Optimization of the PCR test for the mutation causing bovine leukocyte adhesion deficiency.

M. H. Mirck; T. Von Bannisseht-Wijsmuller; W. J. Timmermans-Besselink; J. H. Van Luijk; J. B. Buntjer; J. A. Lenstra

Optimization of the PCR test for the mutation causing bovine leukocyte adhesion deficiency.

M. H. Mirck^*
, T. Von Bannisseht-Wijsmuller
, W. J. Timmermans-Besselink
, J. H. Van Luijk
, J. B. Buntjer
, J. A. Lenstra

^*Corresponding author for this work

Animal Health Service Deventer

Research output: Contribution to journal › Article › Academic › peer-review

Abstract

The recent emergence of the bovine leukocyte adhesion deficiency (BLAD) demonstrated the risks of narrowing the genetic basis of a population. About 6% of the Holstein-Friesian cattle now descends from one bull who was a heterozygous BLAD carrier. Crossing his descendants resulted in the birth of homozygous BLAD calves with a life expectancy of < 1 year. The BLAD syndrome is caused by a point mutation in the gene coding for CD18, a subunit of the beta 2 integrins on the surface of leukocytes. By using a PCR-RFLP test, large numbers of cattle are now being screened in several countries to eradicate the mutant allele. We describe an optimization of the PCR primer set that has led to an improvement of the test.

Original language	English
Pages (from-to)	695-698
Number of pages	4
Journal	Cellular and Molecular Biology
Volume	41
Issue number	5
Publication status	Published - 1 Jul 1995

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SDG 3 Good Health and Well-being

Cite this

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title = "Optimization of the PCR test for the mutation causing bovine leukocyte adhesion deficiency.",

abstract = "The recent emergence of the bovine leukocyte adhesion deficiency (BLAD) demonstrated the risks of narrowing the genetic basis of a population. About 6\% of the Holstein-Friesian cattle now descends from one bull who was a heterozygous BLAD carrier. Crossing his descendants resulted in the birth of homozygous BLAD calves with a life expectancy of < 1 year. The BLAD syndrome is caused by a point mutation in the gene coding for CD18, a subunit of the beta 2 integrins on the surface of leukocytes. By using a PCR-RFLP test, large numbers of cattle are now being screened in several countries to eradicate the mutant allele. We describe an optimization of the PCR primer set that has led to an improvement of the test.",

author = "Mirck, \{M. H.\} and \{Von Bannisseht-Wijsmuller\}, T. and Timmermans-Besselink, \{W. J.\} and \{Van Luijk\}, \{J. H.\} and Buntjer, \{J. B.\} and Lenstra, \{J. A.\}",

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T1 - Optimization of the PCR test for the mutation causing bovine leukocyte adhesion deficiency.

AU - Mirck, M. H.

AU - Von Bannisseht-Wijsmuller, T.

AU - Timmermans-Besselink, W. J.

AU - Van Luijk, J. H.

AU - Buntjer, J. B.

AU - Lenstra, J. A.

PY - 1995/7/1

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N2 - The recent emergence of the bovine leukocyte adhesion deficiency (BLAD) demonstrated the risks of narrowing the genetic basis of a population. About 6% of the Holstein-Friesian cattle now descends from one bull who was a heterozygous BLAD carrier. Crossing his descendants resulted in the birth of homozygous BLAD calves with a life expectancy of < 1 year. The BLAD syndrome is caused by a point mutation in the gene coding for CD18, a subunit of the beta 2 integrins on the surface of leukocytes. By using a PCR-RFLP test, large numbers of cattle are now being screened in several countries to eradicate the mutant allele. We describe an optimization of the PCR primer set that has led to an improvement of the test.

AB - The recent emergence of the bovine leukocyte adhesion deficiency (BLAD) demonstrated the risks of narrowing the genetic basis of a population. About 6% of the Holstein-Friesian cattle now descends from one bull who was a heterozygous BLAD carrier. Crossing his descendants resulted in the birth of homozygous BLAD calves with a life expectancy of < 1 year. The BLAD syndrome is caused by a point mutation in the gene coding for CD18, a subunit of the beta 2 integrins on the surface of leukocytes. By using a PCR-RFLP test, large numbers of cattle are now being screened in several countries to eradicate the mutant allele. We describe an optimization of the PCR primer set that has led to an improvement of the test.

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SN - 0145-5680

VL - 41

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EP - 698

JO - Cellular and Molecular Biology

JF - Cellular and Molecular Biology

IS - 5

ER -

Optimization of the PCR test for the mutation causing bovine leukocyte adhesion deficiency.

Abstract

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