A multiplex two-color real-time PCR method for quality-controlled molecular diagnostic testing of FFPE samples

Jiyoun Yeo; Erin L Crawford; Thomas M Blomquist; Lauren M Stanoszek; Rachel E Dannemiller; Jill Zyrek; Luis E De Las Casas; Sadik A Khuder; James C Willey

doi:10.1371/journal.pone.0089395

A multiplex two-color real-time PCR method for quality-controlled molecular diagnostic testing of FFPE samples

PLoS One. 2014 Feb 21;9(2):e89395. doi: 10.1371/journal.pone.0089395. eCollection 2014.

Authors

Jiyoun Yeo¹, Erin L Crawford¹, Thomas M Blomquist¹, Lauren M Stanoszek¹, Rachel E Dannemiller¹, Jill Zyrek², Luis E De Las Casas², Sadik A Khuder¹, James C Willey³

Affiliations

¹ Division of Pulmonary/Critical Care and Sleep Medicine, Department of Medicine, University of Toledo Health Sciences Campus, Toledo, Ohio, United States of America.
² Department of Pathology, University of Toledo Health Sciences Campus, Toledo, Ohio, United States of America.
³ Division of Pulmonary/Critical Care and Sleep Medicine, Department of Medicine, University of Toledo Health Sciences Campus, Toledo, Ohio, United States of America ; Department of Pathology, University of Toledo Health Sciences Campus, Toledo, Ohio, United States of America.

Abstract

Background: Reverse transcription quantitative real-time PCR (RT-qPCR) tests support personalized cancer treatment through more clinically meaningful diagnosis. However, samples obtained through standard clinical pathology procedures are formalin-fixed, paraffin-embedded (FFPE) and yield small samples with low integrity RNA containing PCR interfering substances. RT-qPCR tests able to assess FFPE samples with quality control and inter-laboratory reproducibility are needed.

Methods: We developed an RT-qPCR method by which 1) each gene was measured relative to a known number of its respective competitive internal standard molecules to control for interfering substances, 2) two-color fluorometric hydrolysis probes enabled analysis on a real-time platform, 3) external standards controlled for variation in probe fluorescence intensity, and 4) pre-amplification maximized signal from FFPE RNA samples. Reagents were developed for four genes comprised by a previously reported lung cancer diagnostic test (LCDT) then subjected to analytical validation using synthetic native templates as test articles to assess linearity, signal-to-analyte response, lower detection threshold, imprecision and accuracy. Fitness of this method and these reagents for clinical testing was assessed in FFPE normal (N = 10) and malignant (N = 10) lung samples.

Results: Reagents for each of four genes, MYC, E2F1, CDKN1A and ACTB comprised by the LCDT had acceptable linearity (R(2)>0.99), signal-to-analyte response (slope 1.0 ± 0.05), lower detection threshold (<10 molecules) and imprecision (CV <20%). Poisson analysis confirmed accuracy of internal standard concentrations. Internal standards controlled for experimentally introduced interference, prevented false-negatives and enabled pre-amplification to increase signal without altering measured values. In the fitness for purpose testing of this two-color fluorometric LCDT using surgical FFPE samples, the diagnostic accuracy was 93% which was similar to that previously reported for analysis of fresh samples.

Conclusions: This quality-controlled two-color fluorometric RT-qPCR approach will facilitate the development of reliable, robust RT-qPCR-based molecular diagnostic tests in FFPE clinical samples.

Publication types

Research Support, N.I.H., Extramural
Research Support, Non-U.S. Gov't

MeSH terms

Humans
Molecular Diagnostic Techniques / methods*
Multiplex Polymerase Chain Reaction / methods*
Paraffin Embedding
Real-Time Polymerase Chain Reaction / methods*
Tissue Fixation

Abstract

Publication types

MeSH terms

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