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Genotyping of bovine k‐casein (k‐CN<sup>A</sup>, k‐CN<sup>B</sup>, k‐CN<sup>C</sup>, k‐CN<sup>E</sup>) following DNA sequence amplification and direct sequencing of k‐CN<sup>E</sup> PCR product

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References

1991

Year

Abstract

Genomic DNA isolated from blood and semen of dairy cattle with known kappa-casein (kappa-CN) genotypes was subjected to Southern blot hybridization and polymerase chain reaction (PCR) using up to 14 restriction endonucleases. kappa-casein genotypes AA, AB and BB were identified using Hin dIII and Hin fI while genotypes with kappa-CNC and kappa-CNE were misidentified. Direct sequencing of the PCR product (kappa-CN EE) showed a substitution of guanine (kappa-CNA,B) by adenine (kappa-CNE) which creates a HaeIII restriction site. Therefore using PCR followed by Hin dIII or HinfI and Hae III digest allows discrimination between kappa-casein A, B and E directly at the DNA level.

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