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Clinical and Diagnostic Laboratory Immunology, Nov 1996, 635-639, Vol 3, No. 6
TD Nguyen, M de Kesel, G Bigaignon, P Hoet, G Pazzaglia, M Lammens and M Delmee
Different techniques for identifying Toxoplasma gondii were compared. PCR
was used to amplify part of the major surface antigen P30 gene of T.
gondii. Amplified-DNA detection with the DNA enzyme immunoassay (PCR- DEIA)
was more sensitive than ethidium bromide staining after agarose gel
electrophoresis and as sensitive as nested PCR. PCR-DEIA, using common
enzyme-linked immunosorbent assay (ELISA) methods, avoids agarose gel
electrophoresis for the identification of amplified products. T. gondii can
also be detected with equal sensitivity in infected fibroblasts, but only
after at least 8 days of cell culture. PCR-DEIA is thus recommended because
of its sensitivity and convenience for detecting early parasitemia in the
surveillance of toxoplasmosis among pregnant women and immunocompromised
hosts. The courses of infection in mice infected with two strains of T.
gondii were compared. Tachyzoites of the virulent strain T. gondii RH,
killing the host in 4 days, were identified in urine specimens and blood
samples of mice 24 to 94 h after inoculation but not in brains, but no
antibodies were detected. After intraperitoneal inoculation with cysts of
the low-level virulence Beverley strain of T. gondii, parasites were
identified in blood samples 4 days later and up to 17 days (but not in
urine specimens) and in the brain from day 6 through day 525. By ELISA,
high antibody titers were found from day 11 to day 525, with parasitemia
preceding the appearance of antibodies. The usefulness of PCR-DEIA tests in
conjunction with the search for circulating antibodies for the early
diagnosis of toxoplasmosis in humans is discussed.
Copyright © 1996 by the American Society for Microbiology. All rights reserved.
Detection of Toxoplasma gondii tachyzoites and bradyzoites in blood, urine, and brains of infected mice
Microbiology Unit, Cliniques Universitaires Saint-Luc, Belgium.
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