Your search keyword '"qPCR"' showing total 25 results

1. Simultaneous Detection of Salmonella spp. and Quantification of Campylobacter spp. in a Real-Time Duplex PCR: Myth or Reality?

Author

Anis, Nagham, Bonifait, Laetitia, Quesne, Ségolène, Baugé, Louise, Chemaly, Marianne, and Guyard-Nicodème, Muriel

Subjects

SALMONELLA detection, CAMPYLOBACTER, CAMPYLOBACTER jejuni, SALMONELLA, FOOD industry, MYTH, LARGE deviations (Mathematics)

Abstract

In Europe, there is a process hygiene criterion for Salmonella and Campylobacter on broiler carcasses after chilling. The criterion gives indicative contamination values above which corrective actions are required by food business operators. The reference methods for verifying compliance with the criterion for Salmonella and Campylobacter are international standards EN ISO 6579-1 (2017) and EN ISO 10272-2 (2017), respectively. These methods are time-consuming and expensive for food business operators. Therefore, it would be advantageous to simultaneously detect Salmonella spp. and quantify Campylobacter in the same analysis, using the same sample after the pre-enrichment step for Salmonella recovery. A duplex PCR for Salmonella detection and Campylobacter spp. enumeration was developed. Considering the method as a whole, the LOD and LOQ for Campylobacter enumeration were slightly over the limit of 3 log CFU/g set by the process hygiene criterion. A comparison of the duplex PCR method developed with the ISO method on artificially contaminated bacterial suspensions and on naturally contaminated samples demonstrated a good correlation of the results for Campylobacter enumeration when the duplex PCR was performed on samples taken before or after the pre-enrichment step, but revealed a slight bias with a large standard deviation resulting in widely spaced limits of agreement. [ABSTRACT FROM AUTHOR]

Published

2023

2. Detection of Anaplasma phagocytophilum in European brown hares (Lepus europaeus) using three different methods.

Author

Lesiczka, Paulina Maria, Modry, David, Sprong, Hein, Fonville, Manoj, Pikula, Jiri, Piacek, Vladimir, Heger, Tomas, and Hrazdilova, Kristyna

Subjects

*ANAPLASMA phagocytophilum, *CASTOR bean tick, *HARES, *GENE targeting

Abstract

European brown hare (Lepus europaeus Pallas 1778) is a broadly distributed lagomorph species in Europe, recognized as a host for Ixodes ricinus and reservoir of a wide range of pathogens with zoonotic potential. Even though Lepus europaeus represents an important game animal in Central Europe, the data available on Anaplasma phagocytophilum in this lagomorph are scarce. In this study, three populations of brown hare from distinct localities in the Czech Republic were analysed for the presence of Anaplasma phagocytophilum DNA. We used standard qPCR, targeting the msp2 gene and adapted the same assay also for digital droplet PCR. Out of 91 samples, these two methods identified 9 and 12 as positive, respectively. For taxonomic analysis, we amplified the groEL gene from five of six samples that were found positive by both methods. In phylogenetic analyses, this haplotype belongs to ecotype 1, and to the subclade with isolates from cervids and I. ricinus. Our findings underline the importance of correct result interpretation and positivity cut‐off set‐up for different detection methods of A. phagocytophilum. This bacterium is characterized by a high intraspecific variability and highly sensitive detection itself, is not enough. Detailed molecular typing is necessary to define the zoonotic potential of different strains and their natural reservoirs. [ABSTRACT FROM AUTHOR]

Published

2021

3. Faecal egg count reduction test in goats: Zooming in on the genus level.

Author

Maurizio, Anna, Škorpíková, Lucie, Ilgová, Jana, Tessarin, Cinzia, Dotto, Giorgia, Reslová, Nikol, Vadlejch, Jaroslav, Marchiori, Erica, di Regalbono, Antonio Frangipane, Kašný, Martin, and Cassini, Rudi

Subjects

*FECAL egg count, *GOAT diseases, *GOATS, *LARVAE, *GOAT farming, *TRICHOSTRONGYLUS

Abstract

The faecal egg count reduction test (FECRT) is the most widely used method to assess treatment efficacy against gastrointestinal nematodes (GIN). Information on genera composition of the GIN community is not available with this test and it is commonly obtained by identifying cultured third-stage larvae (L3) or through molecular assays in the post-treatment survey, but results provided are usually only qualitative or semi-quantitative. The updated WAAVP guidelines now recommend assessing anthelmintic efficacy for each GIN genus/species separately (genus-specific FECRT), but this approach is poorly employed in Europe and in goats especially. For this reason, four FECRT trials were conducted using oxfendazole and eprinomectin in two Italian goat farms. Samples were processed individually using the McMaster technique and then pooled to create two samples from faeces of 5 animals each. Pooled samples were analysed using the McMaster and cultured for seven days at 26°C to obtain L3s. The genus-specific FECRT was based on larval identification, integrating coproculture and FEC results. Larvae were identified as Haemonchus , Trichostrongylus , Teladorsagia , Oesophagostomum / Chabertia and Bunostomum. Molecular assays (a multiplex real-time PCR and two end-point PCRs) were also implemented on pooled samples to support the morphological identification. The Spearmann Rho test confirmed a high correlation between the two approaches (Rho = 0.941 and Rho = 0.914 respectively for Haemonchus and Trichostrongylus , the two most common genera). Both oxfendazole and eprinomectin were effective in one farm, while none in the other farm (FECR = 75.9% and 73.3% respectively). In the second farm, the genus-specific FECRT highlighted a different response to treatment among genera: oxfendazole lacked efficacy against both Haemonchus and Trichostrongylus spp., eprinomectin only against Haemonchus , while all other genera were susceptible to both drugs. This study brings new attention on the importance of adopting a genus-specific approach to identify and quantify differences in susceptibility to anthelmintics among genera in goats, providing support for FECRT interpretation, anthelmintic resistance evaluation and evidence-based GIN control. • Four FECRT trials were conducted and cultured third-stage larvae were identified. • Genera identification from coproculture was confirmed by molecular methods. • The genus-specific FECRT was obtained interpolating larval identification with FEC. • Differences in susceptibility to anthelmintics were detected among genera. [ABSTRACT FROM AUTHOR]

