用聚丙烯酰胺凝胶电泳快速鉴定扩增的人hprt cDNA突变

Fátima Garganta, Günter Krause, Gerhard Scherer
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引用次数: 3

摘要

编制hprt突变谱需要对大量6-硫鸟嘌呤抗性克隆进行分离和分析,以确定特征点突变。由于cDNA扩增在大多数突变体分类方案中是强制性的中间产物,我们建议用聚丙烯酰胺凝胶电泳对其进行初步鉴定,以快速区分克隆和独立突变体,并简化突变体分析程序。基于人类hprt cDNA序列,开发了一种利用少量限制性内切酶分析消化来定位缺失外显子的策略。在突变体分类方案中,alui酶切cDNA扩增片段的聚丙烯酰胺凝胶电泳提高了检测大小减小的RT-PCR产物的敏感性,例如缺失外显子5的情况。对109个独立突变克隆的cDNA扩增片段进行限制性内切分析,结果显示,与自发或bap诱导的突变体相比,NNK诱导后外显子丢失显著增加。对39个独立突变PCR产物进行的cDNA扩增外显子损失测定,可能直接指向携带导致异常剪接的点突变的基因组靶序列,从而消除了费力的包含所有外显子的多重PCR的需要。对已知的5个点突变进行单链构象多态性(SSCP)分析,获得了包含hprt cDNA外显子7和8的亚扩增子。双链PCR产物经过热和碱复合变性后,样品在非变性条件下用预铸聚丙烯酰胺凝胶分离。包括C508T热点突变在内,扩增区域内已知的5个核苷酸替换导致单链带相对于野生型模式的迁移率发生变化。
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Rapid characterization of mutations in amplified human hprt cDNA by polyacrylamide gel electrophoresis

Compiling hprt mutation spectra involves the isolation and analysis of numerous 6-thioguanine-resistant clones for identifying characteristic point mutations. Since cDNA amplificates are compulsary intermediates in most mutant classification protocols, we suggest their preliminary characterization by polyacrylamide gel electrophoresis for the rapid distinction of clonal and independent mutants and for streamlining mutant analysis procedures. Based on the human hprt cDNA sequence a strategy was developed for mapping missing exons by analytical digests with a small panel of restriction enzymes. In mutant classification schemes, polyacrylamide gel electrophoresis of AluI-digested cDNA amplificates increased the sensitivity for detecting RT-PCR products of reduced size, e.g., in the case of missing exon 5. Restriction analysis of cDNA amplificates from 109 independent mutant clones showed a significant increase of exon loss after NNK induction as compared to spontaneous or BaP-induced mutants. The determination of exon loss from cDNA amplificates, as carried out for 39 independent mutant PCR products, might direct towards the genomic target sequences carrying the point mutations, that caused the aberrant splicing, thus eliminating the need of laborious multiplex PCR comprising all exons. For single-strand conformation polymorphism (SSCP) analysis of five known point mutations, sub-amplificates comprising exons 7 and 8 of hprt cDNA were obtained. After a combined heat and alkali denaturation of the double-stranded PCR products, the samples were separated in pre-cast polyacrylamide gels under non-denaturing conditions. Five known nucleotide substitutions within the amplified region, including the C508T hot spot mutation, resulted in mobility shifts of single-strand bands relative to the wild type pattern.

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VOLUME CONTENTS Comprehensive analysis of a large genomic sequence at the putative B-cell chronic lymphocytic leukaemia (B-CLL) tumour suppresser gene locus Mutational analysis within the 3′ region of the PKD1 gene in Japanese families Allelic polymorphisms in the transcriptional regulatory region of human SEL1L CUMULATIVE AUTHOR INDEX FOR MUTNOM 2000
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