Direct and sensitive detection of a pathogenic protozoan, Toxoplasma gondii, by polymerase chain reaction.

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J Clin Microbiol. 1989 August; 27(8): 1787-1792

Direct and sensitive detection of a pathogenic protozoan, Toxoplasma gondii, by polymerase chain reaction.

J L Burg, C M Grover, P Pouletty and J C Boothroyd

Department of Microbiology and Immunology, Stanford University School of Medicine, California 94305-5402.

ABSTRACT

We applied the polymerase chain reaction to detection of thepathogenic protozoan Toxoplasma gondii based on our identificationof a 35-fold-repetitive gene (the B1 gene) as a target. Usingthis procedure, we were able to amplify and detect the DNA ofa single organism directly from a crude cell lysate. This levelof sensitivity also allowed us to detect the B1 gene from purifiedDNA samples containing as few as 10 parasites in the presenceof 100,000 human leukocytes. This is representative of the maximalcellular infiltration (10(5)/ml) in 1 ml of cerebrospinal fluidobtained from patients with toxoplasmic encephalitis. The B1gene is present and conserved in all six T. gondii strains testedto date, including two isolates from patients with acquiredimmunodeficiency syndrome. No signal was detected by using thisassay and DNAs from a variety of other organisms, includingseveral which might be found in the central nervous system ofan immunocompromised host. This combination of sensitivity andspecificity should make detection of the B1 gene based on polymerasechain reaction amplification a very useful method for diagnosisof toxoplasmosis both in immunocompromised hosts and in congenitallyinfected fetuses.

J Clin Microbiol. 1989 August; 27(8): 1787-1792

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