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基于双螺旋微流控芯片和实时 RPA 方法的循环肿瘤细胞中 EGFR 突变的快速检测。

Rapid detection of EGFR mutation in CTCs based on a double spiral microfluidic chip and the real-time RPA method.

机构信息

Department of Laboratory Medicine, Daping Hospital, Army Medical University, Chongqing, China.

Department of Cancer Center, Daping Hospital, Army Medical University, Chongqing, China.

出版信息

Anal Bioanal Chem. 2023 Jul;415(17):3535-3547. doi: 10.1007/s00216-023-04743-2. Epub 2023 May 31.

DOI:10.1007/s00216-023-04743-2
PMID:37254002
Abstract

Circulating tumor cells (CTCs) are cells shed from primary or metastatic tumors and spread into the peripheral bloodstream. Mutation detection in CTCs can reveal vital genetic information about the tumors and can be used for "liquid biopsy" to indicate cancer treatment and targeted medication. However, current methods to measure the mutations in CTCs are based on PCR or DNA sequencing which are cumbersome and time-consuming and require sophisticated equipment. These largely limited their applications especially in areas with poor healthcare infrastructure. Here we report a simple, convenient, and rapid method for mutation detection in CTCs, including an example of a deletion at exon 19 (Del19) of the epidermal growth factor receptor (EGFR). CTCs in the peripheral blood of NSCLC patients were first sorted by a double spiral microfluidic chip with high sorting efficiency and purity. The sorted cells were then lysed by proteinase K, and the E19del mutation was detected via real-time recombinase polymerase amplification (RPA). Combining the advantages of microfluidic sorting and real-time RPA, an accurate mutation determination was realized within 2 h without professional operation or complex data interpretation. The method detected as few as 3 cells and 1% target variants under a strongly interfering background, thus, indicating its great potential in the non-invasive diagnosis of E19del mutation for NSCLC patients. The method can be further extended by redesigning the primers and probes to detect other deletion mutations, insertion mutations, and fusion genes. It is expected to be a universal molecular diagnostic tool for real-time assessment of relevant mutations and precise adjustments in the care of oncology patients.

摘要

循环肿瘤细胞 (CTCs) 是从原发性或转移性肿瘤中脱落并散布到外周血液中的细胞。CTCs 中的突变检测可以揭示有关肿瘤的重要遗传信息,并可用于“液体活检”以指示癌症治疗和靶向药物治疗。然而,目前测量 CTC 中突变的方法基于 PCR 或 DNA 测序,这些方法繁琐且耗时,需要复杂的设备。这些在很大程度上限制了它们的应用,尤其是在医疗保健基础设施较差的地区。在这里,我们报告了一种用于 CTC 突变检测的简单、方便、快速的方法,包括表皮生长因子受体 (EGFR) 外显子 19 (Del19) 缺失的一个例子。首先,通过具有高效和高纯度的双螺旋微流控芯片对非小细胞肺癌 (NSCLC) 患者外周血中的 CTC 进行分选。然后用蛋白酶 K 裂解分选细胞,通过实时重组酶聚合扩增 (RPA) 检测 E19del 突变。将微流控分选和实时 RPA 的优势相结合,无需专业操作或复杂的数据解释,即可在 2 小时内实现准确的突变测定。该方法在强烈干扰背景下检测到的最低细胞数为 3 个,最低靶变体为 1%,因此,表明其在 NSCLC 患者的 E19del 突变非侵入性诊断中具有巨大潜力。通过重新设计引物和探针,可以进一步扩展该方法来检测其他缺失突变、插入突变和融合基因。预计它将成为实时评估相关突变和精确调整肿瘤患者治疗的通用分子诊断工具。

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