Introduction

ETM

Experimental and Therapeutic Medicine

1792-0981 1792-1015

D.A. Spandidos

10.3892/etm.2016.3556

ETM-0-0-3556

Articles

Flavonoids from Artemisia sacrorum Ledeb. and their cytotoxic activities against human cancer cell lines

Yuan

Haidan

1 2 * Lu

Xuyang

3 * Ma

Qianqian

1 Li

1 Xu

Guanghua

1 Piao

Guangchun

1 2

1Department of Pharmacognosy, College of Pharmacy, Yanbian University, Yanji, Jilin 133000, P.R. China 2Key Laboratory of Natural Resources of Changbai Mountain and Functional Molecules, Ministry of Education, Yanbian University, Yanji, Jilin 133000, P.R. China 3Department of Pharmacy, Jilin Central Hospital, Jilin, Jilin 132000, P.R. China

Correspondence to: Dr Guangchun Piao, Department of Pharmacognosy, College of Pharmacy, Yanbian University, 977 Gongyuan Road, Yanji, Jilin 133000, P.R. China, E-mail: gcpiao@ybu.edu.cn *

Contributed equally

09 2016

27 07 2016

12 3 1873 1878 10032015 01062016

2016

Flavonoids have been demonstrated to have cytotoxic activities toward numerous human cancer cells, whereas they have little or no effect on normal cells. The numerous flavonoids in traditional Chinese herbs may be promising candidates for the development of novel anti-cancer drugs. Our previous study demonstrated that CH₂Cl₂ and 95% ethanol eluate (EE) fractions have the strongest cytotoxic activities against human cancer cell lines of the 9 fractions separated from Artemisia sacrorum Ledeb., which is widely used to prevent and treat diverse diseases in Northeast China. In the present study, 8 flavonoids were isolated from the 95% EE fraction of Artemisia sacrorum Ledeb. The chemical structures of the compounds were elucidated by extensive spectroscopic analyses. The following 5 flavonoids were isolated for the first time from this plant: Jaceosidin, kaempferol, quercetin, luteolin and quercitrin. A total of 2 flavonoids from the CH₂Cl₂ fraction and 8 flavonoids from the 95% EE fraction were examined to evaluate their cytotoxic activities against human SK-HEP-1 hepatoma cancer cells and human HeLa cervical cancer cells, respectively. The results revealed that 2 flavonoids had marked cytotoxic activities against HeLa cells.

Artemisia sacrorum Ledeb. flavonoids cytotoxic activities human cancer cell lines

Introduction

The majority of approved anticancer drugs are either natural products or have been developed based on knowledge gained from natural products, which have been important in the search for novel anticancer drugs compared with other areas of drug development (1–5). Traditional Chinese medicine has been historically used to treat disease using natural products. Although certain traditional Chinese herbs should no longer be used, other traditional Chinese herbs that have been proven to be effective have been gradually incorporated into modern medicine (6).

Among these traditional Chinese medicinal plants, Artemisia sacrorum Ledeb (ASL; Compositae) is of particular interest as it is widely used to prevent and treat diverse diseases in the Yanbian area of Northeast China (7,8). Previous studies have indicated that the water-soluble parts of the A. sacrorum extract were protective against carbon tetrachloride and acetaminophen-induced hepatotoxicity in mice, and the underlying mechanisms have been investigated (9–11). In a previous study, A. sacrorum was demonstrated to prevent N-acetyl-p-aminophenol (APAP)-induced apoptosis and necrosis, as indicated by liver histopathological and immunohistochemical analysis, and DNA laddering (9–11). According to the results from a western blot analysis, the ethanol eluate precipitation (EEP) decreased APAP-induced caspase-3 and −8 protein expression levels in mouse livers (9–11). Furthermore, ASL was able to inhibit adipocyte differentiation and adipogenesis through the activation of 5′-adenosine monophosphate-activated protein kinase (AMPK) in 3T3-L1 adipocytes and hepatocellular carcinoma (HepG2) cells, respectively (12,13). Petroleum ether fraction of A. sacrorum Ledeb, another extract from A. sacrorum, inhibited glucose production via the AMPK-glycogen synthase kinase-cAMP response element binding protein signaling pathway in HepG2 cells (14). Notably, the cytotoxicities of the 9 fractions separated from A. sacrorum via the two extraction methods was investigated in our previous study, and the results demonstrated that the CH₂Cl₂ and 95% ethanol eluate (EE) fractions revealed the strongest cytotoxic activities against 3 human cancer cell lines. In addition, a subsequent study demonstrated that 10 compounds, of which 2 were flavonoids, were isolated from the CH₂Cl₂ fraction (15).

