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[拉米夫定相关乙型肝炎病毒聚合酶基因突变检测方法的研究]

[A study on detection method of lamivudine related mutations in hepatitis B virus polymerase gene].

作者信息

Ding Jing-juan, Zhang Wei-san, Zhang Li-sha

机构信息

Department of Infectious Diseases, Guiyang Medical College, Guiyang 550004, China.

出版信息

Zhonghua Shi Yan He Lin Chuang Bing Du Xue Za Zhi. 2004 Mar;18(1):24-7.

PMID:15340520
Abstract

OBJECTIVE

To establish a simple and accurate method for rapid detection of lamivudine related mutations in hepatitis B virus (HBV) polymerase gene.

METHODS

HBV polymerase gene fragments of covering B and C active region were amplified by nested polymerase chain reaction (nPCR) or nested mismatched PCR. The PCR products were digested with Nde I or Nia III and subjected to electrophoresis on agarose gel, respectively. The patterns of restriction fragment length polymorphism (RFLP) were distinguished. Using this method, thirty patients with chronic hepatitis B and treated with lamivudine for at least one year were analysed for the lamivudine related mutations in polymerase gene. Sixteen cases without lamivudine therapy were used as controls. Some of the patients were also analysed by clone sequencing.

RESULTS

The nested mismatched PCR-RFLP method was simple, accurate and rapid. The whole experiments could be finished in eleven hours. The least titers of HBV DNA which could be detected was 10.3 copies/ml. The wild or mutant strains judged by RFLP were identified by clone sequencing. Mutation in the tyrosine methionine aspartic aspartic acid (YMDD) motif of HBV polymerase gene was found in eight patients and mutations of YMDD motif associated with L526M were found in another three patients. However, there were no such mutations in the control cases.

CONCLUSION

The nested PCR-RFLP is considered as a simple and accurate method for rapid detection of lamivudine related mutations in HBV polymerase gene. It is suitable for larger number of sample detection.

摘要

目的

建立一种简便、准确的快速检测乙型肝炎病毒(HBV)聚合酶基因中拉米夫定相关突变的方法。

方法

采用巢式聚合酶链反应(nPCR)或巢式错配PCR扩增覆盖B和C活性区的HBV聚合酶基因片段。PCR产物分别用Nde I或Nia III酶切,然后在琼脂糖凝胶上进行电泳,区分限制性片段长度多态性(RFLP)图谱。用该方法对30例接受拉米夫定治疗至少1年的慢性乙型肝炎患者的聚合酶基因中的拉米夫定相关突变进行分析,16例未接受拉米夫定治疗的患者作为对照。部分患者还用克隆测序法进行了分析。

结果

巢式错配PCR-RFLP方法简便、准确、快速,整个实验可在11小时内完成,能检测到的最低HBV DNA滴度为10.3拷贝/ml。通过克隆测序鉴定了经RFLP判断的野生型或突变型毒株。在8例患者中发现了HBV聚合酶基因酪氨酸-甲硫氨酸-天冬氨酸-天冬氨酸(YMDD)基序突变,在另外3例患者中发现了与L526M相关的YMDD基序突变,而对照病例中未发现此类突变。

结论

巢式PCR-RFLP被认为是一种简便、准确的快速检测HBV聚合酶基因中拉米夫定相关突变的方法,适用于大量样本检测。

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