K. Walawski scite author profile

K. Walawski

5Publications

54Citation Statements Received

47Citation Statements Given

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Affiliations

Institute of Animal Reproduction and Food Research, University of Warmia and Mazury in Olsztyn, Dr Emilio B Espinosa Sr Memorial State College of Agriculture and Technology

Publications

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Deletion/insertion polymorphism of the prion protein gene (PRNP) in Polish Holstein-Friesian cattle

et al. 2007

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The aim of the present study was to identify the deletion/insertion polymorphism of the bovine prion protein gene (PRNP) within the promoter sequence (23 bp), intron 1 (12 bp) and 3' untranslated region (14 bp). DNA was isolated from blood of 234 randomly tested Polish Holstein-Friesian cows and from semen of 47 sires used for artificial insemination (AI) in 2004. No statistically significant differences were found in the frequency of genotypes and alleles between cows and breeding bulls in the 3 analysed polymorphic sites within the PRNP gene. Only 3 haplotypes were identified in sires and 4 haplotypes in cows.

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Application of disease-associated differentially expressed genes – Mining for functional candidate genes for mastitis resistance in cattle

Schwerin¹,

Czernek-Schäfer²,

Goldammer³

et al. 2003

Genet. Sel. Evol.

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-In this study the mRNA differential display method was applied to identify mastitisassociated expressed DNA sequences based on different expression patterns in mammary gland samples of non-infected and infected udder quarters of a cow. In total, 704 different cDNA bands were displayed in both udder samples. Five hundred-and-thirty two bands, (75.6%) were differentially displayed. Ninety prominent cDNA bands were isolated, re-amplified, cloned and sequenced resulting in 87 different sequences. Amongst the 19 expressed sequence tags showing a similarity with previously described genes, the majority of these sequences exhibited homology to protein kinase encoding genes (26.3%), to genes involved in the regulation of gene expression (26.3%), to growth and differentiation factor encoding genes (21.0%) and to immune response or inflammation marker encoding genes (21.0%). These sequences were shown to have mastitis-associated expression in the udder samples of animals with and without clinical mastitis by quantitative RT-PCR. They were mapped physically using a bovine-hamster somatic cell hybrid panel and a 5000 rad bovine whole genome radiation hybrid panel. According to their localization in QTL regions based on an established integrated marker/gene-map and their disease-associated expression, four genes (AHCY, PRKDC, HNRPU, OSTF1) were suggested as potentially involved in mastitis defense. mastitis / expressed sequence tag / gene expression / cattle / RH mapping

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Co‐segregation of alleles at a microsatellite locus within the macrophage expressed lysozyme gene and levels of serum lysozyme activity in two half‐sib families of Polish Black and White Lowland cattle

Pareek¹,

Walawski²,

Czarnik³

et al. 1998

Animal Genetics

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Alleles at a microsatellite locus within the macrophage expressed lysozyme gene were shown to co-segregate with lysozyme activity in two half-sib families of Polish Black and White Lowland cattle. The bimodal distribution of lysozyme activities in both progeny groups is concordant with the occurrence of the alternative paternal alleles. The microsatellite is linked to a locus for high lysozyme activity that accounts for 70-95% of the phenotypic variation of both offspring groups considering the lysozyme activities of animals being older than 1 month.

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Application of disease-associated differentially expressed genes – Mining for functional candidate genes for mastitis resistance in cattle

et al. 2003

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In this study the mRNA differential display method was applied to identify mastitis-associated expressed DNA sequences based on different expression patterns in mammary gland samples of non-infected and infected udder quarters of a cow. In total, 704 different cDNA bands were displayed in both udder samples. Five hundred-and-thirty two bands, (75.6%) were differentially displayed. Ninety prominent cDNA bands were isolated, re-amplified, cloned and sequenced resulting in 87 different sequences. Amongst the 19 expressed sequence tags showing a similarity with previously described genes, the majority of these sequences exhibited homology to protein kinase encoding genes (26.3%), to genes involved in the regulation of gene expression (26.3%), to growth and differentiation factor encoding genes (21.0%) and to immune response or inflammation marker encoding genes (21.0%). These sequences were shown to have mastitis-associated expression in the udder samples of animals with and without clinical mastitis by quantitative RT-PCR. They were mapped physically using a bovine-hamster somatic cell hybrid panel and a 5000 rad bovine whole genome radiation hybrid panel. According to their localization in QTL regions based on an established integrated marker/gene-map and their disease-associated expression, four genes (AHCY, PRKDC, HNRPU, OSTF1) were suggested as potentially involved in mastitis defense.

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Polymorphism of alkaline ribonuclease in the leucocytes of Black‐and‐White cattle

Walawski

Prusinowska

1981

Animal Blood Groups and Biochemical Genetics

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K. Walawski

Deletion/insertion polymorphism of the prion protein gene (PRNP) in Polish Holstein-Friesian cattle

Application of disease-associated differentially expressed genes – Mining for functional candidate genes for mastitis resistance in cattle

Co‐segregation of alleles at a microsatellite locus within the macrophage expressed lysozyme gene and levels of serum lysozyme activity in two half‐sib families of Polish Black and White Lowland cattle

Application of disease-associated differentially expressed genes – Mining for functional candidate genes for mastitis resistance in cattle

Polymorphism of alkaline ribonuclease in the leucocytes of Black‐and‐White cattle

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