Development of specific primers to Hirschmanniella spp. causing damage to lotus and their economic threshold level in Tokushima prefecture in Japan

Nematode diseases caused by Hirschmanniella spp. are becoming a major threat to lotus production in Tokushima Prefecture, a primary production area in Japan. The objectives of this study were: i) to design specific primers to Hirschmanniella spp. causing damage to lotus; ii) to evaluate the relationship between pre-plant density of Hirschmanniella spp. in soil and damage index of lotus; and iii) to establish an economic threshold level. Since two species, Hirschmanniella imamuri and H. diversa, are known as nematode pests on lotus, three real-time PCR primers were designed based on the ITS regions specific to H. imamuri (designated as imaF and imaR), H. diversa (divF and divR), and both species (HdiF and HdiR). The primers imaF and imaR did not react to DNA of nematodes extracted from lotus fields in Tokushima but the primers divF and divR did, suggesting that the damage seen in Tokushima is mainly caused by H. diversa. A calibration curve was made to evaluate the relationship between the number of Hirschmanniella spp. inoculated to soil and the threshold cycle values. The quantification of Hirschmanniella spp. in soil was conducted by real-time PCR method with the primers HdiF and HdiR as well as the Baermann method. The economic threshold level was estimated as ten individuals of Hirschmanniella spp. (100 g fresh soil)−1 with the Baermann method and 50 individuals (100 g oven-dried soil)−1 with real-time PCR.

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Real-Time PCR Assay for Detection and Enumeration of Dekkera bruxellensis in Wine

Applied and Environmental Microbiology ◽

10.1128/aem.69.12.7430-7434.2003 ◽

2003 ◽

Vol 69 (12) ◽

pp. 7430-7434 ◽

Cited By ~ 77

Author(s):

Trevor G. Phister ◽

David A. Mills

Keyword(s):

Real Time ◽

Real Time Pcr ◽

Pcr Primers ◽

Rrna Gene ◽

Dekkera Bruxellensis ◽

Pcr Assay ◽

Specific Pcr ◽

Spoilage Yeast ◽

Pcr Method ◽

26S Rrna

ABSTRACT Traditional methods to detect the spoilage yeast Dekkera bruxellensis from wine involve lengthy enrichments. To overcome this difficulty, we developed a quantitative real-time PCR method to directly detect and enumerate D. bruxellensis in wine. Specific PCR primers to D. bruxellensis were designed to the 26S rRNA gene, and nontarget yeast and bacteria common to the winery environment were not amplified. The assay was linear over a range of cell concentrations (6 log units) and could detect as little as 1 cell per ml in wine. The addition of large amounts of nontarget yeasts did not impact the efficiency of the assay. This method will be helpful to identify possible routes of D. bruxellensis infection in winery environments. Moreover, the time involved in performing the assay (3 h) should enable winemakers to more quickly make wine processing decisions in order to reduce the threat of spoilage by D. bruxellensis.

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Building a molecular typing protocol for rs1801133 based on real-time PCR HRM technique

Science and Technology Development Journal - Natural Sciences ◽

10.32508/stdjns.v2i3.747 ◽

2019 ◽

Vol 2 (3) ◽

pp. 5-13

Author(s):

Linh Thi Nhut Tran ◽

My Thi Huynh Nguyen ◽

Linh Nguy Hoang Le ◽

Khoa Dang Le ◽

Minh Hoang Nhat Nguyen ◽

...

Keyword(s):

Real Time ◽

Real Time Pcr ◽

Neurological Diseases ◽

Human Diseases ◽

Chromosome 1 ◽

Nucleotide Sequencing ◽

Sequencing Method ◽

Mgcl2 Concentration ◽

Clear Differentiation ◽

The Relationship

rs1801133 is a single nucleotide polymorphism (SNP) located in the sequence of MTHFR on human chromosome 1. The alleles of this SNP affect the activity of the MTHFR enzyme. People bearing C/T genotype have 66% activity of MTHFR while people with T/T genotype have only 25% activity. These reduced activities of MTHFR cause homocysteinemia. There are several publications on the relationship between homocysteinemia and human diseases such as cardiovascular disease, neurological diseases, abnormal fetus, infertility and cancer. In this study, we built a molecular protocol for genotyping rs1801133 using real-time PCR HRM technique. This protocol could be used for diagnosis of molecular mechanism of homocysteinemia causing the mentoned above diseases as well as for the study of the relationship between rs1801133 and other human diseases. We successfully designed the primer pairs for genotyping and nucleotide sequencing rs1801133 by real-time PCR HRM and Sanger sequencing method. We also examined the optimal MgCl2 concentration for clear differentiation of three rs1801133 genotypes. Performance characteristics of the real-time PCR HRM protocol included of specificity, repeatability, reproducibility was evaluated and it showed good results. Comparison of genotyping results of rs1801133 between the realtime PCR HRM method and the Sanger nucleotide sequencing method showed good concordances. Finally, this real-time PCR HRM protocol for rs1801133 genotyping was applied on 100 human DNA samples to evaluate the clinical utility of the protocol.

