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190 results on '"Restriction enzyme digestion"'

1. Effective DNA fragmentation technique for simple sequence repeat detection with a microsatellite-enriched library and high-throughput sequencing

Author

Keisuke Tanaka, Rumi Ohtake, Saki Yoshida, and Takashi Shinohara

Subjects
DNA fragmentation, high-throughput sequencing, microsatellite enrichment, restriction enzyme digestion, Myrtaceae, simple sequence repeat, Biology (General), QH301-705.5
Abstract

Two different techniques for genomic DNA fragmentation before microsatellite-enriched library construction—restriction enzyme (NlaIII and MseI) digestion and sonication—were compared to examine their effects on simple sequence repeat (SSR) detection using high-throughput sequencing. Tens of thousands of SSR regions from 5 species of the plant family Myrtaceae were detected when the output of individual samples was >1 million paired-end reads. Comparison of the two DNA fragmentation techniques showed that restriction enzyme digestion was superior to sonication for identification of heterozygous genotypes, whereas sonication was superior for detection of various SSR flanking regions with both species-specific and common characteristics. Therefore, choosing the most suitable DNA fragmentation method depends on the type of analysis that is planned.

Published
2017
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3. Type II restriction modification system in Ureaplasma parvum OMC-P162 strain.

Author

Wu, Heng Ning, Nakura, Yukiko, Yoshimura, Michinobu, Gaddi Tantengco, Ourlad Alzeus, Nomiyama, Makoto, Takayanagi, Toshimitsu, Fujita, Tomio, Yasukawa, Kiyoshi, and Yanagihara, Itaru

Subjects
*UREAPLASMA, *METHYLCYTOSINE, *GESTATIONAL age, *OPERONS, *DNA methyltransferases
Abstract

Ureaplasma parvum serovar 3 strain, OMC-P162, was isolated from the human placenta of a preterm delivery at 26 weeks’ gestation. In this study, we sequenced the complete genome of OMC-P162 and compared it with other serovar 3 strains isolated from patients with different clinical conditions. Ten unique genes in OMC-P162, five of which encoded for hypothetical proteins, were identified. Of these, genes UPV_229 and UPV_230 formed an operon whose open reading frames were predicted to code for a DNA methyltransferase and a hypothetical protein, respectively. DNA modification analysis of the OMC-P162 genome identified N4-methylcytosine (m4C) and N6-methyladenine (m6A), but not 5-methylocytosine (m5C). UPV230 recombinant protein displayed endonuclease activity and recognized the CATG sequence, resulting in a blunt cut between A and T. This restriction enzyme activity was identical to that of the cultivated OMC-P162 strain, suggesting that this restriction enzyme was naturally expressed in OMC-P162. We designated this enzyme as UpaP162. Treatment of pT7Blue plasmid with recombinant protein UPV229 completely blocked UpaP162 restriction enzyme activity. These results suggest that the UPV_229 and UPV_230 genes act as a type II restriction-modification system in Ureaplasma OMC-P162. [ABSTRACT FROM AUTHOR]

Published
2018
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5. Prevalence and molecular characteristics of fowl adenovirus serotype 4 in eastern Saudi Arabia.

Author

HEMIDA, Maged Gomaa and AL-HAMMADI, Mohamed

Subjects
*VIRUS diseases in poultry, *CHICKEN diseases, *DISEASE prevalence, *ANIMAL vaccination, *RESTRICTION fragment length polymorphisms
Abstract

Fowl adenovirus serotype 4 (FAdV-4) is a new emerging viral disease of chickens worldwide. It causes inclusion body hepatitis and hepatitis-hydropericardium syndrome. Little is known about its prevalence in the Middle East. Here we report the prevalence of FAdV-4 in five chicken farms in eastern Saudi Arabia. High mortality rates were reported from birds from those five farms at 15 weeks of age. Gross examination revealed typical hydropericardium syndrome and accumulation of jelly-like materials in the pericardial cavities. We isolated FAdV-4 by using embryonated chicken egg inoculation. The inoculated embryos showed dwarfing, deformities, hemorrhage, and death after 3-5 days of inoculations. Detection of FAdV-4 in the heart and liver tissues was achieved by polymerase chain reaction (PCR) and real-time PCR using the primers targeted to the partial hexon gene. Further confirmation was done by restriction fragment length polymorphism and the digestion patterns of the isolated FAdV-4 DNAs were close to those of other known FAdV-4 strains. The average genome size of the virus was ~43 kb. Phylogenetic analysis of the partial hexon gene sequences confirmed that these strains were closely related to other Asian strains from Kuwait, India, and Pakistan reported to GenBank. To our knowledge, this is the first study that reports the isolation and molecular characterization of FAdV-4 in chickens in Saudi Arabia. [ABSTRACT FROM AUTHOR]

Published
2017
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6. Determination of restriction enzyme activity when cutting DNA labeled with the TOTO dye family.

Author

Maschmann, April and Kounovsky-Shafer, Kristy L.

Subjects
*ENZYME activation, *DNA methylation, *FLUOROPHORES, *CYANINES, *GEL electrophoresis
Abstract

Optical mapping, a single DNA molecule genome analysis platform that can determine methylation profiles, uses fluorescently labeled DNA molecules that are elongated on the surface and digested with a restriction enzyme to produce a barcode of that molecule. Understanding how the cyanine fluorochromes affect enzyme activity can lead to other fluorochromes used in the optical mapping system. The effects of restriction digestion on fluorochrome labeled DNA (Ethidium Bromide, DAPI, H33258, EthD-1, TOTO-1) have been analyzed previously. However, TOTO-1 is a part of a family of cyanine fluorochromes (YOYO-1, TOTO-1, BOBO-1, POPO-1, YOYO-3, TOTO-3, BOBO-3, and POPO-3) and the rest of the fluorochromes have not been examined in terms of their effects on restriction digestion. In order to determine if the other dyes in the TOTO-1 family inhibit restriction enzymes in the same way as TOTO-1, lambda DNA was stained with a dye from the TOTO family and digested. The restriction enzyme activity in regards to each dye, as well as each restriction enzyme, was compared to determine the extent of digestion. YOYO-1, TOTO-1, and POPO-1 fluorochromes inhibited ScaI-HF, PmlI, and EcoRI restriction enzymes. Additionally, the mobility of labeled DNA fragments in an agarose gel changed depending on which dye was intercalated. [ABSTRACT FROM PUBLISHER]

Published
2017
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7. Molecular characterization and evaluation of the emerging antibiotic-resistant Streptococcus pyogenes from eastern India.

Author

Ray, Dipanwita, Saha, Somnath, Sinha, Sukanta, Kumar Pal, Nishith, and Bhattacharya, Basudev

Subjects
*STREPTOCOCCUS pyogenes, *PUBLIC health, *MOLECULAR weights, *ANTIBIOTICS, *DRUG resistance in bacteria
Abstract

Background: Group A Streptococcus strains causing wide variety of diseases, recently became noticeable in eastern India, are not amenable to standard treatment protocol thus enhancing the possibility of disease morbidity by becoming antibiotic resistance. Methods: The association of Lancefield group A Streptococcal variation with degree of vir architectural diversity was evaluated using emm typing and restriction fragment length polymorphism analyses. The antibiotic sensitivity patterns were examined by modified Kirby-Bauer method of disk diffusion. Percentage calculations, 95% confidence interval and one-way ANOVA were used to assess differences in proportions. Results: Our observations revealed 20 different emm types and 13 different HaeIII vir typing patterns. A 1.2 kb fragment was found in all HaeIII typing pattern. Fragments of 1.2 kb and 550 bp were conserved in majority of the isolates. HinfI digestion was found proficient in differentiating the strains of same vir typing patterns. Strong predominance of speC (85%) and speF (80%) genes have been observed encoding exotoxins production. 4 isolates were found to be erythromycin resistant and were of genotype emm49. High degree of tetracycline resistance was shown by 53.57% isolates which belonged to 12 different emm genotypes. Conclusions: These findings suggested that in addition to emm typing, sequential application of HaeIII and HinfI restriction enzymes in vir typing analysis is an effective tool for group A streptococcal molecular characterization associated with antibiotic resistance. [ABSTRACT FROM AUTHOR]

Published
2016
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8. Localization of Low Copy Number Plasmid pRC4 in Replicating Rod and Non-Replicating Cocci Cells of Rhodococcus erythropolis PR4.

