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短的57 kb荧光原位杂交(FISH)探针可有效检测恶性胸膜间皮瘤中9p21位点的短纯合缺失。

Short 57 kb FISH probe effectively detects short homozygous deletion of the 9p21 locus in malignant pleural mesothelioma.

作者信息

Oyama Yuzo, Hamasaki Makoto, Matsumoto Shinji, Sato Ayuko, Tsujimura Tohru, Nabeshima Kazuki

机构信息

Department of Pathology, Fukuoka University Hospital and School of Medicine, Jonan-ku, Fukuoka 814-0180, Japan.

Department of Pathology, Hyogo College of Medicine, Nishinomiya, Hyogo 663-8131, Japan.

出版信息

Oncol Lett. 2021 Dec;22(6):813. doi: 10.3892/ol.2021.13074. Epub 2021 Sep 28.

Abstract

Homozygous deletion (homo-d) of the cyclin-dependent kinase inhibitor 2A () gene is frequently found in malignant pleural mesothelioma (MPM). Fluorescence hybridization (FISH) is commonly used to detect chromosomal deletion, and sometimes reveals more frequent heterozygous deletion (hetero-d) compared with homo-d. In clinical practice, such FISH results belong to the 'borderline' homo-d rate, which makes it difficult to definitively diagnose MPM. Microdeletion, [<200 kilobase (kb)], can induce a 'pseudo' hetero-d signal in FISH assays with long probes owing to redundant probe reactivity. Thus, the present study hypothesized that shorter FISH probes can effectively detect the small deletion status of the gene and increase homo-d rate in MPM, which has high hetero-d and low homo-d status. The present study aimed to evaluate the effectiveness of a shorter FISH probe in diagnosing MPM. FISH with either a 222 kb long probe (L-probe) or a 57 kb short probe (S-probe) was performed in four MPM cases with high hetero-d and low homo-d patterns. Furthermore, immunohistochemistry for methylthioadenosine phosphorylase (MTAP) and quantitative (q)PCR analyses were performed to confirm the microdeletion of the 9p21 locus. The results demonstrated that all four MPM cases retained MTAP protein expression. FISH with L-probe revealed high hetero-d (cases 1-4; 73.3, 37.1, 59.2 and 64.8%, respectively) and low homo-d (cases 1-4; 12.1, 12.4, 25.4 and 22.2%, respectively). FISH with S-probe revealed high homo-d (cases 1-4; 96.8, 90.0, 87.5 and 82.6%, respectively), with low hetero-d (cases 1-4; 0.0, 1.2, 1.2 and 4.3%, respectively). qPCR analysis demonstrated no allele deletions of the gene and two-allele deletions of the gene in 3/4 cases. Taken together, these results suggest that the S-probe detects the short homo-d of the 9p21 locus more effectively than the L-probe in MPM. This can assist in solving diagnostic difficulties in cases involving high hetero-d with low homo-d.

摘要

细胞周期蛋白依赖性激酶抑制剂2A()基因的纯合缺失(homo-d)在恶性胸膜间皮瘤(MPM)中经常被发现。荧光原位杂交(FISH)通常用于检测染色体缺失,有时与纯合缺失相比,杂合缺失(hetero-d)更为常见。在临床实践中,这样的FISH结果属于“临界”纯合缺失率,这使得MPM的明确诊断变得困难。微缺失,[<200千碱基(kb)],由于多余的探针反应性,在使用长探针的FISH检测中可诱导“假”杂合缺失信号。因此,本研究假设较短的FISH探针可以有效地检测基因的小缺失状态,并提高MPM中纯合缺失率,MPM具有高杂合缺失和低纯合缺失状态。本研究旨在评估较短的FISH探针在诊断MPM中的有效性。对4例具有高杂合缺失和低纯合缺失模式的MPM病例进行了222 kb长探针(L-探针)或57 kb短探针(S-探针)的FISH检测。此外,进行了甲硫腺苷磷酸化酶(MTAP)的免疫组织化学和定量(q)PCR分析,以确认9p21位点的微缺失。结果表明,所有4例MPM病例均保留MTAP蛋白表达。L-探针的FISH显示高杂合缺失(病例1-4;分别为73.3%、37.1%、59.2%和64.8%)和低纯合缺失(病例1-4;分别为12.1%、12.4%、25.4%和22.2%)。S-探针的FISH显示高纯合缺失(病例1-4;分别为96.8%) 90.0%、87.5%和82.6%),杂合缺失率低(病例1-4;分别为0.0%、1.2%、1.2%和4.3%)。qPCR分析显示,3/4的病例中基因无等位基因缺失,基因有双等位基因缺失。综上所述,这些结果表明,在MPM中,S-探针比L-探针更有效地检测9p21位点的短纯合缺失。这有助于解决高杂合缺失和低纯合缺失病例的诊断困难。

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