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Developing, Modifying, and Validating a TaqMan Real-Time PCR Technique for Accurate Identification of Leishmania Parasites Causing Most Leishmaniasis in Iran

Frontiers in Cellular and Infection Microbiology ◽

10.3389/fcimb.2021.731595 ◽

2021 ◽

Vol 11 ◽

Author(s):

Reza Fotouhi-Ardakani ◽

Seyedeh Maryam Ghafari ◽

Paul Donald Ready ◽

Parviz Parvizi

Keyword(s):

Real Time ◽

Real Time Pcr ◽

Leishmania Major ◽

Taqman Probe ◽

Amino Acid Permease ◽

Specific Primers ◽

Accurate Identification ◽

Parasitic Load ◽

Species Specific

Many laboratory methods are used to diagnose leishmaniasis because it is characterized by varied symptoms and caused by different Leishmania species. A quantitative real-time PCR method based on a TaqMan probe was developed and modified for accurate identification of human cutaneous leishmaniasis (caused by Leishmania major or Leishmania tropica) from endemic areas of Iran. Two gene regions of amino acid permease 3 (AAP3) and cytochrome oxidase II (COII) were considered. Six new sets of species-specific primers and probes were designed. A total of 123 samples were examined and employed to evaluate and validate real-time PCR. According to parasitic load of the genesig®Leishmania Advanced Standard Kit, a serial dilution of purified plasmid (2–2×107 copies/reaction) was prepared under the same conditions for both genes. Specific primers and probes were able to detect three and six parasite copies in AAP3 and COII genes, respectively, and were able to detect three copies of parasites for L. major and L. tropica. The sensitivities of the reference kit and our method were 98.7 and 98.1%, respectively, and specificity was 100% for detecting parasite genomes in all assays. Designed primers and probes performed well in terms of efficiency and regression coefficient. For AAP3 and COII genes, respectively, the linear log range was 7 and the correlation coefficient (R2) was 0.749 and 0.996 for the reference kit using the standard generated curve and 0.98 and 0.96 with serial dilutions of parasite DNA. This research detected L. major and L. tropica definitely and opens the horizon for the other scientists in the multiplex reactions in designing and optimization of the conditions in silico and in vivo.

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Co-infection of bovine papillomavirus type-1 and -10 in teat warts of dairy cattle

Veterinární Medicína ◽

10.17221/7178-vetmed ◽

2013 ◽

Vol 58 (No. 12) ◽

pp. 605-608

Author(s):

P. Kumar ◽

BL Jangir ◽

G. Saikumar ◽

R. Somvanshi

Keyword(s):

Dairy Cattle ◽

Real Time ◽

Real Time Pcr ◽

Rice Grain ◽

Bovine Papillomavirus ◽

Viral Dna ◽

Specific Primers ◽

Copy Numbers ◽

Pcr Techniques

The present study was carried out to investigate the involvement of different bovine papillomaviruses in the teat warts of cattle. A total of 11 teat wart samples showing rice grain-like and small, sessile elevated greyish or flesh-like growths were collected from dairy cattle. DNA was extracted from these teat wart samples and PCR and real time PCR techniques were applied using specific primers for BPV-1 and -10 to detect the presence of viral nucleic acid. PCR revealed the presence of viral DNA of BPV-1 and -10 in three and seven samples, respectively. Quantification using real time PCR revealed that the copy numbers of the viral DNA of BPV-1 and -10 DNA varied from 1.12E + 04 to 2.99E + 04 and 3.56E + 02 to 5.23E + 06, respectively. From the present study it can be concluded that BPV-1 and -10 are involved in production of rice grain-like and sessile elevated growths on the teats of cattle.

