2009
DOI: 10.1111/j.1439-0523.2009.01730.x
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Allele-specific SNP markers for the new low linolenic mutant genotype of winter oilseed rape

Abstract: One of the goals in oilseed rape breeding is the identification of genotypes with low linolenic acid content in seed oil. Here, we present new genetic markers for mutant alleles of a chemically induced low linolenic rapeseed line DH219/05. Genomic clones comprising fatty acids desaturase 3 (FAD3) genes from the mutant and wild-type rapeseed lines were sequenced. Two statistically important single nucleotide polymorphisms were detected: (1) a C to T substitution in the third position of the sixth codon of the s… Show more

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Cited by 18 publications
(43 citation statements)
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References 22 publications
(26 reference statements)
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“…The FAD3 genes encode for encoplasmic delta-15 linoleate desaturase responsible for desaturation of linoleic acid (C18:2) into linolenic acid. As a result of cloning and sequencing of FAD3 genes from wildtype and LL mutant B. napus plants, we reported two point mutations (BnaA.FAD3 and BnaC.FAD3) responsible for disruption of the FAD3 genes expression and function (Mikolajczyk et al, 2010b) in the new LL mutant rapeseed line (Spasibionek, 2006). One point mutation comprised a C to T transition in the mutant bnaA.fad3 gene leading to a possible Arg to Cys substitution.…”
Section: Wwwintechopencommentioning
confidence: 99%
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“…The FAD3 genes encode for encoplasmic delta-15 linoleate desaturase responsible for desaturation of linoleic acid (C18:2) into linolenic acid. As a result of cloning and sequencing of FAD3 genes from wildtype and LL mutant B. napus plants, we reported two point mutations (BnaA.FAD3 and BnaC.FAD3) responsible for disruption of the FAD3 genes expression and function (Mikolajczyk et al, 2010b) in the new LL mutant rapeseed line (Spasibionek, 2006). One point mutation comprised a C to T transition in the mutant bnaA.fad3 gene leading to a possible Arg to Cys substitution.…”
Section: Wwwintechopencommentioning
confidence: 99%
“…previously by Mikolajczyk et al (2010b) for the analysis of splicing variant (see Table 3 for primer details). The PCR was carried out in a 96-well plate (Brandt, Wertheim, Germany) sealed with silicone compression mat (Axygen, Union City, CA, USA) in a reaction volume of 6 μl containing 2.5 µl of Type-it Microsatellite PCR Kit (Qiagen, Hilden, Germany), 0.2 mM of each primer, and 1 µl of DNA template (50-100 ng).…”
Section: Pcr Amplification Ofmentioning
confidence: 99%
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