2005
DOI: 10.1111/j.1439-0523.2004.01058.x
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Determination of incompatibility genotypes in almond using first and second intron consensus primers: detection of new S alleles and correction of reported S genotypes

Abstract: The work aimed to develop a reliable and convenient PCR approach for determining incompatibility S genotypes in almond. Initially, genomic DNAs of 24 accessions of known S genotype were amplified with novel consensus primers flanking the first and second introns of the S-RNase gene. The PCR products separated on agarose showed length polymorphisms and correlated well with the reference alleles S 1 -S 23 and S f . In addition, to improve discrimination between alleles of similar sizes, the same sets of primers … Show more

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Cited by 61 publications
(114 citation statements)
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“…sequences were used for PCR amplification in accordance with previous reports (Sonneveld et al 2003;Ortega et al 2005;Rahemi et al 2010). The PaConsI-FD forward and EM-Pc1ConsRD reverse primers were designed using the SP of cherry S-RNases (Sonneveld et al 2003) and the first conserved region flanking the first intron, respectively (Ortega et al 2005).…”
Section: Polymerase Chain Reactionsmentioning
confidence: 99%
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“…sequences were used for PCR amplification in accordance with previous reports (Sonneveld et al 2003;Ortega et al 2005;Rahemi et al 2010). The PaConsI-FD forward and EM-Pc1ConsRD reverse primers were designed using the SP of cherry S-RNases (Sonneveld et al 2003) and the first conserved region flanking the first intron, respectively (Ortega et al 2005).…”
Section: Polymerase Chain Reactionsmentioning
confidence: 99%
“…Total genomic DNA was extracted from dried leaves using CTAB protocol (Doyle and Doyle 1987) with some modification (Ortega et al 2005;Rahemi et al 2012b). DNA quantity and quality were determined by spectrophotometry and agarose gel electrophoresis.…”
Section: Dna Extractionmentioning
confidence: 99%
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