Author

Singhi, Divya, Jain, Aayushi, and Srivastava, Preeti

Subjects
*RHODOCOCCUS erythropolis, *DNA copy number variations, *PLASMID replication, *EXPONENTIAL functions, *NUCLEOIDS
Abstract

Rhodococcus are gram-positive bacteria, which can exist in two different shapes rod and cocci. A number of studies have been done in the past on replication and stability of small plasmids in this bacterium; however, there are no reports on spatial localization and segregation of these plasmids. In the present study, a low copy number plasmid pDS3 containing pRC4 replicon was visualized in growing cells of Rhodococcus erythropolis PR4 (NBRC100887) using P1 parS-ParB-GFP system. Cells were initially cocci and then became rod shaped in exponential phase. Cocci cells were found to be non-replicating as evident by the presence of single fluorescence focus corresponding to the plasmid and diffuse fluorescence of DnaB-GFP. Rod shaped cells contained plasmid either present as one fluorescent focus observed at the cell center or two foci localized at quarter positions. The results suggest that the plasmid is replicated at the cell center and then it goes to quarter position. In order to observe the localization of plasmid with respect to nucleoid, plasmid segregation was also studied in filaments where it was found to be replicated at the cell center in a nucleoid free region. To the best of our knowledge, this is the first report on segregation of small plasmids in R. erythropolis. [ABSTRACT FROM AUTHOR]

Published
2016
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9. A Closed-Tube Loop-Mediated Isothermal Amplification Assay for the Visual Detection of Staphylococcus aureus

Author

Jing Xiong, Ji-Song Xu, Wen-Shu Huang, and Huang Bei

Subjects
DNA, Bacterial, 0106 biological sciences, Staphylococcus aureus, Loop-mediated isothermal amplification, Bioengineering, medicine.disease_cause, 01 natural sciences, Applied Microbiology and Biotechnology, Biochemistry, Cresols, Human health, 010608 biotechnology, medicine, Closed tube, Restriction enzyme digestion, Gyrb gene, Molecular Biology, Detection limit, Chromatography, 010405 organic chemistry, Chemistry, General Medicine, 0104 chemical sciences, Visual detection, Molecular Diagnostic Techniques, DNA Gyrase, Food Microbiology, Nucleic Acid Amplification Techniques, Biotechnology
Abstract

Food-borne diseases induced by Staphylococcus aureus contamination seriously affect human health and food safety. Therefore, a closed-tube loop-mediated isothermal amplification (LAMP) assay for the visual detection of S. aureus was developed in this study. Firstly, two pairs of outer and inner primers were designed targeting on a conserved fragment of gyrB gene in different S. aureus strains. Secondly, the weakly buffered gyrB-LAMP assays were optimized under various pH values and other conditions, followed by the visual evaluation of five pH-sensitive indicators, and the cresol-red was chosen as the best dye for the best visual performance. Thirdly, the cresol-red-based LAMP assay showed good sensitivity with the detection limit of 5.4 copies/μL for purified DNAs, and good specificity with no cross-reaction with other related species. The specificity of the amplified products was further confirmed by XbaI restriction enzyme digestion analysis. Finally, the cresol-red-based LAMP assay was validated by the clinical-dried fish samples inoculated with known numbers of S. aureus and further validated by 20 blind samples. To our knowledge, this is the first report of a closed-tube LAMP assay based on pH-sensitive indicators for the visual detection of the food-borne S. aureus by the gyrB gene.

Published
2020

11. Protocols for RLGS Gel Production

Author

Okazaki, Yasushi, Okuizumi, Hisato, Sasaki, Nobuya, Takada, Shuji, Takahara, Tokuei, Hayashizaki, Yoshihide, Hayashizaki, Yoshihide, editor, and Watanabe, Sachihiko, editor

Published
1997
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12. Combining dense and sparse labeling in optical DNA mapping

Author

Torstensson, E., Goyal, G., Johnning, A., Westerlund, F., Ambjörnsson, T., and Publica

Subjects
Molecular biology, Bioinformatics, Science, Evolutionary systematics, Sequence Databases, Evolutionary biology, DNA construction, Data management, Biochemistry, Restriction Enzyme Digestion, Database and Informatics Methods, DNA Barcoding, Taxonomic, DNA barcoding, DNA labeling, Fluorescent Dyes, Molecular systematics, Taxonomy, Computer and information sciences, Biology and life sciences, Optical Imaging, Proteins, DNA, Enzymes, Research and analysis methods, Molecular biology techniques, Biological Databases, Plasmid Construction, Enzymology, Medicine, Nucleic acid labeling, Databases, Nucleic Acid, Enzymatic Digestion Techniques, Sequence Analysis, Sequence Alignment, Plasmids, Research Article, Cell labeling
Abstract

Optical DNA mapping (ODM) is based on fluorescent labeling, stretching and imaging of single DNA molecules to obtain sequence-specific fluorescence profiles, DNA barcodes. These barcodes can be mapped to theoretical counterparts obtained from DNA reference sequences, which in turn allow for DNA identification in complex samples and for detecting structural changes in individual DNA molecules. There are several types of DNA labeling schemes for ODM and for each labeling type one or several types of match scoring methods are used. By combining the information from multiple labeling schemes one can potentially improve mapping confidence; however, combining match scores from different labeling assays has not been implemented yet. In this study, we introduce two theoretical methods for dealing with analysis of DNA molecules with multiple label types. In our first method, we convert the alignment scores, given as output from the different assays, into p-values using carefully crafted null models. We then combine the p-values for different label types using standard methods to obtain a combined match score and an associated combined p-value. In the second method, we use a block bootstrap approach to check for the uniqueness of a match to a database for all barcodes matching with a combined p-value below a predefined threshold. For obtaining experimental dual-labeled DNA barcodes, we introduce a novel assay where we cut plasmid DNA molecules from bacteria with restriction enzymes and the cut sites serve as sequence-specific markers, which together with barcodes obtained using the established competitive binding labeling method, form a dual-labeled barcode. All experimental data in this study originates from this assay, but we point out that our theoretical framework can be used to combine data from all kinds of available optical DNA mapping assays. We test our multiple labeling frameworks on barcodes from two different plasmids and synthetically generated barcodes (combined competitive-binding- and nick-labeling). It is demonstrated that by simultaneously using the information from all label types, we can substantially increase the significance when we match experimental barcodes to a database consisting of theoretical barcodes for all sequenced plasmids.

Published
2021

13. Innovations in double digest restriction-site associated DNA sequencing (ddRAD-Seq) method for more efficient SNP identification.

Author

Magbanua, Zenaida V., Hsu, Chuan-Yu, Pechanova, Olga, Arick II, Mark, Grover, Corrinne E., and Peterson, Daniel G.

Subjects
*SINGLE nucleotide polymorphisms, *DNA sequencing, *TECHNOLOGICAL innovations, *RESTRICTION fragment length polymorphisms, *PRINCIPAL components analysis, *SEQUENCE alignment
Abstract

We present an improved ddRAD-Seq protocol for identifying single nucleotide polymorphisms (SNPs). It utilizes selected restriction enzyme digestion fragments, quick acting ligases that are neutral with the restriction enzyme buffer eliminating buffer exchange steps, and adapters designed to be compatible with Illumina index primers. Library amplification and barcoding are completed in one PCR step, and magnetic beads are used to purify the genomic fragments from the ligation and library generation steps. Our protocol increases the efficiency and decreases the time to complete a ddRAD-Seq experiment. To demonstrate its utility, we compared SNPs from our protocol with those from whole genome resequencing data from Gossypium herbaceum and Gossypium arboreum. Principal component analysis demonstrated that the variability of the combined data was explained by the genotype (PC1) and methodology applied (PC2). Phylogenetic analysis showed that the SNPs from our method clustered with SNPs from the resequencing data of the corresponding genotype. Sequence alignments illustrated that for homozygous loci, more than 90% of the SNPs from the resequencing data were discovered by our method. Our analyses suggest that our ddRAD-Seq method is reliable in identifying SNPs suitable for phylogenetic and association genetic studies while reducing cost and time over known methods. [Display omitted] • Marker search by reduced representation an affordable option over whole genome ways. • Innovations in a reduced representation method led to ample cuts in costs and time. • Number of markers identified with innovations proportional to genome reduction rate. • Usefulness of markers confirmed with phylogenetic and principal component analyses. [ABSTRACT FROM AUTHOR]

Published
2023
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14. Development of a Molecular Tool for Identification of a New Neopestalotiopsis sp. Associated with Disease Outbreaks on Strawberry.

