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在一个跨度为1.2兆碱基对的酵母人工染色体重叠群中对1型脊髓小脑共济失调基因(SCA1)关键区域进行定位和克隆。

Mapping and cloning of the critical region for the spinocerebellar ataxia type 1 gene (SCA1) in a yeast artificial chromosome contig spanning 1.2 Mb.

作者信息

Banfi S, Chung M Y, Kwiatkowski T J, Ranum L P, McCall A E, Chinault A C, Orr H T, Zoghbi H Y

机构信息

Department of Pediatrics, Baylor College of Medicine, Houston, Texas 77030.

出版信息

Genomics. 1993 Dec;18(3):627-35. doi: 10.1016/s0888-7543(05)80365-9.

Abstract

The gene responsible for spinocerebellar ataxia type 1 (SCA1) has been localized to a 6.7-cM region between the centromeric marker D6S109 and the telomeric marker D6S89. We screened two yeast artificial chromosome (YAC) libraries using sequence-tagged sites at D6S89 and at newly identified markers in 6p22-p23. Fifty YAC clones were identified and 34 insert termini were isolated from some of these YACs for detailed overlap mapping and long-range restriction analysis. A large YAC contig estimated to span 2.5 Mb was developed and genetic analysis in five large SCA1 kindreds using highly informative dinucleotide repeat polymorphisms mapped to this contig allowed the identification of D6S274 as the closest centromeric flanking marker for SCA1. Long-range restriction analysis determined the size for the critical SCA1 region, as defined by the two flanking markers D6S274 and D6S89, to be 1.2 Mb. This region is spanned by a minimum set of four nonchimeric YAC clones. The development of a 2.5-Mb YAC contig in 6p22-p23 provides valuable reagents for characterization of this genomic region and for the cloning of the SCA1 gene.

摘要

导致1型脊髓小脑共济失调(SCA1)的基因已被定位到着丝粒标记D6S109和端粒标记D6S89之间6.7厘摩的区域。我们使用D6S89以及6p22 - p23中新鉴定标记的序列标签位点筛选了两个酵母人工染色体(YAC)文库。鉴定出50个YAC克隆,并从其中一些YAC中分离出34个插入末端用于详细的重叠图谱绘制和长程限制性分析。构建了一个估计跨度为2.5兆碱基的大型YAC重叠群,并且利用定位到该重叠群上的信息丰富的二核苷酸重复多态性对五个大型SCA1家系进行遗传分析,从而确定D6S274为SCA1最靠近着丝粒的侧翼标记。长程限制性分析确定了由两个侧翼标记D6S274和D6S89界定的关键SCA1区域大小为1.2兆碱基。该区域由最少四个非嵌合YAC克隆覆盖。在6p22 - p23构建的2.5兆碱基YAC重叠群为该基因组区域的特征描述以及SCA1基因的克隆提供了有价值的试剂。

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