Anders Andersson1, Rolf Bernander, Peter Nilsson. 1. Department of Biotechnology, KTH-Royal Institute of Technology, SE-106 91 Stockholm, Sweden. anders.andersson@biotech.kth.se
Abstract
MOTIVATION: Microarray experiments using probes covering a whole transcriptome are expensive to initiate, and a major part of the costs derives from synthesizing gene-specific PCR primers or hybridization probes. The high costs may force researchers to limit their studies to a single organism, although comparing gene expression in different species would yield valuable information. RESULTS: We have developed a method, implemented in the software DualPrime, that reduces the number of primers required to amplify the genes of two different genomes. The software identifies regions of high sequence similarity, and from these regions selects PCR primers shared between the genomes, such that either one or, preferentially, both primers in a given PCR can be used for amplification from both genomes. To assure high microarray probe specificity, the software selects primer pairs that generate products of low sequence similarity to other genes within the same genome. We used the software to design PCR primers for 2182 and 1960 genes from the hyperthermophilic archaea Sulfolobus solfataricus and Sulfolobus acidocaldarius, respectively. Primer pairs were shared among 705 pairs of genes, and single primers were shared among 1184 pairs of genes, resulting in a saving of 31% compared to using only unique primers. We also present an alternative primer design method, in which each gene shares primers with two different genes of the other genome, enabling further savings. 3. AVAILABILITY: The software is freely available at http://www.biotech.kth.se/molbio/microarray/.
MOTIVATION: Microarray experiments using probes covering a whole transcriptome are expensive to initiate, and a major part of the costs derives from synthesizing gene-specific PCR primers or hybridization probes. The high costs may force researchers to limit their studies to a single organism, although comparing gene expression in different species would yield valuable information. RESULTS: We have developed a method, implemented in the software DualPrime, that reduces the number of primers required to amplify the genes of two different genomes. The software identifies regions of high sequence similarity, and from these regions selects PCR primers shared between the genomes, such that either one or, preferentially, both primers in a given PCR can be used for amplification from both genomes. To assure high microarray probe specificity, the software selects primer pairs that generate products of low sequence similarity to other genes within the same genome. We used the software to design PCR primers for 2182 and 1960 genes from the hyperthermophilic archaea Sulfolobus solfataricus and Sulfolobus acidocaldarius, respectively. Primer pairs were shared among 705 pairs of genes, and single primers were shared among 1184 pairs of genes, resulting in a saving of 31% compared to using only unique primers. We also present an alternative primer design method, in which each gene shares primers with two different genes of the other genome, enabling further savings. 3. AVAILABILITY: The software is freely available at http://www.biotech.kth.se/molbio/microarray/.
Authors: Martin Mehlmann; Erica D Dawson; Michael B Townsend; James A Smagala; Chad L Moore; Catherine B Smith; Nancy J Cox; Robert D Kuchta; Kathy L Rowlen Journal: J Clin Microbiol Date: 2006-08 Impact factor: 5.948
Authors: Ann-Christin Lindås; Erik A Karlsson; Maria T Lindgren; Thijs J G Ettema; Rolf Bernander Journal: Proc Natl Acad Sci U S A Date: 2008-11-05 Impact factor: 11.205
Authors: Anders F Andersson; Erik A Pelve; Stefan Lindeberg; Magnus Lundgren; Peter Nilsson; Rolf Bernander Journal: BMC Genomics Date: 2010-07-28 Impact factor: 3.969
Authors: Anders F Andersson; Magnus Lundgren; Stefan Eriksson; Magnus Rosenlund; Rolf Bernander; Peter Nilsson Journal: Genome Biol Date: 2006-10-26 Impact factor: 13.583