Anti-Toxoplasma Effects of Dracocephalum Polychaetum Essential Oil

Background Toxoplasma gondii is a common parasitic disease with a cosmopolitan prevalence, causing severe health problems. Although chemotherapy for toxoplasmosis is readily available, most have side effects. Objectives This study assesses the Dracocephalum polychaetum essential oil against T. gondii activity. In vitro, the anti-Toxoplasma effects of D. polychaetum essential oils with different concentrations were evaluated. Methods In the present study, T. gondii RH strain tachyzoites were exposed to D. polychaetum essential oil, and their viability effect on the parasite was evaluated. The viability test of tachyzoites was performed by using the staining method trypan blue in vitro. The inhibitory effect of D. polychaetum extract on T. gondii RH strain tachyzoites in the Vero cell line was evaluated. Results D. polychaetum has valuable efficacy in vitro, outperforming pyrimethamine and sulfadiazine at 30 and 90 minutes after exposure (p < 0.05). D. polychaetum essential oil showed anti-Toxoplasma activity in the cell line (IC50: 241.7 μg/mL). After T. gondii-infected Vero cells had been incubated with different concentrations of the D. polychaetum essential oil, their viability decreased in a dose-dependent manner. Conclusions In conclusion, D. polychaetum extract as an herbal medicine might be a valuable alternative to routine chemotherapy for toxoplasmosis.

is protozoan can infect a wide range of warm-blooded vertebrates and humans by living inside the cell. T. gondii can cause severe weakness, miscarriage, or even death. e parasite is usually transmitted by drinking water contaminated with cat feces (containing parasitic oocysts) or by eating meat containing uncooked blood and by transfusion of blood from a person infected with the parasite to a healthy person [3,4].
It is estimated that more than a third of the world's humans have been exposed to toxoplasmosis. About 190,000 people are born with the disease each year [5]. is parasite can spread throughout the host body and uses various tactics to cross the blood-brain barrier and reach the brain [6]. Toxoplasmosis can cause many problems by infecting the fetus by crossing the placenta during pregnancy. Infection in the fetus can manifest itself in the form of growth retardation, mental retardation, eye problems, many other diseases, and fetal death [7]. In the first trimester of pregnancy, if the fetus is infected with the parasite, this infection can cause miscarriage. But if the infection occurs during the second trimester of pregnancy, in that case, this infection can lead to retinochoroiditis and microcephaly in the fetus [8]. If this parasitic infection occurs in the third trimester of pregnancy, it can lead to lymphadenopathy, hepatosplenomegaly, and ocular disorders [8,9]. Toxoplasmosis is usually asymptomatic in people with sound immune systems [9][10][11]. However, in people with defective immune systems or underlying diseases such as diabetes, cancer, or people taking corticosteroids, toxoplasmosis causes encephalitis, fever, swollen lymph nodes, fatigue, muscle pain, sore throat, retinitis (inflammation of the retina), and sometimes skin rash [12,13]. Retinochoroiditis, a symptom of toxoplasmosis, occurs in youth but results from congenital toxoplasmosis [14].
Diagnosis of toxoplasmosis by serological tests is common. However, they are not reliable and can be cited because, as mentioned, there are many anti-Toxoplasma antibodies in the blood of one person, and another serological test should be taken a few days later [15,16].
Toxoplasmosis is usually treated with antiparasitic drugs such as sulfadiazine and pyrimethamine [17], but these drugs have ineffectiveness, resistance, and side effects [18,19]. Herbal remedies are one of the alternative treatments for many diseases [20][21][22][23]. Natural resources, especially medicinal plants, have a high position among the possible new treatments to replace the antiparasitic drugs sulfadiazine and pyrimethamine [24,25]. Chemical drugs used to treat toxoplasmosis increase serum creatinine and liver enzymes, cause megaloblastic anemia, allergic reactions, and agranulocytosis. In addition, many herbs have traditionally been used to treat toxoplasmosis and have been reported to have. In addition, several papers have demonstrated the pharmacological ability of plant extracts to inhibit the growth of T. gondii in vitro [26].
In recent years, the search for new antimicrobial agents has increased, and these agents mainly include plants because about a quarter of the chemical and synthetic drugs currently prescribed are derived from plants or natural sources, which is the case. Studies published in recent years examining natural resources and medicinal plants on protozoan and worm parasites such as Leishmania, Trypanosoma, Toxoplasma, and Echinococcus have shown that these resources can help treat these diseases [21][22][23][24][25]. Furthermore, the work of Menghini et al. shows that female hemp inflorescences constitute a source of biomolecules with potential pharmacological applications, in particular against parasitosis and infectious diseases [27].
is plant species has many uses in Iran due to its many medicinal properties. is plant has been used in the traditional medicine of the Kerman region for a long time due to its pleasant smell and pharmacological properties [29,30]. No scientific studies have been performed on D. polychaetum to replace it with traditional antiparasitic drugs against toxoplasmosis. is study aimed to evaluate the anti-Toxoplasma activity of D. polychaetum extract in vitro. e essential oil of D. polychaetum can inhibit T. gondii tachyzoites in vitro using standard and appropriate methods and was studied to provide scientific data on the anti-Toxoplasma properties of this medicinal plant. erefore, in this study, the therapeutic effect of D. polychaetum on T. gondii infection was investigated in vitro.

