The Array of Antibacterial Action of Protocatechuic Acid Ethyl Ester and Erythromycin on Staphylococcal Strains

The spread of antibiotic resistance among bacteria has become one of the major health problems worldwide. Methicillin-resistant staphylococcal strains are especially dangerous because they are often resistant to other antibiotics. The increasing insensitivity to macrolides, lincosamides and streptogramin B antibiotics of methicillin-resistant staphylococcal isolates has limited the use of these drugs in therapy. The combination of natural compounds and antibiotics can be considered as an alternative tool to fight multi-drug-resistant pathogen infections. The aim of the presented study was to examine the antibacterial activity of protocatechuic acid ethyl ester–erythromycin combination towards Staphylococcus aureus and Staphylococcus epidermidis strains with various resistance profiles to methicillin and macrolides, lincosamides and streptogramin B (MLSB) antibiotics. The in-vitro antibacterial potential of the above combination was investigated by minimum inhibitory concentration assays and checkerboard testing. The observed effects were strain dependent, with 8 of 12 tested staphylococcal strains showing an indifferent effect on the natural compound and erythromycin; for 2 strains, the tested combination had an additive effect, while for another 2, the effect was synergistic. Interestingly, the multi-drug-resistant strains were more sensitive to the cooperative action of the protocatechuic acid ethyl ester and the antibiotic.


Introduction
New resistance mechanisms developed by bacteria have greatly reduced the number of available therapeutic agents effective against bacterial infections. Frequently, microorganisms isolated from hospitalized patients show resistance to more than one group of antibiotics. In recent years, multi-drug-resistant bacteria have become the major concern for global health, so the search for new antimicrobial agents is now a priority for researchers [1]. To date, the beneficial interactions of antibiotics with compounds of plant origin were suggested by many studies [2][3][4]. Staphylococcus aureus is one of the World Health Organization (WHO) priority pathogens for research on new antibiotics. This mainly commensal microorganism can induce diseases of the skin and soft tissues, respiratory, urinary or digestive system. What is more, it could form biofilms on medical devices or surgical sites. In turn, Staphylococcus epidermidis, which colonizes mucous membranes and skin, is one of the main etiological factors of nosocomial infections [2,5], and is a major element in the human body's microbiota [6]. Colonization with coagulase-negative staphylococci (CoNS) takes place at birth and accompanies us throughout all our life [7]. It is currently believed that this opportunistic pathogen is responsible for infections associated with medical accessories, such as central venous ports, catheters, hip prostheses, knee prostheses and various procedures, such as coronary artery bypass surgery, cholecystectomy, laminectomy, colon surgery and cesarean section [8,9]. Due to the ability of S. epidermidis to form biofilms on the surfaces of Antibiotics 2022, 11, 848 2 of 12 medical devices, they are one of the reservoirs of infection [8]. Because multi-drug-resistant staphylococci strains are common in both hospital and community environments, it is very important to search for alternative treatments in staphylococcal infections. Many studies proved the synergistic effect of plant-derived compounds in combination with antibiotics [2,7,[10][11][12]. New drug combinations may lead to the development of new, cheaper, more accessible, more effective, safer-for-the-environment and, above all, for patients, antimicrobial therapies [1]. Protocatechuic acid (PCA) is one of the plant-derived compounds shown to have antimicrobial activity against Gram-positive, Gram-negative bacteria and fungi [13][14][15][16]. Its antimicrobial activity is related to the ability to inhibit bacterial growth and enhance the action of antibiotics and, thus, reduce resistance development [15]. What is more, PCA is non-toxic to humans at an oral dose of 100 mg/kg [15,17]. A usage limitation of phenolic acids, such as PCA as medicinal substances, is their low bioavailability. Moreover, phenolic acids are rapidly metabolized and excreted in the urine. Chemical modifications of phenolic acids may increase their biological activity, e.g., esterification increases the lipophilicity of PCA [18,19]. Figure 1 shows the differences