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前瞻性基于 PCR 的非小细胞肺癌 EML4-ALK 癌基因筛查。

A prospective PCR-based screening for the EML4-ALK oncogene in non-small cell lung cancer.

机构信息

Division of Functional Genomics, Jichi Medical University, Shimotsukeshi, Tochigi, Japan.

出版信息

Clin Cancer Res. 2012 Oct 15;18(20):5682-9. doi: 10.1158/1078-0432.CCR-11-2947. Epub 2012 Aug 20.

DOI:10.1158/1078-0432.CCR-11-2947
PMID:22908099
Abstract

PURPOSE

EML4-ALK is a lung cancer oncogene, and ALK inhibitors show marked therapeutic efficacy for tumors harboring this fusion gene. It remains unsettled, however, how the fusion gene should be detected in specimens other than formalin-fixed, paraffin-embedded tissue. We here tested whether reverse transcription PCR (RT-PCR)-based detection of EML4-ALK is a sensitive and reliable approach.

EXPERIMENTAL DESIGN

We developed a multiplex RT-PCR system to capture ALK fusion transcripts and applied this technique to our prospective, nationwide cohort of non-small cell lung cancer (NSCLC) in Japan.

RESULTS

During February to December 2009, we collected 916 specimens from 853 patients, quality filtering of which yielded 808 specimens of primary NSCLC from 754 individuals. Screening for EML4-ALK and KIF5B-ALK with our RT-PCR system identified EML4-ALK transcripts in 36 samples (4.46%) from 32 individuals (4.24%). The RT-PCR products were detected in specimens including bronchial washing fluid (n = 11), tumor biopsy (n = 8), resected tumor (n = 7), pleural effusion (n = 5), sputum (n = 4), and metastatic lymph node (n = 1). The results of RT-PCR were concordant with those of sensitive immunohistochemistry with ALK antibodies.

CONCLUSIONS

Multiplex RT-PCR was confirmed to be a reliable technique for detection of ALK fusion transcripts. We propose that diagnostic tools for EML4-ALK should be selected in a manner dependent on the available specimen types. FISH and sensitive immunohistochemistry should be applied to formalin-fixed, paraffin-embedded tissue, but multiplex RT-PCR is appropriate for other specimen types.

摘要

目的

EML4-ALK 是一种肺癌致癌基因,ALK 抑制剂对携带该融合基因的肿瘤显示出显著的治疗效果。然而,在福尔马林固定、石蜡包埋组织以外的标本中如何检测融合基因仍未解决。我们在此测试基于逆转录 PCR(RT-PCR)的 EML4-ALK 检测是否是一种敏感和可靠的方法。

实验设计

我们开发了一种多重 RT-PCR 系统来捕获 ALK 融合转录本,并将该技术应用于我们在日本的前瞻性全国非小细胞肺癌(NSCLC)队列。

结果

在 2009 年 2 月至 12 月期间,我们从 853 名患者中收集了 916 份标本,经过质量过滤后,获得了来自 754 名个体的 808 份原发性 NSCLC 标本。使用我们的 RT-PCR 系统对 EML4-ALK 和 KIF5B-ALK 进行筛查,从 32 名个体(4.24%)的 36 份标本(4.46%)中检测到 EML4-ALK 转录本。RT-PCR 产物在支气管灌洗液(n=11)、肿瘤活检(n=8)、切除肿瘤(n=7)、胸腔积液(n=5)、痰(n=4)和转移性淋巴结(n=1)标本中均可检测到。RT-PCR 的结果与敏感的 ALK 抗体免疫组化结果一致。

结论

多重 RT-PCR 被证实是一种可靠的技术,用于检测 ALK 融合转录本。我们建议,应根据可用标本类型选择 EML4-ALK 的诊断工具。FISH 和敏感免疫组化应应用于福尔马林固定、石蜡包埋组织,但多重 RT-PCR 适用于其他标本类型。

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