Evaluation of the In Vitro Wound-Healing Activity and Phytochemical Characterization of Propolis and Honey
by
, and
Alexandra M. Afonso
1, 
Joana Gonçalves
1,2,†,
Ângelo Luís
1,2,*,†,
Eugenia Gallardo
1,2 and
Ana Paula Duarte
1,2,*
1
Centro de Investigação em Ciências da Saúde (CICS-UBI), Universidade da Beira Interior, Avenida Infante D. Henrique, 6200-506 Covilhã, Portugal
2
Laboratório de Fármaco-Toxicologia, UBIMedical, Universidade da Beira Interior, Estrada Municipal 506, 6200-284 Covilhã, Portugal
*
Authors to whom correspondence should be addressed.
†
These authors contributed equally to the work.
Appl. Sci. 2020, 10(5), 1845; https://doi.org/10.3390/app10051845
Submission received: 17 February 2020
/
Revised: 28 February 2020
/
Accepted: 4 March 2020
/
Published: 7 March 2020
(This article belongs to the Special Issue Biological Activity and Applications of Natural Compounds)
Abstract
:Honey and propolis are natural substances produced by Apis mellifera that contain flavonoids, phenolic acids, and several other phytochemicals. The aim of this study was to phytochemically characterize three different types of honey and propolis, both separately and mixed, and to evaluate their wound-healing activity. Total phenolic compounds and flavonoids were determined using the Folin–Ciocalteu’s and aluminum chloride colorimetric methods, respectively. The antioxidant activity was evaluated by both the DPPH free radical scavenging assay and β-carotene bleaching test, and the anti-inflammatory activity was determined by a protein denaturation method. To evaluate the wound-healing activity of the samples, NHDF cells were subjected to a wound scratch assay. The obtained results showed that dark-brown honey presents a higher concentration of phenolic compounds and flavonoids, as well as higher antioxidant and anti-inflammatory activities. Propolis samples had the highest concentrations in bioactive compounds. Examining the microscopic images, it was possible to verify that the samples promote cell migration, demonstrating the wound-healing potential of honey and propolis.
1. Introduction
Honey is a natural substance produced by the western honeybee (Apis mellifera) from nectar and exudates of flowers and trees. Honey contains flavonoids, phenolic compounds, and numerous sugars in its composition, mainly glucose and fructose. It also contains small amounts of minerals, vitamins, proteins, and enzymes [1,2,3,4,5].
Propolis is a resinous substance produced by the same species of bees, being composed of wax, resinous secretions from plants, tree buds, pollen, and salivary enzymes. Propolis contains essential oils and organic compounds such as phenolic acids and flavonoids [4,6,7,8]. Similarly to honey, propolis also contains several minerals, vitamins, and enzymes [9]. This substance is used to protect the beehive, acting as a natural sealant, antiseptic, and embalming agent [1,4,6,7,8,10].
The color and flavor of both honey and propolis vary according to the plant species used in their production, health state of the bees, season, and the environmental conditions to which the beehive is exposed [2,3,4,5]. The color of the honey can vary from deep brown to yellow, and propolis can be found in variations of green, red, or brown [6,7,11]. Differences in their composition result in different biological activities [1,4,7,12]. Honey and propolis have been used in traditional medicine for thousands of years mainly in burns and infected lesions [4,10]. Propolis was used primarily as an oral antiseptic and in dermal lesions. In ancient Egypt, propolis was also employed in mummification [6].
The main mechanism of action of honey derives from its antioxidant and anti-inflammatory activities [1,2,10]. The antioxidant potential of honey is due to the presence of phenolic compounds, namely gallic acid and flavonoids, that promote the free radical scavenging [2,10]. Its anti-inflammatory activity is associated with the ability to increase cellular proliferation, autolytic debridement, and to stimulate the immune system, reducing edema and pain [10]. Propolis has a higher content in flavonoids and phenolic acids than honey, which suggests that propolis should have a higher antioxidant and anti-inflammatory activities [1,7].
Currently, an increasing interest in mixing propolis with honeys was verified, as products including propolis are already available on the market. The commercial achievement of these products is dependent of the level of acceptance and expectations of the consumers [1]. However, the potential benefits of adding propolis to honeys is still to be scientifically validated.
Wounds are responsible for the consumption of large amounts of healthcare resources to ameliorate the quality of life of patients, and so they represent a considerable health challenge. Several scientific experiments have been performed to find novel compounds that possess wound-healing properties, particularly from natural sources [13]. Honey was employed for the repair of battle wounds in both World War I and in modern history. The healing activity of honey in infected wounds was initially described in Europe and USA in mid-20th century [10]. Moreover, evidences suggest that propolis has therapeutic activity, through quantitative and qualitative analyses of collagen types I and III expression and degradation in wounds matrix, which suggests the favorable biochemical environment supporting re-epithelization of propolis [11].
