Introduction

Oral candidiasis is a fungal infection of the oral cavity1, manifested as superficial mucosal lesions, or deep and highly severe lesions due to immune suppression2. It is caused by Candida species, principally Candida albicans3, which has resistance to a range of antifungal drugs4 because of their uncontrolled use5. Besides, C. albicans was found in the root canal system of teeth with periapical lesions6 and has a potential role in the development of the periodontal diseases7,8.

Phytotherapy was indicated for the treatment of some oral conditions because of its biocompatibility, antimicrobial, anti-inflammatory and antioxidant properties9,10,11,12. Rosmarinus officinalis L. popularly called rosemary, is an ancient shrub belonging to the family Lamiaceae and originated from the Mediterranean region13. This herbal medicine has promising biological effects including antimicrobial, antibiofilm, anti-inflammatory, antioxidant, anti-ulcer, antiviral and anticancer effects14,15,16,17,18, besides, it improves memory performance and sleep quality, and reduces anxiety and depression19.

The antifungal effect of R. officinalis was tested against C. albicans, C. dubliniensis, C. glabrata, C. krusei, and C. tropicalis where it was as effective as nystatin20. However, to the best of our knowledge, there is no studies that evaluated the antifungal effect against C. albicans in Galleria mellonella model like other herbal medicines21,22 as in vivo models provides an opportunity to assess the prophylactic potential of a compound acting on the host’s immune system23. Besides, G. mellonella is an adequate an invertebrate model organism to test the antimicrobial action over diverse materials over microorganisms like streptococcus, Escherichia coli, and Klebsiella pneumoniae24,25,26.

This study was elaborated to understand the antifungal effect of R. officinalis and is trying to present this herbal medicine as an alternative medication for oral candidiasis, intracanal medication, endodontic irrigant, or toothpaste and mouthwash component. Therefore, the aim of this study was to evaluate the antifungal effect of R. officinalis against C. albicans and its biocompatibility in G. mellonella model. The null hypothesis was that the R. officinalis has no antifungal effect and it is not biocompatible.

Materials and methods

Plant extract and bacterial strain

Rosmarinus officinalis glycolic extract was obtained of the flowers and leaves of rosemary and formulated at a concentration of 20% (200 mg/mL of the extract) in propylene glycol (Mapric®, São Paulo, SP, Brazil). The extracts were not manipulated in our laboratory, instead they were obtained in a commercial form composed of essential oil made up of terpenic derivatives (pinene, camphene, free borneol, acetate, cineole, camphor); sesquiterpenes; oleanolic acid; tannin; bitter substances; acid saponin and glucoside compounds according to the manufacturer (Mapric®, São Paulo, SP, Brazil).

A standard strain of C. albicans (ATCC 18804) was used in this study. The microorganisms were frozen in BHI broth containing 20% glycerol at − 80 °C. At the moment of use, the microorganisms were seeded on CHROM agar to guarantee the absence of contamination. Only C. albicans colonies that showed green color were used in this study, in which were cultured on Sabouraud Dextrose agar (Himedia Laboratories, Munbai, India) using the depletion technique and incubated for 48 h at 37 °C. Then, the colonies were transferred to the Yeast extract–Peptone–Dextrose (YPD) broth medium and incubated at 37 °C for 24 h.

Inoculum preparation and G. mellonella selection

The inoculum was prepared and standardized following an anterior protocol reported in the literature27. After 24 h incubation in YPD broth, the fungal cells were isolated by centrifugation at 5000 rpm for 10 min, and the supernatant was discarded. The remaining deposit was resuspended in PBS, and vortexed for 30 s. This process was repeated two more times. The standardization of the inoculum was performed using a hemocytometer at 106 cells/larva to be used for the following tests.

Galleria mellonella larvae were obtained from the Invertebrate Laboratory belonging to the Microbiology and Immunology Department of the Institute of Science and Technology of São Paulo State University (ICT-Unesp). Only larvae (I) weighing from 250 to 300 mg; (II) in the last larval stage; (III) light colored; and (IV) without spots or dark pigments in their cuticle were used in this study to avoid the involvement of a probable infectious process.

