Your search keyword '"Electrophoresis"' showing total 3,377 results

1. Purification and Amplification of DNA from Cellulolytic Bacteria: Application for Biogas Production from Crop Residues.

Author

Kamusoko R, Jingura RM, Parawira W, and Chikwambi Z

Subjects

Bacillus genetics, Bacteria classification, Bacteria genetics, Cellulomonas genetics, Clostridium genetics, DNA, Bacterial genetics, Electrophoresis methods, Pseudomonas genetics, Rhodothermus genetics, Biofuels microbiology, DNA, Bacterial isolation & purification, Polymerase Chain Reaction methods

Abstract

Polymerase chain reaction (PCR) is a popular molecular tool for detection of bacteria. PCR allows millions of copies of a target segment of DNA to be produced. The DNA is extracted from overnight grown cultures of pure bacterial isolates using either the organo-solvent method or a commercial DNA extraction kit. The quality and purity of the DNA is determined by performing gel electrophoresis on 0.8% agarose gel. The DNA is amplified by performing PCR assay. Bands of approximately 1.5 kb in size are obtained from the amplified products of DNA. The PCR products run on 1.5% agarose gel are visualized with UV light and imaged by gel documentation system. This chapter outlines the protocol for isolation and amplification of DNA from cellulolytic bacteria. Cellulolytic bacteria are considered a potential source of cellulases for pretreatment of crop residues during biogas production. PCR is considered a very powerful, sensitive, specific, fast, and reliable tool in molecular detection and diagnostics.

Published

2021

2. Battery-operated portable PCR system with enhanced stability of Pt RTD.

Author

Lim J, Jeong S, Kim M, and Lee JH

Subjects

Computer Simulation, DNA, Bacterial genetics, DNA, Bacterial isolation & purification, Electric Impedance, Electric Power Supplies, Electrophoresis, Equipment Design, Escherichia coli genetics, Humans, Platinum, Polymerase Chain Reaction statistics & numerical data, Temperature, Polymerase Chain Reaction instrumentation

Abstract

This paper reports an outdoor-use polymerase chain reaction (PCR) technology in which stability of resistance temperature detectors (RTDs) is remarkably improved. A thin-film RTD made of non-annealed Pt shows accuracy degradation because the resistance of the RTD tends to decrease during the PCR operation. Thus, the annealing process is applied to the Pt RTD to improve the stability, which is a prerequisite to the accurate measurement of the absolute temperature. Both heaters and the RTD are fabricated on a thin quartz substrate whose melting temperature is high enough for annealing. The performances in the PCR time and power consumption are enhanced by reducing the size of the heater chips with no degradation in the temperature uniformity. A spring-loaded electrode is employed to simplify the procedure of electrical connection to the thermal controller and loading/unloading of the PCR chip. The contact area of the electrical connection is so small that the conductive thermal resistance increases; thereby small heat dissipation can be exploited for low-power operation. The stability of the RTD is experimentally confirmed in terms of resistance variation over repeated PCR operations (four times). The least variation of 0.005%, which corresponds to a negligible temperature variation of 0.038 °C for the PCR, is achieved from the RTD annealed for 5 min at 450 °C. The gel-electrophoresis result indicates that the PCR performance of the proposed system using a film-type PCR chip is comparable to that of a conventional system using a vial tube despite its low power consumption., Competing Interests: The authors have declared that no competing interests exist.

Published

2019

3. [Allele-specific polymerase chain reaction and electrophoretic detection in the detection algorithm clinically significant somatic mutations in the gene of calreticulin (calr).]

Author

Gorbenko AS, Stolyar MA, Olkhovskiy IA, Abdullaev AO, Sudarikov AB, Dunaeva EA, Mironov KO, and Shipulin GA

Subjects

Algorithms, Alleles, DNA Mutational Analysis, Humans, Mutation, Myeloproliferative Disorders genetics, Calreticulin genetics, Electrophoresis, Myeloproliferative Disorders diagnosis, Polymerase Chain Reaction

Abstract

The detection of somatic mutations in the 9 exon of the calreticulin gene (CALR) is regulated by the clinical recommendations as a diagnostic criterion for chronic Ph-negative myeloproliferative neoplasms (MPN). Some methods of nucleic acids testing are used to identify CALR gene mutations with different requirements for special skills of personnel and expensive equipment. The purpose of this work is to compare the results of the detection of CALR gene mutations in venous blood samples by allele-specific RT-PCR with subsequent electrophoresis, fragment analysis and Sanger- or pyro- sequencing. We used 1284 blood samples of patients with suspected MPN and 20 blood donor samples. Mutations in the CALR gene of the I and II type were identified using PCR-RT with the original primers and TaqMan probes. Also, all samples were tested for mutations in the CALR gene by electrophoretic detection of PCR results in an agarose gel. The use of allele-specific RT-PCR followed by electrophoretic detection made it possible to determine clinically significant mutations in the CALR gene in 81 venous blood samples of JAK2- and MPL-negative patients, including 42 cases of type I mutation, 33 cases of type II mutation and 8 rare CALR mutations. Mutations in the 9 exon of the CALR gene were not detected in any of the 20 blood donor samples or in 121 blood samples of patients with polycythemia vera. In randomly selected 20 negative samples, CALR gene mutations were also not detected using Sanger sequencing. All positive samples were confirmed by fragment analysis, as well as with Sanger- sequencing and pyro- sequencing. The described combined approach to detect mutations of the CALR gene in peripheral blood samples can be used in clinical diagnostic laboratories that have a standard set of equipment for electrophoresis of nucleic acids and a PCR-RT. We also propose a confirmatory test based on the pyrosequencing of DNA using the system of genetic analysis "PyroMark Q24"., Competing Interests: The authors declare no conflict of interest.

Published

2018

4. Quantitative analysis of single-nucleotide polymorphisms by pyrosequencing with di-base addition.

Author

Pu D, Pan R, Liu W, and Xiao P

Subjects

Base Sequence, Electrophoresis, Gene Frequency, Genotype, Humans, Polymorphism, Single Nucleotide, Sensitivity and Specificity, Nucleotides analysis, Polymerase Chain Reaction methods, Sequence Analysis, DNA methods

Abstract

We have developed and validated a novel method for quantitative detection of SNPs by using pyrosequencing with di-base addition (PDBA). Based on the principle that the signal intensity is proportional to the template concentration within a linear concentration range, linear formula (Y = AX + B) for each genotype is established, and the relationship between two genotypes of a single SNP can be resolved by corresponding linear formulas. Here, PDBA assays were developed to detect variants rs6717546 and rs4148324, and the linear formulas for each genotype of rs6717546 and rs4148324 were established. The method allowed to quantitatively determine each genotype and showed 100% accordant results against a panel of defined mixtures. A set of 24 template fragments containing variants rs6717546 or rs4148324 was tested to evaluate the method. Our results showed that allele frequency of each genotype was accurately quantified, with results comparable to those of conventional pyrosequencing. Furthermore, this method was capable of detecting alleles with frequencies as low as 3%, which was more sensitive than ∼5 to ∼7% level detected by conventional pyrosequencing. This method offers high sensitivity, reproducibility, and relatively low costs, and thus could provide a much-needed approach for quantitative analysis of SNPs in clinical samples., (© 2016 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2017

5. [Letter to the Editor] Isolation of mitochondria is necessary for precise quantification of mitochondrial DNA damage in human carcinoma samples.

Author

Barchiesi A, Baccarani U, Billack B, Tell G, and Vascotto C

Subjects

Carcinoma, Hepatocellular pathology, Electrophoresis, Humans, Liver cytology, Liver Neoplasms pathology, Carcinoma, Hepatocellular genetics, DNA Damage genetics, DNA, Mitochondrial analysis, DNA, Mitochondrial genetics, DNA, Mitochondrial isolation & purification, Liver Neoplasms genetics, Mitochondria genetics, Mitochondria physiology, Polymerase Chain Reaction methods

Abstract

Address correspondence to Carlo Vascotto, Department of Medical and Biological Sciences, University of Udine, Udine, 33100, Italy. E-mail: carlo.vascotto@uniud.it.

Published

2017

6. Long-Term Rasamsonia argillacea Complex Species Colonization Revealed by PCR Amplification of Repetitive DNA Sequences in Cystic Fibrosis Patients.

Author

Mouhajir A, Matray O, Giraud S, Mély L, Marguet C, Sermet-Gaudelus I, Le Gal S, Labbé F, Person C, Troussier F, Ballet JJ, Gargala G, Zouhair R, Bougnoux ME, Bouchara JP, and Favennec L

Subjects

Cluster Analysis, Electrophoresis, Eurotiales genetics, Genotype, Humans, Microbiological Techniques methods, Molecular Epidemiology, Mycoses microbiology, Repetitive Sequences, Nucleic Acid genetics, Cystic Fibrosis complications, Eurotiales classification, Eurotiales isolation & purification, Mycoses diagnosis, Mycoses epidemiology, Polymerase Chain Reaction methods

Abstract

The aim of this work was to document molecular epidemiology of Rasamsonia argillacea species complex isolates from cystic fibrosis (CF) patients. In this work, 116 isolates belonging to this species complex and collected from 26 CF patients and one patient with chronic granulomatous disease were characterized using PCR amplification assays of repetitive DNA sequences and electrophoretic separation of amplicons (rep-PCR). Data revealed a clustering consistent with molecular species identification. A single species was recovered from most patients. Rasamsonia aegroticola was the most common species, followed by R. argillacea sensu stricto and R. piperina, while R. eburnea was not identified. Of 29 genotypes, 7 were shared by distinct patients while 22 were patient specific. In each clinical sample, most isolates exhibited an identical genotype. Genotyping of isolates recovered from sequential samples from the same patient confirmed the capability of R. aegroticola and R. argillacea isolates to chronically colonize the airways. A unique genotype was recovered from two siblings during a 6-month period. In the other cases, a largely dominant genotype was detected. Present results which support the use of rep-PCR for both identification and genotyping for the R. argillacea species complex provide the first molecular evidence of chronic airway colonization by these fungi in CF patients., (Copyright © 2016, American Society for Microbiology. All Rights Reserved.)

