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This is an open access article distributed under the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

1. Introduction

Parthenium hysterophorus L. (Asterales, Asteraceae, Linn) is a flowering plant and an aggressive ubiquitous annual herbaceous weed belonging to the family Asteraceae. P. hysterophorus is commonly known as altamisa, bitter weed, white top, and carrot grass. The flowering of this plant occurs throughout the year [1, 2]. P. hysterophorus thrives in Pakistan, America, Africa, Asia, as well as in Australia. It has multi medicinal traditional usage such as for the treatment of fever, neurologic disorders, diarrhea, dysentery, malaria, urinary tract infections, allergic respiratory problems, mutagenicity in humans, and emmenagogue. In addition, P. hysterophorus has been employed in traditional medicine as a remedy for inflammation and rheumatism, and as an analgesic in muscular rheumatism [3]. This plant is rich in active compounds which are responsible for its use in traditional medicine. However, P. hysterophorus is not well-explored for its phytochemical constituents. Therefore, research is required for the isolation, purification, and structure determination of active constituents of this plant. P. hysterophorus has been reported to contain toxins called sesquiterpene lactones such as the glycoside parthenin [4]. Other phytotoxic compounds or allelochemicals present in this plant are hysterin, ambrosin, and flavonoids such as fumaric acid, quercetagetin 3,7-dimethylether, p-coumaric, p-hydroxybenzoin, vanillic acid, chlorogenic acid, anisic acid, ferulic acid, and various alcohols [5]. Ether and ethyl acetate fractions of P. hysterophorus have led to the isolation of fourteen compounds and some of them having cytotoxic potential [6]. A novel hydroxyproline-rich glycoprotein has been documented from the pollen of P. hysterophorus [7]. Another novel sesquiterpenoid, charminarone, has also been previously reported [8–10]. On the basis of the above-mentioned information, there is a need to fully explore the medicinal potential of P. hysterophorus, and to extract and isolate more active phytochemicals that rationalize its properties and pharmaceutical applications. The present study is an attempt to evaluate the in vitro enzyme (urease, α-glucosidase, and phosphodiesterase) inhibition assays, in vivo analgesic, anti-inflammatory, and sedative effects of the various fractions of P. hysterophorus.

2. Material and Methods

2.1. Plant Collection and Drying

Plant material of P. hysterophorus was collected from various areas of the University of Swabi, Anbar, K.P., Pakistan. The plant specimen was validated by a botanist in the Department of Botany, University of Swabi KP, Pakistan, and voucher specimen NO. BOT.UOS4 was deposited in the said department. The plant material was dried under shade at room temperature and on the ground to obtain a powder for extraction.

2.2. Extraction and Fractionation

The obtained P. hysterophorus powder material was subjected to cold extraction using a polar organic solvent such as methanol or ethanol, distilled water, and n-hexane. The extract was concentrated by means of a rotary evaporator at a low temperature (50–55°C). This was followed by fractionation using organic solvents of different polarities such as Hexane, CHCl₃, EtOAc, and methanol (×3 for each). The extract was then suspended with the minimum amount of water, followed by the addition of different organic solvents starting from nonpolar (n-hexane) to more polar ones such as chloroform, dichloromethane, ethyl acetate, and butanol, respectively. Each collected fraction was concentrated under a vacuum by using a rotary evaporator at a low temperature (50–55°C) to obtain a crude fraction. The crude extracts and fractions were subjected to phytochemical screening before bulk extraction. Finally, the obtained crude extracts and fractions were subjected to in vitro and in vivo biological assays.

2.3. Phytochemical Screening

A phytochemical screening test of extracts/fractions was carried out for identification of active phytochemicals as per reported procedures [11–15].

2.4. In Vitro Enzyme Assays

2.4.1. Urease Inhibition Activity

The urease inhibition activity of the crude extracts and fractions was performed by spectrophotometry in 96-well plates as per the standard method [16]. 5 µL of crude extracts and their fractions (0.5 mM) and 25 µL urease catalyst (1 U/well) were hatched for 15 minutes at 30°C. Then, 55 µL substrate urea (100 mM) was re-brooded at 30°C for 15 minutes. After completion of incubation, 70 µL of alkali reagents (0.1% sodium hypochlorite) and 45 µL of phenol (0.005% w/v, sodium nitroprusside and 1% w/v phenol) were mixed. The incubation of the plates was again performed for 50 minutes at 30°C. The urease screening test was periodically done with continuous urea hydrolysis and ammonia production. The change in absorbance (optical density (OD)) was monitored at 630 nm on an ELISA plate reader (Spectra Max M2, Molecular Devices CA, (USA).

