6363 Dental Journal (Majalah Kedokteran Gigi) 2021 June; 54(2): 63–67 Original article The effectiveness of the combination of Moringa oleifera extract and propolis on Porphyromonas gingivalis biofilms compared to 0.7% tetracycline Hansen Kurniawan, Widyastuti and Mery Esterlita Hutapea Department of Periodontics, Faculty of Dentistry, Universitas Hang Tuah, Surabaya – Indonesia ABSTRACT Background: Periodontitis is an inflammatory disease that occurs in periodontal tissues. Porphyromonas gingivalis is also known as a bacterium commonly associated with the pathogenesis of periodontitis. Tetracycline is one of the antibiotics often used in periodontal tissue treatment. Propolis and Moringa oleifera are also known to have certain compounds assumed to be able to inhibit biofilm growth. Purpose: This study aims to understand the effectiveness of the combination of Moringa oleifera and propolis on porphyomonas gingivalis biofilms compared to 0.7% tetracycline. Methods: A biofilm inhibition activity test was performed using the broth micro dilution method. First, bacteria were prepared by making a suspension in brain heart infusion media and adjusting it to 0.5 McFarland I standard. Second, fifteen samples were divided into five groups; group K as control group (0.1% sodium carboxymethyl cellulose), T (0.7% tetracycline), and treatment groups with the combination of propolis and Moringa oleifera in various concentrations, such as P1(10%+20%), P2(10%+40%), and P3(10%+80%). Third, the result data obtained in the form of optical density (OD) was read by using an ELISA reader. Next, statistical analysis using analysis of the variance test was conducted (p<0.05. Results: There was no significant difference between group T and group P1 (0.075). Nevertheless, there were significant differences between group T and group P2 as well as between group T and group P3 (0.00) (p=< 0.05). Conclusion: The combination of 10% propolis and 40% Moringa oleifera as well as the combination of 10% propolis and 80% Moringa oleifera have better antibacterial effectiveness against Porphyromonas gingivalis biofilm than 0.7% tetracycline. Keywords: biofilm; Moringa oleifera; P. gingivalis; propolis; tetracycline Correspondence: Hansen Kurniawan, Department of Periodontics, Faculty of Dentistry, Universitas Hang Tuah. Jl. Arif Rahman Hakim No. 150 Surabaya, 60111 Indonesia. Email: hansen.kurniawan@hangtuah.ac.id INTRODUCTION Periodontitis is an inflammatory disease that occurs in the supporting tissues of teeth caused by specific microorganisms triggering inflammation on periodontal ligament and alveolar bone.1 Plaque and calculus bacteria are considered to be the main causes of periodontal disease. Plaque containing pathogenic microorganisms plays an important role in causing damage to the periodontal tissue.2 Porphyromonas gingivalis (P. gingivalis), moreover, is a bacterium commonly associated with periodontitis pathogenesis. Almost 40–100% of periodontitis cases are caused by the opportunistic bacterial antigen of P. gingivalis. The presence of these bacteria in chronic periodontitis patients, according to a previous research on subgingival plaque as much as 85.75%.3 Furthermore, biofilm is a collection of microorganisms in which microbial cells attach to each other on a living or non-living surface, producing their own extracellular polymer matrix.4 Biofilm consists of bacterial cells (5–25%) and glycocalyx matrix (75–95%).5 In addition, biofilm is known as a microbial cell encased in a matrix of extracellular polymeric substances, such as polysaccharides, proteins and nucleic acids.6 In the lower layer of biofilm, microbes are bound together in a polysaccharide matrix with other Dental Journal (Majalah Kedokteran Gigi) p-ISSN: 1978-3728; e-ISSN: 2442-9740. Accredited No. 32a/E/KPT/2017. Open access under CC-BY-SA license. Available at https://e-journal.unair.ac.id/MKG/index DOI: 10.20473/j.djmkg.v54.i2.p63–67 mailto:hansen.kurniawan@hangtuah.ac.id https://e-journal.unair.ac.id/MKG/index http://dx.doi.org/10.20473/j.djmkg.v54.i2.p63-67 64 Kurniawan et al./Dent. J. (Majalah Kedokteran Gigi) 2021 June; 54(2): 63–67 organic and inorganic materials, while on the top layer, there is an amorphous layer extending to the medium around it. The fluid layer adjacent to the biofilm has a stationary and dynamic sub-layer.7 Biofilm is also known to have an extracellular polymeric substance (EPS) matrix that is able to prevent the occurrence of antimicrobial diffusion, and, as a result, bacterial resistance to antibiotics increases while cell metabolic activity on the biofilm decreases.8,9 On the other