Search

Your search keyword '"Tejangkura, T."' showing total 22 results
Start Over Author "Tejangkura, T."
22 results on '"Tejangkura, T."'

2. Permanent genetic resources added to Molecular Ecology Resources Database 1 April 2010-31 May 2010

Author

Andree, K., Axtner, J., Bagley, M. J., Barlow, E. J., Beebee, T. J. C., Bennetzen, J. L., Bermingham, E., Boisselier-Dubayle, M. C., Bozarth, C. A., Brooks, C. P., Brown, R. P., Catanese, G., Cavers, S., Ceron-Souza, I., Chak, S. T. C., Chan, M. N., Charles-Dominique, P., Chen, C. Y., Chen, J. D., Chinchilla, L., Da Silva, D., Dafreville, S., Daunt, F., Delatte, H., Dorge, T., Duncan, N., Durand, Jean-Dominique, Duvernell, D., Estep, M., Fan, S., Fattahi, R., Villela, O. F., Fong, Y., Freville, H., Funes, V., Gallardo-Escarate, C., Ganeshaiah, K. N., Ghaffari, M. R., Girod, C., Gomez-Moliner, B. J., Gonzalez-Porter, G. P., Gosa, A., Govers, F., Guerin, F., Guindo, D., Hailer, F., Haye, P. A., Hoelmer, K. A., Hofmann, S., Hong, Y., Hu, C. Q., Huang, S. W., Humeau, L., Infante, C., Jackson, S. A., Jacobsen, E., Jowkar, A., Kafi, M., Kermani, M. J., Kim, H., Kim, K. S., Kim, M. Y., Knibb, W., Koita, O. A., Korpelainen, H., Lambourdiere, J., Lasso, E., Leblois, R., Lee, H., Lee, S. W., Leung, F. C. C., Leung, K. M. Y., Li, C. H., Li, Y., Lieckfeldt, D., Lizana, M., Loughry, W. J., Luo, P., Madeira, M. J., Mahmoodi, P., Maldonado, J. E., Mardi, M., Mendes, O., Miehe, G., Muth, P., Nacci, D., Kumar, L. N., Ng, W. C., Pailler, T., Parzies, H. K., Perez, L., Pfunder, M., Pietilaeinen, M., Pirseyedi, S. M., Porta, D., Porta, J., Porta, J. M., Quilici, S., Rakotoarivelo, F. P., Ramesha, B. T., Ravikanth, G., Riera, B., Risterucci, A. M., Roberts, D. A., Samadi, Sarah, Sarasola-Puente, V., Sarrazin, E., Sarthou, C., Schmidt, A., Segovia, N. I., Shen, K. N., Simiand, C., Bin Sman, M. H., Solhoy, T., Sommer, S., Sumangala, R. C., Taubert, R., Tejangkura, T., Telford, A., Testa, A., Tollon-Cordet, C., Tzeng, W. N., Shaanker, R. U., van der Lee, T. A. J., Van Mourik, T. A., Vasudeva, R., Wai, T. C., Wang, R. L., Welch, M. E., Weltzien, E., Whitehead, A., Woodard, A., Xia, J. J., Zeinolabedini, M., and Zhang, L.

Abstract

This article documents the addition of 396 microsatellite marker loci to the Molecular Ecology Resources Database. Loci were developed for the following species: Anthocidaris crassispina, Aphis glycines, Argyrosomus regius, Astrocaryum sciophilum, Dasypus novemcinctus, Delomys sublineatus, Dermatemys mawii, Fundulus heteroclitus, Homalaspis plana, Jumellea rossii, Khaya senegalensis, Mugil cephalus, Neoceratitis cyanescens, Phalacrocorax aristotelis, Phytophthora infestans, Piper cordulatum, Pterocarpus indicus, Rana dalmatina, Rosa pulverulenta, Saxifraga oppositifolia, Scomber colias, Semecarpus kathalekanensis, Stichopus monotuberculatus, Striga hermonthica, Tarentola boettgeri and Thermophis baileyi. These loci were cross-tested on the following species: Aphis gossypii, Sooretamys angouya, Euryoryzomys russatus, Fundulus notatus, Fundulus olivaceus, Fundulus catenatus, Fundulus majalis, Jumellea fragrans, Jumellea triquetra Jumellea recta, Jumellea stenophylla, Liza richardsonii, Piper marginatum, Piper aequale, Piper darienensis, Piper dilatatum, Rana temporaria, Rana iberica, Rana pyrenaica, Semecarpus anacardium, Semecarpus auriculata, Semecarpus travancorica, Spondias acuminata, Holigarna grahamii, Holigarna beddomii, Mangifera indica, Anacardium occidentale, Tarentola delalandii, Tarentola caboverdianus and Thermophis zhaoermii.

Published
2010

3. Permanent Genetic Resources added to Molecular Ecology Resources Database 1 April 2010 – 31 May 2010: Isolation and characterization of microsatellite markers for the European shag, Phalacrocorax aristotelis.