Ethics Approval.
All applicable international and institutional guidelines for conducting the study. e current study was approved by the Ethics Committee of Islamic Azad University, Shahrekord Branch (code: IR.IAU.SHK. REC.1400.066).

Preparation of the Plant and Essential Oil.
e aerial part of D. polychaetum was prepared, identified, and approved by Kerman province in August 2017, when the plant was fully flowering. In order to prepare the essential oil, the plant was powdered in the dry shade with an electric blender. 100 g of powder was transferred to a 2-liter distillation flask, and 1200 ml of deionized water was added. e essential oil was extracted for 3 hours using a Clevenger essential oil preparation machine. is process was repeated five times to prepare enough essential oil, each time with a new plant. e collected essential oils were then poured on top and dehydrated with anhydrous sodium sulfate, and then stored in a dark closed container away from light and refrigerated [31].

Multiplication, Quantification, and Maintenance of
Tachyzoites. Intraperitoneal passages of T. gondii RH strain tachyzoites were maintained in Balb/c mice and collected in phosphate buffered saline (PBS), pH 7.2, at 3-4-day intervals. e infected mice's peritoneal fluid was collected and centrifuged for 10 minutes at 200 g at room temperature. e host cells and detritus were removed by centrifugation. e parasite-containing supernatant was then collected and centrifuged for 10 minutes at 1,000 g. e pellet was washed twice, once in PBS at pH 7.2 and again in RPMI-1640 (Gibco, USA) without bovine fetal serum. e trypan blue exclusion technique was used to determine the viability of the parasites 30 to 40 minutes after removal from the peritoneal cavity. Light microscopy and a hemocytometer were used to determine the number of tachyzoites. In a humidified 5 percent CO 2 incubator at 37°C, the tachyzoites were injected into a 75 ml tissue culture flask containing proliferating Vero cells.

Vero Cells and Evaluation of Cytotoxicity.
e kidney cell lines "Vero" were acquired from the National Cell Bank of Iran and were derived from a green monkey kidney (NCBI, Pasteur Institute of Iran, Tehran, Iran). Vero cells were cultured in RPMI-1640 media supplemented with 100 g/ml streptomycin, 100 units/ml penicillin (Gibco, Pen-Strep15140), 2 ram l-glutamine, and 10% fetal bovine serum (FBS) at 37°C with 5% CO2 (Bovogen, Australia).
Using 96-well plates, the cytotoxicity of the essential oil was assessed on Vero cells using a modified MTT assay (Sigma Aldrich, USA) with 3(4,5 dimethylthiazolyl) 2,5diphenyltetrazolium bromide. Vero cells were injected at a concentration of 6 × 10 4 cells/mL into each well previously holding 100 L growth media. For 24 hours, the cells were incubated at 37°C in an incubator moistened with 5% CO 2 . Following this, the Vero cells were treated with D. polychaetum extracts at various concentrations: 1000, 500, 100, 50, 10, and 1 μg/ml. Each concentration was placed in its own 96-well plate. Positive controls included pyrimethamine and sulfadiazine (toxoplasmosis reference medications), whereas the control buffer was RPMI-1640. e supernatant was removed after 24 hours. In each well, 100 μl of MTT PBS solution (5 mg/ml) was mixed with RPMI-1640 in a 1 : 9 ratio. After that, the plate was covered with aluminum foil and placed in a 37°C incubator for 4 hours. After discarding the medium, 100 μl of DMSO was added to each well to dissolve the dark blue MTT formazan salt. A Dynex microplate reader was used to determine the optical density at 570 nm absorbance.