in the chemical structure of PCA and protocatechuic acid ethyl ester (EDHB, ethyl 3-4 dihydroxybenzoate). EDHB has not yet been extensively studied for its antibacterial activity. This compound is found in the leaves and roots of many plant species, peanut seed casings and also in tea and wine [20]. EDHB is widely used as a food stabilizer [21] and its antioxidant, neuroprotective, myoand cardioprotective properties were indicated by many authors [21][22][23][24][25][26]. Our previous study proved the antibacterial properties of EDHB against reference and clinical strains of S. aureus [2]. What is more, a decrease in the minimal inhibitory concentrations (MIC) of erythromycin in the presence of this ester was observed. Therefore, it seems important to thoroughly evaluate the interactions of EDHB with erythromycin and to define its potential clinical usefulness. Since erythromycin and PCA have different targets in the bacterial cell, the choice of this combination seems to be justified. Erythromycin inhibits bacterial protein synthesis, while PCA causes membrane lysis of bacteria [16,27,28]. PCA can, thus, enhance the antibacterial effects of erythromycin without fear of interference. Since the esterification of phenolic acid may increase it bioavailability, research on the antibacterial properties of EDHB is more promising than on PCA; therefore, the authors decided to focus on EDHB. The aim of this study was to determine the direction of the influence of EDHB and erythromycin on the reference and clinical strains of S. aureus and S. epidermidis.
Antibiotics 2022, 11, x FOR PEER REVIEW tomy, laminectomy, colon surgery and cesarean section [8,9]. Due to the ab dermidis to form biofilms on the surfaces of medical devices, they are one of of infection [8]. Because multi-drug-resistant staphylococci strains are com hospital and community environments, it is very important to search for alte ments in staphylococcal infections. Many studies proved the synergistic e derived compounds in combination with antibiotics [2,7,[10][11][12]. New drug may lead to the development of new, cheaper, more accessible, more effect the-environment and, above all, for patients, antimicrobial therapies [1]. P acid (PCA) is one of the plant-derived compounds shown to have antimicr against Gram-positive, Gram-negative bacteria and fungi [13][14][15][16]. Its antim ity is related to the ability to inhibit bacterial growth and enhance the action and, thus, reduce resistance development [15]. What is more, PCA is non-tox at an oral dose of 100 mg/kg [15,17]. A usage limitation of phenolic acids, su medicinal substances, is their low bioavailability. Moreover, phenolic acid metabolized and excreted in the urine. Chemical modifications of phenolic crease their biological activity, e.g., esterification increases the lipophilicity o Figure 1 shows the differences in the chemical structure of PCA and protoc ethyl ester (EDHB, ethyl 3-4 dihydroxybenzoate). EDHB has not yet bee studied for its antibacterial activity. This compound is found in the leaves many plant species, peanut seed casings and also in tea and wine [20]. ED used as a food stabilizer [21] and its antioxidant, neuroprotective, myo-and tive properties were indicated by many authors [21][22][23][24][25][26]. Our previous stud antibacterial properties of EDHB against reference and clinical strains of What is more, a decrease in the minimal inhibitory concentrations (MIC) of in the presence of this ester was observed. Therefore, it seems important t evaluate the interactions of EDHB with erythromycin and to define its pot usefulness. Since erythromycin and PCA have different targets in the bac choice of this combination seems to be justified. Erythromycin inhibits bac synthesis, while PCA causes membrane lysis of bacteria [16,27,28]. PCA can, the antibacterial effects of erythromycin without fear of interference. Since tion of phenolic acid may increase it bioavailability, research on the antibac ties of EDHB is more promising than on PCA; therefore, the authors decide EDHB. The aim of this study was to determine the direction of the influence erythromycin on the reference and clinical strains of S. aureus and S. epiderm

Antibiotic Resistance Profile of Tested Strains
The resistance profile of the tested strains is presented in Table 1. Amo S. aureus strains, three were resistant to methicillin (S. aureus ATCC 43300, S 4) and three strains of S. epidermidis were resistant to this antibiotic (S. epid 35984, S. epidermidis 1 and 2). The remaining isolates showed sensitivity to m A. B.

