摘要
目的应用分子生物学技术建立人类颞骨火棉胶切片中的DNA分析方法。方法采用多聚酶链反应(polymerasechainreaction,PCR)配合不同的引物、扩增方式及酶切技术检测长期保存的7例(9侧)颞骨火棉胶切片中微量线粒体DNA的片段缺失及点突变,pGEMT载体进行扩增片段的重组与克隆。结果9侧颞骨DNA提取液中均可见正常的135bp扩增片段,巢式PCR检出其中2例生前患老年聋者(各查1侧)有线粒体DNA大片段缺失,测序结果证实扩增的准确性。结论分子生物学技术在颞骨切片研究中的应用对于提高其回顾性研究水平有重要意义,目前可在耳科疾病的研究中发现相关的基因突变或病原体。
Objective To establish an analytical method of DNA extracted from human celloidinembedded temporal bone sections by molecular biologic technique. Methods Polymerase chain reaction (PCR) with different primers,special amplification methods or coorperated with enzyme restricted reactions was adapted to detect several types of genetic mutations from 9 human celloidinembedded temporal bone sections. The pGEMT vector was used for the recombination and cloning of the amplified DNA fragment. Results The 135 bp fragments of normal mtDNA were detected from all of the 9 cases. The 316bp fragment related to mtDNA 4977bp deletion was also detected in two cases who suffered from presbycusis before death by the nested PCR.The result of sequencing confirmed the accuracy of PCR. Conclusion The application of molecular biologic techniques in temporal bone research is important in improving the quality and value of retrospective study of ear diseases and has resulted in findings of the relevant mutant or pathogenetic genes in the ear diseases such as presbycusis, ototoxic deafness, otosclerosis and viral infections of the ear.
出处
《中华耳鼻咽喉科杂志》
CSCD
1998年第4期206-209,共4页
Chinese Journal of Otorhinolaryngology
关键词
颞骨
线粒体
DNA
重组
聚合酶链反应
介力疾病
Temporal bone DNA,mitochondrial DNA,recombinant Polymerase chain reaction
