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首页> 外文期刊>Breast Cancer Research and Treatment >Molecular detection of breast cancer metastasis in sentinel lymph nodes by reverse transcriptase polymerase chain reaction (RT-PCR): identifying, evaluating and establishing multi-marker panels
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Molecular detection of breast cancer metastasis in sentinel lymph nodes by reverse transcriptase polymerase chain reaction (RT-PCR): identifying, evaluating and establishing multi-marker panels

机译:逆转录聚合酶链反应(RT-PCR)分子检测前哨淋巴结中的乳腺癌转移:鉴定,评估和建立多标记面板

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The potential advantage of using quantitative reverse transcriptase polymerase chain reaction (qRT-PCR) methodology to detect metastasis in sentinel lymph nodes (SLNs) of breast cancer (BC) patients was evaluated in this prospective study. We measured the expression of relevant gene transcripts in SLNs using an innovative algorithm and compared the results of single-marker assays versus multi-marker assays with conventional histological detection methods. SLNs from women aged ≥18 years diagnosed with unilateral BC were examined by haematoxylin-eosin staining and immunohistochemistry and analysed for transcripts of several relevant genes using qRT-PCR (learning group). Four candidate panels of expressed transcript combinations with high sensitivity and specificity were selected for further investigation. The candidate panels were then validated using SLNs from a second group of BC patients (validation group). In the learning group, 74/314 SLN sections from 150 patients were positive for metastasis by histology. The transcripts analysed showed the following individual sensitivities/specificities: cytokeratin 19 (CK19) 94.6%/97.9%; mammaglobin 1 (MGB1) 82.4%/91.7%; mammaglobin 2 (MGB2) 82.4%/96.7%; carcinoembryonic antigen (CEA) 71.6%/97.5%; EPCAM (epithelial cell adhesion molecule) 91.9%/97.1%; and NY-BR-1 82.4%/93.8%. The optimal panel based on the predefined criteria comprised four markers: CK19, MGB1, EPCAM, and NY-BR-1, of which ≥2 had to be positive (95.9% sensitivity, 95.0% specificity, 85.5% positive predictive value (PPV), and 98.7% negative predictive value (NPV)). Overall concordance with histology was 95.2%. In the validation group, 84/315 SLN sections from 235 patients were histologically positive, and panel sensitivity, specificity and overall accuracy were 88.1, 95.2 and 93.3%, respectively, at the SLN section level. In conclusion, molecular staging using expression patterns of relevant transcripts in SLNs could serve as a useful complement to standard diagnostic work-up in BC patients. The proposed flexible multi-parametric approach does not improve the overall accuracy compared with the single-marker approach. However, it overcomes several limitations of the previously reported molecular assays for SLN diagnosis.
机译:在这项前瞻性研究中,评估了使用定量逆转录酶聚合酶链反应(qRT-PCR)方法检测乳腺癌(BC)患者前哨淋巴结(SLN)中转移的潜在优势。我们使用创新的算法测量了SLNs中相关基因转录物的表达,并使用传统的组织学检测方法比较了单标记法与多标记法的结果。通过苏木精-伊红染色和免疫组织化学检查了诊断为单侧BC的≥18岁女性的SLN,并使用qRT-PCR分析了几个相关基因的转录本(学习组)。选择了四个具有高灵敏度和特异性的转录本组合候选候选人进行进一步研究。然后使用第二组BC患者(验证组)的SLN验证候选面板。在学习组中,通过组织学检查,来自150例患者的74/314 SLN切片转移阳性。分析的转录本显示出以下个体敏感性/特异性:细胞角蛋白19(CK19)为94.6%/ 97.9%;乳球蛋白1(MGB1)82.4%/ 91.7%;乳球蛋白2(MGB2)82.4%/ 96.7%;癌胚抗原(CEA)71.6%/ 97.5%; EPCAM(上皮细胞粘附分子)为91.9%/ 97.1%;和NY-BR-1 82.4%/ 93.8%。基于预定义标准的最佳面板包括四个标记:CK19,MGB1,EPCAM和NY-BR-1,其中必须≥2为阳性(95.9%敏感性,95.0%特异性,85.5%阳性预测值(PPV) ,以及98.7%的负面预测值(NPV))。与组织学的总体一致性为95.2%。在验证组中,来自235名患者的84/315个SLN切片在组织学上呈阳性,在SLN切片水平上,小组敏感性,特异性和总体准确性分别为88.1%,95.2%和93.3%。总之,使用SLN中相关转录本的表达模式进行的分子分期可以作为BC患者标准诊断检查的有益补充。与单标记方法相比,所提出的灵活的多参数方法不会提高整体准确性。但是,它克服了先前报道的用于SLN诊断的分子测定法的一些局限性。

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