Introduction
Cancer is one of the most vital causes of death worldwide [1, 2]. Its frequency and death rate show its pace of rise in both emerging and developed nations [3, 4]. Cancer incidence is steadily increasing, with 7.6 million deaths in 2008, and it is expected to quadruple by 2030 [2]. Despite enormous expenditure and breakthroughs in cancer treatment, patient survival in many countries has not increased considerably [5]. There is no anticancer treatment that is 100% effective and has no negative effects, according to various publications [2-4]. As a result, there is still a critical need for novel drug development that results in competent anticancer medicines to combat the difficulties associated with chemotherapeutics, such as drug resistance and toxicity [3]. Because of the severe side effects of conventional chemotherapeutics, great emphasis is being placed on plants as natural sources to improve cancer therapy [6, 7]. More than 60% of licenced anticancer medications are natural products or derivatives of natural products; hence, herbs represent a substantial source of anticancer agents [8-11]. Over 3,000 plant species having anticancer activities have been identified as of today [12]. Plant materials are widely utilised across the world because they are more culturally acceptable, have less side effects, and are compatible with the human body [13]. Medicinal plants have traditionally been used to cure a variety of human ailments. The presence of phytochemicals, also known as plant metabolites, is generally the reason for this application [14]. According to several studies, plant anticancer activity is linked to a variety of natural chemicals such as catechins, polyphenols, and flavonoids.
Cleome viscosa is an ethnomedicinalimportant plant that have high traditional nutrient values. The plant isreported to have several bioactive compounds that can work against number ofdiseases. Several chemicals have been extracted from various parts of Cleomeviscosa. Cleome viscose seeds are high in nutrients and include 26%oil, primarily Linoleic acid, palmitic acid, stearic acid, oleic acid, andlinolenic acid, sugar, and seven important amino acids [15, 16]. Methanolicextracts of Cleome viscose leaves has shown excellent antioxidantactivity. The extract is shown to scavenge 43.33% of DPPH free radicals atminute concentration of 0.1 mg/ml [17]. Several studies on the antioxidantactivity of Cleome viscose leaf extract have proved its therapeuticvalue as an antioxidant in a variety of ailments. Many molecules, includingquercetin-3-O-β-D-glucopyranoside 7-O-α-L-rhamnopyranoside [18], cleomeside A,cleomeside B, cleomeside C andquercetin-3-O-[β-D-glucopyranosyl-(1-2)]-α-L-rhamnopyranoside7-O-α-L-rhamnopyranoside exhibit antioxidant and anticancer properties [19].Nevirapine is said to have anti-proliferative properties [20]. Lactam nonaicacid, which is present in roots, has antibacterial and cytotoxic properties[21, 22]. Cleomaldic acid, present in seed and leaves, is said to be cytotoxic[23].
The present study is to determine the antioxidant and anticancer activity of bioactive purified from methanolic Cleomeviscosa leaf extract against BT474 breast cancer cell and MCF10A as anormal cell line.
Material and methods:
MCF10 and BT-474 cell lines were purchased from NCCS, Pune. Leaves of Cleome viscosa were collected fromKhandwa region of Madhya Pradesh, India and was authenticated by Dr. Anamikasingh, Bardhman college, Bijnor. Leaves were washed, surface sterilized with0.1% HgCl2 and dried under shade for 2-3 weeks. Dried leaves weregrounded to fine powder. Powder was then Soxhlet extracted following 4-5 cyclein methanol. Extract was evaporated to dryness and weighed. The dried extractwas diluted in methanol to get a concentration of 500 mg/ml.
Crude extract was screened for their phytochemical constituents qualitatively and quantitatively. Phytochemical like alkaloids, flavonoids, phenolics and tannins were screened following the previous described methods [24]. While quantitative estimation of phenolic and flavonoid content was performed according to method of Singleton et al., 1999 [25] and Pontis et al., 2014 [26] respectively.
