CDKN2A和MTAP是可通过液滴数字PCR在恶性胸膜间皮瘤中检测到的有用生物标志物:与荧光杂交相比,是一种潜在的诊断替代方法。
CDKN2A and MTAP Are Useful Biomarkers Detectable by Droplet Digital PCR in Malignant Pleural Mesothelioma: A Potential Alternative Method in Diagnosis Compared to Fluorescence Hybridisation.
作者信息
Cheng Yuen Yee, Yuen Man Lee, Rath Emma M, Johnson Ben, Zhuang Ling, Yu Ta-Kun, Aleksova Vesna, Linton Anthony, Kao Steven, Clarke Candice Julie, McCaughan Brian C, Takahashi Ken, Lee Kenneth
机构信息
Asbestos Diseases Research Institute, Concord, NSW, Australia.
Giannoulatou Laboratory, Victor Chang Cardiac Research Institute, Darlinghurst, NSW, Australia.
出版信息
Front Oncol. 2020 Nov 13;10:579327. doi: 10.3389/fonc.2020.579327. eCollection 2020.
BACKGROUND
The diagnosis of malignant pleural mesothelioma (MPM) can be difficult, in part due to the difficulty in distinguishing between MPM and reactive mesothelial hyperplasia (RMH). The tumor suppressor gene, CDKN2A, is frequently silenced by epigenetic mechanisms in many cancers; in the case of MPM it is mostly silenced genomic deletion. Co-deletion of the CDKN2A and methylthioadenosine phosphorylase (MTAP) genes has been researched extensively and discovered to be a highly specific characteristic of MPM. Most studies have used FISH to detect the deletion of CDKN2A and IHC for MTAP as a surrogate for this. In this study, we aim to investigate and validate droplet digital PCR (ddPCR) as an emerging alternative and efficient testing method in diagnosing MPM, by particularly emphasizing on the loss of MTAP and CDKN2A.
METHODS
This study included 75 formalin fixed paraffin embedded (FFPE) MPM tissue, and 12 normal pleural tissue and 10 RMH as control. Additionally, primary MPM cell lines and normal pleural samples were used as biomarker detection controls, as established in our previous publication. All FFPE specimens were processed to isolate the DNA, that was subsequently used for ddPCR detection of CDKN2A and MTAP. FFPE samples were also analyzed by fluorescence hybridization (FISH) for CDKN2A and MTAP deletion, and for MTAP IHC expression. Concordance of IHC and ddPCR with FISH were studied in these samples.
RESULTS
95% and 82% of cases showed co-deletion of both MTAP and CDKN2A when determined by FISH and ddPCR respectively. ddPCR has a sensitivity of 72% and specificity of 100% in detecting CDKN2A homozygous loss in MPM. ddPCR also has a concordance rate of 92% with FISH in detecting homozygous loss of CDKN2A. MTAP IHC was 68% sensitive and 100% specific for detecting CDKN2A homozygous loss in MPM when these losses were determined by ddPCR.
CONCLUSION
Our study confirms that MTAP is often co-deleted with CDKN2A in MPM. Our in-house designed ddPCR assays for MTAP and CDKN2A are useful in differentiating MPM from RMH, and is highly concordant with FISH that is currently used in diagnosing MPM. ddPCR detection of these genetic losses can potentially be utilized as an alternative method in the diagnosis of MPM and for the future development of a less-invasive MPM-specific detection technique on MPM tumor tissue DNA.
背景
恶性胸膜间皮瘤(MPM)的诊断可能存在困难,部分原因是难以区分MPM与反应性间皮增生(RMH)。肿瘤抑制基因CDKN2A在许多癌症中常通过表观遗传机制沉默;在MPM中,它大多因基因组缺失而沉默。CDKN2A和甲硫腺苷磷酸化酶(MTAP)基因的共同缺失已得到广泛研究,并被发现是MPM的一个高度特异性特征。大多数研究使用荧光原位杂交(FISH)检测CDKN2A的缺失,并使用MTAP的免疫组化(IHC)作为替代方法。在本研究中,我们旨在研究和验证液滴数字PCR(ddPCR)作为一种新兴的、高效的检测方法在MPM诊断中的应用,特别强调MTAP和CDKN2A的缺失情况。
方法
本研究纳入75例福尔马林固定石蜡包埋(FFPE)的MPM组织,以及12例正常胸膜组织和10例RMH作为对照。此外,如我们之前发表的文章所述,使用原发性MPM细胞系和正常胸膜样本作为生物标志物检测对照。所有FFPE标本均经过处理以分离DNA,随后用于ddPCR检测CDKN2A和MTAP。FFPE样本还通过荧光原位杂交(FISH)分析CDKN2A和MTAP的缺失情况,以及MTAP的IHC表达。研究这些样本中IHC和ddPCR与FISH的一致性。
结果
分别通过FISH和ddPCR检测时,95%和82%的病例显示MTAP和CDKN2A均存在共同缺失。ddPCR检测MPM中CDKN2A纯合缺失的灵敏度为72%,特异性为100%。在检测CDKN2A纯合缺失方面,ddPCR与FISH的一致性率为92%。当通过ddPCR确定这些缺失时,MTAP的IHC检测MPM中CDKN2A纯合缺失的灵敏度为68%,特异性为100%。
结论
我们的研究证实,在MPM中MTAP常与CDKN2A共同缺失。我们内部设计的用于MTAP和CDKN2A的ddPCR检测方法有助于区分MPM与RMH,并且与目前用于诊断MPM的FISH高度一致。对这些基因缺失的ddPCR检测有可能作为MPM诊断的替代方法,并用于未来开发一种对MPM肿瘤组织DNA侵入性较小的MPM特异性检测技术。
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