The first aim of this study was to phytochemically characterize different samples of honey and propolis together with mixtures of propolis extracts with honey in different concentrations, determining the contents in total phenolic compounds and flavonoids, as well as evaluating the antioxidant and anti-inflammatory activities. The second purpose of this work was to evaluate the in vitro wound-healing activity of the samples using normal human dermal fibroblasts (NHDF) by means of the scratch assay.
2. Materials and Methods
2.1. Honey and Propolis Samples
Honey and propolis samples were collected from a Langstroth beehive in a mountainous forest in the north central Portugal, specifically in the region of Sabugal (Guarda) during September 2018 (GPS coordinates: 40°23′33.5″ N 7°03′45.4″ W).
Three different samples of honey and propolis were collected from the same beehive to maintain consistent the conditions of production. Each honey sample was collected from a different box inside the hive and was then filtered individually until there was no visible debris or particles. Propolis samples were scraped from the boxes and frames of the hive and then separated according to the box from which they were collected. All samples were stored individually in an appropriate sterilized container.
Dark-brown honey was considered as Honey 1 (H1), red honey was labeled as Honey 2 (H2), and light-yellow honey was identified as Honey 3 (H3). Propolis samples were named according to the box from which the honey samples were collected as Propolis 1 (P1), Propolis 2 (P2), and Propolis 3 (P3).
2.2. Propolis Extracts
The samples of propolis were grounded individually in a marble mortar at room temperature. To start the extraction process, 100 mL of ethanol (Scharlab, Spain) were added to 14 g of each pulverized propolis sample. The mixtures were left for 48 h under magnetic stirring at room temperature and in the absence of light. After 48 h, the mixtures were filtered and transferred to round bottom flasks to evaporate the ethanol using a rotary evaporation system at 45 °C. To ensure the complete evaporation, the round bottom flasks were kept in a vacuum oven for 24 h at 35 °C.
The propolis extracts were labelled as Propolis Extract 1 (PE1), Propolis Extract 2 (PE2), and Propolis Extract 3 (PE3) and were frozen at −20 °C until they were used.
2.3. Mixtures of Honey with Propolis
Each propolis extract was added in a concentration of 0.3% (w/w) and 0.5% (w/w) to the Honey 1 (the one that presented the best results), according to the previously published work dealing with the evaluation of the bioactive properties of honey with propolis [1]. The mixtures were prepared by weighting the corresponding amounts of honey and propolis and mixing them to complete 100 g of each mixture. To guarantee the complete homogenization, all mixtures were subjected to mechanical stirring, after which they were stored at −20 °C until further use.
The mixtures were identified as Honey 1 followed by the corresponding Propolis Extract and percentage added resulting in Honey 1-Propolis Extract 1 (H1PE1), Honey 1-Propolis Extract 2 (H1PE2) and Honey 1-Propolis Extract 3 (H1PE3) at 0.3% or 0.5%.
2.4. Fourier-Transform Infrared Spectroscopy (FTIR)
FTIR was used to obtain spectra of the samples of honey, propolis and propolis extracts. These spectra were obtained with 64 scans and a 4 cm−1 resolution, between 4000 and 600 cm−1 using a Nicolet iS10 smart iTRBasic (Thermo Fisher Scientific, Waltham, MA, USA) model.
2.5. Phytochemical Characterization
For the phytochemical characterization, all the samples were diluted with methanol (Scharlab, Spain).
2.5.1. Total Phenolic Compounds Determination
The phenolic compounds were determined by Folin–Ciocalteu’s colorimetric method [14,15], using gallic acid as the standard. Initially, 450 μL of distilled water were mixed with 50 μL of each sample or gallic acid (Sigma-Aldrich, USA) solution. Then, 2.5 mL of Folin–Ciocalteu’s reagent (Sigma-Aldrich, USA) (0.2 N) were added, being the mixtures left for 5 min before the addition of 2 mL of aqueous Na2CO3 (Sigma-Aldrich, USA) (75 g/L). The reaction mixtures were incubated for 90 min at 30 °C. After incubation, the content in total phenolic compounds was determined by colorimetry at 765 nm [14,15].
A standard curve was prepared using methanolic solutions of gallic acid at 500, 300, 250, 200, 150, 100, and 50 mg/L (y = 0.0010x; R2 = 0.9612). The total phenolic compounds content was expressed as g of gallic acid equivalents (GAE)/100 g of sample (honey, propolis, and mixtures of honey with propolis) [14,15].
