results of chi-square comparisons between parasite prevalence applying different techniques and variables of age, sex breed, and type of drinking water, there was no significant relationship (p ≥ .05). However, most of the infected sheep with Fasciola were 3- to 4-year-old females, of the Lori breed and consumed tap water. In many endemic areas, successful prevention and treatment of fascioliasis in animals depend on rapid and accurate diagnosis. Based on the results of the Kappa agreement, the significant agreement among the results of the microscopic examination, PCR and LAMP indicates the accuracy and reliability of these tests in the diagnosis of F. hepatica in sheep. However, molecular methods, especially the LAMP technique, are suggested because of their higher sensitivity and reliability for the diagnosis of F. hepatica even under field conditions., (© 2021 The Authors Veterinary Medicine and Science Published by John Wiley & Sons Ltd.)

Published

2021

35. Pulmonary hydatidosis genotypes isolates from human clinical surgery based on sequencing of mitochondrial genes in Fars, Iran.

Author

Mardani P, Ezabadi AT, Sedaghat B, and Sadjjadi SM

Subjects

Adolescent, Adult, Aged, Animals, Child, Child, Preschool, Echinococcosis, Pulmonary diagnosis, Echinococcus granulosus classification, Echinococcus granulosus isolation & purification, Female, Genetic Markers, Humans, Iran, Male, Middle Aged, Sequence Analysis, Sequence Analysis, DNA, Young Adult, DNA, Helminth analysis, Echinococcosis, Pulmonary parasitology, Echinococcus granulosus genetics, Electron Transport Complex IV genetics, Genes, Mitochondrial, Genotype

Abstract

Background: Cystic echinococcosis (CE)/hydatidosis is an important neglected parasitic zoonotic disease caused by the metacestode of Echinococcus granulosus s.l. The present study was designed to identify the pulmonary CE species/genotypes in isolated human underwent to surgery in our center in Southern Iran., Methods: The study population of this study were all patients in Fars province who were admitted to Namazi Hospitals for pulmonary hydatid cyst surgery. Thoracic surgery was performed in the thoracic ward and the cyst/s was removed by open surgery via posterolateral or lateral thoracotomy. DNA was extracted from the germinal layer or the protoscoleces. PCR technique was performed using the cytochrome C oxidase subunit1 (cox1) gene, and the products were sequenced., Results: A total of 32 pulmonary hydatid cyst samples were collected from 9 (28%) female and 23 (72%) male aged from 4 to 74 years old. A total of 18(56%) cyst/s were in the left lobe and 14 (44%) cysts in the right lobe. Sequence analysis of the cysts showed that 24 samples (75%) were E. granulosus s.s (G1-G3) genotype and 8 (25%) were E. canadensis (G6/G7) genotype., Conclusion: E.granulosus s.s genotype was the most prevalent genotype followed by E. canadensis (G6/G7) genotype. There was no significant statistical correlation between cysts' size, location, genotype strain, and patients' age and gender.

Published

2021

36. A new species of Grillotia Guiart, 1927 (Cestoda: Trypanorhyncha) from the spotted skate, Raja straeleni Poll, in South Africa.

Author

Oosthuizen G, Acosta AA, Smit NJ, and Schaeffner BC

Subjects

Animals, Cestode Infections epidemiology, Cestode Infections parasitology, DNA, Helminth analysis, Fish Diseases parasitology, Host-Parasite Interactions, RNA, Ribosomal, 28S analysis, South Africa epidemiology, Cestoda classification, Cestode Infections veterinary, Fish Diseases epidemiology, Phylogeny, Skates, Fish

Abstract

A new species of Grillotia Guiart, 1927 was recovered from the spotted skate (Raja straeleni Poll) from the south coast of the Western Cape, South Africa. Grillotia sasciae n. sp. is described based on morphological and molecular data. This species most closely resembles species in the subgenus Grillotia (viz., Grillotia borealis Keeney and Campbell, 2001, Grillotia brayi Beveridge and Campbell, 2007, Grillotia dollfusi Carvajal, 1971, Grillotia erinaceus Dollfus, 1969, Grillotia musculara Hart, 1936 and Grillotia patagonica Menoret and Ivanov, 2012) in having four hooks per principal row and intercalary hook rows in the metabasal region of the tentacular armature, a band of hooks on the external tentacular surface, numerous proglottids, and the presence of an uterine pore, a hermaphroditic sac, and internal and external seminal vesicles. The molecular phylogenetic analysis of the partial 28S rDNA gene, confirms the morphological data as it also groups Grillotia sasciae n. sp. within the G. erinaceus species complex. Grillotia sasciae n. sp. is distinctive among all other valid species in the complex by having two enlarged, uncinate hooks in the basal armature, of a different shape and size from the remaining hooks 1(1') in the metabasal armature. In addition, the retractor muscle of Grillotia sasciae n. sp. attaches at the posterior region of the tentacular bulb rather than the middle portion, continuing posteriorly as seen in most congeners (viz., G. erinaceus, G. borealis, G. brayi, G. musculara and G. pantagonica). The new species is the seventh species within the subgenus Grillotia and the first record of a species of Grillotia from southern African waters., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2021

