Your search keyword '"DNA fragment ligation"' showing total 22 results

1. PCR-free whole exome sequencing: Cost-effective and efficient in detecting rare mutations.

Author

Yamaguchi, Izumi, Watanabe, Takashi, Ohara, Osamu, and Hasegawa, Yoshinori

Subjects

*CELL-free DNA, *MOLECULAR biology, *DNA, *MOLECULAR probes, *COMPUTATIONAL biology

Abstract

In this study, we describe the development of a PCR-free whole exome sequencing method. Using this method, 2 μg DNA was sufficient for library preparation for whole exome sequencing. Furthermore, the method is simple and makes use of a commercial kit, with additional step of concentrating the captured library by ethanol precipitation. The accuracy of the PCR-free method was found to be equivalent to that of unique molecular identifier-corrected analysis method, which is the commonly used method to detect rare mutations. Thus, the PCR-free whole exome sequencing method is cost-effective as well as efficient in detecting rare mutations. [ABSTRACT FROM AUTHOR]

Published

2019

2. A simple and dual expression plasmid system in prokaryotic (E. coli) and mammalian cells.

Author

Murakami, Manabu, Ohba, Takayoshi, Murakami, Agnieszka M., Han, Chong, Kuwasako, Kenji, and Itagaki, Shirou

Subjects

*DNA topoisomerase II, *DNA topoisomerase I, *GENE expression, *MOLECULAR biology, *GENE amplification, *PHYSICAL sciences

Abstract

We introduce a simple and universal cloning plasmid system for gene expression in prokaryotic (Escherichia coli) and mammalian cells. This novel system has two expression modes: the (subcloning) prokaryotic and mammalian modes. This system streamlines the process of producing mammalian gene expression plasmids with desired genes. The plasmid (prokaryotic mode) has an efficient selection system for DNA insertion, multiple component genes with rare restriction sites at both ends (termed “units”), and a simple transformation to mammalian expression mode utilizing rare restriction enzymes and re-ligation (deletion step). The new plasmid contains the lac promoter and operator followed by a blunt-end EcoRV recognition site, and a DNA topoisomerase II toxin-originated gene for effective selection with isopropyl-β-D-thiogalactoside (IPTG) induction. This system is highly efficient for the subcloning of blunt-end fragments, including PCR products. After the insertion of the desired gene, protein encoded by the desired gene can be detected in E. coli with IPTG induction. Then, the lac promoter and operator are readily deleted with 8-nucleotide rare-cutter blunt-end enzymes (deletion step). Following re-ligation and transformation, the plasmid is ready for mammalian expression analysis (mammalian mode). This idea (conversion from prokaryotic to mammalian mode) can be widely adapted. The pgMAX system overwhelmingly simplifies prokaryotic and mammalian gene expression analyses. [ABSTRACT FROM AUTHOR]

Published

2019

3. Fragmentation Through Polymerization (FTP): A new method to fragment DNA for next-generation sequencing.

Author

Ignatov, Konstantin B., Blagodatskikh, Konstantin A., Shcherbo, Dmitry S., Kramarova, Tatiana V., Monakhova, Yulia A., and Kramarov, Vladimir M.

Subjects

*NUCLEOTIDE sequence, *NUCLEIC acids, *SINGLE-stranded DNA, *POLYMERIZATION

Abstract

Fragmentation of DNA is the very important first step in preparing nucleic acids for next-generation sequencing. Here we report a novel Fragmentation Through Polymerization (FTP) technique, which is a simple, robust, and low-cost enzymatic method of fragmentation. This method generates double-stranded DNA fragments that are suitable for direct use in NGS library construction and allows the elimination of the additional step of reparation of DNA ends. [ABSTRACT FROM AUTHOR]

Published

2019

4. Novel gateway binary vectors for rapid tripartite DNA assembly and promoter analysis with various reporters and tags in the liverwort Marchantia polymorpha.

Author

Mano, Shoji, Nishihama, Ryuichi, Ishida, Sakiko, Hikino, Kazumi, Kondo, Maki, Nishimura, Mikio, Yamato, Katsuyuki T., Kohchi, Takayuki, and Nakagawa, Tsuyoshi

Subjects

*MARCHANTIA polymorpha, *LIVERWORTS, *MOLECULAR self-assembly, *DNA analysis, *MOLECULAR cloning, *BIOCOMPATIBILITY

Abstract

The liverwort Marchantia polymorpha is an emerging model species for basal lineage plant research. In this study, two Gateway cloning-compatible binary vector series, R4pMpGWB and R4L1pMpGWB, were generated to facilitate production of transgenic M. polymorpha. The R4pMpGWB series allows tripartite recombination of any promoter and any coding sequence with a specific reporter or tag. Reporters/tags for the R4pMpGWB series are GUS, ELuc(PEST), FLAG, 3×HA, 4×Myc, mRFP1, Citrine, mCitrine, ER-targeted mCitrine and nucleus-targeted mCitrine. The R4L1pMpGWB series is suitable for promoter analysis. R4L1pMpGWB vector structure is the same as that of R4pMpGWB vectors, except that the attR2 site is replaced with attL1, enabling bipartite recombination of any promoter with a reporter or tag. Reporters/tags for the R4L1pMpGWB series are GUS, G3GFP-GUS, LUC, ELuc(PEST), Citrine, mCitrine, ER-targeted mCitrine and mCitrine-NLS. Both vector series were functional in M. polymorpha cells. These vectors will facilitate the design and assembly of plasmid constructs and generation of transgenic M. polymorpha. [ABSTRACT FROM AUTHOR]

