Improvements in Bacterial Primers to Enhance Selective SSU rRNA Gene Amplification of Plant-associated Bacteria by Applying the LNA Oligonucleotide-PCR Clamping Technique

Makoto Ikenaga; Shohei Katsuragi; Yoshihiro Handa; Hiroshi Katsumata; Naoya Chishaki; Tomohiro Kawauchi; Masao Sakai

doi:10.1264/jsme2.ME18071

This article has now been updated. Please use the final version.

Improvements in Bacterial Primers to Enhance Selective SSU rRNA Gene Amplification of Plant-associated Bacteria by Applying the LNA Oligonucleotide-PCR Clamping Technique

Makoto Ikenaga, Shohei Katsuragi, Yoshihiro Handa, Hiroshi Katsumata, Naoya Chishaki, Tomohiro Kawauchi, Masao Sakai

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Keywords: PCR clamping, SSU rRNA genes, plant–associated bacteria, LNA oligonucleotide, KU63f and KU1494r

JOURNAL FREE ACCESS Advance online publication

Article ID: ME18071

DOI https://doi.org/10.1264/jsme2.ME18071

The final version of this article is now available: Vol. 33 (2018), No. 3 pp. 340-344

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Abstract

PCR clamping by locked nucleic acid (LNA) oligonucleotides is an effective technique for selectively amplifying the community SSU rRNA genes of plant–associated bacteria. However, the original primer set often shows low amplification efficiency. In order to improve this efficiency, new primers were designed at positions to compete with LNA oligonucleotides. Three new sets displayed higher amplification efficiencies than the original; however, efficiency varied among the primer sets. Two new sets appeared to be available in consideration of bacterial profiles by next-generation sequencing. One new set, KU63f and KU1494r, may be applicable to the selective gene amplification of plant-associated bacteria.

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