Author

Kaur H, Gelain J, Marin MV, Peres NA, and Schnabel G

Subjects
Polymorphism, Restriction Fragment Length, Polymerase Chain Reaction methods, Florida, Fragaria genetics, Xylariales genetics
Abstract

A new Neopestalotiopsis sp. was recently reported causing outbreaks of leaf spot and fruit rot on strawberry in Florida, Georgia, and South Carolina. In contrast to other Pestalotiopsis pathogens, the new species appears more aggressive and destructive on strawberry. Current chemical options for management are disease suppressive at best, and affected growers have been experiencing major yield losses. In this study, we developed a molecular method based on polymerase chain reaction/restriction fragment length polymorphism (PCR/RFLP) for identification of the new Neopestalotiopsis sp. from strawberry. Isolates of the new Neopestalotiopsis sp. collected in Florida; isolates of N. rosae , N. honoluluana , N. ellipsopora , N. saprophytica , N. samarangensis , and P. rhododendri ; and isolates from South Carolina suspected to be the new Neopestalotiopsis sp. were included in this study. This method is based on PCR amplification of a β-tubulin gene fragment using a previously published set of primers (Bt2a and Bt2b), followed by use of the restriction enzyme BsaWI. The enzyme cuts the PCR product from the new Neopestalotiopsis sp. twice, yielding fragments of 290 base pairs (bp) and 130 and 20 bp in size, whereas fragments from other species are only cut once, yielding fragments of 420 and 20 bp. This method will aid research labs and diagnostic clinics in the accurate and fast identification of the aggressive Neopestalotiopsis sp. variant from strawberry., Competing Interests: The author(s) declare no conflict of interest.

Published
2023
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15. Analyses of the Distribution Patterns of Burkholderia pseudomallei and Associated Phages in Soil Samples in Thailand Suggest That Phage Presence Reduces the Frequency of Bacterial Isolation.

Author

Withatanung, Patoo, Chantratita, Narisara, Muangsombut, Veerachat, Saiprom, Natnaree, Lertmemongkolchai, Ganjana, Klumpp, Jochen, Clokie, Martha R. J., Galyov, Edouard E., and Korbsrisate, Sunee

Subjects
*BURKHOLDERIA pseudomallei, *ISOLATION of biotechnological microorganisms, *SOIL sampling, *GEOGRAPHICAL distribution of bacteria, *BACTERIAL cultures, *TRANSMISSION electron microscopy
Abstract

Background: Burkholderia pseudomallei is a soil saprophytic bacterium that causes melioidosis. The infection occurs through cutaneous inoculation, inhalation or ingestion. Bacteriophages (phages) in the same ecosystem may significantly impact the biology of this bacterium in the environment, and in their culturability in the laboratory. Methods/Principal Findings: The soil samples were analysed for the presence of bacteria using culture methods, and for phages using plaque assays on B. pseudomallei strain 1106a lawns. Of the 86 soil samples collected from northeastern Thailand, B. pseudomallei was cultured from 23 (26.7%) samples; no phage capable of infecting B. pseudomallei was detected in these samples. In contrast, phages capable of infecting B. pseudomallei, but no bacteria, were present in 10 (11.6%) samples. B. pseudomallei and their phages were co-isolated from only 3 (3.5%) of soil samples. Since phage capable of infecting B. pseudomallei could not have appeared in the samples without the prior presence of bacteria, or exposure to bacteria nearby, our data suggest that all phage-positive/bacteria-negative samples have had B. pseudomallei in or in a close proximity to them. Taken together, these findings indicate that the presence of phages may influence the success of B. pseudomallei isolation. Transmission electron microscopy revealed that the isolated phages are podoviruses. The temperate phages residing in soil-isolated strains of B. pseudomallei that were resistant to the dominant soil borne phages could be induced by mitomycin C. These induced-temperate phages were closely related, but not identical, to the more dominant soil-isolated phage type. Conclusion/Significance: The presence of podoviruses capable of infecting B. pseudomallei may affect the success of the pathogen isolation from the soil. The currently used culture-based methods of B. pseudomallei isolation appear to under-estimate the bacterial abundance. The detection of phage capable of infecting B. pseudomallei from environmental samples could be a useful preliminary test to indicate the likely presence of B. pseudomallei in environmental samples. [ABSTRACT FROM AUTHOR]

Published
2016
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16. CisSERS: Customizable In Silico Sequence Evaluation for Restriction Sites.

Author

Sharpe, Richard M., Koepke, Tyson, Harper, Artemus, Grimes, John, Galli, Marco, Satoh-Cruz, Mio, Kalyanaraman, Ananth, Evans, Katherine, Kramer, David, and Dhingra, Amit

Subjects
*DNA restriction enzymes, *NUCLEOTIDE sequencing, *GENETIC polymorphisms, *COMPARATIVE genomics, *GENETIC markers, *DATA analysis
Abstract

High-throughput sequencing continues to produce an immense volume of information that is processed and assembled into mature sequence data. Data analysis tools are urgently needed that leverage the embedded DNA sequence polymorphisms and consequent changes to restriction sites or sequence motifs in a high-throughput manner to enable biological experimentation. CisSERS was developed as a standalone open source tool to analyze sequence datasets and provide biologists with individual or comparative genome organization information in terms of presence and frequency of patterns or motifs such as restriction enzymes. Predicted agarose gel visualization of the custom analyses results was also integrated to enhance the usefulness of the software. CisSERS offers several novel functionalities, such as handling of large and multiple datasets in parallel, multiple restriction enzyme site detection and custom motif detection features, which are seamlessly integrated with real time agarose gel visualization. Using a simple fasta-formatted file as input, CisSERS utilizes the REBASE enzyme database. Results from CisSERS enable the user to make decisions for designing genotyping by sequencing experiments, reduced representation sequencing, 3’UTR sequencing, and cleaved amplified polymorphic sequence (CAPS) molecular markers for large sample sets. CisSERS is a java based graphical user interface built around a perl backbone. Several of the applications of CisSERS including CAPS molecular marker development were successfully validated using wet-lab experimentation. Here, we present the tool CisSERS and results from in-silico and corresponding wet-lab analyses demonstrating that CisSERS is a technology platform solution that facilitates efficient data utilization in genomics and genetics studies. [ABSTRACT FROM AUTHOR]

Published
2016
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19. Easy Hi-C: A Low-Input Method for Capturing Genome Organization.

Author

Lu L and Jin F

Subjects
Chromosome Mapping methods, Chromatin genetics, High-Throughput Nucleotide Sequencing methods, Genome, Chromosomes
Abstract

Chromosome conformation capture technology and its derivatives have been widely used to study genome organization. Among them, Hi-C (chromosome conformation capture coupling with high-throughput sequencing) is popular in dissecting chromatin architecture on the genome-wide level. However, the intrinsic limitations prevent its application when it comes to rare samples. Here, we present easy Hi-C, a biotin-free technology that dramatically reduces DNA loss and is suitable for low-input samples., (© 2023. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published
2023
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21. Rapid isolation of DNA from Dioscorea species suitable for PCR, restriction digestion and pathogen screening.

Author

Raj, Mithun, Nath, Vishnu S., Senthil @ Sankar, M., Jeeva, M.L., and Hegde, Vinayaka

Subjects
*YAMS, *POLYMERASE chain reaction, *GENETIC testing, *NUCLEIC acid isolation methods, *POLYSACCHARIDES, *POLYPHENOLS, *CETYLTRIMETHYLAMMONIUM bromide
Abstract

The methods employed for DNA extraction from many plants is difficult because of the metabolites that interfere with DNA isolation procedures. We have developed a reliable and efficient method for isolating genomic DNA free from polysaccharide, polyphenols and protein contaminants fromDioscoreaspp. The method involves inactivation of contaminant proteins by using CTAB/Proteinase K and precipitation of polysaccharides in the presence of high concentration of salt. The purity of genomic DNA was confirmed by A260/280 and A260/230 ratios calculated from the spectrophotometric readings and further by restriction analysis of the isolated DNA using restriction enzymes Eco RI. The total genomic DNA extracted by the new protocol was used for polymerase chain reaction amplification, RAPD analysis, restriction digestion and pathogen screening. The new protocol can be successfully used for both small- and large-scale preparation of genomic DNA from different tissues ofDioscoreaspp. The quarantine of seed tubers and use of pathogen-free tubers for planting is a prerequisite for integrated disease management strategy. The protocol can be used for the isolation of genomic DNA from other crop plants too. [ABSTRACT FROM PUBLISHER]

Published
2014
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22. Development of a loop-mediated isothermal amplification assay based on RoTat1.2 gene for detection of Trypanosoma evansi in domesticated animals