Published

2018

5. Escherichia coli β-clamp slows down DNA polymerase I dependent nick translation while accelerating ligation.

Author

Bhardwaj, Amit, Ghose, Debarghya, Thakur, Krishan Gopal, and Dutta, Dipak

Subjects

*ESCHERICHIA coli, *DNA polymerases, *RNA, *LIGATION reactions, *NUCLEOTIDES

Abstract

The nick translation property of DNA polymerase I (Pol I) ensures the maturation of Okazaki fragments by removing primer RNAs and facilitating ligation. However, prolonged nick translation traversing downstream DNA is an energy wasting futile process, as Pol I simultaneously polymerizes and depolymerizes at the nick sites utilizing energy-rich dNTPs. Using an in vitro assay system, we demonstrate that the β-clamp of the Escherichia coli replisome strongly inhibits nick translation on the DNA substrate. To do so, β-clamp inhibits the strand displacement activity of Pol I by interfering with the interaction between the finger subdomain of Pol I and the downstream primer-template junction. Conversely, β-clamp stimulates the 5’ exonuclease property of Pol I to cleave single nucleotides or shorter oligonucleotide flaps. This single nucleotide flap removal at high frequency increases the probability of ligation between the upstream and downstream DNA strands at an early phase, terminating nick translation. Besides β-clamp-mediated ligation helps DNA ligase to seal the nick promptly during the maturation of Okazaki fragments. [ABSTRACT FROM AUTHOR]

Published

2018

6. Interference with DNA repair after ionizing radiation by a pyrrole-imidazole polyamide.

Author

Diaz-Perez, Silvia, Kane, Nathanael, Kurmis, Alexis A., Yang, Fei, Kummer, Nicolas T., Dervan, Peter B., and Nickols, Nicholas G.

Subjects

*DNA repair, *POLYAMIDES, *IONIZING radiation, *RNA sequencing, *GEL electrophoresis

Abstract

Pyrrole-imidazole (Py–Im) polyamides are synthetic non-genotoxic minor groove-binding small molecules. We hypothesized that Py–Im polyamides can modulate the cellular response to ionizing radiation. Pre-treatment of cells with a Py-Im polyamide prior to exposure to ionizing radiation resulted in a delay in resolution of phosphorylated γ-H2AX foci, increase in XRCC1 foci, and reduced cellular replication potential. RNA-sequencing of cell lines exposed to the polyamide showed induction of genes related to the ultraviolet radiation response. We observed that the polyamide is almost 10-fold more toxic to a cell line deficient in DNA ligase 3 as compared to the parental cell line. Alkaline single cell gel electrophoresis reveals that the polyamide induces genomic fragmentation in the ligase 3 deficient cell line but not the corresponding parental line. The polyamide interferes directly with DNA ligation in vitro. We conclude that Py-Im polyamides may be further explored as sensitizers to genotoxic therapies. [ABSTRACT FROM AUTHOR]

Published

2018

7. Comparative analysis of the end-joining activity of several DNA ligases.

Author

Bauer, Robert J., Zhelkovsky, Alexander, Bilotti, Katharina, Crowell, Laura E., Jr.Evans, Thomas C., McReynolds, Larry A., and Lohman, Gregory J. S.

Subjects

*DNA ligases, *DNA repair, *DNA-binding proteins, *ZINC-finger proteins, *N-terminal residues

Abstract

DNA ligases catalyze the repair of phosphate backbone breaks in DNA, acting with highest activity on breaks in one strand of duplex DNA. Some DNA ligases have also been observed to ligate two DNA fragments with short complementary overhangs or blunt-ended termini. In this study, several wild-type DNA ligases (phage T3, T4, and T7 DNA ligases, Paramecium bursaria chlorella virus 1 (PBCV1) DNA ligase, human DNA ligase 3, and Escherichia coli DNA ligase) were tested for their ability to ligate DNA fragments with several difficult to ligate end structures (blunt-ended termini, 3′- and 5′- single base overhangs, and 5′-two base overhangs). This analysis revealed that T4 DNA ligase, the most common enzyme utilized for in vitro ligation, had its greatest activity on blunt- and 2-base overhangs, and poorest on 5′-single base overhangs. Other ligases had different substrate specificity: T3 DNA ligase ligated only blunt ends well; PBCV1 DNA ligase joined 3′-single base overhangs and 2-base overhangs effectively with little blunt or 5′- single base overhang activity; and human ligase 3 had highest activity on blunt ends and 5′-single base overhangs. There is no correlation of activity among ligases on blunt DNA ends with their activity on single base overhangs. In addition, DNA binding domains (Sso7d, hLig3 zinc finger, and T4 DNA ligase N-terminal domain) were fused to PBCV1 DNA ligase to explore whether modified binding to DNA would lead to greater activity on these difficult to ligate substrates. These engineered ligases showed both an increased binding affinity for DNA and increased activity, but did not alter the relative substrate preferences of PBCV1 DNA ligase, indicating active site structure plays a role in determining substrate preference. [ABSTRACT FROM AUTHOR]

Published

2017

8. GOTHiC, a probabilistic model to resolve complex biases and to identify real interactions in Hi-C data.

Author

Martincorena, Inigo, Darbo, Elodie, Sugar, Robert, Mifsud, Borbala, Luscombe, Nicholas M., Schoenfelder, Stefan, and Fraser, Peter

Subjects

*CELL nuclei, *DNA, *EXPERIMENTAL design, *THRESHOLD signatures, *LIGATION reactions

