Basic research of pancreatic cancer cell-derived extracellular vesicles

Xu Jinxiang; Liu Shanglong; Sun Yuqi; Li Zequn; Liu Hengjian; Zhang Dan; Ren Yuanzhong; Zhou Yanbing

doi:10.3760/cma.j.issn.1001-9030.2020.01.003

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• 胰腺外科 •

胰腺癌细胞源性细胞外囊泡的基础研究

中华实验外科杂志, 2020,37(01) : 12-14. DOI: 10.3760/cma.j.issn.1001-9030.2020.01.003

摘要

目的

分离胰腺癌细胞(PANC-1)和人胰腺导管上皮细胞(HPDE6-C7)细胞培养上清液中的细胞外囊泡，分别比较微小RNA(miRNA，miR)-483-5p在两种细胞及其所分泌的细胞外囊泡中的差异性表达。

方法

超速离心法制备去除胎牛血清源性囊泡的完全培养基，细胞计数试剂盒(CCK-8)检测超速离心前(对照组)与超速离心后(实验组)的完全培养基对细胞增殖作用的差异；用去除血清囊泡的完全培养基培养细胞，超速离心方法提取细胞外囊泡，用二喹啉甲酸(BCA)蛋白浓度测定试剂盒和纳米颗粒跟踪分析(NTA)检测细胞外囊泡(EVs)的浓度；用透射电镜、NTA、蛋白质印迹法(Western blot)鉴定其是否符合细胞外囊泡特征。定量即时聚合酶链反应(qPCR)检测miR-483-5p在两组细胞及其分泌的细胞外囊泡中的表达。CCK-8增殖实验和qPCR实验的结果采用t检验分析。

结果

CCK-8增殖实验结果显示48 h和72 h后，HPDE6-C7的实验组与对照组之间差异无统计学意义(0.674±0.036比0.671±0.016，t＝0.315，P_{48 h}>0.05；0.890±0.027比0.925±0.099，t＝0.581，P_{72 h}>0.05)；PANC-1的实验组与对照组之间差异无统计学意义(0.759±0.004比0.761±0.016，t＝0.249，P_{48 h}>0.05；1.114±0.025比1.145±0.014，t＝1.898，P_{72 h}>0.05)；透射电镜：细胞外囊泡呈"茶杯托盘"状、NTA结果：98%PANC-1源性细胞外囊泡的直径为130.0 nm、98%HPDE6-C7源性细胞外囊泡的直径为129.7 nm；Western blot实验显示：细胞外囊泡表现为CD63、TSG101阳性，而GM130为阴性；蛋白浓度测定试剂盒和NTA分析测得PANC-1和HPDE6-C7源性的细胞外囊泡浓度分别为：1.5 g/L、1.510 11颗粒/毫升和1.3 g/L、1.610 11颗粒/毫升；与HPDE6-C7比较，PANC-1中miR-483-5p的表达显著增加(2.820±0.180比1.000±0.006，t＝－17.539，P<0.01)；与HPDE6-C7源性细胞外囊泡比较，PANC-1源性细胞外囊泡中miR-483-5p的表达显著增加(3.503±0.265比1.002±0.084，t＝－15.582，P<0.01)。

结论

超速离心法去除胎牛血清源性囊泡的完全培养基不影响细胞的正常增殖；鉴定结果显示所分离的沉淀符合细胞外囊泡的特征；根据NTA的结果可以判断其应归类于小细胞外囊泡；qPCR结果表明，miR-483-5p在PANC-1和其分泌的细胞外囊泡中均为高表达。

引用本文: 徐锦翔, 刘尚龙, 孙钰淇, 等. 胰腺癌细胞源性细胞外囊泡的基础研究 [J] . 中华实验外科杂志,2020,37 (01): 12-14. DOI: 10.3760/cma.j.issn.1001-9030.2020.01.003

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细胞外囊泡是机体几乎所有细胞均可分泌的脂质双层膜封闭的多种类型膜性囊泡的统称^[1]。本研究拟制备去除胎牛血清源性囊泡的完全培养基并检测其对细胞增殖的影响；提取和鉴定所提取的细胞外囊泡及其亚型；探索细胞外囊泡浓度的测定方法；比较miR-483-5p在胰腺癌细胞与胰腺导管上皮细胞及其分泌的细胞外囊泡中的差异性表达。

