|本期目录/Table of Contents|

[1]王茂鑫,陈贤明,龚宏勋,等.siRNA沉默环指蛋白8基因对裸鼠人鼻咽癌移植瘤放疗增敏作用的实验研究[J].医学研究与战创伤救治(原医学研究生学报),2021,23(03):244-248.[doi:10.3969/j.issn.1672-271X.2021.03.005]
 WANG Mao-xin,CHEN Xian-ming,GONG Hong-xun,et al.Silencing RNF8 by siRNA enhances the radiation sensitivity of NPC transplantation tumor in nude mice[J].JOURNAL OF MEDICALRESEARCH —COMBAT TRAUMA CARE,2021,23(03):244-248.[doi:10.3969/j.issn.1672-271X.2021.03.005]
点击复制

siRNA沉默环指蛋白8基因对裸鼠人鼻咽癌移植瘤放疗增敏作用的实验研究()
分享到62.8K

《医学研究与战创伤救治》(原医学研究生学报)[ISSN:1672-271X/CN:32-1713/R]

卷:
第23卷
期数:
2021年03期
页码:
244-248
栏目:
基础研究
出版日期:
2021-06-20

文章信息/Info

Title:
Silencing RNF8 by siRNA enhances the radiation sensitivity of NPC transplantation tumor in nude mice
作者:
王茂鑫陈贤明龚宏勋陈十燕杨帆陈函
作者单位:350025福州,联勤保障部队第九○○医院耳鼻咽喉头颈外科(王茂鑫、陈贤明、龚宏勋、陈十燕、杨帆、陈函)
Author(s):
WANG Mao-xin CHEN Xian-ming GONG Hong-xun CHEN Shi-yan YANG Fan CHEN Han
(Otolaryngology Department,the 900th Hospital of the Joint Logistics Support Force,PLA,Fuzhou 350025,Fujian, China)
关键词:
鼻咽癌环指蛋白8放射治疗小干扰RNA 动物试验
Keywords:
nasopharyngeal cancer RNF8 radiotherapy siRNAanimal experiment
分类号:
R739.63
DOI:
10.3969/j.issn.1672-271X.2021.03.005
文献标志码:
A
摘要:
目的探讨环指蛋白8(RNF8)的放疗抵抗作用及沉默RNF8后对鼻咽癌的放疗增敏作用及其机制。方法分别将鼻咽癌CNE-1细胞株及稳定转染的RNF8沉默的CNE-1细胞株注射入裸鼠背部皮下,建立裸鼠鼻咽癌移植瘤模型。将肿瘤长至直径8~10 mm的裸鼠30只按随机数字法分为RNF8未沉默组(RNF8+组)和RNF8沉默组(RNF8-组),每组按放疗照射剂量的不同又分5个亚组,每个亚组3只,分别给予0、4、8、12、16Gy照射,其中0 Gy为对照亚组。采用局部分割照射,每次2 Gy。照射完成10 d后杀鼠取瘤,称重观察抑瘤情况,计算抑瘤率;取2组8Gy剂量亚组肿瘤制成细胞悬液,应用流式细胞仪检测凋亡率,应用流式细胞仪检测2组8 Gy剂量亚组中RNF8和DNA依赖蛋白激酶催化亚单位(DNA-PKcs)、共济失调毛细血管扩张症突变基因(ATM)的表达。结果RNF8在RNF8-组中只有微量表达(0.11±0.03),而在RNF8+组中表达明显升高(1.18±0.23),差异有统计学意义(P<0.01)。RNF8+组和RNF8-组分别在16 Gy时抑瘤率最大。RNF8+组抑瘤率在各个剂量点均低于RNF8-组,其中8 Gy时差异最大(P<0.01)。因此选择RNF8+组8 Gy剂量亚组和RNF8-组8 Gy剂量亚组进行比较。RNF8+组8 Gy剂量亚组凋亡率明显低于RNF8-组8 Gy剂量亚组(P<0.05)。RNF8+组8 Gy剂量亚组中ATM表达(49.3±5.3)较RNF8-组8 Gy剂量亚组(23.4±2.6)明显升高(P<0.01),而DNA-PKcs在组间表达差异无统计学意义(P>0.05)。结论RNF8可以导致鼻咽癌细胞的放疗抵抗,其机制是通过激活以ATM为主的同源重组(HR)途径来修复损伤的肿瘤细胞DNA,沉默RNF8可以增加鼻咽癌的放疗敏感性。
Abstract:
ObjectiveTo explore the role of RNF8 in radioresistance ofnasopharyngeal cancer (NPC) and the irradiation enhancement effect and mechanism to NPC when RNF8 was silenced.MethodsCNE-1 cells and CNE-1 cells in which RNF8 was stably silenced by siRNA were injected to the back of nude mice subcutaneously, respectively. The model of NPC transplantation tumor in nude mice was established. Thirty nude mice with 8-10 mm transplanted tumor were divided to two groups: RNF8+ Group (RNF8 not silenced) and RNF8-Group (RNF8 silenced). Each group was divided to 4 sub-groups and 1 control group. Each sub-group had 3 mice. Tumor of mice in sub-groups received 4 Gy, 8 Gy, 12 Gy and 16 Gy irradiation, respectively. Mice in control groups were received 0 Gy. Local fractional irradiation was used for mice with 2 Gy each time. Mice were killed 10 days after irradiation, then tumors were taken out and weighed. Tumor inhibition rate was calculated. Tumors in 8 Gy sub-group of RNF8+ Group and 8 Gy sub-group of RNF8-Group were made to cell suspension. The apoptosis rate were detected by flow cytometry. The expression of RNF8, DNA-PKcs and ATM was detected in the cell suspension by flow cytometry.ResultsRNF8 was higher expressed in RNF8+ Group (1.18±0.23) than that in RNF8-Group (0.11±0.03, P<0.01). Tumor inhibition rate was the highest when they received 16 Gy radiation in both groups. Tumor inhibition rate in RNF8-Group at every dose point was higher than that in RNF8+ Group, the largest gap was at 8 Gy dose point (P<0.01). The detection index of 8 Gy sub-group of RNF8+ Group was compared to that of 8 Gy sub-group of RNF8-Group. The apoptosis rate in 8 Gy sub-group of RNF8-Group was higher than that in 8 Gy sub-group of RNF8+ Group (P<0.05). The expression of ATM in 8 Gy sub-group of RNF8+ Group (49.3±5.3) was significantly higher than that in 8 Gy sub-group of RNF8-Group [(23.4±2.6), P<0.01]. The expression of DNA-PKcs had no significant differences between both groups (P>0.05).ConclusionRNF8, which can activate homologous recombination (HR) way to repair impaired DNA of cancer cells, mediates the radioresistance ofNPC cells. Silencing RNF8 can enhance radiation sensitivity of NPC.

