1.A Compound Mutation (c.953C < G and c.49G < A) Aggravates Functional Impairments of C1-INH in Hep G2 Cells.
Allergy, Asthma & Immunology Research 2018;10(3):285-286
No abstract available.
Hep G2 Cells*
2.The effect of retinoic acid on cell kinetics in bromodeoxyuridine labelled hep G2 cell line.
Dae Ghon KIM ; Joong Ki AHN ; Dong Suck JANG ; Yee Yup KIM ; Se Ra LEE ; Soo Taek LEE ; Deuk Soo AHN
Korean Journal of Medicine 1993;45(5):561-571
No abstract available.
Bromodeoxyuridine*
;
Hep G2 Cells*
;
Kinetics*
;
Tretinoin*
3.Xylaroisopimaranin A, a New Isopimarane Derivative from an Endophytic Fungus Xylaralyce sp.
Shang Song BAO ; Hui Hui LIU ; Xue Qing ZHANG ; Cheng Xiong LIU ; Xiao Cong LI ; Zhi Yong GUO
Natural Product Sciences 2019;25(3):228-232
Five secondary metabolites, including a new isopimarane derivative xylaroisopimaranin A (1), were isolated from the endophytic fungus Xylaralyce sp. (HM-1), and their structures were elucidated by 1D, 2D NMR, MS and CD spectra. Their bioactivities were performed to antibacterial, Hep G2 cells cytotoxicity and brine shrimp inhibition. The biological evaluation results showed that the xylaroisopimaranin A (1), xylabisboein B (2), griseofulvin (3) , 5-methylmellein (4) and mellein-5-carboxlic acid (5) displayed no significant Hep G2 cells cytotoxicity and antibacterial acitivity, but they inhibited the brine shrimp with IC₅₀ from 0.5 to 25 µmol/mL.
Artemia
;
Fungi
;
Griseofulvin
;
Hep G2 Cells
4.A Study on the Labeling Efficiency and Cytotoxicity of Hepatocyte-targeting Galactosylated Chitosan Compounds.
Dae Weung KIM ; Hwan Jeong JEONG ; Eun Mi KIM ; Se Lim KIM ; Yun Hee KANG ; Min Woo KIM ; Chang Guhn KIM ; Myung Hee SOHN
Korean Journal of Nuclear Medicine 2005;39(5):278-283
PURPOSE: In prior study, we synthesized 99mTc-galactosylated chitosan (GC) and performed in vivo biodistribution study, showed specific targeting to hepatocyte. The aim of this study is to evaluate the labeling efficiency and cytotoxicity of modified galactosylated chitosan compounds, galactosyl methylated chitosan (GMC) and HYNIC-galactosylated chitosan (GCH). MATERIALS AND METHODS: GC, GMC and GCH were synthesized and radiolabeled with 99mTc. Then, they were incubated for 6 hours at room temperature and human serum at 37 degrees C. Labeling efficiencies were determined at 15, 30 m, 1, 2, 3 and 6 h after radiolabeling. To evaluate cytotoxicity, MTT assay was performed in HeLa and HepG2 cells. RESULTS: In comparison with them of 99mTc-GC, labeling efficiencies of 99mTc-GMC were significantly improved (100, 97 and 89% in acetone and 96.3, 95.8 and 75.6% in saline at 15 m, 1 and 6 h, respectively). Moreover, 99mTc-GCH showed more improved labeling efficiencies (> 95% in acetone and human serum and > 90% in saline at 6 h). In MTT assay, cytotoxicity was very low and not different from that of controls. CONCLUSION: These results represent that these compounds are radiochemically compatible radiopharmaceuticals, can be used in hepatocyte specific imaging study and in vivo gene or drug delivery monitoring.
Acetone
;
Chitosan*
;
Hep G2 Cells
;
Hepatocytes
;
Humans
;
Radiopharmaceuticals
5.Expression of apolipoprotein C-II mRNA in cultured HepG2 cell.
Myung Jae PARK ; Dong Hee SEO ; Kwang Sik SEO ; Jeong Taek WOO ; Jin Woo KIM ; Young Seol KIM ; Kwang Won KIM ; Young Kil CHOI
Journal of Korean Society of Endocrinology 1992;7(2):127-135
No abstract available.
Apolipoprotein C-II*
;
Apolipoproteins*
;
Hep G2 Cells*
;
RNA, Messenger*
6.Experimental study on high throughput vitrification by micro-droplet spray method.
