key: cord-0761341-gj4oz6jp
authors: Haroun, Michelyne; Tratrat, Christophe; Kolokotroni, Aggeliki; Petrou, Anthi; Geronikaki, Athina; Ivanov, Marija; Kostic, Marina; Sokovic, Marina; Carazo, Alejandro; Mladěnka, Přemysl; Sreeharsha, Nagaraja; Venugopala, Katharigatta N.; Nair, Anroop B.; Elsewedy, Heba S.
title: 5-Benzyliden-2-(5-methylthiazol-2-ylimino)thiazolidin-4-ones as Antimicrobial Agents. Design, Synthesis, Biological Evaluation and Molecular Docking Studies
date: 2021-03-17
journal: Antibiotics (Basel)
DOI: 10.3390/antibiotics10030309
sha: 869534866b13595b0b940c0ee2ed07bf29165a5c
doc_id: 761341
cord_uid: gj4oz6jp

In this study, we report the design, synthesis, computational and experimental evaluation of the antimicrobial activity, as well as docking studies of new 5-methylthiazole based thiazolidinones. All compounds demonstrated antibacterial efficacy, some of which (1, 4, 10 and 13) exhibited good activity against E. coli and B. cereus. The evaluation of antibacterial activity against three resistant strains, MRSA, P. aeruginosa and E. coli, revealed that compound 12 showed the best activity, higher than reference drugs ampicillin and streptomycin, which were inactive or exhibited only bacteriostatic activity against MRSA, respectively. Ten out of fifteen compounds demonstrated higher potency than reference drugs against a resistant strain of E. coli, which appeared to be the most sensitive species to our compounds. Compounds 8, 13 and 14 applied in a concentration equal to MIC reduced P. aeruginosa biofilm formation by more than 50%. All compounds displayed antifungal activity, with compound 10 being the most active. The majority of compounds showed better activity than ketoconazole against almost all fungal strains. In order to elucidate the mechanism of antibacterial and antifungal activities, molecular docking studies on E. coli Mur B and C. albicans CYP51 and dihydrofolate reductase were performed. Docking analysis of E. coli MurB indicated a probable involvement of MurB inhibition in the antibacterial mechanism of tested compounds while docking to 14α-lanosterol demethylase (CYP51) and tetrahydrofolate reductase of Candida albicans suggested that probable involvement of inhibition of CYP51 reductase in the antifungal activity of the compounds. Potential toxicity toward human cells is also reported.

Despite the achievements in the treatment of infective diseases during the last 50 years, unfortunately, the new infections affecting large populations are instigating significant morbidity and mortality. The most recent case of COVID-19 is the best example. Another crucial problem is the growth of antibiotic resistance (AMR), which represents a significant obstacle for the successful treatment of severe and particularly life-treating infections. The phenomenon of AMR at biochemical and physiological levels may manifest in any single bacterial cell (planktonic growth) or in a sessile complex microbial community (biofilm) [1, 2] .

One of the bacterial growth modes is the development of biofilms, which may be considered a basic endurance strategy in hostile environments [2] . Biofilm formation plays an essential role in bacterial infection and antimicrobial resistance. In general, biofilmembedded bacteria are more resistant to common antimicrobial agents and host defense systems than bacteria in the planktonic state [3] . Established biofilms are less sensitive to elimination by the immune system, and this leads to chronic and persistent infections [4] . The major pathogen, which causes biofilm-associated infections, is Pseudomonas aeruginosa. It is able to form biofilm on a broad range of surfaces [5, 6] . Similarly, there are reports in the literature that biofilm of Candida may be up to 1000 times more resistant to antifungal agents compared to their planktonic cell [7] .

The increasing resistance to the current antimicrobial treatment has resulted in a crucial need for the discovery and development of novel entities for the treatment of infections with different modes of action that could target both sensitive and, in particular resistant strains [8] . This need is even greater for patients suffering from chronic inflammatory bowel diseases as well as cystic fibrosis (CF). During an inflammatory response in the gut, some commensal microorganisms, such as E. coli and C. albicans, can thrive and contribute to illness [9] . While Pseudomonas aeruginosa is an opportunistic pathogen that commonly infects the CF lung, promoting an accelerated decline of pulmonary function [10] .

Although new drugs were introduced in the battle against bacteria and fungi, such as echinocandin derivatives [11, 12] , nevertheless, some fungal species are still resistant.

Consequently, the major clinical challenge is to overcome the need for further new antimicrobial agents that can simultaneously combat the resistance dilemma by designing powerful new drugs being less prone to multiresistance or to toxic side effects.