2.5.2. Flavonoid Determination
The aluminum chloride colorimetric method was used to determine the flavonoids content according to a previously implemented method [14,15]. To 500 μL of each solution, either the samples or the quercetin (Sigma-Aldrich, USA) (used as standard), 1.5 mL of methanol, 0.1 mL of aluminum chloride (Sigma-Aldrich, USA) 10% (w/v), 0.1 mL of 1 M potassium acetate (Sigma-Aldrich, USA) and 2.8 mL of distilled water were added. These solutions remained for 30 min at room temperature and then the absorbances were measured using a spectrophotometer (Helios–Omega, Thermo Scientific, USA) at 415 nm [14,15].
To construct the calibration curve, eight quercetin solutions were prepared in methanol with a concentration of 200, 175, 150, 100, 75, 50, 25, and 12.5 μg/mL (y = 0.0146 x; R2 = 0.9887). The flavonoids content was expressed as g of quercetin equivalents (QE)/100 g of sample (honey, propolis, and mixtures of honey with propolis) [14,15].
2.6. Antioxidant Activity Evaluation
For the antioxidant activity evaluation all the samples were diluted with methanol.
DPPH Free Radical Scavenging Assay
The DPPH (2,2-diphenyl-1-picrylhydrazyl) free radical scavenging assay was used to evaluate the antioxidant activity of the samples [16]. Briefly, to 100 μL of each sample, 3.9 mL of a 0.1 mM DPPH (Sigma-Aldrich, USA) methanolic solution were added, being this mixture stirred until complete homogenization. The control solution consisted in 100 μL of methanol with 3.9 mL of the DPPH solution. The reaction mixtures were kept at room temperature in the absence of light for 30 min, time after which the absorbances were read at 517 nm using a spectrophotometer (Helios–Omega, Thermo Scientific, USA) [16].
The percentage of inhibition (%Inhibition) of DPPH free radical by the samples was determined using the equation %Inhibition = [(Abscontrol − Absample)/Abscontrol] × 100, where Abscontrol corresponds to the absorbance of the control and Abssample is the absorbance of each sample [14,15]. The results were expressed as %Inhibition/100 g sample (honey, propolis, and mixtures of honey with propolis).
β-Carotene Bleaching Test
The β-carotene bleaching test was also employed to evaluate the antioxidant properties of the samples [16]. Firstly, a β-carotene (Sigma-Aldrich, USA) solution in chloroform with a concentration of 20 mg/mL was prepared. To 500 μL of this solution 40 μL of linoleic acid (TCI Europe N.V., Belgium), 400 μL of Tween 40 (Riedel-de H¨aen, Germany) and 1 mL of chloroform (Scharlab, Spain) were added. This mixture was transferred to a round bottom flask and subjected to a rotary evaporation system at 45 °C to ensure complete evaporation of the chloroform. After this, 100 mL of water saturated with oxygen were added to the mixture, forming an emulsion. Secondly, 300 μL of each sample were transferred to test tubes and 5 mL of the previously prepared β-carotene emulsion were added. The tubes were stirred until complete homogenization and were placed in a water bath at 50 °C for 1 h. Using a spectrophotometer (Helios–Omega, Thermo Scientific, USA), the absorbances of the samples were measured at 470 nm at the initial (t = 0 h) and final time (t = 1 h). The antioxidant activity was determined as percentage of inhibition of β-carotene’s oxidation (%Inhibition) using the following equation, %Inhibition = [(Abssample t = 1 h − Abscontrol t = 1 h)/(Abscontrol t = 0 h − Abscontrol t = 1 h)] × 100, where Abscontrol corresponds to the absorbance of the control and Abssample is the absorbance of each sample [14,15]. The results were expressed as %Inhibition/100 g sample (honey, propolis, and mixtures of honey with propolis).
2.7. Assessment of In Vitro Anti-Inflammatory Activity
The anti-inflammatory activity was determined by evaluating the capacity of the samples to inhibit protein denaturation [17]. Initially, a solution of bovine serum albumin (BSA) (Sigma-Aldrich, USA) at 1% (w/v) in phosphate buffer saline (PBS) solution was prepared. The pH of this solution was adjusted to 6.8 using glacial acetic acid (Scharlab, Spain). Then, 100 µL of the samples diluted in methanol were mixed, in test tubes pre-heated at 37 °C, with 900 µL of the BSA solution previously prepared. The control was composed of distilled water. The tubes were then incubated for 10 min at 72 °C and after this period cooled in ice for another 10 min. Finally, measurements of the absorbances were performed using a spectrophotometer (Helios–Omega, Thermo Scientific, USA) at 620 nm. The percentage of inhibition of protein denaturation (%Inhibition) was determined applying the following equation, %Inhibition = 100 − [(Abssample × 100)/Abscontrol], where Abscontrol corresponds to the absorbance of the control and Abssample is the absorbance of each sample [17]. The results were expressed as %Inhibition/100 g sample (honey, propolis, and mixtures of honey with propolis).
