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通过聚合酶链反应检测人类免疫缺陷病毒DNA的干血斑标本的稳定性

Stability of dried blood spot specimens for detection of human immunodeficiency virus DNA by polymerase chain reaction.

作者信息

Cassol S, Salas T, Gill M J, Montpetit M, Rudnik J, Sy C T, O'Shaughnessy M V

机构信息

Centre for Excellence in HIV/AIDS, University of British Columbia, Vancouver, Canada.

出版信息

J Clin Microbiol. 1992 Dec;30(12):3039-42. doi: 10.1128/jcm.30.12.3039-3042.1992.

DOI:10.1128/jcm.30.12.3039-3042.1992
PMID:1452682
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC270585/
Abstract

Blood sampling on filter paper has many advantages for the detection of perinatal human immunodeficiency virus (HIV) infection by the polymerase chain reaction (PCR). However, if the method is to be widely used, an assessment of its performance under field conditions is required. To simulate conditions in the field, 50-microliters aliquots of whole blood containing low levels of HIV proviral DNA (4 to 1,024 copies per 100,000 nucleated cells) were spotted onto filter paper; dried; and subjected to heat, humidity, and prolonged storage at room temperature. After exposure, the DNA was recovered and amplified with primers to human leukocyte antigen DQ alpha- and HIV-specific sequences. Treatment at 37 degrees C and 60% humidity for 7 days, storage for 12 weeks at 22 degrees C, and freeze-thawing twice had no adverse effect on PCR reactivity when compared with the results obtained with reference spots stored at -20 degrees C. The lower limits of HIV detection in all tests ranged from 4 to 16 HIV copies per 100,000 cells. Fixation in 70% ethanol improved the amplification of low levels of HIV DNA and reduced biohazard risks. These findings suggest that dried blood spots will provide a powerful new resource for testing for HIV by PCR, especially in remote areas where refrigeration and immediate sample processing are unavailable.

摘要

通过聚合酶链反应(PCR)检测围产期人类免疫缺陷病毒(HIV)感染时,滤纸采血具有诸多优势。然而,若要广泛应用该方法,需评估其在现场条件下的性能。为模拟现场条件,将含有低水平HIV前病毒DNA(每100,000个有核细胞中含4至1,024个拷贝)的50微升全血等分试样点在滤纸上;干燥;并置于高温、高湿环境下,以及在室温下长期保存。处理后,回收DNA并用针对人类白细胞抗原DQα和HIV特异性序列的引物进行扩增。与储存在-20℃的参比样本的结果相比,在37℃和60%湿度下处理7天、在22℃下保存12周以及冻融两次对PCR反应性均无不利影响。所有检测中HIV的检测下限为每100,000个细胞含4至16个HIV拷贝。用70%乙醇固定可改善低水平HIV DNA的扩增并降低生物危害风险。这些发现表明,干血斑将为通过PCR检测HIV提供一种强大的新资源,尤其是在无法进行冷藏和即时样本处理的偏远地区。

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