Thin layer Chromatography(TLC) of Leaf extract
Thin layer chromatography of extract was performed to evaluate number of phenolics and flavonoid. TLC plates were prepared by weighing ~3 gm of silica gel G and mixing it in 7 to 10 ml of water to make slurry. The slurry was poured over cleaned 7.5*2.5 cm glass slides to make a thin layer of thickness not more than 0.25 mm. The prepared plates were dried at room temperature followed by heating at 90-1000 C to activate silica in hot air oven. TLC chamber wassaturated by solvent system [27] for 15 min. Silica plates were spotted with5-10 µl of extract. Dried the spot. Thesolvent system used for detection of flavonoid and phenolic groups are asfollowed. Solvent system for phenolic: Toluene: Acetone: Formic acid(4.5:4.5:1), Solvent system for flavonoids: n-butanol: Toluene: Ethyl acetate:Glacial Acetic acid (30:40:5). Run and dried the plate. Resolution of extractcomponents was studied by locating different spots on a chromatogram usingFolin-Ciocalteu reagent and sodium carbonate solution for phenolic content; anda mixture of 1% FeCl3 and 1% potassium ferric cyanide forflavonoids. The distance between each spot and its application site wasmeasured and recorded, and the Rf value was determined [28, 29].
Purification of Bioactive compounds
Methanolic extracts were then purified, and the fractions were pre-screened for their anticancer activity.
Column purification of methanolic extract
Crude extract was dried and proceeded for column purification. Column was wet packed using silica gel 60-120 mesh. Silica gel slurry was prepared in hexane and poured over column having hexane solvent. Crude extract dried powdered was mixed with silica gel and poured slowly over the layer of packed silica avoiding disturbance of its layer. Increasing polarity solvent was used to separat compounds in the basis of their polarity. The solvent used for the column purification was according to Bajpai et al., 2016 [30]. With some modifications. Hexane: 20 ml, Hexane: Chloroform (10:1): 22 ml, Hexane: Chloroform (5:1):18 ml, Hexane: Chloroform (1:1): 20 ml, Hexane: Chloroform (1:5): 18 ml, Hexane: Chloroform (1:10): 22 ml, Chloroform: 20 ml, Chloroform: Methanol (10:1): 22 ml, Chloroform: Methanol (5:1): 18 ml, Chloroform: Methanol (1:1): 20 ml, Chloroform: Methanol (1:5): 18 ml, Chloroform: Methanol (1:10): 22 ml, Methanol: 20 ml. Fractions were collected at a constant flow rate. Total 13 fractions were collected. Each of the fractions were screened for the phenolic, flavonoids anticancer activity. The fraction having high phenolic or flavonoid content were proceeded for HPLC purification.
Screening of crude andfraction for their anticancer activity
Anticancer activity of crude and column fractions was estimated by following the protocol of Mossman, 1983 [31].
Isolation of singlebioactive compound by preparative HPLC:
Standards of flavonoids, phenolics and alkaloids (Atropine, Quercetin, Caffeic acid, Gallic acid, Kaempferitrin, Rutin, Nevirapine and Vanillic acid) were prepared at a concentration of 20 µg/ml. Fraction having significant % cytotoxicity against BT-474 was selected for preparative HPLC purification. Bioactive compounds were separated by preparative HPLC according to the protocol of Mansour et al.,2017 [32].All the fractions and standards were filtered through 0.45µm PVDF syringefilters and sonicated at room temperature for 10 min. Preparative HPLC was runon Agilent 1200 series equipped with dual pump and dual wavelength detector.Flow rate was maintained at 18 ml/min. C18 reverse phase column(5µm, 20 mm diameter, 250 mm length) was used. Gradient solvent system forseparation was used. The solvent system was as follow: Solvent A (H2O/0.1%TFA), solvent B (Acetonitrile/0.1%TFA), Solvent A/Solvent B: 99: 1 (0-4 min),Solvent A/Solvent B: 99: 1 (4-12.8 min), Solvent A/Solvent B: 0: 99 (12.8-13min), Solvent A/Solvent B: 10: 100 (13-55 min), Solvent A/Solvent B: 0: 100(55-59 min).
Enlarge this image.Figure 1: Structures of selected alkaloids, flavonoids and phenolic compounds.