37. Morphological and molecular identification of helminths of the greater bulldog bat Noctilio leporinus (Quiroptera: Noctilionidae) from Campeche, Mexico.

Author

Panti-May JA, Hernández-Mena DI, Torres-Castro MA, Estrella-Martínez E, Lugo-Caballero C, Vidal-Martínez VM, and Hernández-Betancourt SF

Subjects

Animals, DNA, Helminth analysis, Female, Male, Mexico epidemiology, Nematode Infections epidemiology, Nematode Infections parasitology, Prevalence, RNA, Ribosomal, 28S analysis, Trematode Infections epidemiology, Trematode Infections parasitology, Chiroptera, Nematoda isolation & purification, Nematode Infections veterinary, Trematoda isolation & purification, Trematode Infections veterinary

Abstract

Surveys on parasites of bats from the Americas have been conducted, but information on helminths is still scarce, especially in the Neotropical region. In Mexico, there are species of bats that lack of a record for helminth species, such as members of the family Noctilionidae. The present study describes for the first time the helminths of Noctilio leporinus in Campeche, Mexico. In 2017, six specimens of N. leporinus were studied for helminths. The species identification of helminths was based on morphological studies and molecular analysis of fragments of the 28S rDNA. All bat specimens were infected for at least one helminth species. Three helminth taxa were identified: the trematode Pygidiopsis macrostomum, and the nematodes Tricholeiperia cf. proencai, and Heligmonellidae gen. sp. The morphological identification of P. macrostomum was confirmed by sequence analysis of 28S rDNA gene. The phylogeny of P. macrostomum grouped our sequence with other sequences of the same species collected in Brazil. The phylogenetic tree of Heligmonellidae gen. sp. indicated that the helminth belongs to clade formed by the species Odilia bainae, Nippostrongylus magnus and Nippostrongylus brasiliensis of the family Heligmonellidae. The phylogenetic analysis of the 28S sequences of T. cf. proencai did not show any similarity or close affinity with nematodes from which that gene has been sequenced to date. The findings of the present study increase the number of helminth species parasitizing bats in Mexico., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2021

38. Exploring Neotropical anuran parasites: a morphological, life cycle and phylogenetic study of Catadiscus marinholutzi (Trematoda: Diplodiscidae).

Author

Queiroz MS, Alves PV, López-Hernández D, Anjos LA, and Pinto HA

Subjects

Animals, Brazil, DNA, Helminth analysis, DNA, Ribosomal analysis, Phylogeny, Trematoda classification, Trematoda genetics, Anura parasitology, Snails parasitology, Trematoda anatomy & histology, Trematoda growth & development

Abstract

Amphistome species belonging to the genus Catadiscus are poorly studied intestinal trematodes found primarily in Neotropical anurans. Herein, developmental stages of an amphistome species found during herpetological and malacological surveys in a temporary marsh pond from Brazil were subjected to morphological (light and scanning electron microscopy) and molecular analyses. Adult parasites recovered from anurans were identified as Catadiscus marinholutzi. Amphistome cercariae found in the planorbid snails Drepanotrema depressissimum and Drepanotrema lucidum from the same waterbody were used for experimental and molecular studies. Immature parasites, morphologically compatible with members of Catadiscus, were experimentally obtained in laboratory-reared tadpoles. Sequencing of a partial region of 28S rDNA gene of both adult and cercariae revealed 100% similarity between these developmental stages, confirming their conspecificity. Phylogenetic analyses were attempted for the first time to reveal the position of a species of Catadiscus in the superfamily Paramphistomoidea. Catadiscus marinholutzi falls in a virtual polytomy together with other paramphistomoids, which leaves its phylogenetic relationships within the group unclear. Moreover, the high genetic divergence to Diplodiscus spp. (10.06–10.84%) cast doubts on the placement of Catadiscus within Diplodiscidae. Hence the species composition of the Diplodiscidae should be re-evaluated in further studies using a broader spectrum of related taxa.

