Regulatory role of long-chain non-coding RNA HIF1A-AS1 on hypoxia-induced the autophagy of pancreatic cancer PANC1 cells

Xu Feng; Xu Yuemei; Xia Feizhen; Jiang Yuhua; Zhang Bo; Li Xianpeng

doi:10.3760/cma.j.issn.1674-1935.2017.03.008

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长链非编码RNA HIF1A-AS1对缺氧诱导的胰腺癌PANC1细胞自噬的调节作用

中华胰腺病杂志, 2017,17(03) : 180-183. DOI: 10.3760/cma.j.issn.1674-1935.2017.03.008

摘要

目的

观察长链非编码RNA HIF1A-AS1对缺氧诱导的胰腺癌PANC1细胞自噬的调节作用。

方法

应用三气培养箱及缺氧混合气体(94%N₂、5% CO₂、1% O₂)缺氧培养胰腺癌PANC1细胞3、6、12、24、36、48 h，实时荧光定量PCR法检测HIF1A-AS1的表达。通过携带HIF1A-AS1过表达的重组腺病毒感染PANC1细胞和通过脂质体将靶向HIF1A-AS1的siRNA转染PANC1细胞分别获得过表达、低表达HIF1A-AS1的PANC1细胞株，以常规培养的PANC1细胞作为对照。对照组、过表达组、低表达组细胞分别缺氧培养24 h，采用实时荧光定量PCR法检测各组PANC1细胞HIF1A-AS1的表达，流式细胞术检测细胞凋亡率，蛋白质印迹法检测自噬相关蛋白Beclin 1的表达。

结果

缺氧培养的PANC1细胞HIF1A-AS1的表达随缺氧时间的延长而增加，36 h时达峰值，从6 h开始均显著高于对照组，差异均有统计学意义(P值均<0.01)。以对照组表达量为1，过表达组、低表达组细胞HIF1A-AS1的表达量分别为4.49±0.53、0.49±0.07，过表达组高于对照组，低表达组低于对照组，差异均有统计学意义(P值均<0.01)。对照组、过表达组、低表达组PANC1细胞经缺氧培养24 h后的细胞凋亡率分别为(8.27±1.28)%、(6.56±1.49)%、(19.9±2.34)%，过表达组低于对照组，低表达组高于对照组，差异均有统计学意义(P值均<0.01)；Beclin 1表达量分别为1.05±0.11、1.29±0.19、0.38±0.18，过表达组高于对照组，低表达组低于对照组，差异均有统计学意义(P值均<0.01)。

结论

HIF1A-AS1可能通过促进缺氧诱导胰腺癌PANC1细胞的自噬，参与胰腺癌的发病过程。

引用本文: 许丰, 徐月梅, 夏菲珍, 等. 长链非编码RNA HIF1A-AS1对缺氧诱导的胰腺癌PANC1细胞自噬的调节作用 [J] . 中华胰腺病杂志,2017,17 (03): 180-183. DOI: 10.3760/cma.j.issn.1674-1935.2017.03.008

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未经授权，不得转载、摘编本刊文章，不得使用本刊的版式设计。

除非特别声明，本刊刊出的所有文章不代表中华医学会和本刊编委会的观点。

缺氧微环境作为胰腺癌等实体肿瘤的重要特征之一，可诱导肿瘤细胞中多种耐药基因的表达，导致化疗耐药^[1]。自噬是真核细胞通过清除损伤细胞器或变性蛋白质维持细胞稳态的降解机制，在肿瘤形成、转移及化疗耐药中起重要作用，但其调控机制尚未阐明^[2,3]。长链非编码RNA(long non-coding RNA, lncRNA)是最新发现的一类在表观遗传、转录水平、翻译水平都具有调节作用的非编码RNA分子^[4,5]，可通过调节肿瘤细胞的自噬水平参与肿瘤的发生、发展和转移进程^[6,7]。存在于缺氧诱导因子1α(hypoxia-inducible factor-1α，HIF-1α)反义链上的lncRNA HIF1A-AS1参与肝癌、非小细胞肺癌等肿瘤的发生和发展^[8,9]。本研究在缺氧环境中培养胰腺癌PANC1细胞，观察细胞HIF1A-AS1表达对细胞自噬活性的影响，探讨其可能的调控机制。