Abstract

Hi-C is one of the main methods for investigating spatial co-localisation of DNA in the nucleus. However, the raw sequencing data obtained from Hi-C experiments suffer from large biases and spurious contacts, making it difficult to identify true interactions. Existing methods use complex models to account for biases and do not provide a significance threshold for detecting interactions. Here we introduce a simple binomial probabilistic model that resolves complex biases and distinguishes between true and false interactions. The model corrects biases of known and unknown origin and yields a p-value for each interaction, providing a reliable threshold based on significance. We demonstrate this experimentally by testing the method against a random ligation dataset. Our method outperforms previous methods and provides a statistical framework for further data analysis, such as comparisons of Hi-C interactions between different conditions. GOTHiC is available as a BioConductor package (). [ABSTRACT FROM AUTHOR]

Published

2017

9. CENP-A and H3 Nucleosomes Display a Similar Stability to Force-Mediated Disassembly.

Author

Kim, Sung Hyun, Vlijm, Rifka, van der Torre, Jaco, Dalal, Yamini, and Dekker, Cees

Subjects

*CENTROMERE, *KINETOCHORE, *CHROMATIN, *MITOSIS, *MICROTUBULES, *NUCLEOTIDE sequence

Abstract

Centromere-specific nucleosomes are a central feature of the kinetochore complex during mitosis, in which microtubules exert pulling and pushing forces upon the centromere. CENP-A nucleosomes have been assumed to be structurally unique, thereby providing resilience under tension relative to their H3 canonical counterparts. Here, we directly test this hypothesis by subjecting CENP-A and H3 octameric nucleosomes, assembled on random or on centromeric DNA sequences, to varying amounts of applied force by using single-molecule magnetic tweezers. We monitor individual disassembly events of CENP-A and H3 nucleosomes. Regardless of the DNA sequence, the force-mediated disassembly experiments for CENP-A and H3 nucleosomes demonstrate similar rupture forces, life time residency and disassembly steps. From these experiments, we conclude that CENP-A does not, by itself, contribute unique structural features to the nucleosome that lead to a significant resistance against force-mediated disruption. The data present insights into the mechanistic basis for how CENP-A nucleosomes might contribute to the structural foundation of the centromere in vivo. [ABSTRACT FROM AUTHOR]

Published

2016

10. A Cost-Effective Approach to Sequence Hundreds of Complete Mitochondrial Genomes.

Author

Nunez, Joaquin C. B. and Oleksiak, Marjorie F.

Subjects

*MITOCHONDRIAL DNA, *NUCLEOTIDE sequencing, *DNA primers, *COMPUTATIONAL biology, *COST effectiveness

Abstract

We present a cost-effective approach to sequence whole mitochondrial genomes for hundreds of individuals. Our approach uses small reaction volumes and unmodified (non-phosphorylated) barcoded adaptors to minimize reagent costs. We demonstrate our approach by sequencing 383 Fundulus sp. mitochondrial genomes (192 F. heteroclitus and 191 F. majalis). Prior to sequencing, we amplified the mitochondrial genomes using 4–5 custom-made, overlapping primer pairs, and sequencing was performed on an Illumina HiSeq 2500 platform. After removing low quality and short sequences, 2.9 million and 2.8 million reads were generated for F. heteroclitus and F. majalis respectively. Individual genomes were assembled for each species by mapping barcoded reads to a reference genome. For F. majalis, the reference genome was built de novo. On average, individual consensus sequences had high coverage: 61-fold for F. heteroclitus and 57-fold for F. majalis. The approach discussed in this paper is optimized for sequencing mitochondrial genomes on an Illumina platform. However, with the proper modifications, this approach could be easily applied to other small genomes and sequencing platforms. [ABSTRACT FROM AUTHOR]

Published

2016

11. The Inhibitory Effect of Non-Substrate and Substrate DNA on the Ligation and Self-Adenylylation Reactions Catalyzed by T4 DNA Ligase.

Author

Bauer, Robert J., JrEvans, Thomas C., and Lohman, Gregory J. S.

Subjects

*DNA ligases, *BIOCHEMICAL substrates, *LIGATURE (Surgery), *CATALYSIS, *DNA replication, *DNA repair

Abstract

DNA ligases are essential both to in vivo replication, repair and recombination processes, and in vitro molecular biology protocols. Prior characterization of DNA ligases through gel shift assays has shown the presence of a nick site to be essential for tight binding between the enzyme and its dsDNA substrate, with no interaction evident on dsDNA lacking a nick. In the current study, we observed a significant substrate inhibition effect, as well as the inhibition of both the self-adenylylation and nick-sealing steps of T4 DNA ligase by non-nicked, non-substrate dsDNA. Inhibition by non-substrate DNA was dependent only on the total DNA concentration rather than the structure; with 1 μg/mL of 40-mers, 75-mers, or circular plasmid DNA all inhibiting ligation equally. A >15-fold reduction in T4 DNA ligase self-adenylylation rate when in the presence of high non-nicked dsDNA concentrations was observed. Finally, EMSAs were utilized to demonstrate that non-substrate dsDNA can compete with nicked dsDNA substrates for enzyme binding. Based upon these data, we hypothesize the inhibition of T4 DNA ligase by non-nicked dsDNA is direct evidence for a two-step nick-binding mechanism, with an initial, nick-independent, transient dsDNA-binding event preceding a transition to a stable binding complex in the presence of a nick site. [ABSTRACT FROM AUTHOR]

Published

2016

12. Rapid Synthesis of a Long Double-Stranded Oligonucleotide from a Single-Stranded Nucleotide Using Magnetic Beads and an Oligo Library.

Author

Pengpumkiat, Sumate, Koesdjojo, Myra, Rowley, Erik R., Mockler, Todd C., and Remcho, Vincent T.