Zixuan YU ; Xiaomin ZHANG ; Xinli ZHOU
Journal of Biomedical Engineering 2019;36(5):850-855
There is a great demand for blood and stem cells in clinic. It is difficult to achieve high throughput and to increase the cooling rate at the same time during vitrification. In this paper, a micro-droplet spray system with a container collection device was fabricated, and HepG2 cells were sprayed by this system for high-throughput vitrification. First, the container collection device and a cryo-paper were used to receive micro-droplets in the spray vitrification system. The results showed that the cell survival rate and 24h adhesion rate in container collection vitrification group were significantly higher than those in cryo-paper collection group. Second, HepG2 cells were sprayed and vitrified at increased cell density, and it was found that the results of micro-droplet spray vitrification did not change significantly. Finally, micro-droplet spray vitrification is compared with slow freezing. Cell processing capacity in the vitrification group increased, meanwhile, the cell survival rate and 24h adhesion rate in the vitrification group were significantly higher than those in slow freezing group. The results indicated that the micro-droplet spray vitrification system with container collection device designed in this paper can achieve high-throughput cell vitrification, which is of great significance for mass preservation of small cells.
Cell Adhesion
;
Cell Survival
;
Cryopreservation
;
Hep G2 Cells
;
Humans
;
Vitrification
7.Research on autophagy induced by two xanthone compounds in HepG2 cells.
Yu-Xuan WANG ; Hai-Ying LIU ; Jin-Hong REN ; Hua-Feng ZHANG ; Hui-Qing XUE
China Journal of Chinese Materia Medica 2020;45(9):2151-2157
To investigate the inhibitory effects of two xanthone compounds, 1-hydroxy-2,3,4,8-4 methoxy xanthone(here in after referred to as Fr15) and 1-hydroxy-2,3,4,6-4 methoxy xanthone(here in after referred to as Fr17), on the proliferation of hepatocellular carcinoma cells HepG2, and to further investigate their mechanism in combination with transcriptomics. Cell counting was used to detect the effects of two kinds of xanthone compounds Fr15 and Fr17(0, 0.03, 0.15, 0.3 mmoL·L~(-1)) on the proliferation of HepG2 cells; the effects of the two compounds Fr15 and Fr17 on HepG2 cell cycle were detected by flow cytometry; the changes of autophagosomes count in cells were observed under fluorescence microscope; the expression of autophagy marker proteins autophagy marker proteins SQSTM 1(p62) and microtubule associated protein 1 light chain 3 Ⅰ/Ⅱ(LC3 Ⅰ/Ⅱ) in the cells was detected by Western blot; the differentially expressed genes between the control group and the experimental group were analyzed by RNA-seq transcriptome sequencing; qRT-PCR was used to verify the differentially expressed genes in sequencing. The results showed that compounds Fr15 and Fr17 inhibited the proliferation of HepG2 cells with the increase of drug concentration and time. Flow cytometry showed that compounds Fr15 and Fr17 had little effect on HepG2 cell cycle. Fluorescence microscopy results showed that the number of autophagosomes in cells increased with the increase of drug concentration. Western blot showed that the expression of p62 protein was decreased and the expression of LC3-Ⅱ protein was significantly increased after drug addition. The results of RNA sequencing showed that 26 102 and 52 351 differentially expressed genes were obtained in Fr15 and Fr17 respectively. Analysis of KEGG showed that drug treatment had a great effect on autophagy pathway. qRT-PCR verified that 6 up-regulated genes were related to autophagy, and their trend was consis-tent with sequencing results, where all 6 genes showed an up-regulated trend. Two xanthone compounds Fr15 and Fr17 may inhibit proliferation of HepG2 cells by inducing autophagy.
Apoptosis
;
Autophagy
;
Cell Cycle
;
Hep G2 Cells
;
Xanthones
8.Optimization of Three-Dimensional Culture Conditions of HepG2 Cells with Response Surface Methodology Based on the VitroGel System.
Jing Bo WANG ; Wen QIN ; Zhuo YANG ; Shi SHEN ; Yan MA ; Li Yuan WANG ; Qin ZHUO ; Zhao Long GONG ; Jun Sheng HUO ; Chen CHEN
Biomedical and Environmental Sciences 2022;35(8):688-698
OBJECTIVE:
This study optimizes three-dimensional (3D) culture conditions of HepG2 using response surface methodology (RSM) based on the VitroGel system to facilitate the cell model in vitro for liver tissues.
