Highly sensitive and accurate detection of ALK-TKI resistance mutations by oligoribonucleotide interference-PCR (ORNi-PCR)-based methods

IF 4.5 2区 医学 Q1 ONCOLOGY Lung Cancer Pub Date : 2024-09-27 DOI:10.1016/j.lungcan.2024.107969
Chiori Tabe , Toshitsugu Fujita , Kageaki Taima , Hisashi Tanaka , Tomonori Makiguchi , Masamichi Itoga , Yoshiko Ishioka , Sadatomo Tasaka , Hodaka Fujii
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Abstract

Background

Patients with anaplastic lymphoma kinase (ALK)-positive non-small cell lung cancer (NSCLC) are treated with ALK tyrosine kinase inhibitors (TKIs). Although most patients benefit from ALK-TKIs, the development of resistance mutations is common and results in NSCLC recurrence. To identify ALK-TKI-resistant NSCLC at the early recurrent phase, highly sensitive and accurate methods for the detection of mutations are essential.

Objective

The aim of this study was to establish highly sensitive, accurate, cost-effective, and clinically practical methods for the detection of two frequent ALK-TKI resistance mutations, ALK G1202R and L1196M, by liquid biopsy.

Methods

The efficacy of oligoribonucleotide interference-PCR (ORNi-PCR) was examined by first optimizing experimental conditions to specifically amplify the ALK-TKI resistance mutant DNA corresponding to ALK G1202R and L1196M mutations. ORNi-PCR was then combined with droplet digital PCR (ddPCR) or real-time PCR to detect these mutations in cell-free DNA (cfDNA) extracted from NSCLC patients.

Results

ORNi-PCR followed by ddPCR/real-time PCR detected 1–10 copy(s) of G1202R and L1196M DNA in model cfDNA. These mutations in patients’ cfDNA were identified using ORNi-PCR-based methods, whereas conventional ddPCR failed to detect them.

Conclusion

ORNi-PCR followed by ddPCR/real-time PCR enables highly sensitive and accurate detection of ALK mutations by liquid biopsy. Although the clinical data are limited, our results show that these methods are potentially useful for identifying ALK-TKI-resistant NSCLC at the early recurrent phase.

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基于寡核苷酸干扰PCR(ORNi-PCR)的方法高灵敏、准确地检测ALK-TKI耐药突变。
背景:无性淋巴瘤激酶(ALK)阳性非小细胞肺癌(NSCLC)患者接受ALK酪氨酸激酶抑制剂(TKIs)治疗。虽然大多数患者都能从ALK-TKIs中获益,但耐药突变的发生很常见,并导致NSCLC复发。要在早期复发阶段识别ALK-TKI耐药的NSCLC,高灵敏度和准确的突变检测方法至关重要:本研究旨在通过液体活检建立高灵敏度、高准确性、高成本效益和临床实用的方法,用于检测两种常见的 ALK-TKI 耐药突变(ALK G1202R 和 L1196M):方法:首先优化实验条件,特异性扩增与ALK G1202R和L1196M突变相对应的ALK-TKI耐药突变DNA,以此检验寡核苷酸干扰PCR(ORNi-PCR)的有效性。然后将 ORNi-PCR 与液滴数字 PCR(ddPCR)或实时 PCR 结合使用,检测从 NSCLC 患者体内提取的无细胞 DNA(cfDNA)中的这些突变:结果:ORNi-PCR 和 ddPCR/real-time PCR 检测出模型 cfDNA 中有 1-10 个 G1202R 和 L1196M DNA 拷贝。使用基于 ORNi-PCR 的方法在患者的 cfDNA 中确定了这些突变,而传统的 ddPCR 则未能检测到这些突变:结论:ORNi-PCR 和 ddPCR/real-time PCR 能够通过液体活检高度灵敏、准确地检测 ALK 基因突变。结论:ORNi-PCR 和 ddPCR/real-time PCR 可通过液体活检高度灵敏、准确地检测 ALK 突变,尽管临床数据有限,但我们的研究结果表明,这些方法可用于在复发早期识别 ALK-TKI 耐药的 NSCLC。
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来源期刊
Lung Cancer
Lung Cancer 医学-呼吸系统
CiteScore
9.40
自引率
3.80%
发文量
407
审稿时长
25 days
期刊介绍: Lung Cancer is an international publication covering the clinical, translational and basic science of malignancies of the lung and chest region.Original research articles, early reports, review articles, editorials and correspondence covering the prevention, epidemiology and etiology, basic biology, pathology, clinical assessment, surgery, chemotherapy, radiotherapy, combined treatment modalities, other treatment modalities and outcomes of lung cancer are welcome.
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