Thiazoles have been found to hold a wide array of pharmacological actions with importance in biological systems. Among the activities mentioned are antimicrobial [13] [14] [15] [16] [17] , local anesthetic [18] , anti-inflammatory [19] [20] [21] , anti-HIV [22, 23] , analgesic and antipyretic [24] , antidiabetic [25, 26] , anticancer [27, 28] , antioxidant [29] and many others [30, 31] . On the other hand, thiazolidinone core attracted the interest of scientists due to its multiple degrees of medicinal and biological activities [20, 23, [32] [33] [34] [35] [36] [37] [38] . Antifungal and antibacterial activities of various thiazole and thiazolidinone skeletons have been extensively studied [20, [39] [40] [41] [42] .

Herein, we illustrate the molecular docking design, preparation and assessment of antimicrobial potency of fifteen new 5-benzyliden-2-(5-methylthiazol-2-ylimino) thiazolidin-4-ones. The design of many thiazolidinones has been accomplished by entering various arylidene groups at the 5 position of the thiazolidinone cores, since as reported in our earlier investigations [43] , which were recently exploited as bioactive arms on heterocycle scaffolds useful to encompass certain physicochemical properties as hydrophobic and steric.

Compound toxicity was predicted utilizing the OpenTox and CBLIGAND programs designed according to the REACH legislation requirements, which favors the practice of alternative testing manipulations to diminish animal experiment practices in testing toxicity. These programs, with the help of in silico standards and algorithms, perform an assessment of the cytotoxicity of compounds [44, 45] .

The results of the toxicity prediction in rats and mice suggested a lack of carcinogenicity and mutagenesis as well as no toxicity to the skin and eyes (Table S1 ). However, these remain predictive data that cannot assure the safety of these compounds.

The designed compounds were synthesized according to the process described in our previous papers [20, 43] and are shown in Scheme 1.

Antibiotics 2020, 9, x FOR PEER REVIEW 3 of 19

The designed compounds were synthesized according to the process described in our previous papers [20, 43] and are shown in Scheme 1.

3-F Scheme 1. Synthesis of titled compounds.

Compounds 1-15 exist as potential E and Z geometrical isomers; the Z conformation of the 5 exocyclic C=C double bonds was assigned on the basis of 1 HNMR spectroscopy and on the basis of literature data for analogous 4-thiazolidinones and 2,4-thiazolidinones [43, 46, 47] . The 1 H NMR spectra of compounds 1-15 showed only one kind of methine proton that, deshielded by the adjacent C=O. It was detected at 7.63-7.97 ppm at higher chemical shift values than the expected ones for E isomers that have a methine proton with a lesser deshielding effect. All compounds were characterized spectroscopically (IR, 1 H-NMR, C-NMR, MS).

The derivatives were evaluated for their inhibitory action on the growth of eight bacterial strains in addition to eight fungi using the microdilution method with the aim of disclosing minimal inhibitory (MIC), minimal bactericidal (MBC) and minimal fungicidal (MFC) concentrations. All compounds demonstrated antibacterial efficiency, but their potency was different. MIC were in the range of 26.3-378.5 μM and MBCs ranged between 52.6-757.0 μM (Table 1 ). The antibacterial activity of these compounds can be presented in the following order: 7 > 2 > 14 > 8 > STM > 13 > 4 > 6 > 3 > 10 > 11 > 5 > 12 > 1 > 15 > 9 > AMP. Compound 7 exhibited the highest antibacterial activity. Its bacteriostatic activity was detected in concentrations of 43.3-86.7 µM and its bactericidal activity at concentrations of 86. 7-173.4 μM. This compound is 6 times more potent than ampicillin and 3 times than streptomycin against all bacteria. Compound 9 was the less active (MIC ranging from 125.4 to 344.8 μM and MBC ranging from 250.7 to 689.6 μM). Surprisingly, most of the derivatives were more efficient than ampicillin and compounds 2-8, 10, 11, 13 and 14 exhibited higher potency than streptomycin towards the majority of tested bacterial pathogens. Compounds 1-15 exist as potential E and Z geometrical isomers; the Z conformation of the 5 exocyclic C=C double bonds was assigned on the basis of 1 HNMR spectroscopy and on the basis of literature data for analogous 4-thiazolidinones and 2,4thiazolidinones [43, 46, 47] . The 1 H NMR spectra of compounds 1-15 showed only one kind of methine proton that, deshielded by the adjacent C=O. It was detected at 7.63-7.97 ppm at higher chemical shift values than the expected ones for E isomers that have a methine proton with a lesser deshielding effect. All compounds were characterized spectroscopically (IR, 1 H-NMR, C-NMR, MS).

