Induction of apoptosis in human hepatocellular carcinoma cells by extracts of Lannea coromandelica (Houtt.) Merr. and Diospyros castanea (Craib) Fletcher

Background

Hepatocellular carcinoma (HCC) in men is the fifth most common malignant tumor in the world and the second most common cause of cancer death [1]. The major risk factors for HCC include infection by hepatitis B and hepatitis C viruses, both of which are endemic in northeastern Thailand [2]. Drug resistance and severe side effects on normal tissues and cells have limited the effectiveness of chemotherapy [3].

Anticancer agents have been found in natural products, such as vincristine and vinblastine from Catharanthus roseus [4], taxol and docetaxel from Taxus brevifolia [5], and camptothecins from Camptotheca acuminata [6–9]. The Plant Genetics Conservation Project (under the patronage of HRH Princess Maha Chakri Sirindhorn) has reported on the cytotoxic and apoptotic effects of medicinal plants against hepatoma cells [10–13]. Subsequent study was performed on the plants locally found in Thailand which were used in this study including Lannea coromandelica (Houtt.) Merr. (LC); Catunaregam tomentosa (Blume ex DC.) Tirveng. (CT); Erythrophleum succirubrum Gagnep (ES); Diospyros castanea (Craib) Fletcher (DC); and Bombax anceps Pierre var. anceps (BA).

DC belongs to the family Ebenaceae, which is widespread in the tropics and subtropics [14]. Many Diospyros species have medicinal uses in Chinese, Ayurvedic, and African traditional medicine. Almost all the major parts of these plants have been used as medicines and reported to have biological and pharmacological activities [14]. LC belongs to the family Anacardiaceae. It is a deciduous tropical tree widely distributed in Bangladesh, India, and some other tropical countries [15–18]. CT belongs to the family Rubiaceae and has been used to treat diabetes mellitus, cancer, and tuberculosis. It possesses antimicrobial, antifungal, hypotensive, analgesic, antimalaria, antioxidant, and antileukemia pharmacological properties [19]. ES belongs to the family Leguminosae (subfamily Caesalpinioideae) and is used in Thai traditional medicines for fever and skin disease. Some isolated compounds (cassaine diterpenoid dimers) from this family contribute to anticancer activity by decreasing apoptosis inhibitors or increasing apoptosis inducers; this leads to tumor necrosis factor (TNF)-related apoptosis-inducing ligand resistance in human gastric adenocarcinoma cells [20]. BA belongs to the family Bombacaceae. Plants in this family are active against many different diseases [21–24] (Table 1); however, the dichloromethane extract from the root of B. malabaricum is inactive in the human epidermoid carcinoma (KB) and human cervical carcinoma (HeLa) cell lines [25].

To our knowledge, the mechanism of anticancer effect of these five plants on HCC is still unknown. This study aims to screen the anticancer activity of a crude 50 % ethanol–water extract of twigs of (a) BA; (b) CT; (c) ES; (d) LC; and (e) leaves and (f) twigs of DC. The cytotoxic and apoptotic actions of the extracts were investigated with a human HCC cell line (HepG2) and compared with their effects on normal Vero cells. One advantage of using the normal Vero cell line is that Vero cell line multiplies indefinitely while primary liver cells have a limited lifetime and die after a given number of generations. Consequently, the Vero cell line is easy to handle and represents an unlimited self-replicating source with a relatively high degree of homogeneity. We then analyzed major compounds common to the different effective extracts using gas chromatography–mass spectrometry (GC–MS).

Methods

Results

Determination of apoptosis pattern using DAPI

Cells were stained with DAPI fluorescent dye to assess apoptosis 24 h after treatment of cell lines with plant extracts at 2 × IC₅₀. Using 40× magnification, all five plant extracts were observed to cause alterations of nuclear morphology, revealing cell shrinkage, membrane blebbing, and apoptotic bodies (Fig. 1). The percentage of apoptotic cells was determined by observation using inverted microscopy for twigs of LC, CT, ES, BA, and leaves of DC. The positive control melphalan showed the highest induction of apoptosis in HepG2 (82.5 ± 8.0 %) and twigs of DC showed the lowest (66.0 ± 11.5 %) (Table 3).

