中华耳科学杂志
中華耳科學雜誌
중화이과학잡지
CHINESE JOURNAL OF OTOLOGY
2013年
1期
14-18
,共5页
张治华%孙莲花%陈洪赛%汪照炎%杨涛%吴皓
張治華%孫蓮花%陳洪賽%汪照炎%楊濤%吳皓
장치화%손연화%진홍새%왕조염%양도%오호
听神经瘤%NF2基因%突变
聽神經瘤%NF2基因%突變
은신경류%NF2기인%돌변
Acoustic neuroma%NF2 gene%mutation
目的明确中国人群听神经瘤中NF2基因突变和大片段缺失比例及其意义.方法收集2007年1月至2010年12月期间84例散发型听神经瘤标本组织,采用标准测序检测患者肿瘤组织和外周血中NF2基因突变,并对其中30例综合采用多重连接依赖探针扩增技术(multiple ligation-dependant probe amplification,MLPA)检测NF2基因大片段缺失.结果标准测序检测听神经瘤组织NF2基因突变率为39.3%,外周血中突变率为零;移码、剪切位点、无义、错义突变比例分别为48.5%、21.2%、24.2%和6.1%,突变分布于第1-15外显子,第8外显子为突变高发外显子(15.2%).氨基端、链接区、α-螺旋结构区、羧基端突变分别占总突变率的63.6%、6.1%、21.2%和6.1%.MLPA检测发现NF2基因大片段缺失达73.3%,以氨基端为主(56.7%).标准测序法结合MLPA法测得NF2基因大片段和突变率累计达80.0%.结论散发型听神经瘤中NF2基因突变和大片段缺失率高,且均为体细胞突变.采用标准测序和MLPA结合技术,有助于提高NF2基因突变检出率和精确性.
目的明確中國人群聽神經瘤中NF2基因突變和大片段缺失比例及其意義.方法收集2007年1月至2010年12月期間84例散髮型聽神經瘤標本組織,採用標準測序檢測患者腫瘤組織和外週血中NF2基因突變,併對其中30例綜閤採用多重連接依賴探針擴增技術(multiple ligation-dependant probe amplification,MLPA)檢測NF2基因大片段缺失.結果標準測序檢測聽神經瘤組織NF2基因突變率為39.3%,外週血中突變率為零;移碼、剪切位點、無義、錯義突變比例分彆為48.5%、21.2%、24.2%和6.1%,突變分佈于第1-15外顯子,第8外顯子為突變高髮外顯子(15.2%).氨基耑、鏈接區、α-螺鏇結構區、羧基耑突變分彆佔總突變率的63.6%、6.1%、21.2%和6.1%.MLPA檢測髮現NF2基因大片段缺失達73.3%,以氨基耑為主(56.7%).標準測序法結閤MLPA法測得NF2基因大片段和突變率纍計達80.0%.結論散髮型聽神經瘤中NF2基因突變和大片段缺失率高,且均為體細胞突變.採用標準測序和MLPA結閤技術,有助于提高NF2基因突變檢齣率和精確性.
목적명학중국인군은신경류중NF2기인돌변화대편단결실비례급기의의.방법수집2007년1월지2010년12월기간84례산발형은신경류표본조직,채용표준측서검측환자종류조직화외주혈중NF2기인돌변,병대기중30례종합채용다중련접의뢰탐침확증기술(multiple ligation-dependant probe amplification,MLPA)검측NF2기인대편단결실.결과표준측서검측은신경류조직NF2기인돌변솔위39.3%,외주혈중돌변솔위령;이마、전절위점、무의、착의돌변비례분별위48.5%、21.2%、24.2%화6.1%,돌변분포우제1-15외현자,제8외현자위돌변고발외현자(15.2%).안기단、련접구、α-라선결구구、최기단돌변분별점총돌변솔적63.6%、6.1%、21.2%화6.1%.MLPA검측발현NF2기인대편단결실체73.3%,이안기단위주(56.7%).표준측서법결합MLPA법측득NF2기인대편단화돌변솔루계체80.0%.결론산발형은신경류중NF2기인돌변화대편단결실솔고,차균위체세포돌변.채용표준측서화MLPA결합기술,유조우제고NF2기인돌변검출솔화정학성.
Objective To study NF2 gene mutations in acoustic neuroma. Methods Tumor tissue and blood samples from 84 patients with acoustic neuroma undergone surgery from January 2007 to December 2010 were collected in this study. Standard sequencing was used to detect NF2 gene mutation. Furthermore, multiple ligation-dependant probe amplifi?cation (MLPA) was performed on 30 patients to detect large deletions in the NF2 gene. Results NF2 gene mutation rate on standard sequencing was 39.3%among tumor specimens, but zero in blood samples. The rate of frame shift, splice site, non?sense and missence mutation was 48.5%, 21.2%, 24.2%and 6.1%, respectively. NF2 gene mutations occurred between ex?on 1 and 15. The exon 8 was the most favorite exon of mutations (15.2%). The rate of mutation in amino terminus, joinning region,α-helical structure and carboxyl terminus were 63.6%, 6.1%, 21.2%and 6.1%, respectively. Large deletions were detected in 73.3%of the patients via MLPA, of which 56.7%were located in amino terminus. The rate of NF2 gene muta?tion or large deletion detection increased to 80.0%when MLPA and standard sequencing were combined. Conclusions So?matic NF2 mutations and large deletions in the NF2 gene are frequent in sporadic acoustic neuroma. Combined MLPA and standard sequencing improves efficacy of NF2 gene mutation screening.