Antibiotic Resistance Profile of Tested Strains
The resistance profile of the tested strains is presented in Table 1. Among the tested S. aureus strains, three were resistant to methicillin (S. aureus ATCC 43300, S. aureus 3 and 4) and three strains of S. epidermidis were resistant to this antibiotic (S. epidermidis ATCC 35984, S. epidermidis 1 and 2). The remaining isolates showed sensitivity to methicillin (S. aureus ATCC 25923, S. epidermidis ATCC 12228, S. aureus 1 and 2, S. epidermidis 3 and 4). S. aureus ATCC 43300, S. epidermidis ATCC 35984, S. aureus 3, S. aureus 4, S. epidermidis 1 and S. epidermidis 2 strains demonstrated the constitutive phenotype of resistance to MLS B antibiotics (cMLS B ). The remaining isolates did not show the MLS B resistance phenotype.

The Fractional Inhibitory Concentration (FIC) Values for Protocatechuic Acid Ethyl Ester and Erythromycin against Staphylococcal Strains
The EDHB inhibited the growth of all the tested S. aureus strains, with MIC values ranging from 16 to 1024 µg/mL. The growth of the S. aureus reference strains was inhibited at a concentration of 512 µg/mL. S. aureus 1 and 2 strains proved to be sensitive to EDHB with MIC 16 µg/mL, while the growth of the S. aureus  Table 2.
Based on the checkerboard assay, MIC values were determined for EDHB in combination with erythromycin and for erythromycin in combination with EDHB.
Erythromycin and EDHB exerted an indifferent effect against five S. aureus strains. The synergistic effect of the compounds was noted only against S. aureus 3. The erythromycin-EDHB combination turned out to be more active against S. epidermidis strains, where in two cases, an additive effect was found (S. epidermidis 12228 and 3) and in one, it was synergistic (S. epidermidis 4). For the remaining strains, the effect of combining the compounds was indifferent. The results of the checkerboard assay for each strain are shown in Figure S1 (Supplementary Materials), while the FIC index and their interpretation are presented in Table 3.   [29,30]. The changes in the MIC value of erythromycin after the addition of EDHB were statistically significant (p = 0.005). Statistical analysis also revealed significant differences between MIC changes for resistant versus susceptible strains (p = 0.002). Interestingly, the strains resistant to MLS B antibiotics and methicillin were more sensitive to the erythromycin-EDHB combination (Table 4).

Discussion
Staphylococcal infections have become one of the most important public health problems, as multi-drug-resistant strains of this microbe are spreading rapidly. This fact stimulates scientists to search for new antimicrobial compounds and therapeutic strategies for staphylococcal disease treatment. A very promising direction of research is the implementation of substances of natural origin to augment routine antimicrobial therapies. The enhancement of antibiotic action by such compounds is due to sensitizing bacterial strains to drugs and enhancing their activity by increasing the bioavailability or simultaneously affecting a different site in the bacterial cell [4].
In this study, the antibacterial effect of the EDHB and erythromycin combination on reference and clinical Staphylococcus spp. strains was assessed. EDHB in combination with erythromycin showed an indifferent effect against five S. aureus isolates, while a synergistic interaction was found for one strain. Interestingly, a synergistic effect was noted against a multi-drug-resistant clinical strain, which, due to its character, should be less susceptible to the combined action of the compounds. In turn, among S. epidermidis strains, three indifferent, two additive and one synergistic effect were noted. A synergistic interaction was found against the sensitive S. epidermidis 4. It should be noted that if one substance is much more active, sometimes it is difficult to distinguish an indifferent effect from an additive effect, especially when using dilutions of the antibiotics [31]. The statistical analysis showed that the resistant strains of the tested staphylococci were more sensitive to the EDHB-erythromycin combination then sensitive isolates. Significant differences were observed in the decrease in erythromycin MIC values after the addition of EDHB (Table 4). Therefore, it is likely that EDHB blocks the mechanisms of bacterial resistance, thus, increasing its sensitivity.
