Anti-proliferative, antioxidant effects of methanol extract of Calotropis procera leaf on lung cancer cells (H1299) and its ameliorative effect on expression of CD146 on blood cells
Calotropis procera leaf is one of the plants commonly utilized in phytomedicine in Nigeria. The present investigation explored the use of the extracts on cell viability and apoptosis respectively. In this study, the expression of the Cluster of differentiation 146 (CD146) in the blood of lung cancer patients on regulatory T cells (Tregs) was determined. The antioxidant and anti-proliferative effects of methanol extracts of Caloropis procera leaf on lung cancer cell H1299 were investigated.
Methods
From the flow cytometry, the expression of the CD146+ in the T cells were evaluated using the healthy patient, adenocarcinoma, squamous, and small cell lung cancer respectively. The apoptosis of granulocytes, monocytes, lymphocytes, CD4+, and Treg were determined by 7-amino-actinomycin D/Annexin V-Allophycocyanin (APC) staining during the resting stage and after 24 h respectively. Immunofluorescence was conducted. Cell viability assay, hydroxyl (OH), hydrogen peroxide (H2O2) and nitric oxide (NO) scavenging radicals were conducted. Reducing power and flavonoid content of Calotropis procera were investigated. The effect of the Calotropis procera at different concentrations at 24hrs was determined.
Results
From the flow cytometry, the expression of the CD146+ on the T cells includes 4.60 % in healthy patients, 10.10, 12.20, 9.80 % in adenocarcinoma, squamous and small cell lung cancer. The apoptosis of granulocytes, monocytes, lymphocytes, CD4+ and Treg were determined by 7-amino-actinomycin D/Annexin V-APC staining during the resting stage and after 24 h which indicate that apoptosis also occurred on Treg. Immunofluorescence shows the presence of CD146 in lung cancer patient’s tissues. The methanol extracts of Calotropis procera leaf have antioxidant and anti-proliferative effects. Methanol extract of Calotropis procera leaf reduced CD146 expression on blood cells at 24 h.
Conclusion
Increased CD146 expression in the Treg of lung cancer patients indicates that it may be a possible target for the treatment of lung cancer by utilizing potent immunotherapy or natural products such as methanol extract of Calotropis procera leaf which may ameliorate the expression of CD146. Calotropis procera has antioxidant, inhibitory capacity on H1299 lung cancer cells, and the ability to scavenge OH, H2O2, and NO radicals. Hence, this investigation strengthens the phyto-medicinal properties of Calotropis procera.
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Lung cancer is a fatal and deadly disease with poor prognosis [1]. It has a variation of histological subtypes, and is the most disastrous cancer globally. The major causes of lung cancer are still debatable. Particulate matter in air pollution with diameter less than 10 μm (PM10) and 2.5 μm (PM2.5) [2], smoking, genetic factors, infections, occupational exposure are some of the possible factors causing lung cancer. The incidence of lung cancer is increasing worldwide striking an excessive danger to human well-being [3]. It is projected that 2.09 million different circumstances of lung cancer happened worldwide in 2018, position first amid all cancer forms [4]. In some industrialized nations, such as Austria and Germany, lung cancer is one of the most common cancers [5]. In the United States lung cancer prevalence has reduced, mostly in current years, comparatively due to the outcome of active tobacco control and health tutelage and promotion agencies. Remarkably, lung cancer occurrence is comparatively little in both male and female in Africa, which may be correlated to low life expectancy [6]. Lung cancer is more widespread in men, both in global and in most countries. Lung cancer is presently the prominent reason of cancer mortality approximately 20 % of all cancer mortality. Lung cancer death in China is moderately high compared to most countries. It is predictable that lung cancer death in China may rise by about 40 % between 2015 and 2030 [7]. Therefore, it is important to unravel a novel biomarker and therapeutic target to ameliorate prevalence and death.
