Abstract

The oral mucosae of the lips and muzzle appeared histologically normal. Mitotic chromosomes were visualised with conventional staining and RBA-banding from non-synchronised cultures of peripheral blood lymphocytes of the affected calves and their relatives (De Grouchy and others 1964, Dutrillaux and others 1973). No abnormality was detected in either the structure or the number of chromosomes. Genealogical data from the Chianina Breed Stud Book, from the Associazione Nazionale Allevatori Bovini Italiani da Carne (ANABIC), were collected to analyse the pedigrees of the two affected animals and of nine other newborn Chianina calves showing the same condition (Fig 3). Wherever possible, blood samples were collected from the affected animals and their sires, dams and siblings. Parentage relationships were verified by microsatellite analysis with StockMarks for Cattle Paternity PCR typing kits (Applied Biosystems). Forty-nine animals of the familial group were evaluated. Analysis of the pedigree information revealed that all clinical cases were generated by consanguineous matings. In particular, three bulls were acknowledged as being disease carriers: bulls 23, 30 and 34 (Fig 3). Bull 23 sired three affected male calves (26, 28 and 48) and two healthy female calves (31 and 35); bull 30 sired two affected male calves (27 and 49) and two healthy calves, one male (34) and one female (46); and bull 34 sired six affected calves, four males (38, 40, 41 and 47) and two females (43 and 44) and four healthy calves, three males (37, 42 and 45) and one female (39). None of the carIchthyosis in Chianina cattle

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