2.4.2. α-Glucosidase Inhibitory Assay

The rat intestinal (CH₃)₂CO (acetone) powder in normal saline (100 : 1; w/v) was sonicated appropriately, and the supernatant was used as a source of basic intestinal α-glucosidase after centrifugation [17]. Shortly, 10 mL of the prepared extract and its isolated fractions of 5 mg/mL in DMSO solution was reconstituted in 100 mL of 100 mM phosphate buffer (pH 6.8) in 96-well microplates. The hatching was done in 50 mL of essential intestinal α-glucosidase for 5 min before 50 mL of substrate (5 mM p-nitrophenyl-a-D-glucopyranoside (p-NPG) was arranged in the similar buffer) was included. The α-glucosidase-mediated conversion of p-NPG into D-glucose and p-nitrophenol at 405 nm was monitored spectrophotometrically every 5 minutes. Singular seats for the screening extract were set up to extract baseline absorbance of the substrate and altered with 50 mL of buffer. The control sample contained 10 mL DMSO alongside screening samples. The percentage of enzyme inhibition was assessed as follows: $\begin{matrix} (1) & 1 - \frac{B}{A} \times 100, \end{matrix}$ where A speaks to the absorbance of the control exclusive of the prepared extract sample, and B connects to absorbance in the attendance of test samples.

2.4.3. Phosphodiesterase Inhibitory Assay

This enzyme assay was performed using snake venom-derived PDE-1 (Sigma P-4631), adopting already published methods with some modifications [18]. 30 mM Mg-acetate and 33 mM Tris-HCl buffer (pH = 8.8) were mixed as a cofactor with 0.000742 U of enzyme in 96-well plates, then 0.33 mM bis (p-nitrophenyl) phosphate (Sigma N-3002) was added as a substrate. Ethylenediaminetetraacetic acid (EDT, E. Merck, Germany) was used as a standard drug. The inculcation was achieved for 30 minutes and the enzyme screening was examined at 37°C using a microtiter plate reader spectrophotometer, by the subsequent discharge of p-nitrophenol from p-nitrophenyl phosphate at 410 nm. All the screening tests were done in triplicate and the initial rates were calculated as the rate of changes in the OD/min (optical density/Min) and then used in the following calculation: $\begin{matrix} (2) & % Inhibition = 100 - \frac{OD testwell}{OD control} \times 100. \end{matrix}$

2.5. In Vivo Biological Screening

2.5.1. Analgesic Activity

BALB/c mice of both sexes (n = 6) weighing 18–22 g were used. All animals were withdrawn from food 3 hours before the start of the experiment and the mice were distributed in different groups. Among the divided animals, group I was injected with normal saline (10 ml/kg) as the control, while group II was administrated with the standard drug (diclofenac sodium; 10 mg/kg), and the rest of the groups were administered with various extracts and fractions (25, 50, and 100 mg/kg i.p). After administration of 30 min, the animals were treated with 1% acetic acid. Then, the number of abdominal constrictions (writhes) was counted after 5 min of acetic acid injection for the period of 10 minutes as per the usual methods [19].

2.5.2. Anti-Inflammatory Activity

The crude extracts and various fractions of P. hysterophorus were also screened for anti-inflammatory activity as per the standard procedure [20]. The animals were divided into different groups of both sexes. Groups I and II were injected with normal saline (10 ml/kg) and diclofenac sodium (10 mg/kg) respectively, while the rest of the groups were administered with extracts/fractions at various doses (25, 50, and 100 mg/kg). After 30 minutes of intraperitoneal treatment, carrageenan (1%, 0.05 ml) was injected subcutaneously into the sub plantar tissue of the hind paw of each mouse. The inflammation was restrained using a plethysmometer (LE 7500 Plan Lab S.L) directly after injection of carrageenan, and then after 1, 2, 3, 4, and 5 hours of carrageenan injection. The regular foot swelling of drug-treated animals, as well as standard, was associated with that of control, and the percent inhibition of edema was calculated using the following formula: $\begin{matrix} (3) & % Inhibition = A - \frac{B}{A} \times 100, \end{matrix}$ where A represents the edema volume of the control and B represents the paw edema volume of the tested group.

2.5.3. Sedative Activity

The crude extracts and various fractions of P. hysterophorus were also screened for muscle relaxation activity. For this screening test, a 30 cm long Pyrex glass tube with a 3 cm diameter was used in this study. From the base, the design tube is marked at 20 cm and the animals were screened after 30, 60, and 90 minutes of treatment. Various groups (n = 5) were treated with normal saline (10 ml/kg), standard drug, and tested extracts and their fractions (5 and 10 mg/kg i.p). The animals were introduced at one edge of the tube and then permitted to move up to the mark 20 cm from the base. When the treated animals touched the 20 cm mark, the tube was moved straight to the perpendicular position and the animals strained to climb again to the tube with a backward effort. The mouse which failed to reach up to the mark within 30 seconds was considered to have relaxed muscles [20].