2.8. Evaluation of the In Vitro Wound-Healing Activity
2.8.1. Cell Culture
Normal human dermal fibroblasts (NHDF) cell line was maintained in RPMI-1640 culture medium (Sigma-Aldrich, USA) supplemented with 10% fetal bovine serum (FBS) (Sigma-Aldrich, USA), 1% mixture of antibiotic/antimycotic (Sigma-Aldrich, USA), 0.01 M of HEPES (Sigma-Aldrich, USA), 0.02 M of L-glutamine (Sigma-Aldrich, USA) and 0.001 M of sodium pyruvate (Sigma-Aldrich, USA). Subsequently, the cells were incubated at 37 °C in an air incubator with a humidified atmosphere with 5% CO2 [18].
2.8.2. Wound Scratch Assay
The samples were tested for wound-healing activity by using the wound scratch assay [13,19]. NHDF cells were seeded in 12-well plates (4 × 104 cells/well) and cultured until a monolayer confluence was reached. After the adhesion of the cells, the medium was removed from the wells and the cell monolayer was scraped in a straight central line using a p200 micropipette tip, creating a scratch, with reference points being marked in the plates. The wells were washed with PBS to remove floating cells and cell debris. Then, the PBS was removed, the samples were prepared in RPMI-1640 and sonicated, then they were added to the wells. Supplemented RPMI-1640 culture medium was added to the control wells. After this, the plates were placed under a phase-contrast microscope and images were acquired at the initial moment (t = 0 h). Then, the plates were incubated at 37 °C (5% CO2) and examined once again under the microscope after 2, 24, and 36 h [13,19].
The size of the scratch zones was assessed manually using a digital image analysis tool (IC Measure software version 2.0.0.161) (The Imaging Source, Germany) that allowed the estimation of the distance between the injury margins. Using the IC Measure, the distance between the margins of the lesion in the control at 0 h was estimated, which was considered the initial one and was used to scale all other measurements to more easily compare the estimated distances of the injuries between the samples and the control.
2.9. Statistical Analysis
The results were presented as mean values ± standard deviation. To determine the reproducibility of the measurements, each assay was performed at least in triplicate. The calculated distance between the margins of the injury were analyzed using the statistical program IBM SPSS Statistics 25 (https://www.ibm.com/analytics/spss-statistics-software) (IBM, Armonk, NY, USA). The significant difference among means was analyzed by Student’s t-test (assuming the normal distribution of the continuous variables). A level of p-value < 0.05 was considered significant.
3. Results and Discussion
3.1. FTIR Analysis of the Samples of Honey, Propolis, and Propolis Extracts
Regarding the honey samples and given the flora that exists at the place of harvest, it is expected that Honey 1 was produced mainly during the autumn from species such as Arbutus unedo, Castanea sativa, Quercus faginea, and Pinus pinaster. Honey 2 was produced during the summer from flowers such as Rosa spp., Dahlia spp., Hydrangea spp., and flowers from fruit trees like Prunus avium, Malus spp., Pyrus communis, and Prunus spinosa. Finally, Honey 3 was produced during the spring, when most wildflowers and aromatic plants bloom (Papaver rhoeas, Chrysanthemum coronarium, Lavandula stoechas, Rosmarinus officinalis, Baccharis trimera, and Thymus mastichina).
The propolis samples subsequently collected did not show a direct correlation with the honey samples, because bees repair their hive continuously throughout the year, whenever this need arises, so the conditions under which propolis is produced will not necessarily be the same conditions under which honey is produced.
The FTIR spectra of the samples of honey, propolis, and propolis extracts were recorded (Figure 1).
The spectra of honeys show a water band at approximately 3300 cm−1 and 1650 cm−1. Near 2900 cm−1 it is possible to observe a band that may be associated with groups present in amino acids. The bands between 1450 and 750 cm−1 may correspond to organic acids and to sugars commonly present in honey, such as sucrose, glucose, and fructose. Even though the honey samples have been produced in different seasons, they present quite similar spectra.
The spectra of propolis samples show approximately the same bands but with great dissimilarity in terms of the intensity of the signal. In these spectra, it can be observed a water band at around 3400 cm−1, and very pronounced bands at nearly 2900 and 2850 cm−1 that may correspond to some aliphatic compounds. The bands observed between 1650 and 1600 cm−1, as well as the bands between 1550 and 1400 cm−1 may be caused by the presence of flavonoids and other aromatic compounds. The band at 1150 cm−1 may be due to the presence of hydroxyflavonoids. Some of the bands were not considered and may be related to wax and other debris present in the samples. The spectra of propolis extracts show approximately the same bands, but with lower intensity than the propolis samples.