Subjects

*OLIGONUCLEOTIDES, *MAGNETIC fields, *DNA analysis, *THERMODYNAMICS, *MACROMOLECULES

Abstract

Chemical synthesis of oligonucleotides is a widely used tool in the field of biochemistry. Several methods for gene synthesis have been introduced in the growing area of genomics. In this paper, a novel method of constructing dsDNA is proposed. Short (28-mer) oligo fragments from a library were assembled through successive annealing and ligation processes, followed by PCR. First, two oligo fragments annealed to form a dsDNA molecule. The double-stranded oligo was immobilized onto magnetic beads (solid support) via streptavidin-biotin binding. Next, single-stranded oligo fragments were added successively through ligation to form the complete DNA molecule. The synthesized DNA was amplified through PCR and gel electrophoresis was used to characterize the product. Sanger sequencing showed that more than 97% of the nucleotides matched the expected sequence. Extending the length of the DNA molecule by adding single-stranded oligonucleotides from a basis set (library) via ligation enables a more convenient and rapid mechanism for the design and synthesis of oligonucleotides on the go. Coupled with an automated dispensing system and libraries of short oligo fragments, this novel DNA synthesis method would offer an efficient and cost-effective method for producing dsDNA. [ABSTRACT FROM AUTHOR]

Published

2016

13. CaBagE: A Cas9-based Background Elimination strategy for targeted, long-read DNA sequencing

Author

Jeff Greenland, Thomas A Sasani, Aaron R. Quinlan, Brent S. Pedersen, Brooke L. Gates, Katherine E. Varley, Jordan Swanier, and Amelia D. Wallace

Subjects

Molecular biology, Genome, Biochemistry, Nanopores, Guide RNA, Database and Informatics Methods, Sequencing techniques, DNA sequencing, Multidisciplinary, DNA Repeat Expansion, High-Throughput Nucleotide Sequencing, Genomics, Nucleic acids, Tandem Repeats, Microsatellite, Medicine, Sequence Analysis, Research Article, Multiple Alignment Calculation, Bioinformatics, Science, Computational biology, Biology, DNA construction, Human Genomics, Tandem repeat, Computational Techniques, Genetics, Humans, Repeated Sequences, C9orf72 Protein, Cas9, Genome, Human, DNA manipulations, Amyotrophic Lateral Sclerosis, DNA fragment ligation, Biology and Life Sciences, Split-Decomposition Method, Research and analysis methods, Molecular biology techniques, Genetic Loci, Minion, RNA, Human genome, Nanopore sequencing, CRISPR-Cas Systems, Sequence Alignment, Microsatellite Repeats

Abstract

A substantial fraction of the human genome is difficult to interrogate with short-read DNA sequencing technologies due to paralogy, complex haplotype structures, or tandem repeats. Long-read sequencing technologies, such as Oxford Nanopore’s MinION, enable direct measurement of complex loci without introducing many of the biases inherent to short-read methods, though they suffer from relatively lower throughput. This limitation has motivated recent efforts to develop amplification-free strategies to target and enrich loci of interest for subsequent sequencing with long reads. Here, we present CaBagE, a method for target enrichment that is efficient and useful for sequencing large, structurally complex targets. The CaBagE method leverages the stable binding of Cas9 to its DNA target to protect desired fragments from digestion with exonuclease. Enriched DNA fragments are then sequenced with Oxford Nanopore’s MinION long-read sequencing technology. Enrichment with CaBagE resulted in a median of 116X coverage (range 39–416) of target loci when tested on five genomic targets ranging from 4-20kb in length using healthy donor DNA. Four cancer gene targets were enriched in a single reaction and multiplexed on a single MinION flow cell. We further demonstrate the utility of CaBagE in two ALS patients with C9orf72 short tandem repeat expansions to produce genotype estimates commensurate with genotypes derived from repeat-primed PCR for each individual. With CaBagE there is a physical enrichment of on-target DNA in a given sample prior to sequencing. This feature allows adaptability across sequencing platforms and potential use as an enrichment strategy for applications beyond sequencing. CaBagE is a rapid enrichment method that can illuminate regions of the ‘hidden genome’ underlying human disease.

Published

2021

14. An efficient ORF selection system for DNA fragment libraries based on split beta-lactamase complementation

Author

Amita Gupta, Vijay K. Chaudhary, Gopal Joshi, and Vaishali Verma

Subjects

0301 basic medicine, DNA cloning, Artificial Gene Amplification and Extension, Polymerase Chain Reaction, Biochemistry, chemistry.chemical_compound, 0302 clinical medicine, DNA library construction, Genomic library, DNA libraries, Cloning, Molecular, Multidisciplinary, Expression vector, Genomics, Nucleic acids, Actinobacteria, Medicine, DNA fragmentation, Research Article, Science, Computational biology, Biology, DNA construction, Research and Analysis Methods, beta-Lactamases, 03 medical and health sciences, Open Reading Frames, Bacterial Proteins, Genetics, Escherichia coli, Molecular Biology Techniques, Gene Prediction, Gene, Molecular Biology, Gene Library, Cloning, Bacteria, DNA manipulations, DNA fragment ligation, Genetic Complementation Test, Organisms, Biology and Life Sciences, Computational Biology, DNA, Mycobacterium tuberculosis, Genome Analysis, Open reading frame, 030104 developmental biology, chemistry, Protein Fragment, 030217 neurology & neurosurgery

