An improved rapid quantitative detection and identification method for a wide range of fungi

To develop a rapid and quantitative diagnostic technique for the detection and identification of a wide range of fungi, an improved molecular method based on real-time PCR and the analysis of its products that targets the internal transcribed spacer (ITS) 2 region was established. The real-time PCR could quantitatively and specifically detect the ITS2 region from all 24 tested pathogenic fungal species at between 101 and 107 copies per test without amplification of bacterial or human DNA. The sequences of the primer-binding sites are conserved in the registered sequences of 34 other pathogenic fungal species, suggesting that the PCR would also detect these species. The hyperpolymorphic nature of the ITS2 region between fungal species in terms of length and nucleotide sequence provided valuable information for the determination of species. By labelling the 5′ end of the reverse primer with NED fluorescent dye, the fragment lengths of the real-time PCR products and their 3′-terminal fragments, derived using restriction enzyme ScrFI digestion, were easily evaluated by capillary electrophoresis. Using this analysis, the number and species of fungi present in samples could be estimated. Moreover, sequence analysis of the real-time PCR products could accurately determine species in samples containing a single species. This diagnostic technique can estimate a wide range of fungi from various clinical samples within 1 day and accurately identify them in 2 days. Quantitative results for fungal titre in samples can also provide useful information for understanding the progression of disease and the efficacy of antifungal chemotherapy.

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Direct Quantitative Detection and Identification of Lactococcal Bacteriophages from Milk and Whey by Real-Time PCR: Application for the Detection of Lactococcal Bacteriophages in Goat's Raw Milk Whey in France

International Journal of Microbiology ◽

10.1155/2011/594369 ◽

2011 ◽

Vol 2011 ◽

pp. 1-9 ◽

Cited By ~ 8

Author(s):

Mai Huong Ly-Chatain ◽

Loïc Durand ◽

Véronique Rigobello ◽

Annabelle Vera ◽

Yann Demarigny

Keyword(s):

Real Time ◽

Real Time Pcr ◽

Direct Detection ◽

Raw Milk ◽

Quantitative Detection ◽

Amplification Efficiency ◽

The Real ◽

Milk Whey ◽

Detection And Identification ◽

Milk Fermentation

The presence ofLactococcusbacteriophages in milk can partly or completely inhibit milk fermentation. To prevent the problems associated with the bacteriophages, the real-time PCR was developed in this study for direct detection from whey and milk of three main groups ofLactococcusbacteriophages, c2, 936, and P335. The optimization of DNA extraction protocol from complex matrices such as whey and milk was optimized allowed the amplification of PCR without any matrix and nontarget contaminant interference. The real-time PCR program was specific and with the detection limit of 102PFU/mL. The curve slopes were −3.49, −3.69, and −3.45 with the amplification efficiency estimated at 94%, 94%, and 98% and the correlation coefficient () of 0.999, 0.999, and 0.998 for c2, 936 and P335 group, respectively. This method was then used to detect the bacteriophages in whey and goat's raw milk coming from three farms located in the Rhône-Alpes region (France).

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Real-Time Polymerase Chain Reaction Detection of Bovine DNA in Meat and Bone Meal Samples

Journal of Food Protection ◽

10.4315/0362-028x-65.7.1158 ◽

2002 ◽

Vol 65 (7) ◽

pp. 1158-1165 ◽

Cited By ~ 31

Author(s):

S. LAHIFF ◽

M. GLENNON ◽

J. LYNG ◽

T. SMITH ◽

N. SHILTON ◽

...

Keyword(s):

Real Time ◽

Real Time Pcr ◽

Meat And Bone Meal ◽

Bone Meal ◽

Chain Reaction ◽

Pcr Assay ◽

The Real ◽

Pcr Product ◽

Pcr Products ◽

Polymerase Chain

We describe a real-time polymerase chain reaction (PCR) assay for the detection of bovine DNA extracted from meat and bone meal (MBM) samples. PCR primers were used to amplify a 271-bp region of the mitochondrial ATPase 8–ATPase 6 gene, and a fluorogenic probe (BOV1) labeled with a 5′ FAM reporter and a 3′ TAMRA quencher was designed to specifically detect bovine PCR product. The specificity of the BOV1 probe for the detection of the bovine PCR product was confirmed by Southern blot hybridization analysis of the probe with PCR products generated from ovine, porcine, and bovine genomic DNA extracted from blood and with PCR products generated from genomic DNA extracted from single-species laboratory scale rendered MBM samples. The specificity of the BOV1 probe was also evaluated in real-time PCR reactions including these genomic targets. Both methods demonstrated that the BOV1 probe was specific for the detection of bovine PCR product. The BOV1 probe had a detection limit of 0.0001% bovine material by Southern blot DNA probe hybridization analysis and a detection limit of 0.001% bovine material in the real-time PCR assay. Application of the real-time PCR assay to six industrial samples that had previously tested positive for the presence of bovine material with a conventional PCR assay yielded positive results with the real-time PCR assay for four samples.