Published

2024

4. Recapitulation of Transcriptomic Characteristics of Primary Breast Tumours in Patient-Derived 3D Cultures in Vitro.

Author

Nitiša, Dina, Jain, Nityanand, Irmejs, Arvīds, Pirsko, Valdis, and Čakstiņa, Inese

Subjects

*BREAST, *TRANSCRIPTOMES, *POLYMERASE chain reaction, *CELL culture, *TUMORS, *GENE expression

Abstract

Breast cancer (BC) is the most common cause of cancer-related deaths among women in Europe and worldwide. Adherent (2D) cell cultures have been the routine in vitro model system employed in preclinical BC research for the last half-century. Over the past decade, new protocols have been developed allowing patient-derived three-dimensional organoid (3D) cell culture development from a range of solid tumours, including BC. These 3D models offer a promise of closer resemblance to the native tumour than the 2D cultures. To test the assumption that an in vitro 3D BC model system provides increased faithfulness to the molecular processes happening in vivo, as compared to 2D BC cultures, post-operational material from three BC patients was used to simultaneously develop 2D and 3D cultures in vitro. When analysed by quantitative polymerase chain reaction (PCR), the gene expression patterns of the cells from 3D cultures resembled the original tissues, while the gene expression patterns of the conventional 2D cultures were more distant. [ABSTRACT FROM AUTHOR]

Published

2021

5. Anopheles sacharovi in Italy: first record of the historical malaria vector after over 50 years.

Author

Raele DA, Severini F, Toma L, Menegon M, Boccolini D, Tortorella G, Di Luca M, and Cafiero MA

Subjects

Animals, Mosquito Vectors, Italy epidemiology, Europe, Malaria epidemiology, Anopheles genetics

Abstract

Background: Anopheles sacharovi, a member of the Anopheles maculipennis complex, was a historical malaria vector in Italy, no longer found since the last report at the end of 1960s. In September 2022, within the Surveillance Project for the residual anophelism, a single specimen of An. maculipennis sensu lato collected in Lecce municipality (Apulia region) was molecularly identified as An. sacharovi. This record led to implement a targeted entomological survey in September 2023., Methods: Investigation was conducted in the areas around the first discovery, focusing on animal farms, riding stables and potential breeding sites. Adult and immature mosquitoes were collected, using active search or traps, in several natural and rural sites. Mosquitoes belonging to An. maculipennis complex were identified morphologically and molecularly by a home-made routine quantitative polymerase chain reaction (qPCR) assay, developed specifically for the rapid identification of An. labranchiae, and, when necessary, by amplification and sequencing of the ITS-2 molecular marker., Results: Out of the 11 sites investigated, 6 were positive for Anopheles presence. All 20 An. maculipennis s.l. (7 adults, 10 larvae and 3 pupae) collected in the areas were identified as An. sacharovi by ITS-2 sequencing., Conclusions: The discovery of An. sacharovi, considered to have disappeared from Italy for over 50 years, has a strong health relevance and impact, highlighting an increase in the receptivity of the southern areas. As imported malaria cases in European countries are reported every year, the risk of Plasmodium introduction by gametocyte carriers among travellers from endemic countries should be taken into greater consideration. Our findings allow rethinking and building new models for the prediction and expansion of introduced malaria. Furthermore, to prevent the risk of reintroduction of the disease, the need to strengthen the surveillance of residual anophelism throughout the South should be considered., (© 2024. The Author(s).)

Published

2024

6. Antibiotic resistance genes in treated wastewater and in the receiving water bodies: A pan-European survey of urban settings.

Author

Cacace, Damiano, Fatta-Kassinos, Despo, Manaia, Celia M., Cytryn, Eddie, Kreuzinger, Norbert, Rizzo, Luigi, Karaolia, Popi, Schwartz, Thomas, Alexander, Johannes, Merlin, Christophe, Garelick, Hemda, Schmitt, Heike, de Vries, Daisy, Schwermer, Carsten U., Meric, Sureyya, Ozkal, Can Burak, Pons, Marie-Noelle, Kneis, David, and Berendonk, Thomas U.

Subjects

*SEWAGE disposal plants, *ANTIBIOTICS, *SEWAGE, *WASTEWATER treatment, *BODIES of water, *GENES

Abstract

There is increasing public concern regarding the fate of antibiotic resistance genes (ARGs) during wastewater treatment, their persistence during the treatment process and their potential impacts on the receiving water bodies. In this study, we used quantitative PCR (qPCR) to determine the abundance of nine ARGs and a class 1 integron associated integrase gene in 16 wastewater treatment plant (WWTP) effluents from ten different European countries. In order to assess the impact on the receiving water bodies, gene abundances in the latter were also analysed. Six out of the nine ARGs analysed were detected in all effluent and river water samples. Among the quantified genes, intI1 and sul 1 were the most abundant. Our results demonstrate that European WWTP contribute to the enrichment of the resistome in the receiving water bodies with the particular impact being dependent on the effluent load and local hydrological conditions. The ARGs concentrations in WWTP effluents were found to be inversely correlated to the number of implemented biological treatment steps, indicating a possible option for WWTP management. Furthermore, this study has identified bla OXA-58 as a possible resistance gene for future studies investigating the impact of WWTPs on their receiving water. Image 1 • Wastewater treatment plants are hotspots for antibiotic resistance. • Set up of a first standard of ARGs abundance in European urban wastewater effluents and receiving river bodies. • Wastewater treatment plants equipped with secondary clarifier release lower levels of ARGs into the environment. • bla OXA58 is considered as a suitable proxy for the understanding of the dynamics for antibiotic resistance in the environment. [ABSTRACT FROM AUTHOR]

Published

2019

7. Stomoxys calcitrans, mechanical vector of virulent Besnoitia besnoiti from chronically infected cattle to susceptible rabbit.

Author

Sharif, S., Jacquiet, P., Prevot, F., Grisez, C., Raymond‐Letron, I., Semin, M. O., Geffré, A., Trumel, C., Franc, M., Bouhsira, É., and Liénard, E.

