Jiang Zhengyu, Slater Carolyn M, Zhou Yan, Devarajan Karthik, Ruth Karen J, Li Yueran, Cai Kathy Q, Daly Mary, Chen Xiaowei
Cancer Epigenetics Program, Fox Chase Cancer Center, Philadelphia, PA, 19111, USA.
Present Address: Department of Medicine, Irving Cancer Research Center, Columbia University, New York, NY, 10032, USA.
Breast Cancer Res. 2017 May 30;19(1):62. doi: 10.1186/s13058-017-0853-2.
Recent genome-wide profiling by sequencing and distinctive chromatin signatures has identified thousands of long non-coding RNA (lncRNA) species (>200 nt). LncRNAs have emerged as important regulators of gene expression, involving in both developmental and pathological processes. While altered expression of lncRNAs has been observed in breast cancer development, their roles in breast cancer progression and metastasis are still poorly understood.
To identify novel breast cancer-associated lncRNA candidates, we employed a high-density SNP array-based approach to uncover intergenic lncRNA genes that are aberrantly expressed in breast cancer. We first evaluated the potential value as a breast cancer prognostic biomarker for one breast cancer-associated lncRNA, LincIN, using a breast cancer cohort retrieved from The Cancer Genome Atlas (TCGA) Data Portal. Then we characterized the role of LincIN in breast cancer progression and metastasis by in vitro invasion assay and a mouse tail vein injection metastasis model. To study the action of LincIN, we identified LincIN-interacting protein partner(s) by RNA pull-down experiments followed with protein identification by mass spectrometry.
High levels of LincIN expression are frequently observed in tumors compared to adjacent normal tissues, and are strongly associated with aggressive breast cancer. Importantly, analysis of TCGA data further suggest that high expression of LincIN is associated with poor overall survival in patients with breast cancer (P = 0.044 and P = 0.011 after adjustment for age). The functional experiments demonstrate that knockdown of LincIN inhibits tumor cell migration and invasion in vitro, which is supported by the results of transcriptome analysis in the LincIN-knockdown cells. Furthermore, knockdown of LincIN diminishes lung metastasis in a mouse tail vein injection model. We also identified a LincIN-binding protein, NF90, through which overexpression of LincIN may repress p21 protein expression by inhibiting its translation, and upregulation of p21 by LincIN knockdown may be associated with less aggressive metastasis phenotypes.
Our studies provide clear evidence to support LincIN as a new regulator of tumor progression-metastasis at both transcriptional and translational levels and as a promising prognostic biomarker for breast cancer.
近期通过测序和独特的染色质特征进行的全基因组分析已鉴定出数千种长链非编码RNA(lncRNA)(>200 nt)。lncRNAs已成为基因表达的重要调节因子,参与发育和病理过程。虽然在乳腺癌发生过程中已观察到lncRNAs表达改变,但其在乳腺癌进展和转移中的作用仍知之甚少。
为了鉴定新的乳腺癌相关lncRNA候选物,我们采用基于高密度SNP阵列的方法来发现乳腺癌中异常表达的基因间lncRNA基因。我们首先使用从癌症基因组图谱(TCGA)数据门户检索的乳腺癌队列评估一种乳腺癌相关lncRNA,即LincIN作为乳腺癌预后生物标志物的潜在价值。然后我们通过体外侵袭试验和小鼠尾静脉注射转移模型来表征LincIN在乳腺癌进展和转移中的作用。为了研究LincIN的作用,我们通过RNA下拉实验鉴定LincIN相互作用蛋白伴侣,随后通过质谱鉴定蛋白质。
与相邻正常组织相比,肿瘤中经常观察到高水平的LincIN表达,并且与侵袭性乳腺癌密切相关。重要的是,对TCGA数据的分析进一步表明,LincIN的高表达与乳腺癌患者的总体生存率低相关(调整年龄后P = 0.044和P = 0.011)。功能实验表明,敲低LincIN可抑制体外肿瘤细胞迁移和侵袭,这得到了LincIN敲低细胞中转录组分析结果的支持。此外,在小鼠尾静脉注射模型中,敲低LincIN可减少肺转移。我们还鉴定了一种LincIN结合蛋白NF90,通过它LincIN的过表达可能通过抑制其翻译来抑制p21蛋白表达,而LincIN敲低导致的p21上调可能与侵袭性较小的转移表型相关。
我们的研究提供了明确的证据,支持LincIN在转录和翻译水平上作为肿瘤进展转移的新调节因子以及作为有前景的乳腺癌预后生物标志物。
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