Abstract

PCR-based amplification of annotated genes has allowed construction of expression clones at genome-scale using classical and recombination-based cloning technologies. However, genome-scale expression and purification of proteins for down-stream applications is often limited by challenges such as poor expression, low solubility, large size of multi-domain proteins, etc. Alternatively, DNA fragment libraries in expression vectors can serve as the source of protein fragments with each fragment encompassing a function of its whole protein counterpart. However, the random DNA fragmentation and cloning result in only 1 out of 18 clones being in the correct open-reading frame (ORF), thus, reducing the overall efficiency of the system. This necessitates the selection of correct ORF before expressing the protein fragments. This paper describes a highly efficient ORF selection system for DNA fragment libraries, which is based on split beta-lactamase protein fragment complementation. The system has been designed to allow seamless transfer of selected DNA fragment libraries into any downstream vector systems using a restriction enzyme-free cloning strategy. The strategy has been applied for the selection of ORF using model constructs to show near 100% selection of the clone encoding correct ORF. The system has been further validated by construction of an ORF-selected DNA fragment library of 30 genes of M. tuberculosis. Further, we have successfully demonstrated the cytosolic expression of ORF-selected protein fragments in E. coli.

Published

2020

15. Enabling one-pot Golden Gate assemblies of unprecedented complexity using data-optimized assembly design

Author

Gregory J. S. Lohman, Eric J. Cantor, Katharina Bilotti, Vladimir Potapov, Rebecca Kucera, and John M. Pryor

Subjects

0106 biological sciences, 0301 basic medicine, Molecular biology, Computer science, DNA cloning, Artificial Gene Amplification and Extension, Biochemistry, Polymerase Chain Reaction, 01 natural sciences, law.invention, Ligases, Synthetic biology, chemistry.chemical_compound, law, A-DNA, Ligation Assay, Polymerase chain reaction, chemistry.chemical_classification, Multidisciplinary, Nucleotides, DNA Restriction Enzymes, Enzymes, Recombinant DNA, Engineering and Technology, Medicine, Synthetic Biology, Research Article, DNA Ligases, Science, Computational biology, DNA construction, Molecular cloning, DNA sequencing, 03 medical and health sciences, Cloning, Molecular Biology Assays and Analysis Techniques, DNA ligase, business.industry, DNA manipulations, DNA fragment ligation, Biology and Life Sciences, Proteins, DNA, Modular design, Research and analysis methods, Restriction enzyme, Molecular biology techniques, 030104 developmental biology, Enzyme, chemistry, Enzymology, business, 010606 plant biology & botany

Abstract

DNA assembly is an integral part of modern synthetic biology, as intricate genetic engineering projects require robust molecular cloning workflows. Golden Gate assembly is a frequently employed DNA assembly methodology that utilizes a Type IIS restriction enzyme and a DNA ligase to generate recombinant DNA constructs from smaller DNA fragments. However, the utility of this methodology has been limited by a lack of resources to guide experimental design. For example, selection of the DNA sequences at fusion sites between fragments is based on broad assembly guidelines or pre-vetted sets of junctions, rather than being customized for a particular application or cloning project. To facilitate the design of robust assembly reactions, we developed a high-throughput DNA sequencing assay to examine reaction outcomes of Golden Gate assembly with T4 DNA ligase and the most commonly used Type IIS restriction enzymes that generate three-base and four-base overhangs. Next, we incorporated these findings into a suite of webtools that design assembly reactions using the experimental data. These webtools can be used to create customized assemblies from a target DNA sequence or a desired number of fragments. Lastly, we demonstrate how using these tools expands the limits of current assembly systems by carrying out one-pot assemblies of up to 35 DNA fragments. Full implementation of the tools developed here enables direct expansion of existing assembly standards for modular cloning systems (e.g. MoClo) as well as the formation of robust new high-fidelity standards.

Published

2020

16. PCR-free whole exome sequencing: Cost-effective and efficient in detecting rare mutations

Author

Osamu Ohara, Yoshinori Hasegawa, Takashi Watanabe, and Izumi Yamaguchi

Subjects

0301 basic medicine, DNA hybridization, Cost-Benefit Analysis, Gene Identification and Analysis, Electrophoretic techniques, DNA electrophoresis, Artificial Gene Amplification and Extension, Biochemistry, Polymerase Chain Reaction, Mechanical Treatment of Specimens, law.invention, 0302 clinical medicine, Sequencing techniques, law, Genomic library, Exome, DNA libraries, DNA sequencing, Analysis method, Exome sequencing, Polymerase chain reaction, Multidisciplinary, DNA–DNA hybridization, High-Throughput Nucleotide Sequencing, Genomics, Nucleic acids, Medicine, Transcriptome Analysis, Research Article, Next-Generation Sequencing, Sequence analysis, Science, Computational biology, Biology, DNA construction, Research and Analysis Methods, Polymorphism, Single Nucleotide, 03 medical and health sciences, Sonication, Rare mutations, Exome Sequencing, Genetics, Humans, Molecular Biology Techniques, Molecular Biology, Mutation Detection, Gene Library, Molecular probe techniques, Biology and life sciences, DNA manipulations, DNA fragment ligation, Computational Biology, DNA, Sequence Analysis, DNA, Genome Analysis, Probe hybridization, 030104 developmental biology, Specimen Preparation and Treatment, Mutation, Ultrasonication, 030215 immunology

Abstract

In this study, we describe the development of a PCR-free whole exome sequencing method. Using this method, 2 μg DNA was sufficient for library preparation for whole exome sequencing. Furthermore, the method is simple and makes use of a commercial kit, with additional step of concentrating the captured library by ethanol precipitation. The accuracy of the PCR-free method was found to be equivalent to that of unique molecular identifier-corrected analysis method, which is the commonly used method to detect rare mutations. Thus, the PCR-free whole exome sequencing method is cost-effective as well as efficient in detecting rare mutations.