Subjects

*RABBITS, *POLYMERASE chain reaction, *CATTLE, *MUSCIDAE, *WEIGHT loss

Abstract

Cattle besnoitiosis caused by Besnoitia besnoiti (Eucoccidiorida: Sarcocystidae) is a re‐emerging disease in Europe. Its mechanical transmission by biting flies has not been investigated since the 1960s. The aim of this study was to re‐examine the ability of Stomoxys calcitrans (Diptera: Muscidae) to transmit virulent B. besnoiti bradyzoites from chronically infected cows to susceptible rabbits. Three batches of 300 stable flies were allowed to take an interrupted bloodmeal on chronically infected cows, followed by an immediate bloodmeal on three rabbits (Group B). A control group of rabbits and a group exposed to the bites of non‐infected S. calcitrans were included in the study. Blood quantitative polymerase chain reaction (qPCR) analyses, and clinical, serological and haematological surveys were performed in the three groups over 152 days until the rabbits were killed. Quantitative PCR analyses and histological examinations were performed in 24 tissue samples per rabbit. Only one rabbit in Group B exhibited clinical signs of the acute phase of besnoitiosis (hyperthermia, weight loss, regenerative anaemia and transient positive qPCR in blood) and was seroconverted. Parasite DNA was detected in four tissue samples from this rabbit, but no cysts were observed on histological examination. These findings indicate that S. calcitrans may act as a mechanical vector of B. besnoiti more efficiently than was previously considered. [ABSTRACT FROM AUTHOR]

Published

2019

8. Laboratory transmission of an Asian strain of Leishmania tropica by the bite of the southern European sand fly Phlebotomus perniciosus.

Author

Bongiorno, Gioia, Di Muccio, Trentina, Bianchi, Riccardo, Gramiccia, Marina, and Gradoni, Luigi

Subjects

*LEISHMANIA, *SAND flies, *PHLEBOTOMUS, *CUTANEOUS leishmaniasis, *LEISHMANIA infantum, *STEREOLOGY

Abstract

• Imported cases of anthroponotic cutaneous leishmaniasis due to Leishmania tropica are increasingly documented in Europe. • Vector competence for an Asian L. tropica was investigated in Phlebotomus perniciosus , a southwestern European sand fly. • Leishmania tropica developed into abundant metacyclic promastigotes in 20% of laboratory-infected P. perniciosus. • Parasites have been successfully transmitted from infected to naive hamsters by the bite of P. perniciosus. • In particular settings P. perniciosus , a Leishmania infantum vector, may play the role of an occasional L. tropica vector. Imported cases of anthroponotic cutaneous leishmaniasis due to Leishmania tropica are increasingly documented in Europe. We investigated the ability of Phlebotomus perniciosus , a competent vector of Leishmania infantum widespread in southwestern Europe, to support the growth and transmissibility of an Asian strain of L. tropica recently isolated from a refugee. Parasite growth behavior was investigated in laboratory-reared sand flies fed artificially with promastigotes as well as in sand flies infected after biting on footpad lesions induced in hamsters by promastigote inoculation. The evolution of infection was checked by gut microscopy and quantitative real-time PCR, and it was found to be similar between promastigote- and amastigote-initiated infections. In 80% of infected sand flies, despite survival and flourishing growth of promastigotes after blood digestion and defecation, either the parasites died, or failed to migrate to the foregut and/or to mature into infective forms. However, in the remaining 20% L. tropica developed into abundant metacyclic promastigotes. The quantitative real-time PCR assay detected variable loads of gut promastigotes irrespective of morphological evidence of viability or progressive/final death. Parasite transmissibility was investigated by exposing naive hamsters to P. perniciosus previously infected on chronic lesions induced in hamsters which survived to take a second blood meal. Two months post exposure, lesions developed in skin sites bitten by sand flies confirmed to harbor metacyclic promastigotes; in the following months, the presence of viable and transmissible L. tropica parasites in lesions was demonstrated by xenodiagnosis assays. Our findings support the hypothesis that, in particular epidemiological situations, P. perniciosus may play the role of an occasional L. tropica vector. [ABSTRACT FROM AUTHOR]

Published

2019

9. The life cycle of Hymenoscyphus fraxineus on Manchurian ash, Fraxinus mandshurica, in Japan.

Author

Inoue, Takahiro, Okane, Izumi, Ishiga, Yasuhiro, Degawa, Yosuke, Hosoya, Tsuyoshi, and Yamaoka, Yuichi

Subjects

*ASH (Tree), *FOREST litter, *POLYMERASE chain reaction, *DEFOLIATION, *EUROPEAN ash

Abstract

Abstract Hymenoscyphus fraxineus causes a lethal disease known as "ash dieback" in the common ash, Fraxinus excelsior , in Europe. It is hypothesized that the fungus originated from East Asia. This fungus is found on the leaf litter of the Manchurian ash, Fraxinus mandshurica , in Japan and is reported to produce apothecia on pseudosclerotial plates formed mainly on decomposing rachises. However, dieback disease has not been reported in Japan, and little is known about the life cycle of H. fraxineus. This study was conducted to explore the behavior and life cycle of this fungus. It was revealed that, after infection by ascospores, H. fraxineus endophytically inhabits the living leaves of F. mandshurica. On fallen leaves, the fungus behaves saprophytically, producing apothecia on pseudosclerotial plates formed mainly on the decomposing rachises. Analysis by real-time quantitative polymerase chain reaction (qPCR) revealed that the amount of H. fraxineus DNA sharply increased in rachises, while such sharp increase of DNA was not found in leaflets. Highlights • Hymenoscyphus fraxineus endophytically inhabits the leaves of Fraxinus mandshurica. • The amount of H. fraxineus DNA sharply increased in senescent leaves just before defoliation. • A sharp increase in the amount of DNA was observed in rachises rather than in leaflets. • Fertilization through asexual morph formation might occur shortly after defoliation. • The pseudosclerotial layer forms quickly on fallen leaves, even under snow. [ABSTRACT FROM AUTHOR]