Antioxidative assay of purified compounds
The purified compounds were assayed for their antioxidant activity against DPPH and ABTS free radicals. DPPH assay and ABTS assay was performed according to the protocol of Blois, 1998 [33] and Pellegrini et al., 1958 [34] respectively. Briefly all the compounds were diluted to 1 mg/ml concentration and a positive standard of ascorbic acid of same concentration was also prepared for the antioxidant assay.
Cell cytotoxicity and cell proliferation assay of isolated components
HPLC purified samples diluted to 1mg/ml concentrations were than tested for their cytotoxicity and cell proliferation assay. Cell cytotoxicity was estimated by following the protocol of Mossmann, 1983 [31]. Cell proliferation was estimated by trypan dye exclusion assay [35].
Cell cytotoxicity assay
Cells were sub-cultured in 20 ml DMEM media with 10% FBS and incubated in CO2 incubator with5% CO2 and 95% humidity at temperature of 350C. Cell weretrypsinized after 70-80% confluency and proceeded for MTT assay.
2,5-diphenyl-2H-tetrazolium bromide (MTT) assay
Cytotoxicity of purified compounds were estimated by 3-(4,5-Dimethylthiazol-2-yl)-2,5-Diphenyltetrazolium Bromide (MTT) assayfollowing the protocol of Mossmann, 1983. The test samples were diluted in different concentrations of 100, 200, 300, 400, 500, 600 µg/ml concentrations. The diluted samples were mixed together with the cell lines that had been grown for 24 hours in a confluent monolayer plate. After 72 hours of incubation at 37°C in a 5% CO2 incubator, the supernatant wascollected, and 25 µl of MTT reagent (2 mg/ml) was applied to each well.Following a 2-hour incubation period at 37°C, each well received 125 µl ofdimethyl sulphoxide to solubilize the formazan precipitate, and the wells wereagitated for another 15 minutes. At a wavelength of 490 nm, the absorbance wasmeasured using an ELISA reader. The control wells were medium only, DMSOcontrol and Cell control (Well having BT-474 cells) without the examinedchemical.
Where: A0is the absorbance of the Cell (BT-474) control and
A1is the absorbance of the well treated with diluted extracts.
Cell morphology and cellviability (trypan blue dye exclusion assay):
BT474 cell lines were incubated at the IC50 concentrations of the compounds. Six well microplates were seeded with ~3.4*105 cells/ml. Incubated for 24 hrs. in CO2incubator with 5% CO2, 95% air and 99% humidity at 370 C.Incubated with the IC50 concentrations of the compounds for 24, 48 and 72 hrs.After each set of time of incubation, each of wells were examined underinverted microscope for their morphological differences. One control withoutany compound was also set. Cells were trypsin-zed and centrifuged forpelleting. Pellets were dissolved in 1 ml of DMEM media. Briefly 100-200 µl of the cellswere mixed with equal volume of trypan blue (0.4%) and placed onhaematocytometer. Observed under the compound microscope in 10X or 40X andcounted the coloured (dead) and non-coloured (viable) cells. Counted all thefour corners chamber of haematocytometer leaving the middle and below line andcalculated the number of cells/ml using the formula:
Viable count (live cells/ml) = (Number of live cells / numbers of total cells) * dilution*10000
Result
Methanolic extract of Cleomeviscosa leaves were dark green colored and clear. Phytochemical screeningof crude extracts showed presence of phenols, flavonoids, alkaloids and tannins(Table 1). These phytoconstituents act as defence molecule against biotic orabiotic stresses and are categorized into secondary metabolites [36].
Table 1: Phytochemical screening of major phytoconstituents.
| Phtochemical test | Result | |
| Alkaloid | Mayer’s test | ++ |
| Dragendorff’s test | – | |
| Wagner test | + | |
| Flavonoid | ++ | |
| Phenol | + | |
| Tannins | + | |
++, +, – means strongly present, present, and absent respectively.
Total phenolics was estimated to be 0.046 mg/gm (Table 2) which is less than the results of Gupta et al., 2011 [37] and much greater than the findings of Govindan et.al., 2018 [38]. Different phenolic content is due to different solvent used for extraction. Total flavonoids content was 0.042 mg/gm which is greater than the previous findings [37, 38].
