Literature DB >> 15349749

Single oligonucleotide nested PCR: a rapid method for the isolation of genes and their flanking regions from expressed sequence tags.

Zsuzsanna Antal1, Christine Rascle, Michel Fèvre, Christophe Bruel.   

Abstract

We report on the development of a new PCR technique for the isolation of genomic fragments that flank known DNA sequences. This technique, single oligonucleotide nested (SON)-PCR, relies on only two amplification reactions with two or three nested sequence-specific primers. It allows the isolation of DNA regions located on either side of a known DNA sequence, with high specificity. DNA products of 2 kb in size can be generated that all contain one copy of the same primer at both ends. Sequence analysis of these products indicates that the binding of the primers to non-specific DNA sites mainly depends on their overall complementarity to the target sequence. Moreover, analysis shows that short extensions of the primers can occur during the first amplification reaction and that a 2-bp overlap between subsequent primers can target their annealing to their predecessor's sequence. Ninety percent of the DNA products larger than 0.5 kb correspond to fragments of interest and we obtained successful results with various templates and primer sets. SON-PCR therefore seems a very efficient and widely applicable method for the rapid identification of large unknown DNA regions. Based on available expressed sequence tags, this technique was applied to isolate the palH and pacC genes of the phytopathogenic fungus Botrytis cinerea, with their 5' or 3' flanking regions.

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Year:  2004        PMID: 15349749     DOI: 10.1007/s00294-004-0524-6

Source DB:  PubMed          Journal:  Curr Genet        ISSN: 0172-8083            Impact factor:   3.886


  20 in total

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Journal:  Biotechniques       Date:  2000-06       Impact factor: 1.993

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Journal:  Biotechniques       Date:  2000-05       Impact factor: 1.993

Review 3.  Genomics of phytopathogenic fungi and the development of bioinformatic resources.

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Journal:  Mol Plant Microbe Interact       Date:  2002-05       Impact factor: 4.171

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Journal:  Nucleic Acids Res       Date:  1991-06-11       Impact factor: 16.971

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Authors:  C L Parks; L S Chang; T Shenk
Journal:  Nucleic Acids Res       Date:  1991-12       Impact factor: 16.971

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Authors:  E K Hui; P C Wang; S J Lo
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7.  Efficient isolation and mapping of Arabidopsis thaliana T-DNA insert junctions by thermal asymmetric interlaced PCR.

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8.  Thermal asymmetric interlaced PCR: automatable amplification and sequencing of insert end fragments from P1 and YAC clones for chromosome walking.

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Journal:  Genomics       Date:  1995-02-10       Impact factor: 5.736

9.  Splinkerettes--improved vectorettes for greater efficiency in PCR walking.

Authors:  R S Devon; D J Porteous; A J Brookes
Journal:  Nucleic Acids Res       Date:  1995-05-11       Impact factor: 16.971

10.  Agrobacterium-mediated transformation of Botrytis cinerea, simple purification of monokaryotic transformants and rapid conidia-based identification of the transfer-DNA host genomic DNA flanking sequences.

Authors:  Stéphane Rolland; Cécile Jobic; Michel Fèvre; Christophe Bruel
Journal:  Curr Genet       Date:  2003-08-21       Impact factor: 3.886

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  16 in total

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6.  Identification of differentially expressed genes in the developing antler of red deer Cervus elaphus.

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7.  Multigene family encoding 3',5'-cyclic-GMP-dependent protein kinases in Paramecium tetraurelia cells.

Authors:  Roland Kissmehl; Tim P Krüger; Tilman Treptau; Marine Froissard; Helmut Plattner
Journal:  Eukaryot Cell       Date:  2006-01

8.  Structural and expressional analysis of the B-hordein genes in Tibetan hull-less barley.

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9.  Molecular analysis of duck enteritis virus US3, US4, and US5 gene.

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10.  Complete genome sequence of the first Chinese virulent infectious laryngotracheitis virus.

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