Author

Binod Kumar, Nilima N. Brahmbhatt, V. L. Parmar, B.R. Maharana, and B. J. Thakre

Subjects
Trypanosoma, genetic structures, 030231 tropical medicine, Pcr cloning, Loop-mediated isothermal amplification, Protozoan Proteins, Antigens, Protozoan, Biology, Polymerase Chain Reaction, Sensitivity and Specificity, 030308 mycology & parasitology, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Trypanosomiasis, Animals, Restriction enzyme digestion, Gene, DNA Primers, 0303 health sciences, General Veterinary, General Medicine, Trypanosoma evansi, DNA, Protozoan, biology.organism_classification, Dna amplification, Molecular biology, eye diseases, Infectious Diseases, chemistry, Molecular Diagnostic Techniques, Insect Science, Animals, Domestic, Agarose gel electrophoresis, Parasitology, Nucleic Acid Amplification Techniques, DNA
Abstract

The early containment of trypanosomosis depends on early, sensitive, and accurate diagnosis in endemic areas with low-intensity infections. The study was planned to develop a simple read out loop-mediated isothermal amplification (LAMP) assay targeting a partial RoTat1.2 VSG gene of Trypanosoma evansi with naked eye visualization of LAMP products by adding SYBR® Green I dye. The visual results were further confirmed with those of agarose gel electrophoresis, restriction enzyme digestion of LAMP products with AluI, and sequencing of the PCR products using LAMP outer primers. The LAMP primers did not show cross reactivity and non-specific reactions with regional common hemoparasitic DNA revealing high specificity of the assay. The threshold sensitivity level of the LAMP assay was determined to be 0.003 fg compared to 0.03 fg RoTat1.2 amplified DNA fragments of T. evansi by PCR assay. Moreover, assessment of 500 blood samples collected from unhealthy domestic animals in field suspected for various hemoparasitic infections was carried out for the presence of T. evansi by microscopy, RoTat1.2 VSG PCR, and LAMP assay. LAMP could detect T. evansi in 36 samples, while PCR and microscopy could detect 33 and 12 samples, respectively. All the samples positive by microscopy and PCR were also confirmed positive by the LAMP assay. The current LAMP assay has appealing point of care characteristics to visually monitor the results, lessen the need of post DNA amplification procedure, and enable this method to be applied as a rapid and sensitive molecular diagnostic tool in under resourced laboratories and field setup.

Published
2020

23. Clinical study and some molecular features of Mexican patients with syndromic craniosynostosis

Author

Angélica Olivo-Díaz, Mirza Romero-Valdovinos, Manuel Almaraz-Salinas, Laura Flores-Peña, Víctor Martínez-Rosas, Aurora Ibarra-Arce, and Gabriela Ortiz de Zarate-Alarcón

Subjects
0301 basic medicine, musculoskeletal diseases, Adult, Male, congenital, hereditary, and neonatal diseases and abnormalities, lcsh:QH426-470, Mutation, Missense, TWIST1, 030105 genetics & heredity, Syndromic craniosynostosis, Craniosynostosis, Clinical study, 03 medical and health sciences, Craniosynostoses, Gene Frequency, Genetics, Medicine, Humans, Restriction enzyme digestion, Hypertelorism, Child, Molecular Biology, Mexico, Genetics (clinical), integumentary system, business.industry, genetic variants, FGFR genes, Twist-Related Protein 1, Genetic variants, Infant, Nuclear Proteins, Original Articles, medicine.disease, Receptors, Fibroblast Growth Factor, Mexican population, eye diseases, Midface hypoplasia, lcsh:Genetics, stomatognathic diseases, craniosynostosis, 030104 developmental biology, Phenotype, Child, Preschool, Original Article, Female, medicine.symptom, business
Abstract

Background Craniosynostosis is one of the major genetic disorders affecting 1 in 2,100–2,500 live newborn children. Environmental and genetic factors are involved in the manifestation of this disease. The suggested genetic causes of craniosynostosis are pathogenic variants in FGFR1, FGFR2, FGFR3, and TWIST1 genes. Methods In order to describe their major clinical characteristics and the presence of pathogenic variants, a sample of 36 Mexican patients with craniosynostosis diagnosed as: Crouzon (OMIM 123,500), Pfeiffer (OMIM 101,600), Apert (OMIM 101,200), Saethre‐Chotzen (OMIM 101,400), and Muenke (OMIM 602,849) was analyzed. Results In addition to craniosynostosis, most of the patients presented hypertelorism, midface hypoplasia, and abnormalities in hands and feet. To detect the pathogenic variants p.Pro252Arg FGFR1 (OMIM 136,350), p.Ser252Trp, p.Pro253Arg FGFR2 (OMIM 176,943), p.Pro250Arg, FGFR3 (OMIM 134,934), and p.Gln119Pro TWIST1 (OMIM 601,622), PCR amplification and restriction enzyme digestion were performed. Four and two patients with Apert presented the pathogenic variants p.Ser252Trp and p.Pro253Arg in FGFR2, respectively (with a frequency of 11.1% and 5.5%). The p.Pro250Arg pathogenic variant of FGFR3 was found in a patient with Muenke (with a frequency of 2.8%). The above percentages were calculated with the total number of patients. Conclusion The contribution of this work is discreet, since only 4 genes were analyzed and sample size is small. However, this strategy could be improved by sequencing the FGFR1, FGFR2, FGFR3, and TWIST1 genes, to determine different pathogenic variants. On the other hand, it would be important to include other genes, such as TCF12 (OMIM 600,480), MSX2 (OMIM 123,101), RAB23 (OMIM 606,144), and EFNB1 (OMIM 300,035), to determine their participation in craniosynostosis in the Mexican population., We describe the major clinical characteristics of Mexican patients with craniosynostosis. Analysis of FGFR1, FGFR2, FGFR3, and TWIST1 genes revealed a higher frequency of variants in Apert.

Published
2020

24. A single-molecule counting approach for convenient and ultrasensitive measurement of restriction digest efficiencies

Author

Kanako Kurosawa, Daisuke Nishiura, Miho Hirai, Shigeru Deguchi, Yi Zhang, Chieko Ishiwata, Takuro Nunoura, and Shigeru Shimamura

Subjects
Gel electrophoresis of nucleic acids, Science, Electrophoretic techniques, DNA electrophoresis, Artificial Gene Amplification and Extension, Computational biology, Biochemistry, Polymerase Chain Reaction, Restriction Enzyme Digestion, chemistry.chemical_compound, Genetics, Molecular Biology Techniques, Molecular Biology, Gel Electrophoresis, Enzyme Kinetics, DNA cleavage, Multidisciplinary, Cell-Free System, Biology and life sciences, Absolute number, Chemistry, Proteins, Marker Genes, Single molecule counting, DNA, DNA Restriction Enzymes, Single Molecule Imaging, Enzymes, Genetic Materials, Nucleic acids, Research and analysis methods, Restriction enzyme, Microscopy, Fluorescence, Enzymology, Medicine, Trace analysis, Restriction digest, CRISPR-Cas Systems, Genetic Engineering, Enzymatic Digestion Techniques, Research Article
Abstract

Restriction endonucleases play a central role in the microbial immune system against viruses and are widely used in DNA specific cleavage, which is called restriction digestion, for genetic engineering. Herein, we applied digital cell-free protein synthesis as an easy-to-use orthogonal readout means to assess the restriction digest efficiency, a new application of digital bioassays. The digital counting principle enabled an unprecedentedly sensitive trace analysis of undigested DNA at the single-molecule level in a PCR-free manner. Our approach can quantify the template DNA of much lower concentrations that cannot be detected by ensemble-based methods such as gold-standard DNA electrophoresis techniques. The sensitive and quantitative measurements revealed a considerable variation in the digest efficiency among restriction endonucleases, from less than 70% to more than 99%. Intriguingly, none of them showed truly complete digestion within reasonably long periods of reaction time. The same rationale was extended to a multiplexed assay and applicable to any DNA-degrading or genome-editing enzymes. The enzyme kinetic parameters and the flanking sequence-dependent digest efficiency can also be interrogated with the proposed digital counting method. The absolute number of residual intact DNA molecules per microliter was concluded to be at least 107, drawing attention to the residual issue of genetic materials associated with the interpretation of nucleases’ behaviors and functions in daily genetic engineering experiments.

