UHRF1免疫组化染色从肉瘤样间皮瘤中分离良性反应性梭形细胞间皮增生。

Hang Yang, Simon Cheung, Andrew Churg
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引用次数: 1

摘要

良性和恶性间皮增生的分离往往是一个困难的病理问题。UHRF1(泛素样植物同源结构域和无名指结构域-1)是DNA甲基化的调节因子和多种人类癌症的表观遗传驱动因子。最近有报道称,UHRF1在间皮瘤中过表达。我们询问UHRF1免疫组织化学是否可以用于分离良性和恶性间皮增生。最初的研究表明,UHRF1可以染色间皮细胞,也可以染色内皮细胞和其他非肿瘤细胞,因此很难准确计数阳性间皮细胞。因此,我们对2个组织微阵列进行了双重UHRF1- ae1 /AE3染色,其中包含40个反应性间皮瘤细胞和61个间皮瘤细胞,仅计数角蛋白阳性细胞的UHRF1染色。平均10.3±8.6% (mean±SD;上皮样间皮瘤细胞染色范围:0%至36%,中位数:6.8%),而反应性上皮间皮瘤细胞染色范围为5.3±4.8%(范围:0%至15%,中位数:4.1%)。这种差异在统计上是显著的,但有太多的重叠,不能用于诊断。相比之下,肉瘤样间皮瘤中有37±26%(范围:2.5%至95%,中位数:31%)的细胞染色,而反应性梭形细胞间皮增生中有1.2±1.2%(范围:0%至3.0%,中位数:1.0%)的细胞染色。为了证实这种差异,我们对21例肉瘤样间皮瘤和19例组织性胸膜炎的全切片进行了染色。在组织性胸膜炎病例中,有2.1±2.4%(范围:0% ~ 6.8%,中位数:1.0%)和44±22%(范围:14% ~ 90%,中位数:41%)的间皮瘤细胞染色。我们得出结论,双重UHRF1-AE1/AE3免疫组化对分离良性梭形细胞间皮增生和肉瘤样间皮瘤非常有用。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
UHRF1 Immunohistochemical Staining Separates Benign Reactive Spindle Cell Mesothelial Proliferations From Sarcomatoid Mesotheliomas.

The separation of benign from malignant mesothelial proliferations is often a difficult pathologic problem. UHRF1 (ubiquitin-like with plant homeodomain and ring finger domains-1) is a regulator of DNA methylation and an epigenetic driver of various human cancers. It has recently been reported that UHRF1 is overexpressed in mesotheliomas. We asked whether UHRF1 immunohistochemistry could be used to separate benign from malignant mesothelial proliferations. Initial studies showed that UHRF1 stained mesothelial cells but also endothelial and other non-neoplastic cells, so that accurate counting of positive mesothelial cells was difficult. Therefore, we ran dual UHRF1-AE1/AE3 stains on 2 tissue microarrays containing 40 reactive mesothelial proliferations and 61 mesotheliomas and only counted UHRF1 staining in keratin-positive cells. On average 10.3±8.6% (mean±SD; range: 0% to 36, median: 6.8%) of epithelioid mesothelioma cells stained compared with 5.3±4.8% (range: 0% to 15%, median: 4.1%) of reactive epithelial mesothelial cells. This difference was statistically significant but there was too much overlap to use diagnostically. In contrast, 37±26% (range: 2.5% to 95%, median: 31%) of cells in sarcomatoid mesotheliomas compared with 1.2±1.2% (range: 0% to 3.0%, median: 1.0%) of cells in reactive spindle cell mesothelial proliferations stained. To confirm this difference we stained whole sections of 21 sarcomatoid mesotheliomas and 19 cases of organizing pleuritis. Staining of mesothelial cells was seen in 2.1±2.4% (range: 0% to 6.8%, median: 1.0%) of organizing pleuritis cases and 44±22% (range: 14% to 90%, median: 41%) of sarcomatoid mesotheliomas. We conclude that dual UHRF1-AE1/AE3 immunohistochemistry is very useful for separating benign spindle cell mesothelial proliferations from sarcomatoid mesotheliomas.

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