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芬兰艾尔夏牛中牛奶不凝固的潜在染色体区域。

Chromosomal regions underlying noncoagulation of milk in Finnish Ayrshire cows.

作者信息

Tyrisevä Anna-Maria, Elo Kari, Kuusipuro Arja, Vilva Veijo, Jänönen Isto, Karjalainen Heidi, Ikonen Tiina, Ojala Matti

机构信息

Department of Animal Science, University of Helsinki, FI-00014 Helsinki, Finland.

出版信息

Genetics. 2008 Oct;180(2):1211-20. doi: 10.1534/genetics.107.083964. Epub 2008 Sep 9.

Abstract

About 10% of Finnish Ayrshire cows produce noncoagulating milk, i.e., milk that does not form a curd in a standard 30-min testing time and is thus a poor raw material for cheese dairies. This phenomenon is associated with peak and midlactation, but some cows produce noncoagulating milk persistently. A genomewide scan under a selective DNA pooling method was carried out to locate genomic regions associated with the noncoagulation of milk. On the basis of the hypothesis of the same historical mutation, we pooled the data across sires. Before testing pools for homogeneity, allele intensities were corrected for PCR artifacts, i.e., shadow bands and differential amplification. Results indicating association were verified using daughter design and selective genotyping within families. Data consisted of 18 sire families with 477 genotyped daughters in total, i.e., 12% of each tail of the milk coagulation ability. Data were analyzed using interval mapping under maximum-likelihood and nonparametric methods. BMS1126 on chromosome 2 and BMS1355 on chromosome 18 were associated with noncoagulation of milk across families on an experimentwise 0.1% significance level. By scanning gene databases, we found two potential candidate genes: LOC538897, a nonspecific serine/threonine kinase on chromosome 2, and SIAT4B, a sialyltransferase catalyzing the last step of glycosylation of kappa-casein on chromosome 18. Further studies to determine the role of the candidates in the noncoagulation of milk are clearly needed.

摘要

约10%的芬兰艾尔夏奶牛产出不凝固的牛奶,即在标准30分钟测试时间内不能形成凝乳的牛奶,因此是奶酪加工厂的劣质原材料。这种现象与泌乳高峰期和中期有关,但一些奶牛持续产出不凝固的牛奶。采用选择性DNA混合方法进行全基因组扫描,以定位与牛奶不凝固相关的基因组区域。基于相同历史突变的假设,我们将公牛的数据进行了合并。在测试混合样本的同质性之前,对PCR假象(即影子条带和差异扩增)校正了等位基因强度。使用子代设计和家系内的选择性基因分型对表明存在关联的结果进行了验证。数据包括18个公牛家系,共有477个基因分型的子代,即牛奶凝固能力分布两端各12%的数据。使用最大似然法和非参数方法下的区间定位对数据进行了分析。在全实验0.1%的显著性水平上,2号染色体上的BMS1126和18号染色体上的BMS1355与全家族牛奶不凝固有关。通过扫描基因数据库,我们发现了两个潜在的候选基因:2号染色体上的LOC538897,一种非特异性丝氨酸/苏氨酸激酶;以及18号染色体上的SIAT4B,一种催化κ-酪蛋白糖基化最后一步的唾液酸转移酶。显然需要进一步研究以确定这些候选基因在牛奶不凝固中的作用。

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