What is more, the combination of "erythromycin-EDHB" turned out to be more effective against coagulase-negative staphylococci. Because S. epidermidis strains produce biofilm, which is the CoNSs' main virulence factor, evaluation of the effective combination of EDHB-erythromycin is of importance. The antibiofilm properties of PCA have been described in many studies [32][33][34][35]. The mechanism of PCA antibiofilm action is attributed to the changes in the properties of bacterial surfaces and inhibition of quorum sensing [32,34,35]. The reference S. epidermidis ATCC 35983 strain has a biofilm-forming ability and possesses icaADBC operon. The direction of the interaction of EDHB-erythromycin for this strain was indifferent. All tested clinical S. epidermidis isolates also have biofilm formation ability (data not shown). Among these strains, two indifferent, one synergistic and one additive interaction were noted. Since the EDHB-erythromycin combination has been shown to be more effective against the CoNS strains, it is possible that EDHB also affects the biofilm formation process. It is believed that natural compounds showing synergism with antibiotics could have potential use in the effective treatment of nosocomial infections caused by the CoNS, especially in cases requiring a non-standard pharmacological approach [3].
Previously, Miklasińska et al. [2] investigated the antibacterial effect of EDHB alone and in combination with four antibiotics: erythromycin, clindamycin, vancomycin and cefoxitin. Twenty clinical strains and three reference strains of S. aureus were tested. The MIC values for EDHB ranged from 64 to 1024 µg/mL, with median 512 µg/mL, while the MIC values for EDHB in this study ranged from 16 µg/mL to 1024 µg/mL (median 512 µg/mL) and were strain dependent. In our previous study, we found that the differences in the EDHB MIC values did not depend on the mechanism of resistance to MLS B antibiotics [2]. What is more, we found out that the presence of EDHB increased the sensitivity of the studied strains to erythromycin, as well as to clindamycin and vancomycin. Among examined strains were two reference isolates (S. aureus ATCC 43300 and S. aureus ATCC 25923), which were also included in this work and showed an indifferent effect to the EDHB-erythromycin combination. For the S. aureus ATCC 43300 strain, both studies showed the same MIC value of 512 µg/mL, while for S. aureus 25923, the obtained MICs were different. In our previous study, it was 256 µg/mL, while in the present work, the MIC was 512 µg/mL. As both experiments were carried out on the same strains, stored in our department and with the use of a compounds purchased from the same company, the probable cause of the difference is a laboratory error. However, it should be noted that the above MIC values do not differ significantly, and these results do not affect the assessment of the antibacterial activity of EDHB against the tested strains. The results of both studies failed to unambiguously demonstrate whether the combination of erythromycin and EDHB would bring a noticeable therapeutic benefit but showed a tendency to decrease erythromycin resistance under the influence of the EDHB.
To the best of our knowledge, there are no studies, except ours, on the antibacterial activity of EDHB, but works on the antimicrobial potential of the PCA are worth discussing. Chai et al. [36] studied the action of PCA and chlorogenic acid in combination with antibiotics against Escherichia coli, S. aureus, Streptococcus iniae and Proteus mirabilis. The authors found that the growth of Gram-negative bacteria was inhibited to a lesser extent by PCA and chlorogenic acid than the growth of Gram-positive pathogens, and that the effect of PCA was more prominent than that of chlorogenic acid. Both of these acids showed the strongest antibacterial activity against S. aureus. Similarly, Stojković et al. [28], in their study, noted the highest PCA activity against the S. aureus strain compared with other Gram-positive and also Gram-negative bacteria. The MIC value of PCA against S. aureus in their study was 300 µg/mL, so it was close to the median obtained in our work for EDHB (512 µg/mL). Chai et al. [36] also studied an interaction between PCA and antibiotics. A synergistic effect against S. aureus was noted for the PCA with clinafloxacin and gatifloxacin, an additive effect for the combination with ciprofloxacin, and an indifferent effect for the combination with