Herdt Leah Rowland, Berroteran Paige, Rajagopalan Malini, Brown Bradley A, Schwartz Jerrod J
ChromaCode Inc., 2330 Faraday Ave, Carlsbad, CA 92008, USA.
Diagnostics (Basel). 2024 Jan 24;14(3):243. doi: 10.3390/diagnostics14030243.
Molecular diagnostics has drastically improved the survival rate of patients diagnosed with non-small cell lung cancer (NSCLC) over the last 10 years. Despite advancements in molecular testing, targeted therapies, and national guideline recommendations, more than half of NSCLC patients in the United States either never receive testing or patient care is not informed via molecular testing. Here, we sought to explore the relationship between DNA/RNA input, the molecular testing method, and test success rates. On a shared set of low-input reference test materials ( = 3), we ran both a hybrid capture-based, next-generation sequencing (NGS) assay and a multiplexed digital PCR (dPCR) panel. The dPCR panel was highly sensitive and specific for low-input samples in dilution studies ranging from 40 to 1 ng DNA and from 20 to 2.5 ng RNA, while NGS had up to an 86% loss in sensitivity as contrived sample inputs were serially diluted. The dPCR panel also demonstrated a high PPA (>95%) at diluted inputs as low as 15/7.5 ng DNA/RNA on 23 banked clinical samples with the same NGS hybrid capture assay at a high input. These data suggest that digital PCR is an accurate and effective way of identifying clinically relevant NSCLC mutations at low nucleotide input and quality.
在过去十年中,分子诊断极大地提高了被诊断为非小细胞肺癌(NSCLC)患者的生存率。尽管在分子检测、靶向治疗和国家指南推荐方面取得了进展,但在美国,超过一半的NSCLC患者要么从未接受检测,要么患者护理未通过分子检测得到告知。在此,我们试图探索DNA/RNA输入量、分子检测方法与检测成功率之间的关系。在一组共享的低输入量参考测试材料(n = 3)上,我们同时进行了基于杂交捕获的下一代测序(NGS)检测和多重数字PCR(dPCR)检测板。在DNA稀释范围为40至1 ng、RNA稀释范围为20至2.5 ng的稀释研究中,dPCR检测板对低输入量样本具有高度敏感性和特异性,而随着人为设定的样本输入量连续稀释,NGS的敏感性损失高达86%。在23份保存的临床样本上,dPCR检测板在低至15/7.5 ng DNA/RNA的稀释输入量下也表现出高阳性百分一致率(>95%),而相同样本在高输入量时采用的是NGS杂交捕获检测。这些数据表明,数字PCR是一种在低核苷酸输入量和质量下识别临床相关NSCLC突变的准确且有效的方法。