The larvae cleaning and feeding were carried out three times a week. The diet was based on wax, and the ration was composed of 25% cornmeal, 15% brewer’s yeast, 10% soy flour, 10% skimmed milk, 20% honey and 20% glycerol, prepared in-house. The larvae were kept at 25 °C until use. After receiving the treatment, the larvae were not fed.

Evaluation of toxicity in G. mellonella model

Four different concentrations (50; 25; 12.5 and 6.25 mg/mL) of R. officinalis glycolic extract at 20% diluted in Phosphate Buffered Saline (PBS) and five different concentrations (100; 50; 25; 12.5 and 6.25%) of nystatin (oral suspension 100,000 IU/mL—Germed) diluted in sterile distilled water were evaluated. The extracts were inoculated in the last right proleg of each larva totaling the n = 15 for each concentration. PBS and another group with no injection were used as control groups.

An aliquot of 10 µL of each concentration was inoculated using Hamilton syringes (Hamilton Inc., USA), then the larvae were kept in Petri dishes at 37 °C in the dark, without nutrition. After 24 h of inoculations, the number of dead G. mellonella larvae was recorded daily until 168 h (7 days) for analysis of the survival curve. Larvae were considered dead when they presented no movement after touch. After obtaining non-toxic concentrations of the plant extract and nystatin in G. mellonella, these concentrations were used to evaluate the antifungal action of R. officinalis L. on C. albicans.

Evaluation of antifungal effect of R. officinalis L. on C. albicans

After determining the non-toxic concentrations of the plant extract, the larvae were randomly divided into six groups (n = 15) and treated according to the following protocols at phase I of the test:

  • Group 1 (Ro 25 mg/mL for 24 h + C. albicans): the larvae were inoculated with 10 µL of R. officinalis extract (25 mg/mL) in the last right proleg, and after 24 h were inoculated with 10 µL C. albicans inoculum in the last left proleg.

  • Group 2 (PBS for 24 h + C. albicans): the larvae were inoculated with 10 µL of PBS in the last right proleg, and after 24 h were inoculated with 10 µL C. albicans inoculum in the last left proleg.

  • Group 3 (C. albicans for 1 h + Ro 25 mg/mL): the larvae were inoculated with 10 µL C. albicans inoculum in the last right proleg, and after 1 h were inoculated with 10 µL of R. officinalis extract (25 mg/mL) in the last left proleg.

  • Group 4 (C. albicans for 1 h + PBS): the larvae were inoculated with 10 µL C. albicans inoculum in the last right proleg, and after 1hwere inoculated with 10 µL of PBS in the last left proleg.

  • Group 5 (C. albicans for 1 h + 25% nystatin): the larvae were inoculated with 10 µL C. albicans inoculum in the last right proleg, and after 1hwere inoculated with 10 µL of 25% nystatin in the last left proleg.

  • Group 6 (PBS for 1 h + PBS): the larvae were inoculated with 10 µL PBS in the last right proleg, and after 1hwere inoculated with 10 µL of PBS in the last left proleg.

Groups (Ro 25 mg/mL for 24 h + C. albicans) and (PBS for 24 h + C. albicans) were simulating the prophylactic effect, in which the extracts were inoculated before the infection exists. However, in groups (C. albicans for 1 h + Ro 25 mg/mL), (C. albicans for 1 h + PBS) and 5, the treatment was applied after the infection, simulating therapeutic effect. Lastly, group (PBS for 1 h + PBS) was considered as a negative control group. After the injections, the larvae were kept in Petri dishes at 37 °C in the dark. The number of dead larvae was observed and recorded daily for 7 days to obtain the survival curve.

Posteriorly, phase II was performed in which the groups were divided as the following:

  • Group 7A: (Ro 12.5 mg/mL for 72 h + C. albicans): the larvae were inoculated with 10 µL of R. officinalis extract (12.5 mg/mL) each 24 h totaling 3 doses in different prolegs, after 24 h were inoculated with 10 µL C. albicans inoculum in a different proleg.

  • Group 7B: (Ro 6.25 mg/mL for 72 h + C. albicans): the same of group (Ro 12.5 mg/mL for 72 h + C. albicans). However, the extract concentration was of 6.25 mg/mL.