Published

2019

10. Field-based recombinase polymerase amplification and lab-based qPCR assays for detection of Helicoverpa armigera.

Author

Rich M, Noh E, Wang H, Greene J, Gilligan T, Reay-Jones FPF, Turnbull M, and Zink F

Subjects

Animals, Australia, Europe, Recombinases, Moths genetics

Abstract

Helicoverpa armigera (Hübner) is a major crop pest native to Europe, Asia, Australia, and Africa which has recently invaded South America and has caused billions of dollars in agricultural losses. Because of challenges in differentiating between H. armigera and Helicoverpa zea (Boddie), a closely related species native to North and South America, genetic tests have previously been developed to detect H. armigera DNA in pooled samples of moth legs. In this study, a field-based recombinase polymerase amplification (RPA) assay using a lateral flow strip and a qPCR melt curve assay were developed for specific detection of H. armigera DNA in pooled moth samples. In addition, a crude DNA extraction protocol for whole moths was developed to allow rapid preparation of DNA samples. The RPA field test was able to detect ≥ 10 pg of purified H. armigera DNA and the crude DNA of one H. armigera sample in a background of 999 H. zea equivalents. The qPCR assay was able to detect ≥ 100 fg of purified H. armigera DNA and the crude DNA of one H. armigera sample in a background of up to 99,999 H. zea equivalents. Both RPA and qPCR assays detected H. armigera in the crude DNA extracted in the field from a pool of one H. armigera moth and 999 H. zea moths. These newly developed molecular assays to detect H. armigera will contribute to large-scale surveillance programs of H. armigera., (© The Author(s) 2023. 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

2023

11. Gene expression analysis at the onset of sex differentiation in turbot (Scophthalmus maximus).

Author

Robledo, Diego, Ribas, Laia, Cal, Rosa, Sánchez, Laura, Piferrer, Francesc, Martínez, Paulino, and Viñas, Ana

Subjects

*GENE expression, *AQUACULTURE, *DIMORPHISM (Biology), *SEX differentiation (Embryology)

Abstract

Background: Controlling sex ratios is essential for the aquaculture industry, especially in those species with sex dimorphism for relevant productive traits, hence the importance of knowing how the sexual phenotype is established in fish. Turbot, a very important fish for the aquaculture industry in Europe, shows one of the largest sexual growth dimorphisms amongst marine cultured species, being all-female stocks a desirable goal for the industry. Although important knowledge has been achieved on the genetic basis of sex determination (SD) in this species, the master SD gene remains unknown and precise information on gene expression at the critical stage of sex differentiation is lacking. In the present work, we examined the expression profiles of 29 relevant genes related to sex differentiation, from 60 up to 135 days post fertilization (dpf), when gonads are differentiating. We also considered the influence of three temperature regimes on sex differentiation. Results: The first sex-related differences in molecular markers could be observed at 90 days post fertilization (dpf) and so we have called that time the onset of sex differentiation. Three genes were the first to show differential expression between males and females and also allowed us to sex turbot accurately at the onset of sex differentiation (90 dpf): cyp19a1a, amh and vasa. The expression of genes related to primordial germ cells (vasa, gsdf, tdrd1) started to increase between 75-90 dpf and vasa and tdrd1 later presented higher expression in females (90-105 dpf). Two genes placed on the SD region of turbot (sox2, fxr1) did not show any expression pattern suggestive of a sex determining function. We also detected changes in the expression levels of several genes (ctnnb1, cyp11a, dmrt2 or sox6) depending on culture temperature. Conclusion: Our results enabled us to identify the first sex-associated genetic cues (cyp19a1a, vasa and amh) at the initial stages of gonad development in turbot (90 dpf) and to accurately sex turbot at this age, establishing the correspondence between gene expression profiles and histological sex. Furthermore, we profiled several genes involved in sex differentiation and found specific temperature effects on their expression. [ABSTRACT FROM AUTHOR]

Published

2015

12. Rapid detection of Campylobacter spp. in chickens before slaughter.

Author

Llarena, Ann-Katrin, Skjerve, Eystein, Bjørkøy, Solfrid, Forseth, Merete, Winge, Julianne, Hauge, Sigrun J., Johannessen, Gro S., Spilsberg, Bjørn, and Nagel-Alne, Gunvor Elise

Subjects

*CAMPYLOBACTER, *CAMPYLOBACTER jejuni, *BROILER chickens, *CHICKEN as food, *SLAUGHTERING, *SENSITIVITY & specificity (Statistics), *NOROVIRUS diseases

Abstract

Campylobacter continues to be the number one cause of bacterial gastroenteritis in Europe. Poultry, and especially broiler chickens, is considered an important reservoir for Campylobacter spp. Poultry producers prioritize to identify and reduce the number of Campylobacter contaminated chicken flocks by tightening biosecurity and mitigation actions at slaughter. Campylobacter- positive flocks must therefore be identified as close to slaughter as possible, and rapid detection methods are needed. Here we evaluated the applicability, sensitivity, and specificity of four commercially available rapid methods to detect Campylobacter in naturally contaminated chicken cecal droppings on-farm before slaughter against an established qPCR method. The Biofire® FilmArray® Gastrointestinal Panel assay, the VIDAS Campylobacter assay, the Singlepath® Campylobacter test, and OptiGenes' Genie Campylobacter isothermal DNA amplification were assessed in a pilot-study. The OptiGenes' Genie Campylobacter isothermal DNA amplification was also tested under field conditions. The Biofire® FilmArray® showed superior sensitivity and specificity compared to the three other rapid tests but had a lower throughput and a higher cost. While the VIDAS Campylobacter , Singlepath® Campylobacter and the isothermal DNA amplification were affordable, their unsatisfactory sensitivity (10%–71%) left these unsuitable to monitor Campylobacter carriage in chickens. An additional finding of this study is that 38% of flocks positive for Campylobacter at slaughter became contaminated during the last week of rearing. Therefore, increased efforts to develop suitable methods to detect Campylobacter rapidly and reliably in chickens close to slaughter are needed. • Four rapid Campylobacter detection methods for chicken dropping tested. • Approximately 70% of Campylobacter positive flocks were detected using an isothermal DNA amplification. • Nearly 40% of Campylobacter positive flocks at slaughter acquire Campylobacter during the last week of rearing. • Increased efforts to detect Campylobacter in chickens at slaughter is needed. [ABSTRACT FROM AUTHOR]