3. Results

Phytochemical analysis of Parthenium hysterophorus is given in Table 1. The crude extracts and fractions exhibited the presence of various secondary metabolites such as steroids, fatty acids, and terpenoids. These identified phytochemicals are responsible for its urease, α-glucosidase, and phosphodiesterase inhibitory effects.

Table 1

Phytochemical screening test of extracts and fractions of P. hysterophorus.

Phytochemicals	MeOH	Hexane	Aqueous	EtOAc	Chloroform	Butanol
Alkaloids	+	−	+	+	−	+
Tannins	+	−	+	+	−	+
Anthraquinones	−	−	−	−	−	−
Glycosides
Reducing sugars	+	−	+	−	+	+
Saponins	+	−	+	−	−	+
Flavonoids	+	−	+	+	+	+
Phlobatannins	+	−	+	+	−	+
Steroids	+	+	+	+	+	+
Terpenoids	+	+	+	+	+	+

where MeOH is the methanolic extract and EtOAc is the ethyl acetate fraction.

3.1. In Vitro Enzyme Inhibition Assays

3.1.1. Urease Inhibition

The urease inhibitory activities of this plant are given in Table 2. The crude extracts and various fractions of Parthenium hysterophorus showed excellent urease inhibition activity. The polar extracts such as ethyl acetate (87.3%), butanol (84%), and aqueous (81.4%) showed excellent activity with IC₅₀ values of 57.3 ± 1.27, 35.3 ± 1.12, and 31.9 ± 2.21, respectively. The inhibitory potential is followed by n-hexane (77.4%), methanolic (74.2%), and chloroform (74.2%) fractions which showed moderate activity with IC₅₀ values of 39.8 ± 0.36, 43.1 ± 1.24, and 49.2 ± 2.16, respectively. Acetohydroxamic acid (96.3%) is used as a standard urease inhibitor with an IC₅₀ value of 20.3 ± 0.43.

Table 2

Urease inhibition activity of extracts and fractions of Parthenium hysterophorus.

Extract/fractions	Concentrations (µg/mL)	% Inhibition	IC50 (µg)
MeOH	0.2	74.2	43.1 ± 1.24
Hexane	0.2	77.4	39.8 ± 0.36
Aqueous	0.2	81.4	31.9 ± 2.21
Ethyl acetate	0.2	87.3	57.3 ± 1.27
Chloroform	0.2	74.2	49.2 ± 2.16
Butanol	0.2	84.0	35.3 ± 1.12
Acetohydroxamic acid	0.2	96.3	20.3 ± 0.43

3.1.2. α-Glycosidase Inhibition

The α-glycosidase inhibitory activities of this plant are given in Table 3. The crude extracts and different fractions of P. hysterophorus showed excellent α-glycosidase inhibition potential. The extracts such as methanolic (94.2%), aqueous (91.4%), and butanol (90.2%) showed excellent activity with IC₅₀ values of 13.1 ± 0.34, 23.1 ± 0.12, and 840 ± 1.73, respectively. The inhibitory potential of α-glucosidase was followed by n-hexane (84.7%), ethyl acetate (82.7%), and chloroform (76.4%) fractions with IC₅₀ values of 840 ± 1.73, 84.2 ± 2.17, and 118.6 ± 3.07, respectively. The standard α-glucosidase inhibitor, acarbose, exhibited percent inhibition (90.2%) with an IC₅₀ value of 840 ± 1.73.

Table 3

α-Glucosidase activity of extracts and fractions of Parthenium hysterophorus.

	Concentrations (µg/mL)	% inhibition	IC50 (µg)
MeOH	0.2	94.2	13.1 ± 0.34
Hexane	0.2	84.7	21.2 ± 1.16
Aqueous	0.2	91.4	23.1 ± 0.12
Ethyl acetate	0.2	82.7	84.2 ± 2.17
Chloroform	0.2	76.4	118.6 ± 3.07
Butanol	0.2	90.2	840 ± 1.73
Acarbose	0.2	90.2	840 ± 1.73

3.1.3. Phosphodiesterase Inhibition

The phosphodiesterase inhibitory activities of this plant are given in Table 4. The crude extract and different fractions of P. hysterophorus showed excellent phosphodiesterase inhibition potential. The extract such as aqueous (91.4%), butanol (88.4%) and n-hexane (82.7%) showed excellent activity with IC₅₀ values of 24.2 ± 0.11, 55.3 ± 2.15, 197.2 ± 3.16, respectively. The inhibitory potential of phosphodiesterase is followed by the methanolic (79%), chloroform (78.4%), and ethyl acetate (76.5%) with IC₅₀ values of 131.1 ± 2.41, 152.4 ± 1.81, and 62.4 ± 2.21, respectively. The standard phosphodiesterase inhibitor, EDTA exhibited 87.9% inhibition with an IC₅₀ value of 265.5 ± 2.25.