Published

2016

7. Validation of Expressmarker mtDNA-SNP60: A mitochondrial SNP kit for forensic application.

Author

Zhang C, Li H, Zhao X, Ma K, Nie Y, Liu W, Jiao H, and Zhou H

Subjects

Animals, DNA, Mitochondrial analysis, Electrophoresis, Escherichia coli, Female, Forensic Genetics standards, Humans, Male, Reproducibility of Results, Species Specificity, DNA, Mitochondrial genetics, Forensic Genetics methods, Polymerase Chain Reaction methods, Polymorphism, Single Nucleotide genetics

Abstract

Expressmarker mtDNA-SNP60 kit, a 3-dye fluorescence labeling forensic mitochondrial-SNP kit, was developed and modified based on previous work. In this study, it was validated through sensitivity, precision, accuracy, reproducibility, species specificity, mixture samples, PCR-based conditions, and inhibitor studies, according to the Scientific Working Group on DNA Analysis Methods guidelines. In the sensitivity study, full profile was obtained from template DNA with the quantity ≥ 4 pg. Consistent profiles were obtained at three different laboratories, which demonstrated the reproducibility of the kit. No peak was observed in the profiles of common animal species and microorganisms demonstrating high species specificity of the kit. In the mixture study, some loci (minor contributors) were missing at 19:1 and 9:1 ratios, whereas all loci could be profiled at other ratios (4:1, 2:1, and 1:1). PCR-based studies demonstrated that there recommended PCR conditions were optimized for the kit, and there was acceptable tolerance of error. The inhibitor study indicated that the kit has varying degrees of resistance to the presence of common inhibitors. Twelve random individuals were profiled by next-generation sequencing to confirm the allele-specific PCR assay, and a consistent result was obtained. Furthermore, 520 individuals from 260 families were profiled and the results showed that all loci of the confirmed mother and child were matched. In addition, forensic population genetics parameters, including random match probability, discrimination power, and haplotype diversity, were calculated (0.0474, 0.9526, and 0.9563, respectively). Our study demonstrates that the Expressmarker mtDNA-SNP60 kit can be a useful supplementary tool for forensic application., (© 2016 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2016

8. Rapid amplification of the RM-Yplex assay.

Author

Abuidrees AS, Alghafri RH, and Hadi S

Subjects

Electrophoresis, Female, Forensic Genetics methods, Humans, Male, Microsatellite Repeats genetics, Mutation genetics, Taq Polymerase, DNA Fingerprinting methods, Polymerase Chain Reaction methods

Abstract

A multiplex PCR assay consisting of 13 Rapidly Mutating Y STR loci called RM-Yplex was previously developed. Platinum ® Taq DNA polymerase was used to amplify the 13 Y STR loci in a single reaction at an amplification time of approximately 2.5 h. In order to shorten the process with reliable results, two DNA polymerases were tested with the multiplex. Phusion ® Flash High Fidelity, TAKARA Z-taq TM , and Platinum ® Taq DNA polymerases were investigated for conducting RM-Yplex assay at various PCR cycling conditions. Rapid, robust, and efficient amplification of all the markers within the multiplex were achieved. The amplification time was reduced from 2.5 h to less than 28 min with Phusion ® Flash High Fidelity DNA polymerase using Veriti ® PCR thermal cycler., (© 2016 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2016

9. Rapid Assays for Specific Detection of Fungi of Scopulariopsis and Microascus Genera and Scopulariopsis brevicaulis Species.

Author

Kordalewska M, Jagielski T, and Brillowska-Dąbrowska A

Subjects

DNA Primers genetics, Electrophoresis, Humans, Sensitivity and Specificity, Time Factors, Transition Temperature, Tubulin genetics, Ascomycota classification, Ascomycota isolation & purification, Dermatomycoses diagnosis, Dermatomycoses microbiology, Molecular Diagnostic Techniques methods, Polymerase Chain Reaction methods

Abstract

Purpose: Fungi of Scopulariopsis and Microascus genera cause a wide range of infections, with S. brevicaulis being the most prevalent aetiological agent of mould onychomycosis. Proper identification of these pathogens requires sporulating culture, which considerably delays the diagnosis. So far, sequencing of rDNA regions of clinical isolates has produced ambiguous results due to the lack of reference sequences in publicly available databases. Thus, there is a clear need for the development of new molecular methods that would provide simple, rapid and highly specific identification of Scopulariopsis and Microascus species. The objective of this study was to develop simple and fast assays based on PCR and real-time PCR for specific detection of fungi from Scopulariopsis and Microascus genera, and separately, S. brevicaulis species., Methods: On the basis of alignment of β-tubulin gene sequences, Microascus/Scopulariopsis-specific primers were designed and S. brevicaulis-specific primers were reevaluated. DNA from cultured fungal isolates, extracted in a two-step procedure, was used in Microascus/Scopulariopsis-specific and S. brevicaulis-specific PCR and real-time PCR followed by electrophoresis or melting temperature analysis, respectively., Results: The specificity of the assays was confirmed, as positive results were obtained only for Scopulariopsis spp. and Microascus spp. isolates tested in Microascus/Scopulariopsis-specific assay, and only for S. brevicaulis and S. koningii (syn. S. brevicaulis) isolates in a S. brevicaulis-specific assay, respectively, and no positive results were obtained neither for other moulds, dermatophytes, yeast-like fungi, nor for human DNA., Conclusions: The developed assays enable fast and unambiguous identification of Microascus spp. and Scopulariopsis spp. pathogens.

Published

2016

10. Validation of a robust PCR-based assay for quantifying fragile X CGG repeats.

Author

Kwok YK, Wong KM, Lo FM, Kong GWS, Moore JK, Wu S, Lam STS, Schermer M, Leung TY, and Choy KW

Subjects

Electrophoresis, Female, Humans, Male, Polymerase Chain Reaction economics, Polymerase Chain Reaction standards, Reference Standards, Fragile X Syndrome genetics, Polymerase Chain Reaction methods, Trinucleotide Repeats genetics

Abstract

Background: Sizing of FMR1 trinucleotide repeats in the clinical laboratory requires the use of capillary sequencer by PCR, or by a labor intensive measurement using Southern blot method. Our aim was to validate an accurate and robust PCR assay for quantification of CGG repeats., Methods: We performed an analytical and clinical validation of a new PCR-based method that utilizes a low-cost capillary electrophoresis instrument and the FragilEase™ reagent kit. First, analytical performance was demonstrated on 12 Coriell reference samples comprising normal through full mutations. Subsequently, a cohort of 112 archived clinical DNA samples, enriched for premutation and full mutations, was analyzed., Results: All samples were amplified successfully. Quantification of repeat numbers was interpreted by the use of standards with known repeats. Twenty-five full-mutation samples were successfully amplified with the largest allele size measured at 1380 repeats. The repeat numbers from the new assay were concordant with those obtained with the reference method. The intra-assay (CV<2.5%) and inter-assay imprecision was within 1 CGG repeat., Conclusion: This new PCR-based method is reproducible and capable of identifying all Fragile X alleles. It is an accurate and robust method that facilitates Fragile X testing in a broader spectrum of clinical laboratories., (Copyright © 2016 Elsevier B.V. All rights reserved.)

Published

2016

11. Advanced lymphoblastic clones detection in T-cell leukemia.

Author

Minervina AA, Komkov AY, Mamedov IZ, and Lebedev YB

Subjects

Bone Marrow metabolism, DNA Primers, Electrophoresis, Genetic Loci, Humans, Jurkat Cells, Leukemia, T-Cell metabolism, Neoplasm, Residual, Precursor T-Cell Lymphoblastic Leukemia-Lymphoma, V(D)J Recombination, Gene Rearrangement, beta-Chain T-Cell Antigen Receptor, Leukemia, T-Cell diagnosis, Leukemia, T-Cell genetics, Polymerase Chain Reaction methods

Abstract

T cell acute lymphoblastic leukemia (T-ALL) is an aggressive malignant neoplasm of the lymphocyte precursors that suffered malignant transformation arresting the lymphoid cell differentiation. Clinical studies revealed monoor, more rarely, oligoclonal nature of the disease. A precise identification of malignant clone markers is both the crucial stage of early diagnostics and the essential prognostic factor for therapeutic treatment. Here we present an improved system for unbiased detection of lymphoblastic clones in bone marrow aspirates of T-ALL patients. The system based on multiplex PCR of rearranged T-cell receptor locus (TRB) and straightforward sequencing of the resulted PCR fragments. Testing of the system on genomic DNA from Jurkat cell line and four clinical bone marrow aspirates revealed a set of unique TRB rearrangements that precisely characterize each of tested samples. Therefore, the outcome of the system produces highly informative molecular genetic markers for further monitoring of minimal residual disease in T-ALL patients.