Published

2021

39. Linking genome size variation to population phenotypic variation within the rotifer, Brachionus asplanchnoidis.

Author

Stelzer CP, Pichler M, and Hatheuer A

Subjects

Animals, DNA, Helminth analysis, Population Dynamics, Rotifera embryology, Biological Variation, Population, DNA, Helminth genetics, Gene Expression Regulation, Developmental, Genome Size, Genome, Helminth, Helminth Proteins genetics, Rotifera genetics

Abstract

Eukaryotic organisms usually contain much more genomic DNA than expected from their biological complexity. In explaining this pattern, selection-based hypotheses suggest that genome size evolves through selection acting on correlated life history traits, implicitly assuming the existence of phenotypic effects of (extra) genomic DNA that are independent of its information content. Here, we present conclusive evidence of such phenotypic effects within a well-mixed natural population that shows heritable variation in genome size. We found that genome size is positively correlated with body size, egg size, and embryonic development time in a population of the monogonont rotifer Brachionus asplanchnoidis. The effect on embryonic development time was mediated partly by an indirect effect (via egg size), and a direct effect, the latter indicating an increased replication cost of the larger amounts of DNA during mitosis. Our results suggest that selection-based change of genome size can operate in this population, provided it is strong enough to overcome drift or mutational change of genome size.

Published

2021

40. Collection and DNA Detection of Dirofilaria immitis (Rhabditida Onchocercidae), Using a Novel Primer Set, in Wild-Caught Mosquitoes From Gainesville, FL.

Author

Holderman C, Abruzzo NO, Abdelsamad NA, Kaufman PE, and DiGennaro PM

Subjects

Animals, DNA, Helminth analysis, Dirofilariasis transmission, Florida, Host-Pathogen Interactions, Specimen Handling, Culicidae parasitology, Dirofilaria immitis isolation & purification, Mosquito Vectors parasitology

Abstract

Dirofilaria immitis, the causative agent of dog heartworm disease, is an important cause of canine morbidity and mortality, expensive to treat, and severe infections are often fatal. Much is known about the pathogen in the canine host, yet little is known on the basic ecology of the nematode in the mosquito vector. Thus, to evaluate the effectiveness of collection techniques on ability to capture dog heartworm-infected mosquitoes (Diptera Culicidae), we conducted a field study spanning 111 wk. Four methods were used: two aspirators types, sweep netting, and a CDC trap. All sites had canines present in either residential yards (n = 4) or dog kennel facilities (n = 3). Collected mosquitoes were sorted by site, trap, species, and date, then pooled into groups of up to 25 individuals. Mosquito head and thorax pools were extracted for DNA, that was screened using currently available protocols. These protocols were found unreliable; thus, we developed a novel qPCR primer and probe set. Using this method, the original samples were re-assayed and provided 494 positive pools. Approximately 10% of positive samples were confirmed by Sanger sequencing. Twenty-two mosquito species tested positive for dog heartworm DNA, including a new association with Wyeomyia mitchellii (Theobald). Although Aedes atlanticus (Dyar and Knab), Anopheles crucians Wiedemann, and Culiseta melanura (Coquillett) composed nearly 36% of the total collection, these species represented 42% of the qPCR positive pools. Infection rates within commonly collected mosquitoes ranged up to 2.5%, with more rarely collected species ranging up to 14%. The CDC trap was the most effective collection method at trapping infected mosquitoes., (© The Author(s) 2020. Published by Oxford University Press on behalf of Entomological Society of America.All rights reserved. For permissions, please e-mail: journals.permissions@oup.com.)

Published

2021

41. Genetic variability, cryptic species and phylogenetic relationship of six cyathostomin species based on mitochondrial and nuclear sequences.