Published
2020

25. Prevalence of the Pfdhfr and Pfdhps mutations among asymptomatic pregnant women in Southeast Nigeria

Author

Costanza Tacoli, Michael Pritsch, Thomas Loescher, Nicole Berens-Riha, Martin M Meremikwu, Prabhanjan P. Gai, and Ekpereonne Esu

Subjects
Adult, 0301 basic medicine, medicine.medical_specialty, Genotype, Plasmodium falciparum, 030231 tropical medicine, 030106 microbiology, Protozoan Proteins, Nigeria, DHPS, Biology, Polymerase Chain Reaction, Asymptomatic, Antimalarials, 03 medical and health sciences, 0302 clinical medicine, Medical microbiology, Mutation Rate, Pregnancy, Internal medicine, Sulfadoxine, parasitic diseases, medicine, Humans, Malaria, Falciparum, Restriction enzyme digestion, Polymorphism, Genetic, General Veterinary, General Medicine, medicine.disease, biology.organism_classification, Dried blood spot, Drug Combinations, Tetrahydrofolate Dehydrogenase, Pyrimethamine, Infectious Diseases, Pregnancy Complications, Parasitic, Insect Science, Mutation, Female, Parasitology, medicine.symptom, Nested polymerase chain reaction, Malaria
Abstract

Sulfadoxine-pyrimethamine (SP) is the recommended drug for intermittent preventive treatment of malaria in pregnancy in most of sub-Saharan Africa. Resistance to SP is related to mutations in the dhfr and dhps gene of Plasmodium falciparum. This study determined the prevalence of Pfdhfr and Pfdhps polymorphisms found in asymptomatic pregnant women attending antenatal care in Calabar, Nigeria. From October 2013 to November 2014, asymptomatic pregnant women attending antenatal care clinics were enrolled after obtaining informed consent. Malaria diagnosis testing was done using thick and thin smears. Dried blood spot filter papers were collected. Parasite DNA was extracted from the filter papers using a chelex extraction. Extraction was followed by nested PCR and restriction enzyme digestion. P. falciparum infection was detected by microscopy in 7% (32/459) participants. Twenty-eight P. falciparum isolates were successfully genotyped. In the Pfdhfr gene, the triple mutation was almost fixed; S108N mutation was (100%), N51I (93%) and C59R mutations (93%), whereas the I164L mutation was absent. The prevalence of Pfdhps S436A, A437G, A581G and A613S mutations was 82.1% (23/28), 96.4% (27/28), 71.4% (20/28) and 71.4% (20/28) respectively. The K540E mutation was absent. The prevalence of the Pfdhfr triple mutation IRNI was 92.9% (26/28). The efficacy of SP as IPTp in Southeast Nigeria may be severely threatened. The continuous monitoring of SP molecular markers of resistance is required to assess thresholds. The evaluation of alternative preventive treatment strategies and drug options for preventing malaria in pregnancy may be necessary.

Published
2018

26. A Novel Assay Coupling Dephosphorylation and Blue/White Colony Screening for the G > A Hotspot Mutation at Codon 13 of KRAS Gene

Author

Weijun Cai, Zifen Guo, Yu-Fang Yin, Dixian Luo, Kai Li, Wanping Sun, Cuilan Zhou, Li Xiao, Wangyang Pu, Cuiying Peng, Chungen Xing, Xuan Liu, Huifen Xu, Fenjiao Wang, Nongyue He, and Duanfang Liao

Subjects
Materials science, Point mutation, Biomedical Engineering, Bioengineering, General Chemistry, Condensed Matter Physics, medicine.disease_cause, Molecular biology, Dephosphorylation, DNA Mutational Analysis, Hotspot mutation, medicine, General Materials Science, Restriction digest, KRAS, Restriction enzyme digestion, Gene
Abstract

Development of sensitive assay for detection of hotspot mutations of cancer driving gene is crucial for circulating tumor DNA analysis. This study tested the possibilities of applying restriction enzyme digestion and dephosphorylation coupled with blue/white screening technology for analyzing a hotspot point mutation in codon 13 of KRAS gene. The present study has documented that the combination of PCR with restriction digestion, dephosphorylation, blue/white screening and Sanger's sequencing can identify rare mutations with sensitivities at 0.003%. This novel assay with high sensitivity may have application in the diagnosis of early cancer targeting ctDNAs.

Published
2018

27. A rapid qualitative molecular method for the identification of Colletotrichum acutatum and C. gloeosporioides.

Author

Liu, Bo, Louws, Frank, Sutton, Turner, and Correll, James

Abstract

Identification of the causal agent for anthracnose caused by C. acutatum and C. gloeosporioides based on morphological and cultural criteria is problematic as both are morphologically and genetically diverse. To evaluate a qualitative molecular method to readily distinguish between these two species, Restriction fragment length polymorphisms (RFLP) of a 1-kb intron of the glutamine synthetase (GS) gene was evaluated utilizing representative isolates from a world-wide collection. Unique band patterns of the 1-kb GS intron were obtained for C. acutatum (two fragments with 600 and 350 bp) and C. gloeosporioides (four fragments with 238-340, 252-254, 204, and 108-116 bp) based on PstI enzyme digestion of the amplified PCR product. These data were also confirmed by PstI digestion of the intron DNA sequences using BioEdit software. The identification based on RFLPs of the 1-kb GS intron was consistent with the identification based on previously evaluated species-specific primers (CaInt2 and CgInt). In addition, both species can be differentiated by multiplex PCR. CaInt2, CgInt and ITS4 in one PCR will distinguish between C. acutatum and C. gloeosporioides by differences in PCR product fragment size: 490 bp and 470 bp, respectively. Also, a rapid DNA extraction method was developed, which reduced the time for DNA extraction from two hours to five minutes. In summary, RFLP of the 1-kb GS intron is a reliable technique for identification and differentiation between both species, does not require a sequencing step, and may be useful to diagnostic clinics in helping to make disease management recommendations. [ABSTRACT FROM AUTHOR]

Published
2012
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28. Identification of seven species of hymenopteran parasitoids of Spodoptera frugiperda, using polymerase chain reaction amplification and restriction enzyme digestion.

Author

Jourdie, Violaine, Alvarez, Nadir, and Turlings, Ted C. J.

Subjects
*FALL armyworm, *LARVAE, *PARASITIC wasps, *BIOLOGICAL pest control, *LEPIDOPTERA, *POLYMERASE chain reaction, *DNA restriction enzymes
Abstract

1 The fall armyworm Spodoptera frugiperda is a voracious pest of numerous crops of economic importance throughout the New World. In its native Mexico, larvae can be attacked by several species of parasitic wasps, which are candidate biological control agents against this and other lepidopteran pests. 2 We attempted to survey the parasitoid fauna on S. frugiperda in maize and sorghum fields throughout Mexico. However, our efforts have been hampered by the incomplete development of parasitoid larvae emerging from collected Spodoptera caterpillars. 3 This problem was solved by developing a method to identify seven species of parasitic wasps using polymerase chain reaction amplification and restriction enzyme digestion. This enables the precise determination of the species of those parasitoid larvae that are usually not morphologically identifiable. [ABSTRACT FROM AUTHOR]

Published
2008
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29. Genotyping‐by‐Sequencing

Author

Jason G. Wallace and Sharon E. Mitchell

Subjects
0301 basic medicine, Genotyping by sequencing, General Medicine, Computational biology, Biology, DNA sequencing, 03 medical and health sciences, chemistry.chemical_compound, Restriction enzyme, 030104 developmental biology, 0302 clinical medicine, chemistry, Genotype, Restriction enzyme digestion, Genotyping, 030217 neurology & neurosurgery, DNA
Abstract

Genotyping-by-sequencing (GBS) refers to a suite of related methods that obtain genotype data from samples by using restriction enzyme digestion followed by high-throughput sequencing. GBS is a refinement of restriction site-associated DNA sequencing (RADseq) methods, with a goal of being able to perform library preparations quickly, cost-effectively, and in a high-throughput manner. This protocol contains the steps necessary to go from purified DNA to Illumina-ready libraries. It also covers the considerations that go into planning a GBS experiment. © 2017 by John Wiley & Sons, Inc.

Published
2017

30. Development of 10 novel SNP-RFLP markers for quick genotyping within the black-capped (Poecile atricapillus) and Carolina (P. carolinensis) chickadee hybrid zone

Author

Scott A. Taylor, Alex Van Huynh, Amber M. Rice, and Michael A. McQuillan

Subjects
0106 biological sciences, 0301 basic medicine, biology, Ecology, Biodiversity, biology.organism_classification, 010603 evolutionary biology, 01 natural sciences, Chickadee, 03 medical and health sciences, 030104 developmental biology, Hybrid zone, Evolutionary biology, Poecile, Genetics, SNP, Restriction enzyme digestion, Restriction fragment length polymorphism, Genotyping, Ecology, Evolution, Behavior and Systematics
Abstract

As species ranges shift due to anthropogenic change, accurate detection of hybridization between species will become increasingly important for conservation biologists. The black-capped (Poecile atricapillus) and Carolina (Poecile carolinensis) chickadee hybrid zone is difficult to study because the parental species possess similar morphologies and song is an unreliable species identifier. Further, the hybrid zone is moving northward rapidly due to environmental change. Here, we present 10 single nucleotide polymorphism markers developed from black-capped and Carolina chickadee transcriptome sequences. This marker set coupled with species-specific restriction enzyme digestion allows fast, easy genotyping of pure species and hybrid individuals within the hybrid zone.