Published

2016

12. PCR Detection of Scopulariopsis brevicaulis.

Author

Kordalewska M and Brillowska-Dąbrowska A

Subjects

Electrophoresis, DNA, Bacterial genetics, Polymerase Chain Reaction methods, Scopulariopsis genetics, Scopulariopsis isolation & purification, Soil Microbiology

Abstract

Scopulariopsis brevicaulis is known as the most common etiological factor of the mould toenail infections. There are also reports indicating that S. brevicaulis could cause organ and disseminated infections. Nowadays microscopic observations from the direct sample and culture are crucial for the appropriate recognition of the infection. In this paper a PCR-based method for S. brevicaulis detection is presented. The specificity of the reaction was confirmed, as positive results were obtained only for tested S. brevicaulis isolates and no positive results were obtained for other moulds, dermatophytes, yeast-like fungi, and human DNA.

Published

2015

13. Enhanced detection of DNA sequences using end-point PCR amplification and online gel electrophoresis (GE)-ICP-MS: determination of gene copy number variations.

Author

González TI, Espina M, Sierra LM, Bettmer J, Blanco-González E, Montes-Bayón M, and Sanz-Medel A

Subjects

Base Sequence, Cell Line, Electrophoresis, Humans, Mass Spectrometry, DNA genetics, DNA Copy Number Variations, Internet, Polymerase Chain Reaction instrumentation

Abstract

The design and evaluation of analytical methods that permit quantitative analysis of specific DNA sequences is exponentially increasing. For this purpose, highly sensitive methodologies usually based on labeling protocols with fluorescent dyes or nanoparticles are often explored. Here, the possibility of label-free signal amplification using end-point polymerase chain reaction (PCR) are exploited using on-column agarose gel electrophoresis as separation and inductively coupled plasma-mass spectrometry (ICP-MS) for the detection of phosphorus in amplified DNA sequences. The calibration of the separation system with a DNA ladder permits direct estimation of the size of the amplified gene fragment after PCR. With this knowledge, and considering the compound-independent quantification capabilities exhibited by ICP-MS for phosphorus (it is only dependent on the number of P atoms per molecule), the correlation of the P-peak area of the amplified gene fragment, with respect to the gene copy numbers (in the starting DNA), is then established. Such a relationship would permit the determination of copy number variations (CNVs) in genomic DNA using ICP-MS measurements. The method detection limit, in terms of the required amount of starting DNA, is ∼6 ng (or 1000 cells if 100% extraction efficiency is expected). The suitability of the proposed label-free amplification strategy is applied to CNVs monitoring in cells exposed to a chemical agent capable of deletion induction, such as cisplatin.

Published

2014

14. An integrated microfluidic device utilizing dielectrophoresis and multiplex array PCR for point-of-care detection of pathogens.

Author

Cai D, Xiao M, Xu P, Xu YC, and Du W

Subjects

Electrophoresis, Escherichia coli genetics, Humans, Pseudomonas aeruginosa genetics, Staphylococcus aureus genetics, Escherichia coli isolation & purification, Microfluidic Analytical Techniques, Point-of-Care Systems, Polymerase Chain Reaction, Pseudomonas aeruginosa isolation & purification, Staphylococcus aureus isolation & purification

Abstract

The early identification of causative pathogens in clinical specimens that require no cultivation is essential for directing evidence-based antimicrobial treatments in resource limited settings. Here, we describe an integrated microfluidic device for the rapid identification of pathogens in complex physiological matrices such as blood. The device was designed and fabricated using SlipChip technologies, which integrated four channels processing independent samples and identifying up to twenty different pathogens. Briefly, diluted whole human blood samples were directly injected into the device for analysis. The pathogens were extracted from the blood by dielectrophoresis, retained in an array of grooves, and identified by multiplex array PCR in nanoliter volumes with end-point fluorescence detection. The universality of the dielectrophoretic separation of pathogens from physiological fluids was evaluated with a panel of clinical isolates covering predominant bacterial and fungal species. Using this system, we simultaneously identified Pseudomonas aeruginosa, Staphylococcus aureus and Escherichia coli O157:H7 within 3 h. In addition to the prompt diagnosis of bloodstream infections, this method may also be utilized for differentiating microorganisms in contaminated water and environmental samples.

Published

2014

15. Synteny analysis provides a route to design genus-specific PCR primers for rapid identification of all Saccharomyces species.

Author

Sharpe B, Hulin M, Thorne-Wallis J, and Wheals A

Subjects

Base Composition, DNA, Fungal chemistry, Electrophoresis, Fungal Proteins genetics, HSP30 Heat-Shock Proteins genetics, Molecular Sequence Data, Sequence Analysis, DNA, Temperature, Time Factors, DNA Primers genetics, DNA, Fungal genetics, Mycology methods, Polymerase Chain Reaction methods, Saccharomyces classification, Saccharomyces genetics, Synteny

Abstract

The genus Saccharomyces comprises seven single-genome species (S. arboricola, S. cerevisiae, S. eubayanus, S. kudriavzevii, S. mikatae, S. paradoxus and S. uvarum) and two hybrid species - S. pastorianus (S. cerevisiae plus S. eubayanus) and S. bayanus (mostly S. uvarum plus S. eubayanus). Species-specific primers have already been developed for the identification of each of the single-genome species, and these primers can usually detect both genomes in hybrids. It would be advantageous if a single reaction could detect any member of the clade. We have investigated three potentially generic approaches to design genus-specific primers. Two methods that both use sequence alignment differences for primer design were only partly successful. A third method used synteny data to identify 136 target genes that are potentially present only in all species of the Saccharomyces clade. HSP30 (YCR021C) was fully successful; different primer pairs were developed with high G+C content for use at 63 °C. In < 3 h, using a robust colony-PCR followed by gel electrophoresis, the method can reliably detect any member of the genus. This novel approach still uses conventional sequence alignment mismatches but relies principally on the presence of the target gene only within the genus Saccharomyces., (© 2013 Federation of European Microbiological Societies. Published by John Wiley & Sons Ltd. All rights reserved.)

Published

2014

16. Introducing basic molecular biology to Turkish rural and urban primary school children via hands-on PCR and gel electrophoresis activities.

Author

Selli C, Yıldırım G, Kaymak A, Karacicek B, Ogut D, Gungor T, Erem E, Ege M, Bümen N, and Tosun M

Subjects

Electrophoresis, Female, Humans, Male, Rural Population, Science, Turkey, Universities, Molecular Biology education, Polymerase Chain Reaction methods, Schools

Abstract

This study includes the results of a 2-day education project titled "Molecular Biology Laboratory Summer School, MoBiLYO." The project was held at a University Research Center by scientists from Department of Pharmacology and graduate students. The project was composed of introductory lectures, model construction, DNA isolation, polymerase chain reaction (PCR), and gel electrophoresis. The participants were 13-year-old eighth-graders attending primary schools affiliated with Ministry of National Education in urban and rural areas of Izmir, Turkey. The purpose of this study was to introduce basic molecular biology concepts through individually performed experiments such as PCR and gel electrophoresis integrated with creative drama. The students were assessed at the beginning and the end of each project day via mini-tests, experimental and presentation skills evaluation forms. Data showed that students' knowledge about DNA structure and basic molecular biology techniques significantly increased. On the basis of experimental and presentational skills, there was no significant difference between kids from urban and rural schools or between public and boarding public schools, whereas the average score of girls was significantly higher than that of boys. In conclusion, individually performed experiments integrated with creative drama significantly increased students' perception of complex experimental procedures on basic molecular biology concepts. Data suggests that integration of these concepts into the science and technology curriculum of Turkish primary education may support the recruitment of future scientists who can handle rapidly developing genomic techniques that will affect our everyday life., (© 2014 by The International Union of Biochemistry and Molecular Biology.)

Published

2014

17. The effect of plant identity and the level of plant decay on molecular gut content analysis in a herbivorous soil insect.

Author

Wallinger C, Staudacher K, Schallhart N, Peter E, Dresch P, Juen A, and Traugott M

Subjects

Animals, DNA Primers genetics, DNA, Chloroplast genetics, Electrophoresis, Germany, Larva physiology, Regression Analysis, Species Specificity, Coleoptera physiology, Gastrointestinal Contents chemistry, Herbivory physiology, Plant Roots genetics, Plant Roots metabolism, Polymerase Chain Reaction methods

Abstract

Plant roots represent an important food source for soil-dwelling animals, but tracking herbivore food choices below-ground is difficult. Here, we present an optimized PCR assay for the detection of plant DNA in the guts of invertebrates, using general plant primers targeting the trnT-F chloroplast DNA region. Based on this assay, we assessed the influence of plant identity on the detectability of ingested plant DNA in Agriotes click beetle larvae. Six different plant species were fed to the insects, comprising a grass, a legume and four nonlegume forbs. Moreover, we examined whether it is possible to amplify DNA of decaying plants and if DNA of decayed plant food is detectable in the guts of the larvae. DNA of the ingested roots could be detected in the guts of the larvae for up to 72-h post-feeding, the maximum digestion time tested. When fed with living plants, DNA detection rates differed significantly between the plant species. This may be ascribed to differences in the amount of plant tissue consumed, root palatability, root morphology and/or secondary plant components. These findings indicate that plant identity can affect post-feeding DNA detection success, which needs to be considered for the interpretation of molecularly derived feeding rates on plants. Amplification of plant DNA from decaying plants was possible as long as any tissue could be retrieved from the soil. The consumption of decaying plant tissue could also be verified by our assay, but the insects seemed to prefer fresh roots over decaying plant material., (© 2012 Blackwell Publishing Ltd.)