The derivatives were evaluated for their inhibitory action on the growth of eight bacterial strains in addition to eight fungi using the microdilution method with the aim of disclosing minimal inhibitory (MIC), minimal bactericidal (MBC) and minimal fungicidal (MFC) concentrations. All compounds demonstrated antibacterial efficiency, but their potency was different. MIC were in the range of 26.3-378.5 µM and MBCs ranged between 52.6-757.0 µM (Table 1 ). The antibacterial activity of these compounds can be presented in the following order: 7 > 2 > 14 > 8 > STM > 13 > 4 > 6 > 3 > 10 > 11 > 5 > 12 > 1 > 15 > 9 > AMP. Compound 7 exhibited the highest antibacterial activity. Its bacteriostatic activity was detected in concentrations of 43.3-86.7 µM and its bactericidal activity at concentrations of 86.7-173.4 µM. This compound is 6 times more potent than ampicillin and 3 times than streptomycin against all bacteria. Compound 9 was the less active (MIC ranging from 125.4 to 344.8 µM and MBC ranging from 250.7 to 689.6 µM). Surprisingly, most of the derivatives were more efficient than ampicillin and compounds 2-8, 10, 11, 13 and 14 exhibited higher potency than streptomycin towards the majority of tested bacterial pathogens. Furthermore, these derivatives exhibited superior potency compared to the references (streptomycin and ampicillin) against E. coli and L. monocytogenes. The same good activity was observed against S. typhimurium and S. aureus.

Thus, compounds 1, 4, 10 and 13 exhibited good activity against E. coli and B. cereus with MIC ranging from 26.3 to 40.5 µM and MBC ranging from 52.6 to 81.0 µM., whereas derivatives 7 and 8 were potent against En. cloacae and E. coli. The range of MIC/MBC for Gram-positive bacteria was 26.3-344.8 µM and MBC at 52.6-689.6 µM, while for Gramnegative it was 26.3-378.5 µM, and MBC 52.6-757.0 µM, respectively showing any preference. In general, bacteria showed some similar sensitivity to compounds tested. Thus, the following bacterial strains S. aureus, M. flavus, L. monocytogenes, P. aeruginosa and En. cloacae responded to tested compounds in a similar way. E. coli emerged as the most sensitive bacterium meanwhile P. aeruginosa demonstrated the highest resistance rates.

The structure-activity relationship analysis revealed that substitution of the parent compound (1) had a positive effect on the antibacterial activity except for two cases (9, 15, i.e., 4-F and 4-Br, respectively). As was mentioned above, the most active compound was the p-nitro derivative, which according to docking prediction at E. coli Mur B active site, showed lower energy. It seems that introducing NO 2 at C-3 of phenyl core is favorable for antibacterial efficiency. Shifting this substituent to C-2 of benzene ring yielded the derivative 6 with reduced potency. Furthermore, beneficial for activity appeared to be the introduction of OH group in C2 of phenyl skeleton (2) . Displacement of the 2-OH group by 4-OH (3) had the same effect as the displacement of the 3-NO 2 group. On the contrary, the replacement of 4-OH by 4-OMe group (4) had a positive effect. However, the presence of two methoxy groups at the 2,5-positions of the benzene ring (5) appears to be not positive with respect to the single methoxy substitution, most likely due to steric hindrances.

Concerning halide derivatives, it was observed that, as in the case of nitro derivatives, the displacement of the fluoro substituent from position 3 of the aromatic ring at position 4 led to a relevant reduction in efficiency. In addition, in the case of bromo-derivatives, position 3 (14) proved to be preferred for action with respect to 4-Br substitution (15) .

Substitution at C-3 of the benzene ring appears to favor antibacterial activity. Regarding dichloro derivatives, the most active one seems to be the 2,6-dichloro derivative. Displacement of chlorine from position 6 to position 3 resulted in a small reduction in antibacterial activity while shifting of chlorine from position 6 to position 4 resulted in a greater decrease in antibacterial activity. In conclusion, the structure-action relationship study showed that antibacterial activity depends upon the nature of the substituent as well as on its position in the aromatic ring.

The compounds have also been studied for their antibacterial efficacy against resistant microbial strains (Table 2) . All compounds exhibited antibacterial activity against the tested resistant bacterial strains (MRSA, Escherichia coli and Pseudomonas aeruginosa), but to varying degrees. MIC of the derivatives was between 29.8-433.5 µM and MBC range between 59.6-867.0 µM. The antibacterial activity of these compounds can be presented in the following order: All derivatives displayed better potency than ampicillin and some even superior activity to that of streptomycin. In particular, compounds 12 and 15 exhibited better effects than streptomycin and ampicillin against all resistant strains of bacteria. Most compounds (1, 3, 4, 5, 7, 8, 10, 12, 13, 15) appeared to be more potent than streptomycin and ampicillin against the resistant strain of E. coli. In addition, compounds 4, 8, 12, 14 and 15 showed better activity than reference drugs against MRSA. The most sensitive bacterium to these compounds was E. coli, whereas methicillin-resistant S. aureus was found to be the most resistant.

