Xu Chun-hai, Li Zhao-shen, Dai Jun-ying, Zhu Hai-yang, Yu Jian-wu, Lv Shu-lan
The Second Affiliated Hospital of Harbin Medical University, 150086, China.
Zhonghua Shi Yan He Lin Chuang Bing Du Xue Za Zhi. 2011 Aug;25(4):307-9.
To establish a nested real-time quantitative polymerase chain reaction (PCR) assay for detection of hepatitis B virus covalently closed circular DNA in PBMC( peripheral blood monocyte) and MMNC (marrow monocyte).
Based on the structural differences between HBVcccDNA and HBV rcDNA, two pairs of specific primers spanned the gap of the positive and negative chains and a specific TaqMan probe situated downstream were designed. To remove rcDNA, cccDNA was processed by Mung Bean Nuclease,and then amplified by nested real-time quantitative PCR using a pair of outer primers and a pair of inner primers. According to the standard preparation, cccDNA levels of specimen were calculated.
We have established a nested real-time fluorescent quantitative PCR method for HBV cccDNA successfully, and the linear range is from 5.0 x 10(2) to 3. 9 x 10(7) copies per milliliter. Of the 25 PBMC samples and 7 MMNC samples of the chronic hepatitis B or liver cirrhosis patients, 3 MMNC samples and 9 PBMC samples were HBV cccDNA positive, while all of the 21 healthy donator blood PBMC samples were negative.
The nested real-time fluorescent quantitative PCR method may be applied to detect HBVcccDNA level in PBMC and MMNC. HBVcccDNA can be detected in PBMC and MMNC.
建立一种巢式实时定量聚合酶链反应(PCR)检测方法,用于检测外周血单核细胞(PBMC)和骨髓单核细胞(MMNC)中的乙型肝炎病毒共价闭合环状DNA(HBVcccDNA)。
基于HBVcccDNA与HBV复制型DNA(rcDNA)的结构差异,设计了两对跨越正链和负链缺口的特异性引物以及一条位于下游的特异性TaqMan探针。通过绿豆核酸酶处理去除rcDNA,然后使用一对外引物和一对内引物进行巢式实时定量PCR扩增。根据标准品制备情况,计算标本的cccDNA水平。
我们成功建立了一种用于HBVcccDNA的巢式实时荧光定量PCR方法,线性范围为每毫升5.0×10²至3.9×10⁷拷贝。在慢性乙型肝炎或肝硬化患者的25份PBMC样本和7份MMNC样本中,3份MMNC样本和9份PBMC样本HBVcccDNA呈阳性,而21份健康献血者血液PBMC样本均为阴性。
巢式实时荧光定量PCR方法可用于检测PBMC和MMNC中的HBVcccDNA水平。在PBMC和MMNC中均可检测到HBVcccDNA。
