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Molecular methods for the detection of mutations.

机译:用于检测突变的分子方法。

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摘要

We report the results of a collaborative study aimed at developing reliable, direct assays for mutation in human cells. The project used common lymphoblastoid cell lines, both with and without mutagen treatment, as a shared resource to validate the development of new molecular methods for the detection of low-level mutations in the presence of a large excess of normal alleles. As the "gold standard, " hprt mutation frequencies were also measured on the same samples. The methods under development included i) the restriction site mutation (RSM) assay, in which mutations lead to the destruction of a restriction site; ii) minisatellite length-change mutation, in which mutations lead to alleles containing new numbers of tandem repeat units; iii) loss of heterozygosity for HLA epitopes, in which antibodies can be used to direct selection for mutant cells; iv) multiple fluorescence-based long linker arm nucleotides assay (mf-LLA) technology, for the detection of substitutional mutations; v) detection of alterations in the TP53 locus using a (CA) array as the target for the screening; and vi) PCR analysis of lymphocytes for the presence of the BCL2 t(14:18) translocation. The relative merits of these molecular methods are discussed, and a comparison made with more "traditional" methods.
机译:我们报告了一项旨在开发可靠,直接的人类细胞突变检测方法的合作研究结果。该项目使用经过诱变处理或未经诱变处理的常见淋巴母细胞系作为共享资源,以验证开发了用于在存在大量过量正常等位基因的情况下检测低水平突变的新分子方法。作为“金标准”,还对相同样品测量了hprt突变频率。正在开发的方法包括:i)限制性位点突变(RSM)分析,其中的突变导致限制性位点的破坏; ii)小卫星长度变化突变,其中突变导致等位基因包含新数目的串联重复单元; iii)HLA表位的杂合性丧失,其中抗体可用于指导突变细胞的选择; iv)多种基于荧光的长接头臂核苷酸测定技术(mf-LLA),用于检测取代突变; v)使用(CA)阵列作为筛选目标来检测TP53基因座中的改变; vi)淋巴细胞的PCR分析中是否存在BCL2 t(14:18)易位。讨论了这些分子方法的相对优点,并与更多“传统”方法进行了比较。

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