In the case of resistant bacteria, it appears that in addition to the position of the substituents, the electron properties of the substituents play a significant role. In particular, it was observed that the first three best compounds contain electron acceptor groups.

The activity order of the tested compounds was different in resistant bacteria with respect to nonresistant. Compound 12, the most potent against resistant strains, was one of the less active against nonresistant and vice versa. This is likely due to the different mechanisms of action in resistant bacteria, as they develop better defense mechanisms, producing chemicals and forming dense colonies, making them more difficult to be inhibited.

Five compounds (2, 7, 8, 13, 14) were also tested for inhibition of P. aeruginosa biofilm formation.

All examined compounds were able to reduce the biofilm-forming abilities of P. aeruginosa ( Table 3) . Percentage of reduction recorded after application of concentration equal to their MIC was above 50% for 8, 13 and 14, indicating good biofilm inhibiting potential. Com-pound 2 was the least active one in this assay, suggesting that inhibition of planktonic growth rather than biofilms is its mechanism of activity. 

The compounds were then studied for their antimycotic activity, and results are displayed in Table 4 .

All compounds showed very good antifungal activity. Particularly, the ranges of MIC and MFC were 27. Bifonazole and ketoconazole, used as reference compounds, showed MIC in the range from 480 to 640 µM and from 380 to 4750 µM, respectively, whereas MFC were in the range from 640 to 800 µM and from 950 to 5700 µM, respectively. It is worth noting that all compounds exhibited much better action in comparison with references. In addition, all compounds indicated superior potency than reference drugs against T. viride, which was considered as the most sensitive fungus. Moreover, compounds 3, 4, 5, 10, 13, 14 exhibited better potency compared to standard drugs against all fungal filaments. Compounds 1, 2, 6, 7, 9, 12 displayed inhibitory actions on the growth of A. fumigatus, A. niger, P. funiculosum and P. verrucosum. P. ochrochloron emerged as the most resistant fungal species. Nevertheless, most derivatives were more efficacious than standard drugs against these fungi.

As in the antibacterial potency case, studies of structure-activity relationship revealed the dependence of the antifungal efficiency on the nature of substituents as well as on their position on the benzene skeleton. Thus, derivatives with 2,6-dichloro, 2,5-dimethoxy, 2,4-dichloro, 3-bromo, 4-hydroxy, 4-chloro, 4-methoxy, 3-nitro and 2-nitro substituents exhibited better antifungal activity than the parent compound, whereas the fluoro, 4bromo, 2,3-dichloro and 2-hydroxy derivatives were less active than the parent compound (1). It seems that 4-chloro substitution is beneficial for antifungal activity (10), while its replacement with 4-fluoro (9) resulted in a significant reduction in activity, which decreased more upon replacement with 4-bromo (15) . Among the dichloro-derivatives, 2,6-dichloro had the strongest effect. Displacement of 6-Cl at position 4 resulted in a compound with lesser action (12) , while the shift of 6-Cl to position 3 (11) led to a larger reduction in activity.

Considerable antifungal activity was also demonstrated by the 2,5-OMe derivative (5) . The mono substitution with the methoxy group at C-4 induced a reduction in activity. With regard to nitro derivatives, the activity of the 3-NO 2 compound was better compared to 2-NO 2 ; the same was observed for antibacterial activity. From all the above-mentioned, it can be concluded that the antifungal-promoting substituents are 4-chloro, 2,5-dimethoxy, 2,6-dichloro and 3-bromo. An important parameter for predicting membrane passage capability is the polar surface area (PSA) of a molecule, which is defined as the sum of the surface of polar atoms in a molecule. In particular, drugs with relatively small PSA < 140 A 2 are almost completely absorbed through the small intestine with passive diffusion.

As can be seen from the above table (Table 5) , no association was observed in any violation of the Lipinski rule. Therefore, all the compounds synthesized can very likely permeate the biological membranes as they have the appropriate physicochemical characteristics. The topological polar surface area (TPSA) of most compounds is less than 60 A 2 , which means that by oral administration, compounds are likely to be almost completely absorbed through the small intestine by passive diffusion. It was previously demonstrated that thiazolidinone derivatives act as MurB inhibitors [48] [49] [50] [51] . MurB is an enzyme belonging to the superfamily of flavoproteins and plays a key role in cell wall biosynthesis as it participates in the second stage of synthesis of peptidoglycan, which is a crucial component of the bacterial cell wall. In particular, it catalyzes the final UDP-N-acetylmuramic acid (UDPMurNAc) formation step by reducing the NADPH-dependent enol pyruvate. Taking this into account and looking to study the mode of action of our compounds, a theoretical study of their binding to the E. coli-MurB enzyme active site (PDB: 2Q85) was accomplished. Results are presented in Table S2 .

