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利用PCR-RF-SSCP技术检测水稻蜡质突变体中的突变

Mutation detection in rice waxy mutants by PCR-RF-SSCP.

作者信息

Sato Y, Nishio T

机构信息

Graduate School of Agricultural Science, Tohoku University, Sendai 981-8555, Japan.

出版信息

Theor Appl Genet. 2003 Aug;107(3):560-7. doi: 10.1007/s00122-003-1282-4. Epub 2003 May 7.

DOI:10.1007/s00122-003-1282-4
PMID:12734656
Abstract

PCR-RF-SSCP (PRS), which combines cleaved amplified polymorphic sequence (CAPS) and single-strand conformation polymorphism (SSCP), is expected to be a useful technique for DNA polymorphism analysis. We evaluated the ability of PRS to detect single nucleotide polymorphism (SNP) using the Waxy gene, Wx, of rice, and subsequently were able to identify point mutations in wx mutant lines. The approximately 6-kb Wx gene was divided into five regions for PCR amplification. Two regions, in which most of the point mutations of the wx mutants have been identified, were amplified by PCR and cloned into a vector, and those clones containing SNPs produced as a result of the inherent inaccuracy of PCR were used for the evaluation of PRS. The efficiency of PRS in the detection of SNPs of these clones was over 70%. PRS analysis of the wx genes in 18 waxy mutants was carried out in the five regions using two different restriction endonucleases and two gel conditions, with and without glycerol. Of the 18 lines tested, 17 showed band patterns different from that of the wild type. Most of the mutations identified in this study were nucleotide changes in exons, which result in amino acid changes. One mutation generated an in-frame stop codon, and another was a frame shift mutation by one-base deletion. Two mutations found at a splice site were considered to inhibit normal splicing of mRNA. These results show that PRS is a useful technique for detecting point mutations in large plant genes.

摘要

聚合酶链反应-限制性片段-单链构象多态性分析(PRS)结合了酶切扩增多态性序列(CAPS)和单链构象多态性(SSCP),有望成为一种用于DNA多态性分析的有用技术。我们利用水稻的蜡质基因Wx评估了PRS检测单核苷酸多态性(SNP)的能力,随后能够鉴定wx突变系中的点突变。将约6kb的Wx基因分为五个区域进行PCR扩增。通过PCR扩增并克隆到载体中的两个区域,其中已鉴定出大多数wx突变体的点突变,并且将那些由于PCR固有不准确性而产生SNP的克隆用于PRS评估。这些克隆的SNP检测中PRS的效率超过70%。使用两种不同的限制性内切酶和两种凝胶条件(含甘油和不含甘油),在五个区域对18个蜡质突变体中的wx基因进行了PRS分析。在测试的18个品系中,17个显示出与野生型不同的条带模式。本研究中鉴定出的大多数突变是外显子中的核苷酸变化,导致氨基酸变化。一个突变产生了框内终止密码子,另一个是单碱基缺失导致的移码突变。在剪接位点发现的两个突变被认为会抑制mRNA的正常剪接。这些结果表明,PRS是检测大型植物基因中点突变的有用技术。

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