胃泌素对胃癌细胞SGC7901 Reg I 基因转录因子的效应

doi:10.3969/j.issn.0529-1356.2013.02.014

解剖学报 ›› 2013, Vol. 44 ›› Issue (2 ): 219-223.doi: 10.3969/j.issn.0529-1356.2013.02.014

胃泌素对胃癌细胞SGC7901 Reg I 基因转录因子的效应

吴艳芳^1,2 郭林霞¹ 乐晓萍¹ 丁一^1*

1. 郑州大学基础医学院组织学胚胎学教研室，郑州 450001; 2. 新乡医学院基础医学院人体解剖学实验室，河南新乡 453003

收稿日期:2012-05-18 修回日期:2012-07-05 出版日期:2013-04-06 发布日期:2013-04-06
通讯作者: 丁一 E-mail:dingyi@zzu.edu.cn
基金资助:
河南省医学科技攻关计划项目

Effects of gastrin on Reg I gene transcription factors in SGC7901 cell

WU Yan-fang ^1,2 GUO Lin-xia¹ LE Xiao-ping¹ DING Yi ^1* 

1. Department of Histology and Embryology, College of Basic Medicine, Zhengzhou University, Zhengzhou 450001, China;2. Laboratory of Human Anatomy, College of Basic Medicine, Xinxiang Medical College, He’nan Xinxiang 453003, China

Received:2012-05-18 Revised:2012-07-05 Online:2013-04-06 Published:2013-04-06

摘要/Abstract

摘要：

目的探讨胃泌素对胃癌细胞SGC7901 Reg I（Reg I）基因转录因子的效应。方法应用巢式PCR技术从胃癌细胞SGC7901基因组DNA扩增Reg I基因启动子1414bp片段，将该片段插入pMD19-T载体，序列分析鉴定。应用随机引物法以地高辛分别标记1414bp及其Hind Ⅲ酶切800bp 和614bp片段，经灵敏度检测后，作为探针。应用Genomatix MatInspector在线分析软件分析Reg I基因启动子1414bp片段的转录因子结合位点。分别以10^-7 mol/L和10^-8 mol/L胃泌素G-17处理胃癌细胞SGC7901 48h，提取核蛋白。应用DNA-蛋白质印迹法（Southern blotting），分别以地高辛标记的1414bp、800bp 和614bp片段为探针检测胃泌素对胃癌细胞SGC7901 Reg I基因转录因子的效应。结果 1414bp 探针可检测到20条蛋白主带。胃泌素孵育后，带型没有变化，但是一些条带的灰度值改变，带9、12、13、14、15和16的灰度值明显降低( P＜0.05)；不同浓度胃泌素处理组之间上述6个条带的灰度值差异不明显( P >0.05)。614bp探针可检测到灰度值变化的6条主带中的带9、12和13，胃泌素处理后，此3条主带的灰度值明显降低( P＜0.05)。800bp探针可检测到灰度值变化的6条主带中的带9、12和14，胃泌素处理后，仅带14的灰度值明显降低( P＜0.05)。614bp和800bp探针均未检出带15和带16。结论胃癌细胞SGC7901 Reg I基因表达由多个转录因子协同调控。降低几个转录因子的结合活性可能是胃泌素上调胃癌细胞SGC7901 Reg I基因表达的途径之一。

关键词: Reg I基因 , 胃泌素 , 转录因子 , 胃癌细胞 , DNA-蛋白质印迹法

Abstract:

Objective To study the effects of gastrin on regenerating gene I(Reg I) gene transcription factors (TFs) in gastric cancer cell SGC7901. Methods Reg I gene promoter 1414bp fragment was amplified from gastric cancer cell SGC7901 genomic DNA by nest-PCR. The fragment was inserted into PMD19-T vector and identified by sequencing. The 1414bp fragment and its HindⅢ digestion 800bp and 614bp fragments were digoxin-labeled by random primer assay. After sensitivity detection, the three fragments were used as probes. Transcription factor binding sites (TFBS) in Reg I gene promoter 1414bp fragment were analyzed by online software Genomatix MatInspector. Gastric cancer cell SGC7901 was incubated with gastrin-G17 for 48 hours at final concentrations of 10^-7 mol/L and 10 ^-8 mol/L, and the nuclear proteins were extracted, respectively. Effects of gastrin on Reg I gene TFs were detected by Southwestern blotting using digoxinlabeled 1414bp, 800bp and 614bp as probes, respectively. Results Twenty major bands of proteins with different molecular weight were detected with 1414bp probe. After treatment with gastrin, the pattern of bands showed no change. However, the densities of some bands were changed, the densities of band 9, 12, 13, 14, 15 and 16 decreased significantly ( P＜0.05). The densities of 6 bands above mentioned between those in the two groups treated with gastrin at different final concentration had no significant difference ( P >0.05). Of the 6 changed bands detected with 1414bp probe, three bands including band 9, 12 and 13 were detected with proximal 614bp probe. The densities of the three bands also decreased after gastrin incubation ( P＜0.05). Three bands including band 9, 12 and 14 detected with distal 800bp probe. However, only the densities of band 14 decreased after gastrin incubation ( P＜0.05). Band 15 and band 16 were not detected with proximal 614bp or distal 800bp probe. Conclusion The results suggest that Reg I gene may be transcriptionally regulated by cooperation of many TFs in gastric cancer cell SGC7901. Decreasing binding activities of some TFs may be one of pathways of gastrin up-regulating Reg I gene expression in gastric cancer cell SGC7901.

Key words: Reg I gene , Gastrin , Transcription factor , Gastric cancer cell , Southwestern blotting

吴艳芳郭林霞乐晓萍丁一*. 胃泌素对胃癌细胞SGC7901 Reg I 基因转录因子的效应[J]. 解剖学报, 2013, 44(2 ): 219-223.

WU Yan-fang GUO Lin-xia LE Xiao-ping DING Yi* . Effects of gastrin on Reg I gene transcription factors in SGC7901 cell[J]. AAS, 2013, 44(2 ): 219-223.

参考文献

［1］ Ding Y, Li JK, Xing WY, et al. Inhibition effects of various gastrin-shRNAs on gastrin expression in gastric cancer cell line BGC-823［J］. Acta Anatomica Sinica, 2007, 38(2): 182-186.（in Chinese）

丁一，李军扩，邢文英，等.shRNA对胃癌细胞系BGC823胃泌素表达的抑制效应［J］.解剖学报，2007，38（2）：182- 186. 

［2］Kinoshita Y, Ishihara S, Kadowaki Y, et al. Reg protein is a unique growth factor of gastric mucosal cells［J］. J Gastroenterol, 2004, 39(6): 507-513.

［3］Dhar DK, Udagawa J, Ishihara S, et al. Expression of regenerating gene I in gastric adenocarcinomas: correlation with tumor differentiation status and patient survival ［J］. Cancer, 2004, 100(6): 1130-1136.

［4］Sekikawa A, Fukui H, Fujii S, et al. REG I alpha protein may function as a trophic and/or antiapoptotic factor in the development of gastric cancer ［J］. Gastroenterology, 2005, 128(3): 642-653.

［5］Fukui H, Kinoshita Y, Maekawa T, et al. Regenerating gene protein may mediate gastric mucosal proliferation induced by hypergastrinemia in rats ［J］. Gastroenterology, 1998, 115(6): 1483-1493.

［6］Ashcroft FJ, Varro A, Dimaline R, et al. Control of expression of the lectin-like protein Reg-1 by gastrin: role of the Rho family GTPase RhoA and a C-rich promoter element ［J］. Biochem J, 2004, 381(Pt 2): 397-403.

［7］Steele IA, Dimaline R, Pritchard DM, et al. Helicobacter and gastrin stimulate Reg1 expression in gastric epithelial cells through distinct promoter elements ［J］. Am J Physiol Gastrointest Liver Physiol, 2007, 293(1): G347-354.

［8］Narlikar L, Ovcharenko I. Identifying regulatory elements in eukaryotic genomes ［J］. Brief Funct Genomic Proteomic, 2009, 8(4): 215-230.

［9］Quandt K, Frech K, Karas H, et al. MatInd and MatInspector: new fast and versatile tools for detection of consensus matches in nucleotide sequence data ［J］. Nucleic Acids Res, 1995, 23(23): 4878-4884.

［10］Gigoux V, Clerc P, Sanchez D, et al. Reg genes are CCK2 receptor targets in ElasCCK2 mice pancreas ［J］. Regul Pept, 2008, 146(1): 88-98.

［11］Judd LM, Bredin K, Kalantzis A, et al. STAT3 activation regulates growth, inflammation, and vascularization in a mouse model of gastric tumorigenesis ［J］. Gastroenterology, 2006, 131(4): 1073-1085. 