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Real-time PCR Assay with SNP-specific Primers for the Detection of a G143A Mutation Level in Venturia inaequalis Field Populations

Journal of Phytopathology ◽

10.1111/j.1439-0434.2011.01805.x ◽

2011 ◽

Vol 159 (7-8) ◽

pp. 569-578 ◽

Cited By ~ 8

Author(s):

Monika Michalecka ◽

Tadeusz Malinowski ◽

Agata Broniarek-Niemiec ◽

Anna Bielenin

Keyword(s):

Real Time ◽

Real Time Pcr ◽

Venturia Inaequalis ◽

Pcr Assay ◽

Specific Primers

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Evaluation of Two DNA Extraction Methods for Detection of Strongyloides stercoralis Infection

Journal of Clinical Microbiology ◽

10.1128/jcm.01941-17 ◽

2018 ◽

Vol 56 (4) ◽

Cited By ~ 5

Author(s):

Beatrice Barda ◽

Rahel Wampfler ◽

Somphou Sayasone ◽

Khampheng Phongluxa ◽

Syda Xayavong ◽

...

Keyword(s):

Real Time ◽

Real Time Pcr ◽

Strongyloides Stercoralis ◽

Extraction Methods ◽

Molecular Techniques ◽

Diagnostic Methods ◽

Content Type ◽

Stool Samples ◽

Dna Extraction Methods ◽

Baermann Method

ABSTRACT Strongyloides stercoralis is present worldwide, but its prevalence is still uncertain, mainly due to the lack of sensitivity of diagnostic methods. Molecular techniques are under development, but a standardized protocol is still unavailable. We compared the sensitivity of real-time PCR, using two extraction protocols, with that of the Baermann technique. Samples were collected in the framework of the baseline screening of a randomized clinical trial evaluating moxidectin against S. stercoralis in Lao People's Democratic Republic. Two stool samples from each participant were processed by the Baermann method, and one subsample was processed by PCR. DNA was extracted using the QIAamp DNA stool minikit based on the standard protocol for the QIAamp DNA minikit (QIA) and using a modification of the QIA procedure (POL). Subsequently, all extracted samples were analyzed by real-time PCR. Overall, 95 samples were analyzed by the three diagnostic methods. Sixty-nine (72.6%) samples were positive according to the Baermann method, 25 (26.3%) by the QIA method, and 62 (65.3%) by the POL method. The sensitivities were 86% (95% confidence interval [CI], 76.7 to 92.9), 31.0% (95% CI, 21.3 to 42.6), and 78.0% (95% CI, 66.8 to 86.1) for the Baermann, QIA, and POL methods, respectively. The sensitivities calculated for each day of the Baermann method separately were 60% (48.4 to 70.8%) and 64% (52.2 to 74.2%) for days 1 and 2, respectively. In conclusion, the POL method revealed a good performance and was comparable to the Baermann test performed on two stool samples and superior to the Baermann method performed on one stool sample. Additional studies are needed to standardize a PCR protocol for S. stercoralis diagnosis.

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Decreased miRNA-146A in Glioblastoma Multiforme and Regulation of Cell Proliferation and Apoptosis by Target Notch1

The International Journal of Biological Markers ◽

10.5301/jbm.5000194 ◽

2016 ◽

Vol 31 (3) ◽

pp. 270-275 ◽

Cited By ~ 8

Author(s):

Hong-qi Hu ◽

Lai-guang Sun ◽

Wu-jun Guo

Keyword(s):

Glioblastoma Multiforme ◽

Cell Viability ◽

Real Time ◽

Real Time Pcr ◽

Glioma Cells ◽

Viability Analysis ◽

Nontumor Tissue ◽

Proliferation And Apoptosis ◽

A Cell ◽

The Relationship

Objective The primary purpose of this paper is to investigate the relationship between the microRNA 146a (miR-146a) and the proliferation of cells occurring in glioblastoma multiforme. The secondary purpose of the paper is to investigate abnormalities of expression in miR-146a. Methods A real-time PCR assay was used to investigate the abnormal expression of miR-146a in glioma and adjacent tissue. Lipofection was used to transfect a mimic of miR-146a and induce the upregulation of miR-146a. Real-time PCR was used to observe the expression level of miR-146a. A cell viability analysis was conducted using MTT. A luciferase report vector was used to identify potential targets for miR-146a. Results The miR-146a component was found to be downregulated in glioma tissue compared with adjacent nontumor tissue (p<0.05). The upregulation of miR-146a in glioma cells through miR-146a mimic transfection led to reduction of cell viability and to an increase in the percentage of apoptosis. Notch1 was the name of the potential targeted gene for miR-146a in glioma. Conclusions The study found that the presence of miR-146a potentially affected the proliferation of glioma cells by regulating the rate of Notch1 expression.

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Quantitative PCR with 16S rRNA-Gene-Targeted Species-Specific Primers for Analysis of Human Intestinal Bifidobacteria

Applied and Environmental Microbiology ◽

10.1128/aem.70.1.167-173.2004 ◽

2004 ◽

Vol 70 (1) ◽

pp. 167-173 ◽

Cited By ~ 309

Author(s):

Takahiro Matsuki ◽

Koichi Watanabe ◽

Junji Fujimoto ◽

Yukiko Kado ◽

Toshihiko Takada ◽

...