sulfamonomethoxine. Sanhueza et al. [37] also assessed the interactions between PCA and antibiotics with a different mechanism of action (oxacillin, ampicillin, nalidixic acid, ciprofloxacin, norfloxacin, levofloxacin, tetracycline and chloramphenicol) against five clinical and one reference strain of S. aureus (ATCC 6538). The analysis of the FIC index by the checkerboard method showed values below 0.5 for all tested combinations of antibiotics, phenolic compounds and bacterial strains, which pointed to a synergistic effect. The results of the above studies may suggest that the direction of EDHB's effect does not depend on the mechanism of action of the antibiotic. Erythromycin, used in our work, inhibits the synthesis of bacterial proteins by binding to the 50S ribosome subunit, while clinafloxacin, gatifloxacin, ciprofloxacin, nalidixic acid, norfloxacin and levofloxacin interfere with the synthesis of bacterial DNA. On the other hand, oxacillin and ampicillin interfere with the synthesis of the cell wall and tetracycline inhibits bacterial proteins synthesis by binding to the 30S ribosome subunit. Since PCA causes membrane lysis of bacteria [16,27,28], it is Antibiotics 2022, 11, 848 7 of 12 more probable that the synergistic effect is related to the stimulation of other sites in the bacterial cell. Because the influence of PCA-antibiotics combinations is strain dependent, it may be related to other bacterial resistance mechanisms. Mandalari et al. [38] evaluated the FIC values for catechin, PCA and epicatechin combinations against Gram-negative and Gram-positive bacteria. Further, in their study, the S. aureus strain turned out to be most susceptible to the examined compounds. An indifference towards synergism was observed between naringenin and PCA against S. aureus. Since naringenin affects the bacterial cell membrane [39], and PCA causes membrane lysis [16,27,28], the direction of the interaction may be justified by reinforcing one other's action.
The above studies and the results of the presented work indicate that natural compounds, including EDHB, can modify the antibacterial action of antibiotics against staphylococcal strains. The experiments showed a better effect from PCA on Gram-positive bacteria, in particular, S. aureus, and this should be the focus of future studies. As numerous works imply the antibacterial properties of protocatechuic acid and its chemical derivatives, such studies should be carried out with a greater number of strains to precisely evaluate the antimicrobial potential of phenolic compounds, with associations with antibiotics with different mechanisms of action. Efforts should also be directed to precisely determine the mechanism of action of EDHB on bacterial cells and its potential applications in the treatment of staphylococcal infections. This line of research may, in the future, provide a new, effective method of antibacterial therapy.

Bacterial Strains
The antibacterial activity of EDHB was assessed against four clinical S. aureus strains isolated (S. aureus 1, 2, 3 and 4) from clinical wound samples and four clinical S. epidermids strains (S. epidermidis 1, 2, 3 and 4) isolated from blood together with four reference strains: S. aureus ATCC 25923, S. aureus ATCC 43300, S. epidermidis ATCC 12228 and S. epidermidis ATCC 35984. The species of the clinical strains was confirmed by assessing their phenotypic features, such as: morphology of colonies grown on blood agar, type of hemolysis, growth on Chapman medium and production of coagulase and catalase. The Oxoid Staphytect Plus test and the API Staph test (bioMerieux, Marcy-l'Étoile, France) were also performed. To ensure that the clinical strains were identified correctly the PCR-RFLP reaction was carried out. GeneMATRIX Tissue & Bacterial DNA Purification KIT (EuRx Ltd., Gdańsk, Poland) was used for bacterial genomic DNA isolation [40]. The PCR reaction was performed using 10× PCR RED master mix kit (BLIRT SA, Gdańsk, Poland) in a MJ Mini Personal Thermal Cycler (Bio-Rad, Hercules, CA, USA). To confirm the classification of species, the specific restriction profiles after cleaving of PCR products with 10 U of restriction enzymes XapI and Bsp143I (Fermentas, Vilnius, Lithuania) were analyzed. All the tested strains were stored in the Trypticase Soy Broth medium with 20% glycerol at −80 • C. EDHB used in this study was received from Sigma Chemical Co. (St. Louis, MO, USA) and dissolved in DMSO immediately prior to use.