The water band observed in both propolis samples and extracts is less pronounced than the band registered in the honeys. In contrast, the bands identified as possible aromatic compounds and flavonoids in propolis samples and extracts spectra are more pronounced. Finally, the sugar bands in honey spectra are more evident and better outlined.
3.2. Phytochemical Characterization
Plant polyphenols present at least 8000 distinct known structures, being the most important class of natural bioactive compounds, which exhibit various biological activities [22]. Honey presents three classes of flavonoids with analogous structure: flavonols, flavones, and flavanones. Flavonoids are responsible for the color, taste, and flavor of the honey and they also improve its beneficial health effects [22]. Furthermore, the floral sources used by bees to produce honey, whose predominance depends on seasonal and environmental issues, influences the phenolic composition and antioxidant activity of honey.
The results of the phytochemical characterization of the samples regarding total phenolics and flavonoids contents are presented in Table 1.
Total phenolic compounds content of honey samples ranged from 0.029 to 0.107 g GAE/100 g sample, the values observed for propolis extracts ranged from 21.747 to 28.947 g GAE/100 g sample, and finally for the mixtures of honey with propolis ranged from 1.219 to 3.506 g GAE/100 g sample. The honey that presented the highest content in phenolic compounds is Honey 1 and the lowest content can be found in Honey 3. These differences may be related with the different seasons in which the honeys were produced, as mentioned above.
Propolis extracts showed a much higher concentration of phenolic compounds than honey samples, with the highest content found in Propolis Extract 1 followed by Propolis Extract 3 and Propolis Extract 2. An increase in phenolic content was observed with the addition of higher concentrations of propolis extracts to honey, and the highest value was obtained with H1PE3 at 0.5%.
Flavonoids were almost absent from honey samples. The only one that presents flavonoids in its composition is Honey 1, but even this sample has a very low content. In contrast, the flavonoids determined in the propolis extracts ranged from 1.786 to 5.494 g QE/100 g sample, and in the mixtures ranged from 0.054 to 0.452 g QE/100 g sample. Propolis extracts showed a higher concentration of flavonoids than honey samples, with the highest content in Propolis Extract 1 followed by Propolis Extract 3 and Propolis Extract 2. An increase in flavonoid content was observed in all samples with the addition of higher concentrations of propolis extract to honey, as expected.
The values of total phenolic compounds and flavonoids determined in the present work are very similar to the ones obtained for selected Czech honeys [23].
3.3. Antioxidant and Anti-Inflammatory Activities
Honey is an important natural source of antioxidants and has potential therapeutic value in several inflammatory diseases and in the treatment of heart disease, cancer, and cataracts, in addition to its sweetening capacity and lower glycemic load [24]. The biological properties of honey comprise antioxidant, antimicrobial, anti-inflammatory, and wound-healing activities [24].
In this work, the antioxidant activity of the samples was evaluated by two different methods that measure distinct antioxidant properties (Table 2). The DPPH free radical scavenging assay is based on the capacity of the samples to scavenge free radicals, while the β-carotene bleaching test allows the indirect evaluation of the capacity of the samples to inhibit the lipid peroxidation [25].
The honey that presented the highest antioxidant activity measured by the DPPH assay was Honey 1, opposed to Honey 3 that showed no relevant activity measured by this method. Propolis extracts revealed extremely high levels of antioxidant activity across all samples, with Propolis Extract 3 presenting the highest value. An increase in the antioxidant activity was observed in all samples with the addition of propolis extract to honey, however adding a higher concentration of propolis did not result in a considerable rase in activity in most cases.
Concerning the results of β-carotene bleaching test, the honey that revealed the highest antioxidant activity was once again Honey 1. The antioxidant activity of this honey measured by both methods is related with the presence of great amounts of phenolic compounds, as previously mentioned. Propolis extracts revealed high levels of antioxidant activity measured by β-carotene bleaching test as it was also verified by DPPH assay.
Analyzing the data obtained throughout the different assays it was possible to verify that dark-brown honey (H1) presented a higher content in phenolic compounds and flavonoids, followed by red honey (H2) and finally by light-yellow honey (H3). These results were consistent with the bioactive activity of the different samples. Since Honey 1 presented better phytochemical results, it was used in all the mixtures of honey with propolis.