Prepared derivatives 1-15 and standard drug were subjected to docking with lanosterol 14α-demethylase from pathogenic yeast C. albicans (CYP51 Ca ) and dihydrofolate reductase to predict the probable mechanism of action using PDB: 5V5Z and PDB: 4HOF), respectively. The docking scores disclosed that CYP51 Ca was the most adequate to antifungal potency (Table S3 ).

In the last step, the potential cytotoxicity of all compounds was experimentally assessed. Based on our reported MICs and MBCs, an initial concentration of 50 µM was selected ( Figure 1A ). Five compounds (6, 7, 12, 14 and 15 ) showed high toxicity in breast cancer cell line MCF7/S0.5, suggesting that their effect toward tested bacterial and fungal species can also be partly mediated by direct cytotoxicity. Importantly, the active derivatives 1, 3, 8 and 10, which were active toward some bacterial species with MIC ranging from 26 to 63 µM, were not toxic to human cells neither at a concentration of 50 µM, which is a relatively high concentration. In the next experiments, we also tested the concentrationdependent toxicity of the three active compounds (2, 7 and 14) , which caused toxicity with different intensities at a concentration of 50 µM. As observed in Figure 1B , at lower concentrations, they were clearly non-toxic. The toxicity of nitro-compounds (6 and 7) is a general but not always presented phenomenon [52] [53] [54] Nitro-group could be reduced likely in cells of different origin, and the process is associated with a highly reactive radical formation and tissue damage. These radicals are responsible not only for their cytotoxic effect but also for the antimicrobial properties of these compounds. Moreover, lipophilicity can contribute to better intracellular permeability and higher toxicity.

According to the literature, the majority of halogenated drugs are fluorine drugs, followed by chlorine ones, while bromine derivatives are rare [55] . Interestingly, our data on mono fluorine, chlorine and bromide compounds seems to fit in the general scheme, where fluorine and chlorine compounds are inert and hence non-toxic, while bromine compounds more easily release bromine and, in comparison, to previous ones are more toxic [56] . The toxicity shown by dichlorine-containing derivatives is peculiar and not understandable by the existed data. A possibility exists that may induce membrane permeability differently, thus accordingly altering their intracellular concentration. Another explanation may be focused on differences inherent to their molecular binding capacity within the cancer cells. At the same time, they can also target P-glycoprotein with various binding capacities, a fact that may cause limitation in a different degree to their achieved intracellular concentrations. However, this is only a hypothesis that deserves further investigation.

Even if noncancerous cells are in general more resistant toward cytotoxicity than cancer cells, the 5 most active compounds (1, 2, 4, 8 and 10 ) were tested toward a renal cell line HK-2 for confirmation of safety ( Figure 1C) . As in the case of tumor cells, compounds 1, 8 and 10 were non-toxic. In contrast to cancer cells, compound 2 did not decrease the proliferation of tested noncancerous cell lines. Contrarily, compound 10 was mildly cytotoxic. 11.82, 115.03, 116.12, 127.91, 130.68, 131.12, 138.71,  143.03, 157.77, 158.02, 171.03, 174.19 . Anal. Calcd. for C 14 

This compound was published in our previous paper [48] .

2-(5-methylthiazol-2-ylimino)-5-(3-nitrobenzyliden) thiazolidin-4-one (7) This compound was published in our previous paper [48] . 13 India), BP agar and chromogenic culture media (chromID MRSA, bioMérieux, Durham, NC, USA) chromID MRSA. Suspected colonies of S. aureus on the blood agar and green colonies on chromogenic media were transferred to individual plates to obtain pure cultures. The identification was confirmed using a BBL Crystal G/P ID kit (Becton Dickinson, Nairobi, Kenya). Antimicrobial susceptibility testing was performed by the disk diffusion method with 30 µg cefoxitin discs (Rosco, Taastrup, Denmark) in accordance with the Clinical and Laboratory Standard Institute recommendations. All isolated strains of S. aureus were tested for the presence of penicillin-binding protein (PBP2) with latex agglutination tests (Slidex MRSA detection, bioMérieux, Zhujiang, New Town, China ). Staphylococcus aureus ATCC 25923 was used as the control strain. All isolates were tested for the presence of the mecA gene by PCR [59] .