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DEVELOPMENT OF THE REAL-TIME PCR METHODOLOGY FOR TESTING MYCOTOXIGENIC MICROORGANISMS IN GRAPE MARC

Journal of Engineering Science ◽

10.52326/jes.utm.2021.28(3).15 ◽

2021 ◽

Vol 28 (3) ◽

pp. 187-194

Author(s):

Rodica Sturza ◽

◽

Valentin Mitin ◽

Irina Mitina ◽

Dan Zgardan ◽

...

Keyword(s):

Real Time ◽

Ochratoxin A ◽

Real Time Pcr ◽

Modern Society ◽

Fungal Species ◽

Peptide Sequence ◽

Wine Production ◽

The Real ◽

Grape Marc ◽

Industrial Waste Management

Agro-industrial waste management is an important problem of modern society as agriculture and food industry are important sources of waste. Wine production generates a considerable amount of winemaking waste (grape marc). Grape marc can be a source of natural dyes, antioxidants and could have various applications, if it is confirmed that it does not contain technogenic contaminants or unwanted microorganisms, for example, producers of mycotoxins. The paper developed the Real -Time Polymerase Chain Reaction (Real-Time PCR) methodology for testing the presence of potentially mycotoxogenic fungal species capable of producing ochratoxin A (OTA), which could be applied before grape marc processing. Based on the non-ribosomal peptide sequence of OTA, involved in ochratoxin biosynthesis, the primers have been developed for the detection of microorganisms potentially capable of producing ochratoxin A.

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Comparison of Real-Time Polymerase Chain Reaction and Enzyme-Linked Immunosorbent Assay for Sensitive and Quantitative Detection of Hazelnuts in Nut Pastes

Journal of AOAC International ◽

10.5740/jaoacint.18-0017 ◽

2018 ◽

Vol 101 (6) ◽

pp. 1864-1867 ◽

Cited By ~ 1

Author(s):

Ľubica Piknová ◽

Veronika Janská ◽

Tomáš Kuchta ◽

Peter Siekel

Keyword(s):

Real Time ◽

Real Time Pcr ◽

Sandwich Elisa ◽

Pcr Analysis ◽

Quantitative Detection ◽

Enzyme Linked Immunosorbent Assay ◽

Chain Reaction ◽

Wide Range ◽

Order Of Magnitude ◽

Polymerase Chain

Abstract Background: Hazelnuts, being a frequent agent of allergenic reactions, need to be detected in food products. Thus, it is necessary to develop and further investigate appropriate methods for detection. Objective: The aim of the study was to compare the analysis of nut pastes (peanut paste spiked with different amounts of hazelnut paste) as a model of contamination of confectionery. Methods: Real-time PCR and sandwich ELISA (RidaScreen Hazelnut Fast Kit) were used. Results: For real-time PCR, LOQ of 2 mg/kg and a quantification range from 2 to 10 000 mg/kg were determined. For ELISA, LOQ of 1 mg/kg and a quantification range from 1 to 100 mg/kg were determined. Conclusions: The comparison shows that the methods had comparable sensitivity with LOQs in the same order of magnitude. Although ELISA was slightly more sensitive, it required dilution of samples at higher concentrations of the analyte because of its narrow quantification range. Results of this study suggest that real-time PCR and ELISA are both suitable methods for the analysis of nut pastes over a wide range of concentrations. Achieved results could be useful for control as well as for technological purposes. Highlights: Real-time PCR analysis of peanut paste spiked with different amounts of hazelnut paste as a model is proposed. Sandwich ELISA analysis of peanut paste spiked with different amounts of hazelnut paste as a model is proposed. The analytical parameters of real-time PCR and ELISA methods are compared.

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Establishment of a PCR Assay for the Detection and Discrimination of Authentic Cordyceps and Adulterant Species in Food and Herbal Medicines

Molecules ◽

10.3390/molecules23081932 ◽

2018 ◽

Vol 23 (8) ◽

pp. 1932 ◽

Cited By ~ 4

Author(s):

Byeong Moon ◽

Wook Kim ◽

Inkyu Park ◽

Gi-Ho Sung ◽

Pureum Noh

Keyword(s):

