| 顺序特异性引物法快速检测胰腺癌K—ras基因点突变 |
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| 引用本文: | 戴存才,刘训良,等.顺序特异性引物法快速检测胰腺癌K—ras基因点突变[J].胰腺病学,2002,2(1):22-24. |
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| 作者姓名: | 戴存才 刘训良 |
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| 作者单位: | 南京医科大学第一附属医院普外科,南京210029 |
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| 摘 要: | 目的:研究简捷、特异、敏感的检测胰腺癌K-ras基因点突变的方法及其在胰腺疾病中定性诊断的价值。方法:采用针对K-ras基因点突变方式(CGT、GAT、GTT)设计的顺序特异性引物(SSP),先后对胰腺癌石蜡包埋组织、冰冻新鲜组织、细针穿刺组织及胰液进行多聚酶链反应(PCR),扩增产物借助常规电泳和染色检测有无K-ras基因突变及突变方式。结果:胰腺癌石蜡包埋组织、冰冻新鲜组织、细针穿刺组织及胰液中K-ras基因点突变率分别为74.2%、95.1%、91.4%及94.1%,而所有被检测的慢性胰腺炎、胰岛素瘤、壶腹癌、胆管癌、十二指肠乳头癌及外伤胰腺的组织标本和胰液标本均无K-ras基因突变发生。结论:该检测法简便、快速、特异、敏感,具有临床实用性,可以作为鉴别胰腺肿块良恶性和诊断胰腺癌的一种方法。
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| 关 键 词: | 胰腺癌 K-ras基因 基因点突变 诊断 多聚酶链反应-顺序特异性引物 |
| 修稿时间: | 2001年9月21日 |
Rapid detection of K-ras gene point mutation in pancreatic adenocarcinonia by sequence special primer PCR |
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| DAI Cuncai,LIU Xunliang,MIAOYi,et al..Rapid detection of K-ras gene point mutation in pancreatic adenocarcinonia by sequence special primer PCR[J].Chinese JOurnal of Pancreatology,2002,2(1):22-24. |
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| Authors: | DAI Cuncai LIU Xunliang MIAOYi |
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| Institution: | DAI Cuncai,LIU Xunliang,MIAOYi,et al. Department of General Surgery,the Affiliated Hospital,Nanjing Medical University,Nanjing 210029,China |
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| Abstract: | Objective To explore a simple, rapid, specific and sensitive method of detecting K-ras gene point mutation and evaluate its qualitative diagnostic value in pancreatic adenocarcinoma. Methods According to the K-ras point mutant type (CGT, GTT and GAT) in pancreatic adenocarcinoma, three kinds of sequence special primer (SSP) for ploymerase chain reaction were designed, where K-ras gene fragment was amplified from frozen or paraffin embedded pancreatic adenocarcinoma tissues, fine needle aspiration sample from pancreatic adenocarcinoma and pancreatic juice of patients with pancreatic carcinoma. K-ras point mutation of the amplified product was detected by gel electrophoresis. Results K-ras gene point mutation rate was 74.2% (23/31) in paraffin embedded pancreatic adenocarcinoma tissues, 95.1%(39/41) in frozen pancreatic adenocarcinoma tissues, 91.4%(31/35) in fine needle aspiration sample and 94.1%(16/17) in pancreatic juice. No mutant K-ras gene was found in tissues and pancreatic juice of patients with chronic pancreatitis, insulinoma, ampullary carcinoma, bile duct carcinoma, duodenum papillary adenocarcinoma and injured pancreas. Conclusions Detecting the mutant K-ras with PCR-SSP is rapid, convenient, specific and as sensitive. It may serve as a practical method for distinguishing pancreatic benign masses from malignant ones, and can make a definitive diagnosis of pancreatic adenocarcinoma. |
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| Keywords: | Pancreatic adenocarcinoma K-ras gene mutation Ploymerase chain reaction-sequence special primer |
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