METHOD:
HepG2 cell was 3D cultured on the VitroGel system. Cell viability was detected using Cell Counting Kit-8 (CCK-8) assay of HepG2 lived cell numbers. The proliferation of HepG2 cell and clustering performance was measured via fluorescence staining test. Albumin concentration in the culture medium supernatant as an index of HepG2 cell biological function was measured with ELISA kit. Independent factor tests were conducted with three key factors: inoculated cell concentration, cultured time, and dilution degree of the hydrogel. The preliminary results of independent factor tests were used to determine the levels of factors for RSM.
RESULT:
The selected optimal culture conditions are as follows: concentration of inoculated cells was 4.44 × 10 5/mL, culture time was 4.86 days, and hydrogel dilution degree was 1:2.23. The result shows that under optimal conditions, the predicted optical density (OD) value of cell viability was 3.10 and measured 2.978 with a relative error of 3.94%.
CONCLUSION
This study serves as a reference for the 3D HepG2 culture and constructs liver tissues in vitro. Additionally, it provides the foundation for repeated dose high-throughput toxicity studies and other scientific research work.
Albumins
;
Cell Culture Techniques/methods*
;
Hep G2 Cells
;
Humans
;
Hydrogels
9.Triterpenes constituents from male flowers of Eucommia ulmoides.
Yan-Xia DING ; Teng-Yu WANG ; Yao-Wen ZHANG ; Yu-Mei HUANG ; Lin MA ; Dong-dong LI ; De-Qiang DOU ; Qin LI
China Journal of Chinese Materia Medica 2014;39(21):4225-4229
Nine triterpenes compounds were isolated from the male flowers of Eucommia ulmoides by recrystallization and chromatographic techniques over silica gel, Sephadex LH-20, and RP-18 gel. Their chemical structures were identified on the basis of spectral analysis and as 3-oxo-12-en-ursane-28-O-α-L-arabinofuranosyl (1 --> 6) -β-D-glucopyranoside (1), 2α, 3β-dihydroxyurs-12-en-28-oic acid(28 --> 1) -β-D-glucopyranosyl ester (2), ursolic acid (3), α-amyrin (4), uvaol (5), ursolic acid acetate (6), 3-O-acetate oleanoic acid (7), betulinic acid (8), and betulinol (9). Compound 1 was a new compound, and compounds 2, 4-7 were isolated from the Eucommiu genus for the first time. Cytotoxic activity was tested for all the compounds against K562 and HepG2 cells. The results showed that only compound 3, exhibited cytotoxic activity.
Antineoplastic Agents, Phytogenic
;
pharmacology
;
Eucommiaceae
;
chemistry
;
Hep G2 Cells
;
Humans
;
K562 Cells
;
Triterpenes
;
analysis
;
pharmacology
10.Anti-tumor activity of components isolated from purple sweet potato polysaccharides.
Jing ZHAO ; Hong RUAN ; Qiu-ping GAO ; Meng-ya LI ; Ye-qi TAO ; Ying ZHENG
Journal of Zhejiang University. Medical sciences 2011;40(4):365-373
OBJECTIVETo isolate and purify components from polysaccharides of purple sweet potato (PPSP) and to test their anti-tumor activity.
METHODSDEAE-Cellulose and CM-Cellulose exchange chromatography were applied to separate components of PPSP. The anti-tumor activities of each component were measured by MTT assay on Hela and HepG(2) cells and their monosaccharide composition were analyzed by TLC chromatography, followed by infrared spectroscopy studies.
RESULTSThrough weak anion exchange chromatography and gradient elution by sodium chloride solution, four components were separated and named as PPSP, PPSPII, PPSPIII and PPSPIV, respectively. MTT tests showed that PPSP II and PPSPIII inhibited Hela and HepG2 tumor cells in a certain extent. The structural analysis revealed that PPSPI was mainly composed of glucose and galactose, PPSP II was composed of glucose and had a typical absorption peak of β-D-glucose chitosan pyranose, PPSP III was a glycoprotein showing a protein absorption peak.
CONCLUSIONFour components were separated from PPSP successfully, among which PPSP II and PPSP III shows anti-tumor activities on Hela and HepG(2) cells in vitro.
Antineoplastic Agents, Phytogenic ; pharmacology ; HeLa Cells ; Hep G2 Cells ; Humans ; Ipomoea batatas ; chemistry ; Polysaccharides ; pharmacology