hand, Moringa oleifera, also known as Moringa, is a plant widely used as a traditional medicine or for mystical therapy in Indonesia.10 Moringa oleifera is also known to have anti-cancer, antibacterial and hypotensive properties that can inhibit bacterial and fungal activities.11 According to Septiyani et al.12 Moringa oleifera extract can be effective in inhibiting the growth of P. gingivalis bacteria at doses of 80% and 40%. Similarly, propolis, according to previous research, has natural antibacterial and antibiotic properties.13 Propolis, one of the natural products produced by honey bees, has been widely used not only as a medicine or supplement, mouth wash, anti-inflammatory and disease therapy, but also for accelerating the wound-healing process. In addition, propolis has many special benefits and potential since it has antibacterial and antiviral properties, so it can inhibit cancer growth.14,15 According to Suryono et al.16 10% propolis even has an ability to inhibit P. gingivalis bacterial activities optimally. Tetracycline is one of the oldest classes of broad- spectrum antibiotics in use. In addition to its antibacterial activity, tetracyclines are also known to have anti- inflammatory, anti-collagenase and wound healing properties, as well as the ability to reduce bone loss.17 Tetracyclines, consequently, can be used as antibiotics for periodontitis cases. The biocompatibility of tetracyclines, mostly studied in the form of tetracycline gel with a concentration of 0.7%, is acceptable for tissue and can remove the smir layer and open dentinal tubules and the collagen matrix.18 Finally, it can be said that propolis and Moringa oleifera contain different secondary metabolites that have anti-bacterial activity. Meanwhile, tetracycline is one of the antibiotics that has been widely used for the therapy of periodontal disease. However, whether the combination of propolis and Moringa oleifera will be as effective as tetracyclines and whether propolis and Moringa oleifera have side effects is still debatable. Therefore, this research aims to explore the antibacterial effectiveness of the combination of propolis extract and Moringa oleifera leaf extract against P. gingivalis biofilms compared to 0.7% tetracycline. MATERIALS AND METHODS This research is a true laboratory experimental research with the post only control group design. In this research, Moringa oleifera extract was prepared with a maceration technique, in which 100 g of Moringa oleifera simplisa powder was put into erlernmeyer, immersed in 500 mL of 96% ethanol solution and covered with aluminium foil for five days, while being stirred occasionally. After five days, the sample was filtered using filter paper to produce filtrate 1 and residue 1. The residue was then added to 250 ml of 96% ethanol solution, covered with aluminium foil for two days, being stirred occasionally.11 After two days, the sample was filtered using filter paper to produce filtrate 2 and residue 2, then mixed into one and evaporated using a rotary evaporator to obtain Moringa oleifera extract. The Moringa oleifera extract obtained was kept in a water bath until all the ethanol solvent evaporated. The extract obtained was then weighed and stored in a closed glass container before used for testing. In total there were three test solutions made, namely Moringa oleifera extract at a concentration of 20% (0.2:0.8), Moringa oleifera extract at a concentration of 40% (0.4:0.8), and Moringa oleifera extract at a concentration of 80% (0.8:0.2).11 Afterwards, 800 g of propolis was cooled in a refrigerator, then put in an oven at 40°C for three days, and 2L of 70% ethanol liquid was added. To speed up the dissolving process, propolis was crushed with a stirrer and allowed to stand for a moment.18 After that, the propolis was stirred every day and filtered, but the obtained filtrate was left to stand to precipitate substances that were not needed, but not dissolved in ethanol. The remaining filtrate was then put into a 90% ethanol solution. All of these steps were repeated three to five times, and the filtering process was also repeated three times until a thick propolis extract was obtained. Next, 0.1 g of the thick propolis extract was dissolved in 1 mL of 0.1% sodium carboxymethyl cellulose (Na CMC) so that the concentration of the propolis extract obtained became 10%.19 Subsequently, 0.7% tetracycline was prepared. First, tetracycline tablets were crushed. Afterwards, 175 mg of the crushed tetracycline was dissolved in 25 ml of aquadest.20 Next, Moringa oleifera extract and propolis at various concentrations were mixed in