Samples of rectal swabs, feces and intestines from diseased pigs were taken. In order to isolate E. coli strains, the following nutrition media were used: MacConkey agar (Torlak, Beograd, Serbia), Columbia agar (Torlak, Beograd, Serbia) with 5% defibrinated sheep blood and brilliant green agar (Torlak). For the identification of the isolated strains, laboratory tests with the following nutritious media and reagents were performed: Simmons citrate agar (Torlak), MR/VP broth (Torlak), Christensen urea agar (Torlak, Beograd, Serbia), peptone water for the indole test (Torlak), catalase and oxidase, triple sugar agar (Torlak), as well as identification systems BBL crystal entero/nonfermenter ID kit (Becton Dickinson Nairobi, Kenya,). Sensitivity studies on the isolated bacteria were completed by the disc diffusion method on Mueller-Hinton agar with the use of antibiogram discs (Bioanalyse, Ankara, Turkey) and tablets (Torlak) for the following antibiotics: penicillin, ampicillin, amoxicillin, tetracycline, neomycin, gentamicin, colistin, ceftriaxone, sulfamethoxazole with trimethoprim, enrofloxacin and florfenicol. All isolated E. coli strains were resistant to all tested antibiotics with the exception of enrofloxacin, colistin and florfenicol [60] .

The strains were isolated from cats and dogs. Samples were inoculated on Columbia agar plates (Torlak, Serbia) containing 5% sheep blood, nutrition agar (HiMedia) and MacConkey agar (Torlak) and incubated under aerobic conditions at temperatures of 37 • C and 42 • C for 24 h. Pure cultures were identified on the basis of morphological and biochemical characteristics. For identification of pigment production, subcultivation on the corresponding medium was carried out. Identification was confirmed using a BBL crystal entero/nonfermenter ID kit (Becton Dickinson). Sensitivity studies were completed by the disc diffusion method on Mueller-Hinton agar with the use of antibiogram discs (Bioanalyse) and tablets (Torlak) for the following antibiotics: penicillin G, ampicillin, amoxicillin, tetracycline, neomycin, gentamicin, ceftriaxone, sulfamethoxazole with trimethoprim, enrofloxacin and florfenicol. All isolated Pseudomonas aeruginosa strains were resistant to all tested antibiotics with the exception of enrofloxacin and florfenicol [60] .

The method was performed as described by us [61] with some modifications. Briefly, P. aeruginosa resistant strain was incubated with MIC and subMIC of tested compounds in tryptic soy broth enriched with 2% glucose at 37 • C for 24 h. After 24 h, each well was washed twice with sterile PBS (phosphate-buffered saline, pH 7.4) and fixed with methanol for 10 min. Methanol was then removed, and the plate was air-dried. Biofilm was stained with 0.1% crystal violet (Bio-Merieux, Marcy l'Etoile, France) for 30 min. Wells were washed with water, air dried, and 100 µL of 96% ethanol (Zorka, Sabac, Serbia) was added. The absorbance was read at 620 nm on a Multiskan™ FC microplate photometer, Thermo Scientific™. The percentage of inhibition of biofilm formation was calculated by the formula:

[(A 620 control − A 620 sample)/A 620 control) × 100]

For the antifungal bioassays, eight fungi were used: Aspergillus niger (ATCC 6275), Aspergillus ochraceus (ATCC 12066), Aspergillus fumigatus (human isolate), Aspergillus versicolor (ATCC 11730), Penicillium funiculosum (ATCC 36839), Penicillium ochrochloron (ATCC 9112), Trichoderma viride (IAM 5061), Penicillium verrucosum var. cyclopium (food isolate). The organisms were obtained from the Mycological Laboratory, Department of Plant Physiology, Institute for Biological Research "Siniša Stankovic", Belgrade, Serbia. All experiments were performed in duplicate and repeated three times [62, 63] .

All tests were performed three times, and the values were determined as standard deviation (SD) and mean values. A one-way ANOVA test was allowed to determine variance analysis with Tukey HSD Test (0.05 levels). The analysis was executed with the help of SPSS statistics software (version 18).

CellTiter 96 ® aqueous nonradioactive cell proliferation assay (Promega, Madison, WI, USA) was performed to evaluate the in vitro effects of evaluated compounds in breast adenocarcinoma MCF7/S0.5 (parental MCF7 cells adapted to low-sera conditions) and human kidney immortalized cell line HK-2. The employed method uses the bioreduction of tetrazolium salt of MTS (3-(4,5-dimethylthiazol-2-yl)-5-(3-carboxymethoxyphenyl)-2-(4sulfophenyl)-2H-tetrazolium) into a colored formazan with an absorbance peak maximum at wavelength 490 nm. Only viable cells are able to metabolize the compound. Experiments were conducted in accordance with manufacturer guidelines. Briefly, cells were treated with the test compounds, negative control (SDS 10%) or vehicle (DMSO 0.1%) for 48 h in 96wells plates. At the end of the treatment, 20 µL of MTS reagent was added to each well and incubated for a further 3 h prior to absorbance measurement using a plate reader (Hidex Sense Beta Plus plate reader, Hidex, Turku, Finland). MCF7/S0.5 cell line was cultivated in DMEM/F-12 media w/o phenol red supplemented with 1% FBS and insulin 6 ng/mL. HK-2 cells were cultivated in DMEM with high-glucose and L-glutamine, supplemented with 10% FBS. Results are expressed as the relative cell viability, considering the vehicle to have 100% viability.

