Construction of long DNA molecules using long PCR-based fusion of several fragments simultaneously

Shevchuk, Nikolai A; Bryksin, Anton V.; Nusinovich, Yevgeniya; Cabello, Felipe C.; Sutherland, Margaret; Ladisch, Stephan

doi:10.1093/nar/gnh014

Cited by 295 publications

(256 citation statements)

References 10 publications

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“…The genes for the full-length p70 and p180 C (1265-1444) with an N-terminal His 8 -SUMO tag were subcloned into the pETDuet-1 vector (Novagen) using NcoI/ BamHI and NdeI/KpnI (TaKaRa) restriction sites, respectively. The DNA coding for the His 8 -SUMO tag was amplified from a pETHSUL vector (two histidines were added to original His 6 tag at that time) and attached to the fragment encoding p180 C by fusion PCR (38). The human His-SUMO-p180 C -p70 complex was expressed for 16 h (18°C) in Escherichia coli strain Rosetta-2(DE3) in LB medium after induction with 1 mM isopropyl ␤-D-1-thiogalactopyranoside.…”

Section: Data Collection Nativementioning

confidence: 99%

Crystal Structure of the Human Pol α B Subunit in Complex with the C-terminal Domain of the Catalytic Subunit

Suwa¹,

Gu²,

Baranovskiy³

et al. 2015

Journal of Biological Chemistry

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Background: DNA polymerase ␣ (Pol ␣) initiates DNA synthesis and is indispensable for genome replication.Results: We present a crystal structure of human Pol ␣ minus the catalytic core at 2.5 Å resolution. Conclusion:The mode of interaction between the Pol ␣ subunits is evolutionarily conserved. Significance: The data provide structural insight into the function of the primase-Pol ␣ complex.

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Section: Data Collection Nativementioning

confidence: 99%

Crystal Structure of the Human Pol α B Subunit in Complex with the C-terminal Domain of the Catalytic Subunit

Suwa¹,

Gu²,

Baranovskiy³

et al. 2015

Journal of Biological Chemistry

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“…According to this method the target gene is inactivated by chromosomal integration of the whole vector, which contains an internal fragment of the target gene, via a single crossover event. A method, which combines site-specific recombination system (Cre/lox system) (Abremski et al 1983) and high-fidelity fusion PCR method (Shevchuk et al 2004) was developed to introduce unmarked mutations into the B. subtilis genome (Xin et al 2008). Fabret et al (2002) described a protocol based on the use of upp, which encodes uracil phosphoribosyl-transferase, as a counterselectable marker to engineer B. subtilis genome.…”

Section: Deletion Of Ppk Gene By a Pcr Based Methodsmentioning

confidence: 99%

An efficient gene deletion system for Bacillus thuringiensis

Doruk

Gedik

2013

Biologia

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It is not easy to manipulate biosynthetic genes of Bacillus thuringiensis since there is a powerful methyl-specific restriction system in this microorganism. In this study, a PCR-based system was used to delete polyphosphate kinase gene (ppk) of Bacillus thuringiensis israelensis (Bti) by replacing the wild-type gene with a cassette containing the apramycin resistance gene as selectable marker. λ-Red was used to promote recombination in Escherichia coli between a PCR-amplified apramycin resistance cassette (linear deletion cassette selectable in E. coli and Bti) and Bti DNA on a plasmid. The isolated mutant plasmid was transferred to Bti by conjugation. Double cross-over transformants were screened for their antibiotic resistance and the mutation was proven by PCR, southern blot hybridization and RT-PCR. The described method, which uses the advantage of quick plasmid construction in E. coli and simple transformation of linear deletion cassette, is very useful to delete entire gene/genes of Bti without any polar effects on genes transcriptionally downstream.

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“…While this technique allows for the production of chimeras with specific/known junction points, the availability of unique restriction enzyme sites can impose limitations on the design of potential chimeras. In contrast, the PCR fusion technique (Shevchuk et al, 2004) creates chimeric junctions at any amino acid, without the need for restriction enzyme sites. In this method (Fig.…”

Section: Pcr Fusion Methodologymentioning

confidence: 99%

Directed Mutagenesis in Structure Activity Studies of Neurotransmitter Transporters

Carland¹,

Edington

Scopelliti³

et al. 2013

Genetic Manipulation of DNA and Protein - Examples From Current Research

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Construction of long DNA molecules using long PCR-based fusion of several fragments simultaneously

Cited by 295 publications

References 10 publications

Crystal Structure of the Human Pol α B Subunit in Complex with the C-terminal Domain of the Catalytic Subunit

Crystal Structure of the Human Pol α B Subunit in Complex with the C-terminal Domain of the Catalytic Subunit

An efficient gene deletion system for Bacillus thuringiensis

Directed Mutagenesis in Structure Activity Studies of Neurotransmitter Transporters

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