Immunotherapy specifically may be a possible strategy promising to reduce the occurrences and mortality of lung cancer [8]. However, the realization of such therapy has been inadequate up to these days, perhaps because of features of the tumor. Antitumor response of most patients is not adequate. Regulatory T cells (Tregs) have engrossed considerable attention, because of their important functions of immunosuppression of self-antigen response [9, 10]. T cells (Tregs) denote about 4–5 % of the CD4+ T cells. They are important for the avoidance of autoimmunity and preform developing roles in cancer immunology [11, 12]. Different investigations have been conducted, which revealed an increased in the Treg in the cancer patients [13‐15]. This may promote tumor progression, metastasis and poor prognosis [13].
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CD146 is a multipurpose molecule that is associated to numerous molecular, biochemical, and pathophysiological processes relating to therapeutic, immune system, stem cell differentiation, signal transduction [16, 17] and angiogenesis [18, 19]. Currently, different researchers discovered that CD146 overexpression meaningfully correlate with the metastasis, progression and formation of new blood vessels of some malignant tumors which was studied in prostate cancer, melanoma, ovarian carcinoma esophageal cancer, gallbladder adenocarcinoma, and lung cancer [20‐26].
Calotropis procera is a very unique plant which is commonly found in Africa, Asia and Middle East. It had been widely used in alternative medicine to ameliorate and treat different diseases because of its pharmacologically active compounds revealed in the plant’s parts, leaves, flowers, roots, and its milky latex [27, 28]. C. procera had been explored to comprise of some vital compounds which includes anthocyanins, trierpenoids, norditerpenic esters, organic acid, cysteine protease procerain, phenol, alkaloids, flavonoids, cardenolides [29, 30]. The phytocompounds are known to be important in eradicating and ameliorating various diseases [31]. C. procera has different parts which are known for medicinal benefits to mankind. It is useful as analgestic, antispasmodic, anti-inflammatory, antimalarial, and hepatoprotective [29, 32‐34]. Hence, this investigation unravels the possible antioxidant, anti-proliferative and immunotherapeutic effects of methanol extract of C. procera leaf by reduction of the expression of CD146 on the Treg.
Materials and methods
Materials
3-(4,5-Dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT), dimethyl sulfoxide (DMSO), propidium iodide (PI) Rnase, The Annexin V-FITC apoptosis detection kit and Cell cycle kit were purchased from KeyGEN Biology Co. Ltd (Nanjing, China). CD146 monoclonal antibody was purchased from thermofisher scientific (USA).
Cell culture
The human HCC cell lines H1299 was obtained from the China Center for Type Culture Collection (CTCCC, Wuhan, China). The cells were maintained in DMEM medium supplemented with 10 % fetal bovine serum and 1 % ampicillin and streptomycin incubated in a humified atmosphere at 37oC under 5 % CO2.
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Flow cytometry for detection of CD146
Blood samples were collected from patients which include healthy patients, adenocarcinoma, squamous lung cancer and small cell lung cancer patients respectively and the flow cytometry was used to detect the percentage of the CD146 expression on the Treg (CD4+, CD25+, CD127 dim/-) respectively. Monocytes, lymphocytes and granulocytes percentage were also determined.
Determination of Apoptosis
Blood samples were also used to the detection of the apoptosis of the lymphocytes, monocytes, granulocytes during 0 and 24 h respectively using the Annexin- V and 7AAD. The Treg apoptosis was also conducted to verify may be there was apoptosis in the Treg.
Immunofluorescence of normal and lung cancer patient’s tissues
Paraffin-embedded lung tissue Secs. (5-µm thick) were deparaffinized in xylene and rehydrated in a graded ethanol series to PBS (pH 7.2). Antigen retrieval was performed by pressure cooking of lung sections in citrate buffer (pH 6.0) for 15 min. Immunofluorescence staining of lung sections was performed using primary antibodies E-caderin polyclonal antibody (20874-1-AP). After overnight incubation, slides were washed and incubated with the respective secondary antibodies, Alexa 488 (Dylight 488, Goat Anti Mouse IgG (H + L) E032210 EarthOX) conjugated secondary antibodies for 1 h. All sections were counterstained with nuclear 4′,6-diamidino-2-phenylindole (DAPI) and mounted with fluorescent mounting medium. Images were taken using a confocal laser scanning microscope (Olympus FLUOVIEW FV 1000) with an Olympus IX81 digital camera.
