CAJ | 학술논문

从福建某奶牛场250头进口荷斯坦牛采血提取牛血液DNA，根据已知牛染色体上CD18编码基因序列383位碱基由A 变为G 而引起牛白细胞粘附缺陷病设计特异性野生型和突变型探针，建立实时荧光定量PC R 检测方法用于牛白细胞粘附缺陷病的基因分型检测。结果检出2头母牛为牛白细胞粘附缺陷病携带者，检出率为0.8%，没有发现患病牛。结果证明本研究建立的实时荧光定量PC R 检测方法是一种敏感性和特异性很高的筛选奶牛牛白细胞粘附缺陷病有害基因的新方法。
종복건모내우장250두진구하사탄우채혈제취우혈액DNA，근거이지우염색체상CD18편마기인서렬383위감기유A 변위G 이인기우백세포점부결함병설계특이성야생형화돌변형탐침，건립실시형광정량PC R 검측방법용우우백세포점부결함병적기인분형검측。결과검출2두모우위우백세포점부결함병휴대자，검출솔위0.8%，몰유발현환병우。결과증명본연구건립적실시형광정량PC R 검측방법시일충민감성화특이성흔고적사선내우우백세포점부결함병유해기인적신방법。
A MGB two probe assay based on real-time PCR was developed and applied to detect bovine leukocyte adhesion deficiency in Holstein cows. Atotal of 250 Holstein cows im ported from foreign countries were genotyped. Two cows were identified as BLAD carriers, corresponding to the carrier frequency 0.8% , there was no patient cow. The results showed that MGB two probe assay based on real-time PCR is anew sensitive and specific assay for genotyping BLAD .