Table 4

Phosphodiesterase activity of extracts and fractions of Parthenium hysterophorus.

Extract/fractions	Concentrations (μM) (µg/mL)	% inhibition	IC50 (µg)
MeOH	0.2	79.0	131.1 ± 2.41
Hexane	0.2	82.7	197.2 ± 3.16
Aqueous	0.2	91.4	24.2 ± 0.11
Ethyl acetate	0.2	76.5	62.4 ± 2.21
Chloroform	0.2	78.4	152.4 ± 1.81
Butanol	0.2	88.4	55.3 ± 2.15
EDTA	0.2	87.9	265.5 ± 2.25

where EDTA is for ethyl amine tetra acetic acid.

3.2. In Vivo Activities

3.2.1. Analgesic Effect

The crude extracts and various fractions of P. hysterophorus including methanol, hexane, aqueous, ethyl acetate, chloroform, and butanol were assessed for analgesic activity. All the extracts/fractions were tested at 25, 50, and 100 mg/kg and the effects were observed to be dose-dependent. Among the tested extracts, butanol, ethyl acetate, and methanol showed maximum analgesic effect as compared to the standard drug (Table 5). The aqueous, chloroform, and n-hexane fraction of P. hysterophorus exhibited a moderate analgesic effect (Table 5).

Table 5

The analgesic effect of crude extracts and various fractions of P. hysterophorus.

Treatment	Dose (mg/kg)	No. of writhing
Normal saline	10 ml/kg	65.77 ± 3.46
Diclofenac sodium	10	17.67 ± 1.14

MeOH	25	51.48 ± 2.45
	50	32.76 ± 1.19
	100	16.87 ± 1.00

Hexane	25	66.85 ± 2.41
	50	48.45 ± 1.17
	100	32.54 ± 1.99

Aqueous	25	60.87 ± 2.67
	50	41.45 ± 1.56
	100	25.45 ± 1.98

Ethyl acetate	25	55.54 ± 2.49
	50	33.76 ± 1.90
	100	18.98 ± 1.71

Chloroform	25	61.45 ± 2.40
	50	42.98 ± 1.14
	100	26.98 ± 1.98

Butanol	25	48.45 ± 2.41
	50	29.98 ± 1.98
	100	14.96 ± 1.78

3.2.2. Anti-Inflammatory Effect

The crude extracts and various fractions were assessed for anti-inflammatory. Among the tested extracts, the methanolic and butanol extracts exhibited maximum inhibition after 3 hours of administration of extracts, as shown in Figure 1. However, the percent inhibition of the standard diclofenac sodium drug was promising throughout 6 hours of the experiment duration.

[figure(s) omitted; refer to PDF]

3.2.3. Sedative Effect

The crude extracts and various fractions of P. hysterophorus including methanol, hexane, aqueous, ethyl acetate, chloroform, and butanol were assessed for sedative activity. Among the tested extracts, the aqueous and butanol extracts exhibited maximum sedative effect followed by chloroform, ethyl acetate, and methanolic fractions as compared to the standard drug (Table 6).

Table 6

The sedative effect of crude extracts and various fractions of P. hysterophorus.

Treatment	Dose	No. of lines crossed
Normal saline	10 ml/kg	126 ± 1.25
Diazepam	0.5 mg/kg	6 ± 0.13 $^{* * *}$

MeOH	25	110.51 ± 4.23
	50	102.60 ± 3.44
	100	94.68 ± 3.35 $^{*}$

Hexane	25	115.90 ± 4.21
	50	108.69 ± 3.40
	100	100.99 ± 3.30 $^{*}$

Aqueous	25	98.51 ± 4.29
	50	88.63 ± 3.24
	100	80.61 ± 3.14 $^{* * *}$

Ethyl acetate	25	107.51 ± 3.99
	50	97.61 ± 3.29
	100	89.66 ± 3.00 $^{* *}$

Chloroform	25	105.55 ± 4.34
	50	94.65 ± 3.20
	100	83.69 ± 3.10 $^{* *}$

Butanol	25	100.54 ± 4.200
	50	90.69 ± 3.23
	100	81.65 ± 3.13 $^{* * *}$

where, $P < {0.05}^{*}$ , $P < {0.03}^{* *}$ , and $P < {0.01}^{* * *}$ .