Fig. 1

Nuclei morphological change of HepG2 cells stained with DAPI fluorescent dye at 24 h. a Untreated HepG2 cells; b 80 μg/mL of melphalan; c 500 μg/mL of L. coromandelica (twig) extract; d 500 μg/mL of C. tomentosa (twig) extract; e 400 μg/mL of E. succirubrum (twig) extract; f 300 μg/mL of D. castanea (leaf) extract; g 300 μg/mL of D. castanea (twig) extract; and h 400 μg/mL of B. anceps (twig) extract. Arrows indicate apoptotic nuclei based on heterogeneous staining, DNA condensation, and apoptotic bodies at ×40 objective magnification

Table 3

Apoptosis induction of ethanolic plant extracts in HepG2 (mean ± SD) (n = 3)

Sample	Part	Apoptosis induction
		% DAPI positive cell	DNA laddering
L. coromandelica (LC)	Twig	79.5 ± 5.5	Positive
C. tomentosa (CT)	Twig	69.0 ± 6.5	Negative
E. succirubrum (ES)	Twig	77.0 ± 13.5	Negative
D. castanea (DC)	Leaves	72.5 ± 12.5	Negative
D. castanea (DC)	Twig	66.0 ± 11.5	Positive
B. anceps (BA)	Twig	68.5 ± 7.5	Negative
Melphalan	–	82.5 ± 8.0	Positive

Apoptosis induction by plant extracts determined by DNA laddering assay

After treatment of HepG2 cell lines for 24 h with plant extracts, the DNA fragmentation of apoptotic cells was observed as DNA ladders using agarose gel electrophoresis. The results of DNA laddering showed that only LC and DC (twig) induced late-state apoptosis in HepG2 (Fig. 2); the other extracts did not induce late-stage apoptosis in HepG2 cells.

Fig. 2

DNA fragmentation in treated HepG2 cells. DNA laddering visualized in HepG2 cells after 24 h exposed to 50 % ethanol–water crude extracts of D. castanea and L. coromandelica. Untreated cells and 80 μg/mL of melphalan were used as negative and positive controls, respectively

Discussion

The five plants (LC, CT, ES, DC leaves, DC twig, and BA) used in this study are found in northeastern Thailand and were selected based on their ethnopharmacology. All the crude extracts showed significantly lower cytotoxicity than melphalan (P < 0.001, P < 0.001, P < 0.001, P = 0.002, P = 0.023 and P < 0.001, respectively). Based on their cytotoxicity and selectivity classification, the extracts could be categorized as follows: (a) potentially cytotoxic (IC₅₀ < 10 μg/mL) with high selectivity (SI > 3); (b) moderately cytotoxic (IC₅₀ < 100 μg/mL) with high selectivity (SI > 3); (c) moderately cytotoxic (IC₅₀ < 100 μg/mL) with less selectivity (SI < 3); (d) cytotoxic to only normal cells with less selectivity; and (e) nontoxic [32]. Only the crude extract of DC (twig) could be classified as highly cytotoxic toward HepG2 cells and highly selective (SI = 4.5). The SI of this extract was not significantly different from melphalan (P = 0.959). DC (leaf) and other crude plant extracts had moderate cytotoxicity and less selectivity (SI < 3). The LC showed a cytotoxic effect against normal cells with low selectivity (SI < 3). To our knowledge, this study demonstrates for the first time the anticancer potential of LC extract against human HCC (HepG2) cancer cells. The extracts of CT, ES, and BA showed moderate cytotoxicity on HepG2 cells but with less selectivity.

Several chemotherapeutic compounds have been reported to induce apoptosis [36]. In apoptotic cells, specific DNA cleavage is evident on electrophoretic analysis as a characteristic ladder pattern resulting from the multiple DNA fragments of oligonucleosomal size (180–200 bp) [37]. The DNA ladder assay has a lower sensitivity for apoptosis detection [38] because ladder formation can only be clearly observed when the extent of oligonucleosomal cleavage is extensive. Although more than 50 % of the apoptotic cells were observed with the DAPI staining assay in all of the ethanolic plant extracts, only LC and DC were positive according to the DNA ladder assay.

It was necessary to standardize the two potential crude extracts for quality control experiments as 50 % ethanol–water crude extracts of DC (twig) and LC (twig) were used in the current study. We then determined which phytochemicals in the crude extracts were associated with the apoptosis effects using GC–MS analyses.

2-Palmitoylglycerol was the major compound common to the LC (twig) and DC (twig) crude extracts. 2-Palmitoylglycerol is involved in the regulation of endogenous cannabinoid receptor activity by increasing the biological activity of 2-arachidonylglycerol, and inhibition of adenyl cyclase 2-palmitoylglycerol significantly inhibits the inactivation of 2-arachidonylglycerol by neuronal and basophilic cells [39].

