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首页> 外文期刊>Applied immunohistochemistry and molecular morphology: AIMM >Validation of a Manual Protocol for BRAF V600E Mutation-specific Immunohistochemistry
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Validation of a Manual Protocol for BRAF V600E Mutation-specific Immunohistochemistry

机译:验证BRAF V600E突变特异性免疫组织化学手册的方法

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Detection of BRAF V600E has diagnostic, prognostic, and therapeutic relevance. The recently developed BRAF V600E mutation-specific antibody has evolved into a feasible alternative to DNA analysis. The plethora of immunohistochemical protocols makes implementation tedious and, here we tested a set of manual and automated protocols and compared test performance with sequencing results. For assays, we employed formalin-fixed, in part decalcified, and paraffin-embedded tissue samples. Empiric testing of manual protocols included 10 variables in 17 protocols. Automated immunohistochemical staining and BRAF pyrosequencing served as independent test methods. Test performance measures were compared without considering 1 method as a standard. Four well-fixed samples (2WT/2Mut) were used for testing of all protocols and indicated 2 correctly classifying procedures. Practical performance assessment employed 33 independent tissue samples, composed of 27 leukemias (by pyrosequencing: 8 wild-type; 18 mutated; 1 noninformative) and 6 melanomas (V600E; V600K; wild-type, 2 each). Manual V600E staining was positive in 20 cases (19 of 20 V600E-con-taining samples plus the 1 sample that was noninformative), whereas all wild-type and V600K cases were immunonegative. Manual or automated staining as well as pyrosequencing would have missed an equal number of V600E-mutated cases and the correlation coefficient for these methods was 0.75 to 0.93 (substantial to almost perfect); the Youden index was 0.95. Detection of V600E-mutated BRAF at the protein level in routine and decalcified tissue samples is possible, and the presented manual protocols should expedite implementation in routine diagnostic practice. Our results indicate that both molecular techniques should be considered complementary.
机译:检测BRAF V600E具有诊断,预后和治疗意义。最近开发的BRAF V600E突变特异性抗体已发展成为DNA分析的可行替代方案。大量的免疫组化方案使实施变得乏味,在这里,我们测试了一组手动和自动化方案,并将测试性能与测序结果进行了比较。对于测定,我们采用了福尔马林固定的,部分脱钙的和石蜡包埋的组织样品。手动协议的经验测试包括17个协议中的10个变量。自动化的免疫组织化学染色和BRAF焦磷酸测序是独立的测试方法。比较了测试性能指标,而未考虑将一种方法作为标准。使用四个固定良好的样品(2WT / 2Mut)测试所有方案,并指出2种正确的分类程序。实际表现评估使用了33个独立的组织样本,包括27个白血病(通过焦磷酸测序:8个野生型; 18个突变; 1个非信息性)和6个黑色素瘤(V600E; V600K;野生型,每个2个)。手动V600E染色在20例中为阳性(20个包含V600E的样本中有19个加上1个非参考性样本),而所有野生型和V600K病例均为免疫阴性。手工或自动染色以及焦磷酸测序将漏掉相等数量的V600E突变病例,而这些方法的相关系数为0.75至0.93(基本到几乎完美)。尤登指数为0.95。可以在常规和脱钙的组织样品中检测蛋白水平的V600E突变型BRAF,并且提出的手册操作规程应加快常规诊断实践中的实施。我们的结果表明,两种分子技术都应被认为是互补的。

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