Fifteen newly designed and synthesized 5-benzyliden-2-(5-methylthiazol-2-ylimino) thiazolidin-4-ones exhibited significant inhibition of the growth of a wide spectrum of Gram-positive, Gram-negative bacteria and fungi. The majority of derivatives were more efficient than the standard antibacterial drug ampicillin. Compounds 2-8, 10, 11, 13 and 14 also exhibited higher potency than streptomycin. The most sensitive bacterium was E. coli; meanwhile, P. aeruginosa demonstrated the highest resistance rates.

Furthermore, some of the compounds showed better or comparable potency compared to streptomycin, with the most potent among them being compound 8 (15 and 7-fold more active than ampicillin and streptomycin, respectively). It was observed that, among the Gram-negative bacteria, the most sensitive to the tested compounds was E. coli, while S. typhimurium was the most resistant one. Regarding the Gram-positive bacteria, the most sensitive one was B. cereus, while L. monocytogenes were found to be the most resistant bacterium.

Furthermore, all compounds exhibited antibacterial potency against the tested resistant bacterial strains displaying better efficacy than ampicillin and some of them (12 and 15) even higher than streptomycin . Compounds 1, 3, 4, 5, 7, 8, 10, 12, 13 , 15 appeared to be more potent than streptomycin and ampicillin against the resistant strain of E. coli, which was the most sensitive, while some of them (4, 8, 12, 14 and 15 ) exhibited better activity than reference drugs against methicillin-resistant Staphylococcus aureus, the most resistant strain. Compounds 8, 13 and 14 exhibited significant antibiofilm activity.

As regards antifungal activity, most of the examined compounds displayed better potency than reference drugs, ketoconazole and bifonazole. Thus, the most active compound 10 was found to be 4-8 and 7-13-fold more active than bifonazole and ketoconazole, respectively. Docking analysis to E. coli MurB indicated a probable involvement of MurB inhibition in the antibacterial mechanism of compounds tested, while docking to 14α-lanosterol demethylase (CYP51) and tetrahydrofolate reductase of Candida albicans indicated a probable implication of CYP51 reductase at the antifungal activity of the compounds.

Finally, toxicity prediction revealed that compounds are not toxic. In addition, according to the prediction of physicochemical parameters for the passage through biological membranes, they will likely be absorbed via passive diffusion when given orally. Anyway, their toxicity toward a human cell line was experimentally assessed at a relatively high concentration of 50 µM. Several active compounds were not toxic even at this high concentration.

Supplementary Materials: The following are available online at https://www.mdpi.com/2079-6 382/10/3/309/s1, Table S1 : Predict toxicity of compounds with OpenTox and CBLIGAND title, 1H-13C-NMR spectra mass spectras, docking studies. 

The data presented in this study are available on request from the corresponding author.

-methylthiazol-2-ylimino)-5-(2,4-dichlorobenzyliden) thiazolidin-4-one (12) Yield: 57.7%, mp. 260-261 • C (dioxane), R f = 0

Found (%): C, 45.36

2-(5-methylthiazol-2-ylimino)-5-(2,6-dichlorobenzyliden) thiazolidin-4-one (13) Yield: 94.6%, mp. 225-226 • C (dioxane), R f = 0

33 (s, 1H

PhCH 3: C 2 H 5 OH 8:2), IR: (cm −1 , Nujol), 1704 (carbonyl), 2356 (N-H amide); 1 H-NMR (DMSO-d 6 ; 300 MHz) δ: 2.36 (s, 3H

PhCH 3: C 2 H 5 OH 8:2), IR: (cm −1 , Nujol), 1711 (carbonyl), 3249 (-N-H amide). 1 H-NMR: (δ, DMSO-d 6, 300 MHz 2.2 (s, 3H

Antibacterial Action Bacterial strains utilized include Gram-negative: Salmonella typhimurium

Enterobacter cloacae (ATCC 35030) and Gram-positive bacteria: Micrococcus flavus (ATCC 10240), Bacillus cereus (isolated clinically), Staphylococcus aureus (ATCC 6538) and Listeria monocytogenes (NCTC 7973) bacteria. Pathogens were provided from the Mycological Laboratory, Institute for Biological Research "Siniša Stankovic" Belgrade. Resistant strains used were MRSA, E. coli and P. aeruginosa. The MIC/MBC were effectuated utilizing microdilution assay as previously described