Published

2022

13. Genotype-specific Taqman® assays for the detection and rapid characterisation of European strains of viral haemorrhagic septicaemia virus

Author

Bland, Fiona, Snow, Michael, Garver, Kyle A., and Matejusova, Iveta

Subjects

*SEPSIS, *CAUSES of death, *ETIOLOGY of diseases, *MARINE fishes, *FRESHWATER fishes, *RAINBOW trout

Abstract

Abstract: Viral haemorrhagic septicaemia virus (VHSV) is the agent of a disease that causes mortality events in marine and freshwater fish. It is one of the most important pathogens in European rainbow trout (Oncorhynchus mykiss) aquaculture. Four major genotypes of the virus are recognised reflecting different geographic and host ranges. Genotyping of VHS isolates is important for disease management enabling monitoring of disease spread into new geographical regions or susceptible species. This study sought to develop molecular tools for rapid and efficient classification of European VHSV genotypes. Specificity of genotype-specific real-time reverse transcription polymerase chain reaction (RT-qPCR) assays targeting the viral nucleoprotein (N) gene was tested using 66 viral isolates. All designed Taqman® RT-qPCR assays were genotype specific, displayed a high sensitivity and together constituted a diagnostic method for the rapid discrimination of European VHSV genotypes. Practical diagnostic applications of such assays demonstrated in this study include: (1) rapid genotype determination of isolates; and (2) identification of mixed-genotype isolates originating from pooled samples in areas where genotype distribution is known to overlap. However, the most important application will be supporting international VHSV surveillance programmes through the provision of a rapid specific and sensitive isolate characterisation method. [Copyright &y& Elsevier]

Published

2013

14. A closer look on the variety and abundance of the faecal resistome of wild boar.

Author

Dias, Diana, Fonseca, Carlos, Mendo, Sónia, and Caetano, Tânia

Subjects

WILD boar, MOBILE genetic elements, OMNIVORES, FECAL contamination, PHENOTYPES, METAGENOMICS, POLLUTION

Abstract

Antimicrobial resistance (AMR) is a serious problem for public and animal health, and also for the environment. Monitoring and reporting the occurrence of AMR determinants and bacteria with the potential to disseminate is a priority for health surveillance programs around the world and critical to the One Health concept. Wildlife is a reservoir of AMR, and human activities can strongly influence their resistome. The main goal of this work was to study the resistome of wild boar faecal microbiome, one of the most important game species in Europe using metagenomic and culturing approaches. The most abundant genes identified by the high-throughput qPCR array encode mobile genetic elements, including integrons, which can promote the dissemination of AMR determinants. A diverse set of genes (n = 62) conferring resistance to several classes of antibiotics (ARGs), some of them included in the WHO list of critically important antimicrobials were also detected. The most abundant ARGs confer resistance to tetracyclines and aminoglycosides. The phenotypic resistance of E. coli and Enterococcus spp. were also investigated, and together supported the metagenomic results. As the wild boar is an omnivorous animal, it can be a disseminator of AMR bacteria and ARGs to livestock, humans, and the environment. This study supports that wild boar can be a key sentinel species in ecosystems surveillance and should be included in National Action Plans to fight AMR, adopting a One Health approach. [Display omitted] • Tetracycline was the most abundant class of ARGs in wild boar faeces. • Resistant bacteria were isolated from the three locations studied. • Resistome includes clinically relevant genes. • Higher variety and abundance of AMR determinants in anthropogenic areas. • Wild boar can be a sentinel species for environmental pollution by AMR bacteria. [ABSTRACT FROM AUTHOR]

Published

2022

15. A Novel Real Time PCR Method for the Detection and Quantification of Didymella pinodella in Symptomatic and Asymptomatic Plant Hosts.

Author

Šišić, Adnan, Oberhänsli, Thomas, Baćanović-Šišić, Jelena, Hohmann, Pierre, and Finckh, Maria Renate

Subjects

*POLYMERASE chain reaction, *MYCOSPHAERELLA pinodes, *HOST plants, *DNA

Abstract

Didymella pinodella is the major pathogen of the pea root rot complex in Europe. This wide host range pathogen often asymptomatically colonizes its hosts, making the control strategies challenging. We developed a real-time PCR assay for the detection and quantification of D. pinodella based on the TEF-1 alpha gene sequence alignments. The assay was tested for specificity on a 54-isolate panel representing 35 fungal species and further validated in symptomatic and asymptomatic pea and wheat roots from greenhouse tests. The assay was highly consistent across separate qPCR reactions and had a quantification/detection limit of 3.1 pg of target DNA per reaction in plant tissue. Cross-reactions were observed with DNA extracts of five Didymella species. The risk of cross contamination, however, is low as the non-targets have not been associated with pea previously and they were amplified with at least 1000-fold lower sensitivity. Greenhouse inoculation tests revealed a high correlation between the pathogen DNA quantities in pea roots and pea root rot severity and biomass reduction. The assay also detected D. pinodella in asymptomatic wheat roots, which, despite the absence of visible root rot symptoms, caused wheat biomass reduction. This study provides new insights into the complex life style of D. pinodella and can assist in better understanding the pathogen survival and spread in the environment. [ABSTRACT FROM AUTHOR]

Published

2022

16. Taqman qPCR Quantification and Fusarium Community Analysis to Evaluate Toxigenic Fungi in Cereals.

Author

Sohlberg, Elina, Virkajärvi, Vertti, Parikka, Päivi, Rämö, Sari, Laitila, Arja, and Sarlin, Tuija

Subjects

*TOXIGENIC fungi, *FUSARIUM, *PLANT diseases, *DETECTION limit, *OATS, *FOOD safety, *GRAIN

