Department of Genetics, The Scripps Research Institute, La Jolla, California 92037, USA.
Genetics. 2010 Dec;186(4):1139-46. doi: 10.1534/genetics.110.121160. Epub 2010 Oct 5.
Phenovariance may be obscured when genetic mapping is performed using highly divergent strains, and closely similar strains are preferred if adequate marker density can be established. We sequenced the C57BL/10J mouse genome using the Applied Biosystems SOLiD platform and here describe a genome-wide panel of informative markers that permits the mapping of mutations induced on the closely related C57BL/6J background by outcrossing to C57BL/10J, and backcrossing or intercrossing. The panel consists of 127 single nucleotide polymorphisms validated by capillary sequencing: 124 spaced at ∼20-Mb intervals across the 19 autosomes, and three markers on the X chromosome. We determined the genetic relationship between four C57BL-derived substrains and used the panel to map two N-ethyl-N-nitrosourea (ENU)-induced mutations responsible for visible phenotypes in C57BL/6J mice through bulk segregation analysis. Capillary sequencing, with computation of relative chromatogram peak heights, was used to determine the proportion of alleles from each strain at each marker.
表型变异可能会在使用高度分化的品系进行遗传作图时被掩盖,如果能够建立足够的标记密度,则优选密切相关的品系。我们使用 Applied Biosystems SOLiD 平台对 C57BL/10J 小鼠基因组进行了测序,在此我们描述了一个全基因组信息标记面板,该面板允许对通过与 C57BL/10J 进行杂交、回交或杂交而在密切相关的 C57BL/6J 背景上诱导的突变进行作图。该面板由通过毛细管测序验证的 127 个单核苷酸多态性组成:124 个分布在 19 条常染色体上,每个约 20-Mb 间隔,X 染色体上有三个标记。我们确定了四个源自 C57BL 的亚系之间的遗传关系,并使用该面板通过群体分离分析对两个 N-乙基-N-亚硝脲(ENU)诱导的突变进行了作图,这些突变导致 C57BL/6J 小鼠出现可见表型。我们使用毛细管测序和相对色谱峰高度的计算来确定每个标记处每个品系的等位基因比例。