Author

Louro M, Kuzmina TA, Bredtmann CM, Diekmann I, de Carvalho LMM, von Samson-Himmelstjerna G, and Krücken J

Subjects

Animals, DNA, Helminth analysis, DNA, Helminth genetics, DNA, Mitochondrial analysis, Genetic Variation, Germany, Horse Diseases parasitology, Horses parasitology, Intestinal Diseases, Parasitic, Parasite Egg Count veterinary, Phylogeny, Sequence Analysis, DNA, Ukraine, Cell Nucleus genetics, Mitochondria genetics, Strongyloidea classification, Strongyloidea genetics

Abstract

Cyathostomins are important intestinal nematode parasites of equines and include 50 accepted species. Their taxonomy has been frequently revised and the presence of cryptic species suggested. Furthermore, usually molecular- and morphology-based phylogenetic analyses give divergent results. In this study, the nucleotide sequences of the nuclear second internal transcribed spacer (ITS-2) and the mitochondrial partial cytochrome c oxidase subunit I (COI) were determined for adults of six cyathostomin species (Coronocyclus coronatus, Coronocyclus labiatus, Cylicocyclus nassatus, Cylicostephanus calicatus, Cylicostephanus longibursatus, Cylicostephanus minutus) collected from different equine species within two geographic regions. Maximum likelihood trees were calculated for ITS-2, COI, and concatenated data. No obvious differentiation was observed between geographic regions or equine host species. As previously reported, Coronocyclus coronatus and Cylicostephanus calicatus revealed a close relationship. Cryptic species were detected in Cylicostephanus minutus and Cylicostephanus calicatus. Cylicocyclus nassatus and Coronocyclus labiatus showed diverse mitochondrial and nuclear haplotypes occurring in different combinations, while Cylicostephanus longibursatus was comparatively homogenous. In conclusion, a combined analysis of nuclear and mitochondrial haplotypes improved resolution of the phylogeny and should be applied to the remaining cyathostomin species and across additional equine host species and geographic regions.

Published

2021

42. Evaluating DNA damage response through immunofluorescence staining of primordial germ cells in Caenorhabditis elegans L1 larva.

Author

Ou HL and Schumacher B

Subjects

Animals, Caenorhabditis elegans cytology, DNA, Helminth analysis, DNA, Helminth chemistry, Germ Cells chemistry, Germ Cells pathology, Larva cytology, Signal Transduction, DNA Damage genetics, Fluorescent Antibody Technique methods, Germ Cells cytology

Abstract

C. elegans L1 larvae have two well-defined primordial germ cells embedded in a niche comprising two somatic gonad precursor cells. Thus, C. elegans provides an ideal model for studying intercellular signaling in response to DNA damage. However, existing staining protocols are focused on worms in later developmental stages and are not optimized for the L1 larvae. Here, we present a revised protocol for assessing the DNA damage response utilizing immunofluorescence staining specifically in C. elegans L1 larva. For complete details on the use and execution of this protocol, please refer to Ou et al. (2019)., Competing Interests: The authors declare no competing interests., (© 2021 The Authors.)

Published

2021

43. Molecular confirmation of Dicrocoelium dendriticum in the Himalayan ranges of Pakistan.

Author

Khan MA, Afshan K, Nazar M, Firasat S, Chaudhry U, and Sargison ND

Subjects

Animals, DNA, Helminth analysis, DNA, Ribosomal analysis, Dicrocoeliasis parasitology, Dicrocoelium enzymology, Dicrocoelium genetics, Electron Transport Complex IV analysis, Helminth Proteins analysis, Pakistan epidemiology, Sheep, Sheep, Domestic, Dicrocoeliasis veterinary, Dicrocoelium isolation & purification, Sheep Diseases parasitology

Abstract

Lancet liver flukes of the genus Dicrocoelium (Trematoda: Digenea) are recognised parasites of domestic and wild herbivores. The aim of the present study was to confirm the species identity of Dicrocoeliid flukes collected from the Chitral valley in the Himalayan ranges of Pakistan. The morphology of 48 flukes belonging to eight host populations was examined; but overlapping traits prevented accurate species designation. Phylogenetic comparison of published D. dendriticum ribosomal cistron DNA, and cytochrome oxidase-1 (COX-1) mitochondrial DNA sequences with those from D. chinensis was performed to assess within and between species variation and re-affirm the use of species-specific single nucleotide polymorphism markers. PCR and sequencing of 34 corresponding fragments of ribosomal DNA and 14 corresponding fragments of mitochondrial DNA from the Chitral valley flukes, revealed 10 and 4 unique haplotypes, respectively. These confirmed for the first time the molecular species identity of Pakistani lancet liver flukes as D. dendriticum. This work provides a preliminary illustration of a phylogenetic approach that could be developed to study the ecology, biological diversity, and epidemiology of Dicrocoeliid lancet flukes when they are identified in new settings., (Copyright © 2020 Elsevier B.V. All rights reserved.)

Published

2021

44. First steps to understand the systematics of Echinorhynchidae Cobbold, 1876 (Acanthocephala), inferred through nuclear gene sequences.

