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尤文肉瘤中致癌性螺旋-环-螺旋蛋白Id2的上调。

Upregulation of the oncogenic helix-loop-helix protein Id2 in Ewing sarcoma.

作者信息

Park Hye-Rim, Jung Woon Won, Kim Hyun Sook, Santini-Araujo Eduard, Kalil Ricardo K, Bacchini Patrizia, Bertoni Franco, Unni K Krishnan, Park Yong-Koo

机构信息

Department of Pathology, College of Medicine, Hallym University, Anyang, Korea.

出版信息

Tumori. 2006 May-Jun;92(3):236-40.

Abstract

AIMS AND BACKGROUND

Id helix-loop-helix proteins function as regulators of cell growth and differentiation. However, they can induce malignant transformation when overexpressed. The EWS/ETS chimeric proteins in Ewing sarcoma act as aberrant transcription factors leading to tumorigenic processes. An enhanced expression of the Id2 gene in Ewing sarcoma cells was previously shown by gene array techniques. We investigated the expression of Id2 at the protein and gene level in Ewing sarcoma.

METHODS

We evaluated the expression of Id2 protein using immunohistochemistry in formalin-fixed, paraffin-embedded specimens from a total of 71 cases of Ewing sarcoma. Additionally, a Ewing sarcoma cell line was examined by real-time quantitative PCR.

RESULTS

Id2 expression was observed in 65 cases (91.5%) of the 71 total cases examined and a high level of Id2 expression was observed in 45 of these cases (63.8%). In tumor cells, Id2 proteins displayed cytoplasmic as well as nuclear localization. The amplification of the Id2 gene was not noted in a Ewing sarcoma cell line using real-time quantitative PCR. The crossing points of Id2 in the Ewing sarcoma cell line, control fibroblast, and osteosarcoma cell line were 18.54 +/- 0.16, 18.25, and 18.34, respectively.

CONCLUSIONS

Our data support a role for increased Id2 protein expression in Ewing sarcoma. However, this overexpression of the Id2 protein could not be confirmed by a corresponding change at the gene level in a Ewing sarcoma cell line.

摘要

目的与背景

Id螺旋-环-螺旋蛋白作为细胞生长和分化的调节因子发挥作用。然而,当它们过度表达时可诱导恶性转化。尤因肉瘤中的EWS/ETS嵌合蛋白作为异常转录因子导致致瘤过程。先前通过基因芯片技术显示尤因肉瘤细胞中Id2基因表达增强。我们研究了尤因肉瘤中Id2在蛋白和基因水平的表达。

方法

我们使用免疫组织化学评估了来自总共71例尤因肉瘤的福尔马林固定、石蜡包埋标本中Id2蛋白的表达。此外,通过实时定量PCR检测了一种尤因肉瘤细胞系。

结果

在总共检查的71例病例中的65例(91.5%)观察到Id2表达,其中45例(63.8%)观察到高水平的Id2表达。在肿瘤细胞中,Id2蛋白显示出胞质和核定位。使用实时定量PCR在尤因肉瘤细胞系中未发现Id2基因的扩增。尤因肉瘤细胞系、对照成纤维细胞和骨肉瘤细胞系中Id2的交叉点分别为18.54±0.16、18.25和18.34。

结论

我们的数据支持Id2蛋白表达增加在尤因肉瘤中所起的作用。然而,在尤因肉瘤细胞系中,这种Id2蛋白的过度表达无法通过基因水平的相应变化得到证实。

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