Published

2019

17. A simple and dual expression plasmid system in prokaryotic (E. coli) and mammalian cells

Author

Takayoshi Ohba, Agnieszka M. Murakami, Kenji Kuwasako, Manabu Murakami, Shirou Itagaki, and Chong Han

Subjects

0301 basic medicine, Luminescence, Molecular biology, Gene Expression, lac operon, Artificial Gene Amplification and Extension, Protein Engineering, Polymerase Chain Reaction, 0302 clinical medicine, Plasmid, Cloning, Molecular, Promoter Regions, Genetic, Mammals, Multidisciplinary, Chemistry, Physics, Electromagnetic Radiation, Escherichia coli Proteins, DNA Restriction Enzymes, Cell biology, 030220 oncology & carcinogenesis, Physical Sciences, Medicine, Research Article, Plasmids, Science, Genetic Vectors, DNA construction, Molecular cloning, Transfection, Fluorescence, 03 medical and health sciences, Genetics, Escherichia coli, Animals, Gene, Biology and life sciences, Base Sequence, DNA manipulations, DNA fragment ligation, Subcloning, Research and analysis methods, EcoRV, Transformation (genetics), Restriction enzyme, Molecular biology techniques, 030104 developmental biology, Prokaryotic Cells, Plasmid Construction, Cloning

Abstract

We introduce a simple and universal cloning plasmid system for gene expression in prokaryotic (Escherichia coli) and mammalian cells. This novel system has two expression modes: the (subcloning) prokaryotic and mammalian modes. This system streamlines the process of producing mammalian gene expression plasmids with desired genes. The plasmid (prokaryotic mode) has an efficient selection system for DNA insertion, multiple component genes with rare restriction sites at both ends (termed "units"), and a simple transformation to mammalian expression mode utilizing rare restriction enzymes and re-ligation (deletion step). The new plasmid contains the lac promoter and operator followed by a blunt-end EcoRV recognition site, and a DNA topoisomerase II toxin-originated gene for effective selection with isopropyl-β-D-thiogalactoside (IPTG) induction. This system is highly efficient for the subcloning of blunt-end fragments, including PCR products. After the insertion of the desired gene, protein encoded by the desired gene can be detected in E. coli with IPTG induction. Then, the lac promoter and operator are readily deleted with 8-nucleotide rare-cutter blunt-end enzymes (deletion step). Following re-ligation and transformation, the plasmid is ready for mammalian expression analysis (mammalian mode). This idea (conversion from prokaryotic to mammalian mode) can be widely adapted. The pgMAX system overwhelmingly simplifies prokaryotic and mammalian gene expression analyses.

Published

2019

18. Novel gateway binary vectors for rapid tripartite DNA assembly and promoter analysis with various reporters and tags in the liverwort Marchantia polymorpha

Author

Ryuichi Nishihama, Kazumi Hikino, Katsuyuki T. Yamato, Tsuyoshi Nakagawa, Sakiko Ishida, Takayuki Kohchi, Shoji Mano, Mikio Nishimura, and Maki Kondo

Subjects

0106 biological sciences, 0301 basic medicine, Time Factors, Molecular biology, lcsh:Medicine, Genetically modified crops, Plant Science, 01 natural sciences, Genetically Modified Plants, Marchantia polymorpha, Plasmid, Genes, Reporter, Arabidopsis thaliana, Coding region, Vector (molecular biology), Promoter Regions, Genetic, lcsh:Science, Multidisciplinary, Genetically Modified Organisms, Eukaryota, Vector Construction, Plants, Experimental Organism Systems, Engineering and Technology, Cellular Structures and Organelles, Genetic Engineering, Research Article, Biotechnology, DNA, Plant, Imaging Techniques, Transgene, Arabidopsis Thaliana, Genetic Vectors, Bioengineering, Computational biology, Brassica, Biology, DNA construction, 03 medical and health sciences, Model Organisms, Plant and Algal Models, Fluorescence Imaging, Gene Expression and Vector Techniques, Peroxisomes, Marchantia, Cloning, Molecular Biology Assays and Analysis Techniques, DNA manipulations, DNA fragment ligation, lcsh:R, Organisms, Biology and Life Sciences, Cell Biology, Vector Cloning, biology.organism_classification, Artificial Gene Fusion, Research and analysis methods, 030104 developmental biology, Molecular biology techniques, Animal Studies, Plant Biotechnology, lcsh:Q, 010606 plant biology & botany

Abstract

The liverwort Marchantia polymorpha is an emerging model species for basal lineage plant research. In this study, two Gateway cloning-compatible binary vector series, R4pMpGWB and R4L1pMpGWB, were generated to facilitate production of transgenic M. polymorpha. The R4pMpGWB series allows tripartite recombination of any promoter and any coding sequence with a specific reporter or tag. Reporters/tags for the R4pMpGWB series are GUS, ELuc(PEST), FLAG, 3×HA, 4×Myc, mRFP1, Citrine, mCitrine, ER-targeted mCitrine and nucleus-targeted mCitrine. The R4L1pMpGWB series is suitable for promoter analysis. R4L1pMpGWB vector structure is the same as that of R4pMpGWB vectors, except that the attR2 site is replaced with attL1, enabling bipartite recombination of any promoter with a reporter or tag. Reporters/tags for the R4L1pMpGWB series are GUS, G3GFP-GUS, LUC, ELuc(PEST), Citrine, mCitrine, ER-targeted mCitrine and mCitrine-NLS. Both vector series were functional in M. polymorpha cells. These vectors will facilitate the design and assembly of plasmid constructs and generation of transgenic M. polymorpha.

