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在一项对早期激素阴性乳腺癌的回顾性研究中,恶性肿瘤以及癌症相关基质中低水平的ATM蛋白表达是独立的预后因素。

Low ATM protein expression in malignant tumor as well as cancer-associated stroma are independent prognostic factors in a retrospective study of early-stage hormone-negative breast cancer.

作者信息

Feng Xiaolan, Li Haocheng, Dean Michelle, Wilson Holly E, Kornaga Elizabeth, Enwere Emeka K, Tang Patricia, Paterson Alexander, Lees-Miller Susan P, Magliocco Anthony M, Bebb Gwyn

机构信息

Department of Oncology, Tom Baker Cancer Centre and University of Calgary, 1331 29th Street NW, Calgary, AB, T2N 4 N2, Canada.

Department of Community Health Science, TRW Building, University of Calgary, 3280 Hospital Drive NW, Calgary, AB, T2N 4Z6, Canada.

出版信息

Breast Cancer Res. 2015 May 3;17(1):65. doi: 10.1186/s13058-015-0575-2.

Abstract

INTRODUCTION

The serine/threonine protein kinase ataxia telangiectasia mutated (ATM) is critical in maintaining genomic integrity. Upon DNA double-strand breaks, ATM phosphorylates key downstream proteins including p53 and BRCA1/2, thereby orchestrating complex signaling pathways involved in cell cycle arrest, DNA repair, senescence and apoptosis. Although sporadic mutation of ATM occurs rarely in breast cancer, the status of its protein expression and its clinical significance in breast cancer remain not well established. Our study was designed to investigate the influence of ATM protein in both tumor and cancer-associated stroma on clinical outcome in hormone-positive (HPBC) and hormone-negative (HNBC) early-stage breast cancer (EBC).

METHODS

Tissue microarrays (TMAs), containing formalin-fixed, paraffin-embedded resected tumors from two cohorts of patients (HPBC cohort: n=130; HNBC cohort: n=168) diagnosed at the Tom Baker Cancer Centre, Calgary, Canada, were analyzed for ATM protein expression using fluorescence immunohistochemistry (IHC) and automated quantitative analysis (AQUA). ATM expression levels were measured within the tumor as a whole (tATM) as indicated by pan-cytokeratin expression, tumor nuclear compartment (nATM) as indicated by both DAPI and pan-cytokeratin-positive results, and cancer-associated stroma (csATM) as indicated by vimentin-positive and pan-cytokeratin-negative results. ATM expression levels within these compartments were correlated with clinical outcome.

RESULTS

While tATM and nATM were significantly lower in tumors compared to normal breast epithelial tissues, csATM was significantly higher than the corresponding normal tissue compartment. In addition, the median expression level of both tATM and nATM were two- to threefold lower (P<0.001) in HNBC than in HPBC. In both HNBC and HPBC cohorts, patients with low tATM, nATM and csATM tumors had significantly poorer survival outcomes than those with a high tATM, nATM and csATM, but this effect was more pronounced in HNBC. A multivariate analysis demonstrates that these biomarkers predict survival independent of tumor size and lymph node status, but only in the HNBC cohort (P<0.001).

CONCLUSIONS

Low ATM protein expression in both malignant tumor and stromal compartments likely contributes to the aggressive nature of breast cancer and is an independent prognostic factor associated with worse survival in HNBC patients.

摘要

引言

丝氨酸/苏氨酸蛋白激酶共济失调毛细血管扩张症突变体(ATM)在维持基因组完整性方面至关重要。在DNA双链断裂时,ATM会磷酸化包括p53和BRCA1/2在内的关键下游蛋白,从而协调参与细胞周期停滞、DNA修复、衰老和凋亡的复杂信号通路。尽管ATM的散发性突变在乳腺癌中很少见,但其蛋白表达状态及其在乳腺癌中的临床意义仍未完全明确。我们的研究旨在调查肿瘤和癌症相关基质中ATM蛋白对激素阳性(HPBC)和激素阴性(HNBC)早期乳腺癌(EBC)临床结局的影响。

方法

使用荧光免疫组织化学(IHC)和自动定量分析(AQUA)对组织微阵列(TMA)进行分析,该TMA包含来自加拿大卡尔加里汤姆·贝克癌症中心诊断的两组患者(HPBC组:n = 130;HNBC组:n = 168)的福尔马林固定、石蜡包埋的切除肿瘤。如全细胞角蛋白表达所示,在整个肿瘤(tATM)中测量ATM表达水平;如DAPI和全细胞角蛋白阳性结果所示,在肿瘤核区室(nATM)中测量;如波形蛋白阳性和全细胞角蛋白阴性结果所示,在癌症相关基质(csATM)中测量。这些区室中的ATM表达水平与临床结局相关。

结果

与正常乳腺上皮组织相比,肿瘤中的tATM和nATM显著降低,而csATM显著高于相应的正常组织区室。此外,HNBC中tATM和nATM的中位表达水平比HPBC低两到三倍(P<0.001)。在HNBC和HPBC队列中,tATM、nATM和csATM低表达肿瘤的患者的生存结局明显比tATM、nATM和csATM高表达的患者差,但这种影响在HNBC中更为明显。多变量分析表明,这些生物标志物可独立于肿瘤大小和淋巴结状态预测生存,但仅在HNBC队列中(P<0.001)。

结论

恶性肿瘤和基质区室中低ATM蛋白表达可能导致乳腺癌的侵袭性,并且是与HNBC患者较差生存相关的独立预后因素。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7b26/4453198/6f95023724f9/13058_2015_575_Fig1_HTML.jpg

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