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Literature DB >> 10911610

Restriction primers as short as 6-mers for PCR amplification of bacterial and plant genomic DNA and plant viral RNA.

Abstract

Amplification of DNA or RNA sequences using the polymerase chain reaction (PCR) or reverse transcriptase PCR (RT-PCR) requires primers of an appropriate length to be designed. Two hexamer restriction primers, denoted as E101 and H301, which correspond to sequences of EcoRI and HindIII recognition sites, respectively, were selected and used as primers in PCR and RT-PCR. We first applied the restriction primers to the plasmid DNA and bacterial (Pseudomonas) and plant (Cymbidium) genomic DNAs. We observed positive DNA amplifications with the recombinant plasmid DNA and bacterial and plant genomic DNAs. Purified viral RNA was used for template in the RT-PCR with the primers and successful DNA amplification was obtained. These results suggest that the 6-mer restriction primers can be useful for new applications in PCR.

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Year: 2000 PMID： 10911610 DOI： 10.1385/MB:14:1:01

Source DB: PubMed Journal: Mol Biotechnol ISSN： 1073-6085 Impact factor: 2.695

7 in total

1. The effect of temperature and oligonucleotide primer length on the specificity and efficiency of amplification by the polymerase chain reaction.

Authors: D Y Wu; L Ugozzoli; B K Pal; J Qian; R B Wallace
Journal: DNA Cell Biol Date: 1991-04 Impact factor: 3.311

7. Cloning of the 3'-terminal region encoding movement and coat proteins of a Korean isolate of odontoglossum ringspot virus.

Authors: K H Ryu; C W Choi; J K Choi; W M Park
Journal: Arch Virol Date: 1995 Impact factor: 2.574

7 in total

1 in total

1. Single Core Genome Sequencing for Detection of both Borrelia burgdorferi Sensu Lato and Relapsing Fever Borrelia Species.

Authors: Sin Hang Lee; John Eoin Healy; John S Lambert
Journal: Int J Environ Res Public Health Date: 2019-05-20 Impact factor: 3.390

1 in total

Restriction primers as short as 6-mers for PCR amplification of bacterial and plant genomic DNA and plant viral RNA.

1. The effect of temperature and oligonucleotide primer length on the specificity and efficiency of amplification by the polymerase chain reaction.

2. Accurate sequencing by hybridization for DNA diagnostics and individual genomics.

3. Short synthetic oligonucleotide repeats detect human genomic variation.

4. Effect of concentration of MgCl2 on random-amplified DNA polymorphism.

5. Rapid detection and identification of odontoglossum ringspot virus by polymerase chain reaction amplification.

6. Oligonucleotides as short as 7-mers can be used for PCR amplification.

7. Cloning of the 3'-terminal region encoding movement and coat proteins of a Korean isolate of odontoglossum ringspot virus.

1. Single Core Genome Sequencing for Detection of both Borrelia burgdorferi Sensu Lato and Relapsing Fever Borrelia Species.