The present study aimed to investigate the isolation and structure of the compounds from the 95% EE fraction of A. sacrorum. The results demonstrated that this fraction was markedly rich in flavonoids. Flavonoids are cancer-preventive agents, and have been shown to be particularly important (16–18). Therefore, the present study was further conducted to evaluate the cytotoxic activities of all flavonoids from the CH₂Cl₂ and 95% EE fractions.

Materials and methods <sec> <title>General experimental procedures

The nuclear magnetic resonance (NMR) spectra of compounds 1, 2, 3, 5, 6, and 7 were recorded on a Bruker 500 MHz NMR spectrometer (Bruker Corporation, Billerica, MA, USA), operating at a frequency of 500 MHz for ¹H and 125 MHz for ¹³C nuclei at room temperature, and with TMS as the internal standard. The NMR spectra of compounds 4 and 8 were recorded on a Bruker 300 MHz NMR spectrometer, operating at 300 MHz for ¹H and 75 MHz for ¹³C nuclei at room temperature with tetramethylsilane (TMS) as the internal standard. Chemical shifts (δ) were expressed in parts per million (ppm) relative to TMS. The chemical shifts (δ) and coupling constant values were reported in ppm and Hz, respectively. Compounds 1, 2, 3, 4, 6, and 7 were dissolved in CD₃OD, 5 was dissolved in dimethyl sulfoxide (DMSO), and 8 was dissolved in acetone-d₆. Column chromatography (CC) was performed on a Sephadex LH-20 (18–111 µm; GE Healthcare Biosciences, Pittsburgh, PA, USA), YMC-GEL octadecyl (ODS)-A (50 µm; YMC Co., Ltd., Kyoto, Japan) and silica gel (200–300 mesh, Qingdao Marine Chemical, Ltd., Qingdao, China) columns. D-101 macroporous absorption resin was purchased from Tianjin Haiguang Chemical Co., Ltd. (Tianjin, China). Silica gel 60 F254 plates (20×20 cm; 0.2 mm thick; Merck, Darmstadt, Germany) and silica gel GF 254 (Qingdao Marine Chemical Co., Ltd.) were used for thin-layer chromatography (TLC) analysis. The CH₃OH used for column chromatography was high performance liquid chromatography-grade (Jiangsu Hanbang Science and Technology Co., Ltd., Jiangsu, China). All other chemicals and reagents used in the present study were of analytical grade.

Plant material

The aerial parts of ASL (Compositae) were collected in July 2008 from Xidong, Yanji in Jilin. The plant was taxonomically identified and authenticated by Professor Huizi Lv (College of Pharmacy, Yanbian University of China, Yanji, China). A specimen of the plant was deposited at the College of Pharmacy, Yanbian University.

Extraction and isolation

A total of 5 kg of the aerial parts of A. sacrorum were collected, air-dried in the shade, and dissolved in boiling water twice (Figs. 1 and 2). The extract was then separated on a D-101 macroporous absorption resin to elute water, 50% EE and 95% EE fractions. From this separation, the 95% EE fraction (16.03 g) was chromatographed on a silica-gel column (200–300 mesh) with petroleum ether-EtOAc in a stepwise gradient elution (50:1-0:100). The eluates were combined based on the TLC results in order to produce 8 fractions (1–8).