MTT Test and In Vitro Infection.
For this stage, Vero cells were employed. Exponential growth was used to create the cells. Each well received 3 × 10 5 parasites/ml, resulting in a total volume of 200 µl. Six hours after inoculation, the infected cells were washed twice with RPMI-1640 FBS free media to eliminate extracellular parasites. After an 18-hour incubation period, 100 μl of RPMI-1640 media with 2% FBS was added to each well, along with various concentrations of essential oil/pyrimethamine and sulfadiazine. e anti-T. gondii activity and cytotoxicity of the essential oil were measured in 96-well plates using the thiazolyl blue tetrazolium bromide (MTT) technique (Sigma, St. Louis, MO, USA). e cell line was given the essential oil. A MTT solution was added to the cells after 24 hours, and the presence of purple matrices was determined using a plate reader. All of the data points are the average of three separate trials. e concentration of extracts, controls, and essential oils that effectively inhibited 50% of T. gondii tachyzoites was used to calculate the mean inhibitory concentration (IC50). e mean IC50 value for Vero cells compared to the mean IC50 value for T. gondii is known as selectivity.
T-IC 50 and V-IC 50 are the median inhibitory concentrations required to inhibit T. gondii and Vero cells, respectively [24].

Tachyzoite Viability by Trypan Blue Exclusion.
In vitro, a tachyzoite viability test was performed. In 96-well microplates, 45 μl of tachyzoite solution containing 10 6 cells/ml and D. polychaetum essential oil at six different concentrations (1, 10, 50, 100, 500, and 1000 µg) are mixed. e entire mixture was incubated at 37°C. A trypan blue dye exclusion test for tachyzoites is performed under an inverted microscope after 30, 90, and 180 minutes of incubation in 5% CO 2 at 37°C. e percentage viability of the results was calculated. e positive controls were 96-well plates containing 100 mg/ml of pyrimethamine and sulfadiazine, whereas the negative controls were PBS. After that, the plates were spread out on a glass slide and examined under an optical microscope. ree times the trials were carried out.

Statistical Analysis.
ANOVA was used in the statistical analysis using SPSS software (Ver. 18.0). e level of significance was considered to be p < 0.05. All data were reported as mean ± SD. Table 1, six substances were identified. ey represent 88.3% of all the oil. e main substances were methyl cyclogeranete (43.86%), neral (19.98%), and limonene (16.42%). Figure 1 presents the typical total ion current chromatograms of the essential oil.

MTT Test for Cytotoxicity Activity, In Vitro Infection, and
Effectors. Table 2 shows the MTT test results for various concentrations of D. polychaetum essential oils and negative control cells. In vitro tests against T. gondii were conducted using a positive control and various concentrations of D. polychaetum.

