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Comparison of EGFR mutation detection between the tissue and cytology using direct sequencing, pyrosequencing and peptide nucleic acid clamping in lung adenocarcinoma: Korean multicentre studyopen access

Authors
Min, Kyueng-WhanKim, Wan-SeopJang, Se JinChoi, Yoo DukChang, SunheeJung, Soon HeeKim, LuciaRoh, Mee SookLee, Choong SikShim, Jung WeonKim, Mi JinLee, Geon Kook
Issue Date
Mar-2016
Publisher
OXFORD UNIV PRESS
Citation
QJM-AN INTERNATIONAL JOURNAL OF MEDICINE, v.109, no.3, pp.167 - 173
Indexed
SCIE
SCOPUS
Journal Title
QJM-AN INTERNATIONAL JOURNAL OF MEDICINE
Volume
109
Number
3
Start Page
167
End Page
173
URI
https://scholarworks.bwise.kr/hanyang/handle/2021.sw.hanyang/154913
DOI
10.1093/qjmed/hcv103
ISSN
1460-2725
Abstract
Background: The importance of sensitive methods for the detection of epidermal growth factor receptor (EGFR) mutation is emphasized. The aim of this study is to perform comparative and concordance analyses of direct sequencing, pyrosequencing and peptide nucleic acid (PNA) clamping for detecting EGFR gene mutations using archived tissue and cytology specimens. Methods: Samples from a total of 112 cases, which were diagnosed with adenocarcinoma of the lung at nine hospitals in Korea were collected. Using the above three methods, the concordance rates of EGFR mutations in exons 18, 19, 20 and 21 were analysed and validated in comparative tissue and cytology specimens. Results: Comparison of EGFR mutation detection between the tissue and cytology had a high concordance rate. The diagnostic performance of pyrosequencing and PNA clamping in tissue was higher than that of direct sequencing as well as cytology. Additionally, among some of the patients who had EGFR wild type by single method, EGFR mutations were detected by other methods. Cytology specimens had a diagnostic performance for the detection of EGFR mutations. Conclusions: Cytology specimens had a diagnostic performance for the detection of EGFR mutations that was comparable to that of tissues. For detecting EGFR mutations, pyrosequencing or PNA clamping was more sensitive than direct sequencing. In EGFR mutation negative patients who are difficult to obtain tissue, repeating test using pyrosequencing or PNA clamping is recommended to improve the detection rate of EGFR mutation than only one, especially in cytology.
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