Published
2017

31. Prevalence and molecular characteristics of fowladenovirus serotype 4 in eastern Saudi Arabia

Author

Maged Gomaa Hemida and Mohamed Al-Hammadi

Subjects
0301 basic medicine, Genetics, Serotype, General Veterinary, 040301 veterinary sciences, 04 agricultural and veterinary sciences, Biology, Hexon gene, Virology, law.invention, 0403 veterinary science, 03 medical and health sciences, 030104 developmental biology, law, Fowl adenovirus, Restriction enzyme digestion, Polymerase chain reaction
Published
2017

32. A Simple Extraction Method Suitable for PCR-Based Analysis of Plant, Fungal, and Bacterial DNA.

Author

Mahuku, George S.

Subjects
*DNA, *MICROORGANISMS, *PLANTS, *POLYSACCHARIDES, *CHLOROFORM
Abstract

A simple and easy protocol for extracting high-quality DNA from microorganisms and plants is presented. The method involves inactivating proteins by using SDS/proteinase K and precipitating polysaccharides in the presence of high salt. Further purification is based on differential solubility of DNA and high-molecular-weight polysaccharides in aqueous media. The procedure does not use the toxic and potentially hazardous phenol and chloroform, and as many as 100 samples can be processed per day. Absorbency ratios (A260/A280) of 1.6-2.0 indicated a minimal presence of contaminating metabolites. The DNA was completely digested with 5 restriction enzymes: EcoR I, Rsa I, Taq I, EcoR V, and Hind III. PCR analysis using enterobacterial repetitive intergenic consensus (ERIC) sequence, sequence-characterized amplified region (SCAR), and random amplified microsatellite (RAMS) primers showed the DNA's compatibility with downstream applications. This procedure is applicable to a range of pathogens and plants and thus may find wide application in quarantine services and marker-assisted selection (MAS) breeding. [ABSTRACT FROM AUTHOR]

Published
2004
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33. Errors in ABO typing of blood stains using PCR.

Author

Ringel, P. F., Weiler, G., and Bein, G.

Abstract

Genotypes of the ABO blood group system were investigated using a multiplex PCR and subsequent restriction enzyme digestion on experimental blood stains. Differences were found when typing blood between the PCR and serological methods and one blood sample, typed as B with the agglutination test was classified as AB using the method described here. The subsequent sequencing procedure revealed the genotype to be BB. Methodological causes for errors in typing which should be taken into consideration are discussed. [ABSTRACT FROM AUTHOR]

Published
2000
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34. Detection of Human Herpesvirus 6 Variant A in Peripheral Blood Mononuclear Cells from Multiple Sclerosis Patients.

Author

Kim, Joong-Seok, Lee, Kwang-Soo, Park, Ji-Hyun, Kim, Mi-Young, and Shin, Wan-Sik

Subjects
*HUMAN herpesvirus-6, *HERPESVIRUSES, *MULTIPLE sclerosis, *POLYMERASE chain reaction, *DNA restriction enzymes
Abstract

Several authors report that human herpesvirus 6 (HHV-6) variants have different epidemiologies, in vivo tropism and pathogenic potentials. However, it is not well known what pathogenic roles its neurotropism might have in the variant type. As some active plaques of multiple sclerosis (MS) brain tissue harbor HHV-6 DNA divergent from the prototype virus, the possibility that the variant strain may play a role in the pathogenesis of MS has been suggested. Therefore, we tried to investigate the role of HHV-6 variants in the pathogenesis of MS. As HHV-6 is predominantly a T-cell-tropic virus, we examined HHV-6 DNA sequences in peripheral blood mononuclear cells (PBMC) from 34 MS patients, 6 with idiopathic transverse myelitis, 2 with optic neuritis and 20 healthy controls. Nested polymerase chain reaction was used to detect the HHV-6 genome. To discern HHV-6 variants A and B, amplification products were digested by restriction enzyme. We found that 7 of 34 MS patients and 2 of 6 patients with idiopathic transverse myelitis had the HHV-6 genome. On the contrary, there was no HHV-6 genome in the control group. All genomic sequences were of HHV-6 variant A (HHV-6A). Our results suggest that the detection of HHV-6A in the PBMC of patients with MS may raise the possibility of a relationship between latent HHV-6A infection and the pathogenesis of MS.Copyright © 2000 S. Karger AG, Basel [ABSTRACT FROM AUTHOR]

Published
2000
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35. Analysis of polyclonal vector integration sites using Nanopore sequencing as a scalable, cost-effective platform

Author

Ping Zhang, Lachlan J. M. Coin, Son Hoang Nguyen, Devika Ganesamoorthy, Siok-Keen Tey, and Raymond Au

Subjects
0303 health sciences, biology, Inverse polymerase chain reaction, Computational biology, Vector integration, 03 medical and health sciences, 0302 clinical medicine, Polyclonal antibodies, 030220 oncology & carcinogenesis, biology.protein, Nanopore sequencing, Vector (molecular biology), Restriction enzyme digestion, 030304 developmental biology
Abstract

Vector integration site analysis can be important in the follow-up of patients who received gene-modified cells, but current platforms based on next-generation sequencing are expensive and relatively inaccessible. We analyzed polyclonal T cells transduced by a gammaretroviral vector, SFG.iCasp9.2A.ΔCD19, from a clinical trial. Following restriction enzyme digestion, the unknown flanking genomic sequences were amplified by inverse polymerase chain reaction (PCR) or cassette ligation PCR. Nanopore sequencing could identify thousands of unique integration sites within polyclonal samples, with cassette ligation PCR showing less bias. The assay is scalable and requires minimum capital, which together enable cost-effective and timely analysis.

Published
2019
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37. An Efficient Approach for Two Distal Point Site-Directed Mutagenesis from Randomly Ligated PCR Products

Author

Bagher Yakhchali, Ali Asghar Karkhane, Mohammad Hossein Sangtarash, and Jafar Khezri

Subjects
0106 biological sciences, Pcr cloning, Genetic Vectors, Mutagenesis (molecular biology technique), Bioengineering, Computational biology, Biology, 01 natural sciences, Applied Microbiology and Biotechnology, Biochemistry, Polymerase Chain Reaction, law.invention, chemistry.chemical_compound, Plasmid Vector, law, 010608 biotechnology, Restriction enzyme digestion, Cloning, Molecular, Site-directed mutagenesis, Molecular Biology, Polymerase chain reaction, DNA Primers, 010405 organic chemistry, General Medicine, 0104 chemical sciences, chemistry, Mutagenesis, Site-Directed, Ligation, DNA, Biotechnology
Abstract

Site-directed mutagenesis is one of the most important tools in molecular biology. The majority of the mutagenesis methods have been developed to mutate one region of target DNA in each cycle of mutagenesis, while in some cases there is a need to mutate several distal points. We used a new method to simultaneously mutate two distal points in the target DNA. Different regions of the target DNA were amplified in three separate PCR reactions. The PCR products were back-to-back and together they made the complete length of the template DNA. Mutations were introduced to PCR products by middle mutagenic primers. PCR products were mixed and ligated with random blunt ligation, and then the desired mutated DNA fragments were selected in two steps by flanking restriction enzyme digestion and size selection. Selected fragments were amplified in another PCR reaction using flanking primers and finally cloned into the plasmid vector. This mutagenesis process is simple, there is no need to use modified primers and long or difficult PCR reactions.

Published
2019

38. An improved simple method for DNA extraction from fungal mycelia

Author

Jie Feng, Yalong Yang, and Krista Zuzak

Subjects
0106 biological sciences, 0301 basic medicine, Chromatography, fungi, Extraction (chemistry), Single sample, Plant Science, Biology, 01 natural sciences, DNA extraction, Microbiology, 03 medical and health sciences, chemistry.chemical_compound, genomic DNA, 030104 developmental biology, chemistry, Restriction enzyme digestion, Alkaline lysis, Agronomy and Crop Science, DNA, Mycelium, 010606 plant biology & botany
Abstract

A simple and inexpensive method for extraction of genomic DNA from mycelia of filamentous fungi was developed and the standardization of the protocol is described. The protocol includes both mycelium culturing and DNA extraction. By incorporating a selected commercial sand product into the culture media, the collection and the grinding of mycelia was simple and quick. The protocol of DNA extraction was derived from the alkaline lysis method for plasmid DNA extraction and modified to facilitate efficient extraction of fungal genomic DNA. It has increased efficiency and fidelity compared to the other simple DNA extraction protocols. Relative to a commonly used commercial DNA extraction kit, this extraction protocol is faster, easier and can generate more DNA without compromising quality. From a single sample of mycelium, genomic DNA can be prepared within 20 min, including concentration measurement. The DNA can be used in restriction enzyme digestion and as a template in PCR to amplify DNA fragments...