a ratio of 1:1. Meanwhile, 0.1% Na CMC solution was divided into several groups. First, in the control group (K), 0.1 mL of P. gingivalis biofilm mixed with 0.1 mL of 0.1% Na CMC was put on a microtiter plate. Second, in the tetracycline (T) group, 0.1 mL of P. gingivalis biofilm mixed with 0.1 mL of 0.7% tetracycline was put on a microtiter plate. Third, in treatment group 1 (P1), 10% propolis extract mixed with 0.1 mL of 20% Moringa oleifera leaf extract was put on a microtiter plate. Fourth, in treatment group 2 (P2), 10% propolis extract mixed with 0.1 mL of 40% Moringa oleifera leaf extract was put on a microtiter plate. And, in treatment group 3 (P3), 10% propolis mixed with 0.1 mL of 80% Moringa oleifera leaf extract was put on a microtiter plate. After that, a detection test for the formation of P. gingivalis bacterial biofilm was carried out using the congo red agar (CRA) method. First, P. gingivalis bacteria were inoculated on congo red agar and incubated for 48 hours at Dental Journal (Majalah Kedokteran Gigi) p-ISSN: 1978-3728; e-ISSN: 2442-9740. Accredited No. 32a/E/KPT/2017. Open access under CC-BY-SA license. Available at https://e-journal.unair.ac.id/MKG/index DOI: 10.20473/j.djmkg.v54.i2.p63–67 https://e-journal.unair.ac.id/MKG/index http://dx.doi.org/10.20473/j.djmkg.v54.i2.p63-67 65Kurniawan et al./Dent. J. (Majalah Kedokteran Gigi) 2021 June; 54(2): 63–67 37°C under anaerobic conditions. Congo red agar that can interact directly with polysacharida intercellular adhesion formed a colour complex. After 48 hours, the plates were examined. If black colonies were formed, this indicated that the bacterial strain had produced biofilms. Meanwhile, if the colony showed a red colour, this illustrated that the strain had not formed any biofilm.21 In addition, a biofilm inhibition test was conducted by using the broth micro dilution method. First, bacteria were prepared by making a suspension in a brain heart infusion (BHI) media and adjusted to 0.5 McFarland I standard. Second, the equalized suspension of P. gingivalis bacteria was then diluted to a ratio of 1:100. Third, the bacterial suspension was inserted into a 96-well round bottomed plastic tissue culture plate (microtiter plate) with a total volume of 0.1 mL (100 µL)/ in each well using a micropipette. Fourth, observation was conducted on each test plate and each blank plate. Fifth, the test plate filled with a bacterial suspension was put on microtiter plate and then incubated at 37°C for 24 hours. Sixth, after 24 hours, the microtiter plate was removed from the incubator, and then the test extract solution was inserted into the microtiter plate filled with bacterial suspension, while the blank plate was filled with the test extract solution without bacteria. Seventh, the microtiter plate was put back into the incubator for 24 hours.22 Eighth, the microtiter plate was removed from the incubator, and then the test solution was discarded and washed three times with 0.2 mL of phosphate buffer saline. Ninth, the microtiter plate was dried, and then 0.2 mL (200 µL) of 1% crystal violet was added to each well and left to stand for 15 minutes. Tenth, it was rinsed using distilled water and then dried for 15 minutes in an incubator at 37°C. In the last step, 0.2 mL of 2% 80 Tween was added to each microtiter plate.22 Next, an optical density (OD) test was performed. The values of density (OD) values obtained and were read using an ELISA reader at a wavelength of 515 nm. Afterwards, the inhibitory power of biofilm formation generated from the test solution was measured by the following formula: Note: ODs : Optical density (515 nm) of tested sample ODbs : Optical density of blank sample ODp : (OD of test solvent - OD of blank solvent) The reading results of the optical density values obtained with the ELISA reader were in the form of quantitative data. The data were then tested using the one-way analysis of variance (ANOVA) test. RESULTS The research data were analysed descriptively to depict the distribution of data as well as summarise the characteristics of data in order to clarify the presentation of the data results. The data shown in Table 1 illustrates that the highest mean percentage of P. gingivalis biofilm inhibition was in the P3 group, with a value of 72.4, while the lowest mean percentage was in the K group, with a value of 0. Moreover, it also demonstrates that the mean percentage of P. gingivalis biofilm inhibition in the T group was 31.8, 36.4 in the P1 group, and 57.8 in the P2 group. Based on Table 2, the results of the LSD test showed that there was a significant difference in the