The fractions were chromatographed as follows: Fraction 2 was chromatographed on an ODS column by eluting with gradient mixtures of CH₃OH and H₂O (8:2 to 10:0) in order to obtain 7 subfractions (2.1–7). Subfraction 2.3 was rechromatographed on a Sephadex LH-20 column by eluting with gradient mixtures of CH₃OH and H₂O (8:2 to 10:0) to obtain compound A (3.0 mg). Fraction 3 was rechromatographed on an ODS column by eluting with gradient mixtures of CH₃OH and H₂O (7:3 to 10:0) to afford compound 1 (23.2 mg). Fraction 4 was rechromatographed on an ODS column by eluting with gradient mixtures of CH₃OH and H₂O (6:4 to 10:0) to obtain 11 subfractions (4.1–11). Subfraction 4.3 was rechromatographed on a Sephadex LH-20 column by eluting with gradient mixtures of CH₃OH and H₂O (8:2 to 10:0) to obtain compound 2 (2.6 mg) and compound 3 (1.5 mg). Subfraction 4.6 was subjected to a Sephadex LH-20 column by eluting with gradient mixtures of CH₃OH and H₂O (7:3 to 10:0) to obtain compound 4 (8.2 mg). Fraction 5 was rechromatographed on a Sephadex LH-20 column by eluting with CH₃OH-H₂O (7:3 to 10:0) to obtain compound 5 (2.0 mg) and 12 subfractions (5.1–12). Subfraction 5.10 was subjected to a Sephadex LH-20 column by eluting with gradient mixtures of CH₃OH and H₂O (8:2 to 10:0) to obtain compound 6 (1.5 mg). Fraction 6 was rechromatographed on an ODS column by eluting with gradient mixtures of CH₃OH and H₂O (6:4 to 10:0) to obtain eight subfractions (6.1–8). Subfraction 6.6 was subjected to a Sephadex LH-20 column repeatedly to obtain compound 7 (2.6 mg). Fraction 7 was rechromatographed on a Sephadex LH-20 column by eluting with gradient mixtures of CH₃OH-H₂O (4:6 to 10:0) to produce 5 subfractions (7.1–5). Finally, subfraction 7.2 was subjected to a Sephadex LH-20 column once more by eluting with gradient mixtures of CH₃OH and H₂O (6:4 to 10:0) to afford compound 8 (6.0 mg).

Cell culture and MTS assay

The two human cancer cell lines (SK-HEP-1 and HeLa) and one normal human cell line (HEK293) used in the cytotoxic assay were purchased from American Type Culture Collection (Manassas, VA, USA). All cell lines were cultured in Dulbecco's modified Eagle medium supplemented with 10% fetal bovine serum, 100 units/ml penicillin and 100 mg/ml streptomycin and kept at 37°C in a humidified atmosphere containing 5% CO₂.

A 200-µl aliquot of adherent cells was used to seed 96-well cell culture plates at 3×10⁴ cells/well and allowed to adhere for 6 h prior to drug addition. Each cell line was treated with 0, 5, 10, 25, 50, 100 and 200 µM of flavonoids for 48 h. Subsequently, 20 µl MTS reagent was added into each well and incubated for 1 h. The cell viability was detected by the CellTiter 96 AQueous One solution Cell Proliferation Assay kit (Promega Corporation, Madison, WI, USA).

Results and Discussion

To observe the cytotoxic activity of the herb, A. sacrorum was extracted and isolated by 95% EtOH and water, as described in our previous study (15). Following extraction with 95% EtOH extract with various solvents, and separation of the water extract with a D-101 macroporous resin column, 9 fractions of A. sacrorum were obtained, of which the 95% EE and CH₂Cl₂ fraction revealed the strongest cytotoxity against 3 human cancer cell lines. In a subsequent study, 2 flavonoids were isolated from the CH₂Cl₂ fraction (15). In the present study, 9 compounds were isolated from the 95% EE fraction.

