For genotyping of feline major histocompatibility complex (FLA) class II DRB, the polymerase chain reaction (PCR)-restriction fragment length polymorphism (RFLP) method using group-specific primers was tried. Sixty-six DRB genes were classified into 8 groups according to differences in the first 5' amino acid sequences. The group-specific primers were designed as forward ones, which were specific for 5' base sequences of genes in each group. Three to 7 appropriate restricted enzymes were selected by computer analysis for RFLP typing of the genes divided into each group. In 6 out of 9 cats, the results of DRB typed by direct sequence method agreed with results of the PCR-RFLP method using group-specific primers. In the other 3 cats, the number of genes amplified by group-specific primers was I or 2 more than those detected by direct sequence method. The direct sequence method in 9 cats identified 5 new FLA-DRB genes. The PCR-RFLP method using group-specific primers could divide 66 genes into 37 genes and 10 subgroups from the RFLP pattern. One to 6 genes in each cat, and a total of 203 genes and subgroups were detected in 68 domestic cats. The genes detected might be biased to the subgroup G1-1a (28.8%), DRB*0501 (10.3%), G1-2a (9.4%) and G6b (7.4%). The PCR-RFLP method using group-specific primers may be useful in typing FLA class II DRB.
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http://dx.doi.org/10.1292/jvms.62.1283 | DOI Listing |
Trop Anim Health Prod
January 2025
Department of Micrology, College of Medicine, Taif University, Taif, 21944, Egypt.
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November 2024
Plant and Forest Health Unit, Life Sciences Department, Walloon Agricultural Research Centre, Rue de Liroux 2, 5030, Gembloux, Belgium.
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September 2024
Department of Laboratory Medicine, National Taiwan University Hospital, Taipei, Taiwan.
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July 2024
Department of Bioinformatics, University of British Columbia, Vancouver, British Columbia, Canada.
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Department of Pharmacy, University of Salerno, I-84084 Fisciano, Italy.
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