[Verification of the diagnosis of supratentorial ependymomas by real-time PCR].

Q4 Medicine

Arkhiv patologii Pub Date : 2023-01-01 DOI:10.17116/patol2023850315

S A Galstyan, E N Telysheva, A O Lavrinovich, E G Shaikhaev, G P Snigireva, E I Petrova, S K Gorelyshev, O G Zheludkova, Y V Kushel, E V Kumirova, M V Ryzhova

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引用次数: 0

Abstract

Background: Differential diagnosis of supratentorial ependymomas is of particular difficulty in neurooncology due to nonspecific clinical and radiographic findings, a rare seen «classic» morphological picture, and a nonspecific immunophenotype. Thanks to molecular genetic methods, in particular real-time PCR, it has become possible to verify supratentorial ependymomas and identify their molecular group, on which further prognosis depends.

Objective: To develop a set of molecular genetic tests based on real-time PCR to verify supratentorial ependymomas.

Material and methods: 56 tissue samples were collected from patients with supratentorial ependymomas, WHO Grade II, and anaplastic ependymomas, WHO Grade III. We developed primers and fluorescent TaqMan probes for real-time PCR analysis to detect the ZFTA::RELA, ZFTA::MAML2, ZFTA::NCOA2, ZFTA::MAML3, YAP1::MAMLD1, and YAP1::FAM118B gene fusions. For immunohistochemical analysis, monoclonal rabbit anti-NF-kb p65 antibodies (HUABIO, China) were used, the study was carried out on AutostainerLink 48 immunostainer (DAKO, Denmark).

Results: Real-time PCR was able to verify the diagnosis for 69.9% (n=39) of samples and classify them into molecular groups of ZFTA- or YAP1-positive supratentorial ependymomas. Immunohistochemically it was possible to verify 58% (n=29) ependymomas.

Conclusion: Diagnosis by real-time PCR is a relatively fast, accessible and easily interpreted method that allows verification of the molecular group in 70% of cases of supratentorial ependymomas without the use of additional methods.

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[实时荧光定量PCR诊断幕上室管膜瘤的验证]。

背景:在神经肿瘤学中，幕上室管膜瘤的鉴别诊断是特别困难的，因为它的临床和影像学表现是非特异性的，罕见的“经典”形态学图像，以及非特异性的免疫表型。由于分子遗传学方法，特别是实时PCR，已经有可能验证幕上室管膜瘤，并确定其分子群，进一步的预后取决于。目的:建立一套实时荧光定量PCR检测幕上室管膜瘤的分子遗传学方法。材料和方法:收集幕上室管膜瘤(WHO II级)和间变性室管膜瘤(WHO III级)患者的56份组织样本。我们开发了引物和荧光TaqMan探针，用于实时PCR分析ZFTA::RELA、ZFTA::MAML2、ZFTA::NCOA2、ZFTA::MAML3、YAP1::MAMLD1和YAP1::FAM118B基因融合。免疫组化分析采用兔抗nf -kb p65单克隆抗体(中国华比奥)，在AutostainerLink 48免疫染色仪(丹麦DAKO)上进行。结果:实时荧光定量PCR对69.9% (n=39)的样本诊断正确，并将其分类为ZFTA-或yap1阳性的幕上室管膜瘤分子组。免疫组织化学可以证实58% (n=29)室管膜瘤。结论:实时荧光定量PCR诊断是一种相对快速、方便且易于解释的方法，在70%的幕上室管膜瘤病例中，无需使用其他方法即可验证分子群。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Arkhiv patologii Medicine-Pathology and Forensic Medicine

CiteScore

0.90

自引率

0.00%

发文量

期刊介绍： The journal deals with original investigations on pressing problems of general pathology and pathologic anatomy, newest research methods, major issues of the theory and practice as well as problems of experimental, comparative and geographic pathology. To inform readers latest achievements of Russian and foreign medicine the journal regularly publishes editorial and survey articles, reviews of the most interesting Russian and foreign books on pathologic anatomy, new data on modern methods of investigation (histochemistry, electron microscopy, autoradiography, etc.), about problems of teaching, articles on the history of pathological anatomy development both in Russia and abroad.