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溶液杂交后通过部分RNA:DNA杂交体的电泳检测镰状细胞突变

Detection of sickle-cell mutation by electrophoresis of partial RNA:DNA hybrids following solution hybridization.

作者信息

Jones F S, Grimberg J I, Fischer S G, Ford J P

出版信息

Gene. 1985;39(1):77-83. doi: 10.1016/0378-1119(85)90110-6.

Abstract

We have developed a method in which partially single-stranded (ss) DNA molecules containing a defined region of duplex RNA:DNA are electrophoretically separated in agarose gels. The partial hybrids are formed by solution hybridization with a uniform length RNA probe complementary to part of the DNA sequence of interest. Following hybridization, the RNA/DNA mixture is fractionated by agarose gel electrophoresis at high temperature to minimize intrastrand base pairing which causes mobility heterogeneity. Not requiring the steps of DNA transfer from the gel to a solid support and subsequent probing, pre-electrophoretic hybridization allows the direct identification of single-copy fragments. Conditions for the detection of single-copy genes in human DNA digested with specific restriction endonucleases were developed and applied to the diagnosis of sickle-cell disease. This method should be applicable for the analysis of DNAs of high complexity where the presence of DNA polymorphisms and interspersed repeated DNA sequences often make impossible the creation of complete RNA:DNA hybrids.

摘要

我们开发了一种方法,其中含有特定双链RNA:DNA区域的部分单链(ss)DNA分子在琼脂糖凝胶中进行电泳分离。部分杂交体通过与与感兴趣的DNA序列部分互补的均匀长度RNA探针进行溶液杂交形成。杂交后,RNA/DNA混合物在高温下通过琼脂糖凝胶电泳进行分级分离,以尽量减少导致迁移率异质性的链内碱基配对。预电泳杂交不需要将DNA从凝胶转移到固体支持物并随后进行探测的步骤,可直接鉴定单拷贝片段。开发了用于检测用特定限制性内切酶消化的人类DNA中单个拷贝基因的条件,并将其应用于镰状细胞病的诊断。该方法应适用于分析高复杂性DNA,在这种情况下,DNA多态性和散布的重复DNA序列的存在常常使得无法形成完整的RNA:DNA杂交体。

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