Compound 1 was isolated as yellow, needle-like crystals (acetone). The ¹H-NMR and ¹³C-NMR spectra of the compound revealed the characteristic signals of a flavonoid. The ¹H-NMR spectrum exhibited two proton signals at δ 6.56 (1H; s) and 6.61 (1H; s), which represented the proton signals of C3-H and C8-H of the A ring, respectively. Signals at δ 7.45 (1H; d; J=2.0 Hz), 6.92 (1H; d; J=8.35 Hz) and 7.49 (1H; dd; J=2.0; 8.35 Hz) represented the proton signals of C2′-H, C5′-H and C6′-H of the B ring. δ 3.96 (3H; s) and 3.88 (3H; s) corresponded to the proton signals of the 2 methoxy groups. The ¹³C-NMR spectrum showed 17 carbon signals of which δ_C 184.23 was the carbonyl signal, whereas 56.71 and 60.94 were assigned to 2 methoxy groups. By analyzing these data and comparing them with those in the literature (19), the structure of compound 1 was determined as jaceosidin (Fig. 3).

Compound 2 was obtained as a yellow powder (MeOH). The ¹H-NMR spectrum demonstrated 2 meta-coupled proton signals at δ 6.18 (1H; d; J=2.0 Hz; H-6) and 6.40 (1H; d; J=2.0 Hz; H-8) of the A ring. Two groups of meta-coupled proton signals at δ 6.90 (2H; d; J=9.0 Hz; H-3′; H-5′) and 8.09 (2H; d; J=9.0 Hz; H-2′; H-6′) were assigned to 4 protons in the B ring. The ¹³C-NMR spectrum revealed carbon signals of δ_C 148.15, 137.17, 177.44, 158.35, 99.38, 165.77, 94.55, 162.53, and 104.56 for the A ring, and 123.81, 130.69, 116.35, 160.57, 116.35, and 130.69 for the B ring. Based on the above spectral data and comparison with a previous study (20), the chemical structure of compound 2 was determined as kaempferol.

Compound 6 was obtained as yellow, needle-like crystals (MeOH). The ¹H-NMR spectrum revealed 2 isolated proton signals at δ 6.58 (1H; s; H-3) and 6.67 (1H; s; H-8), which were attributed to H-3 (C-ring) and H-8 (A-ring), respectively. Two groups of meta-coupled proton signals at δ 6.92 (2H; d; J=8.75 Hz; H-3′; H-5′) and 7.84 (2H; d; J=8.75 Hz; H-2′; H-6′) were assigned to 4 protons of the B ring. The ¹³C-NMR spectrum showed δ_C values of 164.46, 102.46, 184.31, 152.69, 131.70, 157.66, 94.17, 152.69, and 104.87 for the A ring, and 122.14, 128.45, 116.15, 161.32, 116.15, and 128.45 for the B ring. These spectroscopic data were characteristic of a flavonoid. Based on the above spectral data and comparison with previous studies (21,22), the chemical structure of compound 6 was determined as hispidulin.

Compound 8 was obtained as a yellow powder (acetone). ¹H-NMR revealed, in the aromatic region, 2 meta-coupled proton signals at δ 6.25 (1H; d; J=2.07 Hz; H-6) and 6.46 (1H; d; J=2.07 Hz; H-8) for the A ring. ¹H-NMR also demonstrated 2 meta-coupled proton signals at δ 7.49 (1H; d; J=2.07 Hz; H-2′), 7.39 (1H; dd; J=2.07; 8.34 Hz; H-6′), and 1 isolated proton signal at δ 6.98 (1H; d; J=8.34 Hz; H-5′) for the B ring. These 3 proton signals exhibited the typical three-spin system of the 1′,3′,4′-trisubstituted B ring. δ 5.28 (1H; d; J=1.5 Hz; H-1′′) was the anomeric proton signal of sugar. The ¹³C-NMR spectrum revealed a carbonyl proton signal at δ_C 179.18, which was assigned to C-4, and 17.63–102.57 ppm for a group of 6-carbon sugar signals revealing the presence of an aglycone moiety. Based on the above spectral data and a comparison with previous studies (23,24), the chemical structure of compound 8 was determined as quercitrin.