Author

García-Varela M and Andrade-Gómez L

Subjects

Acanthocephala genetics, Animals, Cell Nucleus genetics, Female, Male, Phylogeny, Acanthocephala classification, DNA, Helminth analysis, DNA, Ribosomal analysis

Abstract

Acanthocephalans of the order Echinorhynchida are one of the most diverse groups in their phylum, with approximately 470 species classified into 11 families that largely consist of parasites of freshwater, brackish and marine fishes and, sporadically, reptiles and amphibians distributed worldwide. Previous phylogenies inferred with molecular data have supported the paraphyly or polyphyly of some families, suggesting that most of them have been diagnosed based on unique combinations of characters, rather than shared derivative features. We expand the taxonomic sampling of several genera such as Acanthocephalus, Echinorhynchus and Pseudoacanthocephalus of Echinorhynchidae from diverse biogeographical zones in the Americas, Europe and Asia with the aim of testing the monophyly of the family by using two molecular markers. Sequences from small (SSU) and large (LSU) subunits of ribosomal DNA were obtained for six species representing the genera Acanthocephalus and Echinorhynchus from the Neotropical, Nearctic, Palearctic and Oriental regions. These sequences were aligned with other sequences available in the GenBank dataset from Echinorhynchidae. Phylogenetic trees inferred with the combined (SSU + LSU) and the individual data sets consistently placed the genera Acanthocephalus, Pseudoacanthocephalus and Echinorhynchus into three independent lineages. Two families, Paracanthocephalidae Golvan, 1960, and Pseudoacanthocephalidae Petrochenko, 1956, were resurrected to accommodate the genera Acanthocephalus and Pseudoacanthocephalus, respectively. The species of the genus Acanthocephalus from the Nearctic, Palearctic and Oriental biogeographic regions formed a clade that was well supported. However, Acanthocephalus amini from the Neotropical region was nested inside Arhythmacanthidae. Therefore, the genus Calakmulrhynchus was created to accommodate A. amini and resolve the paraphyly of Acanthocephalus. Finally, the diagnoses of the families Echinorhynchidae and Arhythmacanthidae were amended. The molecular phylogenies should be used as a taxonomic framework to find shared derived characters (synapomorphies) and build a more robust classification scheme that reflects the evolutionary history of the acanthocephalans., (Copyright © 2020 Elsevier B.V. All rights reserved.)

Published

2021

45. Host-induced phenotypic plasticity in Saccocoelioides lamothei Aguirre-Macedo and Violante-González, 2008 (Digenea: Haploporidae) a parasite of freshwater, brackish and marine fishes from Middle America.

Author

González-García MT, Andrade-Gómez L, Pinacho-Pinacho CD, Sereno-Uribe AL, and García-Varela M

Subjects

Animals, Central America, DNA, Helminth analysis, DNA, Ribosomal analysis, Fresh Water parasitology, Helminth Proteins analysis, Mexico, Pacific Ocean, Phylogeny, Seawater parasitology, Trematoda classification, Trematode Infections parasitology, Adaptation, Physiological, Fish Diseases parasitology, Host-Parasite Interactions, Trematoda physiology, Trematode Infections veterinary

Abstract

Saccocoelioides is a genus of trematodes associated with fishes from the Americas. In the current research, morphologically distinct specimens of Saccocoelioides spp. were collected from six countries in Middle America. Specimens were sequenced using three molecular markers, the domains D1-D3 of the large subunit (LSU) from the nuclear rDNA, the cytochrome c oxidase subunit 1 (cox1) and nicotinamide adenine dinucleotide dehydrogenase subunit 1 (nad1) from mitochondrial DNA. A total of 74 new sequences were compared and aligned with other sequences available in GenBank. Maximum likelihood and Bayesian inference analyses were inferred from the LSU and cox1 datasets, revealing unequivocally that all the specimens correspond to S. lamothei. A haplotype network was built with 119 sequences of the nad1 gene. The network detected 57 distinct haplotypes divided into three haplogroups. To explore morphological differences among samples of S. lamothei, 17 morphological features were measured from 53 specimens from three fish families: Eleotridae, Mugilidae and Gobiidae. Principal component analysis yielded three main polygons that corresponded with each family analysed, suggesting host-induced phenotypic plasticity. The current evidence suggests that S. lamothei infects at least five fish families along the Pacific coasts of Mexico, Guatemala, El Salvador, Honduras, Nicaragua and Costa Rica.