Author

Andree, K., Axtner, Jan, Bagley, M.J., Barlow, E.J., Beebee, T.J.C., Bennetzen, Jeffrey L., Bermingham, Eldredge, Boisselier-Dubayle, M.C., Bozart, Christine A., Brooks, Christopher P., Brown, R.P., Catanese, Gaetano, Cavers, S., Ceron-Souza, Ivania, Chak, Solomon T.C., Chan, M.N., Charles-Dominique, P., Chen, C.Y., Chen, J.D., Chinchilla, Leah, Da Silva, D., Dafreville, S., Daunt, F., Delatte, H., Dorge, T., Duncan, N., Durand, J.D., Duvernell, D., Estep, Matt, Fan, Sigang, Fattahi, R., Villela, Oscar Flores, Fong, Yokking, Freville, H., Funes, Victoria, Gallardo-Escarte, C., Ganeshaiah, K.N., Ghaffari, M.R., Girod, C., Gomez-Moliner, B.J., Gonzalez-Porter, Gracia P., Gosa, A., Govers, F., Guerin, F., Guindo, Diarah, Hailer, Frank, Haye, P.A., Hoelmer, Kim A., Hofmann, S., Hong, Yan, Hu, Chaoqun, Huang, S.W., Humeau, L., Infante, Carlos, Jackson, S.A., Jacobsen, E., Jowkar, A., Kafi, M., Kermani, J., Kim, Hyojoong, Kim, Kyung Seok, Knibb, W., Koita, Ousmane A., Korpelainen, H., Lambourdiere, J., Lasso, Eloisa, Leblois, R., Lee, Hang, Lee, Seunghwan, Leung, F.C.C., Leung, Kenneth M.Y., Li, Chunjong, Li, Y., Lieckfeldt, Dietmar, Lizana, M., Loughry, W.J., Luo, Peng, Madeira, M.J., Mahmoodi, P., Maldonado, Jesus E., Mardi, M., Mendes, O., Miehe, G., Muth, Peter, Nacci, D., Kumar, Naveen, Ng, Wai-Chuen, Pailler, T., Parzies, Heiko K., Perez, Laura, Pfunder, M., Pietilainen, M., Pirseyedi, S.M., Porta, D., Porta, J., Porta, J.M., Quilici, S., Rakotoarivelo, F.P., Ramesha, B.T., Ravikanth, G., Riera, B., Risterucci, A.M., Roberts, D.A., Samadi, S., Sarasola-Puente, V., Sarrazin, E., Sarthou, C., Schmidt, Anke, Segovia, N.I., Shen, K.N., Simiand, C., Sman, Muhammad Hidayat Bin, Solhoy, T., Sommer, Simone, Sumangala, R.C., Taubert, Ramona, Tejangkura, T., Telford, A., Testa, A., Tollon-Cordet, C., Tzeng, W.N., Uma-Shaanker, R., Van Der Lee, T.A.J., Van Mourik, Thomas A., Vasudeva, R., Wai, T.C., Wang, R.L., Welch, Mark E., Weltzein, Eva, Whitehead, A., Woodard, Anastasia, Xia, Jianjun, Zeinolabedini, M., Zhang, Lvping, Andree, K., Axtner, Jan, Bagley, M.J., Barlow, E.J., Beebee, T.J.C., Bennetzen, Jeffrey L., Bermingham, Eldredge, Boisselier-Dubayle, M.C., Bozart, Christine A., Brooks, Christopher P., Brown, R.P., Catanese, Gaetano, Cavers, S., Ceron-Souza, Ivania, Chak, Solomon T.C., Chan, M.N., Charles-Dominique, P., Chen, C.Y., Chen, J.D., Chinchilla, Leah, Da Silva, D., Dafreville, S., Daunt, F., Delatte, H., Dorge, T., Duncan, N., Durand, J.D., Duvernell, D., Estep, Matt, Fan, Sigang, Fattahi, R., Villela, Oscar Flores, Fong, Yokking, Freville, H., Funes, Victoria, Gallardo-Escarte, C., Ganeshaiah, K.N., Ghaffari, M.R., Girod, C., Gomez-Moliner, B.J., Gonzalez-Porter, Gracia P., Gosa, A., Govers, F., Guerin, F., Guindo, Diarah, Hailer, Frank, Haye, P.A., Hoelmer, Kim A., Hofmann, S., Hong, Yan, Hu, Chaoqun, Huang, S.W., Humeau, L., Infante, Carlos, Jackson, S.A., Jacobsen, E., Jowkar, A., Kafi, M., Kermani, J., Kim, Hyojoong, Kim, Kyung Seok, Knibb, W., Koita, Ousmane A., Korpelainen, H., Lambourdiere, J., Lasso, Eloisa, Leblois, R., Lee, Hang, Lee, Seunghwan, Leung, F.C.C., Leung, Kenneth M.Y., Li, Chunjong, Li, Y., Lieckfeldt, Dietmar, Lizana, M., Loughry, W.J., Luo, Peng, Madeira, M.J., Mahmoodi, P., Maldonado, Jesus E., Mardi, M., Mendes, O., Miehe, G., Muth, Peter, Nacci, D., Kumar, Naveen, Ng, Wai-Chuen, Pailler, T., Parzies, Heiko K., Perez, Laura, Pfunder, M., Pietilainen, M., Pirseyedi, S.M., Porta, D., Porta, J., Porta, J.M., Quilici, S., Rakotoarivelo, F.P., Ramesha, B.T., Ravikanth, G., Riera, B., Risterucci, A.M., Roberts, D.A., Samadi, S., Sarasola-Puente, V., Sarrazin, E., Sarthou, C., Schmidt, Anke, Segovia, N.I., Shen, K.N., Simiand, C., Sman, Muhammad Hidayat Bin, Solhoy, T., Sommer, Simone, Sumangala, R.C., Taubert, Ramona, Tejangkura, T., Telford, A., Testa, A., Tollon-Cordet, C., Tzeng, W.N., Uma-Shaanker, R., Van Der Lee, T.A.J., Van Mourik, Thomas A., Vasudeva, R., Wai, T.C., Wang, R.L., Welch, Mark E., Weltzein, Eva, Whitehead, A., Woodard, Anastasia, Xia, Jianjun, Zeinolabedini, M., and Zhang, Lvping