Published

2018

19. Interference with DNA repair after ionizing radiation by a pyrrole-imidazole polyamide

Author

Peter B. Dervan, Nathanael Kane, Nicholas G. Nickols, Nicolas Kummer, Silvia Diaz-Perez, Fei Yang, Alexis A. Kurmis, and Sobol, Robert W

Subjects

0301 basic medicine, Ionizing, DNA Repair, Molecular biology, Cytotoxicity, Cell, lcsh:Medicine, Toxicology, Pathology and Laboratory Medicine, Biochemistry, Ionizing radiation, Ligases, XRCC1, DNA Ligase ATP, 0302 clinical medicine, Radiation, Ionizing, Medicine and Health Sciences, 2.1 Biological and endogenous factors, Cell Cycle and Cell Division, Aetiology, Post-Translational Modification, Phosphorylation, lcsh:Science, Genetic Interference, chemistry.chemical_classification, Multidisciplinary, Tumor, Radiation, Chemistry, Physics, Imidazoles, Enzymes, Nucleic acids, medicine.anatomical_structure, Cell Processes, 030220 oncology & carcinogenesis, Polyamide, Physical Sciences, Research Article, DNA repair, General Science & Technology, DNA construction, Cell Line, Small Molecule Libraries, 03 medical and health sciences, Cell Line, Tumor, medicine, Genetics, Humans, Pyrroles, Fragmentation (cell biology), Nuclear Physics, DNA ligase, DNA manipulations, DNA fragment ligation, lcsh:R, Biology and Life Sciences, Proteins, DNA, Cell Biology, Research and analysis methods, Nylons, 030104 developmental biology, Molecular biology techniques, X-ray Repair Cross Complementing Protein 1, Cell culture, Ionizing Radiation, Biophysics, Enzymology, lcsh:Q, DNA Damage

Abstract

Pyrrole-imidazole (Py-Im) polyamides are synthetic non-genotoxic minor groove-binding small molecules. We hypothesized that Py-Im polyamides can modulate the cellular response to ionizing radiation. Pre-treatment of cells with a Py-Im polyamide prior to exposure to ionizing radiation resulted in a delay in resolution of phosphorylated γ-H2AX foci, increase in XRCC1 foci, and reduced cellular replication potential. RNA-sequencing of cell lines exposed to the polyamide showed induction of genes related to the ultraviolet radiation response. We observed that the polyamide is almost 10-fold more toxic to a cell line deficient in DNA ligase 3 as compared to the parental cell line. Alkaline single cell gel electrophoresis reveals that the polyamide induces genomic fragmentation in the ligase 3 deficient cell line but not the corresponding parental line. The polyamide interferes directly with DNA ligation in vitro. We conclude that Py-Im polyamides may be further explored as sensitizers to genotoxic therapies.

Published

2018

20. Comparative analysis of the end-joining activity of several DNA ligases

Author

Robert J. Bauer, Larry A. McReynolds, Katharina Bilotti, Thomas C. Evans, Alexander M. Zhelkovsky, Gregory J. S. Lohman, and Laura E. Crowell

Subjects

0301 basic medicine, Gel electrophoresis of nucleic acids, Molecular biology, genetic processes, Electrophoretic techniques, DNA electrophoresis, lcsh:Medicine, Biochemistry, Ligases, chemistry.chemical_compound, Sticky and blunt ends, Nucleic Acids, DNA Breaks, Double-Stranded, Ligation Assay, lcsh:Science, chemistry.chemical_classification, Multidisciplinary, Blunt-End Ligation, Physics, Condensed Matter Physics, Enzymes, Physical Sciences, Research Article, DNA Ligases, Materials Science, Material Properties, DNA construction, DNA-binding protein, 03 medical and health sciences, DNA-binding proteins, Genetics, Humans, Molecular Biology Assays and Analysis Techniques, DNA ligase, DNA manipulations, DNA fragment ligation, lcsh:R, Electrophoresis, Capillary, Biology and Life Sciences, Proteins, DNA, DNA-binding domain, Research and analysis methods, enzymes and coenzymes (carbohydrates), Molecular biology techniques, 030104 developmental biology, chemistry, Enzymology, Anisotropy, lcsh:Q, Ligation

Abstract

DNA ligases catalyze the repair of phosphate backbone breaks in DNA, acting with highest activity on breaks in one strand of duplex DNA. Some DNA ligases have also been observed to ligate two DNA fragments with short complementary overhangs or blunt-ended termini. In this study, several wild-type DNA ligases (phage T3, T4, and T7 DNA ligases, Paramecium bursaria chlorella virus 1 (PBCV1) DNA ligase, human DNA ligase 3, and Escherichia coli DNA ligase) were tested for their ability to ligate DNA fragments with several difficult to ligate end structures (blunt-ended termini, 3′- and 5′- single base overhangs, and 5′-two base overhangs). This analysis revealed that T4 DNA ligase, the most common enzyme utilized for in vitro ligation, had its greatest activity on blunt- and 2-base overhangs, and poorest on 5′-single base overhangs. Other ligases had different substrate specificity: T3 DNA ligase ligated only blunt ends well; PBCV1 DNA ligase joined 3′-single base overhangs and 2-base overhangs effectively with little blunt or 5′- single base overhang activity; and human ligase 3 had highest activity on blunt ends and 5′-single base overhangs. There is no correlation of activity among ligases on blunt DNA ends with their activity on single base overhangs. In addition, DNA binding domains (Sso7d, hLig3 zinc finger, and T4 DNA ligase N-terminal domain) were fused to PBCV1 DNA ligase to explore whether modified binding to DNA would lead to greater activity on these difficult to ligate substrates. These engineered ligases showed both an increased binding affinity for DNA and increased activity, but did not alter the relative substrate preferences of PBCV1 DNA ligase, indicating active site structure plays a role in determining substrate preference.