  • Group 8A: (Ro 12.5 mg/mL for 48 h + C. albicans): the larvae were inoculated with 10 µL of R. officinalis extract (12.5 mg/mL) each 24 h totaling 2 doses in different prolegs, after 24 h were inoculated with 10 µL C. albicans inoculum in a different proleg.

  • Group 8B: (Ro 6.25 mg/mL for 48 h + C. albicans): the same of group (Ro 12.5 mg/mL for 48 h + C. albicans). However, the extract concentration was of 6.25 mg/mL.

  • Group 9A: (Ro 12.5 mg/mL for 24 h + C. albicans): the larvae were inoculated with 10 µL of R. officinalis extract (12.5 mg/mL) (1 dose), after 24 h were inoculated with 10 µL C. albicans inoculum in a different proleg.

  • Group 9B: (Ro 6.25 mg/mL for 24 h + C. albicans): the same of group (Ro 12.5 mg/mL for 24 h + C. albicans). However, the extract concentration was of 6.25 mg/mL.

  • Group 10: (PBS for 24 h + C. albicans): the larvae were inoculated with 10 µL of PBS, after 24 h were inoculated with 10 µL C. albicans inoculum in a different proleg.

  • Group 11: (PBS for 24 h + PBS): the larvae were inoculated with 10 µL of PBS, after 24 h were inoculated with 10 µL PBS in a different proleg.

Phase 2 was performed to evaluate the difference between 1, 2 and 3 doses of the extract for prophylactic effect, in which the extracts were inoculated before the infection exists as in groups (Ro 12.5 mg/mL for 72 h + C. albicans), (Ro 6.25 mg/mL for 72 h + C. albicans), (Ro 12.5 mg/mL for 48 h + C. albicans), (Ro 6.25 mg/mL for 48 h + C. albicans), (Ro 12.5 mg/mL for 24 h + C. albicans) and (Ro 6.25 mg/mL for 24 h + C. albicans). Groups (PBS for 24 h + C. albicans) and (PBS for 24 h + PBS) were considered as control groups. After the injections, the larvae were kept in Petri dishes at 37 °C in the dark. The number of dead larvae was observed and recorded daily for 7 days to obtain the survival curve.

Statistical analysis

Galleria mellonella survival curves were plotted using the Kaplan–Meier method and statistical analysis was performed using the log-rank test (Mantel–Cox). The analyzes were performed using the GraphPad Prism statistical software and the significance level was set at (α < 0.05).

Results

Evaluation of toxicity in G. mellonella model

In the control groups and R. officinalis extracts (6.25, 12.5 and 25 mg/mL), all larvae survived after 7 days. R. officinalis extracts (50 mg/mL) caused death rate of 6.6% of the larvae. However, there was no significant difference among the groups (Fig. 1A).

Figure 1
figure 1

Galleria mellonella survival curve after inoculation of Rosmarinus officinalis glycolic extract and nystatin in different concentrations. (A) To compare the biocompatibility of different concentrations of the Rosmarinus officinalis glycolic extract with the control group (PBS). (B) To compare the biocompatibility of different concentrations of the nystatin with the control group (PBS).

Conversely, PBS and nystatin (6.25 and 12.5 mg/mL) where biocompatible, however, there was a death rate 6.6% with nystatin 25%, 13.3% with nystatin 50% and 26.6% with nystatin 100% (Fig. 1B) with p value = 0.034.

Evaluation of antifungal effect of R. officinalis L. on C. albicans

When evaluating the prophylactic treatment groups, it was found that group (Ro 25 mg/mL for 24 h + C. albicans) promoted an increase in the survival of the larvae in comparison with group (PBS for 24 h + C. albicans) in the first 24 h in which the survival rate was 57.2% with the group (PBS for 24 h + C. albicans); 92.9% with the group (Ro 25 mg/ mL for 24 h + C. albicans); and 100% with the control group (PBS for 1 h + PBS). After 7 days, there was no statistically significant difference among the prophylactic treatment groups (Fig. 2A).

Figure 2
figure 2

Galleria mellonella survival curve after treatment with different groups. (A) To compare the antifungal action of the prophylactic groups with the control group (PBS + PBS). (B) To compare the antifungal action of the therapeutic groups with the control group (PBS + PBS). Ca Candida albicans, Ro Rosmarinus officinalis, Nys Nystatin.