Susceptibility Testing of Staphylococcal Strains to Erythromycin and EDHB Using the Microdilution Method
The standard microdilution method in sterile 96-well polystyrene plates (FL Medical, Torreglia, Italy) was used to determine the minimum inhibitory concentrations of EDHB and erythromycin towards the staphylococcal strains [41,42]. Serial dilutions were made as follows: 11 wells of 96-well polystyrene plates were filled with Mueller-Hinton; in the Antibiotics 2022, 11, 848 8 of 12 next step, 100 µL of EDHB or erythromycin stock solution was added to the first well and mixed thoroughly, and subsequently 100 µL was transferred to the next and remaining wells in the same manner, and finally, from the last well 100 µL was removed. In the next step, 100 µL of the 0.5 McFarland bacterial suspension was added to the wells containing the EDHB and erythromycin dilutions. The organization of the titration plate is shown in Figure 2. The absorbance was assessed in wavelength λ = 595 nm by spectrophotometry (Thermo Electron Corp., Vantoa, Finland). The MIC is defined as the lowest compound concentration that yields no visible microorganism growth, and it indicates the resistance of bacteria to an antimicrobial agent and determines the potency of new antimicrobial agents [31,41]. All experiments were carried out in triplicate. The obtained MIC values were used to design a "checkerboard" to determine the FIC value.
The standard microdilution method in sterile 96-well polystyrene plates (FL Medical, Torreglia, Italy) was used to determine the minimum inhibitory concentrations of EDHB and erythromycin towards the staphylococcal strains [41,42]. Serial dilutions were made as follows: 11 wells of 96-well polystyrene plates were filled with Mueller-Hinton; in the next step, 100 µL of EDHB or erythromycin stock solution was added to the first well and mixed thoroughly, and subsequently 100 µL was transferred to the next and remaining wells in the same manner, and finally, from the last well 100 µL was removed. In the next step, 100 µL of the 0.5 McFarland bacterial suspension was added to the wells containing the EDHB and erythromycin dilutions. The organization of the titration plate is shown in Figure 2. The absorbance was assessed in wavelength λ = 595 nm by spectrophotometry (Thermo Electron Corp., Vantoa, Finland). The MIC is defined as the lowest compound concentration that yields no visible microorganism growth, and it indicates the resistance of bacteria to an antimicrobial agent and determines the potency of new antimicrobial agents [31,41]. All experiments were carried out in triplicate. The obtained MIC values were used to design a "checkerboard" to determine the FIC value.

Determination of the Susceptibility of Staphylococcal Strains to the Erythromycin and EDHB Combination
The susceptibility of staphylococcal strains to the combination of erythromycin and EDHB was assessed by determining the fractional inhibitory concentration (FIC) value for each strain. The checkerboard microdilution method with modifications was used to determine the total susceptibility effect of the tested strains [35,36]. Briefly, the erythromycin and EDHB solutions corresponding to an MIC value of 8 were prepared. Then, a series of 1/8 MIC dilutions was made. The MIC values of the substances were determined in the

Determination of the Susceptibility of Staphylococcal Strains to the Erythromycin and EDHB Combination
The susceptibility of staphylococcal strains to the combination of erythromycin and EDHB was assessed by determining the fractional inhibitory concentration (FIC) value for each strain. The checkerboard microdilution method with modifications was used to determine the total susceptibility effect of the tested strains [35,36]. Briefly, the erythromycin and EDHB solutions corresponding to an MIC value of 8 were prepared. Then, a series of 1/8 MIC dilutions was made. The MIC values of the substances were determined in the previous step. As such, 95 µL of dual-concentrated Mueller-Hinton medium was added to each well of the titration plate. Then, 50 µL of EDHB and appropriate concentration of erythromycin were added. Finally, 5 µL of a 0.5 McFarland staphylococcal bacterial suspension was added. The volume of each well was 200 µL. Therefore, the solutions corresponding to the concentrations of 8 MIC, 4 MIC, 2 MIC, MIC, 1/2 MIC, 1/4 MIC and 1/8 MIC were prepared for erythromycin and EDHB to take into account the dilution of 50 µL of these substances in 200 µL of the solution and obtained as follows: 2 MIC, MIC, 1/2 MIC, 1/4 MIC, 1/8 MIC, 1/16 MIC and 1/32 MIC in each of the wells. To the last column and row, respectively, instead of EDHB and erythromycin, 50 µL of medium was added. The resulting "checkerboard" is shown in Figure 3.