4. Discussion

Phytochemicals in medical plants play key roles in their biological potency. Phytochemical analysis plays a significant role in the isolation of new active and rare compounds. The biomedical importance of plants is correlated due to the presence of secondary metabolites. Our plant of interest, P. hysterophorus, was collected, processed, and extracted with various solvents to obtain crude extracts and fractions. The crude extracts and fractions exhibited the presence of various secondary metabolites such as steroids, fatty acids, terpenoids alkaloids, tannins, reducing sugars, saponins, flavonoids, and phlorotannins. P. hysterophorus is already reported as an ailment for various diseases in the traditional system. The plant is reported to have a diverse nature of compounds including allelochemicals (such as hysterin and ambrosin), flavonoids(such as fumaric acid, quercetagetin 3, 7-dimethylether, p-coumaric, p-hydroxybenzoin, vanillic acid, chlorogenic acid, anisic acid, and ferulic acid), and various alcohols [5]. A novel hydroxyproline-rich glycoprotein has been documented from the pollen of P. hysterophorus [7]. Another novel sesquiterpenoid, charminarone, has also been previously reported [8–10].

The extracts and fractions of P. hysterophorus were screened for in vitro selective enzyme inhibition assays including urease, α-glucosidase, and phosphodiesterase. The ethyl acetate (87.3%), butanol (84%), and aqueous (81.4%) fractions of P. hysterophorus exhibited maximum inhibition of urease enzyme compared to other fractions, however, exhibited less activity than the standard acetohydroxamic acid (96.3%). Urease is a metalloenzyme found in bacteria and plants. The urease inhibitors are important in the conditions associated with ureolytic bacteria [21]. Furthermore, the urease inhibitor is effective against H pylori infections [22]. In agriculture, urease inhibitors are associated with the proper utilization of urea fertilizers and modifying the nitrogen cycle [23]. Furthermore, α-glucosidase inhibition by various fractions of P. hysterophorus highlighted its importance for controlling hyperglycemia in diabetic patients [24, 25].

The phosphodiesterase inhibition by the fractions of P. hysterophorus is worth noting. Phosphodiesterase (PDE) has more than 40 isoforms, further subdivided into eleven families. These enzymes (present in each cell) hydrolyze the intercellular second messengers, cyclic nucleotide adenosine-3′, 5′- cyclic monophosphate (cAMP), and guanosine-3′, 5′-cyclic monophosphate (cGMP), thus altering cell response [24]. The PDEs are considered potential targets for combating various diseases including Alzheimer’s disease, erectile dysfunction, and asthma [26]. The PDE isoforms expressed in cardiovascular systems and CNS are targeted in the treatment of pulmonary hypertension and cardiovascular disorders [27].

The acetic acid-induced writhing test is used to examine the preliminary analgesic properties of P. hysterophorus extracts and fractions [28]. The acetic acid causes the generation of pain mediators, thereby resulting in the constriction of the abdominal muscles [28, 29]. Our data exhibited promising analgesic effects in the butanol, ethyl acetate, and methanol extracts P. hysterophorus, whereas aqueous, chloroform, and n-hexane fractions exhibited moderate analgesic activity. Therefore, the phytochemical constituents of P. hysterophorus may play a role in inhibiting the release of pain-stimulating mediators such as prostaglandins (PGs), bradykinin, and histamine [30, 31]. Among these mediators, PGs are mostly responsible for the induction of pain. The selected plant probably inhibits cyclo-oxygenase, and thus, blocks the production of PGs and other intracellular cascades leading to pain, inflammation, and pyrexia.

The traction and chimney screening tests are common tools for the in vivo assessment of the skeleton muscle relaxation potential of substances [28]. In our findings, the aqueous and butanol extracts exhibited maximum sedative effect followed by chloroform, ethyl acetate, and methanolic fractions as compared to the standard drug, diazepam. The sedative and muscle relaxant effect suggested that the chemical constituents of this plant keep the anion neuronal channels open, especially the chloride channels which leads to central nervous system depression. The induction of anion influx is mostly related to the stimulation of GABA (gamma-aminobutyric acid) receptors, thereby hyperpolarizing the neuronal membrane via more chloride influx [32]. It is also suggested that the extracts or fractions might be accelerating the action of GABA neurotransmitters which are responsible for sedation and muscle relaxant effect.

5. Conclusion

It is concluded that crude extracts and various fractions showed the presence of active phytochemicals such as steroids, alkaloids, and terpenoids. The polar extracts and fractions exhibited excellent enzyme inhibition potency, thereby signifying the inhibition potential of urease, α-glucosidase, and phosphodiesterase by its phytochemical constituents. The sedative, anti-inflammatory, and analgesic potential of plants are also validated experimentally. Based on our data, we can conclude that P. hysterophorus could be a potential source of new, less toxic, safe, and more effective candidate drugs for pharmaceutical industries, thereby decreasing the economic burden for the therapy of different diseases involving the targets such as urease, α-glucosidase, and phosphodiesterase.

Acknowledgments

The authors acknowledge the Pakistan Science Foundation Project NO. PSF/NSLP/KP-UoS (737) for providing research funds for this work.

