Establishment of a Protocol for Viability qPCR in Dental Hard Tissues

Author:

Sterzenbach Torsten1,Neumann Vanessa1,Trips Evelyn2ORCID,Basche Sabine1,Hannig Christian1,Kühne Marie-Theres1ORCID

Affiliation:

1. Policlinic of Operative Dentistry, Periodontology and Pediatric Dentistry, Medical Faculty Carl Gustav Carus, Dresden University of Technology, 01307 Dresden, Germany

2. Coordination Centre for Clinical Trials, Faculty of Medicine Carl Gustav Carus, Dresden University of Technology, Fetscherstraße 74, 01309 Dresden, Germany

Abstract

The aim of the study was to establish a live/dead qPCR with propidium monoazide (PMA) that can quantitatively differentiate between viable/non-viable microorganisms in dental hard tissues. Human premolars (n = 88) were prepared with nickel–titanium instruments and incubated with E. faecalis (21 d). Subsequently, the bacteria in half of the teeth were devitalized by heat inactivation (100 °C, 2 h). The following parameters were tested: PMA concentrations at 0 µmol (control), 50 µmol, 100 µmol, and 200 µmol; PMA incubation times of 30 min and 60 min, and blue light treatment for 30 min and 60 min. The teeth were ground using a cryomill and the bacterial DNA was quantified using qPCR, ANOVA, and p = 0.05. The qPCR of the control group detected a similar number of avital 9.94 × 106 and vital 1.61 × 107 bacterial cells. The use of PMA inhibited the amplification of DNA from non-viable cells during qPCR. As a result, the best detection of avital bacteria was achieved with the following PMA parameters: (concentration, incubation time, blue light treatment) 200-30-30; 5.53 × 104 (avital) and 1.21 × 100.7 (vital). The live/dead qPCR method using PMA treatment is suitable for the differentiation and quantification of viable/non-viable microorganisms in dentin, as well as to evaluate the effectiveness of different preparation procedures and antimicrobial irrigants in other biological hard substances.

Funder

German Society of Dentistry and Oral Medicine

Publisher

MDPI AG

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