When evaluating the therapeutic treatment groups, there was no significant difference between groups (C. albicans for 1 h + Ro 25 mg/mL) and (C. albicans for 1 h + PBS). However, group (C. albicans for 1 h + 25% nystatin) presented a significant difference in comparison with the groups (C. albicans for 1 h + Ro 25 mg/mL) and (C. albicans for 1 h + PBS) as it promoted the survival rate of the larvae up to 60% after 7 days (Fig. 2B).

In phase 2 of the analysis, there was a significant difference between the group (Ro 12.5 mg/mL for 24 h + C. albicans) and (PBS for 24 h + C. albicans) (p = 0.032); however, there was no significant difference between the groups (Ro 12.5 mg/mL for 48 h + C. albicans) and (PBS for 24 h + C. albicans) (p = 0.09). In Fig. 3A, it was observed that in the 4th day, the survival rate with group (PBS for 24 h + C. albicans) was 26.7% and with the group (Ro 12.5 mg/mL for 24 h + C. albicans) was 57.2%.

Figure 3
figure 3

Galleria mellonella survival curve after treatment with different groups. (A) To compare the antifungal action of the prophylactic groups of 12.5 mg/mL with the control group (PBS + PBS). (B) To compare the antifungal action of the prophylactic groups of 6.25 mg/mL with the control group (PBS + PBS). Ca Candida albicans, Ro Rosmarinus officinalis, Nys Nystatin.

Besides, there was a significant difference between the group (Ro 6.25 mg/mL for 72 h + C. albicans) and (PBS for 24 h + C. albicans) (p = 0.017). After 7 days, 100% of the larvae were dead with the group (PBS for 24 h + C. albicans), and the survival rate was 35% with the group (Ro 12.5 mg/mL for 24 h + C. albicans). In the 3rd day, it was verified that the survival rate was of 79.4% with the group (Ro 6.25 mg/mL for 72 h + C. albicans) and 26.6% with the group (PBS for 24 h + C. albicans). After 7 days, all larvae in the group (PBS for 24 h + C. albicans) had died and the survival rate in the group (Ro 6.25 mg/mL for 72 h + C. albicans) was 14.4% (Fig. 3B).

The groups (Ro 6.25 mg/mL for 72 h + C. albicans) and (Ro 12.5 mg/mL for 24 h + C. albicans) promoted the survival rate of the larvae in comparison with the group (PBS for 24 h + C. albicans) with a significant difference (p = 0.017) e (p = 0.032) respectively.

Discussion

Candida albicans are opportunistic microorganisms, that may cause a fungal infection, as in situations where the immune system is compromised like in coronavirus disease 19 (COVID-19) infections caused by severe acute respiratory syndrome of coronavirus-2 (SARS-CoV2), making the clinical course of these patients more complicated28,29. The aim of this study was to evaluate the antifungal effect of R. officinalis against C. albicans and its biocompatibility in G. mellonella model. It was found that the extract has an effective antifungal effect against C. albicans and is biocompatible thus the null hypothesis was rejected.

In this study it was found that, R. officinalis extracts (6.25, 12.5 and 25 mg/mL) were as biocompatible as the control group in which all the larvae survived after 7 days. However, R. officinalis extract of 50 mg/mL caused death rate of 6.6% of the larvae. Still, there was no significant difference among the groups (Fig. 1A). To the best of our knowledge, there are no studies in the literature that evaluated the toxicity of R. officinalis in G. mellonella model. However, in the literature, it was found that rosemary products such as extracts and essential oils do not present toxicity over fibroblasts and macrophages30,31. Besides, some reports on the use of the R. officinalis extract in murine models were found: the administration of a single dose of R. officinalis extract at a concentration of 2000 mg/kg in rats was described to be safe32 and the single lethal dose median (LD50) of rosemary essential oil in rats was 4753.3 mg/kg33.

Galleria mellonella model is an adequate model to test the toxicity of medicinal plants, in a recent study, the model was used to test seven well known plants from Cameroon using the G. mellonella larvae, in which it was found that the plant materials and the extracts type (ethanolic or aqueous) affect the toxicity34. In the present study, the dead larvae counting was recorded until 7 days as reported in anterior studies in the literature27,35.