参考文献/References:

[1]周方正,陈洁,王小聪,等.鼻咽癌初治患者实施调强放疗的远期疗效及预后影响因素[J].中国临床研究,2018,31(1):81-84.
[2]邱元正,刘超,李果.鼻咽癌放射治疗的现状与对策[J].中国耳鼻咽喉颅底外科杂志,2015,21(6):435-438.
[3]张攀,张迪,戴晓波.复发鼻咽癌再程放射治疗的研究进展[J].实用肿瘤学杂志,2019, 33(1):92-96.
[4]Wang M, Chen X, Chen H, et al. RNF8 plays an important role in the radioresistance of human nasopharyngeal cancer cells in vitro[J]. Oncol Rep, 2015,34(1): 341-349.
[5]Du J, Yin N, Xie T. et al.Quantitative assessment of HR and NHEJ activities via CRISPR/Cas9-induced oligodeoxynucleotide-mediated DSB repair[J]. DNA Repair (Amst), 2018, 70(10):67-71.
[6]Santivasi W,Xia F. Ionizing radiation-induced DNA damage, response, and repair[J]. Antioxid Redox Signal, 2014, 21(2): 251-259.
[7]Jachimowicz RD, Goergens J, Reinhardt HC.DNA double-strand break repair pathway choice - from basic biology to clinical exploitation[J].Cell Cycle, 2019,18(13):1423-1434.
[8]Jin MH, Oh DY. ATM in DNA repair in cancer[J]. Pharmacol Ther,2019, 203(11):107391.
[9]Zhou T, Yi F, Wang Z,et al. The functions of DNA damage factor RNF8 in the pathogenesis and progression of cancer[J]. Int J Biol Sci,2019, 15(5):909-918.
[10]Tsai LJ, Lopezcolorado FW, Bhargava R,et al. RNF8 has both KU-dependent and independent roles in chromosomal break repair[J]. Nucleic Acids Res,2020, 48(11):6032-6052.
[11]Li F, Liu B, Zhou X,et al. Silencing of E3 Ubiquitin Ligase RNF8 Enhances Ionizing Radiation Sensitivity of Medulloblastoma Cells by Promoting the Deubiquitination of PCNA[J]. Oncol Res, 2018, 26(9):1365-1373.
[12]Zhou T, Yi F, Wang Z, et al. The Functions of DNA Damage Factor RNF8 in the Pathogenesis and Progression of Cancer[J].Int J Biol Sci, 2019,15(5):909-918.
[13]Tan Q, Niu K, Zhu Y, et al. RNF8 ubiquitinates RecQL4 and promotes its dissociation from DNA double strand breaks[J]. Oncogenesis,2021,10(3):24.
[14]Lu C, Truong L, Aslanian A, et al. The RING finger protein RNF8 ubiquitinates Nbs1 to promote DNA double-strand break repair by homologous recombination[J]. J Biol Chem,2012, 287(52): 43984-43994.
[15]Wu J, Chen Y, Lu L, et al. Chfr and RNF8 synergistically regulateATM activation[J]. Nat Struct Mol Biol, 2011, 18(7): 761-768.
[16]王茂鑫,陈贤明,张贤,等.环指蛋白8在鼻咽癌组织中的表达及其与预后的关系[J].东南国防医药,2019,21(2):147-151.