Published

2013

18. Mixed donor chimerism in non-malignant haematological diseases after allogeneic bone marrow transplantation.

Author

Shamshad GU, Ahmed S, Bhatti FA, and Ali N

Subjects

Adolescent, Adult, Anemia, Aplastic genetics, Bone Marrow Transplantation adverse effects, Child, Child, Preschool, Chromosome Mapping, Electrophoresis, Female, Gene Amplification, Genetic Markers, Humans, Male, Microsatellite Repeats, Middle Aged, Taq Polymerase, Tissue Donors, Transplantation, Homologous, Young Adult, beta-Thalassemia genetics, Anemia, Aplastic surgery, Bone Marrow Transplantation methods, Chimerism, DNA analysis, Polymerase Chain Reaction methods, beta-Thalassemia surgery

Abstract

Objective: To determine the frequency of mixed donor chimerism in patients of non-malignant haematological diseases after allogeneic bone marrow transplant., Study Design: A cross-sectional, observational study., Place and Duration of Study: Department of Haematology, Armed Forces Institute of Pathology (AFIP), Rawalpindi, from July 2010 to June 2011., Methodology: Donor chimerism was assessed in patients of aplastic anaemia and beta-thalassaemia major who underwent allogeneic bone marrow transplantation (BMT). Peripheral blood samples were used to assess chimerism status by analysis of short tandem repeats (STR). In patients where pre-transplant blood sample was not available, swab of buccal mucosa was used for pre-transplant STR profile. A standard set of primers for STR markers were used and the amplified DNA was resolved by gel electrophoresis and stained with silver nitrate. The percentage of donor origin DNA was estimated by densitometer., Results: Out of 84 patients, 52 (62%) were males, while 32 (38%) were females. In patients of beta-thalassaemia major, 31 (62%) developed mixed donor chimerism (MC), 13 (26%) developed complete donor chimerism (CC) and 6 (12%) had graft failure. In aplastic anaemia, 17 patients (50%) achieved MC, 13 (38.2%) had CC and 4 (11.8%) developed graft failure. The combined frequency of mixed donor chimerism for both the diseases was 58.3%. D3S1358 was the most informative STR marker in these patients., Conclusion: Majority of the studied patients developed mixed donor chimerism following bone marrow transplantation, whereas only a minor percentage of the patients had graft failure. Analysis of D3S1358 was the most informative in assessing donor chimerism in patients who underwent BMT.

Published

2012

19. [Study on optimization of SRAP-PCR reaction system for Pinellia ternata in Suzhou].

Author

Zhang AM, Lu HD, Xue JP, Tao XK, Xue T, Sheng W, and Zhu YF

Subjects

China, DNA Primers genetics, Electrophoresis, Magnesium metabolism, Nucleotides genetics, Reproducibility of Results, Taq Polymerase metabolism, Templates, Genetic, DNA, Plant genetics, Nucleic Acid Amplification Techniques methods, Pinellia genetics, Polymerase Chain Reaction methods

Abstract

Objective: To investigate the optimization system of SRAP-PCR molecular marker technology in the analysis on Pinellia ternata., Method: SRAP-PCR reaction system for P. ternata was optimized by L16 (5(4)) orthogonal design with five elements (dNTPs, Mg2+, the template DNA, primers, Taq enzyme) and four standards., Result: The most suitable forward primer for SRAP for Pinellia ternata was 5'-TGAGTCCAAACCGGAAG-3', while the reverse primer was 5'-GACTGCGTACGAATTACG-3'. The optimized reaction system contained 70 ng DNA template, 0.9 micromol x L(-1) primer, 0.20 mmol x L(-1) dNTP s, 1.5 - 2.0 mmol x L(-1) Mg2+, and 2 U Taq enzyme., Conclusion: SRAP-PCR system for P. ternata is established to lay a foundation for future construction of SRAP genetic map of P. ternata.

Published

2012

20. Identification and secondary structure analysis of a region affecting electrophoretic mobility of the STR locus SE33.

Author

Wang DY, Green RL, Lagacé RE, Oldroyd NJ, Hennessy LK, and Mulero JJ

Subjects

Alleles, Black People genetics, DNA Fingerprinting, Female, Genotype, Humans, Inverted Repeat Sequences, Male, Mutagenesis, Site-Directed, Polymerase Chain Reaction instrumentation, Polymorphism, Single Nucleotide, Sequence Analysis, DNA, Thermodynamics, White People genetics, DNA Primers, Electrophoresis, Microsatellite Repeats, Polymerase Chain Reaction methods

Abstract

SE33 is one of the most informative markers in forensic use due to its high power of discrimination. During the course of developing the AmpFℓSTR(®) NGM SElect™ PCR Amplification Kit several SE33 primer designs were screened with one primer pair yielding a high frequency of discordant alleles when compared to the AmpFℓSTR(®) SEfiler Plus™ PCR Amplification Kit. This discordance was mostly specific to samples of African descent with an estimated frequency of 5.1% and was a result of a mobility shift of approximately +0.84nt. The sequence analysis of the affected alleles revealed that the only difference from the wild type sequence was a single nucleotide polymorphism (SNP) outside of the SE33 repeat but within the amplicon of this particular set of experimental primers. In total, we identified three different SNPs all within 9nt of each other, each of which could cause the mobility shift individually. Further characterization of this region via site directed mutagenesis and thermostability measurements strongly suggests that this polymorphic region contains a secondary structure that, when disrupted due to the presence of a variant SNP, results in a mobility shift relative to the wild type sequence. To overcome this problem, the SE33 primers used in the final configuration of the NGM SElect™ Kit avoided the amplification of this polymorphic region yielding in turn results highly concordant with the SEfiler Plus™ Kit., (Copyright © 2011 Elsevier Ireland Ltd. All rights reserved.)

Published

2012

21. Developmental validation of the AmpFℓSTR® Identifiler® Plus PCR Amplification Kit: an established multiplex assay with improved performance.

Author

Wang DY, Chang CW, Lagacé RE, Calandro LM, and Hennessy LK

Subjects

Animals, DNA Degradation, Necrotic, DNA Primers, Electrophoresis, Gene Frequency, Genetics, Population, Genotype, Humans, Microsatellite Repeats, Primates genetics, Racial Groups, Species Specificity, DNA Fingerprinting instrumentation, Polymerase Chain Reaction instrumentation

Abstract

Analysis of length polymorphism at short tandem repeat (STR) loci utilizing multiplex polymerase chain reaction (PCR) remains the primary method for genotyping forensic samples. The AmpFℓSTR(®) Identifiler(®) Plus PCR Amplification Kit is an improved version of the AmpFℓSTR(®) Identifiler(®) PCR Amplification Kit and amplifies the core CODIS loci: D3S1358, D5S818, D7S820, D8S1179, D13S317, D16S539, D18S51, D21S11, CSF1PO, FGA, TH01, TPOX, and vWA. Additional loci amplified in the multiplex reaction are the sex-determinant, amelogenin, and two internationally accepted loci, D2S1338 and D19S433. While the primer sequences and dye configurations were unchanged, the AmpFℓSTR(®) Identifiler(®) Plus PCR Amplification Kit features an enhanced buffer formulation and an optimized PCR cycling protocol that increases sensitivity, provides better tolerance to PCR inhibitors, and improves performance on mixture samples. The AmpFℓSTR(®) Identifiler(®) Plus PCR Amplification Kit has been validated according to the FBI/National Standards and Scientific Working Group on DNA Analysis Methods (SWGDAM) guidelines. The validation results support the use of the AmpFℓSTR(®) Identifiler(®) Plus PCR Amplification Kit for human identity and parentage testing., (© 2011 American Academy of Forensic Sciences.)

Published

2012

22. Highly parallel and short-acting amplification with locus-specific primers to detect single nucleotide polymorphisms by the DigiTag2 assay.

Author

Nishida N, Mawatari Y, Sageshima M, and Tokunaga K

Subjects

DNA-Directed DNA Polymerase metabolism, Electrophoresis, Genotype, Genotyping Techniques, Humans, Reproducibility of Results, Biological Assay methods, DNA Primers metabolism, Genetic Loci genetics, Polymerase Chain Reaction methods, Polymorphism, Single Nucleotide genetics

Abstract

The DigiTag2 assay enables analysis of a set of 96 SNPs using Kapa 2GFast HotStart DNA polymerase with a new protocol that has a total running time of about 7 hours, which is 6 hours shorter than the previous protocol. Quality parameters (conversion rate, call rate, reproducibility and concordance) were at the same levels as when genotype calls were acquired using the previous protocol. Multiplex PCR with 192 pairs of locus-specific primers was available for target preparation in the DigiTag2 assay without the optimization of reaction conditions, and quality parameters had the same levels as those acquired with 96-plex PCR. The locus-specific primers were able to achieve sufficient (concentration of target amplicon ≥5 nM) and specific (concentration of unexpected amplicons <2 nM) amplification within 2 hours, were also able to achieve detectable amplifications even when working in a 96-plex or 192-plex form. The improved DigiTag2 assay will be an efficient platform for screening an intermediate number of SNPs (tens to hundreds of sites) in the replication analysis after genome-wide association study. Moreover, highly parallel and short-acting amplification with locus-specific primers may thus facilitate widespread application to other PCR-based assays.