In addition to the above-mentioned compounds, 5 other compounds were also identified as chrysoeriol (compound 3) (25), quercetin (compound 4) (26), apigenin (compound 5) (27), luteolin (compound 7) (28,29) and scopoletin (compound A) (30). These were identified by interpretation of their spectroscopic data and comparison of the data with the reported values. Among them, compounds 1–8 were flavonoids, and flavonoids 1, 2, 4, 7 and 8 were isolated for the first time from A. sacrorum. The structures of the 8 flavonoids are depicted in Fig. 3 and all ¹³C-NMR spectra data were listed in Table I.

A total of 8 flavonoids isolated from the 95% EE fraction of A. sacrorum were designated as flavonoids 1–8, and 2 flavonoids (genkwanin and acacetin) previously isolated from the CH₂Cl₂ fraction were designated as flavonoids 9 and 10. Although these 10 flavonoids were not novel compounds, their possible biological activities should not be ignored because they have previously been identified. Furthermore, not every novel compound is examined for all its activities (even in vitro experiments before it is considered to be old). Conversely, the majority of novel compounds have only undergone in vitro activity tests.

In the present study, the cytotoxic activities against the 10 flavonoids on SK-HEP-1, HeLa and HEK293 cell growth were determined using an MTS assay (31). Their IC₅₀ values were presented in Table II, in which apigenin (flavonoid 5) and luteolin (flavonoid 7) exhibited strong cytotoxic activities against human cervical cancer HeLa cells. Conversely, they had no cytotoxic activity against normal human embryonic kidney HEK293 cells.

The structures of the 10 flavonoids are similar. However, certain flavonoids revealed different cytotoxic activity against the two human liver cancer SK-HEP-1 and human cervical cancer HeLa cells. Although certain flavonoids have similar chemical structures, there are still compound-specific effects on certain neoplasms that are relevant to adjust specific biochemical processes to treat certain neoplasms differentially (32,33). In the present study, the majority of the 10 flavonoids demonstrated no cytotoxic activity against normal human embryonic kidney cells.

Flavonoids may serve as clinically significant chemotherapeutic agents in the treatment of cancer. Indeed, flavonoids have been demonstrated to reveal cytotoxic activities towards numerous human cancer cells, whilst having little or no effect on normal cells. This has led to interest in the development of potential flavonoid-based chemotherapeutics for anticancer treatment (34–37). Traditional Chinese herbs, which depend predominantly on empirical medication, have been used for thousands of years in the treatment of numerous diseases, often with few adverse effects. Furthermore, many of the active flavonoids in traditional Chinese herbs have been the subject of studies aiming to develop novel anti-cancer drugs by demonstrating their activity through in vivo and in vitro experiments (38–40). The diverse flavonoids in these herbal medicines may be promising candidates in the development of novel anti-cancer drugs.

Acknowledgements

The present study was supported by the Natural Science Foundation of China (grant no. 81260669). The authors are grateful to Mr. Guang-Hao Zheng and Mr. Zhi-Yong Li for their support during the extraction and fractionation procedures. We also thank Dr. Ming-Shan Zheng for her help in the chemical structure elucidation of several compounds.