Abstract

Fusarium head blight (FHB) is an economically important plant disease. Some Fusarium species produce mycotoxins that cause food safety concerns for both humans and animals. One especially important mycotoxin-producing fungus causing FHB is Fusarium graminearum. However, Fusarium species form a disease complex where different Fusarium species co-occur in the infected cereals. Effective management strategies for FHB are needed. Development of the management tools requires information about the diversity and abundance of the whole Fusarium community. Molecular quantification assays for detecting individual Fusarium species and subgroups exist, but a method for the detection and quantification of the whole Fusarium group is still lacking. In this study, a new TaqMan-based qPCR method (FusE) targeting the Fusarium-specific elongation factor region (EF1α) was developed for the detection and quantification of Fusarium spp. The FusE method was proven as a sensitive method with a detection limit of 1 pg of Fusarium DNA. Fusarium abundance results from oat samples correlated significantly with deoxynivalenol (DON) toxin content. In addition, the whole Fusarium community in Finnish oat samples was characterized with a new metabarcoding method. A shift from F. culmorum to F. graminearum in FHB-infected oats has been detected in Europe, and the results of this study confirm that. These new molecular methods can be applied in the assessment of the Fusarium community and mycotoxin risk in cereals. Knowledge gained from the Fusarium community analyses can be applied in developing and selecting effective management strategies for FHB. [ABSTRACT FROM AUTHOR]

Published

2022

17. A qPCR Assay for the Fast Detection and Quantification of Colletotrichum lupini.

Author

Kamber, Tim, Malpica-López, Nachelli, Messmer, Monika M., Oberhänsli, Thomas, Arncken, Christine, Alkemade, Joris A., and Hohmann, Pierre

Subjects

SUSTAINABLE agriculture, COLLETOTRICHUM, LUPINUS albus, INFECTIOUS disease transmission, ANTHRACNOSE

Abstract

White lupin (Lupinus albus) represents an important legume crop in Europe and other parts of the world due to its high protein content and potential for low-input agriculture. However, most cultivars are susceptible to anthracnose caused by Colletotrichum lupini, a seed- and air-borne fungal pathogen that causes severe yield losses. The aim of this work was to develop a C. lupini-specific quantitative real-time TaqMan PCR assay that allows for quick and reliable detection and quantification of the pathogen in infected seed and plant material. Quantification of C. lupini DNA in dry seeds allowed us to distinguish infected and certified (non-infected) seed batches with DNA loads corresponding to the disease score index and yield of the mother plants. Additionally, C. lupini DNA could be detected in infected lupin shoots and close to the infection site, thereby allowing us to study the disease cycle of this hemibiotrophic pathogen. This qPCR assay provides a useful diagnostic tool to determine anthracnose infection levels of white lupin seeds and will facilitate the use of seed health assessments as a strategy to reduce the primary infection source and spread of this disease. [ABSTRACT FROM AUTHOR]

Published

2021

18. Gammaherpesvirus Infections in Cattle in Europe.

Author

Rosato G, Ruiz Subira A, Al-Saadi M, Michalopoulou E, Verin R, Dettwiler M, Nordgren H, Chiers K, Groβmann E, Köhler K, Suntz M, Stewart JP, and Kipar A

Subjects

Animals, Cattle, Europe, Cattle Diseases virology, Herpesviridae isolation & purification, Herpesviridae Infections epidemiology, Herpesviridae Infections veterinary

Abstract

The genus Macavirus, subfamily Gammaherpesvirinae, comprises ungulate viruses that infect domestic and wild ruminants and swine. They cause asymptomatic latent infections in reservoir hosts and malignant catarrhal fever in susceptible species. Lung, spleen, bronchial lymph node, and tongue were collected from 448 cattle (348 necropsied, 100 slaughtered) in Switzerland, United Kingdom, Finland, Belgium, and Germany to determine their infection with bovine herpesvirus-6 (BoHV-6) and gammaherpesviruses of other ruminants, i.e., ovine herpesvirus-1 and -2, caprine herpesvirus-2, and bison lymphotropic herpesvirus, using quantitative PCR. Only BoHV-6 was detected, with an overall frequency of 32%, ranging between 22% and 42% in the different countries. Infection was detected across all ages, from one day after birth, and was positively correlated with age. There was no evidence of an association with specific disease processes. In positive animals, BoHV-6 was detected in all organs with high frequency, consistently in the lungs or spleen. Viral loads varied substantially. In BoHV-6-positive gravid cows, organs of fetuses tested negative for infection, indicating that the virus is not vertically transmitted. Our results confirm previous data indicating that BoHV-6 is a commensal of domestic cattle not associated with disease processes and confirm that infections with other macaviruses are rare and sporadic.

Published

2021

19. Short term effects of climate change and intensification of management on the abundance of microbes driving nitrogen turnover in montane grassland soils.

Author

Andrade-Linares DR, Zistl-Schlingmann M, Foesel B, Dannenmann M, Schulz S, and Schloter M

Subjects

Climate Change, Europe, Germany, Grassland, Soil Microbiology, Nitrogen analysis, Soil

Abstract

Montane grasslands in Europe are exposed to increasing temperatures twice as fast as the global average. Changes in climatic conditions are possibly accompanied by an increase in land use intensity, caused by a prolongation of the vegetation period and the need to improve productivity. Therefore, the investigation of combined effects of climate change and land use intensity is needed to further implement agricultural management strategies. Here we present results from a study performed in the pre-alpine region of southern Germany, where intact plant-soil mesocosms from grasslands, were translocated along an altitudinal gradient, resulting in an increase in soil temperature (moderate treatment: +0.5 K; strong treatment: +1.9 K warming) during the experimental period. Additionally, we applied an extensive or intensive agricultural management (two vs. five times of mowing and slurry application) on the transplanted mesocosms. After an exposure of one year, we measured plant growth and soil properties and quantified abundances of soil microorganisms catalyzing key steps in the nitrogen (N) cycle. Our data indicate, significant interactions between climate change and management. For example, microbial biomass was significantly reduced (-47.7% and -49.8% for C mic and N mic respectively), which was further accompanied by lower abundances of N 2 -fixing bacteria (up to -89,3%), as well as ammonia oxidizing bacteria (-81.4%) under intensive management, whereas N-mineralizing bacteria increased in abundance (up to +139.8%) under extensive management. Surprisingly, the abundances of denitrifying bacteria as well as mean N 2 O emissions were not affected by the treatments. Overall, our data suggest pronounced shifts in the abundance of microbes driving the N cycle in soil as a result of combined climate change and land use intensification already after a short simulation period of one year., 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 © 2021 The Authors. Published by Elsevier B.V. All rights reserved.)