The results of the present study are significant since there are no reports in the literature about the biocompatibility of the commercially used nystatin suspension on G. mellonella. The R. officinalis extract of 50 mg/mL presented a death rate of only 6.6% of the larvae, compared to nystatin, the main antifungal administered in cases of oral candidosis, which presented a death rate of 26.6% when administered alone.

On the other hand, the antifungal action of R. officinalis extracts were evaluated in G. mellonella model as in the protocol of another study36. In this study, the therapeutic inoculation with the antifungal agent was performed after 1 h of infection to maintain a survival rate of 60% of the larvae; however, in another study the antimicrobial treatment was performed 3 h after infection37.

In phase 1 of the present study, it was found that there was no significant difference between groups (C. albicans for 1 h + Ro 25 mg/mL) and (C. albicans for 1 h + PBS), the therapeutic treatment groups. However, group (C. albicans for 1 h + 25% nystatin) presented a significant difference in comparison with the groups (C. albicans for 1 h + Ro 25 mg/mL) and (C. albicans for 1 h + PBS) as it promoted the survival rate of the larvae up to 60% after 7 days (Fig. 2B). In the literature, R. officinalis L. extract showed antifungal effect on Candida spp. without a significant difference with nystatin in vitro20; however, they were not tested in in G. mellonella model as in the present study.

In a comparative analysis, it is possible to verify that the prophylactic protocol of group (Ro 25 mg/mL for 24 h + C. albicans) promoted greater survival of the larvae, since on the first day of counting, most of the larvae survived and then the survival curve declined. However, even at the end of the 7th day of counting, there were still surviving larvae in the group previously treated with extract. When the prophylactic group was compared to the group (PBS for 24 h + C. albicans) with the p value = 0.08.

In another study, the prophylactic potential of using Lactobacillus spp. on G. mellonella infected by Candida spp. was verified 24 h before the infection, while the conventional treatment occurred after 30 min of the yeast inoculation. At the end of the study, the results showed benefits in the use of the prophylactic protocol because the larvae that were inoculated with Lactobacillus spp. prophylactically had a longer survival compared to those who received conventional treatment38. This finding corroborates our results, in which the group that received prophylactic treatment (24 h before infection) with 25 mg/mL of R. officinalis extract had greater survival than the group with conventional treatment.

In phase 2 of this study, the groups (Ro 6.25 mg/mL for 72 h + C. albicans) and (Ro 12.5 mg/mL for 24 h + C. albicans) of 12.5 mg/mL for 24 h as prophylactic treatments promoted the survival rate of the larvae in comparison with the group (PBS for 24 h + C. albicans) with a significant difference (p = 0.017) e (p = 0.032) respectively.

Almeida et al. evaluated the antifungal potential of pomegranate in vivo on G. mellonella infected by C. albicans. After comparative analysis of the prophylactic and therapeutic protocols using the plant extract, the study reported that prophylaxis with pomegranate had better results39, which is in line with our findings. In their study, only one concentration of pomegranate was tested, while in the present study, a total of three concentrations of rosemary were tested. The same study verified that with multiple administrations of the plant extracts before fungal infection the percentage of larvae survival was higher when compared to prophylaxis in a single dose.

The initial mechanisms of the larval immune response to the infectious process can be divided into two phases: (I) phase 1 corresponds to the first 6 h, in which there is a decrease in fungal load, which can be correlated with an increase in hemocyte density and an increase in antimicrobial peptides and immune system proteins; (II) phase 2, from 6 to 24 h, yeast cells proliferate and the number of hemocytes decreases, resulting in larval death40. The results of the present study suggest that these deleterious effects on the immune system of the larvae caused by C. albicans infection were attenuated by the prophylactic administration of rosemary extract, since the antimicrobial activity of the plant extract is already well founded41. The present study elucidated important findings on the application of R. officinalis extract against C. albicans, mainly on the prophylactic action. The contributions of this in vivo study are relevant and notorious for the advancement of research on the biological properties of this plant.

Conclusion

The prophylactic antifungal effect found in this study suggest the use of R. officinalis extract as an alternative medication for fungal infection.