Abstract

This article documents the addition of 396 microsatellite marker loci to the Molecular Ecology Resources Database. Loci were developed for the following species: Anthocidaris crassispina, Aphis glycines, Argyrosomus regius, Astrocaryum sciophilum, Dasypus novemcinctus, Delomys sublineatus, Dermatemys mawii, Fundulus heteroclitus, Homalaspis plana, Jumellea rossii, Khaya senegalensis, Mugil cephalus, Neoceratitis cyanescens, Phalacrocorax aristotelis, Phytophthora infestans, Piper cordulatum, Pterocarpus indicus, Rana dalmatina, Rosa pulverulenta, Saxifraga oppositifolia, Scomber colias, Semecarpus kathalekanensis, Stichopus monotuberculatus, Striga hermonthica, Tarentola boettgeri and Thermophis baileyi. These loci were cross-tested on the following species: Aphis gossypii, Sooretamys angouya, Euryoryzomys russatus, Fundulus notatus, Fundulus olivaceus, Fundulus catenatus, Fundulus majalis, Jumellea fragrans, Jumellea triquetra Jumellea recta, Jumellea stenophylla, Liza richardsonii, Piper marginatum, Piper aequale, Piper darienensis, Piper dilatatum, Rana temporaria, Rana iberica, Rana pyrenaica, Semecarpus anacardium, Semecarpus auriculata, Semecarpus travancorica, Spondias acuminata, Holigarna grahamii, Holigarna beddomii, Mangifera indica, Anacardium occidentale, Tarentola delalandii, Tarentola caboverdianus and Thermophis zhaoermii.

Published
2010

8. Hybrid zone genetics and within-island diversity of the gecko Tarentola boettgeri

Author

Tejangkura, T

Subjects
QL, GE, QH426
Abstract

This study builds on a previous study that demonstrates the existence of deep mitochondrial lineages in the gecko Tarentola boettgeri within Gran Canaria (Gubitz et al. 2005). Here, I identified and analyzed the area where the two most divergent mitochondrial •lineages meet. The primary aim was to examine how geographical structuring of mtDNA has been maintained after secondary contact. MtDNA analyses used a 608 basepair fragment of the cytochrome b (cyt b) gene from 389 individuals sampled from 14 populations along a 32 km southeast (SE) transect across Gran Canaria. It revealed a low degree of mtDNA admixture and negligible gene flow across the contact zone. This led to the hypothesis that reproductive barriers may have formed between populations from different mtDNA lineages. Analyses of seven body dimension and scalation characters revealed that spatial patterns of morphological changes were not associated with the transition in mtDNA lineage frequency across the transect. This contrasted with another lizard species on the same island, Chalcides sexlineatus, in which phylogeography and morphology are highly correlated. This study identified ten unique microsatellite markers in T. boettgeri. Like morphology, analyses of these microsatellites did not reveal a pronounced spatial pattern of differentiation in the nuclear genome. These results appear to reject the hypothesis of a physical or genetic barrier to reproduction. Studies of micro satellites also suggested that T. boettgeri is a low dispersal species and this might explain the persistence of mtDNA contact zone. However, evidence of concordant spatial patterns between divergence in the nuclear genome and morphology was detected. The discordant spatial patterns of mitochondrial and nuclear genotype frequencies do not appear to be explained by sex-biased gene flow, and are difficult to understand because of expected interactions between the two genomes. Thus, further investigation is suggested to allow clarification of the causes of mito-nuclear discordance in T. boettgeri.

9. A simple color absorption analysis of colorimetric loop-mediated isothermal amplification for detection of Raillietina spp. in clinical samples using a 3D-printed tube holder coupled with a smartphone camera and notebook screen.

Author

Panich W, Puttharugsa C, Tejangkura T, and Chontananarth T

Subjects
Animals, Limit of Detection, Rosaniline Dyes chemistry, Molecular Diagnostic Techniques instrumentation, Molecular Diagnostic Techniques methods, Feces chemistry, Feces microbiology, Colorimetry methods, Colorimetry instrumentation, Nucleic Acid Amplification Techniques methods, Smartphone, Printing, Three-Dimensional, Chickens
Abstract

A simple method has been developed for semi-quantitative analysis of the colorimetric output of loop-mediated isothermal amplification (LAMP) using a 3D-printed tube holder with a smartphone and notebook for the detection of Raillietina, which is the cause of Raillietiniasis affecting free-range chicken farming. In this method, a light is directed from a notebook screen to the LAMP products in the tube holder and the color absorption of the LAMP products is measured by using the appropriate smartphone application. It was found that the malachite green dye-coupled LAMP (MaG-LAMP) assay showed the highest sensitivity and specificity for detecting Raillietina without any cross-reaction with other related parasites and hosts. The limit of detection was 10 fg/μL of DNA. A total of 60 fecal samples were infectively confirmed by microscopic examination and the results of microscopy compared with those of MaG-LAMP and triplex PCR assays. Microscopy and MaG-LAMP based on the color absorption demonstrated high agreement in Raillietina detection with kappa = 1. Rapid, simple, cost-effective, and easy interpretation of colorimetric LAMP assays and their high sensitivity make them superior to PCR and morphological investigation, demonstrating the feasibility of this assay in point-of-care screening to support farm management and solve chicken health problems. Our study presents is an alternative diagnostic method using semi-quantitative analysis of colorimetric LAMP based on the differing solution color absorptions between positive and negative reactions for infectious disease diagnosis., (© 2024. The Author(s), under exclusive licence to Springer-Verlag GmbH Austria, part of Springer Nature.)