Published

2021

46. Detecting and identifying Schistosoma infections in snails and aquatic habitats: A systematic review.

Author

Kamel B, Laidemitt MR, Lu L, Babbitt C, Weinbaum OL, Mkoji GM, and Loker ES

Subjects

Animals, DNA, Environmental analysis, DNA, Helminth analysis, Molecular Diagnostic Techniques methods, Nucleic Acid Amplification Techniques methods, Real-Time Polymerase Chain Reaction methods, Schistosoma genetics, Schistosomiasis epidemiology, Schistosomiasis prevention & control, Snails genetics, Schistosoma isolation & purification, Snails parasitology, Water parasitology

Abstract

Background: We were tasked by the World Health Organization (WHO) to address the following question: What techniques should be used to diagnose Schistosoma infections in snails and in the water in potential transmission sites? Our goal was to review and evaluate the available literature and provide recommendations and insights for the development of WHO's Guidelines Development Group for schistosomiasis control and elimination., Methodology: We searched several databases using strings of search terms, searched bibliographies of pertinent papers, and contacted investigators who have made contributions to this field. Our search covered from 1970 to Sept 2020. All papers were considered in a PRISMA (Preferred Reporting Items for Systematic Reviews and Meta-Analyses) framework, and retained papers were grouped by technique and subjected to our GRADE (Grading of Recommendations, Assessment, Development and Evaluations) evidence assessment profile determined in consultation with WHO. We also considered issues of sensitivity, specificity, coverage, cost, robustness, support needs, schistosome species discrimination, and relevant detection limits., Principal Findings: Our PRISMA process began with the perusal of 949 articles, of which 158 were retained for data extraction and evaluation. We identified 25 different techniques and for each applied a GRADE assessment considering limitations, inconsistency, imprecision, indirectness, and publication bias. We also provide advantages and disadvantages for each category of techniques., Conclusions: Our GRADE analysis returned an assessment of moderate quality of evidence for environmental DNA (eDNA), qPCR and LAMP (Loop-mediated isothermal amplification). No single ideal diagnostic approach has yet been developed, but considerable recent progress has been made. We note a growing trend to use eDNA techniques to permit more efficient and replicable sampling. qPCR-based protocols for follow-up detection offer a versatile, mature, sensitive, and specific platform for diagnosis though centralized facilities will be required to favor standardization. Droplet digital PCR (ddPCR) can play a complementary role if inhibitors are a concern, or more sensitivity or quantification is needed. Snail collection, followed by shedding, is encouraged to provide specimens for sequence verifications of snails or schistosomes. LAMP or other isothermal detection techniques offer the prospect of less expensive and more distributed network of analysis but may face standardization and verification challenges related to actual sequences amplified. Ability to detect schistosome infections in snails or in the water is needed if control and elimination programs hope to succeed. Any diagnostic techniques used need to be regularly verified by the acquisition of DNA sequences to confirm that the detected targets are of the expected species. Further improvements may be necessary to identify the ideal schistosome or snail sequences to target for amplification. More field testing and standardization will be essential for long-term success., Competing Interests: The authors have declared that no competing interests exist.

Published

2021

47. Analysis of the misdiagnosis of 8 adult cases of paragonimiasis with lung masses as the main manifestation in Xishuangbanna, Yunnan.

Author

Shu QH, Yang Y, Li SD, Zhao JS, Li SH, Wang MM, Wang WQ, Tian M, He SM, Ma ZQ, Zhu M, and Wang WL

Subjects

Animals, Antibodies, Helminth analysis, China epidemiology, DNA, Helminth analysis, Diagnosis, Differential, Diagnostic Errors, Enzyme-Linked Immunosorbent Assay, Female, Humans, Incidence, Lung parasitology, Lung Diseases, Parasitic epidemiology, Lung Diseases, Parasitic parasitology, Male, Middle Aged, Paragonimiasis drug therapy, Paragonimiasis parasitology, Paragonimus genetics, Paragonimus immunology, Retrospective Studies, Thorax pathology, Tomography, X-Ray Computed, Lung diagnostic imaging, Lung Diseases, Parasitic diagnosis, Paragonimiasis diagnosis