The anti-inflammatory activity was evaluated using an in vitro assay that studied the ability of the samples to inhibit protein denaturation using a BSA solution (Table 2). It was noted that propolis extracts reveal a higher anti-inflammatory activity than honeys. The honey that presented the highest activity was Honey 2, and among the Propolis Extracts, PE3 revealed the highest activity. Generally, an increase in the anti-inflammatory activity was observed in all samples when adding propolis extract to honey. In a previous work involving Malaysian honeys, the authors concluded that the anti-inflammatory activity may be attributed, at least in part, to the phenolic compounds [24].
3.4. Wound-Healing Activity
In the present study, NHDF cells were used in a scratch assay. Although all the preliminary characterization data showed that the propolis extracts always presented better results than the other samples under study, it was decided to also evaluate the wound-healing activity for all the samples including the mixtures of honey with propolis.
It is already known that honey is not toxic against normal cells but is extremely cytotoxic to the tumor or cancer cells, as it was previously described [26]. Similar results were found in propolis extracts, which demonstrated cytotoxicity in human fibrosarcoma and colon adenocarcinoma cells while presenting no cytotoxic action in normal human skin fibroblasts [27].
By using the microscopic images, it was possible to evaluate the evolution of the gap created in the confluent cell monolayer in the presence of the samples (Table 3, Table 4, and Table 5).
Analyzing the different images and comparing them to the control samples it is possible to say that the honey that shows better results after 36 h is Honey 2 (Table 3), while the propolis extract that presented better results was Propolis Extract 2 at 0.5% (Table 4); the best mixture is the honey with propolis—H1PE3 0.3% (Table 5).
Examining all the images, it is possible to observe that the cells continue alive when incubated with the samples. Moreover, it is clear that the samples promote cell migration, demonstrating the wound-healing potential of honey and propolis.
Furthermore, by estimating the distance between the margins of the scratch (Table 6) the conclusions were the same. For all the samples, except for Honey 3 at 2 h, a significant (p-value < 0.05) reduction of the scratch was observed when compared to the control at the same time of incubation. In general, the samples that showed the best results were the mixtures of honey with propolis. However, the sample that presented the maximum activity was the Propolis Extract 2 at 0.5%.
In opposition to what was previously observed [1], in the present work the obtained results suggest that the effect of combining propolis with honey is not synergistic but just the combined effect of honey and propolis. This may be due to the chemical composition of each particular honey that will directly influence its bioactivities. In the honey samples now studied, the concentration in total phenolic compounds is relatively lower than in other samples of honey [1]. Moreover, flavonoids were not detected in the honey samples. These observations may explain the additive results observed for the mixtures of honey with propolis, suggesting the contribution of the propolis compounds to the biological activities.
Considering all the obtained results, it is possible to verify that the samples that presented higher cell migration levels also presented higher bioactivity.
During the inflammation process, honey promotes the release of inflammatory cytokines (TNF-α IL-6, IL-1β, and NO) by monocytes, which might stimulate collagen synthesis by fibroblasts, playing important roles in the initiation and amplification of this process [10]. The modulation of the severity of inflammation can be associated with the anti-inflammatory properties of the polyphenols present in honey. Honey initiates an active but controlled inflammation but does not let the inflammation to develop in a chronic or exaggerated state, modulating the inflammatory phase of wound-healing [10]. The anti-ulcerous activity of honey and propolis can be attributed to flavonoids that can act alone or in combination with other compounds such as sterols, terpinens, saponins, gums, and mucilage [4].
A recently published paper, in which the potential wound-healing properties of propolis was evaluated, demonstrated that propolis promoted a marked increase in the wound repair capacity of keratinocytes [28]. It was also proved that the regenerative properties of propolis are mainly due to H2O2 (which is extracellularly released and passes across the plasma membrane) is able to modulate intracellular mechanisms [28].
4. Conclusions
This work demonstrated the biological potential of honey and propolis, particularly the wound-healing activity, which is related with their antioxidant and anti-inflammatory properties. Further studies should be performed to clarify the mechanism of action of honey and propolis by which cell migration is stimulated.
Author Contributions
Conceptualization, A.P.D.; methodology, A.M.A., J.G., and Â.L.; Formal analysis, E.G. and A.P.D.; Investigation, A.M.A., J.G., and Â.L.; Resources, E.G. and A.P.D.; Data curation, E.G. and A.P.D.; Writing—original draft preparation, A.M.A.; Writing—review and editing, J.G., Â.L., E.G., and A.P.D.; Supervision, A.P.D. All authors have read and agreed to the published version of the manuscript.
Funding
This work was partially supported by CICS-UBI that is financed by National Funds from Fundação para a Ciência e a Tecnologia (FCT) and Community Funds (UIDB/00709/2020). Joana Gonçalves acknowledges the PhD fellowship from FCT (reference: SFRH/BD/149360/2019). Ângelo Luís acknowledges the contract of Scientific Employment in the scientific area of Microbiology also financed by FCT.
