Treponema pallidum ssp. pallidum identification by real-time PCR targetting the polA gene in paraffin-embedded samples positive by immunohistochemistry-Reference-Cited by-同舟云学术

Treponema pallidum ssp. pallidum identification by real-time PCR targetting the polA gene in paraffin-embedded samples positive by immunohistochemistry

Published:2017-04-11 Issue:13 Volume:28 Page:1299-1304
ISSN:0956-4624
Container-title:International Journal of STD & AIDS
language:en
Short-container-title:Int J STD AIDS

Author:

Gama A¹,Carrillo-Casas EM²,Hernández-Castro R³,Vázquez-Aceituno VA³,Toussaint-Caire S¹,Xicohtencatl-Cortes J⁴,Fernández-Martínez R⁵,Moreno-Coutiño G⁵

Affiliation:

1. Dermatology Service, General Hospital Dr. Manuel Gea González, Tlalpan, Mexico

2. Department of Biology and Histocompatibility, General Hospital Dr. Manuel Gea González, Tlalpan, Mexico

3. Department of Ecology of Pathogen Agents, General Hospital Dr. Manuel Gea González, Tlalpan, Mexico

4. Intestinal Bacteriology Laboratory, Childrens Hospital of Mexico Dr. Federico Gómez, Mexico

5. Mycology Service, General Hospital Dr. Manuel Gea González, Tlalpan, Mexico

Abstract

Syphilis is a systemic and sexually transmitted infection caused by Treponema pallidum ssp. pallidum. This spirochete causes different clinical and subclinical stages depending on the duration of infection and immune status of the host. Several tests have been developed for diagnosis, and are classified into direct and indirect methods. The first one includes dark field microscopy, direct fluorescent antibody test in fluids or tissue, and molecular biology techniques. In the indirect method (serologic), the routine tests are used, and are divided in two categories: non-treponemal and treponemal ones. The objective of this work was to identify T. pallidum ssp. pallidum in paraffin-embedded skin biopsies positive by immunohistochemistry, using conventional polymerase chain reaction (PCR) and quantitative real time PCR (qPCR). We included a sample of 17 paraffin-embedded biopsies. DNA was extracted and processed by conventional PCR and real-time PCR with a TaqMan® probe to identify the polA gene. Using PCR, 11 tested positive (64.7%) and 6 (35.3%) were negative. With qPCR and TaqMan® probe, 100% of samples tested positive. The minimum number of spirochetes detected in each sample was 2. With this work, we can conclude that qPCR is a fast and very accurate method for diagnosis of syphilis in tissue specimens.

Publisher

SAGE Publications

Subject

Infectious Diseases,Pharmacology (medical),Public Health, Environmental and Occupational Health,Dermatology

Link

http://journals.sagepub.com/doi/pdf/10.1177/0956462417704123

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