Preparation of methanol extract of Calotropis procera leaf
C. procera leaf was harvested from Ikare-Akoko, Ondo State in Nigeria in the beginning of the rainy season. It was authenticated at the Department of Botany; University of Ibadan and the voucher specimens were deposited at the herbarium (UI00167). Clean tap water was used to eliminate dirty materials and was air dried in the laboratory for several weeks. The dried materials were ground into coarse powder. About 1 kg of each powdered plant materials were soaked with 2.5 L of methanol for 96 h with intermittent stirring for cold extraction. The extracts were filtered via muslin cloth and evaporated to dryness at 40 °C with rotary evaporator. The dried extracts were preserved in an air-tight container inside and frigerated until use.
Determination of flavonoid content of Calotropis procera leaf
The total flavonoid content was determined with a colorimetric method described by Jia et al. [35] with some modifications. Briefly, between 10 and 1000 µg of the extract in 1 mL of distilled water was added to 75 µL of 5 % NaNO2.After five minutes, 150 µL of 10 % followed by 500µL of 1 M NaOH and 275 µL of distilled water. The solution was properly mixed and the colour intensity of the mixture read at 510 nm after 15 min while catechin served as standard.
Methanol extract of Calotropis procera leaf reduced CD146 expression on blood cells at 24 h
Methanol extract of C. procera leaf was prepared into different concentrations 0 ug/ml, 0.5 ug/ml, 1.0 ug/ml and 1.5 ug/ml respectively and used on the healthy patient blood samples for 24 h in CO2 5 % incubator. RPMI 1650 media with 10 % FBS was used as the media and for the dilution of the extract. The effects of the C. procera on the Treg, CD146+, CD4+, monocytes, granulocytes and lymphocytes were determined respectively (Fig. 1).
Fig. 1
Methanol extract of Calotropis procera leaf reduced CD146 expression on blood cells at 24 h. CP was used on the blood cells and we discovered that it reduced the expression of CD146, increased the expression of CD4+ and dose dependent. It shows that CP may be an immunotherapy
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Determination of the reducing power
Reducing power was investigated utilizing the protocol of according Oyaizu [36]. The concentration range was 1.0 mL of plant extract and catechin (10 − 1000 ug/mL). It was mixed with phosphate buffer (pH 6.6) and potassium ferricyanide. The mixture was incubated at 50 °C for 20 min and trichloroacetic acid (10 %, 2.5 mL) was added to the mixture. A portion of the resulting mixture was mixed with ferric chloride [FeCl3] (0.1 %, 0.5 mL) and the absorbance was measured at 700 nm in a spectrophotometer manufactured by Trulab India. Higher absorbance of the reaction mixture indicated reductive potential of the extract.
Determination of H2O2 scavenging radical
The capability of C. procera leaf extract to scavenge hydrogen peroxide was determined according to the methods of Nabavi et al. [37]. A solution of hydrogen peroxide (40 mM) was prepared in phosphate buffer (pH 7.4). The concentration of hydrogen peroxide was determined by absorption at 230 nm using a spectrophotometer. Extracts (0.1 − 1 mg/mL) in distilled water were added to a hydrogen peroxide solution (0.6 mL, 40 mM). The absorbance of hydrogen peroxide was determined after 10 min against a blank solution containing phosphate buffer without hydrogen peroxide. The percentage of hydrogen peroxide scavenged by the extracts and standard was calculated as follows:
Where Ao is the absorbance of the control and A1 is the absorbance in the presence of the extracts or standard.