Published

2021

20. High incidence of cold-tolerant Clostridium frigoriphilum and C. algidicarnis in vacuum-packed beef on retail sale in Germany.

Author

Mang S, Schwaiger K, Lindner R, Gareis M, and Dorn-In S

Subjects

Animals, Cattle, Clostridium classification, Clostridium physiology, Cold Temperature, Europe, Germany, Multiplex Polymerase Chain Reaction, RNA, Ribosomal, 16S genetics, Vacuum, Clostridium isolation & purification, Food Packaging, Red Meat microbiology

Abstract

Sixty vacuum-packed beef samples retailed in Germany were investigated for the occurrence of cold-tolerant Clostridium spp. After a storage period at 4 °C for eight weeks, meat juice from all samples was processed for culturing, DNA extraction and SYBR green qPCR for Clostridium species. After that, a previously developed multiplex qPCR, sequence analysis of the 16S rRNA gene, and MALDI-TOF MS were applied in order to identify Clostridium spp. found in samples. Subsequently, 23 samples were found positive for C. frigoriphilum (n = 19), C. estertheticum (n = 2), C. tagluense (n = 1) and C. lacusfryxellense/C. frigoris (n = 1). By using a new multiplex qPCR and a new RFLP method developed in this study, a further 15 meat juice samples were revealed to be contaminated with C. algidicarnis. With some samples being co-contaminated with two different species, 53% (n = 32) of all investigated vacuum-packed beef samples were found to be positive for cold-tolerant clostridia. This is the first report of detection and identification of C. algidicarnis in meat samples in Germany and Central Europe., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2021

21. Real-time PCR detection of Toxoplasma gondii in tissue samples of wild boars (Sus scrofa) from southern Italy reveals high prevalence and parasite load.

Author

Santoro, Mario, Viscardi, Maurizio, Sgroi, Giovanni, DʼAlessio, Nicola, Veneziano, Vincenzo, Pellicano, Roberta, Brunetti, Roberta, and Fusco, Giovanna

Subjects

*WILD boar, *TOXOPLASMA gondii, *MASSETER muscle, *MYOCARDIUM, *TISSUES, *CHAGAS' disease

Abstract

Background: Toxoplasmosis is a zoonotic parasitic disease caused by Toxoplasma gondii, a widespread protozoan in the phylum Apicomplexa. In Europe, several studies have demonstrated the presence of the parasite in tissues of wild boars (Sus scrofa), but no data exists on the T. gondii load in tissues which in turn may be an useful way to assess the infection risk for the consumer of wild boar meat. Methods: We sampled and tested a total of 472 tissue samples of brain, heart and masseter muscle from 177 wild boars from the Campania region of southern Italy by real-time PCR analyses for detection and quantification of T. gondii. The sensitivity and specificity of the method were calculated by ROC analysis curves. Results: PCR analysis revealed the presence of T. gondii in tissue samples of 78 out of 177 (44%) wild boars. In general, the brain presented the highest PCR prevalence (31%), followed by the heart (28.3%) and the masseter muscle (24.2%), with the highest estimated parasite numbers observed in the brain followed by the heart and masseter muscle. The PCR method showed an excellent discriminating ability for each of the examined tissues. According to the ROC analysis curves, the respective sensitivity and specificity were 99 and 100% for masseter muscle, 98 and 98% for brain and 96 and 98% for heart samples. Conclusions: The high prevalence of infection here detected suggests a widespread distribution of the parasite in the wildlife of the Campania region of southern Italy. The T. gondii burdens detected may potentially represent a source of infection for humans. [ABSTRACT FROM AUTHOR]

Published

2019

22. Sustainable alternatives to 1,3-dichloropropene for controlling root-knot nematodes and fungal pathogens in melon crops in Mediterranean soils: Efficacy and effects on soil quality.

Author

Montiel-Rozas MDM, Hurtado-Navarro M, Díez-Rojo MÁ, Pascual JA, and Ros M

Subjects

Animals, Europe, Mediterranean Region, Plant Diseases microbiology, Plant Diseases parasitology, Soil Pollutants chemistry, Allyl Compounds pharmacology, Crops, Agricultural microbiology, Crops, Agricultural parasitology, Cucurbitaceae microbiology, Cucurbitaceae parasitology, Fungi drug effects, Hydrocarbons, Chlorinated pharmacology, Nematoda drug effects, Pesticides pharmacology

Abstract

The control of agricultural pests is key to maintain economically viable crops. Increasing environmental awareness, however, is leading to more restrictive European policies regulating the use of certain pesticides due to their impact on human health and the soil system. Given this context, we evaluated the efficacy of three alternatives to the soil fumigant 1,3-dichloropropene (1,3-D), which is currently banned in Europe: two non-fumigant nematicides [oxamyl (OX) and fenamiphos (FEN)] and the soil fumigant dimethyl disulfide (DMDS). We analysed the efficiency of these pesticides against root-knot nematodes and soil fungal pathogens (determined by qPCR) as well as the soil biological quality after treatments application (estimated by enzyme activities). Among treatments, 1,3-D and DMDS significantly reduced nematode populations. FEN was more effective in sandy soil, while OX had no effect in any soil. OX and FEN had no effect on fungal pathogens, whereas DMDS reduced the abundance of Rhizoctonia solani and Fusarium solani at the root level in clay-loam soil. Soil quality decreased after treatment application but then recovered throughout the experiment, indicating the possible dissipation of the pesticides. Our findings support DMDS as a potential sustainable alternative for controlling root-knot nematodes and fungal pathogens due to its effectiveness in both studied soils, although its negative impact on soil biological quality in sandier soils must be taken into account. Main finding of the work. DMDS is a reliable alternative to 1,3-D for controlling agricultural pest but its inhibitory effect on soil enzyme activities varied according to the soil characteristics., (Copyright © 2019 Elsevier Ltd. All rights reserved.)

