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PCR-ELISA检测疟原虫DNA的研究
引用本文:张龙兴,汤林华,冯晓平,王聚君,. PCR-ELISA检测疟原虫DNA的研究[J]. 中国寄生虫学与寄生虫病杂志, 1998, 26(1): 11-15
作者姓名:张龙兴  汤林华  冯晓平  王聚君  
作者单位:中国预防医学科学院寄生虫病研究所
摘    要:目的:介绍一种诊断疟疾的新方法PCR-ELISA。方法:根据业已报道的疟原虫SSUr-RNA基因保守序列,设计并合成一对通用于恶性疟原虫和间日疟原虫的引物,其中一引物的5’端加以生物素标记。经PCR扩增后,携带有生物素的扩增产物与先期包被于ELISA板上的亲和素结合,再经与恶性疟原虫、间日疟原虫特异、荧光素标记的寡核苷酸探针分别杂交,底物显色等步骤,使PCR产物得以半定量地检出。结果:对于恶性疟原虫和间日疟原虫,本法检出最低原虫密度阈值分别为4和10个原虫/μl血(取血20μl),本法检测两种疟原虫未发现交叉反应。结论:本试验具有较高的敏感度和特异性,可望用于疟疾流行病学调查

关 键 词:PCR-ELISA  疟原虫  DNA检测

STUDY ON DETECTION OF MALARIA PARASITE DNA BY PCR ELISA *
Zhang Longxing,Tang Linhua,Feng Xiaoping,Wang Jujun. STUDY ON DETECTION OF MALARIA PARASITE DNA BY PCR ELISA *[J]. Chinese Journal of Parasitology and Parasitic Diseases, 1998, 26(1): 11-15
Authors:Zhang Longxing  Tang Linhua  Feng Xiaoping  Wang Jujun
Affiliation:Institute of Parasitic Diseases, Chinese Academy of Preventive Medicine, Shanghai 200025.
Abstract:AIM: To present a new malaria diagnostic method based on detection of malaria parasite DNA by PCR-ELISA. METHODS: According to the conserved sequence of Plasmodium SSUrRNA genes reported, a pair of primers in which one primer was biotinylated and another was unbiotinylated, suitable for DNA amplification of both falciparum and vivax malaria parasites were designed and synthesized. After denaturation and washing, the incorporated biotinylated product with avidin coated on plates previously was hybridized with the fluorescein-labelled oligonucleotide probes specific for Plasmodium falciparum or Plasmodium vivax. The color developed after adding POD conjugated with antibody to fluorescein and substrate can be semi-quantitated spectrophotometrically. RESULTS: The thresholds of parasite density for the detection of Plasmodium falciparum and Plasmodium vivax by this test were shown to be as low as 4 and 10 parasites per microliter of blood, respectively and no cross reaction was seen in the detection of falciparum and vivax malaria parasites. CONCLUSION: With promising sensitivity and specificity, this test can be used in malaria survey.
Keywords:PCR ELISA   malaria parasite   DNA detection
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