Nitric oxide radical scavenging assay
The scavenging effect of the extract on NO radical was measured according to the method of Ebrahimzadeh et al. [38]. Briefly, 1 mL of sodium nitroprusside (5 mM) in phosphate buffered saline (PBS) was mixed with different concentrations of extracts and distilled water. The concentration range was 1.0 mL of plant extract and catechin (10 − 1000 ug/mL). This was incubated at room temperature for 150 min after which 0.5 mL of Griess reagent was added. The absorbance of the pink chromophore formed was read at 546 nm in a double beam UV visible spectrophotometer manufactured by Trulab India. Catechin was used as positive control. The percentage inhibition was calculated as:
The hydroxyl scavenging activity of extracts was conducted using the procedures of Halliwell [39]. The assay was performed by addition of 0.1 mL of EDTA, 0.1 mL of hydrogen peroxide (H2O2), 0.36 mL of deoxyribose, 1.0 mL of plant extract (10 − 1000 ug/mL), 0.33 mL of phosphate buffer (50 mM, pH 7.4) and 0.1 mL of ascorbic acid in sequence. The mixture was then incubated at 37 °C for 1 h. About 1.0 mL of 10 % TCA and 1.0 mL of 0.5 % TBA were added to develop the pink chromogen which was measured at 532 nm in a double beam UV visible spectrophotometer(Trulab India) [40].
Cell viability assay
The effects of CP on cell viability were assessed by using MTT assay. Concisely, a number of 2–5 × 10− 3 cells of H1299 per well in 100 mL were seeded in 96-well plates 24 h before the experiment and then 100 mL of medium with various concentrations of extract (0, 5, 10, 20, 40, 80 ug/ml) added and incubated for 48 h. Then 20 mL of MTT (5 mg/mL) was added to each well and incubated for an additional 2–4 h. The medium was removed and 150 mL DMSO was added to dissolve the formazan crystal. The absorbance of each well was measured using a Spectra Max M5 microplate spectrophotometer (Molecular Devices) at 570 nm wavelength. Each assay was repeated 3 times.
The effect of apoptosis of CP was determined utilizing the Annexin V-FITC apoptosis detection kit. Cells were incubated with Annexin V-FITC and PI for 15 min in the dark then the stained cells were detected by FCM and the data were analyzed with FlowJo software.
Statistical analysis
Experimental results were expressed as mean ± standard deviation (SD). All measurements were replicated three times. The results were analyzed with Statistical Package for the Social Sciences (SPSS) version 20 using one-way analysis of variance (ANOVA). The level of significance used was p < 0.05.
Results
CD146 in healthy and lung cancer patients’ blood
The expression of CD 146 + was significantly higher in patients than in controls (P < 0.05). The flow cytometry was used for the investigations which showed that the expression of the CD 146 + in the T cells includes 4.60 % in healthy patients, 10.10 %, 12.20 %, 9.80 % in adenocarcinoma, squamous and small cell lung cancer respectively (Fig. 2; Table 1).
Fig. 2
CD146 expression on T cells in lung cancer patients. From the flow cytometry, the expression of the CD 146+ in the T cells includes 4.60 % in healthy patients, 10.10 %, 12.20 %, 9.80 % in adenocarcinoma, squamous and small cell lung cancer respectively
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Table 1
Expression of CD146 on Treg in healthy and lung cancer patients showing number of patients
Healthy Patients
Adenocarcinoma
Squamous
SCLC
Expression of CD146 in Treg (%)
4.60
10.10
12.20
7
No of Patients
11
9
5
7
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Immunofluorescence of normal and lung cancer patient’s tissues
Immunofluorescence of normal and lung cancer patient’s tissues indicate the presence of CD146 in the lung cancer patient’s tissues (Fig. 3).
Fig. 3
CD146 expression on T cells in lung cancer patients. From the flow cytometry, the expression of the CD 146+ in the T cells includes 4.60 % in healthy patients, 10.10 %, 12.20 %, 9.80 % in adenocarcinoma, squamous and small cell lung cancer respectively
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Flavonoid content of Calotropis procera leaf
The flavonoid content in the C. procera leaf was determined using colorimetric technique. It was found that at 1000 ug/ml of CP, it has some flavonoid compared to catechin (standard) Fig. 4.
Fig. 4
Flavonoid content of Calotropis procera leaf. It revealed that at 1000 ug/ml, the flavonoid content was similar to the standard catechin. Data are expressed as mean ± SD (n = 4)
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Apoptosis was conducted to verify the cell death
Apoptosis was conducted in the different blood cells. The cells include lymphocytes, monocytes, granulocytes, CD4 + and Treg. It was observed at the resting stage Fig. 5a and after 24 h Fig. 5b. It was verified that apoptosis also occurs in the Treg cells.
