Browsing by Subject "Real time quantitative PCR"
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Publication Entwicklung und Validierung schneller und selektiver Verfahren zum Nachweis von Salmonella enterica, Cronobacter spp. und Bacillus cereus in Milcherzeugnissen(2014) Zimmermann, Jennifer; Schmidt, HerbertThe presence of pathogens is a serious problem in the food industry and contaminations of food with Bacillus cereus, Cronobacter spp. and Salmonella enterica are responsible for a large number of diseases worldwide. Milk products like milk, whey or cream powder are widely used in industry as an ingredient in other foods. Therefore it requires a fast and reliable identification of pathogenic microorganisms. The official methods according to § 64 LFGB or ISO/TS 22964 apply a common scheme of pre-enrichment, selective enrichment, detection and confirmation and take between three and six days. The aim of this work was the development and validation of a real-time PCR based method, which identifies the existence of the three pathogens in dairy products within 24 hours. The identification of B. cereus, Cronobacter spp. and S. enterica with the developed TaqMan real-time PCR was performed using specific genetic characteristics and an internal amplification control to eliminate false negative results. For B. cereus, the groEL gene, which codes for a heat shock protein, was selected as target. For the detection of Cronobacter spp. the ompA gene and for S. enterica the invA gene was chosen. Both genes are responsible for the invasion of the pathogens in the human epithelial cells. The adaptation of the method to the food matrix and an optimization of the enrichment time were affected by an artificial contamination of various dry dairy products. It was possible to detect 105 cfu/g C. sakazakii and S. Enteritidis cells with an initial concentration of 100 cfu/g in reconstituted powdered infant formula after enrichment of six hours. To simulate a natural contamination, powdered infant formula was contaminated with desiccated C. sakazakii cells in various concentrations and analyzed with the developed real-time PCR method. It was possible to detect an inoculum concentration of 0.01 CFU/g dry stressed C. sakazakii cells at low aw values (0.22). The new TaqMan real-time PCR is fast, reliable and specific for the clearly detection of the three major pathogenic microorganisms in milk products and was carried out within 24 hours.Publication Etablierung eines Wirts-induzierten RNAi-Systems für die Kontrolle des Asiatischen Sojabohnenrostes Phakopsora pachyrhizi(2015) Müller, Manuel; Vögele, RalfPhakopsora pachyrhizi, the causal agent of Asian Soybean Rust is a devastating plant pathogen that can cause significant yield losses in soybean production. So far, Phakopsora pachyrhizi is controlled by the use of fungicides and cultivation practices. A future perspective for the control of obligate biotrophic pathogens such as Phakopsora pachyrhizi, is Host-induced Gene Silencing (HIGS), which utilizes the naturally occuring phenomenon of RNA-interference (RNAi). The basic principle of HIGS is the induction of RNAi targeted against RNA of the fungal pathogen by means of transgenic expression of double stranded RNA (dsRNA) in the host plant. HIGS can be performed by either generating stable transgenic plants or using transient expression systems mainly based on recombinant viral vector systems. Recently, the basic principle of HIGS has been demonstrated in a variety of obligate biotrophic fungal pathogens including the powdery mildew fungus Blumeria graminis or the cereal rusts Puccinia striiformis f. sp. tritici and Puccinia triticina. Furthermore, work on different Fusarium spp. clearly indicates that the use of HIGS can be transferred to pertotrophic pathogens. Althought there is remarkable progress in utilizing HIGS in cereal rusts, to date, no such system has been reported for legume rusts. Thus, the work presented was focused on the development and testing of a HIGS system for the Asian Soybean Rust Phakopsora pachyrhizi. An initial set of ten target genes, presumably essential for signaling, nutrient uptake and host-pathogen interaction, was selected from a database reflecting the haustorial transcriptome of Phakopsora pachyrhizi. Expression of dsRNA complementary to the selected target genes was done using a viral vector system based on the Bean Pod Mottle Virus (BPMV). As an alternative method the use of agroinfiltration for the expression of hairpin RNA (hpRNA) was examined. By using the viral vector system silencing effects were observed for the three target