References 1

LiWeber

New therapeutic aspects of flavones: The anticancer properties of Scutellaria and its main active constituents Wogonin, Baicalein and Baicalin

Cancer Treat Rev3557682009

10.1016/j.ctrv.2008.09.005

19004559

Samarghandian

Afshari

Davoodi

Chrysin reduces proliferation and induces apoptosis in the human prostate cancer cell line pc-3

Clinics (Sao Paulo)66107310792011

10.1590/S1807-59322011000600026

21808878

Tundis

Loizzo

Menichini

Bonesi

Colica

Menichini

In vitro cytotoxic activity of extracts and isolated constituents of Salvia leriifolia Benth. against a panel of human cancer cell lines

Chem Biodivers8115211622011

10.1002/cbdv.201000311

21674787

Sak

Cytotoxicity of dietary flavonoids on different human cancer types

Pharmacogn Rev81221462014

10.4103/0973-7847.134247

25125885

Newman

Cragg

Natural products as source of new drugs over the last 25 years

J Nat Prod704614772007

10.1021/np068054v

17309302

Dong

The relationship between traditional chinese medicine and modern medicine

Evid Based Complement Alternat Med20131531482013

10.1155/2013/153148

23983772

Piao

Cui

Zhang

Korean ethnic Materia Medica in ChinaYanji, China

Yanbian People Press

Yan Bian Ren Min Chu Ban She2442452012

Jia

Chinese ethnic Materia Medica

Zhong Guo Yi Yao Ke Ji Chu Ban She692005

Piao

Quan

Protective effects of extracts of Artemisia sacrorum Ledeb. on acute hepatic injury in mice

Shi Zhen Guo Yi Guo Yao18164616472007(In Chinese)

Yuan

Jin

Piao

Protective effects of the supernatant of ethanol eluate from Artemisia sacrorum Ledeb. against acetaminophen-induced liver injury in mice [corrected]

Biol Pharm Bull32168316882009

10.1248/bpb.32.1683

19801828

Yuan

Jin

Piao

Hepatoprotective effects of an active part from Artemisia sacrorum Ledeb. against acetaminophen-induced toxicity in mice

J Ethnopharmacol1275285332010

10.1016/j.jep.2009.10.002

19833181

Yuan

Piao

An active part of Artemisia sacrorum Ledeb. inhibits adipogenesis via the AMPK signaling pathway in 3T3-L1 adipocytes

Int J Mol Med275315362011

21327327

Yuan

Chung

Jin

Piao

An active part of Artemisia sacrorum Ledeb. attenuates hepatic lipid accumulation through activating AMP-activated protein kinase in human HepG2 cells

Biosci Biotechnol Biochem743223282010

10.1271/bbb.90651

20139613

Yuan

Piao

An active part of Artemisia sacrorum Ledeb. inhibits adipogenesis via the AMPK signaling pathway in 3T3-L1 adipocytes

Int J Mol Med275315362011

21327327

Piao

Yuan

Jin

Cytotoxic fraction from Artemisia sacrorum Ledeb. against three human cancer cell lines and separation and identification of its compounds

Nat Prod Res26148314912012

10.1080/14786419.2011.565473

22008023

Chien

Shen

Huang

Shih

Antimetastatic potential of fisetin involves inactivation of the PI3K/Akt and JNK signaling pathways with downregulation of MMP-2/9 expressions in prostate cancer PC-3 cells

Mol Cell Biochem3331691802010

10.1007/s11010-009-0217-z

19633975

Chung

Jiang

Cheng

Birt

Impact of adenomatous polyposis coli (APC) tumor supressor gene in human colon cancer cell lines on cell cycle arrest by apigenin

Mol Carcinog467737822007

10.1002/mc.20306

17620292

Takagaki

Sowa

Oki

Nakanishi

Yogosawa

Sakai

Apigenin induces cell cycle arrest and p21/WAF1 expression in a p53-independent pathway

Int J Oncol261851892005

15586239

Wang

Study on chemical constituents of Artemisia frigida (II)

Chin Tradit Herb Drug42107510782011

Yang

Analytical Chemistry Handbook, Vol 72nd edition

Beijing Chemical industry Press

820

Beijing

8201999

Hazekamp

Verpoorte

Panthong

Isolation of a bronchodilator flavonoid from the Thai medicinal plant Clerodendrum petasites