Fig. 5
a Apoptosis of lymphocyte, monocytes, granulocyte, CD4+ and Treg at 0h. A= CD45 APC-cy7-A Vs SSC-A, B=FSC-A Vs CD4 V450-A, C= CD127 APC-A Vs CD25 PECy7-A, D= Apoptosis of Lymphocytes, E= Apoptosis of Monocytes, F= Apoptosis of Granulocytes, G=Apoptosis of CD4+, H= Apoptosis of Treg. b Apoptosis of lymphocyte, monocytes, granulocyte, CD4+ and Treg at 24 hrs. A= CD45 APC-cy7-A Vs SSC-A, B=FSC-A Vs CD4 V450-A, C= CD127 APC-A Vs CD25 PECy7-A, D= Apoptosis of Lymphocytes, E= Apoptosis of Monocytes, F= Apoptosis of Granulocytes, G=Apoptosis of CD4+, H= Apoptosis of Treg
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Reducing power
Figure 6 shows the dose-response curves for the reducing powers of the extract. It was found that the reducing powers of the extract increased with the increase of its concentration. The extract showed very high activity. The reducing power of extract was comparable with catechin at 1000 ug/ml.
Fig. 6
Reducing power assay of Calotropis procera leaf. It revealed that at 1000 ug/ml, the reducing power was similar to the standard catechin. Data are expressed as mean ± SD (n = 4)
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NO Scavenging Radicals of Calotropis procera leaf
The NO scavenging activities of CP are shown in Table 2. It elicited dose-dependent and significant scavenging of NO in vitro. The NO scavenging effect of CP was similar to that of catechin from 250 − 1000 µg/mL.
Table 2
NO scavenging Radical of Calotropis procera leaf
Percentage Inhibition
Conc (ug/ml)
Catechin
CP
Control
0.00 ± 0.00
0.00 ± 0.00
10
13.1 ± 1.22*
2.90 ± 0.05*
50
26.9 ± 2.16*
5.20 ± 0.12*
100
54.5 ± 1.58*
20.0 ± 0.80*
250
71.5 ± 3.28*
50.0 ± 0.10*
500
78.7 ± 3.99*
70.0 ± 0.20*
750
88.2 ± 2.83*
72.0 ± 0.30*
1000
82.4 ± 3.20*
75.0 ± 0.20*
Data are expressed as mean ± SD (n = 4); *significantly different from control (p < 0.05)
Where CP = Calotropis procera leaf
OH scavenging radicals of Calotropis procera leaf
Table 3 shows the OH scavenging activity of CP. At concentration of 100 ug/ml, 250 ug/ml, 500 µg/mL, 750 ug/ml and 1000 ug/ml the scavenging activities of CP was 68 %, 70 %, 75 %, 77 and 80 % respectively. While that of the standard (catechin) was 61 %,70 %, 76 %, 81 %, 85 % respectively. It indicates that CP had OH scavenging radical activities similar to catechin.
Table 3
OH scavenging Radical of Calotropis procera leaf
Percentage Inhibition
Conc (ug/ml)
Catechin
CP
Control
0.00 ± 0.00
0.00 ± 0.00
10
46.1 ± 3.22*
50.0 ± 1.00*
50
55.1 ± 1.74*
60.0 ± 1.24*
100
61.9 ± 0.4*
68.0 ± 0.05*
250
70.4 ± 1.59*
70.0 ± 2.66*
500
78.6 ± 1.19*
75.0 ± 1.00*
750
81.4 ± 2.02*
77.0 ± 0.05*
1000
85.1 ± 2.05*
80.0 ± 0.10*
Data are expressed as mean ± SD (n = 4); *significantly different from control (p < 0.05)
Where CP = Calotropis procera leaf
H2O2Scavenging radical of methanol extract of Calotropis procera leaf
Table 4 indicates that C. procera leaf scavenged H2O2 radical successfully. At concentration of 500 µg/mL, 750 ug/ml and 1000 ug/ml the scavenging activities of CP was 77 , 78 and 85 % respectively. The scavenging activity for the standard (catechin) was 75.7, 78.2 and 80.4 % respectively. It indicates that CP effectively H2O2 scavenging radical activities at 85 % which was higher than catechin.