Published

2012

23. A primer design strategy for PCR amplification of GC-rich DNA sequences.

Author

Li LY, Li Q, Yu YH, Zhong M, Yang L, Wu QH, Qiu YR, and Luo SQ

Subjects

Electrophoresis, Exons genetics, DNA Primers genetics, GC Rich Sequence genetics, Polymerase Chain Reaction methods

Abstract

Objectives: To establish a primer design method for amplification of GC-rich DNA sequences., Design and Methods: A group of 15 pairs of primers with higher T(m) (>79.7°C) and lower level ΔT(m) (<1°C) were designed to amplify GC-rich sequences (66.0%-84.0%). The statistical analysis of primer parameters and GC content of PCR products was performed and compared with literatures. Other control experiments were conducted using shortened primers for GC-rich PCR amplifications in this study, and the statistical analysis of shortened primer parameters and GC content of PCR products was performed compared with primers not shortened. A group of 26 pairs of primers were designed to test the applicability of this primer designing strategy in amplifications of non-GC-rich sequences (35.2%-53.5%)., Results: All the DNA sequences in this study were successfully amplified. Statistical analyses show that the T(m) and ΔT(m) were the main factors influencing amplifications., Conclusions: This primer designing strategy offered a perfect tool for amplification of GC-rich sequences. It proves that the secondary structures cannot be formed at higher annealing temperature conditions (>65°C), and we can overcome this difficulty easily by designing primers and using higher annealing temperature., (Crown Copyright © 2011. Published by Elsevier Inc. All rights reserved.)

Published

2011

24. Molecular detection of vertebrates in stream water: a demonstration using Rocky Mountain tailed frogs and Idaho giant salamanders.

Author

Goldberg CS, Pilliod DS, Arkle RS, and Waits LP

Subjects

Animals, Electrophoresis, Idaho, Species Specificity, Water, Anura genetics, Aquatic Organisms genetics, DNA isolation & purification, Ecosystem, Polymerase Chain Reaction methods, Rivers, Urodela genetics

Abstract

Stream ecosystems harbor many secretive and imperiled species, and studies of vertebrates in these systems face the challenges of relatively low detection rates and high costs. Environmental DNA (eDNA) has recently been confirmed as a sensitive and efficient tool for documenting aquatic vertebrates in wetlands and in a large river and canal system. However, it was unclear whether this tool could be used to detect low-density vertebrates in fast-moving streams where shed cells may travel rapidly away from their source. To evaluate the potential utility of eDNA techniques in stream systems, we designed targeted primers to amplify a short, species-specific DNA fragment for two secretive stream amphibian species in the northwestern region of the United States (Rocky Mountain tailed frogs, Ascaphus montanus, and Idaho giant salamanders, Dicamptodon aterrimus). We tested three DNA extraction and five PCR protocols to determine whether we could detect eDNA of these species in filtered water samples from five streams with varying densities of these species in central Idaho, USA. We successfully amplified and sequenced the targeted DNA regions for both species from stream water filter samples. We detected Idaho giant salamanders in all samples and Rocky Mountain tailed frogs in four of five streams and found some indication that these species are more difficult to detect using eDNA in early spring than in early fall. While the sensitivity of this method across taxa remains to be determined, the use of eDNA could revolutionize surveys for rare and invasive stream species. With this study, the utility of eDNA techniques for detecting aquatic vertebrates has been demonstrated across the majority of freshwater systems, setting the stage for an innovative transformation in approaches for aquatic research.

Published

2011

25. Modification of a commercially available kit for the improvement of PCR efficiency.

Author

Hua Zhang A, Bum Seo S, Yi JA, Yeon Kim H, and Deok Lee S

Subjects

Electrophoresis, Forensic Sciences methods, Forensic Sciences trends, Gene Amplification, Humans, Korea, Pilot Projects, Polymerase Chain Reaction economics, Reproducibility of Results, DNA analysis, Microsatellite Repeats genetics, Polymerase Chain Reaction instrumentation, Polymorphism, Genetic, Reagent Kits, Diagnostic standards

Abstract

The polymorphism of short tandem repeats (STRs) is commonly used for human identity testing. Many commercial kits are available for this purpose, in which multiplex PCR for 10-16 STRs is usually used. For optimal results, the kits recommend rather limited conditions, which not all forensic samples can satisfy. We increased the efficiency of several commercial kits by modifying the components and reaction parameters (primer concentration and cycle number, and annealing and extension time). To simulate low copy number, we used 1:10 and 1:100 diluted samples compared to the recommended concentration. A change in cycle number, annealing and extension time, and primer concentration showed various results. Fine-tuning of PCR conditions by combining the described changes, decreasing the primer concentration, and increasing the annealing and extension time together with increasing the cycling number dramatically increased the efficiency of the reaction, even in low-copy-number simulated samples. Detailed information for several kit components or kits with different components targeting difficult sample conditions, including low copy number, would be of great help in forensics.

Published

2010

26. Generation of DNA profiles from fabrics without DNA extraction.

Author

Linacre A, Pekarek V, Swaran YC, and Tobe SS

Subjects

Clothing, Cotton Fiber, DNA isolation & purification, DNA Fingerprinting economics, Drug Stability, Electrophoresis, Forensic Medicine methods, Gene Amplification, Humans, Nylons, Polyesters, DNA genetics, DNA Fingerprinting methods, Polymerase Chain Reaction methods, Textiles analysis

Abstract

DNA profiles can be obtained from fabrics where a person has made direct contact with clothing. A standard approach is to cut out a section of the fabric and then use a commercially available method to extract and isolate the DNA. Alternative methods to isolate DNA include the use of adhesive tape to remove traces of cellular material from the fabric prior to extraction. We report on a process to obtain full DNA profiles using direct amplification from a range of fabrics. The absence of an extraction step both reduces the opportunity for contamination and reduces the loss of DNA during the extraction process, increasing the sensitivity of the process of generating a DNA profile. The process does not require the use of commercially available extraction kits thus reducing the cost of generating a DNA profile from trace amounts of starting material. The results are in part dependent upon the nature of the fabric used to which the DNA has been transferred.

Published

2010

27. Identification of cystic fibrosis variants by polymerase chain reaction/oligonucleotide ligation assay.

Author

Schwartz KM, Pike-Buchanan LL, Muralidharan K, Redman JB, Wilson JA, Jarvis M, Cura MG, and Pratt VM

Subjects

Electrophoresis, Gene Frequency, Humans, Cystic Fibrosis diagnosis, Cystic Fibrosis genetics, Mutation genetics, Polymerase Chain Reaction methods

Abstract

The purpose of this work is to define rare variants of cystic fibrosis (CF) that are potential sources of error and can confound molecular genetic testing methods. We performed routine, clinical CF mutation screening using a laboratory-developed test and the oligonucleotide ligation assay reagents from Abbott/Celera. In this report, we describe 11 unique allele drop outs [3849 + 10kb C>T (NM&#95;000492.2:c.3718-2477C>T), V520F (c.1558G>T), 1078delT (c.948delT), A455E (c.1364C>A), R347P (c.1040G>C), 2184delA (c.2052delA), W1282X (c.3846G>A), R117H (c.350G>A), G85E (c.254G>A), 621 + 1G>T (c.489 + 1G>T), and 2789 + 5G>A (c.2657 + 5G>A)] observed with this platform. The allele drop outs account for less than 0.01% of all results reported in our laboratory. Both the recognition and enumeration of such variants along with clinical information in CF testing is valuable in avoiding false-positive and false-negative results.

Published

2009

28. A vector for purification-free cloning of polymerase chain reaction products.

Author

Park HK and Zeng C

Subjects

Base Sequence, Electrophoresis, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, Molecular Sequence Data, Time Factors, Cloning, Molecular methods, Genetic Vectors genetics, Polymerase Chain Reaction methods

Abstract

Conventional cloning requires the purification of restriction-enzyme-digested vectors prior to the ligation reaction. The purification often involves the separation of restriction fragments via electrophoresis, the cutting out of a piece of gel, and the gel extraction of the linearized vector. In addition to the loss of significant amounts of DNA, reduced cloning efficiency, time, and cost, these steps are also mutagenic to DNA and hazardous to humans. We developed a purification-free cloning vector pGT3 with a bright green fluorescent protein indicator that is suitable for TA cloning of polymerase chain reaction (PCR) products. PCR products were cloned into pGT3 efficiently without the gel purification steps.

Published

2008

29. Direct PCR of intact bacteria (colony PCR).

Author

Woodman ME

Subjects

Electrophoresis, Bacteria genetics, Colony Count, Microbial methods, Polymerase Chain Reaction methods

Abstract

This protocol describes an efficient method for screening intact bacteria for the presence of desired DNA sequences using polymerase chain reaction (PCR). This method is commonly referred to as colony PCR.

Published

2008

30. Effect of nitrate injection on the bacterial community in a water-oil tank system analyzed by PCR-DGGE.

Author

Jurelevicius D, von der Weid I, Korenblum E, Valoni E, Penna M, and Seldin L

Subjects

Brazil, DNA, Bacterial genetics, DNA, Ribosomal genetics, Oxidoreductases Acting on Sulfur Group Donors genetics, RNA, Ribosomal, 16S genetics, Sulfides metabolism, Sulfur-Reducing Bacteria genetics, Sulfur-Reducing Bacteria isolation & purification, Electrophoresis, Fuel Oils microbiology, Nitrates pharmacology, Polymerase Chain Reaction, Sulfur-Reducing Bacteria classification, Sulfur-Reducing Bacteria metabolism

Abstract

Sulfide production by sulfate-reducing bacteria (SRB) is a major concern for the petroleum industry since it is toxic and corrosive, and causes plugging due to the formation of insoluble iron sulfides (reservoir souring). In this study, PCR followed by denaturing gradient gel electrophoresis (PCR-DGGE) using two sets of primers based on the 16S rRNA gene and on the aps gene (adenosine-5-phosphosulfate reductase) was used to track changes in the total bacterial and SRB communities, respectively, present in the water-oil tank system on an offshore platform in Brazil in which nitrate treatment was applied for 2 months (15 nitrate injections). PCR-DGGE analysis of the total bacterial community showed the existence of a dominant population in the water-oil tank, and that the appearance and/or the increase of intensity of some bands in the gels were not permanently affected by the introduction of nitrate. On the other hand, the SRB community was stimulated following nitrate treatment. Moreover, sulfide production did not exceed the permissible exposure limit in the water-oil separation tank studied treated with nitrate. Therefore, controlling sulfide production by treating the produced water tank with nitrate could reduce the quantity of chemical biocides required to control microbial activities.

