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首页> 美国卫生研究院文献>Cancers >Targeted Gene Next-Generation Sequencing Panel in Patients with Advanced Lung Adenocarcinoma: Paving the Way for Clinical Implementation
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Targeted Gene Next-Generation Sequencing Panel in Patients with Advanced Lung Adenocarcinoma: Paving the Way for Clinical Implementation

机译:晚期肺腺癌患者的靶向基因下一代测序组:为临床实施铺平道路

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Identification of targetable molecular changes is essential for selecting appropriate treatment in patients with advanced lung adenocarcinoma. Methods: In this study, a Sanger sequencing plus Fluorescence In Situ Hybridization (FISH) sequential approach was compared with a Next-Generation Sequencing (NGS)-based approach for the detection of actionable genomic mutations in an experimental cohort (EC) of 117 patients with advanced lung adenocarcinoma. Its applicability was assessed in small biopsies and cytology specimens previously tested for epidermal growth factor receptor (EGFR) and anaplastic lymphoma kinase (ALK) mutational status, comparing the molecular changes identified and the impact on clinical outcomes. Subsequently, an NGS-based approach was applied and tested in an implementation cohort (IC) in clinical practice. Using Sanger and FISH, patients were classified as EGFR-mutated (n = 22, 18.8%), ALK-mutated (n = 9, 7.7%), and unclassifiable (UC) (n = 86, 73.5%). Retesting the EC with NGS led to the identification of at least one gene variant in 56 (47.9%) patients, totaling 68 variants among all samples. Still, in the EC, combining NGS plus FISH for ALK, patients were classified as 23 (19.7%) EGFR; 20 (17.1%) KRAS; five (4.3%) B-Raf proto-oncogene (BRAF); one (0.9%) Erb-B2 Receptor Tyrosine Kinase 2 (ERBB2); one (0.9%) STK11; one (0.9%) TP53, and nine (7.7%) ALK mutated. Only 57 (48.7%) remained genomically UC, reducing the UC rate by 24.8%. Fourteen (12.0%) patients presented synchronous alterations. Concordance between NGS and Sanger for EGFR status was very high (κ = 0.972; 99.1%). In the IC, a combined DNA and RNA NGS panel was used in 123 patients. Genomic variants were found in 79 (64.2%). In addition, eight (6.3%) EML4-ALK, four (3.1%), KIF5B-RET, four (3.1%) CD74-ROS1, one (0.8%) TPM3-NTRK translocations and three (2.4%) exon 14 skipping MET Proto-Oncogene (MET) mutations were detected, and 36% were treatable alterations. Conclusions: This study supports the use of NGS as the first-line test for genomic profiling of patients with advanced lung adenocarcinoma.
机译:鉴定可靶向分子变化对于选择晚期肺腺癌患者的适当治疗至关重要。方法:在这项研究中,将Sanger测序加荧光原位杂交(FISH)顺序方法与基于下一代测序(NGS)的方法相比较,以检测117例实验队列(EC)中可操作的基因组突变晚期肺腺癌。在先前针对表皮生长因子受体(EGFR)和间变性淋巴瘤激酶(ALK)突变状态进行测试的小型活检和细胞学标本中评估了其适用性,比较了鉴定出的分子变化及其对临床结果的影响。随后,在临床实践的实施队列(IC)中应用了基于NGS的方法并对其进行了测试。使用Sanger和FISH,将患者分为EGFR突变(n = 22,18.8%),ALK突变(n = 9、7.7%)和无法分类(UC)(n = 86,73.5%)。用NGS对EC进行重新测试导致在56名(47.9%)患者中鉴定出至少一个基因变异,在所有样本中总共有68个变异。尽管如此,在EC中,结合NGS和FISH治疗ALK,患者被分类为23种(19.7%)EGFR。 20(17.1%)KRAS;五个(4.3%)B-Raf原癌基因(BRAF);一种(0.9%)Erb-B2受体酪氨酸激酶2(ERBB2);一(0.9%)STK11; 1个(0.9%)TP53和9个(7.7%)ALK突变。基因组上仅剩下57(48.7%)个UC,使UC率降低了24.8%。十四名(12.0%)患者出现同步改变。 NGS和Sanger对EGFR状态的一致性非常高(κ= 0.972; 99.1%)。在IC中,DNA和RNA NGS的组合用于123位患者。发现基因组变异的有79个(64.2%)。此外,八(6.3%)EML4-ALK,四(3.1%),KIF5B-RET,四(3.1%)CD74-ROS1,一(0.8%)TPM3-NTRK易位和三(2.4%)外显子14跳过MET检测到原癌基因(MET)突变,其中36%是可治疗的改变。结论:该研究支持NGS作为晚期肺腺癌患者基因组概况分析的一线测试。

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