Published
2016

39. Extrachromosomal DNA of pea-root ( Pisum sativum) has repeated sequences and ribosomal genes.

Author

Kraszewska, E., Bjerknes, C., Lamm, S., and 't Hof, J.

Abstract

Restriction endonuclease digestion and Southern blotting procedure were used to determine differences between extrachromosomal, nuclear, plastid, and mitochondrial DNAs from meristematic cells of cultured pea roots. Extrachromosomal and nuclear DNA are highly methylated and neither DNA is homologous to plastid or mitochondrial DNA. Hybridization of extrachromosomal DNA to nuclear DNA indicated that extrachromosomal DNA differed quantitatively from total nuclear DNA in repetitive sequences. Cloned rDNA showed that extrachromosomal DNA contains rRNA genes but the hybridization signal indicated that the copy number was less than that expected if the molecules were amplified. These and cytological findings suggest that extrachromosomal DNA is involved in or a product of genomic changes associated with the onset of differentiation by precursor cells of vascular parenchyma and the root cap. [ABSTRACT FROM AUTHOR]

Published
1985
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40. Cloning of Mouse β-actin Gene

Author

Mingli Wang, Chengjun Ji, and Xuedong Wen

Subjects
Cloning, β actin gene, Chemistry, Gene expression, RNA, General Materials Science, macromolecular substances, Restriction enzyme digestion, Gene, Molecular biology, Actin, Nuclear DNA
Abstract

β-actin gene is a kind of actin, in a variety of cells and tissues, β-actin gene expression is relatively stable [1], and β-actin gene in nuclear DNA has multiple copies, increased The detection rate of nuclear DNA [2], which is often used as an internal reference in PCR. In this experiment, the β-actin gene with good purity was obtained by PT-PCR, amplification, cloning, screening and PCR identification and restriction enzyme digestion of the RNA extracted from the mouse liver, which laid the foundation for the later experiment.

Published
2018

41. Isolation and Characterization of T7-Like Lytic Bacteriophages Infecting Multidrug Resistant Pseudomonas aeruginosa Isolated from Egypt

Author

Ahmed Askora, Gamal El Didamony, and Aya A. Shehata

Subjects
Restriction Mapping, Applied Microbiology and Biotechnology, Microbiology, Podoviridae, Bacteriolysis, Multiplicity of infection, Microscopy, Electron, Transmission, Drug Resistance, Multiple, Bacterial, Restriction enzyme digestion, Sewage, biology, Short tail, Virion, Multidrug resistant Pseudomonas aeruginosa, Genetic Variation, General Medicine, biology.organism_classification, Isolation (microbiology), Lytic cycle, DNA, Viral, Pseudomonas aeruginosa, Egypt, Pseudomonas Phages, Bacteria
Abstract

In this study, two lytic phages designated as ϕPSZ1 and ϕPSZ2 infecting multidrug resistant Pseudomonas aeruginosa were isolated from sewage samples collected in Zagazig, Egypt. Morphological analysis by transmission electron microscopy revealed that both phages belong to the podoviridae family and resembles typical T7-like phages. ϕPSZ1 has a head of about 60 ± 5 nm in diameter with a short tail of 19 ± 2 nm in length, while ϕPSZ2 has a head of about 57 ± 5 nm in diameter with a short tail of 14 ± 2 nm in length. Both phages were shown to be able to infect 13 different P. aeruginosa strains and has no effect on other tested bacteria. In spite of morphological similarity, these phages showed diverged genomic sequences revealed by restriction enzyme digestion analysis. One-step growth curves of bacteriophages revealed eclipse and latent periods of 12 min for ϕPSZ1 and 15 min for ϕPSZ2, respectively, with burst sizes of about 100 per infected cell. Phage treatment prevented the growth of P. aeruginosa for up to 18 h with multiplicity of infection ratios of 1. These results suggest that both phages have a high potential for phage application to control P. aeruginosa.

Published
2015

42. Plasmonic Photothermal Gold Bipyramid Nanoreactors for Ultrafast Real-Time Bioassays

Author

Bozhi Tian, Yossi Weizmann, Timothy M. Cronin, Zoya Cheglakov, Kyle J. Gibson, Jung-Hoon Lee, and Jaeseok Yi

Subjects
Chemistry, technology, industry, and agriculture, Nanotechnology, 02 engineering and technology, General Chemistry, Nucleic acid amplification technique, Nanoreactor, Photothermal therapy, 010402 general chemistry, 021001 nanoscience & nanotechnology, 01 natural sciences, Biochemistry, Catalysis, 0104 chemical sciences, Bipyramid, Colloid and Surface Chemistry, Nucleic acid, Restriction enzyme digestion, 0210 nano-technology, Ultrashort pulse, Plasmon
Abstract

Nucleic acid amplification techniques have been among the most powerful tools for biological and biomedical research, and the vast majority of the bioassays rely on thermocycling that uses time-consuming and expensive Peltier-block heating. Here, we introduce a plasmonic photothermal method for quantitative real-time PCR, using gold bipyramids and light to achieve ultrafast thermocycling. Moreover, we successfully extend our photothermal system to other biological assays, such as isothermal nucleic acid amplification and restriction enzyme digestion.

Published
2017

43. Restriction Digestion Method for Haplotyping the Potato Psyllid,Bactericera Cockerelli

Author

Kylie D. Swisher and James M. Crosslin

Subjects
Mitochondrial DNA, Bactericera cockerelli, Ecology, biology, business.industry, fungi, Haplotype, food and beverages, Computational biology, Ribosomal RNA, biology.organism_classification, Biotechnology, Insect Science, Small subunit, Restriction digest, PEST analysis, Restriction enzyme digestion, business, Agronomy and Crop Science
Abstract

A restriction digestion method has been developed for haplotyping the potato psyllid, Bactericera cockerelli Sulc., an economically important pest of solanaceous crops. This method differentiates the four known potato psyllid haplotypes by using restriction enzyme digestion of a portion of the mitochondrial large subunit ribosomal RNA, tRNA-Val, and a portion of the small subunit ribosomal RNA, providing a second target within the mitochondrial DNA for haplotyping studies. This technique also provides a good alternative to the current method of potato psyllid haplotyping which uses high-resolution melting analysis, a technique that requires access to a real-time PCR machine with high-resolution melting capabilities. Potato psyllid haplotyping by restriction digestion is done using basic laboratory equipment that is readily available for smaller laboratories with budgetary limitations, thereby providing an excellent tool for laboratories of all sizes to identify psyllid populations.

Published
2014

44. Molecular characterization and evaluation of the emerging antibiotic-resistant Streptococcus pyogenes from eastern India

Author

Sukanta Sinha, Dipanwita Ray, Nishith Kumar Pal, Somnath Saha, and Basudev Bhattacharya

Subjects
DNA, Bacterial, 0301 basic medicine, Genotype, Streptococcus pyogenes, Tetracycline, Antibiotic sensitivity, 030106 microbiology, Exotoxins, India, Antibiotic sensitivity patterns, Biology, medicine.disease_cause, Streptococcus pyogenes (GAS), HaeIII, Microbiology, 03 medical and health sciences, 0302 clinical medicine, Antibiotic resistance, Bacterial Proteins, Exotoxin gene, Streptococcal Infections, Drug Resistance, Bacterial, medicine, Humans, Restriction enzyme digestion, 030212 general & internal medicine, Typing, vir typing, Anti-Bacterial Agents, Erythromycin, Molecular Typing, Infectious Diseases, emm typing, Virulence regulon, bacteria, Restriction fragment length polymorphism, Polymorphism, Restriction Fragment Length, Research Article, medicine.drug
Abstract

Background Group A Streptococcus strains causing wide variety of diseases, recently became noticeable in eastern India, are not amenable to standard treatment protocol thus enhancing the possibility of disease morbidity by becoming antibiotic resistance. Methods The association of Lancefield group A Streptococcal variation with degree of vir architectural diversity was evaluated using emm typing and restriction fragment length polymorphism analyses. The antibiotic sensitivity patterns were examined by modified Kirby-Bauer method of disk diffusion. Percentage calculations, 95% confidence interval and one-way ANOVA were used to assess differences in proportions. Results Our observations revealed 20 different emm types and 13 different HaeIII vir typing patterns. A 1.2 kb fragment was found in all HaeIII typing pattern. Fragments of 1.2 kb and 550 bp were conserved in majority of the isolates. HinfI digestion was found proficient in differentiating the strains of same vir typing patterns. Strong predominance of speC (85%) and speF (80%) genes have been observed encoding exotoxins production. 4 isolates were found to be erythromycin resistant and were of genotype emm49. High degree of tetracycline resistance was shown by 53.57% isolates which belonged to 12 different emm genotypes. Conclusions These findings suggested that in addition to emm typing, sequential application of HaeIII and HinfI restriction enzymes in vir typing analysis is an effective tool for group A streptococcal molecular characterization associated with antibiotic resistance. Electronic supplementary material The online version of this article (doi:10.1186/s12879-016-2079-9) contains supplementary material, which is available to authorized users.