Table 4
H2O2 Scavenging Radical of methanol extract of Calotropis Procera leaf
Percentage Inhibition
Conc (ug/ml)
Catechin
CP
Control
0.00 ± 0.00
0.00 ± 0.00
10
13.1 ± 1.22*
3.50 ± 0.65*
50
20.9 ± 0.16*
4.20 ± 0.22*
100
44.5 ± 0.58*
31.0 ± 0.90*
250
61.5 ± 2.18*
55.0 ± 0.30*
500
75.7 ± 1.99*
77.0 ± 0.50*
750
78.2 ± 0.83*
78.0 ± 0.20*
1000
80.4 ± 2.20*
85.0 ± 0.10*
Data are expressed as mean ± SD (n = 4); *significantly different from control (p < 0.05)
Where CP = Calotropis procera leaf
Methanol extract of Calotropis proceraleaf reduced CD146 expression on blood cells at 24 h
The effects of the CP on the Treg, CD146+, CD4+, monocytes, granulocytes and lymphocytes were determined respectively. The result shows that CP at 1.5 ug/ml CD146 reduced while CD4 + increased. Hence, CP may be a potent immunotherapy.
MTT assay
MTT assay was conducted to unveil the ability of Calotropis procera leaf extracts to inhibit the cell proliferation. Here, at 40 ug/ml CP inhibit the cell effectively and the cell inhibition proliferation was dose dependent. Figs. 7 and 8.
Fig. 7
Cell viability of H1299 cell line using methanol extract of Calotropis procera leaf. Data are expressed as mean ± SD (n = 3)
Fig. 8
Representation of Treg unveils activities of CD146, Calotropis procera and apoptosis
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Discussion
CD146 is an important molecule which is a possible biomarker and therapeutic target. It can be found in different types of cells which include lymphocytes, pericytes, immune cells, alveolar sheet and endothelial cells etc. This investigation indicates a possible means by which CD146 may be a biomarker for the detection of lung cancer in patients. Here, we use the flow cytometry to determine the different percentage of CD146 in healthy, adenocarcinoma, squamous and small cell lung cancer patients. Increased in the proportion of CD146 in lung cancer patients is in line with previous investigations [41‐43]. Apoptosis conducted in the study shows that it does not only occur on the CD4 + cells but apoptosis also occurs on the Treg. The immunofluorescence shows that CD146 is presence in lung cancer patient’s tissues.
Flavonoid was present in the C. procera leaf which makes it a potential antioxidant. It has been investigated by previous researcher that CP may be a potential therapeutics [27]. Flavonoids are responsible for numerous varieties of pharmacological activities and involve huge collection of polyphenolic compounds having a benzo-γ-pyrone structure and universally exist in plants. They are produced by phenylpropanoid pathway [44, 45]. In the reducing power assay, the appearance of reductants (antioxidants) would lead to the reduction of iron (III) [Fe3+] to iron (II) [Fe2+] by donating an electron which serves as a significant indicator of antioxidant activity [46]. The result indicates that the C. procera leaf shows reducing power at 1000 ug/ml which is similar to that of catechin.
Nitric oxide is a very important intracellular and intercellular controller of multiple biological functions, including macrophage-mediated cytotoxicity for tumor cells, smooth muscle cells and responsible for sensory transmission [47, 48]. Previously, nitric oxide was believed to have only advantageous characteristics, but it is now identified that overproduction of NO is associated with various pathological diseases, such as pulmonary hypertension, septic shock, cirrhosis, chronic inflammation, brain inflammation and cancer [49]. The NO radicals play an important role in inducing inflammatory response in the lungs and brain which can be highly toxic and their toxicity increases when they react with superoxide radicals to form peroxynitrite which harms the biomolecules [50]. NO is produced by three isoforms of the enzyme nitric oxide synthase (NOS), neuronal NOS, endothelial NOS, and inducible NOS (iNOS). In this investigation, the NO radical scavenging activity was based on the principle that sodium nitroprusside in an aqueous solution at physiological pH spontaneously generates NO, which interacts with oxygen to produce nitrite ions that can be estimated using a Griess reagent. Scavengers of NO act against oxygen, leading to reduced production of nitrite ions which can be monitored at 546 nm. The results indicate that the methanol extract of C. procera leaf tested, successfully scavenged NO radical in vitro; CP revealed dose-dependent NO scavenging capabilities which were similar to that of catechin in all the tested concentrations.