贡献者信息

许丰

315040　宁波，宁波大学医学院附属鄞州医院消化科

徐月梅

315040　宁波，宁波大学医学院附属鄞州医院消化科

夏菲珍

315040　宁波，宁波大学医学院附属鄞州医院消化科

姜玉华

315040　宁波，宁波大学医学院附属鄞州医院消化科

张波

315040　宁波，宁波大学医学院附属鄞州医院消化科

李先鹏

315040　宁波，宁波大学医学院附属鄞州医院消化科

通信作者

李先鹏

315040　宁波，宁波大学医学院附属鄞州医院消化科

Email：849840290@qq.com

关键词

胰腺; 细胞系，肿瘤; 长链非编码RNA; HIF1A-AS1; 自噬; 缺氧;

基金项目

浙江省自然科学基金（LY16H160004）

历史

出版日期：2017-06-20

收稿日期：2017-01-04

本文编辑

冀凯宏

Original Article

Regulatory role of long-chain non-coding RNA HIF1A-AS1 on hypoxia-induced the autophagy of pancreatic cancer PANC1 cells

Xu Feng, Xu Yuemei, Xia Feizhen, Jiang Yuhua, Zhang Bo, Li Xianpeng

Published 2017-06-20

Cite as Chin J Pancreatol, 2017,17(03): 180-183. DOI: 10.3760/cma.j.issn.1674-1935.2017.03.008

Abstract

Objective

To observe the regulatory role of long non-coding RNA HIF1A-AS1 on the autophagy of pancreatic cancer PANC1 cells induced by hypoxia.

Methods

The pancreatic cancer PANC1 cells were cultured in a three-gas incubator filled with hypoxic gas mixture (94% N₂, 5% CO₂, 1% O₂) for 3, 6, 12, 24, 36 and 48 h. HIF1A-AS1 overexpression and low expression PANC1 cells were obtained by the infection of recombinant adenovirus carrying HIF1A-AS1 and the transfection of HIF1A-AS1 targeting siRNA by liposome, and routinely cultured PANC1 cells served as control. The expression of HIF1A-AS1 of PANC1 cells was detected by real-time quantitative PCR after being cultured in hypoxia-induced condition for 24 h. The apoptosis rate was detected by flow cytometry. The autophagy related proteins Beclin 1 were detected by western blot.

Results

The expression of HIF1A-AS1 in hypoxic cells was increased as the hypoxic time increased since 6 h and peaked at 36 h, which was significantly higher than that in control group (P<0.01). HIF1A-AS1 relative expression in HIF1A-AS1 overexpression and low expression PANC1 cells was 4.49±0.53 and 0.49±0.07, which were normalized to that of control group with the relative expression of 1. Control group had lower HIF1A-AS1 expression than HIF1A-AS1 overexpression PANC1 cells but higher HIF1A-AS1 in HIF1A-AS1 low expression PANC1 cells, and the differences were statistically significant (P<0.01). The cell apoptosis rate of control, HIF1A-AS1 overexpression and low expression PANC1 cells was (8.27±1.28)%, (6.56±1.49)% and (19.9±2.34)% after 24 h hypoxic culture. Control group had higher HIF1A-AS1 expression than HIF1A-AS1 overexpression PANC1 cells but lower HIF1A-AS1 in HIF1A-AS1 low expression PANC1 cells, and the differences were statistically significant (P<0.01). The expression of Beclin 1 protein was protein 1.05±0.11, 1.29±0.19 and 0.38±0.18, respectively. Control group had lower Beclin 1 expression than HIF1A-AS1 overexpression PANC1 cells but higher Beclin 1 in HIF1A-AS1 low expression PANC1 cells, and the differences were statistically significant (P<0.01).

Conclusions

HIF1A-AS1 can promote autophagy of pancreatic cancer PANC1 cells induced by hypoxia and participate in the pathogenesis and metastasis of pancreatic cancer.

Key words:

Pancreas; Cell line, tumor; Long non-coding RNA; HIF1A-AS1; Autophagy; Anoxia

Contributor Information

Xu Feng

Department of Gastroenterology, Yinzhou Hospital, Medical School, Ningbo University, Ningbo 315040, China

Xu Yuemei

Xia Feizhen

Jiang Yuhua

Zhang Bo

Li Xianpeng

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