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使用脱落标本和细针穿刺涂片进行肺腺癌的突变检测

Use of Exfoliative Specimens and Fine-Needle Aspiration Smears for Mutation Testing in Lung Adenocarcinoma.

作者信息

Jain Deepali, Ramachandrappa Vijayakumar S, Singh Varsha, Malik Prabhat S, Madan Karan, Faruq Mohammed, Guleria Randeep

机构信息

Department of Pathology, All India Institute of Medical Sciences (AIIMS), New Delhi, India.

出版信息

Acta Cytol. 2017;61(6):455-461. doi: 10.1159/000479217. Epub 2017 Aug 22.

DOI:10.1159/000479217
PMID:28848083
Abstract

OBJECTIVE

Cytology specimens are considered to be a promising alternative for detecting driver mutations in lung cancer patients. We aimed to explore the suitability and utility of various cytology samples of non-small-cell lung cancer (NSCLC) patients for mutation testing. In addition to mutation detection, the importance of preanalytic factors was discussed.

DESIGN

A total of 116 cytology samples including 32 controls comprising pleural effusions, bronchial washings, and direct fine-needle aspiration (FNA) smears were included in the study for the detection of EGFR, KRAS, and Her-2/neu gene mutations. Tumor content was checked by microscopic evaluation. Tumor enrichment was done by scraping direct smears. DNA yield was assessed before selecting the method of mutation detection. Sanger sequencing and real-time PCR-based methods were used.

RESULTS

Overall, 20.23% EGFR mutations and 2.74% KRAS mutations were observed in this study. Nondriver genetic polymorphisms were observed in EGFR exon 20 in 37% cases. The coexistence of the EGFR mutation and EGFR polymorphism was seen in 7 cases. DNA yield was better in pleural effusions and bronchial washings. Real-time PCR was used in specimens of low DNA yield.

CONCLUSIONS

Cytology samples are useful in ascertaining molecular diagnostic information for treatment purposes if they are optimized judiciously in their preanalytic phase.

摘要

目的

细胞学标本被认为是检测肺癌患者驱动基因突变的一种有前景的替代方法。我们旨在探讨非小细胞肺癌(NSCLC)患者的各种细胞学样本用于突变检测的适用性和实用性。除了突变检测,还讨论了分析前因素的重要性。

设计

本研究共纳入116份细胞学样本,包括32份对照样本,样本类型有胸腔积液、支气管灌洗和直接细针穿刺(FNA)涂片,用于检测EGFR、KRAS和Her-2/neu基因突变。通过显微镜评估检查肿瘤含量。通过刮取直接涂片进行肿瘤富集。在选择突变检测方法之前评估DNA产量。使用了桑格测序和基于实时PCR的方法。

结果

总体而言,本研究中观察到20.23%的EGFR突变和2.74%的KRAS突变。在37%的病例中,EGFR外显子20存在非驱动基因多态性。7例病例中观察到EGFR突变与EGFR多态性共存。胸腔积液和支气管灌洗中的DNA产量较好。DNA产量低的样本使用实时PCR。

结论

如果在分析前阶段进行明智的优化,细胞学样本可用于确定分子诊断信息以指导治疗。

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