Table 2: Total phenolic and total flavonoid content of crudes.
| Test | mg/gm |
| Total phenolic content (mg GAE/gm) | 46±1.56 |
| Total Flavonoid content (mg rutin/gm) | 42.5±3.05 |
Data are represented as mean± Std. dev.
TLC analysis of Cleome viscosa crude for phenolics and flavonoids.
Three flavonoids with Rf value of 0.86, 0.47 and 0.25 were found in the Cleome viscosa leaf extract. Whilenumber of phenolic compounds as observed by peaks numbers are also three withRf values of 0.67, 0.49 and 0.124. TLC plate under long wavelength of UVindicates presence of seven fluorescent compounds with Rf values of 0.751,0.612, 0.338, 0.299, 0.166, 0.114, 0.062. Their intensity indicating theirconcentrations can be observed by bar charts or chromatogram generated throughJustTLC software (Figure 2).
Enlarge this image.Figure 2: Thin layer Chromatography of Cleome viscosa. A: Flavonoids, B: Phenolic, C: Uv (Long wavelength), D: Graph between Volume (Y-axis) and number of spots in each plate, E: TLC profile of each plate (X-axis: Rf, Y-axis: Intensity).
Total of thirteen fraction were collected. Each of the fraction was proceeded for preliminary screening of phenolic and flavonoids along with their anti-cancer activity.
Table 3: Preliminary screening of fractions based on their phenol, flavonoid presence and % cytotoxicity in breast cancer cell line at a fix concentration of 1mg/ml.
| Fraction | Solvent (ml) | Phenols | Flavonoids | % Cytotoxicity at 1mg/ml coc. (BT-474) |
| F1 | H (20) | – | + | 7 |
| F2 | H: Chl (10:1) | – | + | 8 |
| F3 | H: Chl (5:1) | – | – | 10 |
| F4 | H: Chl (1:1) | – | – | 21 |
| F5 | H: Chl (1:5) | + | – | 20 |
| F6 | H: Chl (1:10) | + | – | 17 |
| F7 | Chl (20 ml) | + | – | 27 |
| F8 | Chl: Meth (10:1) | + | + | 18 |
| F9 | Chl: Meth (5:1) | + | + | 14 |
| F10 | Chl: Meth (1:1) | ++ | + | 38 |
| F11 | Chl: Meth (1:5) | +++ | + | 47 |
| F12 | Chl: Meth (1:10) | +++ | + | 49 |
| F13 | Meth (20) | +++ | ++ | 86 |
-, +, ++, +++ indicate absence, presence, moderate presence and strongly present respectively. H: Hexane, Chl: Chloroform, Meth: Methanol solvents.
Out of thirteen fractions only last methanolic fraction having highest phenol and flavonoid presence and maximum percentage cytotoxicity was chosen for preparative HPLC purification of single compound (Table 3).
Preparative HPLC purification ofselected fraction:
The selected methanolic fraction was further HPLC purified to isolate single components.
Enlarge this image.Figure 3: HPLC profile of F13 fraction
HPLC profiling of the F13 fraction indicated the presence of 14 compounds. The compounds were identified by comparing the retention time of each peak with that of standards (Table 4). The identified compounds are tabulated in Table 5. Several bioactive were identified through HPLC profiling of Cleome viscosa leaf extract,including gallic acid, quercetin, catechin, chlorogenic acid, p-hydroxybenzoicacid, coumaric acid, viscosin, kaempferitrin, cleomeolide, nevirapine,cleomiscosin A and B, and several others. [39, 40]
Table 4: Standard phenolic, flavonoid and alkaloids with their retention time, area of peak and response factor.
| Secondary Metabolites | R. T. (min) | Area (mAU) | Response Factor |
| Atropine | 7.124 | 156 | 7.8 |
| Nevirapine | 18.656 | 62.2 | 3.11 |
| Caffeic Acid | 14.852 | 1112.01 | 55.6 |
| Gallic Acid | 16.092 | 1654.02 | 82.7 |
| Quercetin | 7.092 | 204.01 | 10.2 |
| Kaempferitrin | 12.588 | 79.02 | 3.95 |
| Rutin | 13.728 | 1920.02 | 96 |
| Vanillic Acid | 9.968 | 659.02 | 32.95 |
Table 5: Identified secondary metabolites with their retention time, area of peak and concentration.