Dietary Supplements ◽

Real Time ◽

Real Time Pcr ◽

Herbal Medicines ◽

Fungal Species ◽

Scar Markers ◽

Pcr Assay ◽

Food Ingredients ◽

The Real ◽

Species Specific

Accurate detection and differentiation of adulterants in food ingredients and herbal medicines are crucial for the safety and basic quality control of these products. Ophiocordyceps sinensis is described as the only fungal source for the authentic medicinal ingredient used in the herbal medicine “Cordyceps”, and two other fungal species, Cordyceps militaris and Isaria tenuipes, are the authentic fungal sources for food ingredients in Korea. However, substitution of these three species, and adulteration of herbal material and dietary supplements originating from Cordyceps pruinosa or Isaria cicadae, seriously affects the safety and reduces the therapeutic efficacy of these products. Distinguishing between these species based on their morphological features is very difficult, especially in commercially processed products. In this study, we employed DNA barcode-based species-specific sequence characterized amplified region (SCAR) markers to discriminate authentic herbal Cordyceps medicines and Cordyceps-derived dietary supplements from related but inauthentic species. The reliable authentication tool exploited the internal transcribed spacer (ITS) region of a nuclear ribosomal RNA gene (nrDNA). We used comparative nrDNA-ITS sequence analysis of the five fungal species to design two sets of SCAR markers. Furthermore, we used a set of species-specific SCAR markers to establish a real-time polymerase chain reaction (PCR) assay for the detection of species, contamination, and degree of adulteration. We confirmed the discriminability and reproducibility of the SCAR marker analysis and the real-time PCR assay using commercially processed food ingredients and herbal medicines. The developed SCAR markers may be used to efficiently differentiate authentic material from their related adulterants on a species level. The ITS-based SCAR markers and the real-time PCR assay constitute a useful genetic tool for preventing the adulteration of Cordyceps and Cordyceps-related dietary supplements.

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Multiplex Fast Real-Time PCR for Quantitative Detection and Identification of cos- and pac-Type Streptococcus thermophilus Bacteriophages

Applied and Environmental Microbiology ◽

10.1128/aem.00295-08 ◽

2008 ◽

Vol 74 (15) ◽

pp. 4779-4781 ◽

Cited By ~ 23

Author(s):

Beatriz del Rio ◽

María Cruz Martín ◽

Noelia Martínez ◽

Alfonso H. Magadán ◽

Miguel A. Alvarez

Keyword(s):

Real Time ◽

Real Time Pcr ◽

Industrial Process ◽

Streptococcus Thermophilus ◽

Quantitative Detection ◽

Detection And Identification ◽

Pcr Method

ABSTRACT The fermentation of milk by Streptococcus thermophilus is a widespread industrial process that is susceptible to bacteriophage attack. In this work, a preventive fast real-time PCR method for the detection, quantification, and identification of types of S. thermophilus phages in 30 min is described.

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Rapid and Simultaneous Quantitation of Escherichia coli O157:H7, Salmonella, and Shigella in Ground Beef by Multiplex Real-Time PCR and Immunomagnetic Separation†

Journal of Food Protection ◽

10.4315/0362-028x-70.6.1366 ◽

2007 ◽

Vol 70 (6) ◽

pp. 1366-1372 ◽

Cited By ~ 104

Author(s):

LUXIN WANG ◽

YONG LI ◽

AZLIN MUSTAPHA

Keyword(s):

Escherichia Coli ◽

Detection Limit ◽

Real Time ◽

Real Time Pcr ◽

Ground Beef ◽

Immunomagnetic Separation ◽

Quantitative Detection ◽

Escherichia Coli O157 ◽

The Real ◽

E Coli

The objective of this study was to establish a multiplex real-time PCR for the simultaneous quantitation of Escherichia coli O157:H7, Salmonella, and Shigella. Genomic DNA for the real-time PCR was extracted by the boiling method. Three sets of primers and corresponding TaqMan probes were designed to target these three pathogenic bacteria. Multiplex real-time PCR was performed with TaqMan Universal PCR Master Mix in an ABI Prism 7700 Sequence Detection System. Final standard curves were calculated for each pathogen by plotting the threshold cycle value against the bacterial number (log CFU per milliliter) via linear regression. With optimized conditions, the quantitative detection range of the real-time multiplex PCR for pure cultures was 102 to 109 CFU/ml for E. coli O157:H7, 103 to 109 CFU/ml for Salmonella, and 101 to 108 CFU/ml for Shigella. When the established multiplex real-time PCR system was applied to artificially contaminated ground beef, the detection limit was 105 CFU/g for E. coli O157:H7, 103 CFU/g for Salmonella, and 104 CFU/g for Shigella. Immunomagnetic separation (IMS) was further used to separate E. coli O157:H7 and Salmonella from the beef samples. With the additional use of IMS, the detection limit was 103 CFU/g for both pathogens. Results from this study showed that TaqMan real-time PCR, combined with IMS, is potentially an effective method for the rapid and reliable quantitation of E. coli O157:H7, Salmonella, and Shigella in food.