Published
2024
Full Text
View/download PDF

10. Development and utilization of a visual loop-mediated isothermal amplification coupled with a lateral flow dipstick (LAMP-LFD) assay for rapid detection of Echinostomatidae metacercaria in edible snail samples.

Author

Panich W, Jaruboonyakorn P, Raksaman A, Tejangkura T, and Chontananarth T

Subjects
Animals, Echinostomatidae isolation & purification, Echinostomatidae genetics, Echinostomatidae classification, Thailand, Sensitivity and Specificity, Molecular Diagnostic Techniques methods, Food Parasitology, Nucleic Acid Amplification Techniques methods, Snails parasitology
Abstract

Trematodes belonging to the family Echinostomatidae are food-borne parasites which cause echinostomiasis in animals and humans. This is a global public health issue, particularly in East and Southeast Asia. A method to detect the infective stage of Echinostomatidae species is required to prevent transmission to humans. In this study, a loop-mediated isothermal amplification coupled with a lateral flow dipstick (LAMP-LFD) assay was developed for visual detection of the metacercarial stage in edible snails of the genus Filopaludina from local markets in Thailand. The LAMP-LFD method can be performed within 70 min at a consistent temperature of 66 °C, and the results can be interpreted with the naked eye. The detection limits of the assay using Echinostoma mekongi, E. macrorchis, E. miyagawai and Hypoderaeum conoideum genomic DNA were equal between the four species at 50 pg/μL. A specificity evaluation demonstrated that the LAMP-LFD assay had no cross-reaction with another parasite (Thapariella species) or with the snail host species (Filopaludina martensi martensi, F. sumatrensis speciosa, and F. s. polygramma). Clinical test assessments were compared to microscopic examination in 110 edible snail samples. The clinical sensitivity and specificity of the tests were 84.62 % and 100 %, respectively, with a strong level of agreement based on the kappa statistic and the results of both methods were not significantly different (p > 0.05) per McNemar's test. The test successfully developed in this study may be useful for the detection of the metacercarial stage in edible snails for epidemiological investigations, control, surveillance, and to prevent future echinostomiasis health issues., 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
Full Text
View/download PDF

11. Assay for the simultaneous detection of Raillietina spp. (R. echinobothrida, R. tetragona, and R. cesticillus) and Ascaridia galli infection in chickens using duplex loop-mediated isothermal amplification integrated with a lateral flow dipstick assay.

Author

Panich W, Tejangkura T, and Chontananarth T

Subjects
Animals, Feces parasitology, Molecular Diagnostic Techniques veterinary, Molecular Diagnostic Techniques methods, Chickens parasitology, Nucleic Acid Amplification Techniques veterinary, Nucleic Acid Amplification Techniques methods, Poultry Diseases parasitology, Poultry Diseases diagnosis, Ascaridia isolation & purification, Ascaridia genetics, Ascaridiasis veterinary, Ascaridiasis diagnosis, Ascaridiasis parasitology, Sensitivity and Specificity
Abstract

Raillietina species and Ascaridia galli are two of the significant intestinal parasites that affect chickens in a free-range system production. They destroy the intestinal mucosa layer, leading to several clinical symptoms such as weight loss, a slowed growth rate, and economic value loss. Thus, the objective of this study was to develop an assay for simultaneously detecting Raillietina spp. (R. echinobothrida, R. tetragona, and R. cesticillus) and A. galli in a single reaction using duplex loop-mediated isothermal amplification (dLAMP) coupled with a lateral flow dipstick (LFD) assay. The analytical specificity of the dLAMP-LFD assay showed a high specific amplification of Raillietina spp. and A. galli without non-target amplification. Regarding the analytical sensitivity, this approach was capable of simultaneously detecting concentrations as low as 5 pg/μL of mixed-targets. To evaluate the efficiency of the dLAMP assay, 30 faecal samples of chickens were verified and compared through microscopic examination. The dLAMP-LFD assay and microscopic examination results showed kappa values of Raillietina spp. and A. galli with moderate (K= 0.615) to high (K= 1) agreements, respectively, while the McNemar's test indicated that the efficiency between assays was not significantly different. Therefore, the developed dLAMP-LFD assay can be used as an alternative screening method to the existing classical method for epidemiological investigation, epidemic control, and farm management, as well as for addressing poultry health problems., 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
Full Text
View/download PDF

12. Evaluation of semi-quantitative colorimetric assays based on loop-mediated isothermal amplification indicators by using image analysis.

Author

Panich W, Nak-On S, Sabaijai M, Raksaman A, Puttharugsa C, Tejangkura T, and Chontananarth T

Subjects
Humans, Coloring Agents, Molecular Diagnostic Techniques, Colorimetry methods, Nucleic Acid Amplification Techniques methods
Abstract

Colorimetric assays are some of the most convenient detection methods, creating discoloration in solutions that is visible to the naked eye. However, colorimetric reactions have some limitations regarding the variability in the color perception of individuals caused by factors such as color blindness, experience, and gender. Semi-quantitative chromatic analysis has been used as an alternative method to differentiate between two colors and accurately interpret the results from a numerical value, with high confidence. Therefore, we developed and determined the optimal model between Red-Green-Blue (RGB) and Commission Internationale de l'Eclairage (CIE) Lab color spaces to establish a semi-quantitative colorimetric assay via image analysis by the ImageJ program for loop-mediated isothermal amplification (LAMP), using the dyes malachite green and phenol red. The semi-quantitative colorimetric assays using the color distance values of the CIELab color space (ΔE ab ) were more suitable than those using the RGB color space (ΔE RGB ) for chromatic differentiation between positive and negative reactions in both indicator dyes, demonstrating the feasibility of this assay to be applied in the detection of a wide range of pathogens and infectious diseases., 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 Inc. All rights reserved.)