Published

2008

31. Prevalence of Porphyromonas gingivalis and Bacteroides forsythus in chronic periodontitis by multiplex PCR.

Author

Faghri J, Moghim Sh, Abed AM, Rezaei F, and Chalabi M

Subjects

Adult, Aged, Bacteroides metabolism, Case-Control Studies, DNA, Bacterial analysis, Electrophoresis, Female, Humans, Male, Middle Aged, Models, Genetic, Porphyromonas gingivalis metabolism, Prevalence, Bacteroides genetics, Periodontitis epidemiology, Periodontitis microbiology, Polymerase Chain Reaction methods, Porphyromonas gingivalis genetics

Abstract

The present research decided to study prevalence of Porphyromonas gingivalis and Bacteroides forsythus in chronic periodontitis patient by use of Multiplex PCR. The subgingival plaque samples from 61 patients suffering from chronic periodontitis with probing depth PD > or = 6 and 40 healthy controls were collected by sterile curette. In this study we used two species-specific Forward primers in combination with a single Reverse primer. These primers target variable and conserved region of 16S rRNA gene, respectively. The study included 61 patients (34 women, 27 men; 24-69 years of age; mean 43) and 40 periodontally healthy controls (22 Women, 18 men, 21-69 years in age; mean 41.35%). Porphyromonas gingivalis was detected in 51 samples (83.61%) and 16 samples (40%) of chronic periodontitis patients and healthy subjects, respectively and Bacteroides forsythus was detected in 32 samples (52.50%) of chronic periodontitis patients and was not detected in any sample from healthy persons. We set up Multiplex PCR in order to detect P. gingivalis and B. forsythus simultaneously. The present data suggest that P. gingivalis is a more important cofactor in etiology of chronic periodontitis. Further studies are needed to determine spectrum of pathogenicity of the disease and effective management of diagnosis and treatment in order to decrease the risk of periodontic complicates such as systemic infection.

Published

2007

32. [Rapid DNA extraction from archival paraffin-embedded tissue: a modified method available to PCR analysis for diagnostic pathology].

Author

Jiang W, Liu WP, Li L, and Li GD

Subjects

Electrophoresis, Feasibility Studies, Humans, Lymphoma diagnosis, Lymphoma genetics, Lymphoma pathology, Recombination, Genetic, Specimen Handling, Time Factors, DNA genetics, DNA isolation & purification, Diagnosis, Paraffin Embedding methods, Polymerase Chain Reaction

Abstract

Objective: To modify a method for rapid DNA extraction from paraffin-embedded tissue and to evaluate its efficiency and feasibility available to the PCR analysis for the diagnostic pathology., Methods: Rapid DNA extraction by simply boiling was performed on 52 archival paraffin-embedded tissues including lymphoma and reactive hyperplasia. The traditional phenol-chloroform and DNeasy mini kit methods were also used as controls. The DNA quality was confirmed by PCR amplification of housekeeping gene beta-Globin. The accuracy of target fragment was reconfirmed by sequencing analysis. Based on the clinical pathologic diagnosis to diseases, the IgH and TCRY gene were selected for their gene rearrangements detected., Results: The amplification efficiency of beta-Globin and the detective rate of IgH and TCRY gene rearrangements showed no statistic significance between rapid method and the controls, although an obvious lower DNA concentration extracted by rapid method was showed by spectrophotometer. The sequencing result of PCR product was thoroughly consistent with the DNA sequence of corresponding target gene. The DNA in extract could be stored at -20 degrees C for at least 4 weeks., Conclusion: The rapid method of DNA extracted from archival paraffin-embedded tissue can provide enough DNA served as PCR template, and be regarded as a reliable, stable and economical method with prospect in being used to PCR analysis for the diagnostic pathology.

Published

2007

33. [Determination of Herpes simplex virus DNA with the use of solid-phase methods for the detection of PCR products].

Author

Rar VA, Terekhova DA, Pyshnyĭ DV, Pyshnaia IA, and Morozova OV

Subjects

Biotinylation, Cells, Cultured, Digoxigenin, Electrophoresis, Herpes Simplex virology, Herpesvirus 1, Human genetics, Herpesvirus 2, Human genetics, Humans, Molecular Diagnostic Techniques, Sensitivity and Specificity, DNA, Viral genetics, Herpes Simplex diagnosis, Herpesvirus 1, Human isolation & purification, Herpesvirus 2, Human isolation & purification, Polymerase Chain Reaction methods

Abstract

To determine DNA of herpes simplex virus (HSV), types 1 and 2, the polymerase chain reaction (PCR) method was developed with the subsequent detection of amplification products by means of electrophoresis or the molecular hybridization of nucleic acids (MHNA). Two variants of MHNA have been compared: hybridization in the solution of a biotinylated probe with digoxigenin-labeled PCR with the subsequent sorption of hybridization complexes onto streptavidin-covered plates and solid-phase hybridization of digoxigenin-labeled PCR with a biotinylated probe. Effective hybridization was observed after the denaturation of targets at 95 degrees C in the solution of 50 mM NaOH, but not in neutral solutions. To increase the level of sensitivity of hybridization in solution, the exact selection of the amount of the probe was shown to be necessary, for both its excess and deficiency essentially decreased the method sensitivity. A decrease in the ionic power of hybridization solutions from 6 h SSC to 1 h SSC led to greater specificity of hybridization without a decrease in the method sensitivity. A rise in the temperature of hybridization and subsequent washing to 45 degrees C decreased the sensitivity of the method. The limit of the sensitivity PCR with electrophoretic detection was 30 HSV genome equivalents, and 10 genome equivalents in the presence MHNA in the solution and on the solid phase.

Published

2006

34. Species identification of Crassostrea and Ostrea oysters by polymerase chain reaction amplification of the 5S rRNA gene.

Author

Cross I, Rebordinos L, and Diaz E

Subjects

Animals, Base Sequence, Cloning, Molecular, DNA metabolism, DNA Primers chemistry, DNA, Ribosomal Spacer, Electrophoresis, Electrophoresis, Agar Gel methods, Molecular Sequence Data, Ostreidae, Sequence Homology, Amino Acid, Species Specificity, Chemistry Techniques, Analytical methods, Crassostrea genetics, Ostrea genetics, Polymerase Chain Reaction methods, RNA, Ribosomal, 5S genetics

Abstract

A specific multiplex polymerase chain reaction (PCR) was developed for the identification of Crassostrea angulata, C. gigas, Ostrea edulis, and O. stentina oyster species. Universal primers were used for the amplification of complete repetition units of 5S rDNA in each of the 4 species. The alignment of the obtained sequences was the basis for the specific design of species-specific primers (ED1, ED2, ST1, ST2, CR1, and CR2) located in the nontranscribed spacer regions. The different sizes of the species-specific amplicons, separated by agarose gel electrophoresis, allowed identification of Crassostrea and Ostrea species. A multiplex PCR with a set of the 6 designed primers showed that they did not interfere with each other and bound specifically to the DNA target. This genetic marker can be very useful for traceability of the species, application in the management of oyster cultures, and conservation of the genetic resources of the species.

Published

2006

35. Micromachined polymerase chain reaction system for multiple DNA amplification of upper respiratory tract infectious diseases.

Author

Liao CS, Lee GB, Wu JJ, Chang CC, Hsieh TM, Huang FC, and Luo CH

Subjects

Hot Temperature, Time Factors, Electrophoresis, Polymerase Chain Reaction, Respiratory Tract Infections metabolism

Abstract

This paper presents a micro polymerase chain reaction (PCR) chip for the DNA-based diagnosis of microorganism genes and the detection of their corresponding antibiotic-resistant genes. The micro PCR chip comprises cheap biocompatible soda-lime glass substrates with integrated thin-film platinum resistors as heating/sensing elements, and is fabricated using micro-electro-mechanical-system (MEMS) techniques in a reliable batch-fabrication process. The heating and temperature sensing elements are made of the same material and are located inside the reaction chamber in order to ensure a uniform temperature distribution. This study performs the detection of several genes associated with upper respiratory tract infection microorganisms, i.e. Streptococcus pneumoniae, Haemopilus influenze, Staphylococcu aureus, Streptococcus pyogenes, and Neisseria meningitides, together with their corresponding antibiotic-resistant genes. The lower thermal inertia of the proposed micro PCR chip relative to conventional bench-top PCR systems enables a more rapid detection operation with reduced sample and reagent consumption. The experimental data reveal that the high heating and cooling rates of the system (20 and 10 degrees C/s, respectively) permit successful DNA amplification within 15 min. The micro PCR chip is also capable of performing multiple DNA amplification, i.e. the simultaneous duplication of multiple genes under different conditions in separate reaction wells. Compared with the large-scale PCR system, it is greatly advantageous for fast diagnosis of multiple infectious diseases. Multiplex PCR amplification of two DNA segments in the same well is also feasible using the proposed micro device. The developed micro PCR chip provides a crucial tool for genetic analysis, molecular biology, infectious disease detection, and many other biomedical applications.

