摘要
目的对我们发现的中国人Brugada综合征新的SCN5A基因突变K317N进行体外定点诱变研究,并构建携带有基因突变K317N的pRc/CMV-hH1的表达载体。方法采用PCR定点突变技术,根据突变位置附近的两个单一限制性内切酶位点AgeI/Sse8387I设计一对定点诱变引物,将突变位点设计在引物上,通过PCR扩增,使扩增片段上含有所需要的突变位点,最后将扩增片段克隆入pRc/CMV-hH1载体中。结果DNA测序表明,在预期位点巳经发生突变,SCN5A基因在第317密码子由赖氨酸(K)突变为天冬氨酸(N),成功实现定点诱变。结论PCR技术诱导定点突变,准确、高效。pRc/CMV-hH1(K317N)的成功构建,为进一步进行该突变的结构与功能研究奠定了基础。
Objective To perform PCR-based site-directed mutagenesis of a new SCN5A mutation (K317N) identified in a Chinese family with Brugada syndrome and construct the recombinant expression plasmid pRc/CMV-Hh1containing the human cardiac sodium channel α subunit (hH1), mutant cDNA. Methods A pair of primers was designed according to the restricted sites Sse 8387I and Age I of the SCN5A sequence with the mismatches introduced into primers. Mutagenesis was performed in a single-step PCR, and the fragments amplified by PCR containing the mutation site were subcloned into the pRc/CMV-hH1 vector. Results Sequence analysis confirmed the presence of the desired mutation site, and a mutation from K (Lys) to N (Asn) in codon 317 was identified in the SCN5A gene, indicating the successful induction of the mutation at K317N of the SCN5A gene. Conclusion PCR site-directed mutagensis is accurate and highly efficient, and the successfully constructed recombinant expression plasmid pRc/CMV-hH1 (K317N) may provide a molecular basis for further functional and genomic investigation of SCN5A.
出处
《第一军医大学学报》
CSCD
北大核心
2003年第11期1139-1142,共4页
Journal of First Military Medical University
基金
国家自然科学基金(30278368)
广东省自然科学基金(20042)~~