Keyword(s):

Real Time ◽

Quantitative Pcr ◽

Real Time Pcr ◽

Intestinal Flora ◽

Healthy Adults ◽

Pcr Detection ◽

Distribution Analysis ◽

Specific Primers ◽

Cell Counts ◽

Species Specific

ABSTRACT A highly sensitive quantitative PCR detection method has been developed and applied to the distribution analysis of human intestinal bifidobacteria by combining real-time PCR with Bifidobacterium genus- and species-specific primers. Real-time PCR detection of serially diluted DNA extracted from cultured bifidobacteria was linear for cell counts ranging from 106 to 10 cells per PCR assay. It was also found that the method was applicable to the detection of Bifidobacterium in feces when it was present at concentrations of >106 cells per g of feces. Concerning the distribution of Bifidobacterium species in intestinal flora, the Bifidobacterium adolescentis group, the Bifidobacterium catenulatum group, and Bifidobacterium longum were found to be the three predominant species by examination of DNA extracted from the feces of 46 healthy adults. We also examined changes in the population and composition of Bifidobacterium species in human intestinal flora of six healthy adults over an 8-month period. The results showed that the composition of bifidobacterial flora was basically stable throughout the test period.

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Variance Calculations for Quantitative Real-Time PCR Experiments with Multiple Levels of Replication

Advanced Materials Research ◽

10.4028/www.scientific.net/amr.825.172 ◽

2013 ◽

Vol 825 ◽

pp. 172-176

Author(s):

Susana Soto-Rojo ◽

Gary Glonek ◽

Cecilia Demergasso ◽

Pedro A. Galleguillos ◽

Patty Solomon ◽

...

Keyword(s):

Real Time ◽

Real Time Pcr ◽

Industrial Process ◽

Error Variance ◽

Low Grade ◽

Sulphide Ores ◽

Polymerase Chain ◽

Frequent Sampling ◽

The Relationship ◽

Proportional Reduction

Heap bioleaching is an established technology for recovering copper from low-grade sulphide ores. Recently, genetics-based approaches have been employed to characterize mineral-processing bacteria. In these approaches, data analysis is a key issue. Consequently, it is of fundamental importance to provide adequate mathematical models and statistical tools to draw reliable conclusions. The present work relates to current studies of the consortium of organisms inhabiting the bioleaching heap of the Escondida mine in Northern Chile. These studies aim to describe and understand the relationship between the dynamics of the community and the performance of the industrial process. Here, we consider a series of quantitative real-time polymerase chain reaction (PCR) experiments performed to quantify six different microorganisms at various stages of the bioleaching cycle. Establishing the reliability of the data obtained by real-time PCR requires the estimation of the error variance at several different levels. The results obtained show that the sampling component of the error variance is the dominant source of variability for most microorganisms. An estimate for the proportional reduction in residual standard deviation from the use of extraction and real-time PCR triplicates was found to range from 3% to 27% for the different organisms. This result suggests that triplicate assays would produce only a modest reduction in error variance compared to more frequent sampling from the heap.

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Differentiation of infectious bronchitis virus vaccine strains Ma5 and 4/91 by TaqMan real-time PCR

Polish Journal of Veterinary Sciences ◽

10.1515/pjvs-2017-0073 ◽

2017 ◽

Vol 20 (3) ◽

pp. 599-601 ◽

Cited By ~ 5

Author(s):

T. Stenzel ◽

D. Dziewulska ◽

M. Śmiałek ◽

B. Tykałowski ◽

J. Kowalczyk ◽

...

Keyword(s):

Real Time ◽

Virus Vaccine ◽

Infectious Bronchitis Virus ◽

Real Time Pcr ◽

Cross Reactivity ◽

Specific Primers ◽

Assay Sensitivity ◽

Infectious Bronchitis ◽

Molecular Assays ◽

Rapid Molecular Assays

Abstract The aim of this study was to develop rapid molecular assays for differentiating vaccine strains Ma5 and 4/91 of the infectious bronchitis virus (IBV). Specific primers and probes for S1 and N genes were designed based on the nucleotide sequences of both vaccine strains. Cross-reactivity was not observed. Assay sensitivity was 2.373 × 103 copies of the Ma5 strain, and 3.852 x 103 copies of the 4/91 strain. Samples belonging to a known genotype demonstrated that the designed assays supported rapid and sensitive detection of Ma5 and 4/91 vaccine strains of IBV.

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