Published

2005

36. Introduction of the QF-PCR analysis for the purposes of prenatal diagnosis in Bulgaria--estimation of applicability of 6 STR markers on chromosomes 21 and 18.

Author

Andonova S, Vazharova R, Dimitrova V, Mazneikova V, Toncheva D, and Kremensky I

Subjects

Bulgaria, Chromosome Disorders genetics, Electrophoresis, Female, Fluorescence, Genetic Markers, Gestational Age, Humans, Pregnancy, Trisomy diagnosis, Aneuploidy, Chromosome Disorders diagnosis, Chromosomes, Human, Pair 18, Chromosomes, Human, Pair 21, DNA analysis, Polymerase Chain Reaction methods, Prenatal Diagnosis methods

Abstract

Objective: The aim of our study was to estimate the observed heterozygosity and informativeness of 6 STR markers on chromosomes 18 and 21 in the Bulgarian population. We have evaluated the applicability of these markers used from other investigators for QF-PCR prenatal diagnosis of the most common autosomal aneuploidies in Bulgaria., Methods: DNA samples (n = 486) were extracted from different fetal tissues (amniotic fluid cells, chorionic villus samples, and fetal tissue after abortions). PCR amplifications of 4 STR markers located on chromosome 21 (D21S11, D21S1411, D21S1270, and D21S1440) and 2 on chromosome 18 (D18S535 and D18S51) were performed. They were analysed on an automated sequencer, and the allele dosage ratios were calculated., Results: The results indicate the selected markers as highly informative for our population and suitable for QF-PCR prenatal diagnosis in Bulgaria. All samples with trisomy 21 (n = 8), trisomy 18 (n = 4) and triploidy (n = 1) were correctly detected by our analysis. Thus, no false-negative results were observed., Conclusion: QF-PCR analysis could be an applicable alternative in prenatal and postnatal diagnosis in cases with a strong suspicion for particular autosomal aneuploidies (including chromosomes 21, 18, and 13) in small countries with limited resources like Bulgaria., (Copyright 2004 John Wiley & Sons, Ltd.)

Published

2004

37. A new approach to extending the wheat marker pool by anchored PCR amplification of compound SSRs.

Author

Hayden MJ, Stephenson P, Logojan AM, Khatkar D, Rogers C, Koebner RM, Snape JW, and Sharp PJ

Subjects

Chromosome Mapping, DNA Primers, Electrophoresis, Fluorescence, Silver Staining, Alleles, Minisatellite Repeats genetics, Polymerase Chain Reaction methods, Triticum genetics

Abstract

A study was undertaken to determine the utility in bread wheat of anchored PCR for the development of single locus SSR markers targeted at compound repeat motifs. In anchored PCR, microsatellite amplification is achieved using a single primer complementary to the flanking sequence, and one which anchors to the repeat junction of the compound SSR. The recovery rate of useable markers was found to be similar (43%) to that reported for conventionally generated SSRs. Thus, anchored PCR can be used to reduce the costs of marker development, since it requires that only half the number of primers be synthesised. Where fluorescence-based platforms are used, marker deployment costs are lower, since only the anchoring primers need to be labelled. In addition, anchored PCR improves the recovery of useful markers, as it allows assays to be generated from microsatellite clones with repeat sequences located close to their ends, a situation where conventional PCR amplification fails as two flanking primers cannot be designed. Strategies to permit the large-scale development of compound SSR markers amplified by anchored PCR are discussed.

Published

2004

38. Autoclave method for rapid preparation of bacterial PCR-template DNA.

Author

Simmon KE, Steadman DD, Durkin S, Baldwin A, Jeffrey WH, Sheridan P, Horton R, and Shields MS

Subjects

Antarctic Regions, DNA, Bacterial chemistry, Electrophoresis, Enterococcus chemistry, Enterococcus isolation & purification, Escherichia coli chemistry, Escherichia coli isolation & purification, Florida, Geologic Sediments, Random Amplified Polymorphic DNA Technique, Soil Microbiology, DNA, Bacterial isolation & purification, Enterococcus genetics, Escherichia coli genetics, Polymerase Chain Reaction methods, Templates, Genetic

Abstract

An autoclave method for preparing bacterial DNA for PCR template is presented, it eliminates the use of detergents, organic solvents, and mechanical cellular disruption approaches, thereby significantly reducing processing time and costs while increasing reproducibility. Bacteria are lysed by rapid heating and depressurization in an autoclave. The lysate, cleared by microcentrifugation, was either used directly in the PCR reaction, or concentrated by ultrafiltration. This approach was compared with seven established methods of DNA template preparation from four bacterial sources which included boiling Triton X-100 and SDS, bead beating, lysozyme/proteinase K, and CTAB lysis method components. Bacteria examined were Enterococcus and Escherichia coli, a natural marine bacterial community and an Antarctic cyanobacterial-mat. DNAs were tested for their suitability as PCR templates by repetitive element random amplified polymorphic DNA (RAPD) and denaturing gradient gel electrophoresis (DGGE) analysis. The autoclave method produced PCR amplifiable template comparable or superior to the other methods, with greater reproducibility, much shorter processing time, and at a significantly lower cost.

Published

2004

39. Nonelectrophoretic method for high-throughput HLA-DRB1 group genotyping.

Author

Hampe J, Valentonyte R, Manaster C, Teuber M, Jenisch S, Entz P, Nagy M, and Schreiber S

Subjects

DNA Probes, HLA genetics, Electrophoresis, Genetic Testing, Genotype, HLA Antigens genetics, HLA-DRB1 Chains, Humans, User-Computer Interface, Gene Expression Profiling methods, HLA-DR Antigens genetics, Oligonucleotide Array Sequence Analysis methods, Polymerase Chain Reaction methods, Software

Published

2004

40. Co-amplification of ENFSI-loci D3S1358, D8S1179 and D18S51: validation of new primer sequences and allelic distribution among 2874 individuals.

Author

Pötter T

Subjects

Animals, Cats, Cattle, Chickens, Columbidae, Cricetinae, DNA isolation & purification, Dogs, Electrophoresis, Genetics, Population, Humans, Male, Mice, Pan troglodytes, Rabbits, Rats, Sheep, Species Specificity, Swine, DNA Fingerprinting methods, DNA Primers, Gene Frequency, Polymerase Chain Reaction methods, Sequence Analysis, DNA methods, Tandem Repeat Sequences

Abstract

The present communication presents a new triplex PCR co-amplifying three loci (D3S1358, D8S1179 and D18S51) recommended for STR typing by the European Network of Forensic Science Institutes (ENFSI). Twenty-two different primers were tested to optimise the PCR. Four of the six primer sequences finally chosen were self selected, the fifth was a published one and the sixth derived from a commercially available multiplex kit. Using this PCR-setup, even minimum amounts of genomic DNA are sufficient to analyse the STR loci D3S1358, D8S1179 and D18S51 in parallel. Especially in forensic casework, where DNA is mostly limited and often contaminated with enzyme inhibitors, this new PCR proved to be very advantageous. To demonstrate the reliability, buccal swabs from 2874 persons were typed not only with the new triplex PCR but also with a commercially available multiplex kit.

Published

2003

41. Detection of Edwardsiella infections in Opsanus tau by polymerase chain reaction.

Author

Baird KD, Chikarmane HM, Smolowitz R, and Uhlinger KR

Subjects

Animals, Aquaculture, DNA Primers, Edwardsiella physiology, Electrophoresis, Genes, rRNA genetics, Batrachoidiformes microbiology, Edwardsiella genetics, Enterobacteriaceae Infections diagnosis, Enterobacteriaceae Infections veterinary, Polymerase Chain Reaction methods

Published

2003

42. Identification of moulds belonging to the Penicillium genus using a polymerase chain reaction (PCR-SSCP) method followed by 'computer assisted' statistical analysis of the electrophoretic patterns.

Author

Colombo F, Vallone L, Capoferri R, and Dragoni I

Subjects

Animals, Base Sequence, Cattle, DNA Primers, DNA, Fungal genetics, DNA, Fungal isolation & purification, Electrophoresis, Mathematical Computing, Penicillium classification, Penicillium genetics, Penicillium chrysogenum genetics, Penicillium chrysogenum isolation & purification, Phylogeny, Dairy Products microbiology, Penicillium isolation & purification, Polymerase Chain Reaction methods, Polymorphism, Single-Stranded Conformational

Published

2003

43. STR DNA typing: increased sensitivity and efficient sample consumption using reduced PCR reaction volumes.

Author

Leclair B, Sgueglia JB, Wojtowicz PC, Juston AC, Frégeau CJ, and Fourney RM

Subjects

Case-Control Studies, Electrophoresis, Feasibility Studies, Female, Forensic Medicine methods, Humans, Male, Sensitivity and Specificity, DNA analysis, DNA Fingerprinting methods, Polymerase Chain Reaction methods, Tandem Repeat Sequences

Abstract

Improvements in detection limits/sensitivity and lower sample consumption are potential benefits of reducing PCR reaction volumes used in forensic DNA typing of crime scene samples. This premise was studied first with experimental mixtures and a nine-loci megaplex, which demonstrated stochiometric amplification and accurate detection. Next, adjudicated casework samples were subjected to amplification under 15 different template DNA to PCR reaction volume ratios. Reduction of PCR reaction volume and DNA down to 10 microL and 0.500 ng, respectively, produced identical profiles with the same signal intensity and heterozygous allele peak height ratio (HR). Reduction to 5 microL and 0.063 ng yielded HR values that were slightly affected in one to three STR loci. PCR reaction volume reduction can enhance detection and sensitivity while reducing the consumption of irreplaceable crime scene samples.

