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Identification of polymorphisms by genomic denaturing gradient gel electrophoresis: application to the proximal region of human chromosome 21

机译:通过基因组变性梯度凝胶电泳鉴定多态性:应用于人类21号染色体的近端区域。

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Genomic Denaturing Gradient Gel Electrophoresis (gDGGE) provides an alternative to the standard method of restriction fragment length polymorphism (RFLP) analysis for identifying polymorphic sequence variation in genomic DNA. For gDGGE, genomic DNA is cleaved by restriction enzymes, separated in a polyacrylamide gel containing a gradient of DNA denaturants, and then transferred by electroblotting to nylon membranes. Unlike other applications of DGGE, gDGGE is not limited by the size of the probe and does not require probe sequence information. gDGGE can be used in conjunction with any unique DNA probe. Here we use gDGGE with probes from the proximal region of the long arm of human chromosome 21 to identify polymorphic DNA sequence variation in this segment of the chromosome. Our screening panel consisted of DNA from nine individuals, which was cleaved with five restriction enzymes and submitted to electrophoresis in two denaturing gradient conditions. We detected at least one potential polymorphism for nine of eleven probes that were tested. Two polymorphisms, one at D21S4 and one at D21S90, were characterized in detail. Our study demonstrates that gDGGE is a fast and efficient method for identifying polymorphisms that are useful for genetic linkage analysis.
机译:基因组变性梯度凝胶电泳(gDGGE)为限制基因组片段长度多态性(RFLP)分析的标准方法提供了一种替代方法,用于鉴定基因组DNA中的多态性序列变异。对于gDGGE,基因组DNA被限制性酶切割,在含有梯度DNA变性剂的聚丙烯酰胺凝胶中分离,然后通过电印迹转移到尼龙膜上。与DGGE的其他应用程序不同,gDGGE不受探针大小的限制,并且不需要探针序列信息。 gDGGE可与任何独特的DNA探针结合使用。在这里,我们将gDGGE与人类21号染色体长臂近端的探针一起使用,以鉴定该染色体片段中的多态性DNA序列变异。我们的筛选小组由来自9个个体的DNA组成,这些DNA被5种限制酶切割并在两种变性梯度条件下进行了电泳。我们检测了11个探针中的9个探针的至少一种潜在多态性。详细描述了两种多态性,一种在D21S4,一种在D21S90。我们的研究表明,gDGGE是一种快速有效的方法,可用于鉴定对遗传连锁分析有用的多态性。

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