percentage value of biofilm inhibition (p <0.05) in all groups, except between T and P1 (0.075> 0.05). DISCUSSION The prevalence and severity of periodontal disease can be reduced by scaling root planning and antibacterial therapy. The antibacterial therapy often used to treat periodontal disease is tetracycline. Hence, this study aims to see the effect of Moringa oleifera extract at concentrations of 20%, 40% and 80% combined with 10% propolis on the biofilm formation of P. gingivalis bacteria strain ATCC 33277, compared with 0.7% tetracycline. Moringa oleifera is known to have antibacterial ability in P. gingivalis at concentrations of 40% and 80%.12 Similarly, propolis is also known to have antibacterial ability against P. gingivalis bacteria.23 The inhibition ability of Moringa oleifera is known to be caused by a variety of active metabolic compounds it contains. Not only does Moringa oleifera contain great antibacterial properties consisting of saponins, triterpenoids and tannins, which work by damaging cells from bacteria, but also flavonoids as antioxidants playing a role in damaging the permeability of bacterial cell walls, microsomes and lysosomes as a result of the interaction between flavonoids and bacterial DNA.24 Table 1. The average (%) of P. gingivalis bacterial biofilm inhibition Group Mean (%) Std. Deviation K 0 0 T 31.8 3.76051 P1 36.4 0.71531 P2 57.8 3.40274 P3 72.4 2.10350 Table 2. The results of LSD Post-Hoc test Group T P1 P2 P3 K 0.000* 0.000* 0.000* 0.000* T 0.075 0.000* 0.000* P1 0.000* 0.000* P2 0.000* * p <0.05 (There are differences) Dental Journal (Majalah Kedokteran Gigi) p-ISSN: 1978-3728; e-ISSN: 2442-9740. Accredited No. 32a/E/KPT/2017. Open access under CC-BY-SA license. Available at https://e-journal.unair.ac.id/MKG/index DOI: 10.20473/j.djmkg.v54.i2.p63–67 https://e-journal.unair.ac.id/MKG/index http://dx.doi.org/10.20473/j.djmkg.v54.i2.p63-67 66 Kurniawan et al./Dent. J. (Majalah Kedokteran Gigi) 2021 June; 54(2): 63–67 Propolis, on the other hand, is a natural material collected by honey bees from various plants, such as poplar, palm, pine, coniferous secretions, sap, resin, mucus and leaf buds. It is collected and carried by honey bees and used to seal the gaps in their hives. Initially, it acts as an antiseptic that prevents the beehive from microbial infection as well as the decomposition of intruders.25 Propolis is known to have antibacterial, anti-viral, anti-fungal, antioxidant and anti- inflammatory functions that enhance the body’s system.26 Propolis is also known to contain amino acids, terpenoids and polyphenols (phenolic acids, esters and flavonoids).27 Flavonoid is one of the important ingredients in propolis, and has antioxidant, anti-cancer, anti-inflammatory, allergy, antiviral and antibacterial effects.28–30 Hence, flavonoids can eliminate the permeability of P. gingivalis bacterial cells.31 Flavonoids can damage bacterial cells by lysing bacteria through protein binding so that bacteria will die.32 According to the study of Asdar and Cindrakori, propolis contains apigenin and tt-farnesol which can decrease the amount of polysaccharides in the biofilm of microorganisms, so the biofilm formation can be stopped.33 Previous research conducted by Septiyani et al.12 shows that Moringa oleifera extract at concentrations of 40% and 80% was able to reduce the biofilm formation of P. gingivalis bacteria. This previous research also reveals that 20% Moringa oleifera extract combined with 10% propolis even can inhibit the biofilm formation of P. gingivalis bacteria. Therefore, it can be said that based on this previous research, the combination of 10% propolis extract and 20% Moringa oleifera extract can be used for an alternative antimicrobial treatment as effective as 0.7% tetracycline. Meanwhile, the combination of 10% propolis and 40% Moringa oleifera as well as the combination of 10% propolis and 80% Moringa oleifera can be more effective than tetracycline 0.7%. Hence, two materials can be used synergistically to inhibit the biofilm formation of P. gingivalis bacteria. Finally, it can be concluded that the combination of propolis extract and Moringa oleifera can generate antibacterial power to inhibit the biofilm formation of P. gingivalis bacteria. It is also known that 10% propolis and 20% Moringa oleifera have antibacterial power as great as 0.7% tetracycline. 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Accredited No. 32a/E/KPT/2017. Open access under CC-BY-SA license. Available at https://e-journal.unair.ac.id/MKG/index DOI: 10.20473/j.djmkg.v54.i2.p63–67 https://e-journal.unair.ac.id/MKG/index