genes Pp_contig01251, Pp_contig05320, and Pp_contig3015. Furthermore, the silencing of Pp_contig05320 resulted in inhibited growth of Phakopsora pachyrhizi as indicated by a reduced number of uredia. The use of agroinfiltration for the expression of hpRNA was not successful. Infiltration of soybean using a syringe resulted in deformation and necrosis of the infiltrated leaf areas. Although the expression of hpRNA could not be realized, the transient transformation of Glycine max via the use of agroinfiltration was demonstrated using a marker gene construct. Concerning the analysis of silencing effects via the use of RT-qPCR, the expression stability of 15 genes from Phakopsora pachyrhizi and 10 genes from Glycine max was analyzed to identify stably expressed reference genes. These studies resulted in the identification of several reference genes, suitable for the normalization of expression data collected under different experimental conditions. The results from this work provide a foundation for further examinations and experiments. Open questions especially concern the factors delimiting a gene as a suitable target gene for HIGS and the molecular mechanism behind the uptake and the translocation of silencing signals in Phakopsora pachyrhizi. Answering these questions will promote the establishment of HIGS as a promising perspective for modern plant protection.Publication Species of the Diaporthe/Phomopsis Complex (DPC) in European soybean and establishment of quadruplex Real-Time PCR for diagnosis(2022) Hosseini, Behnoush; Vögele, RalfDiaporthe seed decay is among the most disruptive soybean diseases around the world, which cause significant yield losses and affect soybean quality. Different Diaporthe species cause this disease, while Diaporthe longicolla is considered the main causal agent. The species of this fungal complex (genus Diaporthe is also called the Diaporthe/Phomopsis Complex / DPC) have to be accurately identified for epidemiological studies of the disease and for optimal control measures. To identify the major causal agents of seed decay in Europe, DPC-damaged soybean seeds of various cultivars, that were collected from different fields in Germany, France, and Austria were tested by seed plating. 32 Diaporthe isolates could be obtained. The isolates were morphologically identified by the colors and shape of the colony, conidia dimensions, and by whether pycnidia with α- and/or β-conidia or perithecia with ascospores are formed. To corroborate morphological identification, sequences of the internal transcribed spacer (ITS), translation elongation factor 1-α (TEF1), and beta-tubulin (TUB) sequences were obtained. From the results of both morphological and molecular analyses it became clear that all isolates belong to one of the four species D. longicolla, D. caulivora, D. eres, and D. novem. The pathogenicity of all strains on soybean was tested. Molecular phylogenies were calculated and based on the above results updated species descriptions were created. This study identified these four species as the main Diaporthe pathogens for soybean in central Europe. A sensitive and accurate method for quick detection of these pathogens was developed based on multiplex real-time PCR. Specific TaqMan primer-probe sets for the four species were designed based on TEF1 sequences. The primer-probe sets were tested for specificity and efficiency using PCR products and genomic DNA from the four Diaporthe species and several other soybean pathogens. These primer-probe sets reliably distinguish the different species and they can be used to detect them in the same reaction by quadruplex real-time PCR. DNA from different soybean plant materials including healthy and infected seeds or seed coats, stems, and leaves was used to test the quadruplex real-time PCR assay. Application of the assay was extended to quantify the pathogens. Standard curves for the four species were created from serial dilutions of genomic DNA diluted with DNA from soybean tissue. An additional standard curve was created from serial dilutions of soybean DNA diluted with ddH2O. To gain the ratio of fungal DNA per plant DNA (ng/ng), DNA samples from soybean tissues can now be examined in the new assay and a parallel SYBR® Green-based real-time PCR. The assay was first applied to six soybean seed lots with putative Diaporthe contamination. In all seed lots seeds contaminated with Diaporthe species and even some seeds infected with more than one Diaporthe species were found, while other seeds were free of the pathogens. The load of fungal biomass varies strongly between individual seeds.