Hydroxyl radicals can be produced by biochemical reaction in which superoxide radical is transformed by superoxide dismutase to hydrogen peroxide, which can then produce exceedingly reactive hydroxyl radicals in the presence of divalent metal ions, such as iron and copper. Thus, elimination of the hydroxyl radical is probably one of the most active defenses of a living body against various diseases such as lung cancer. In this study, we demonstrate that C. procera leaf had considerable hydroxyl radical scavenging activity when compared with standard antioxidant (catechin) and could serve as an anticancer agent by inhibiting the interaction of hydroxyl radical with DNA. The result from this study indicates the effectiveness of extracts from C. procera leaf successfully scavenge HO radical in vitro. The HO radical scavenging activity of CP was high and statistically similar to catechin. Hence, it is a very good antioxidant which may be useful to combat carcinogenesis.
Hence, we utilized the C. procera leaf on the blood cells and it unveiled that it may ameliorate the expression of CD146. This may be due to the fact that it is a good antioxidant and may have the possible immunotherapy effects for the reduction of the CD146 which may serve as a good biomarker and therapeutic target of great significance. The capability of C procera to inhibit cancer cell line was unraveled utilizing H1299. Thus, H1299 was used for this study because of the prevalence of adenocarcinoma lung cancer in most of the patients admitted, which may be useful as a novel drug candidate that can be used for the treatment of the disease. The results show the anti-proliferative and hydrogen peroxide scavenging radical capability of C. procera. Hydrogen peroxide is a reactive oxygen radical and, at increased concentration, may become toxic and injure cells and tissues when it is changed into hydroxyl radical which can start lipid peroxidation and DNA alteration [51]. The investigation unveils the capability of the methanol extract of C. procera leaf to successfully scavenge H2O2 radical in vitro. The H2O2 radical scavenging activities of C. procera were similar to catechin. The cell viability shows that C. procera was able to inhibit H1299 cancer cell lines effectively and it was dose dependent which indicates that it is a potential drug candidate which could be used to ameliorate lung cancer. Hence, CP is very effective for the amelioration of cancer which can serve as an anti-cancer therapy in the nearest future.
Conclusions
Increased CD146 expression in the Treg of lung cancer patients indicate that it may be a possible target for the treatment of lung cancer by utilizing potent immunotherapy or natural products such as methanol extract of C procera leaf that may ameliorate the expression of CD146. It is also a potential biomarker and therapeutic target of clinical significance in lung cancer patients. This study establishes antiproliferative effects of C. procera via decrease in cell viability, and capability to scavenge OH, NO2 and H2O2 radicals. Hence, this investigation strengthens the phyto-medicinal properties of C. procera. This investigation also shows that more study is required on molecular mechanisms underlying the effect of methanol extracts of C. procera, angiogenic, and other signaling pathways before isolation and characterization of active components.
Acknowledgements
We thank Henan Provincial People Hospital and National Natural Science Foundation for financial support and fellowship.
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Compliance with ethical guidelines.
Consent for publication
Not applicable.
Competing interests
The authors declare that they have no competing interests.
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Anti-proliferative, antioxidant effects of methanol extract of Calotropis procera leaf on lung cancer cells (H1299) and its ameliorative effect on expression of CD146 on blood cells
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Ayobami Matthew Olajuyin Adefunke Kafayat Olajuyin Ziqi Wang Xingru Zhao Zhiwei Xu Quncheng Zhang Xiaoju Zhang
