包体痣BCL-2的免疫组织化学表达:组织芯片研究。

IF 4.4 Q1 PATHOLOGY
PATHOLOGICA Pub Date : 2023-05-01 DOI:10.32074/1591-951X-824
Muna Al-Jabri, Suaad Al-Badi, Hunaina Al-Kindi, Mohammad Arafa
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引用次数: 0

摘要

背景:包体痣(HM)是妊娠滋养细胞疾病(GTD)的成员,在某些情况下,可能发展为妊娠滋养细胞瘤(GTN)。hmm分为部分(PHM)和完全(CHM)。一些HMs在精确的组织病理学诊断方面具有挑战性。本研究旨在利用组织微阵列技术(Tissue MicroArray, TMA),通过免疫组化(IHC)方法研究BCL-2在人造血干细胞和正常滋养细胞组织“受孕产物(POC)和胎盘”中的表达。方法:利用237例HMs (PHM组织95例,CHM组织142例)和202例对照正常滋养细胞组织的档案材料构建tma;POC和不明显的胎盘。切片采用抗BCL-2抗体免疫组织化学染色。对不同细胞成分(滋养层细胞和基质细胞)的染色进行半定量评估(阳性细胞的强度和百分比)。结果:BCL-2在PHM、CHM和对照组的滋养细胞中均有95%以上的细胞质表达。染色结果显示,细胞强度从对照组(73.7%)、PHMs(76.3%)到CHM(26.9%)显著降低。PHM与CHM在强度(p值0.0005)和总分(p值0.0005)上差异有统计学意义,但在百分比得分上差异无统计学意义(p值> 0.05)。各组间绒毛间质细胞阳性率差异无统计学意义。在90%以上的病例中,使用两个斑点/病例(每个直径3毫米)的TMA模型可以看到所有细胞成分。结论:与PHM和正常滋养细胞相比,CHM中BCL-2表达降低表明细胞凋亡增加,滋养细胞增殖不受控制。使用直径为3mm的核构建重复的TMA可以克服复杂病变的组织异质性。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Immunohistochemical expression of BCL-2 in hydatidiform moles: a tissue microarray study.

Immunohistochemical expression of BCL-2 in hydatidiform moles: a tissue microarray study.

Immunohistochemical expression of BCL-2 in hydatidiform moles: a tissue microarray study.

Immunohistochemical expression of BCL-2 in hydatidiform moles: a tissue microarray study.

Background: Hydatidiform moles (HM) are members of gestational trophoblastic diseases (GTD) and, in some cases, might progress to gestational trophoblastic neoplasia (GTN). HMs are either partial (PHM) or complete (CHM). Some HMs are challenging in arriving at a precise histopathological diagnosis. This study aims to investigate the expression of BCL-2 by immunohistochemistry (IHC) in HMs as well as in normal trophoblastic tissues "products of conception (POC) and placentas" using Tissue MicroArray (TMA) technique.

Methods: TMAs were constructed using the archival material of 237 HMs (95 PHM and 142 CHM) and 202 control normal trophoblastic tissues; POC and unremarkable placentas. Sections were immunohistochemically stained using antibodies against BCL-2. The staining was assessed semi-quantatively (intensity and percentage of the positive cells) in different cellular components (trophoblasts and stromal cells).

Results: BCL-2 showed cytoplasmic expression in more than 95% of trophoblasts of PHM, CHM and controls. The staining showed a significant reduction of the intensity from controls (73.7%), PHMs (76.3%) to CHM (26.9%). There was a statistically significant difference between PHM and CHM in the intensity (p-value 0.0005) and the overall scores (p-value 0.0005), but not the percentage score (p-value > 0.05). No significant difference was observed in the positivity of the villous stromal cells between the different groups. All cellular components were visible using the TMA model of two spots/case (3 mm diameter, each) in more than 90% of cases.

Conclusions: Decreased BCL-2 expression in CHM compared to PHM and normal trophoblasts indicates increased apoptosis and uncontrolled trophoblastic proliferation. Construction of TMA in duplicates using cores of 3 mm diameter can overcome tissue heterogeneity of complex lesions.

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来源期刊
PATHOLOGICA
PATHOLOGICA PATHOLOGY-
CiteScore
5.90
自引率
5.70%
发文量
108
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