［12］Higham AD, Bishop LA, Dimaline R, et al. Mutations of Reg I alpha are associated with enterochromaffin-like cell tumor development in patients with hypergastrinemia ［J］. Gastroenterology, 1999, 116(6): 1310-1318.

［13］ Cheng Sh, Ding Y, Zhang QX. Role of Reg I in the pathway of gastrin stimulating proliferation of gastric cancer cells in vitro［J］.Acta Anatomica Sinica, 2012, 43(1):63-67.(in Chinese)

程珊，丁一，张钦宪. Reg I在胃泌素促胃癌细胞体外增殖通路中的作用［J］. 解剖学报，2012，43(1)： 63-67.

[1]	王子慧郭建林臧夏炎薛奇杰林凯琳张春博韩璐林俊堂徐存拴 . 大鼠肝再生的肝细胞干性变化中性别决定区转录因子2 mRNA和其他非编码RNA的表达变化与作用[J]. 解剖学报, 2023, 54(2): 202-207.
[2]	卢芬杨晴邵文君孙振坤王恩漫张伟娜. 微小RNA-98-5p靶向Kruppel样转录因子9对大鼠心肌缺血再灌注损伤的保护作用[J]. 解剖学报, 2022, 53(3): 347-353.
[3]	赵媛陶月佳余广福郭嘉欣李梦琪徐远义黄允宁. 丝裂原活化蛋白激酶激酶1在胃癌中的表达及其临床意义[J]. 解剖学报, 2022, 53(3): 309-316.
[4]	林宝勇徐进超应涵韬蒋欣刘焕彩王箐王巧真陈燕春. DEAD-box RNA解旋酶5和转录因子12与肌萎缩侧索硬化症的关系[J]. 解剖学报, 2021, 52(5): 698-705.
[5]	许晨胡雪峰. 上腭发生的分子调控机制[J]. 解剖学报, 2021, 52(2): 317-322.
[6]	邹琳清衣昕何辉单柏权金国华李浩明 . 海马去神经支配损伤后放射状胶质细胞表达RUNX1T1的变化及向神经元分化的影响[J]. 解剖学报, 2020, 51(6): 809-814.
[7]	丁小明许嵘张文州谢志新. 膀胱尿路上皮癌中候选生物标志物转录因子21的甲基化机制及意义[J]. 解剖学报, 2019, 50(5): 608-612.
[8]	邓学军龚邵新杨胜辉黄丽荣周芳. MicroRNA-539靶向调控E2F转录因子3抑制肝癌的发生与发展[J]. 解剖学报, 2018, 49(4): 469-474.
[9]	杨艳萍栗前李杰曹锡梅李海荣景雅乔从进张涛. 转录因子Tbx3在小鼠胚胎第二生心区的表达规律[J]. 解剖学报, 2018, 49(1): 87-92.
[10]	刘超任丽莉王一曌刘乙蒙肖建英. 支架蛋白活化蛋白激酶C受体1在胃癌细胞中的表达及其与胃癌细胞增殖的关系[J]. 解剖学报, 2017, 48(5): 545-549.
[11]	张泳张居适陈健尔刘学红*. 少突胶质细胞转录因子和神经钙黏附蛋白在人胚胎脊髓发育阶段的表达[J]. 解剖学报, 2015, 46(5): 655-659.
[12]	牛世伟武俊紫李晓波王文林李燕* 李树德*. 利拉鲁肽调控高脂诱导的非酒精性脂肪肝病的分子机制[J]. 解剖学报, 2014, 45(6): 800-808.
[13]	徐丽金清东宫喜刘卉周瑞祥*. MT2受体介导褪黑素对小鼠胃癌细胞的抑制作用[J]. 解剖学报, 2014, 45(3): 344-349.
[14]	牛苗苗战军* 张宏权. HOX基因在肿瘤发生发展中的作用[J]. 解剖学报, 2014, 45(3): 430-436.
[15]	代稳丁一张钦宪*. ZAC基因在奥曲肽抑制胃癌细胞体外增殖通路的作用[J]. 解剖学报, 2013, 44(4 ): 492-497.

胃泌素对胃癌细胞SGC7901 Reg I 基因转录因子的效应

Effects of gastrin on Reg I gene transcription factors in SGC7901 cell

可视化

摘要/Abstract

引用本文

使用本文

参考文献

相关文章 15

编辑推荐

Metrics

本文评价