Published
2024
Full Text
View/download PDF

13. Visualization and development of colorimetric loop-mediated isothermal amplification for the rapid detection and diagnosis of paramphistome infection: colorimetric PAR-LAMP.

Author

Nak-On S, Sabaijai M, Raksaman A, Panich W, Tejangkura T, and Chontananarth T

Subjects
Animals, Sensitivity and Specificity, DNA, Colorimetry methods, Nucleic Acid Amplification Techniques methods, Rosaniline Dyes, Molecular Diagnostic Techniques
Abstract

Colorimetric detection can be applied to differentiate between positive and negative conditions. It can be coupled with loop-mediated isothermal amplification to diagnose rumen fluke or paramphistome infection, also called colorimetric PAR-LAMP. This study conducted LAMP using three candidate indicator dyes, namely malachite green (MLG), methyl green (MTG), and neutral red (NTR), and the results were observed by the naked eye. The dye concentration was optimized to obtain the most pronounced positive-negative result discrimination. Subsequently, we conducted target sensitivity tests using the DNA of Fischoederius elongatus at different concentrations. To validate the detection accuracy, the result was confirmed by gel electrophoresis. The sensitivity test presented the lowest detectable DNA concentration or limit of detection (LOD), with 1 pg for MLG, 0.5 ng for MTG, and 50 pg for NTR. Different LODs revealed inhibition of LAMP reaction and reduced efficiency of result presentation for colorimetric-based detection, particularly NTR and MTG. For MLG-LAMP, we observed no cross-reaction of non-target DNA and improved reaction with the DNA of Fischoederius cobboldi and Calicophoron sp., with multi-detection. In addition, naked eye observation and agarose gel electrophoresis (AGE) evaluation of the MLG-LAMP results showed a moderate and strong agreement with LAMP-AGE and microscopic examinations. Based on our results, colorimetric PAR-LAMP is a rapid, comfortable, and point-of-care procedure for the diagnosis of paramphistome infection., (© 2024. The Author(s), under exclusive licence to Springer-Verlag GmbH Germany, part of Springer Nature.)

Published
2024
Full Text
View/download PDF

14. Feasibility of a DNA biosensor assay based on loop-mediated isothermal amplification combined with a lateral flow dipstick assay for the visual detection of Ascaridia galli eggs in faecal samples.

Author

Panich W, Tejangkura T, and Chontananarth T

Subjects
Animals, Feasibility Studies, Ovum, Feces parasitology, DNA, Ascaridia, Chickens parasitology
Abstract

Ascaridia galli is an important nematode that causes ascaridiasis in free-range and indoor system chicken farms. Infection with A. galli may damage the intestinal mucosa and inhibit nutrient absorption, leading to a reduced growth rate, weight loss and a decreased egg production. Consequently, A. galli infection is a significant health problem in chickens. In this study, we developed a loop-mediated isothermal amplification coupled with a lateral flow dipstick (LAMP-LFD) assay for the visual detection of A. galli eggs in faecal samples. The LAMP-LFD assay consists of six primers and one DNA probe that recognize the internal transcribed spacer 2 (ITS2) region; it can be performed within 70 min and the results can be interpreted with the naked eye. Using the LAMP-LFD assay developed in this study, A. galli DNA was specifically amplified without any cross-reactions with other related parasites ( Heterakis gallinarum , Raillietina echinobothrida , R. tetragona , R. cesticillus , Cotugnia sp., Echinostoma miyagawai ) and definitive hosts ( Gallus gallus domesticus , Anas platyrhynchos domesticus ). The minimum detectable DNA concentration was 5 pg/μl, and the detectable egg count was 50 eggs per reaction. The assay can be performed in a water bath, without the need for post-mortem morphological investigations and laboratory instruments. It is therefore a viable alternative for the detection of A. galli in chicken faeces and can replace classical methods in field screening for epidemiological investigations, veterinary health and poultry farming management. RESEARCH HIGHLIGHTS This is the first study using the LAMP-LFD assay for Ascaridia galli detection.The results can be observed by the naked eye.The developed assay can be used to detect Ascaridia galli eggs in faecal samples.

Published
2023
Full Text
View/download PDF

15. Multi-detection for paramphistomes using novel manually designed PAR-LAMP primers and its application in a lateral flow dipstick (LAMP-LFD) system.

Author

Nak-On S, Tejangkura T, and Chontananarth T

Subjects
Animals, Cattle, Sensitivity and Specificity, Thailand, Base Sequence, DNA Primers genetics, Nucleic Acid Amplification Techniques veterinary, Biological Assay veterinary
Abstract

Loop-mediated isothermal amplification (LAMP) has been applied for the detection of various parasites, and its application in lateral flow dipstick (LFD) can improve the convenience of point-of-care diagnosis. A novel PAR-LAMP probe and primers were designed by manual selection from a region of low variation in the ITS-2 DNA sequence. Up to six species of rumen fluke were detected by LAMP and LAMP-LFD in this study. Target specificity and sensitivity were tested, revealing a high target specificity (accuracy) and a low limit of detection (sensitivity). Different target sensitivities of paramphistome were presented, including 5 pg for Gastrothylax crumenifer and Carmyerius sp.; 1 pg for Fischoederius elongatus, Orthocoelium parvipapillatum, and O. dicranocoelium; and 0.1 pg for Paramphistomum epiclitum. LAMP-LFD can detect a paramphistome egg even in contaminated in feces that was spiked with the egg under laboratory conditions. In addition, natural paramphistome infection in cattle from Surat Thani and Khon Kaen provinces, Thailand, was evaluated by detection of egg contamination in fecal specimens using PAR-LAMP primers. The PAR-LAMP detection result was also statistically evaluated by microscopic examination of feces. This study presents the application of novel manually designed primers in a LAMP-LFD system for improving performance in detection and diagnosis assays for paramphistomosis., Competing Interests: Declaration of Competing Interest The authors declare the following financial interests/personal relationships which may be considered as potential competing interests: The primers in this study were described in form of approving patent number 2203001221 by department of intellectual property (DIP), Thailand., (Copyright © 2023 Elsevier B.V. All rights reserved.)