J Ethnopharmacol7845492001

10.1016/S0378-8741(01)00320-8

11585687

Zhou

Guo

Yang

Compounds from roots of Chirita fimbrisepala Hand.-Mazz

Zhongguo Zhong Yao Za Zhi261141172001(In Chinese)

12525106

Wang

Cao

Yang

Chemical constituents in aerial parts of Polygonum capitatum

Zhong Cao Yao4424302013

Kong

Studies on the Constituents of Hypericum japonicum Thunb. Ex Murray

Zhong Guo Xian Dai Zhong Yao912132007

Wei

Chen

Cai

Lin

Chemical constituents in whole herb of Cardiospermum halicacabum (I)

Zhong Cao Yao42150915112011

Luo

Liu

Fan

Ding

Yao

Studies on the anti-hypoxia active Constituents of Artemisia scoparia

Zhong Cao Yao Zeng Kan371992012006

Nan

Zhang

Chemical constituents from Clerodendrum inerme

Zhong Cao Yao364924942005

Wei

Yan

Guan

Liu

Wei

Analysis of the chemical constituents of the ground part of Sedum sarmentosum

J B Univ TCM2659612003

Wei

Feng

Flavonoids from Lespedeza davurica

Acta Bot Boreal-Occident Sin30148514892010

Xie

Liang

Liu

Wang

Wei

Yang

Chemical Study on Artemisia scoparia

J China Pharm Univ354014032004

Kometani

Yoshino

Miura

Okazaki

Ohba

Takenaka

Shoji

Yano

Maehara

Benzo[a]pyrene promotes proliferation of human lung cancer cells by accelerating the epidermal growth factor receptor signaling pathway

Cancer Lett27827332009

10.1016/j.canlet.2008.12.017

19181443

Bonham

Posakony

Coleman

Montgomery

Simon

Nelson

Characterization of chemical constituents in Scutellaria baicalensis with antiandrogenic and growth-inhibitory activities toward prostate carcinoma

Clin Cancer Res11390539142005

10.1158/1078-0432.CCR-04-1974

15897592

Zheng

Hirose

Yoshimi

Murakami

Koshimizu

Ohigashi

Sakata

Matsumoto

Sayama

Mori

Further investigation of the modifying effect of various chemopreventive agents on apoptosis and cell proliferation in human colon cancer cells

J Cancer Res Clin Oncol1285395462002

10.1007/s00432-002-0373-y

12384797

Cai

Guan

Wang

Liu

Baicalin induces human mucoepidermoid carcinoma Mc3 cells apoptosis in vitro and in vivo

Invest New Drugs296376452011

10.1007/s10637-010-9402-x

20204673

Chen

Hsieh

Tsai

Kang

Chang

Protoapigenone, a natural derivative of apigenin, induces mitogen-activated protein kinase-dependent apoptosis in human breast cancer cells associated with induction of oxidative stress and inhibition of glutathione S-transferase TT

Invest New Drugs29134713592011

10.1007/s10637-010-9497-0

20686818

Plochmann

Korte

Koutsilieri

Richling

Riederer

Rethwilm

Schreier

Scheller

Structure-activity relationships of flavonoid-induced cytotoxicity on human leukemia cells

Arch Biochem Biophys460192007

10.1016/j.abb.2007.02.003

17353006

BenSghaier

Skandrani

Nasr

Franca

ChekirGhedira

Ghedira

Flavonoids and sesquiterpenes from Tecurium ramosissimum promote antiproliferation of human cancer cells and enhance antioxidant activity: A structure-activity relationship study

Environ Toxicol Pharmacol323363482011

10.1016/j.etap.2011.07.003

22004952

Luo

Sun

Dong

Wang

Qin

Sun

Isorhamnetin attenuates atherosclerosis by inhibiting macrophage apoptosis via PI3K/AKT activation and HO-1 induction