previous step. As such, 95 µL of dual-concentrated Mueller-Hinton medium was a to each well of the titration plate. Then, 50 µL of EDHB and appropriate concentrat erythromycin were added. Finally, 5 µL of a 0.5 McFarland staphylococcal bacteria pension was added. The volume of each well was 200 µL. Therefore, the solutions sponding to the concentrations of 8 MIC, 4 MIC, 2 MIC, MIC, 1/2 MIC, 1/4 MIC an MIC were prepared for erythromycin and EDHB to take into account the dilution of of these substances in 200 µL of the solution and obtained as follows: 2 MIC, MI MIC, 1/4 MIC, 1/8 MIC, 1/16 MIC and 1/32 MIC in each of the wells. To the last co and row, respectively, instead of EDHB and erythromycin, 50 µL of medium was a The resulting "checkerboard" is shown in Figure 3.  The prepared plates were incubated at 37 • C for 24 h. The absorbances were then read at 595 nm. The percent increase in individual wells in relation to the growth control was calculated using the formula: where A is the absorbance. The MIC was re-established for EDHB and erythromycin for each strain. Then the FIC [35,36] was calculated for EDHB and erythromycin and their sum for each well. The following formula was used: Many different combinations are observed in the checkerboard test; therefore, only the FIC values of the most efficient combination of compounds are used to calculate the FICI [35,36]. Based on the FIC index value for each strain, the relationship between EDHB and erythromycin was assessed according to the following scale: FIC ≤ 0.5-means synergism; 0.5 < FIC ≤ 1-means additive effect; 1 < FIC ≤ 4-means indifference; FIC > 4-means antagonism [1]. A synergistic effect can be found when the joint effect of the substances is greater than the sum of the individual effects. An additive effect can be observed when the sum of the effects of the substances themselves is equal to the joint effect. A neutral effect is characterized by a lack of interaction between the compounds [29]. An antagonistic effect is defined as a decreased collective interaction of the compounds compared to the interaction of the compounds themselves [31].

Statistical Analysis
Wilcoxon signed-rank test was used to determine whether the differences in the MIC values of erythromycin after the addition of EDHB were statistically significant. To assess the relationship between the presence of resistance mechanisms and the change in erythromycin MIC values following the addition of EDHB for a given strain the t-student test was used. For all used tests p ≤ 0.05 was considered as statistically significant. The data were analyzed with the use of STATISTICA v 13.0 software (StatSoft, Krakow, Poland).

Conclusions
The results of this study demonstrate that multi-drug-resistant strains turned out to be more sensitive to the combination of antibiotics and EDHB than sensitive isolates. The combination of "erythromycin-EDHB" was more effective against coagulase-negative staphylococci. The in vitro additive effect and synergy of EDHB and erythromycin can indicate that EDHB is capable of augmenting the antimicrobial potential of antibiotics in vivo, but since this effect is strain dependent, further studies are necessary to evaluate the exact mechanisms of action of protocatechuic acid and EDHB.
Supplementary Materials: The following supporting information can be downloaded at: https:// www.mdpi.com/article/10.3390/antibiotics11070848/s1, Figure S1: The checkerboard assay results for staphylococcal strains. The dark grey represents greater than 50% bacterial growth in a well, while the light grey shows smaller than 50% bacterial growth in a well compared to the growth control. The blue represents an indifferent, pink additive, while green synergistic interaction. The red framed box represents FIC index for each strain. The values highlighted in yellow show the MICs for EDHB and erythromycin.