贡献者信息

徐锦翔

青岛大学　266071

刘尚龙

青岛大学附属医院胃肠外科　266005

孙钰淇

青岛大学　266071

李泽群

青岛大学附属医院胃肠外科　266005

刘恒健

青岛大学　266071

张丹

青岛大学　266071

任远中

青岛大学　266071

周岩冰

青岛大学附属医院胃肠外科　266005

通信作者

周岩冰

青岛大学附属医院胃肠外科　266005

Email：zhouyanbing999@aliyun.com

关键词

胰腺癌; 细胞外囊泡; 超速离心; 微小RNA-483-5p;

基金项目

国家自然科学基金（81572314、81802888）

山东省重点研究开发项目（2018GSF118088）

利益冲突

利益冲突　所有作者均声明不存在利益冲突

历史

出版日期：2020-01-08

收稿日期：2019-06-11

Pancreatic Surgery

Basic research of pancreatic cancer cell-derived extracellular vesicles

Xu Jinxiang, Liu Shanglong, Sun Yuqi, Li Zequn, Liu Hengjian, Zhang Dan, Ren Yuanzhong, Zhou Yanbing

Published 2020-01-08

Cite as Chin J Exp Surg, 2020,37(01): 12-14. DOI: 10.3760/cma.j.issn.1001-9030.2020.01.003

Abstract

Objective

To isolate extracellular vesicles (VEs) from the culture supernatant of pancreatic cancer (PANC-1) and human pancreatic ductal epithelial cells (HPDE6-C7), and to compare the differential expression of microRNA (miRNA, miR)-483-5p in the two kinds of cells and their secreted EVs.

Methods

Ultracentrifugation method was used to prepare the complete culture medium of depletion of serum-derived vesicles. Cell count Kit (CCK-8) was used to detect the effect of complete medium on cell proliferation without ultracentrifugation (control group) and with ultracentrifugation (experimental group). Cells were cultured in vesicle-depleted complete medium, and EVs were extracted by ultracentrifugation. The concentration of EVs was detected by BCA protein concentration determination kit and nanoparticles tracking analysis (NTA). Transmission electron microscope, NTA, and Western blotting were used to identify whether they, obtained by ultracentrifugation, were in accordance with the characteristics of EVs. The expression of miR-483-5p was detected by quantitative real time polymerase chain reaction (qPCR). The results of CCK-8 proliferation test and qPCR test were expressed by mean±standard deviation (SD). The statistical method was t test.

Results

The results of CCK-8 proliferation test showed that there was no significant difference between the experimental group and the control group after 48 h and 72 h in HPDE6-C7 cells (HPDE6-C7, 0.674±0.036 vs. 0.671±0.016, t=0.315, P_{48 h}>0.05; 0.890±0.027 vs. 0.925±0.099, t=0.581, P_{72 h}>0.05), as well as the PANC-1 (0.759±0.004 vs. 0.761±0.016, t=0.249, P_{48 h}>0.05; 1.114±0.025 vs. 1.145±0.014, t=1.898, P_{72 h}>0.05). The transmission electron microscopy showed that the EVs were "tea-cup tray" . The results of NTA showed that the diameter of 98% PANC-1 derived EVs was 130.0 nm, and that of 98% HPDE6-C7 derived EVs was 129.7 nm. Western blotting showed that CD63 and TSG101 were positive, but GM130 was negative. The concentration of EVs secreted by PANC-1 and HPDE6-C7 was measured by protein concentration assay kit and NTA as follows: 1.5 g/L, 1.510 11 particles/mland 1.3 g/L, 1.610 11 particles/ml, respectively. Compared with HPDE6-C7, the expression of miR-483-5p in PANC-1 was significantly increased (2.820±0.180 vs. 1.000±0.006, t=-17.539, P<0.01). Compared with HPDE6-C7 derived EVs, the expression of miR-483-5p in PANC-1 derived EVs was significantly increased (3.503±0.265 vs. 1.002±0.084, t=-15.582, P<0.01).

Conclusion

The ultracentrifugation method does not affect the normal proliferation of cells while removing fetal bovine serum-derived vesicles in the complete medium; the identification results show that the isolated pellets correspond to the characteristics of EVs. According to the results of NTA, it can be judged that they should be classified as small EVs. The results of qPCR show that miR-483-5p is highly expressed in PANC-1 and the secreted EVs.

Key words:

Pancreatic cancer; Extracellular vesicles; Ultracentrifugation; MicroRNA-483-5p

Contributor Information

Xu Jinxiang