2-Arachidonylglycerol inhibits the production of TNF-alpha by mouse macrophages in vitro and the effect is enhanced in the presence of 2-palmitoylglycerol [40]. 2-Palmitoylglycerol is also a key component in modulating pain sensitivity as a result of its ability to interact with endocannabinoids [41]. In the present study, 2-palmitoylglycerol was the one compound found in both DC and LC extracts; however, the 2-palmitoylglycerol content was twice as low in the DC (twig) (7.5 %) than in the LC (twig) (14.0 %) and the DC extracts were more cytotoxic. It was not possible to specifically identify 2-palmitoylglycerol as the key compound; therefore, more detailed chemical identification of the plant extracts is required.

Pyrogallol was predominantly found (18.7 %) in the DC (twig) crude extract, which possessed high toxicity and selectivity against the HepG2 cells. Pyrogallol is a superoxide anion generator because it potently increases intracellular superoxide anion levels and decreases glutathione content in HeLa cells [42]. Research shows that pyrogallol-induced apoptosis resulting from the loss of mitochondrial membrane potential in calf pulmonary artery endothelial cells is accompanied by glutathione depletion [43]. In one study, the apoptosis induction of pyrogallol was indicated by a pyrogallol-type structure in a B-ring of catechins. DNA fragmentation activity was exhibited in a concentration-dependent manner in histiocytic lymphoma U937 cells after treatment with catechins containing a pyrogallol-type structure in a β-ring. Notwithstanding, catechins without a pyrogallol-type structure in any position did not show apoptosis-inducing activity [44]. A 3-O-gallate residue with cis-relationship to the β-ring enhanced the activity and the destruction of a pyrogallol-type structure by its methylation reduced this effect. By contrast, a 3-O-gallate residue in trans-relationship to the β-ring had little effect [44].

DC (twig) crude extract also contained lupeol as the third major compound (5.8 %). In a previous study, two hepatoma cell lines (SMMC7721 and HepG2) treated with lupeol decreased in a concentration-dependent manner (a) cell viability, (b) the induction of active caspase-3 and poly (ADP-ribose) polymerase cleavage, (c) cell accumulation in the S phase, and (d) apoptosis. Treatment with lupeol three times a week also resulted in chemosensitization of hepatoma cells and significantly inhibited tumor growth in nude mice implanted with SMMC7721 cells [45]. Lupeol chemosensitized hepatoma cells synergistically with a PI3-kinase inhibitor (S14161) in both in vitro and in vivo models [46]. In the present study, the lupeol content of the DC (twig) extract (5.8 %) was higher than that of LC (twig) extract (1.0 %). Pyrogallol was the major compound in the DC (twig) extract but not in the LC (twig) extract. These two major compounds might contribute to the high cytotoxicity and high SI of DC (twig) extract as well as the high toxicity with lesser selectivity of LC (twig) extract.

Hexadecanoic acid and octadecenoic acid were also identified as the major compounds in LC (twig) crude extract in this study. The crystal structure (at a resolution of 2.5 Å) and kinetics studies have shown that n-hexadecanoic acid can act as an anti-inflammatory compound by inhibiting phospholipase A₂ in a competitive manner [47]. This fatty acid possibly contributes as the antihepatoma cell potential in the 50 % hydroethanolic herb extracts [13]. Pereira et al. [48] showed that the lipophilic extract from Marthasterias glacialis L. contained mainly palmitic acid and the sterol ergosta-7,22-dien-3-ol: these affected DNA synthesis, lipid droplets, and chromatin condensation, compatible with apoptosis in human breast cancer (MCF-7) and human neuroblastoma (SH-SY5Y) cell lines.

n-Hexadecanoic acid and 9,12-octadecadienoic acid (Z, Z) are fatty acids commonly found in the CO₂ supercritical fluid extraction that mediates apoptosis in human hepatoma SMMC-7721 cells, involving a reactive oxygen species-mediated mitochondrial signaling pathway [49]. The mixture of an octadecenoic acid extract—comprising mainly oleic and linoleic acids—from Euphorbia kansui resulted in a concentration-dependent reduction in the number of human gastric (SGC-7901), HCC (BEL-7402), and leukemia (HL-60) cells and significantly inhibited cell proliferation, with induced apoptosis and G₀/G₁ phase cell cycle arrest [50]. The octadecenoic acids not only caused cell apoptosis/necrosis but also functional and structural damage to the tumor cell membrane and cell ultrastructures [50]. A fraction of the dichloromethane extract of Protaetia brevitarsis larva (composed of at least three free fatty acids: palmitic acid, (Z)-9-octadecenoic acid, and octadecenoic acid) expresses apoptosis-inducing activity as shown by DNA laddering and caspase-3 activation in colon 26 tumor cells [51].

Conclusion

Ethanolic extracts from DC and LC twigs induced apoptosis in the HepG2 cell line. Pyrogallol and lupeol in DC (twig) might be responsible for the cytotoxicity toward the HepG2 cancer cells.