Addamo-De Nard Bianca, Geissmann Meret, Akhoundova Dilara, Pistoni Clelia, Brezina Tomas, Zoche Martin, Weber Achim, Hussung Saskia, Fritsch Ralph
Department of Medical Oncology and Hematology, University Hospital Zurich, Zurich, Switzerland.
Department of Medical Oncology, Bern University Hospital, University of Bern, Bern, Switzerland.
Diagn Pathol. 2025 May 24;20(1):62. doi: 10.1186/s13000-025-01637-y.
KRAS exon 2 mutations are highly prevalent in human malignancies, making them attractive targets for detection and monitoring in cell-free DNA (cfDNA) of cancer patients. Drop-off assays designed for digital polymerase chain reaction (ddPCR drop-off) span entire mutational hotspots and detect any mutated allele within the covered region, overcoming a major limitation of mutation-specific ddPCR assays. We therefore set out to develop a novel KRAS codon 12/13 ddPCR drop-off assay for the robust, highly sensitive and specific detection of KRAS exon 2 hotspot mutations in cfDNA.
We designed, optimized and extensively validated a KRAS codon 12/13 ddPCR drop-off assay. We compared assay performance to a commercially available KRAS multiplex assay. For clinical validation, we analyzed plasma samples collected from patients with KRAS-mutated gastrointestinal malignancies.
Limit of detection of the newly established ddPCR drop-off assay was 0.57 copies/µL, limit of blank was 0.13 copies/µ. The inter-assay precision (r) was 0.9096. Our newly developed KRAS ddPCR drop-off assay accurately identified single nucleotide variants in 35/36 (97.2%) of circulating tumor DNA-positive samples from the patient validation cohort. Assay cross-validation showed that the newly established KRAS codon 12/13 ddPCR drop-off assay outperformed a commercially available KRAS multiplex ddPCR assay in terms of specificity. Moreover, the newly developed assay proved to be suitable for multiplexing with mutation-specific probes.
We developed and clinically validated a highly accurate ddPCR drop-off assay for KRAS exon 2 hot-spot detection in cfDNA with broad applicability for clinic and research.
KRAS外显子2突变在人类恶性肿瘤中高度普遍,使其成为癌症患者游离DNA(cfDNA)检测和监测的有吸引力的靶点。为数字聚合酶链反应设计的缺失检测法(ddPCR缺失检测法)覆盖整个突变热点区域,并检测覆盖区域内的任何突变等位基因,克服了突变特异性ddPCR检测法的一个主要局限性。因此,我们着手开发一种新型的KRAS密码子12/13 ddPCR缺失检测法,用于在cfDNA中稳健、高度灵敏且特异检测KRAS外显子2热点突变。
我们设计、优化并广泛验证了一种KRAS密码子12/13 ddPCR缺失检测法。我们将该检测法的性能与市售的KRAS多重检测法进行了比较。为进行临床验证,我们分析了从KRAS突变的胃肠道恶性肿瘤患者采集的血浆样本。
新建立的ddPCR缺失检测法的检测限为0.57拷贝/微升,空白限为0.13拷贝/微升。批间精密度(r)为0.9096。我们新开发的KRAS ddPCR缺失检测法在患者验证队列中35/36(97.2%)的循环肿瘤DNA阳性样本中准确鉴定出单核苷酸变体。检测交叉验证表明,新建立的KRAS密码子12/13 ddPCR缺失检测法在特异性方面优于市售的KRAS多重ddPCR检测法。此外,新开发的检测法被证明适用于与突变特异性探针进行多重检测。
我们开发并临床验证了一种高度准确的ddPCR缺失检测法,用于在cfDNA中检测KRAS外显子2热点突变,在临床和研究中具有广泛的适用性。
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