Yourno J, Conroy J
New York State Department of Health, Wadsworth Center for Laboratory and Research, Empire State Plaza, Albany, New York 12201-0509.
J Clin Microbiol. 1992 Nov;30(11):2887-92. doi: 10.1128/jcm.30.11.2887-2892.1992.
A method for detection of proviral human immunodeficiency virus DNA in dried blood spots on filter paper by direct polymerase chain reaction (PCR) has been developed. To develop the method, a standard system was used which was prepared from cells each containing a single integrated provirus and titrated with normal donor blood. This rapid procedure provides virtually quantitative yields of nuclear DNA and exploits most of the standard methodology described for blood specimens. A nested PCR using SK38-SK39 gag as the internal primer pair was also designed; this PCR detected a single copy of provirus per filter at near theoretical frequency with SK19 probe. The utility of the procedure was demonstrated with clinical specimens. Blood spot filters from human immunodeficiency virus-infected and uninfected individuals were readily and unequivocally discriminated. The method is designed for ultimate use with large (1.5-ml) sample preparation tubes that are compatible as PCR tubes with thermal cyclers. This will permit convenient, direct single-tube PCR of dried blood specimens on filters. It should be adaptable to analysis of dried blood spots for a variety of infectious or genetic diseases.
已开发出一种通过直接聚合酶链反应(PCR)检测滤纸上干血斑中前病毒人类免疫缺陷病毒DNA的方法。为开发该方法,使用了一个标准系统,该系统由每个都含有单个整合前病毒的细胞制备而成,并用正常供体血液进行滴定。这种快速程序可提供几乎定量的核DNA产量,并利用了所述血液标本的大部分标准方法。还设计了一种使用SK38-SK39 gag作为内部引物对的巢式PCR;该PCR用SK19探针以接近理论频率检测每个滤膜上的单个前病毒拷贝。临床标本证明了该程序的实用性。来自人类免疫缺陷病毒感染和未感染个体的血斑滤膜很容易且明确地被区分。该方法设计用于最终与大型(1.5毫升)样品制备管一起使用,这些管与热循环仪兼容作为PCR管。这将允许对滤纸上的干血标本进行方便、直接的单管PCR。它应该适用于对各种传染病或遗传疾病的干血斑进行分析。