Published
2016

45. Molecular approach for analysis of in situ feeding by the dinoflagellate Noctiluca scintillans.

Author

Nishitani, Goh, Shiromoto, Masaomi, Sato-Okoshi, Waka, and Ishikawa, Akira

Subjects
*DINOFLAGELLATES, *GYMNODINIUM, *CHRYSOPHYTES, *RED tide, *POLYMERASE chain reaction, *GREEN algae, *NUCLEOTIDE sequence, *DIATOMS
Abstract

• The red tide forming species noctiluca scintillans is a marine heterotrophic dinoflagellate. • We analyzed the prey organisms within natural cells of N. scintillans using two genetic methods. • Restriction enzyme digestion and blocking primer methods were applied. • DNA sequences of surprisingly diverse taxa were obtained from the natural cells of N. scintillans. • Molecular prey analyses may reveal undiscovered interactions within the plankton community. The red tide forming heterotrophic dinoflagellate Noctiluca scintillans is common in temperate to tropical waters around the world. Understanding the in situ prey of N. scintillans is essential for elucidating its role in marine microbial food webs. In this study, we applied two polymerase chain reaction (PCR)-based cloning techniques, a predator-specific restriction enzyme, and a blocking primer. The PCR of nuclear 18S rDNA was performed on single N. scintillans cells that were collected from Ishinomaki Bay, Japan, in May 2018. The maximum detection rates of non- Noctiluca sequences were 56% using the restriction enzyme method and 87% with the blocking primer method, representing a broad taxonomic range of organisms, including diatom, dinoflagellate, bolidophyte, haptophyte, euglenophyte, green algae, golden algae, ciliate, heliozoa, copepod, brown seaweed, sponge, bivalve, and polychaete. The diverse DNA was probably ingested by N. scintillans directly or indirectly through secondary predation or ingestion of marine snow or detritus containing many organisms. The application of molecular approaches to various species may reveal undiscovered interactions within the phytoplankton community, including prey-predator, or symbiotic relationships. [ABSTRACT FROM AUTHOR]

Published
2020
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46. Construction of a Full-Length 3'UTR Reporter System for Identification of Cell-Cycle Regulating MicroRNAs.

Author

Kaźmierczak D and Hydbring P

Subjects
Binding Sites, Cell Cycle, Cell Cycle Proteins chemistry, Cell Line, Genes, Reporter, Humans, RNA, Messenger chemistry, RNA, Messenger genetics, 3' Untranslated Regions, Cell Cycle Proteins genetics, Luciferases genetics, MicroRNAs analysis
Abstract

Three prime untranslated region (3'UTR) reporter constructs are widely used by the scientific community to functionally link microRNAs (miRNAs) to suppression of mRNA expression. However, full-length 3'UTR vectors are rarely employed due to labor-intensive cloning work. Instead, 3'UTR fragments containing putative miRNA binding sites are commonly utilized to mechanistically validate miRNAs. Assaying truncated 3'UTRs may falsely validate miRNAs due to altered positioning of binding sites in respect to 3'UTR length and RNA secondary structure. Here we present a detailed protocol for the construction of full-length 3'UTR luciferase reporter constructs that was used to unveil miRNAs regulating multiple cell-cycle factors.

Published
2021
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47. Integrated three-dimensional system-on-chip for direct quantitative detection of mitochondrial DNA mutation in affected cells

Author

Gwo-Bin Lee, Yau-Huei Wei, Chen Min Chang, Dar-Bin Shieh, and Li Fang Chiu

Subjects
Genetics, Mitochondrial DNA, DNA Mutational Analysis, Microfluidics, Biomedical Engineering, Biophysics, Micromixer, Equipment Design, General Medicine, Computational biology, Microfluidic Analytical Techniques, Biology, Real-Time Polymerase Chain Reaction, DNA, Mitochondrial, chemistry.chemical_compound, chemistry, Mutation (genetic algorithm), Electrochemistry, Humans, Point Mutation, System on a chip, Restriction enzyme digestion, Mitochondrial mutation, DNA, Biotechnology
Abstract

We report a microfluidic system for automatic mitochondrial mutation diagnostics from sample purification to quantitative analysis. The system achieved direct DNA (mtDNA) mutation quantification in affected cells using a new 3D-microfluidic system, which integrated a mtDNA extraction module and a mutation detection module. Effective direct mtDNA extraction from the cells was realized using magnetic field manipulation. The obtained mtDNAs were subject to a fully automatic processing for quantitative mutation detection using integrated micropumps, micromixer and microtemperature control modules capable of mutation sensing by restriction enzyme digestion and real-time on-chip micro-PCR. Compared with traditional methods, this microfluidic system demonstrates the advantages of faster detection, requirement of fewer amount of specimens and reagents, much compact design and lower cost as well as lower risks for human errors. Thus, such system-on-chip would encourage the future translational development of rapid pathogenic mtDNA defects detection to provide more efficient clinical diagnosis and disease management strategies.

Published
2013

49. Cryptosporidium canis in Two Mexican Toddlers

Author

Isaac Villegas-Gómez, Adriana Garibay-Escobar, Alejandro Urrea-Quezada, Lihua Xiao, María Durazo, Olivia Valenzuela, Mariana González-Díaz, and Jesús Hernández

Subjects
0301 basic medicine, Microbiology (medical), Diarrhea, Fever, Genotype, Sequence analysis, 030106 microbiology, 030231 tropical medicine, Antiprotozoal Agents, Cryptosporidiosis, Cryptosporidium, 18S ribosomal RNA, law.invention, Microbiology, 03 medical and health sciences, 0302 clinical medicine, law, medicine, Humans, Restriction enzyme digestion, Mexico, Polymerase chain reaction, Cryptosporidium canis, biology, business.industry, digestive, oral, and skin physiology, DNA, Protozoan, biology.organism_classification, Infectious Diseases, Canis, Chronic malnutrition, Child, Preschool, Pediatrics, Perinatology and Child Health, medicine.symptom, business, human activities
Abstract

Cryptosporidium canis is reported for the first time in 2 toddlers in Northwestern Mexico. The 2 toddlers (33 and 34 months old) were symptomatic at diagnosis, presenting diarrhea and fever, and 1 case presented chronic malnutrition. Both toddlers were HIV-negative. C. canis was identified by SspI and VspI restriction enzyme digestion of the 18S rRNA polymerase chain reaction products and confirmed by sequence analysis.

Published
2016

50. Genetic polymorphism of growth hormone releasing hormonegene in exotic and crossbred pigs

Author

Soumen Naskar, D. K. Sarma, Purabi Kaushik, Habibur Rahman, and Pratap J. Handique

Subjects
Genetics, medicine.medical_specialty, General Veterinary, North east, Amplicon, Biology, Growth hormone, Growth hormone–releasing hormone, Crossbreed, Exon, Endocrinology, Internal medicine, Genotype, medicine, Animal Science and Zoology, Restriction enzyme digestion
Abstract

Growth hormone releasing hormone (GHRH) plays a central role in growth and production through its influence on important metabolic activities in mammals which prompted its wide commercial use including use as a candidate marker. In present experiment, polymorphism at exon 2 and 3 of Growth Hormone Releasing Hormone gene (GHRH) was studied using PCR–RFLP in crossbred and exotic pigs, commonly found in north east India. Restriction enzyme digestion of 467 bp PCR amplicon with AluI revealed 1 genotype. Comparison of obtained sequences revealed large scale nucleotide and residue substitutions. Observed polymorphism may be associated with wide variability in growth (rate) of different breeds of pig.

Published
2016

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