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用于人及病毒DNA的PCR扩增的石蜡包埋组织提取方法的评估

Evaluation of extraction methods from paraffin wax embedded tissues for PCR amplification of human and viral DNA.

作者信息

Chan P K, Chan D P, To K F, Yu M Y, Cheung J L, Cheng A F

机构信息

Department of Microbiology, The Chinese University of Hong Kong, Prince of Wales Hospital, Shatin, New Territories, Hong Kong SAR, China.

出版信息

J Clin Pathol. 2001 May;54(5):401-3. doi: 10.1136/jcp.54.5.401.

DOI:10.1136/jcp.54.5.401
PMID:11328843
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1731425/
Abstract

AIM

To evaluate the efficiency of phenol/chloroform, microwave, and Qiagen spin column based DNA extractions from paraffin wax embedded tissue for use in the polymerase chain reaction (PCR). In addition, to assess the reliability of amplifying a housekeeping gene to indicate successful viral DNA extraction.

METHODS

DNA samples extracted from 20 blocks of cervical carcinoma tissues using the three methods were subjected to PCRs targeting 509 bp and 355 bp of the beta globin gene, and 450 bp and 150 bp of human papillomavirus (HPV) DNA.

RESULTS

Microwave extraction showed the highest positive rate for beta globin PCR, whereas the spin column method was the most efficient for HPV DNA extraction. When the 509 bp beta globin and 450 bp HPV PCR results were correlated, two of 10, eight of 12, and nine of 10 beta globin positive extractions prepared by means of the phenol/chloroform, microwave, and spin column methods, respectively, yielded HPV DNA of the expected size. For the beta globin negative samples, HPV was detected in three of 10, two of eight, and four of 10 samples.

CONCLUSIONS

HPV DNA extraction was most efficient using the Qiagen spin column and had the highest positive predictive value when a housekeeping gene was used as an indicator of successful viral DNA extraction; the phenol/chloroform method was the least efficient. The potential drawbacks of some extraction methods when using a human housekeeping gene to assess the quality of viral DNA extraction need to be considered.

摘要

目的

评估采用苯酚/氯仿法、微波法以及基于Qiagen旋转柱法从石蜡包埋组织中提取用于聚合酶链反应(PCR)的DNA的效率。此外,评估扩增管家基因以表明病毒DNA成功提取的可靠性。

方法

使用这三种方法从20个宫颈癌组织块中提取的DNA样本,进行靶向β珠蛋白基因509 bp和355 bp以及人乳头瘤病毒(HPV)DNA 450 bp和150 bp的PCR。

结果

微波提取法在β珠蛋白PCR中显示出最高的阳性率,而旋转柱法在HPV DNA提取方面效率最高。当将509 bpβ珠蛋白和450 bp HPV的PCR结果进行对比时,通过苯酚/氯仿法、微波法和旋转柱法分别制备的10个β珠蛋白阳性提取物中,有2个、12个中的8个以及10个中的9个产生了预期大小的HPV DNA。对于β珠蛋白阴性样本,在10个样本中有3个、8个样本中有2个以及10个样本中有4个检测到了HPV。

结论

使用Qiagen旋转柱提取HPV DNA效率最高,并且在将管家基因用作病毒DNA成功提取的指标时具有最高的阳性预测值;苯酚/氯仿法效率最低。在使用人类管家基因评估病毒DNA提取质量时,需要考虑某些提取方法的潜在缺点。