References

[1] R. K. Meena, B. Dutt, R. Kumar, K. R. Sharma, "Phyto-chemistry of congress grass ( Parthenium hysterophorus L.) and harmful and beneficial effect on human and animals: a review," International Journal of Chemical Studies, vol. 5 no. 4, pp. 643-647, 2017.

[2] S. Patel, "Harmful and beneficial aspects of Parthenium hysterophorus: an update," 3 Biotech, vol. 1 no. 1,DOI: 10.1007/s13205-011-0007-7, 2011.

[3] A. I. Maishi, P. K. Shoukat Ali, S. A. Chaghtai, G. Khan, "A proving of Parthenium hysterophorus , L," British Homeopathic Journal, vol. 87 no. 01, pp. 17-21, DOI: 10.1016/s0007-0785(98)80005-7, 1998.

[4] A. Rauf, A. Khan, N. Uddin, M. Akram, M. Arfan, G. Uddin, M. Qaisar, "Preliminary phytochemical screening, antimicrobial and antioxidant activities of Euphorbia milli," Pakistan Journal of Pharmaceutical Sciences, vol. 27 no. 4, pp. 947-951, 2014.

[5] H. C. Evans, "Parthenium hysterophorus. a review of its weed status and the possibilities for biological control," Biocontrol News and Information, vol. 18, pp. 89-98, 1997.

[6] M.-H. Wang, J.-J. Gan, W.-H. Chen, Y.-L. Guan, "Chemical constituents of Parthenium hysterophorus," Chemistry of Natural Compounds, vol. 56 no. 3, pp. 556-558, DOI: 10.1007/s10600-020-03090-3, 2020.

[7] H. Lata, V. K. Garg, R. K. Gupta, "Sequestration of nickel from aqueous solution onto activated carbon prepared from Parthenium hysterophorus L.," Journal of Hazardous Materials, vol. 157 no. 2-3, pp. 503-509, DOI: 10.1016/j.jhazmat.2008.01.011, 2008.

[8] N. Gupta, B. M. Martin, D. D. Metcalfe, P. V. S. Rao, "Identification of a novel hydroxyproline-rich glycoprotein as the major allergen in Parthenium pollen," The Journal of Allergy and Clinical Immunology, vol. 98 no. 5, pp. 903-912, DOI: 10.1016/s0091-6749(96)80006-6, 1996.

[9] A. Joshi, R. K. Bachheti, A. Sharma, R. Mamgain, "Parthenium hysterophorus . L. (asteraceae): a boon or curse? (a review)," Oriental Journal of Chemistry, vol. 32 no. 3, pp. 1283-1294, DOI: 10.13005/ojc/320302, 2016.

[10] A. Ramos, R. Rivero, A. Visozo, J. Piloto, A. García, "Parthenin, a sesquiterpene lactone of Parthenium hysterophorus L. is a high toxicity clastogen," Mutation Research, vol. 514 no. 1-2, pp. 19-27, DOI: 10.1016/s1383-5718(01)00321-7, 2002.

[11] N. R. Farnsworth, "Biological and phytochemical screening of plants," Journal of Pharmaceutical Sciences, vol. 55 no. 3, pp. 225-276, DOI: 10.1002/jps.2600550302, 1966.

[12] J. R. Shaikh, M. Patil, "Qualitative tests for preliminary phytochemical screening: an overview," International Journal of Chemical Studies, vol. 8 no. 2, pp. 603-608, DOI: 10.22271/chemi.2020.v8.i2i.8834, 2020.

[13] S. C. Chhabra, F. C. Uiso, E. N. Mshiu, "Phytochemical screening of Tanzanian medicinal plants. I," Journal of Ethnopharmacology, vol. 11 no. 2, pp. 157-179, DOI: 10.1016/0378-8741(84)90037-0, 1984.

[14] A. Doss, "Preliminary phytochemical screening of some Indian medicinal plants," Ancient Science of Life, vol. 29 no. 2, pp. 12-16, 2009.

[15] O. A. Aiyegoro, A. I. Okoh, "Preliminary phytochemical screening and in vitro antioxidant activities of the aqueous extract of Helichrysum longifolium DC," BMC Complementary and Alternative Medicine, vol. 10 no. 1,DOI: 10.1186/1472-6882-10-21, 2010.

[16] A. Hameed, M. Al-Rashida, M. Uroos, S. U. Qazi, S. Naz, M. Ishtiaq, K. M. Khan, "A patent update on therapeutic applications of urease inhibitors (2012–2018)," Expert Opinion on Therapeutic Patents, vol. 29 no. 3, pp. 181-189, DOI: 10.1080/13543776.2019.1584612, 2019.

