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在实验性小鼠模型中灵敏且特异的弓形虫DNA检测:刚地弓形虫特异性cDNA及聚合酶链反应的应用

Sensitive and specific detection of toxoplasma DNA in an experimental murine model: use of Toxoplasma gondii-specific cDNA and the polymerase chain reaction.

作者信息

Weiss L M, Udem S A, Salgo M, Tanowitz H B, Wittner M

机构信息

Department of Medicine (Division of Infectious Diseases) and Albert Einstein College of Medicine, Bronx, New York 10461.

出版信息

J Infect Dis. 1991 Jan;163(1):180-6. doi: 10.1093/infdis/163.1.180.

DOI:10.1093/infdis/163.1.180
PMID:1984466
Abstract

Toxoplasma gondii, an apicomplexan parasite of mammals and birds, is well recognized as a cause of encephalitis in AIDS patients and as a cause of congenital infections. The polymerase chain reaction (PCR) and toxoplasma cDNA clones were used to diagnose T. gondii infection in an acute murine model of toxoplasmosis. Diagnosis of tissue infection by Southern blot hybridization with cDNA clones of T. gondii was possible within 5 days of infection. This technique could detect as few as 10,000 organisms. Specific T. gondii gene amplification by PCR using the primers 5'CACACGGTTGTATGTCGGTTTCGCT3' and 5'TCAAGGAGCTCAATGTTACAGCCT3' followed by oligonucleotide hybridization using 5'GCGGTCATTCTCACACCGACGGAGAACCACTTCACTCTCA3' allowed detection of T. gondii in the tissue of mice by day 2 after infection and in the blood of mice by day 5 after infection with RH strain T. gondii. This technique could detect as few as 10 organisms. Thus, these techniques may be useful in the diagnosis of toxoplasmosis.

摘要

刚地弓形虫是一种寄生于哺乳动物和鸟类的顶复门寄生虫,是艾滋病患者脑炎和先天性感染的公认病因。在急性小鼠弓形虫病模型中,利用聚合酶链反应(PCR)和弓形虫cDNA克隆来诊断弓形虫感染。在感染后5天内,通过与弓形虫cDNA克隆进行Southern印迹杂交可诊断组织感染。该技术可检测低至10000个生物体。使用引物5'CACACGGTTGTATGTCGGTTTCGCT3'和5'TCAAGGAGCTCAATGTTACAGCCT3'通过PCR进行特异性弓形虫基因扩增,随后使用5'GCGGTCATTCTCACACCGACGGAGAACCACTTCACTCTCA3'进行寡核苷酸杂交,可在感染刚地弓形虫RH株后第2天检测到小鼠组织中的弓形虫,并在感染后第5天检测到小鼠血液中的弓形虫。该技术可检测低至10个生物体。因此,这些技术可能有助于弓形虫病的诊断。

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