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The canine major histocompatibility complex
Authors:Robert F.  Raff H. Joachim  Deeg VERNON T. Farewell   Susan  DeRose Rainer  Storb
Affiliation:The Fred Hutchinson Cancer Research Center and the Division of Oncology, Department of Medicine and Department of Biostatistics, University of Washington School of Medicine, Seattle, Washington, U.S.A.
Abstract:
The frequencies of 12 DLA-D alleles in a random canine population were determined in one-way mixed lymphocyte cultures using a panel of homozygous typing cells established in this laboratory. The homozygous typing cells served as stimulators for responder lymphocytes obtained from 160 random dogs. The results of these studies were compared to those with lymphocytes from 75 dogs in our research laboratory. DLA-D allelic frequencies were estimated by maximum likelihood techniques. The use of a relative response (RR) ≫5% as a definition of a typing response resulted in the recognition of a total allele frequency of 59% in dogs from the research laboratory. Three of the 12 DLA-D alleles were not detected. Typing responses of cells from random dogs to the 12 DLA-D alleles were determined using RRs °5%, °10%, °15%, and °20%. With RRs of °5%, °10%, and °15%, the total allele frequencies recognized were 39%, 47%, and 55%, respectively. Within each of these %RR ranges all but one of the DLA-D alleles were detected. With an RR °20% the total allele frequency recognized was 58% and all 12 alleles were detected. Our results indicate that an RR of °10% could be used to define a phenotypic DLA-D typing response in the dog. The level of allelic frequencies detected in both the research and random canine populations indicates the need to identify additional DLA-D alleles through expanded family studies using mixed lymphocyte culture and homozygous cell typing.
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