| Compound | R. T. (min) | Area (mAU) | Conc. (µg/ml) |
| Atropine | 7.124 | 589.21 | 75.54 |
| Unidentified | 8.492 | 1020.02 | |
| Vanillic Acid | 10.184 | 2561.24 | 77.73 |
| Unidentified | 10.788 | 394.551 | |
| Unidentified | 14.052 | 174.942 | |
| Gallic Acid | 15.916 | 222.033 | 2.68 |
| Nevirapine | 18.656 | 790.569 | 254.2 |
| Kaempferitrin | 12.588 | 991.254 | 250.87 |
| Caffeic Acid | 14.808 | 413.563 | 7.44 |
| Unidentified | 16.284 | 193.613 |
Enlarge this image.Figure 4: Structures of isolated major compounds of Cleome viscosa leaf fraction.
Antioxidative activity ofpurified compounds.
DPPH and ABTS scavenging activity of all the purified (known and unknown) were estimated. Rather than ABTS, all the isolated compounds were shown to be more efficient against the DPPH free radical. Kaempferitrin was found to have maximum DPPH scavenging activity with 94% DPPH inhibition. While nevirapine was found to inhibit 76% of ABTS free radicals (Figure 5). The unidentified compounds were not showing effective antioxidant activity.
Enlarge this image.Figure 5: Antioxidant activity of the purified compounds. Data are in mean ± SD. Where n=3.
Anticancer activityand cell cytotoxicity of the purified compounds:
All the compounds were tested against BT-474 cell lines for their potent anticancer activity. Fifty percent inhibitory concentration of all the compounds were calculated. Out of six selected compounds based on their antioxidant activity namely, Atropine, Vanillic acid, Gallic acid, Nevirapine, Kaempferitrin and Caffeic acid only three showed potent anticancer activity and exhibited good cell cytotoxicity against BT474 cell lines. These compounds are Atropine, Vanillic acid and Kaempferitrin with the IC50 values (concentration of compounds that results in 50% cell viability for MCF10A and BT474 cells) values of 18.87, 1.316 and 46.42 µg/ml respectively (Figure 6).
Enlarge this image.Figure 6: Cell cytotoxicity assay of A: Atropine, B: Vanillic acid and C: Kaempferitrin. All the data are in mean ± SD. Where n=3.
Cell morphology andcell viability at IC50 concentration of purified compounds
The BT474 cells treated with the IC50 doses revealed a substantial drop in cell number after 0, 24, 48, and 72 hours of incubation (Figure 7). There was no discernible morphological change between the treated and untreated cell. Cell viability falls dramatically as incubation time increases, with the exception of cells treated with the IC50 concentration of atropine between 24 and 48 hours of incubation, where there is no significant loss in viability with time.
Enlarge this image.Figure 7: A: Cell morphology after treatment of IC50 concentration of purified compound after 72 hrs of incubation. B: Graph showing cell number (cell/ml) after treatment with compounds at different time of incubations.
Conclusion
Cleome viscosais anethnomedicinal significant plant with a large number of potent bioactives thatcan help with a variety of diseases. Atropine, vanillic acid, gallic acid,nevirapine, kaempferitrin, caffeic acid, along with some unidentifiedcompounds, were purified from the methanolic extract of Cleome viscosaleaves. Kaempferitrin was found to have maximum antioxidant activity. All ofthe purified compounds having significant antioxidant activity also havepotential anticancer activity against breast cancer cell lines, but threecompounds, namely Atropine, Vanillic acid, and Kaempferitrin, have maximum cellcytotoxicity against the breast cancer cell line. From the results, it wasconcluded that isolated Kaempferitrin has good antioxidant and anticanceractivity. Although Atropine has a high anticancer activity, it has a lowantioxidant capacity.
Acknowledgement
I acknowledge ChemGeneics research foundation, Noida to let me use their lab and facility. I acknowledge Dr. Anamika Singh to help in authenticating the plant.
Conflictof interest
The authors state that they have no financial or other conflicts of interest.
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