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This article has a correction

Please see: J Clin Pathol 2008;61:400

J Clin Pathol 2008;61:132-137 doi:10.1136/jcp.2007.047266
  • Original article

Effects of fixation on RNA integrity in a liquid-based cervical cytology setting

  1. C Horvath1,
  2. G Boulet1,
  3. S Sahebali1,
  4. J Bogers1,2,
  5. C Depuydt2,
  6. A Vereecken2,
  7. T Vermeulen3,
  8. D Vanden Broeck4
  1. 1
    AMBIOR, Laboratory of Cell Biology and Histology, University of Antwerp, Antwerp, Belgium
  2. 2
    Laboratory for Clinical Pathology (Labo Lokeren, campus RIATOL), Antwerp, Belgium
  3. 3
    Laboratory of Cell Biology and Histology, University of Antwerp, Antwerp, Belgium
  4. 4
    International Centre for Reproductive Health (ICRH), Ghent University, De Pintelaan 185, 9000 Ghent, Belgium
  1. Caroline Horvath, Applied Molecular Biology Research group (AMBIOR), Laboratory of Cell Biology and Histology, University of Antwerp, Groenenborgerlaan 171, BE-2020 Antwerp; caroline.horvath{at}ua.ac.be
  • Accepted 29 March 2007
  • Published Online First 27 April 2007

Abstract

Aims: Despite many improvements, cervical cancer screening is still subject to shortcomings. Diagnostic accuracy may improve by using molecular biological techniques, requiring RNA of superior quality. This study determined the effect of SurePath fixation on RNA integrity to assess the suitability of clinical samples collected in this medium for RNA-based molecular assays.

Methods: RNA isolation was performed on fresh and fixed HeLa cells and exfoliated cervical cells fixed in SurePath. The RNA integrity was evaluated by analysis of ribosomal RNA as an indicator of quality. The effect of SurePath preservation on PCR amplification was evaluated by real-time reverse transcriptase (RT)-PCR.

Results: In contrast to unfixed cells, SurePath-fixed cells yielded less and severely degraded RNA, as shown by the absence of ribosomal RNA bands. RNA derived from SurePath-fixed cells showed poor real-time RT-PCR amplification characteristics, as evidenced by the absent correlation between threshold values and log cDNA concentration.

Conclusions: Implementation of molecular biology in a clinical context is on the rise and may alleviate shortcomings in current screening and diagnostics. This study shows that SurePath fixation gives rise to highly fragmented RNA with insufficient quality for further reliable analysis by standard real-time RT-PCR applications. The increasing prominence of molecular screening stresses the importance of this finding, which must be considered in relation to choice of an appropriate liquid-based cytology system.

Footnotes

  • Funding: CH is supported by the Institute for Promotion of Innovation through Science and Technology in Flanders (IWT-Vlaanderen, 1556). GB is supported by the Fund for Scientific Research Flanders (FWO-Vlaanderen). JB is supported by the Fund for Scientific Research Flanders (FWO-Vlaanderen, G.0205.04) and the Belgian Cancer Foundation (Belgische Stichting tegen Kanker).

  • Competing interests: None.

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