Published
2023
Full Text
View/download PDF

16. Novel high-performance detection of Raillietina echinobothrida, Raillietina tetragona, and Raillietina cesticillus using loop-mediated isothermal amplification coupled with a lateral flow dipstick (LAMP-LFD).

Author

Panich W, Tejangkura T, and Chontananarth T

Subjects
Animals, Cestoda classification, Cestoda genetics, DNA, Helminth genetics, RNA, Helminth genetics, RNA, Ribosomal, 28S genetics, Species Specificity, Cestoda isolation & purification, Molecular Diagnostic Techniques methods, Nucleic Acid Amplification Techniques methods
Abstract

Cestodes belonging to the genus Raillietina are a major veterinary health problem in the poultry industry, especially in chickens (Gallus gallus domesticus) and ducks (Anas playtrhynchos domesticus). In this study, loop-mediated isothermal amplification coupled with a lateral flow dipstick (LAMP-LFD) assay was established and validated for the detection of R. echinobothrida, R. tetragona, and R. cesticillus in one reaction. The LAMP-LFD assay can be completed in 75 min under isothermal conditions at 66 °C and the results can be obtained by observation with the naked eye. This assay was very specific and had no cross-amplification with other closely related parasites (Cotugnia sp., Diorchis formosensis, Fimbriaria sp., Echinostoma sp., E. miyagawai, Hypoderaeum conoideum, Prosthogonimus cuneatus, and Ascaridia galli) or their definitive hosts (G. g. domesticus, A. p. domesticus). The sensitivity of the LAMP-LFD assay was detected with three Raillietina species at 0.5 ng, which was enough for gravid proglottid DNA detection. The accuracy test showed that the LAMP-LFD assay demonstrated accurate verification results when compared to morphological results. This is a novel LAMP-LFD assay that is highly specific and sensitive for the detection of Raillietina species. It can be applied to detection for epidemiological investigations, monitoring programs, surveillance, control, and to solve veterinary health problems for the poultry industry in Raillietina endemic areas., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published
2021
Full Text
View/download PDF

17. Molecular classification of rumen fluke eggs in fecal specimens from Suphanburi Province, Thailand, based on cytochrome C oxidase subunit 1.

Author

Anucherngchai S, Chontananarth T, Tejangkura T, and Wongsawad C

Subjects
Animals, Cattle, Cattle Diseases epidemiology, Cattle Diseases parasitology, Cattle Diseases prevention & control, DNA Barcoding, Taxonomic methods, Electron Transport Complex IV analysis, Feces parasitology, Helminth Proteins analysis, Ovum, Polymerase Chain Reaction veterinary, Rumen parasitology, Thailand epidemiology, Trematoda classification, Trematode Infections diagnosis, Trematode Infections parasitology, Trematode Infections prevention & control, Cattle Diseases diagnosis, DNA Barcoding, Taxonomic veterinary, Epidemiological Monitoring veterinary, Trematoda isolation & purification, Trematode Infections veterinary
Abstract

Rumen fluke infections have been known to cause paramphistomiasis in both wild and domestic animals worldwide. Occasionally, coinfections of rumen flukes (Carmyerius, Fischoederius, and Paramphistomum) with liver flukes (Fasciola) have been observed due to the similar life cycles that these two species share. This study involved an alternative approach that was developed to classify and distinguish rumen fluke eggs from other genera by using the polymerase chain reaction (PCR) method based on cytochrome c oxidase subunit 1 (COI). Thirty-eight fecal specimens of Bos taurus from Suphanburi Province, Central Thailand were examined using the formalin-ether sedimentation technique. PCR detection was then performed using COI-specific primers that were developed in this study. The results showed that this primer set can classify and distinguish the egg specimens into a separate clade of the genera comprising Gastrothylax, Carmyerius, Fischoederius, Paramphistomum, Explanatum, and Fasciola. Moreover, epidemiological mapping revealed coinfections of three genera of rumen flukes at some collection sites, leading to the need to further investigate Paramphistomoidea infection along with Fasciolidae infection within the endemic area. This data is important for monitoring the outbreak of these parasites in Suphanburi Province, Thailand. It can be applied for initiating surveillance programs of paramphistomiasis and fascioliasis in veterinary studies., (Copyright © 2020 Elsevier B.V. All rights reserved.)

Published
2020
Full Text
View/download PDF

18. The study of Cytochrome B ( CYTB ): species-specific detection and phylogenetic relationship of Echinostoma revolutum , (Froelich, 1802).

