[En1 promotes cell proliferation and migration via Hedgehog signaling pathway in esophageal squamous cell carcinoma].

Q3 Medicine
N Zhao, T Y Gong, Z C Wei, J Cong, Z H Liu, H Y Chen
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引用次数: 0

Abstract

Objective: To explore the function and mechanism of transcription factor En1 in esophageal squamous cell carcinoma (ESCC). Methods: The correlations of En1 with prognosis were analyzed using the overall survival data of 9 397 pan-cancer patients and progression-free survival data of 4 349 pan-cancer patients from The Cancer Genome Atlas (TCGA) database. The En1 expression data in 53 and 155 cases of ESCC and their paired adjacent tissues were from Gene Expression Omnibus (GEO) database and National Genomics Data Center-Genome Sequence Archive(NGDC-GSA)database. Lentivirus was used to generate En1 stable knockout cell lines KYSE180 and KYSE450. The proliferation ability of the cells was detected by cell counting kit 8 and clone formation assay. The migration ability of the cells was detected by Transwell assay. The effect of En1 on the proliferation of ESCC was detected by xenograft experiment in BALB/c-nu/nu mice. Real-time fluorescence quantitative polymerase chain reaction (RT-qPCR) was used to detect the expressions of En1, glioma-associated oncogene family zinc finger 1 (GLI1), glioma-associated oncogene family zinc finger 2 (GLI2) and smoothened (SMO). Results: Pan-cancer data from TCGA showed that patients with low En1 expression had longer overall survival and progression-free survival than patients with high En1 expression (P< 0.001). Data from GEO and GSA databases also showed a high expression level of En1 in ESCC tissues compared with paired tissues (P<0.001). Proliferation was inhibited after knockout of En1 in KYSE180 and KYSE450 cells (P<0.001). The colony formation numbers decreased. The colony formation numbers of KYSE180 cells in the shEn1#1 group and the shEn1#2 group were 138.33±23.07 and 127.00±19.70, respectively, significantly lower than that of the shNC group 340.67±12.06 (P<0.001). The colony formation numbers of KYSE450 cells in the shEn1#1 group and the shEn1#2 group were 65.33±2.52 and 9.00±3.00, respectively, significantly lower than that of the shNC group 139.00±13.00 (P<0.001). The migration numbers was inhibited after knockout of En1 [the Transwell numbers of KYSE180 cells in the shEn1#1 group and the shEn1#2 group were 66.67±12.66 and 71.33±11.02, respectively, significantly lower than that of the shNC group 334.67±16.56 (P<0.001). The Transwell numbers of KYSE450 cells in the shEn1#1 group and the shEn1#2 group were 112.33±14.57 and 54.33±5.51, respectively, significantly lower than that of the shNC group 253.33±21.03 (P<0.001)]. Xenograft model showed a slower growth rate of shEn1#1 and shEn1#2 cell lines (P<0.001). The tumor weights of KYSE450 cells in the shEn1#1 group and the shEn1#2 group were (0.046±0.026)g and (0.047±0.025)g, respectively, significantly lower than that of the shNC group (0.130±0.038)g (P<0.001). After knockdown of En1, the relative expression levels of GLI1 in KYSE180 cells of the shEn1#1 group and the shEn1#2 group were 0.326±0.162 and 0.322±0.133, and the relative expression levels of GLI1 in KYSE450 cells of the shEn1#1 and shEn1#2 groups were 0.131±0.006 and 0.352±0.050, respectively, which were all lower than that in the shNC group (P<0.01). After knockdown of En1, overexpression of GLI1 attenuated the inhibitory effect of knockdown of En1 on cell proliferation (P<0.001), colony formation[the colony formation numbers of the shEn1#1-GLI1 group were 151.00±9.54, higher than 102.33±10.02 (P=0.004) of the shEn1#1-vector group] and migration [the migration numbers of the shEn1#1-GLI1 group were 193.67±10.07, higher than 109.33±11.50 (P<0.001) in the shEn1#1-vector group]. In clinical samples of ESCC, major regulatory factors of the Hedgehog pathway were up-regulated and the pathway was activated. Conclusion: En1 promotes the proliferation and migration of ESCC cells by regulating the Hedgehog pathway and can be used as a new potential target for targeted therapy of ESCC.

[En1通过刺猬信号通路促进食管鳞状细胞癌细胞的增殖和迁移]
目的探讨转录因子 En1 在食管鳞状细胞癌(ESCC)中的功能和机制。方法利用癌症基因组图谱(TCGA)数据库中9 397例泛癌患者的总生存数据和4 349例泛癌患者的无进展生存数据,分析En1与预后的相关性。53例和155例ESCC及其配对邻近组织的En1表达数据来自基因表达总库(GEO)数据库和美国国家基因组学数据中心-基因组序列档案(NGDC-GSA)数据库。使用慢病毒生成 En1 稳定敲除细胞株 KYSE180 和 KYSE450。用细胞计数试剂盒 8 和克隆形成试验检测细胞的增殖能力。细胞迁移能力由 Transwell 试验检测。在 BALB/c-nu/nu 小鼠中进行异种移植实验,检测 En1 对 ESCC 增殖的影响。采用实时荧光定量聚合酶链反应(RT-qPCR)检测En1、胶质瘤相关癌基因家族锌指1(GLI1)、胶质瘤相关癌基因家族锌指2(GLI2)和smoothened(SMO)的表达。结果来自TCGA的泛癌症数据显示,En1低表达患者的总生存期和无进展生存期均长于En1高表达患者(P< 0.001)。GEO和GSA数据库的数据也显示,与配对组织相比,En1在ESCC组织中的表达水平较高(P<0.001)。敲除 En1 后,KYSE180 和 KYSE450 细胞的增殖受到抑制(P<0.001)。集落形成数减少。shEn1#1 组和 shEn1#2 组 KYSE180 细胞的集落形成数分别为 138.33±23.07 和 127.00±19.70,显著低于 shNC 组的 340.67±12.06(PPPPP<0.001)。shEn1#1 组和 shEn1#2 组 KYSE450 细胞的肿瘤重量分别为(0.046±0.026)g 和(0.047±0.025)g,明显低于 shNC 组(0.130±0.038)g(P<0.001)。敲除 En1 后,shEn1#1 组和 shEn1#2 组 KYSE180 细胞中 GLI1 的相对表达水平分别为 0.326±0.162 和 0.322±0.133,而 shEn1#1 组和 shEn1#2 组 KYSE450 细胞中 GLI1 的相对表达水平分别为 0.131±0.006 和 0.352±0.050,均低于 shNC 组(P<0.01)。敲除 En1 后,过表达 GLI1 可减轻敲除 En1 对细胞增殖的抑制作用(P<0.001),菌落形成[shEn1#1-GLI1 组菌落形成数为 151.00±9.54,高于 shEn1#1-vector 组的 102.33±10.02(P=0.004)]和迁移[shEn1#1-GLI1 组的迁移数为 193.67±10.07,高于 shEn1#1-vector 组的 109.33±11.50(P0.001)]。在 ESCC 临床样本中,刺猬通路的主要调节因子被上调,通路被激活。结论En1通过调节刺猬蛋白通路促进ESCC细胞的增殖和迁移,可作为靶向治疗ESCC的潜在新靶点。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
中华肿瘤杂志
中华肿瘤杂志 Medicine-Medicine (all)
CiteScore
1.40
自引率
0.00%
发文量
10433
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