Published

2003

44. AmpFlSTR profiler Plus short tandem repeat DNA analysis of casework samples, mixture samples, and nonhuman DNA samples amplified under reduced PCR volume conditions (25 microL).

Author

Frégeau CJ, Bowen KL, Leclair B, Trudel I, Bishop L, and Fourney RM

Subjects

Alleles, Animals, Bacteria genetics, Case-Control Studies, Electrophoresis, Female, Forensic Medicine methods, Humans, Male, Sensitivity and Specificity, Yeasts genetics, DNA analysis, DNA Fingerprinting methods, Polymerase Chain Reaction methods, Tandem Repeat Sequences

Abstract

As part of the validation of the AmpFlSTR Profiler Plus short tandem repeat (STR) system, under reduced polymerase chain reaction (PCR) volume conditions (i.e., 25 microL), a total of 275 casework samples were processed. Examples of profiles are presented along with amplification conditions to improve the odds of obtaining balanced and complete profiles for samples showing partial results or profiles with a descending slope. Data collected and used to develop our interpretation guidelines are included. From the mixture studies, full profiles were obtained for minor contributors, using 2 ng of DNA, with ratios of 10:1 or 1:20 and using 1 ng of DNA, with ratios of 10:1 and 1:8. The specificity of the Profiler Plus amplification reaction performed in 25 microL was examined and confirmed using a large spectrum of nonhuman DNAs. This report supports the use of the AmpFlSTR Profiler Plus STR system for casework DNA typing under reduced PCR volume conditions.

Published

2003

45. Polymerase chain reaction amplification of samples from Japanese monkeys using primers for human short tandem repeat loci.

Author

Ago K, Ago M, Orihara Y, Nakagawa S, and Ogata M

Subjects

Animals, DNA analysis, Electrophoresis, Humans, Macaca fascicularis genetics, Species Specificity, DNA Primers analysis, Polymerase Chain Reaction methods, Tandem Repeat Sequences

Abstract

We examined the species specificity of six commercially available human short tandem repeat systems (for CSF1PO, TPOX, TH01, F13A01, FESFPS and vWA) using six samples obtained from the Japanese monkey Macaca fuscata. Macaque genes were amplified with human TPOX and F13A01 primers. During electrophoresis, macaque polymerase chain reaction (PCR) products amplified with the TPOX primer migrated more slowly than human ones, and migrated close to human CSF1PO bands. Macaque PCR products amplified with the F13A01 primer also migrated more slowly than the human equivalent. The six macaque samples were classified into three types by the TPOX primer and into six types by the F13A01 primer. These results suggest that the primers for human TPOX and F13A01 loci can be used to distinguish between human and Japanese macaque samples.

Published

2003

46. Identification of Nile perch (Lates niloticus), grouper (Epinephelus guaza), and wreck fish (Polyprion americanus) fillets by PCR amplification of the 5S rDNA gene.

Author

Asensio L, González I, Fernández A, Céspedes A, Rodríguez MA, Hernández PE, García T, and Martín R

Subjects

Animals, Base Sequence, DNA, Ribosomal chemistry, Electrophoresis, Fishes classification, Molecular Sequence Data, Perches classification, Species Specificity, DNA, Ribosomal analysis, Fishes genetics, Perches genetics, Polymerase Chain Reaction, RNA, Ribosomal, 5S genetics

Abstract

Nile perch (Lates niloticus), grouper (Epinephelus guaza), and wreck fish (Polyprion americanus) were differentiated by polymerase chain reaction (PCR) amplification of the nuclear 5S rDNA gene. The design of 3 species-specific primers complementary to the nontranscribed intergenic spacer region from the 5S rDNA molecule allowed amplification of clearly distinguishable gene fragments in each fish species. This approach is rapid and reliable and offers the potential to detect fraudulent or unintentional mislabeling of these species in routine seafood authentication analysis.

Published

2001

47. [Analysis of the non-deletion alpha-thalassemia mutations by PCR temperature gradient gel electrophoresis].

Author

Zhao Y, Xu X, and Yang Y

Subjects

Electrophoresis, Globins genetics, Humans, Polymorphism, Genetic, Temperature, Point Mutation, Polymerase Chain Reaction, alpha-Thalassemia genetics

Abstract

Objective: To develop a PCR-temperature gradient gel electrophoresis(TGGE) method applied to screening for the point mutations causing the non-deletion alpha-thalassemia., Methods: The entire alpha2-globin gene fragment (1085 bp) was selectively amplified from human genomic DNA with different genotypes of alpha-thalassemia and a 543 bp fragment spanning the exon 2 and exon 3 of the alpha2-globin gene was amplified with a pair of nested primers. The condition of perpendicular and parallel TGGE for the two different fragments in length was optimized and the candidate mutant was confirmed by DNA sequencing. In pilot study, 15 samples with suspected non-deletion alpha-thalassemia were screened for point mutations in alpha-globin gene., Results: Hb Constant Spring (Hb CS) and Hb Quong Sze (Hb QS), two most commonly types of the non-deletion alpha-thalassemia distributed in Chinese, and a rare type of the Hb Westmead mutation, alpha2 CD122 CAC-->CAG(His-->Gln) could be detected by PCR-TGGE. Among those 15 samples screened for alpha-thalassemia mutation were 10 samples with Hb CS mutation, 2 samples with Hb QS mutation, 2 samples with Hb Westmead mutation, and a previously unreported one, alpha2 CD31 AGG-->AAG(Arg-->Lys), confirmed by DNA sequencing., Conclusion: The present PCR-TGGE method could be a useful tool for the molecular screening for the point mutations causing alpha-thalassemia and alpha-globin gene polymorphism.

Published

2001

48. Direct polymerase chain reaction from whole blood without DNA isolation.

Author

Nishimura N, Nakayama T, Tonoike H, Kojima K, and Kato S

Subjects

Animals, DNA chemistry, Electrophoresis, Globins genetics, Globins metabolism, Humans, Indicators and Reagents chemistry, Indicators and Reagents metabolism, Reproducibility of Results, Sensitivity and Specificity, DNA blood, Polymerase Chain Reaction methods

Abstract

Blood and other animal fluids contain a variety of substances that inhibit the polymerase chain reaction (PCR), so that isolation of DNA is generally necessary prior to PCR. We have developed a novel reagent cocktail that effectively suppresses these inhibitory substances and makes DNA isolation from blood unnecessary for PCR. When this reagent was included in the PCR mixture, DNA fragments of the beta-globin gene could be efficiently amplified directly from human blood samples treated with various anticoagulants or PCR-inhibitory substances. We confirmed the usefulness of this cocktail by examining a large number of blood samples with various PCR primer sets. In addition to fresh blood, this method enabled PCR amplification from blood samples stored at 4 degrees C, -20 degrees C or -80 degrees C for a minimum of 1 year.

Published

2000

49. Integrated system for rapid PCR-based DNA analysis in microfluidic devices.

Author

Khandurina J, McKnight TE, Jacobson SC, Waters LC, Foote RS, and Ramsey JM

Subjects

Electrophoresis, Microcomputers, DNA analysis, Polymerase Chain Reaction methods

Abstract

An integrated system for rapid PCR-based analysis on a microchip has been demonstrated. The system couples a compact thermal cycling assembly based on dual Peltier thermoelectric elements with a microchip gel electrophoresis platform. This configuration allows fast (approximately 1 min/ cycle) and efficient DNA amplification on-chip followed by electrophoretic sizing and detection on the same chip. An on-chip DNA concentration technique has been incorporated into the system to further reduce analysis time by decreasing the number of thermal cycles required. The concentration injection scheme enables detection of PCR products after performing as few as 10 thermal cycles, with a total analysis time of less than 20 min. The starting template copy number was less than 15 per injection volume.

Published

2000

50. Randomly amplified polymorphic DNA (RAPD) PCR for the identification of yeasts isolated from dairy products.

Author

Andrighetto C, Psomas E, Tzanetakis N, Suzzi G, and Lombardi A

Subjects

Base Sequence, DNA Primers genetics, Electrophoresis, Molecular Sequence Data, Polymorphism, Genetic genetics, Sequence Analysis, DNA, Species Specificity, Yeasts genetics, Cheese microbiology, DNA, Fungal analysis, Food Microbiology, Polymerase Chain Reaction methods, Yeasts classification

Abstract

In the present work randomly amplified polymorphic DNA-polymerase chain reaction (RAPD-PCR) with primers M13 and RF2 was applied to the identification at species level of yeast strains isolated from cheeses. RAPD-PCR analysis of the type strains of different yeast species gave distinctive band profiles that allowed a clear differentiation of all the considered species. Forty-two of the 48 dairy associated yeasts were clearly assigned to the species Saccharomyces cerevisiae, Kluyveromyces marxianus (anamorph Candida kefyr), Kluyveromyces lactis (anamorph Candida sphaerica), Debaryomyces hansenii (anamorph Candida famata), Yarrowia lipolytica and Torulaspora delbrueckii (anamorph Candida colliculosa). The method, which is rapid and easy to perform, could be a useful tool for the identification of yeasts present in dairy products.

Published

2000