Effects of Essential Oil on Tachyzoite
Viability. Six concentrations of D. polychaetum essential oil (1, 10, 50, 100, 500, and 1,000 µg) were incubated for 30, 90, and 180 minutes. e vitality of the tachyzoites was determined using trypan blue stain. e parasiticidal impact of essential oil was substantially better than the positive control in all exposure durations, indicating that D. polychaetum had adequate effectiveness in vitro ( Table 3).
As shown in Figure 2, all three groups were parallel until 90 minutes, and the essential oil group was lower than the two control groups. However, after 90 minutes, this trend was reversed. At 180 minutes, the average viability in the group was that the essential oil was placed above the 2 control groups. D. polychaetum essential oil showed anti-Toxoplasma activity in the Vero cell (IC50 : 241.7 μg/mL). After T. gondii-infected Vero cells had been incubated with different concentrations of the D. polychaetum essential oil, their viability decreased in a dose-dependent manner (Figure 2). e viability showed no significant decreases, compared with the control, at all concentrations of the extracts (p > 0.05). e mean viability and cytotoxicity between the groups are almost the same. e viability results between groups with different concentrations and at different times of 30, 90, and 180 minutes showed that in all 3 groups (essential oil and 2 control groups), there was a significant difference between different concentrations (Table 3). ere is a measurement in all 3 times. It decreases with increasing concentration to arrive at the highest concentration, i.e., 1000, its lowest value. For pyrimethamine and sulfadiazine, the mean viability at 180 was less than the other two. Simultaneous examination of 3 groups at different times also showed that the interaction between time and group was significant (p < 0.001), which indicates that the changes in mean viability depended on the group and the time of measurement.

Discussion
Numerous studies have been performed to evaluate the anti-Toxoplasma activity of plant extracts and essential oils when evaluated in vitro. However, valuable and appropriate studies have been performed on natural substances and the identification of essential oils with low toxicity to host cells [24,25]. It has not been done, and many studies are still needed to determine this issue. e World Health Organization (WHO) recommends using herbal remedies and natural resources for the treatment of toxoplasmosis [32]. People use medicinal plants every day in developing countries because these products are safe, have low side effects, and are available at a low cost [33,34]. e chemical drugs used to treat this disease have high side effects and common side effects. Numerous studies have been performed to evaluate the anti-Toxoplasma activity of plant extracts and essential oils when evaluated in vitro [24,25]. However, valuable and appropriate studies have been performed on natural substances and the identification of essential oils with low toxicity to host cells. It has not been done, and many studies are still needed to determine this issue [24]. Many herbal plants have been introduced as anti-T. gondii agents globally. However, there is no research on     [18,19,35]. e anti-Toxoplasma activity of D. kotschyi extracts showed that this species had anti-Toxoplasma activity [25], so the current work was accomplished [24,25]. In the current work, we evaluated the efficacy of D. polychaetum essential oil on T. gondii infection for the first time in Iran. A study conducted by Daryani et al. [35] to investigate the anti-Toxoplasma activity of Sambucus nigra (Caprifoliaceae) fruit and   Interdisciplinary Perspectives on Infectious Diseases 5 leaf extract showed that the survival of a group of T. gondii parasites exposed to a methanolic extract of Sambucus nigra was greater than the other control groups for the first time (30 min), which was not consistent with our study [14,15,26]. e selective toxicity of D. polychaetum essential oil was near the positive group, but the difference was insignificant.
is result was consistent with a previous study [36]. e activity of the essential oil is related to the quality of the active molecules present in it. e presence of active agents in the plant essential oil was determined in the previous studies [37,38]. Kariminik et al. [16] found that D. polychaetum essential oil contains methyl cyclogeranate, limonene, linalool, sabinene, and p-menth-1-en-9-ol. e anti-Toxoplasma activity of these active agents was determined too, so the present study was performed. For the first time, we report the activity of D. polychaetum essential oil against toxoplasmosis in vitro. Supplementary work is needed to identify active compounds of D. polychaetum essential oil associated with anti-Toxoplasma activity.

Conclusion
We report for the first time the anti-Toxoplasma D. polychaetum activity in vitro. is potential is associated with low toxicity to the host cell. Additional work is needed to identify active compounds associated with anti-Toxoplasma activity.

Data Availability
e datasets from the present study are available from the corresponding author upon request.

Ethical Approval
is article results from a research project (code: IR.IAU.SHK.REC.1400.066) in Islamic Azad University, Shahrekord Branch. Disclosure e funder had no role in the study design, data collection and analysis, decision to publish, or preparation of the manuscript.

Conflicts of Interest
All authors declare that there are no conflicts of interest.