Conflicts of Interest
The authors declare no conflict of interest.
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Figure 1.
FTIR spectra of the samples.
Table 1.
Total phenolic compounds and flavonoids content of the samples.
| Samples | Total Phenolic Compounds | Flavonoids |
|---|---|---|
| (g GAE/100 g Sample) 1 | (g QE/100 g Sample) 1 | |
| H1 | 0.107 ± 0.016 | 0.007 ± 0.001 |
| H2 | 0.046 ± 0.005 | Not detected |
| H3 | 0.029 ± 0.003 | Not detected |
| PE1 | 28.947 ± 1.329 | 5.494 ±0.335 |
| PE2 | 21.747 ± 1.062 | 1.786 ± 0.029 |
| PE3 | 28.667 ± 0.774 | 4.280 ± 0.123 |
| H1PE1 0.3% | 2.394 ± 0.227 | 0.290 ± 0.007 |
| H1PE1 0.5% | 3.324 ± 0.044 | 0.452 ± 0.012 |
| H1PE2 0.3% | 1.219 ± 0.049 | 0.115 ± 0.005 |
| H1PE2 0.5% | 1.750 ± 0.076 | 0.199 ± 0.018 |
| H1PE3 0.3% | 1.969 ± 0.071 | 0.054 ± 0.011 |
| H1PE3 0.5% | 3.506 ± 0.257 | 0.308 ± 0.006 |
1 Results expressed as mean ± standard deviation.
Table 2.
Antioxidant and anti-inflammatory activities of the samples.
| Samples | DPPH | β-Carotene Bleaching Test | Anti-Inflammatory Activity |
|---|---|---|---|
| % Inhibition/100 g Sample 1 | % Inhibition/100 g Sample 1 | % Inhibition/100 g Sample 1 | |
| H1 | 0.431 ± 0.023 | 0.809 ± 0.042 | 20.625 ± 0.884 |
| H2 | 0.133 ± 0.019 | 0.684 ± 0.032 | 23.438 ± 3.094 |
| H3 | Not detected | 0.349 ± 0.028 | Not detected |
| PE1 | 92.506 ± 1.249 | 51.441 ± 4.477 | 15.000 ± 3.536 |
| PE2 | 92.012 ± 0.258 | 48.660 ± 1.876 | 31.250 ± 1.768 |
| PE3 | 93.245 ± 0.687 | 53.909 ± 2.328 | 48.750 ± 1.768 |
| H1PE1 0.3% | 8.271 ± 0.044 | 3.027 ± 0.070 | 36.408 ± 6.865 |
| H1PE1 0.5% | 8.119 ± 0.040 | 3.929 ± 0.105 | 28.571 ± 0.001 |
| H1PE2 0.3% | 7.921 ± 0.097 | 2.878 ± 0.096 | 40.049 ± 1.716 |
| H1PE2 0.5% | 8.154 ± 0.158 | 3.108 ± 0.049 | 45.238 ± 0.001 |
| H1PE3 0.3% | 8.165 ± 0.026 | 2.919 ± 0.106 | 36.408 ± 3.433 |
| H1PE3 0.5% | 8.396 ± 0.321 | 3.596 ± 0.089 | 40.476 ± 6.734 |
1 Results expressed as mean ± standard deviation.
Table 3.
Microscopic images obtained from the scratch wound-healing assay with the honeys (magnification: 100×).
Table 3.
Microscopic images obtained from the scratch wound-healing assay with the honeys (magnification: 100×).
Representative Image of the Cells at the Initial Moment (0 h) | |||
| Samples | 2 h | 24 h | 36 h |
| Control |  |  |  |
| H1 |  |  |  |
| H2 |  |  |  |
| H3 |  |  |  |
Table 4.
Microscopic images obtained from the scratch wound-healing assay with the propolis extracts (magnification: 100×).
Table 4.
Microscopic images obtained from the scratch wound-healing assay with the propolis extracts (magnification: 100×).
| Samples | 2 h | 24 h | 36 h |
|---|---|---|---|
| PE1 0.3% |  |  |  |
| PE1 0.5% |  |  |  |
| PE2 0.3% |  |  |  |
| PE2 0.5% |  |  |  |
| PE3 0.3% |  |  |  |
| PE3 0.5% |  |  |  |
Table 5.
Microscopic images obtained from the scratch wound-healing assay with the mixtures of honey with propolis (magnification: 100×).
Table 5.