Published

2019

23. Internal validation of GPS ™ MONODOSE CanAur dtec-qPCR kit following the UNE/EN ISO/IEC 17025:2005 for detection of the emerging yeast Candida auris.

Author

Martínez-Murcia A, Navarro A, Bru G, Chowdhary A, Hagen F, and Meis JF

Subjects

Africa, Candida classification, Candida genetics, Candidiasis diagnosis, Europe, Humans, Mycological Typing Techniques, Reproducibility of Results, Candida isolation & purification, Candidiasis microbiology, Real-Time Polymerase Chain Reaction methods

Abstract

Candida auris is an emerging multidrug resistant pathogenic fungus that causes candidaemia with high mortality rates and exhibits the ability to persist within the hospital environment. Candida auris is phylogenetically closely related to Candida haemulonii, C. lusitaniae, C. pseudohaemulonii and C. duobushaemulonii and is frequently misidentified by commercial identification methods. In the present study, the GPS ™ MONODOSE dtec-qPCR kit (dried single-dose PCR tubes) for the detection of C. auris was validated following the guidelines of the UNE/EN ISO/IEC 17025:2005, the French Standard NF T90-471:2010 and using fast-cycling protocols. Validation terms included in vitro specificity (inclusivity/exclusivity), quantitative phase analysis (10-10 6  standard DNA copies), reliability (repeatability/reproducibility) and sensitivity (detection/quantification limits). GPS ™ dtec-qPCR kits passed validation with strict acceptance criteria (n ≥ 10 repetitions). In silico specificity was proven by the designer (GPS ™ ). Experimental inclusiveness was achieved in two independent laboratories by testing strain JCM15448 T and 117 clinical C. auris isolates from Asia, the Middle-East Africa, Latin America and Europe. Exclusiveness was evaluated with 25 strains of closely related Candida spp. Use of the MONODOSE format provided considerable advantages allowing the detection of C. auris to be accurately achieved in less than an hour. The GPS ™ MONODOSE dtec-qPCR kit is ready to undergo clinical evaluation., (© 2018 Blackwell Verlag GmbH.)

Published

2018

24. Seek and Find! PCR analyses of skin infections in West-European travelers returning from abroad with an eschar.

Author

Morand A, Angelakis E, Ben Chaabane M, Parola P, Raoult D, and Gautret P

Subjects

Adolescent, Adult, Aged, Child, DNA, Bacterial, Diagnosis, Differential, Europe ethnology, Female, Humans, Male, Middle Aged, Necrosis microbiology, RNA, Ribosomal, 16S, Polymerase Chain Reaction methods, Skin Diseases, Infectious diagnosis, Skin Diseases, Infectious microbiology, Travel-Related Illness

Abstract

Background: Skin infections are among the leading causes of diseases in travelers. Diagnosing pathogens could be difficult., Method: We applied molecular assays for the diagnostic of a large collection of skin biopsies and swabs from travelers with suspected skin infections. All samples were tested by qPCR for Coxiella burnetti, Bartonella sp., Rickettsia sp., Borrelia sp., Ehrlichia sp., Tropheryma whipplei, Francisella tularensis, Mycobacteria sp., Staphylococcus aureus, Streptococcus pyogenes, Leishmania spp., Ortho poxvirus and Para poxvirus and then screened for the presence of bacteria by PCR amplification and sequencing, targeting the 16S rRNA gene., Results: From January 2009 to January 2017, 100 international travelers presenting with a suspected skin infection were enrolled. We detected 51 patients with an identified pathogen on skin samples. Travelers presenting with eschars were more likely to have a positive PCR sample (n = 44/76, 57.9%) compared to other patients (n = 7/24, 29.2%). Spotted fever group Rickettsia (n = 28) was the most frequently detected pathogens (19 R. africae, 6 R. conorii, 3 R. mongolitimonae); S. aureus were detected in 11 patients; S. pyogenes in 3; Leishmania sp.; M. leprae and B. henselae in 1 patient, respectively., Conclusion: By targeting the most commonly encountered causative agents of travel-related skin infections, our strategy provides a sensitive and rapid diagnostic method., (Copyright © 2018. Published by Elsevier Ltd.)

Published

2018

25. A unigene set for European beech (Fagus sylvatica L.) and its use to decipher the molecular mechanisms involved in dormancy regulation.

Author

Lesur I, Bechade A, Lalanne C, Klopp C, Noirot C, Leplé JC, Kremer A, Plomion C, and Le Provost G

Subjects

Europe, Expressed Sequence Tags, Gene Expression Profiling, Gene Library, Gene Ontology, Molecular Sequence Annotation, Molecular Sequence Data, Polymorphism, Single Nucleotide, Real-Time Polymerase Chain Reaction, Sequence Analysis, DNA, Fagus genetics, Fagus physiology, Gene Expression Regulation, Plant, Genetic Association Studies, Plant Dormancy

Abstract

Systematic sequencing is the method of choice for generating genomic resources for molecular marker development and candidate gene identification in nonmodel species. We generated 47,357 Sanger ESTs and 2.2M Roche-454 reads from five cDNA libraries for European beech (Fagus sylvatica L.). This tree species of high ecological and economic value in Europe is among the most representative trees of deciduous broadleaf forests. The sequences generated were assembled into 21,057 contigs with MIRA software. Functional annotations were obtained for 85% of these contigs, from the proteomes of four plant species, Swissprot accessions and the Gene Ontology database. We were able to identify 28,079 in silico SNPs for future marker development. Moreover, RNAseq and qPCR approaches identified genes and gene networks regulated differentially between two critical phenological stages preceding vegetative bud burst (the quiescent and swelling buds stages). According to climatic model-based projection, some European beech populations may be endangered, particularly at the southern and eastern edges of the European distribution range, which are strongly affected by current climate change. This first genomic resource for the genus Fagus should facilitate the identification of key genes for beech adaptation and management strategies for preserving beech adaptability., (© 2015 John Wiley & Sons Ltd.)

Published

2015