Abstract

Objective: To summarize the clinical characteristics of adult cases of paragonimiasis with lung masses as the main manifestation in Xishuangbanna, Yunnan Province, analyze the causes of misdiagnosis, and improve the levels of clinical diagnosis and treatment., Method: We conducted a retrospective analysis of the clinical data and diagnosis and treatment of 8 adult cases of paragonimiasis with lung masses as the main manifestation that were diagnosed in the Oncology Department of People's hospital of Xishuangbanna Dai Autonomous Prefecture from July 2014 to July 2019., Result: All 8 patients were from epidemic paragonimiasis areas and had a confirmed history of consuming uncooked freshwater crabs. The clinical manifestations were mainly fever, dry cough, and chest pain. The disease durations were long, and peripheral blood eosinophil counts were elevated. The cases had been misdiagnosed as pneumonia or pulmonary tuberculosis. After years of anti-inflammatory or anti-tuberculosis treatment, the symptoms had not improved significantly. Patients eventually sought treatment from the oncology department for hemoptysis. Chest computed tomography showed patchy consolidation in the lungs, with nodules, lung masses, and enlarged mediastinal lymph nodes., Conclusion: Paragonimiasis is a food-borne parasitic disease. Early clinical manifestations and auxiliary examination results are nonspecific. The parasite most often invades the lungs, and the resulting disease is often misdiagnosed as pneumonia, pulmonary tuberculosis, or lung cancer (Acta Trop 199: 05074, 2019). To avoid misdiagnosis, clinicians should inquire, in detail, about residence history and history of unclean food and exposure to infected water and make an early diagnosis based on the inquired information and imaging examination results. For patients who have been diagnosed with pneumonia or pulmonary tuberculosis and whose symptoms do not improve significantly after anti-inflammatory or anti-tuberculosis treatments, their epidemiological history should be traced to further conduct differential diagnosis and avoid misdiagnosis.

Published

2021

48. A Real-Time PCR Assay for the Diagnosis of Intestinal Schistosomiasis and Cure Assessment After the Treatment of Individuals With Low Parasite Burden.

Author

Siqueira LMV, Senra C, de Oliveira ÁA, Carneiro NFF, Gomes LI, Rabello A, Coelho PMZ, and Oliveira E

Subjects

Adolescent, Adult, Aged, Aged, 80 and over, Animals, Child, Child, Preschool, Cross-Sectional Studies, DNA, Helminth isolation & purification, Feces chemistry, Female, Helminths genetics, Humans, Infant, Male, Middle Aged, Oligodeoxyribonucleotides genetics, Parasite Egg Count, Schistosoma mansoni drug effects, Schistosomiasis mansoni drug therapy, Schistosomiasis mansoni parasitology, Sensitivity and Specificity, Species Specificity, Treatment Outcome, Young Adult, Anthelmintics therapeutic use, DNA, Helminth analysis, Feces parasitology, Praziquantel therapeutic use, Real-Time Polymerase Chain Reaction methods, Schistosoma mansoni isolation & purification, Schistosomiasis mansoni diagnosis

Abstract

The laboratorial diagnosis of the intestinal schistosomiasis is always performed using Kato-Katz technique. However, this technique presents low sensitivity for diagnosis of individuals with low parasite burden, which constitutes the majority in low endemicity Brazilian locations for the disease. The objective of this study was developed and to validate a real-time PCR assay (qPCR) targeting 121 bp sequence to detect Schistosoma spp. DNA for the diagnosis of intestinal schistosomiasis and a sequence of the human β-actin gene as internal control. Firstly, the qPCR was standardized and next it was evaluated for diagnosis and cure assessment of intestinal schistosomiasis in the resident individuals in Tabuas and Estreito de Miralta, two locations in Brazil endemic for intestinal schistosomiasis. The qPCR assay results were compared with those of the Kato-Katz (KK) test, examining 2 or 24 slides, Saline Gradient (SG) and "reference test" (24 KK slides + SG). The cure assessment was measured by these diagnostic techniques at 30, 90, and 180 days post-treatment. In Tabuas, the positivity rates obtained by the qPCR was 30.4% (45/148) and by "reference test" was of 31.0% (46/148), with no statistical difference (p = 0.91). The presumed cure rates at 30, 90, and 180 days post-treatment were 100, 94.4, and 78.4% by the analysis of 24 KK slides, 100, 94.4, and 78.4% by the SG, and 100, 83.3, and 62.1% by the qPCR assay. In Estreito de Miralta, the positivity obtained by qPCR was 18.3% (26/142) and with "reference test" was 24.6% (35/142), with no statistical difference (p = 0.20). The presumed cure rates were 93.3, 96.9, and 96.5% by the KK, 93.3, 96.9, and 100% by the SG, and 93.3, 93.9, and 96.5% by the qPCR at 30, 90, and 180 days post-treatment, respectively. This study showed that the diagnostic techniques presented different performance in the populations from the two districts (Tabuas and Estreito de Miralta) and reinforces the need of combining techniques to improve diagnosis accuracy, increasing the detection of individuals with low parasite burden. This combination of techniques consists an important strategy for controlling the disease transmission., Competing Interests: The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2021 Siqueira, Senra, de Oliveira, Carneiro, Gomes, Rabello, Coelho and Oliveira.)