Microscopic images obtained from the scratch wound-healing assay with the mixtures of honey with propolis (magnification: 100×).
| Samples | 2 h | 24 h | 36 h |
|---|---|---|---|
| H1PE1 0.3% |  |  |  |
| H1PE1 0.5% |  |  |  |
| H1PE2 0.3% |  |  |  |
| H1PE2 0.5% |  |  |  |
| H1PE3 0.3% |  |  |  |
| H1PE3 0.5% |  |  |  |
Table 6.
Calculated distance between the margins of the injury.
| Samples | 0 h 1 | 2 h 1 | p-Value | 24 h 1 | p-Value | 36 h 1 | p-Value |
|---|---|---|---|---|---|---|---|
| Control | 1.00 ± 0.05 | 0.99 ± 0.05 | 0.818 | 0.99 ± 0.05 | 1.000 | 0.98 ± 0.05 | 0.817 |
| H1 | 0.71 ± 0.04 | 0.002 * | 0.59 ± 0.03 | 0.001 * | 0.48 ± 0.02 | 0.001 * | |
| H2 | 0.83 ± 0.04 | 0.011 * | 0.37 ± 0.02 | 0.001 * | 0.33 ± 0.02 | 0.001 * | |
| H3 | 0.90 ± 0.05 | 0.062 | 0.57 ± 0.03 | 0.001 * | 0.49 ± 0.02 | 0.001 * | |
| PE1 0.3% | 0.80 ± 0.04 | 0.006 * | 0.78 ± 0.04 | 0.005 * | 0.69 ± 0.03 | 0.002 * | |
| PE1 0.5% | 0.84 ± 0.04 | 0.014 * | 0.81 ± 0.04 | 0.009 * | 0.78 ± 0.04 | 0.005 * | |
| PE2 0.3% | 0.54 ± 0.03 | 0.001 * | 0.39 ± 0.02 | 0.001 * | 0.34 ± 0.02 | 0.001 * | |
| PE2 0.5% | 0.66 ± 0.03 | 0.001 * | 0.52 ± 0.03 | 0.001 * | 0.27 ± 0.01 | 0.001 * | |
| PE3 0.3% | 0.74 ± 0.04 | 0.003 * | 0.62 ± 0.03 | 0.001 * | 0.53 ± 0.03 | 0.001 * | |
| PE3 0.5% | 0.45 ± 0.02 | 0.001 * | 0.41 ± 0.02 | 0.001 * | 0.39 ± 0.02 | 0.001 * | |
| H1PE1 0.3% | 0.74 ± 0.04 | 0.003 * | 0.63 ± 0.03 | 0.001 * | 0.55 ± 0.03 | 0.001 * | |
| H1PE1 0.5% | 0.43 ± 0.02 | 0.001 * | 0.43 ± 0.02 | 0.001 * | 0.42 ± 0.02 | 0.001 * | |
| H1PE2 0.3% | 0.54 ± 0.03 | 0.001 * | 0.37 ± 0.02 | 0.001 * | 0.49 ± 0.02 | 0.001 * | |
| H1PE2 0.5% | 0.64 ± 0.03 | 0.001 * | 0.58 ± 0.03 | 0.001 * | 0.46 ± 0.02 | 0.001 * | |
| H1PE3 0.3% | 0.80 ± 0.04 | 0.006 * | 0.44 ± 0.02 | 0.001 * | 0.31 ± 0.02 | 0.001 * | |
| H1PE3 0.5% | 0.74 ± 0.04 | 0.001 * | 0.45 ± 0.02 | 0.001 * | 0.34 ± 0.02 | 0.001 * |
1 Results expressed as mean ± standard deviation; * Indicates a significant result (p-value < 0.05).
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MDPI and ACS Style
M. Afonso, A.; Gonçalves, J.; Luís, Â.; Gallardo, E.; Duarte, A.P. Evaluation of the In Vitro Wound-Healing Activity and Phytochemical Characterization of Propolis and Honey. Appl. Sci. 2020, 10, 1845. https://doi.org/10.3390/app10051845
AMA Style
M. Afonso A, Gonçalves J, Luís Â, Gallardo E, Duarte AP. Evaluation of the In Vitro Wound-Healing Activity and Phytochemical Characterization of Propolis and Honey. Applied Sciences. 2020; 10(5):1845. https://doi.org/10.3390/app10051845
Chicago/Turabian StyleM. Afonso, Alexandra, Joana Gonçalves, Ângelo Luís, Eugenia Gallardo, and Ana Paula Duarte. 2020. "Evaluation of the In Vitro Wound-Healing Activity and Phytochemical Characterization of Propolis and Honey" Applied Sciences 10, no. 5: 1845. https://doi.org/10.3390/app10051845
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