Author

Anucherngchai S, Chontananarth T, Tejangkura T, and Chai JY

Abstract

Echinostoma revolutum is known as a significant intestinal trematode in various species of animals and humans. It presents complexities in terms of both the morphological and molecular biological data. This is the first study of the application of Cytochrome B gene ( CYTB ) as a target for studying the phylogeny and designing species-specific primer of E. revolutum . Adult trematodes were harvested from experimentally infected hamsters at 18 days of post-infection. Each worm was identified based on their morphological appearance. The novel CYTB primers were designed from other Echinostoma species to initially amplify CYTB region in E. revolutum . All sequence data of E. revolutum in five provinces of Central Thailand were used as the target for designing the species-specific primer for E. revolutum . The results revealed that CYTB gene can separate E. revolutum into two sister groups by geographical distribution, comprising the eastern and western area groups. Moreover, it also separates E. revolutum from other Echinostoma species, including two sibling species; E. caproni and E. paraensei . In addition, we developed the high performance species-specific primer of E. revolutum . It can detect DNA from a single egg, as well as cercaria, metacercaria and adult stages of this trematode with no cross-reactions to other trematodes and their hosts. Therefore, this research is a positive initial step for the future study of E. revolutum CYTB . The future studies based on this gene should be continued with all species in revolutum complex to overcome the problems of systemic classification that arise in this complex group., Competing Interests: Compliance with ethical standardsWe declare that all authors have no conflict of interest.

Published
2019
Full Text
View/download PDF

19. The rapid detection method by polymerase chain reaction for minute intestinal trematodes: Haplorchis taichui in intermediate snail hosts based on 18s ribosomal DNA.

Author

Chontananarth T, Anucherngchai S, and Tejangkura T

Abstract

The minute intestinal trematode, Haplorchis taichui , is an important parasite species that can infect humans and other mammals. This study investigated the outbreak of H. taichui in thiarid snails in the lower part of the Chao Phraya Basin, Thailand by employing morphological and molecular-based methods. In development of a specific primer of H. taichui , the PCR reaction was conducted with no cross-reaction to their hosts and other related trematode species. The highest level of sensitivity that could be amplified was 0.50 ng/μl and this was detected with only one egg in the sample. In terms of the epidemic results, the parapleurolophocercous cercaria infected only two species of thiarid snails ( Melanoides tuberculata and Tarebia granifera ) with an overall prevalence of 3.80% (23/605). The process of molecular identification revealed positive results indicating that eleven from twenty-three of parapleurolophocercous cercariae specimens in the lower part of the Chao Phraya Basin were H. taichui . In conclusion, this study has developed a rapid detection method, which can discriminate H. taichui from other parapleurolophocercous cercaria in intermediate snail hosts with a high level of sensitivity. Moreover, the high proportion of H. taichui in parapleurolophocercous cercaria (47.83%) indicated that H. taichui was the dominant species of this cercarial type and could infect cyprinoid fish in the lower part of the Chao Phraya Basin leading to public health problems in this area. Thus, a specific primer could be useful in the detection and surveillance of H. taichui outbreaks in their hosts. Recognition of this has resulted in the creation of important prevention programs in these infected areas in the further study., Competing Interests: Compliance with ethical standardsThe authors declare that they have no conflict of interest.

Published
2018
Full Text
View/download PDF

20. Morphological Characteristics and Phylogenetic Trends of Trematode Cercariae in Freshwater Snails from Nakhon Nayok Province, Thailand.

Author

Chontananarth T, Tejangkura T, Wetchasart N, and Chimburut C

Subjects
Animals, Cluster Analysis, DNA, Helminth chemistry, DNA, Helminth genetics, DNA, Ribosomal Spacer chemistry, DNA, Ribosomal Spacer genetics, Microscopy, Phylogeny, Prevalence, Sequence Analysis, DNA, Thailand, Trematoda anatomy & histology, Trematoda genetics, Fresh Water, Snails parasitology, Trematoda classification, Trematoda isolation & purification
Abstract

The prevalence of cercarial infection in freshwater snails and their evolutionary trends were studied in Nakhon Nayok province, Thailand. A total of 2,869 individual snails were examined for parasitic infections. The results showed that 12 snail species were found to host larval stages of trematodes with an overall prevalence of 4.7%. The infected specimens included 7 types at the cercarial stage; cercariae, megalurous cercariae, echinostome cercariae, furcocercous cercariae, parapleurolophocercous cercariae, virgulate cercariae, and xiphidiocercariae. Regarding molecular identification, ITS2 sequence data of each larval trematode were analyzed, and a dendrogram was constructed using the neighbor-joining method with 10,000 replicates. The dendrogram was separated into 6 clades (order/family), including Echinostomatida/Echinostomatidae, Echinostomatida/Philophthalmidae, Opisthorchiida/Heterophyidae, Plagiorchiida/Prosthogonimidae, Plagiorchiida/Lecithodendriidae, and Strigeatida/Cyathocotylidae. These findings were used to confirm morphological characteristics and evolutionary trends of each type of cercariae discovered in Nakhon Nayok province. Furthermore, this investigation confirmed that the ITS2 data of cercariae could be used to study on phylogenetic relationships or to determine classification of this species at order and/or family level when possible.