Published

2021

49. Morphological and molecular analysis of Henneguya lagunensis n. sp. (Cnidaria, Myxosporea) parasitizing the gills of Eugerres brasilianus from Brazil.

Author

de Azevedo RK, Negrelli DC, de Oliveira CP, Abdallah VD, Camara JPS, Matos ER, and Vieira DHMD

Subjects

Animals, Brazil, DNA, Helminth analysis, DNA, Ribosomal analysis, Phylogeny, Fish Diseases parasitology, Myxozoa anatomy & histology, Myxozoa genetics, Parasitic Diseases, Animal parasitology, Perciformes

Abstract

Plasmodia containing myxospores belonging to the genus Henneguya Thélohan, 1892 were found in the gills of Eugerres brasilianus (Cuvier, 1830). Despite the economic importance, few parasitological studies have been done with this species. We describe Henneguya lagunensis n. sp. using morphological and molecular data. The mature myxospores were rounded, measuring 29.1 ± 2.2 μm in total length, 8.2 ± 1.0 μm in body length, 7.9 ± 0.2 μm in body width, 20.7 ± 2.4 μm in tail length and 4.8 ± 1.0 μm in thickness. The polar capsules measured 3.3 ± 0.4 in length and 1.7 ± 0.3 μm in width. Polar filaments had 4-5 turns, helical. Phylogenetic analysis showed Henneguya lagunensis n. sp. as a sister species of Henneguya cynoscioni Dyková, Buron, Roumillat and Fiala, 2011, within a clade that contained mostly Henneguya species that parasitize marine fish of the order Perciformes. This is the first report of a species of Henneguya parasitizing Eugerres brasilianus., (Copyright © 2020 Elsevier B.V. All rights reserved.)

Published

2021

50. Morphological and molecular characterization of larval digenean trematodes (Parvatrema: Gymnophallidae) and their pathological effects on the clam Leukoma thaca (=Protothaca thaca) (Bivalvia:Veneridae) (Molina, 1782) from northern Chile.

Author

Montenegro D, Romero MS, and González MT

Subjects

Animals, Cercaria anatomy & histology, Cercaria genetics, Cercaria growth & development, Cercaria ultrastructure, Chile, DNA, Helminth analysis, DNA, Ribosomal analysis, Metacercariae anatomy & histology, Metacercariae genetics, Metacercariae growth & development, Metacercariae ultrastructure, Microscopy, Electron, Scanning, Trematoda anatomy & histology, Trematoda genetics, Trematoda ultrastructure, Bivalvia parasitology, Trematoda isolation & purification

Abstract

Trematodes are one of the largest taxa of mollusk parasites. The clam Leukoma thaca is an economically exploited bivalve found along the south-eastern Pacific coast of Peru and Chile. This bivalve is parasitized by various unidentified larval stages of digeneans in the mantle, gonads and digestive gland. The aims of this study were to determine and describe the different larval stages of the digeneans based on morphological characteristics, to identify them at the species level by performing molecular analyses, and to evaluate pathologies associated with the parasites of this clam. Individuals of L. thaca were collected in San Jorge Bay (23°S), Chile, between November 2018 and February 2019. Morphological description was carried out using in vivo and fixed specimens, and analyses including histological and scanning electron microscopy were performed. Individuals were also isolated for molecular analysis using nuclear ribosomal internal transcribed spacer 1 (ITS1), including partial subunit 18S rDNA (18S) and small subunit 5.8S gene (5.8S). Morphological characteristics indicated that the metacercaria larval stage belongs to the family Gymnophallidae, genus Parvatrema, which was supported by molecular analysis. Molecular results revealed that metacercaria, sporocysts and cercaria stages found in this clam belong to the same species of Parvatrema (genetic distance 0%), evidencing that this species uses L. thaca as the first and second intermediate host. Pathologies examined in the host were similar in nature to those reported in other gymnophallids in bivalves, but high prevalence of cercariae (20%) in gonads suggested an important castrator effect on the host., (Copyright © 2020 Elsevier B.V. All rights reserved.)

Published

2021