相似文献/References:

[1]范志刚,林焕新,柳仲秋,等.阿米福汀对鼻咽癌放射性口腔黏膜及涎腺损伤的保护作用[J].医学研究与战创伤救治(原医学研究生学报),2011,13(02):146.
 FAN Zhi-gang,LIN Huan-xin,LIU Zhong-qiu,et al.Protective effect of amifostine in irradiation mucositis of the oral cavity and dry mouth after nasapharyngeal carcinoma[J].JOURNAL OF MEDICALRESEARCH —COMBAT TRAUMA CARE,2011,13(03):146.
[2]艾书跃,吴建伟,吕毛古,等.双时相18F -氟代脱氧葡萄糖PET/CT 在鼻咽癌诊断中的应用价值[J].医学研究与战创伤救治(原医学研究生学报),2009,11(04):329.
 AI Shu-yue,WU Jian-wei,LV Mao-gu,et al.The applied value of Two-Phase 18F-fluorodeoxyglucose PET/CT in diagnosis of Nasopharyngeal Carcinoma[J].JOURNAL OF MEDICALRESEARCH —COMBAT TRAUMA CARE,2009,11(03):329.
[3]蒋静.鼻咽癌化疗患者恶心呕吐的护理[J].医学研究与战创伤救治(原医学研究生学报),2009,11(05):404.
[4]陈争明,范静平,林顺涨,等.枢丹治疗鼻咽癌化疗消化道反应疗效观察[J].医学研究与战创伤救治(原医学研究生学报),2008,10(03):206.
[5]陈贤明,黄少华,杨 帆,等.影响鼻咽癌预后的相关因素分析[J].医学研究与战创伤救治(原医学研究生学报),2014,16(06):584.[doi:10.3969/j.issn.1672-271X.2014.06.008]
 CHEN Xian-ming,HUANG Shao-hua,YANG Fan,et al.Analysis of factors related to the NPC patients prognosis[J].JOURNAL OF MEDICALRESEARCH —COMBAT TRAUMA CARE,2014,16(03):584.[doi:10.3969/j.issn.1672-271X.2014.06.008]
[6]洪君,张艳,张晓晔,等.不同测量方法对鼻咽癌容积调强弧形治疗验证通过率的影响[J].医学研究与战创伤救治(原医学研究生学报),2020,22(4):414.[doi:10.3969/j.issn.1672-271X.2020.04.018]
[7]华羽晨,唐媛媛,黄晓萍,等.耳穴贴压技术联合康复新液改良式喷雾给药在鼻咽癌放疗患者中的应用[J].医学研究与战创伤救治(原医学研究生学报),2022,24(5):537.[doi:10.3969/j.issn.1672-271X.2022.05.020]
[8]王茂鑫,陈贤明,张贤,等.环指蛋白8在鼻咽癌组织中的表达及其与预后的关系[J].医学研究与战创伤救治(原医学研究生学报),2019,21(02):147.[doi:10.3969/j.issn.1672-271X.2019.02.007]
 WANGMao-xin,CHENXian-ming,ZHANGXian,et al.Expression of RNF8 in nasopharyngeal carcinoma and its relationship with prognosis[J].JOURNAL OF MEDICALRESEARCH —COMBAT TRAUMA CARE,2019,21(03):147.[doi:10.3969/j.issn.1672-271X.2019.02.007]

备注/Memo

备注/Memo:
基金项目:福建省自然科学基金(2015J01485)
更新日期/Last Update: 2021-06-17