PLoS One10e01202592015

10.1371/journal.pone.0120259

25799286

Chen

Zhang

Yuan

Yang

Liu

Zhao

Liu

Wang

Zheng

Isoliquiritigenin-induced differentiation in mouse melanoma B16F0 cell line

Oxid Med Cell LongevDec102012(Epub ahead of print) doi: 10.1155/2012/534934

10.1155/2012/534934

Wang

General research on effects of flavonoids ingredients on Chinese herbs on anti-cancer

Zhe Jiang Zhong Yi Yao Da Xue Xue368388402012(In Chinese)

Figure 1.

Extraction scheme for the isolation of 10 flavonoids from the 2 most cytotoxic fractions of Artemisia sacrorum Ledeb. By shade-dried we mean that the aerial parts of the herb were air-dried in the shade. EE, ethanol eluate; PE, petroleum ether; EEP, ethanol eluate precipitation; EES, ethanol eluate supernatant.

Figure 2.

Extraction and separation of 8 flavonoids and 1 coumarin from the 95% EE fraction. Fr, fraction; EE, ethanol eluate.

Figure 3.

Chemical structures of 8 flavonoids from the 95% EE fraction from Artemisia sacrorum Ledeb. 1–8 represent the compound numbers. EE, ethanol eluate.

Table I.

¹³C-NMR spectra data of compounds 1–8 (δ, ppm; compounds 4 and 8 were detected at 75 MHz, others at 125 MHz; compounds 1, 2, 3, 4, 6 and 7 dissolved in CD₃OD, compound 5 dissolved in DMSO, and compound 8 dissolved in acetone-d₆; OMe, OCH3).

Compound no.	1	2	3	4	5	6	7	8
2	166.24	148.15	160.89	147.99	164.17	164.46	164.73	158.15
3	103.80	137.17	104.15	137.24	103.04	102.46	104.62	135.63
4	184.23	177.44	183.79	177.34	181.77	184.31	183.66	179.18
5	154.70	158.35	163.13	158.23	157.48	152.69	162.33	163.06
6	132.97	99.38	123.75	99.22	98.90	131.70	99.78	99.35
7	158.90	165.77	166.09	162.52	163.88	157.66	165.61	164.77
8	95.38	94.55	95.31	94.39	94.16	94.17	94.75	94.35
9	154.70	162.53	156.19	165.58	161.22	152.69	158.25	157.63
10	105.78	104.56	105.39	104.52	103.77	104.87	103.89	105.75
1′	123.78	123.81	124.69	148.77	121.38	122.14	122.31	122.43
2′	110.75	130.69	110.70	115.98	128.56	128.45	114.22	115.99
3′	149.52	116.35	149.58	124.14	116.05	116.15	146.78	145.68
4′	152.13	160.57	152.52	146.22	161.06	161.32	150.71	148.85
5′	116.81	116.35	116.86	116.22	116.05	116.15	116.01	116.56
6′	121.76	130.69	121.77	121.67	128.56	128.45	120.46	122.73
OMe	56.71		56.72			59.85
OMe	60.94
1′′								102.57
2′′								71.26)
3′′								71.97)
4′′								72.86)
5′′								71.19
6′′								17.63

The table values represent ¹³C-NMR spectra data of compounds 1–8. OMe represents OCH₃. NMR, nuclear magnetic resonance; DMSO, dimethyl sulfoxide.

Table II.

Cytotoxities of 10 flavonoids isolated from Artemisia sacrorum (IC₅₀, µM).

Flavonoids	SK-HEP1	HeLa	HEK293
1	>50	>50	14.1380
2	>50	45.809	>50
3	47.19	>50	>50
4	45.96	>50	>50
5	46.56	6.092	>50
6	49.93	>50	>50
7	>50	16.254	>50
8	>50	>50	>50
9	>50	47.834	>50
10	>50	>50	>50

All compounds with IC₅₀ values >50 µM were considered inactive.