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作 者:门美超[1] 薛晋杰[2] 蒋璐[1] 王鸿涵[1] 潘乾[2] 冯永[1]
机构地区:[1]中南大学湘雅医院耳鼻咽喉科,长沙410008 [2]中南大学中国医学遗传学国家重点实验室,长沙410078
出 处:《中南大学学报(医学版)》2011年第11期1079-1084,共6页Journal of Central South University :Medical Science
基 金:supported by 11th 5-Year Plan(2007BAI18B13);the National Natural Science Foundation of China(30671150;81170923);“863”Program(2007AA02Z445),P.R.China
摘 要:目的:探寻在不同人群中应用快速、准确的检测非综合征性耳聋的方法。方法:将引物延伸及变性高效液相色谱法相结合,检测180例中国人群的6种常见耳聋突变点(GJB2-235delC,GJB2-299delAT,PDS-A2168G,PDS IVS7-2A>G,mtDNA-A1555G,以及mtDNA-C1494T)。PCR扩增的靶序列,经引物延伸,得到中国人遗传性非综合征性耳聋6个常见突变的特异性延伸片段,用全变性高效液相色谱分析延伸片段混合物,分离图谱可鉴定被检样本的基因型。结果:盲法分析显示180例样品的引物延伸变性高效液相色谱法与直接测序法检测结果完全符合。结论:该法是一种准确、高效的检测非综合征性遗传性耳聋突变的分析方法,并可以探讨将其应用到其他遗传病的检测中。Objective To find a rapid and accurate genotyping method for specific non-syndromic hearing loss(NSHL)-causing gene mutations for disease diagnosis in different ethnic populations.Methods We performed a novel multiplex primer extension(PE) reaction in combination with denaturing high-performance liquid chromatography(DHPLC) to simultaneously detect and genotype the 6 most common mutations in 180 patients with NSHL(GJB2-235delC,GJB2-299delAT,PDS-A2168G,PDS IVS7-2AG,mtDNA-A1555G,and mtDNA-C1494T) in Chinese population.This method involved the amplification of the target sequence,followed by a purification step,a multiplex PE reaction,and DHPLC analysis performed on the Transgenomic Wave DNA fragment analysis system under fully-denaturing conditions.Results In a blind analysis,this technique successfully and accurately genotyped 100% of the samples simultaneously characterized by direct sequencing.Conclusion Combination of PE and DHPLC is simple,rapid,accurate,and cost-effective for genotyping common disease-causing mutations,including substitutions,insertions,and deletions in NSHL,and may be successfully used in other genetic diseases.
关 键 词:遗传性耳聋 变性高效液相色谱 基因突变 引物延伸
分 类 号:R764.43[医药卫生—耳鼻咽喉科]
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