[17] F. Shaheen, M. Ahmad, S. Nahar Khan, S. Samreen Hussain, S. Anjum, B. Tashkhodjaev, K. Turgunov, M. N. Sultankhodzhaev, M. I. Choudhary, "New α -glucosidase inhibitors and antibacterial compounds from Myrtus communis L," European Journal of Organic Chemistry, vol. 10, pp. 2371-2377, DOI: 10.1002/ejoc.200500936, 2006.

[18] D. Saleheen, S. Bukhari, S. R. Haider, A. Nazir, S. Khanum, S. Shafqat, M. K. Anis, P. Frossard, "Association of phosphodiesterase 4D gene with ischemic stroke in a Pakistani population," Stroke, vol. 36 no. 10, pp. 2275-2277, DOI: 10.1161/01.str.0000182242.59466.ee, 2005.

[19] N. Muhammad, R. Lal Shrestha, A. Adhikari, A. Wadood, H. Khan, A. Z. Khan, F. Maione, N. Mascolo, V. De Feo, "First evidence of the analgesic activity of govaniadine, an alkaloid isolated from Corydalis govaniana Wall," Natural Product Research, vol. 29 no. 5, pp. 430-437, DOI: 10.1080/14786419.2014.951933, 2015.

[20] N. Muhammad, M. Saeed, S. N. Gilani, "Analgesic and anti-inflammatory profile of n-hexane fraction of viola betonicifolia," Tropical Journal of Pharmaceutical Research, vol. 11 no. 6, pp. 963-969, DOI: 10.4314/tjpr.v11i6.13, 2013.

[21] N. Muhammad, M. Saeed, H. Khan, I. Haq, "Evaluation of n -hexane extract of viola betonicifolia for its neuropharmacological properties," Journal of Natural Medicines, vol. 67,DOI: 10.1007/s11418-012-0636-0, 2013.

[22] L. V. Modolo, A. X. de Souza, L. P. Horta, D. P. Araujo, A. de Fatima, "An overview on the potential of natural products as ureases inhibitors: a review," Journal of Advanced Research, vol. 6 no. 1, pp. 35-44, DOI: 10.1016/j.jare.2014.09.001, 2015.

[23] J. T. Zhou, C. L. Li, L. H. Tan, Y. F. Xu, Y. H. Liu, Z. Z. Mo, Y. X. Dou, R. Su, Z. R. Su, P. Huang, J. H. Xie, "Inhibition of Helicobacter pylori and its associated urease by palmatine: investigation on the potential mechanism," PLoS One, vol. 12 no. 1,DOI: 10.1371/journal.pone.0168944, 2017.

[24] T. Hara, J. Nakamura, N. Koh, F. Sakakibara, N. Takeuchi, N. Hotta, "An importance of carbohydrate ingestion for the expression of the effect of α -glucosidase inhibitor in NIDDM," Diabetes Care, vol. 19 no. 6, pp. 642-647, DOI: 10.2337/diacare.19.6.642, 1996.

[25] E. M. Kawakami, D. M. Oosterhuis, J. L. Snider, M. Mozaffari, "Physiological and yield responses of field-grown cotton to application of urea with the urease inhibitor NBPT and the nitrification inhibitor DCD," European Journal of Agronomy, vol. 43, pp. 147-154, DOI: 10.1016/j.eja.2012.06.005, 2012.

[26] S. Uckert, P. Hedlund, E. Waldkirch, M. Sohn, U. Jonas, K.-E. Andersson, C. G. Stief, "Interactions between cGMP-and cAMP-pathways are involved in the regulation of penile smooth muscle tone," World Journal of Urology, vol. 22 no. 4, pp. 261-266, DOI: 10.1007/s00345-003-0394-4, 2004.

[27] J. Prickaerts, P. R. A. Heckman, A. Blokland, "Investigational phosphodiesterase inhibitors in phase I and phase II clinical trials for Alzheimer’s disease," Expert Opinion on Investigational Drugs, vol. 26 no. 9, pp. 1033-1048, DOI: 10.1080/13543784.2017.1364360, 2017.

[28] M. M. Rahman, F. Islam, A. Parvez, M. A. Azad, G. M. Ashraf, M. F. Ullah, M. Ahmed, "Citrus limon L.(lemon) seed extract shows neuro-modulatory activity in an in vivo thiopental-sodium sleep model by reducing the sleep onset and enhancing the sleep duration," Journal of Integrative Neuroscience, vol. 21 no. 1, 2022.

[29] S. Bawazeer, M. Ibrar, N. Ikram, A. Rauf, T. B. Hadda, S. Bawazeer, H. Khan, S. Pervez, "In vivo antinociceptive and muscle relaxant activity of leaf and bark of Buddleja asiatica L," Pakistan Journal of Pharmaceutical Sciences, vol. 29 no. 5, pp. 1509-1512, 2016.

