Use of polymerase chain reaction and rabbit infectivity testing to detect Treponema pallidum in amniotic fluid, fetal and neonatal sera, and cerebrospinal fluid.

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J Clin Microbiol. 1991 August; 29(8): 1711-1718

Use of polymerase chain reaction and rabbit infectivity testing to detect Treponema pallidum in amniotic fluid, fetal and neonatal sera, and cerebrospinal fluid.

E Grimprel, P J Sanchez, G D Wendel, J M Burstain, G H McCracken Jr, J D Radolf and M V Norgard

Department of Pediatrics, University of Texas Southwestern Medical Center, Dallas 75235.

ABSTRACT

The diagnosis of congenital syphilis continues to pose a difficultclinical challenge. Because the serodiagnosis of congenitalsyphilis has significant limitations, the direct detection ofTreponema pallidum in suspect neonatal tissues or body fluidsrepresents a desirable alternate diagnostic strategy. We developedand applied the polymerase chain reaction (PCR) for the detectionof T. pallidum in clinical material relevant to the diagnosisof congenital syphilis but which typically contain factors inhibitoryfor the PCR. Four methods of specimen processing were examinedto circumvent PCR inhibition; clinical materials included amnioticfluids, neonatal sera, and neonatal cerebrospinal fluids. ThePCR was 100% specific for T. T. pallidum compared with the sensitiverabbit infectivity test (RIT) for all clinical materials tested.For amniotic fluids, the PCR was 100% sensitive when correlatedwith the RIT but had a lesser sensitivity when applied to seraor cerebrospinal fluids, which typically contain few treponemes.The combined sensitivity of the PCR for all clinical sampleswas 78%. Positive PCR results also were obtained among someclinical specimens for which RIT was not performed; these resultscorrelated well with either stigmata or risk factors for congenitalsyphilis. The combined results suggest that the PCR can be auseful adjunct to the diagnosis and clinical management of congenitalsyphilis and that it will provide a valuable tool for investigationsof the pathogenesis of the disorder.

J Clin Microbiol. 1991 August; 29(8): 1711-1718

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