Published

2017

21. Rapid Synthesis of a Long Double-Stranded Oligonucleotide from a Single-Stranded Nucleotide Using Magnetic Beads and an Oligo Library

Author

Todd C. Mockler, Vincent T. Remcho, Erik R. Rowley, Myra T. Koesdjojo, and Sumate Pengpumkiat

Subjects

0301 basic medicine, Time Factors, Molecular biology, Polymers, Oligonucleotides, lcsh:Medicine, Artificial Gene Amplification and Extension, Bioinformatics, 01 natural sciences, Polymerase Chain Reaction, Biochemistry, DNA annealing, Ligases, chemistry.chemical_compound, Sequencing techniques, Genomic library, DNA sequencing, lcsh:Science, Sanger sequencing, Gel electrophoresis, Electrophoresis, Agar Gel, Multidisciplinary, Physics, Microspheres, Enzymes, Nucleic acids, Chemistry, Macromolecules, Physical Sciences, Nucleic acid thermodynamics, symbols, Research Article, Materials by Structure, Materials Science, Annealing (genetics), Molecular Sequence Data, Biophysics, DNA, Single-Stranded, DNA construction, 010402 general chemistry, 03 medical and health sciences, symbols.namesake, Magnetics, Sequence Homology, Nucleic Acid, Genetics, Gene Library, DNA synthesis, Biology and life sciences, Base Sequence, Models, Genetic, Oligonucleotide, DNA manipulations, lcsh:R, DNA fragment ligation, Proteins, Reproducibility of Results, DNA, Polymer Chemistry, Combinatorial chemistry, 0104 chemical sciences, Research and analysis methods, 030104 developmental biology, Molecular biology techniques, chemistry, Nucleic acid, Enzymology, lcsh:Q

Abstract

Chemical synthesis of oligonucleotides is a widely used tool in the field of biochemistry. Several methods for gene synthesis have been introduced in the growing area of genomics. In this paper, a novel method of constructing dsDNA is proposed. Short (28-mer) oligo fragments from a library were assembled through successive annealing and ligation processes, followed by PCR. First, two oligo fragments annealed to form a dsDNA molecule. The double-stranded oligo was immobilized onto magnetic beads (solid support) via streptavidin-biotin binding. Next, single-stranded oligo fragments were added successively through ligation to form the complete DNA molecule. The synthesized DNA was amplified through PCR and gel electrophoresis was used to characterize the product. Sanger sequencing showed that more than 97% of the nucleotides matched the expected sequence. Extending the length of the DNA molecule by adding single-stranded oligonucleotides from a basis set (library) via ligation enables a more convenient and rapid mechanism for the design and synthesis of oligonucleotides on the go. Coupled with an automated dispensing system and libraries of short oligo fragments, this novel DNA synthesis method would offer an efficient and cost-effective method for producing dsDNA.

Published

2016

22. The Inhibitory Effect of Non-Substrate and Substrate DNA on the Ligation and Self-Adenylylation Reactions Catalyzed by T4 DNA Ligase

Author

Robert J. Bauer, Thomas C. Evans, and Gregory J. S. Lohman

Subjects

0301 basic medicine, DNA polymerase, lcsh:Medicine, Electrophoretic Mobility Shift Assay, Restriction Fragment Mapping, Biochemistry, Ligases, Enzyme Inhibitors, lcsh:Science, chemistry.chemical_classification, Multidisciplinary, DNA clamp, biology, Enzymes, Circular DNA, Nucleic acids, DNA supercoil, Research Article, DNA Replication, DNA Ligases, Forms of DNA, DNA polymerase II, DNA construction, In Vitro Techniques, Research and Analysis Methods, Catalysis, 03 medical and health sciences, Genetics, Molecular Biology Techniques, Molecular Biology, Replication protein A, DNA ligase, 030102 biochemistry & molecular biology, DNA manipulations, Gene Mapping, DNA fragment ligation, lcsh:R, DNA replication, Biology and Life Sciences, Proteins, DNA structure, DNA, Macromolecular structure analysis, Kinetics, 030104 developmental biology, chemistry, Enzymology, biology.protein, lcsh:Q, DNA polymerase I

Abstract

DNA ligases are essential both to in vivo replication, repair and recombination processes, and in vitro molecular biology protocols. Prior characterization of DNA ligases through gel shift assays has shown the presence of a nick site to be essential for tight binding between the enzyme and its dsDNA substrate, with no interaction evident on dsDNA lacking a nick. In the current study, we observed a significant substrate inhibition effect, as well as the inhibition of both the self-adenylylation and nick-sealing steps of T4 DNA ligase by non-nicked, non-substrate dsDNA. Inhibition by non-substrate DNA was dependent only on the total DNA concentration rather than the structure; with 1 μg/mL of 40-mers, 75-mers, or circular plasmid DNA all inhibiting ligation equally. A >15-fold reduction in T4 DNA ligase self-adenylylation rate when in the presence of high non-nicked dsDNA concentrations was observed. Finally, EMSAs were utilized to demonstrate that non-substrate dsDNA can compete with nicked dsDNA substrates for enzyme binding. Based upon these data, we hypothesize the inhibition of T4 DNA ligase by non-nicked dsDNA is direct evidence for a two-step nick-binding mechanism, with an initial, nick-independent, transient dsDNA-binding event preceding a transition to a stable binding complex in the presence of a nick site.

Published

2016