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A single nucleotide polymorphism in the sheep κ-casein coding region

Published online by Cambridge University Press:  09 May 2005

Maria Feligini
Affiliation:
Istituto Sperimentale Italiano “Lazzaro Spallanzani”, Laboratorio di Epigenomica Applicata, Viale Giovanni XXIII 7, I-26900 Lodi, Italy
Slavica Vlaco
Affiliation:
Istituto Sperimentale Italiano “Lazzaro Spallanzani”, Laboratorio di Epigenomica Applicata, Viale Giovanni XXIII 7, I-26900 Lodi, Italy
Vlatka Cubric Curik
Affiliation:
Dairy Science Department, Faculty of Agriculture, University of Zagreb, Svetosimunska 25, HR-10 000 Zagreb, Croatia
Pietro Parma
Affiliation:
Istituto Sperimentale Italiano “Lazzaro Spallanzani”, Laboratorio di Epigenomica Applicata, Viale Giovanni XXIII 7, I-26900 Lodi, Italy
GianFranco Greppi
Affiliation:
Istituto Sperimentale Italiano “Lazzaro Spallanzani”, Laboratorio di Epigenomica Applicata, Viale Giovanni XXIII 7, I-26900 Lodi, Italy Dipartimento di Clinica Medica Veterinaria, Università degli Studi di Milano, Via Celoria 10, Milan, Italy
Giuseppe Enne
Affiliation:
Istituto Sperimentale Italiano “Lazzaro Spallanzani”, Laboratorio di Epigenomica Applicata, Viale Giovanni XXIII 7, I-26900 Lodi, Italy Dipartimento di Scienze Zootecniche, Facoltà di Agraria, Università di Sassari, Via De Nicola, Sassari, Italy

Abstract

Genetic polymorphisms in CSN3 gene in Pag (Croatia), Sarda (Italy) and Pramenka (Serbia) sheep breeds were investigated. A single nucleotide polymorphism (SNP) was localized by sequence analysis (sequence submitted to GenBank under accession AY237637) relying on an original primer pair. Primers for sequencing (κ-casF and κ-casR) were designed on the available CSN3 sequences to amplify the genomic region encoding the major part of the mature protein (exon 4). An SNP was detected at position 237 of the sheep κ-casein mRNA (reference sequence: GenBank X51822), where a thymine was substituted for a cytosine. The SNP was typed by conventional PCR and SYBR Green I-based real-time PCR. C and T alleles were discriminated using a dedicated set of primers that consisted of one common forward primer (SNP-TC) and two reverse primers (SNP-T and SNP-C), the latter two differing in the 3′ end base and in the presence of a 12 bp poly-G tail in SNP-C. The SNP was found in both the heterozygous and the homozygous state in Sarda and Pramenka breeds, and in the heterozygous state only in the Pag breed. The observed allelic frequencies of the SNP were 0·12 in Pag, 0·27 in Sarda and 0·45 in Pramenka.

Type
Research Article
Copyright
© Proprietors of Journal of Dairy Research 2005

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