[30] J. Zhao, F. Fang, L. Yu, G. Wang, L. Yang, "Anti-nociceptive and anti-inflammatory effects of Croton crassifolius ethanol extract," Journal of Ethnopharmacology, vol. 142 no. 2, pp. 367-373, DOI: 10.1016/j.jep.2012.04.050, 2012.

[31] I. D. Duarte, M. Nakamura, S. H. Ferreira, "Participation of the sympathetic system in acetic acid-induced writhing in mice," Brazilian Journal of Medical and Biological Research, vol. 21 no. 2, pp. 341-343, 1988.

[32] H. Khan, M. Saeed, A. U. H. Gilani, M. A. Khan, A. Dar, I. Khan, "The antinociceptive activity of Polygonatum verticillatumrhizomes in pain models," Journal of Ethnopharmacology, vol. 127 no. 2, pp. 521-527, 2010.

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The main aim of this research was to explore Parthenium hysterophorus Linn phytochemically and pharmacologically. Phytochemical screening is important for the isolation of active compounds before bulk extraction. The crude extracts and their fractions were screened for enzyme (urease, α-glycosidase, and phosphodiesterase) inhibition assays, in vivo analgesic, anti-inflammatory, and sedative effects. Results indicated the presence of steroids, flavonoids, etc. The crude extracts such as methanol, hexane, aqueous, ethyl acetate, chloroform, and butanol exhibited excellent urease inhibitory activities with IC₅₀ = 43.1 ± 1.24, 31.9 ± 2.21, 31.9 ± 2.21, 57.3 ± 1.27, 49.2 ± 2.16, and 35.3 ± 1.12, respectively, as compared to standard acetohydroxamic acid (20.3 ± 0.43). The extracts (methanol, hexane, aqueous, ethyl acetate, chloroform, and butanol) also showed promising α-glycosidase potency with IC₅₀ = 13.1 ± 0.34, 21.2 ± 1.16, 23.1 ± 0.12, 84.2 ± 2.17, 118.6 ± 3.07, and 840 ± 1.73, respectively against acarbose (840 ± 1.73). The phosphodiesterase activity of the mentioned extracts was also excellent with IC₅₀ = 131.1 ± 2.41, 197.2 ± 3.16, 24.2 ± 0.11, 62.4 ± 2.21, 152.4 ± 1.81, and 55.3 ± 2.15, respectively, against the standard (265.5 ± 2.25). Furthermore, butanol (14.96 ± 1.78), ethyl acetate (18.98 ± 1.71), and methanol (16.87 ± 1.00) showed dose-dependent analgesic effects with a maximum inhibition of acetic acid-induced writhes. Whereas, methanolic and butanol extracts exhibited maximum inhibition of inflammation in the carrageenan paw edema test. The aqueous ( $p < 0.01$ ) and butanol ( $p < 0.01$ ) extracts exhibited maximum a sedative effect followed by chloroform ( $p < 0.05$ ), ethyl acetate ( $p < 0.05$ ), and methanolic ( $p < 0.05$ ) fractions as compared to the standard drug. The current research concluded that Parthenium hysterophorus Linn has important phytochemical constituents having inhibitory effects on urease, α-glycosidase, and phosphodiesterase enzymes. Furthermore, the plant has analgesic, anti-inflammatory, and sedative effects. The P. hysterophorus needs to further be explored for the candidate molecules responsible for the abovementioned activities.

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Title

Phytochemical Analysis and In Vitro and In Vivo Pharmacological Evaluation of Parthenium hysterophorus Linn

Author

Gul¹; Rauf, Abdur²

; Imtiaz Ali Khan³; Sulaiman Mohammad Alnasser⁴; Syed Uzair Ali Shah¹; Rahman, Md Mominur⁵

¹ Department of Pharmacy, University of Swabi, Anbar 23561, Khyber Pakhtunkhwa, Pakistan
² Department of Chemistry, University of Swabi, Anbar 23561, Khyber Pakhtunkhwa, Pakistan
³ Department of Entomology, The University of Agriculture, University of Peshawar, Peshawar, Khyber Pakhtunkhwa, Pakistan
⁴ Department of Pharmacology and Toxicology, Unaizah College of Pharmacy, Qassim University, Unayzah, Saudi Arabia
⁵ Department of Pharmacy, Faculty of Allied Health Sciences, Daffodil International University, Dhaka 1207, Bangladesh

Editor

Atul Kabra

Publication year

2022

Publication date

2022

Publisher

John Wiley & Sons, Inc.

ISSN

1741427X

e-ISSN

17414288

Source type

Scholarly Journal

Language of publication

English

DOI

https://doi.org/10.1155/2022/6088585

ProQuest document ID

2680910250

Phytochemical Analysis and In Vitro and In Vivo Pharmacological Evaluation of Parthenium hysterophorus Linn

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