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20 February 2015

Inosine at Different Primer Positions to Study Structure and Diversity of Prokaryotic Populations

and
1
Department of Life Sciences, Achva Academic College, MP Shikmim, 79800, Israel
2
Department of Biotechnology Engineering and National Institute for Biotechnology in the Negev, Ben-Gurion University of the Negev, PO Box 653, Be’er-Sheva 84105, Israel
3
School of Materials Science and Engineering, Nanyang Technological University, Singapore 637819, Singapore
*
Author to whom correspondence should be addressed.

Abstract

Culture-independent methods, employed to study the diversity and complexity of microbial communities that are based on amplification of rRNA genes with universal primers, include gradient gel electrophoresis (denaturing or temperature), single-strand-conformation polymorphism, restriction fragment length polymorphism, qPCR and high-throughput DNA sequencing. Substituting one or more base(s) within or at the 3'-termi of the universal primers by inosine can overcome some of their shortcomings improving amplification capacity. Universal primer sets do not usually amplify sequences with nucleotide mismatch to the templates, particularly in the last three bases, whereas inosine-modified primers anneal and amplify a variety of rRNA gene sequences. Inosine-containing primers are therefore might be useful to detect more species in diverse prokaryotic populations. The article summarizes the pros and cons of using inosine especially at the 3' termini of universal primers in nucleic acid amplification for the study of microbial diversity.

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