Comparison of RNA Extraction Methods for Molecular Analysis of Oral Cytology

Overview

Journal Acta Stomatol Croat

Specialty Dentistry

Date 2016 Oct 30

PMID 27789907

Citations 8

Authors

Monica Ghislaine Oliveira Alves

Mario Perez-Sayans

Maria-Elena Padin-Iruegas

Maria Dolores Reboiras-Lopez

Jose Manuel Suarez-Penaranda

Rafael Lopez-Lopez

Celina Faig Lima Carta

Jaqueline Scholz Issa

Abel Garcia-Garcia

Janete Dias Almeida

Affiliations

Soon will be listed here.

Abstract

Objective Of Work: The aim of this study was to compare three methods of RNA extraction for molecular analysis of oral cytology to establish the best technique, considering its concentration and purity for molecular tests of oral lesions such as real-time reverse transcriptase reaction.

Material And Methods: The sample included exfoliative cytology from the oral cavity mucosa of patients with no visible clinical changes, using Orcellex Rovers Brush. The extraction of total RNA was performed using the following three techniques: 30 samples were extracted by Trizol® technique, 30 by the Direct-zol RNA Miniprep system and 30 by the RNeasy mini Kit. The absorbance was measured by spectrophotometer to estimate the purity. The estimated RNA concentration was obtained by multiplying the value of A260 (ng/mL) by 40. Statistical analysis of the obtained data was performed using GraphPad Prism 5.03 software with Student t, analysis of variance and Bonferroni tests, considering p ≤0.05.

Results: Trizol® group revealed higher average concentration, followed by Direct-zol and Rneasy group. It was observed that the RNA Direct-zol group had the highest purity, followed by RNeasy and Trizol® groups, allowing for the two ratios.

Conclusion: Considering all aspects, concentration, purity and time spent in the procedures, the Direct-zol group showed the best results.

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