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A Real-Time, Quantitative PCR Seed Assay for Botrytis spp. that Cause Neck Rot of Onion

Plant Disease ◽

10.1094/pdis-91-5-0599 ◽

2007 ◽

Vol 91 (5) ◽

pp. 599-608 ◽

Cited By ~ 52

Author(s):

Martin I. Chilvers ◽

Lindsey J. du Toit ◽

Hajime Akamatsu ◽

Tobin L. Peever

Keyword(s):

Real Time ◽

Real Time Pcr ◽

Intergenic Spacer ◽

Fungal Species ◽

Pcr Assay ◽

The Real ◽

Real Time Quantitative Pcr ◽

Onion Seed ◽

Pure Cultures ◽

Fluorescent Polymerase Chain Reaction

A real-time fluorescent polymerase chain reaction (PCR) assay was developed using SYBR Green chemistry to quantify the Botrytis spp. associated with onion (Allium cepa) seed that are also able to induce neck rot of onion bulbs, i.e., B. aclada, B. allii, and B. byssoidea. The nuclear ribosomal intergenic spacer (IGS) regions of target and nontarget Botrytis spp. were sequenced, aligned, and used to design a primer pair specific to B. aclada, B. allii, and B. byssoidea. Primers and amplification parameters were optimized to avoid amplifying the related species B. cinerea, B. porri, and B. squamosa, as well as Sclerotinia sclerotiorum and isolates of 15 other fungal species commonly found associated with onion seed. The primers reliably detected 10 fg of genomic DNA per PCR reaction extracted from pure cultures of B. aclada and B. allii. Conventional assays of surface-disinfested and nondisinfested seed on an agar medium were used to determine the incidence of neck rot Botrytis spp. associated with each of 23 commercial onion seed lots, and the real-time PCR assay was used to determine the quantity of DNA of neck rot Botrytis spp. in each seed lot. A linear relationship could not be found between the incidence of seed infected with the neck rot Botrytis spp. using the conventional agar seed assays and the quantity of DNA of the neck rot Botrytis spp. detected by the real-time PCR assay. However, the real-time PCR assay appeared to be more sensitive than the conventional agar assay, allowing detection of neck rot Botrytis spp. in 5 of the 23 seed lots that tested negative using the conventional agar seed assay.

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Research of the Real Time PCR method for detection and identification phytoplasmas on grapevine

RUDN Journal of Agronomy and Animal Industries ◽

10.22363/2312-797x-2015-4-7-14 ◽

2015 ◽

pp. 7-14

Author(s):

G.N. Matyashova ◽

◽

V.G. Zaets ◽

Keyword(s):

Real Time ◽

Real Time Pcr ◽

The Real ◽

Detection And Identification ◽

Pcr Method

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A Real-Time PCR Assay for Early Detection of Eastern Filbert Blight

Plant Disease ◽

10.1094/pdis-11-12-1041-re ◽

2013 ◽

Vol 97 (6) ◽

pp. 813-818 ◽

Cited By ~ 6

Author(s):

Thomas J. Molnar ◽

Emily Walsh ◽

John M. Capik ◽

Vidyasagar Sathuvalli ◽

Shawn A. Mehlenbacher ◽

...

Keyword(s):

Real Time ◽

Real Time Pcr ◽

Diagnostic Methods ◽

Economic Losses ◽

Pcr Assay ◽

The Real ◽

Detection And Identification ◽

Anisogramma Anomala ◽

Eastern Filbert Blight ◽

Branch Dieback

Eastern filbert blight (EFB) is a devastating disease of European hazelnut, Corylus avellana, which causes economic losses in Oregon, where 99% of the U.S. crop is produced. The causal fungus, Anisogramma anomala, is native to eastern North America, where it is found associated with the American hazelnut (C. americana). Although C. americana is tolerant, EFB causes cankers, branch dieback, and death of C. avellana. Detection and identification of A. anomala is time consuming using conventional methods because the fungus can only be cultured from sporulating perithecia and the disease symptoms and signs only show 12 to 16 months after infection. In this study, a TaqMan real-time polymerase chain reaction (PCR) assay based on a ribosomal DNA internal transcribed spacer was developed for A. anomala. The assay was validated with multiple isolates of A. anomala, closely related species, common environmental microorganisms, and over 100 C. avellana samples. The real-time PCR assay detected as low as 0.12 pg of A. anomala genomic DNA, and positively diagnosed EFB on 82% of asymptomatic plants as early as 15 weeks from infection. The real-time PCR assay is more sensitive and faster than traditional diagnostic methods. It can facilitate hazelnut breeding and disease management by early and accurate diagnosis of EFB.

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