Published
2017
Full Text
View/download PDF

21. Permanent Genetic Resources added to Molecular Ecology Resources Database 1 April 2010 - 31 May 2010.

Author

Andree K, Axtner J, Bagley MJ, Barlow EJ, Beebee TJ, Bennetzen JL, Bermingham E, Boisselier-Dubayle MC, Bozarth CA, Brooks CP, Brown RP, Catanese G, Cavers S, Ceron-Souza I, Chak ST, Chan MN, Charles-Dominique P, Chen CY, Chen JD, Chinchilla L, DA Silva D, Dafreville S, Daunt F, Delatte H, Dorge T, Duncan N, Durand JD, Duvernell D, Estep M, Fan S, Fattahi R, Villela OF, Fong Y, Fréville H, Funes V, Gallardo-Escarate C, Ganeshaiah KN, Ghaffari MR, Girod C, Gomez-Moliner BJ, Gonzalez-Porter GP, Gosa A, Govers F, Guérin F, Guindo D, Hailer F, Haye PA, Hoelmer KA, Hofmann S, Hong Y, Hu C, Huang SW, Humeau L, Infante C, Jackson SA, Jacobsen E, Jowkar A, Kafi M, Kermani MJ, Kim H, Kim KS, Kim MY, Knibb W, Koita OA, Korpelainen H, Lambourdiere J, Lasso E, Leblois R, Lee H, Lee S, Leung FC, Leung KM, Li C, Li Y, Lieckfeldt D, Lizana M, Loughry WJ, Luo P, Madeira MJ, Mahmoodi P, Maldonado JE, Mardi M, Mendes O, Miehe G, Muth P, Nacci D, Naveen Kumar L, Ng WC, Pailler T, Parzies HK, Perez L, Pfunder M, Pietiläinen M, Pirseyedi SM, Porta D, Porta J, Porta JM, Quilici S, Rakotoarivelo FP, Ramesha BT, Ravikanth G, Riéra B, Risterucci AM, Roberts DA, Samadi S, Sarasola-Puente V, Sarrazin E, Sarthou C, Schmidt A, Segovia NI, Shen KN, Simiand C, Sman MH, Solhoy T, Sommer S, Sumangala RC, Taubert R, Tejangkura T, Telford A, Testa A, Tollon-Cordet C, Tzeng WN, Uma Shaanker R, Van Der Lee TA, VAN Mourik TA, Vasudeva R, Wai TC, Wang RL, Welch ME, Weltzien E, Whitehead A, Woodard A, Xia J, Zeinolabedini M, and Zhang L

Abstract

This article documents the addition of 396 microsatellite marker loci to the Molecular Ecology Resources Database. Loci were developed for the following species: Anthocidaris crassispina, Aphis glycines, Argyrosomus regius, Astrocaryum sciophilum, Dasypus novemcinctus, Delomys sublineatus, Dermatemys mawii, Fundulus heteroclitus, Homalaspis plana, Jumellea rossii, Khaya senegalensis, Mugil cephalus, Neoceratitis cyanescens, Phalacrocorax aristotelis, Phytophthora infestans, Piper cordulatum, Pterocarpus indicus, Rana dalmatina, Rosa pulverulenta, Saxifraga oppositifolia, Scomber colias, Semecarpus kathalekanensis, Stichopus monotuberculatus, Striga hermonthica, Tarentola boettgeri and Thermophis baileyi. These loci were cross-tested on the following species: Aphis gossypii, Sooretamys angouya, Euryoryzomys russatus, Fundulus notatus, Fundulus olivaceus, Fundulus catenatus, Fundulus majalis, Jumellea fragrans, Jumellea triquetra Jumellea recta, Jumellea stenophylla, Liza richardsonii, Piper marginatum, Piper aequale, Piper darienensis, Piper dilatatum, Rana temporaria, Rana iberica, Rana pyrenaica, Semecarpus anacardium, Semecarpus auriculata, Semecarpus travancorica, Spondias acuminata, Holigarna grahamii, Holigarna beddomii, Mangifera indica, Anacardium occidentale, Tarentola delalandii, Tarentola caboverdianus and Thermophis zhaoermii., (© 2010 Blackwell Publishing Ltd.)

Published
2010
Full Text
View/download PDF

22. Molecular isolation and characterization of a novel occlusion body protein gene from Penaeus monodon nucleopolyhedrovirus.

Author

Chaivisuthangkura P, Tawilert C, Tejangkura T, Rukpratanporn S, Longyant S, Sithigorngul W, and Sithigorngul P

Subjects
Amino Acid Sequence, Animals, Antibodies, Viral, Antibody Specificity, Base Sequence, Blotting, Western, Chromatography, Liquid, Gene Library, Hepatopancreas virology, Mass Spectrometry, Molecular Sequence Data, Open Reading Frames, Recombinant Proteins immunology, Recombinant Proteins metabolism, Sequence Alignment, Viral Proteins immunology, Viral Proteins isolation & purification, Gene Expression Regulation, Viral, Nucleopolyhedroviruses genetics, Nucleopolyhedroviruses metabolism, Penaeidae virology, Viral Proteins genetics, Viral Proteins metabolism
Abstract

The full-length of the occlusion body (OB) protein gene of Penaeus monodon nucleopolyhedrovirus (PemoNPV) was successfully isolated. The OB gene sequence contained an open reading frame (ORF) of 1359 nucleotides encoding a protein of 452 amino acid residues with a predicted molecular mass of 50.6 kDa. A putative late promoter element, TAAG, was identified 72 nt upstream of the translation start site. The amino acid sequences of tryptic digested peptides of PemoNPV OB protein obtained from LC-MS analysis matched quite well with various regions of deduced amino acid sequences. Recombinant PemoNPV OB proteins specifically reacted with monoclonal antibodies to PemoNPV OB protein. After comparison with nucleotide database, the PemoNPV OB ORF demonstrated 67% identity to an uncharacterized ORF of a baculovirus pathogenic for Penaeus vannamei. However, comparison against protein databases revealed no significant homology to other known proteins. To our knowledge, this PemoNPV OB gene is the first isolated and characterized gene of nucleopolyhedrovirus from shrimp.

Published
2008
Full Text
View/download PDF

Catalog

Books, media, physical & digital resources
See catalog results