After incubation at 37 • C for 24 h, the colonies were presumptively identified according to morphological features, pigment production, Gram staining results, catalase and oxidase tests, type of hemolysis and characteristic growth on Baird-Parker agar plates

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Understanding the mechanisms and drivers of antimicrobial resistance

The dynamics of gut-associated microbial communities during inflammation

Cystic Fibrosis and Pseudomonas aeruginosa: The Host-Microbe Interface

Antifungal drug resistance: Mechanisms, epidemiology, and consequences for treatment

Echinocandin resistance in human pathogenic fungi

Synthesis of 2-phenylamino-thiazole derivatives as antimicrobial agents

Synthesis and study of 1,3,5-triazine based thiazole derivatives as antimicrobial agents

Antibacterial Characterization of Novel Synthetic Thiazole Compounds against Methicillin-Resistant Staphylococcus pseudintermedius

Synthesis of thiazole derivatives as antimicrobial agents by green chemistry technology

New Series of Thiazole Derivatives: Synthesis, Structural Elucidation, Antimicrobial Activity, Molecular Modeling and MOE Docking. Molecules

Evaluation the local anaesthetic activity of derivatives of 3-amino-1,2-[d]benzoisothiazoles on sciatic nerve of rat

Synthesis and in silico investigation of thiazoles bearing pyrazoles derivatives as anti-inflammatory agents

Synthesis and biological evaluation of some 5-arylidene-2-(1,3-thiazol-2-ylimino)-1,3-thiazolidin-4-ones as dual anti-inflamatory/antimicrobial agents

Anti-inflammatory and Anti-ulcer Activities of New Fused Thiazole Derivatives Derived from 2-(2-Oxo-2H-chromen-3-yl)thiazol-4(5H)-one

Trisubstituted thiazole derivatives: A novel and potent class of non-nucleoside inhibitors of wild type and mutant HIV-1 reverse transcriptase

Novel thiazolidin-4-ones as potential non-nucleoside inhibitors of HIV-1 reverse transcriptase

Synthesis of Novel Thiazole Derivatives as Analgesic Agents

Novel hybrids of pyrazolidinedione and benzothiazole as tzd analogues. Rationale, design, synthesis and in vivo anti-diabetic evaluation

A Retrospect Study on Thiazole Derivatives as the Potential Antidiabetic Agents in Drug Discovery and Developments

Synthesis, anticancer activity and mechanism of action of new thiazole derivatives

Anticancer Potential of Thiazole Derivatives: A Retrospective Review

Cytotoxicity and Antioxidant Potential of Novel2-(2-((1H-indol-5yl)methylene)-hydrazinyl)-thiazoleDerivatives

Antifungal and anthelmintic activity of novel benzofuran derivatives containing thiazolo benzimidazole nucleus: An in vitro evaluation

A Review on Biological Activity of Imidazole and thiazole moieties and their derivative

Exploring Anti-inflammatory Potential of Thiazolidinone Derivatives of Benzenesulfonamide via Synthesis

Design, synthesis and biological screening of Novel 2,4-dichlorophenoxy acetic acid substituted thiazolidin-4-ones as anti-inflammatory agents

Docking assisted design of novel 4-adamantanyl-2-thiazolylimino-5-arylidene-4-thiazolidinones as potent NSAIDs

Synthetic and medicinal perspective of thiazolidinones: A review

In vitro antioxidant activity of thiazolidinone derivatives of 1,3-thiazole and 1,3,4-thiadiazole

Study of novel anticancer 4-thiazolidinone derivatives

Synthesis, characterization and biological evaluation of thioureas, acylthioureas and 4-thiazolidinones as anticancer and antiviral agents

Novel 4-Thiazolidinone Derivatives as Anti-Infective Agents: Synthesis, Characterization, and Antimicrobial Evaluation

4-Thiazolidinone derivatives: Synthesis, antimicrobial, anticancer evaluation and QSAR studies

4-thiazolidinone derivatives: Synthesis and biological study

Characterization and Antifungal Activity of Some Substituted 4-thiazolidinone Derivatives

Synthesis and antimicrobial activity of novel 2-thiazolylimino-5-arylidene-4-thiazolidinones

Collaborative development of predictive toxicology applications

Synthesis and aldose reductase inhibitory activity of 5-arylidene-2,4-thiazolidinediones

5-Arylidene-2-imino-4-thiazolidinones: Design and synthesis of novel anti-inflammatory agents

Novel thiazole-based thiazolidinones as potent anti-infective Agents: In silico PASS and toxicity prediction, Synthesis, Biological Evaluation and Molecular Modelling

Antimicrobial Evaluation and Molecular Modeling Study of 1,2,4-Triazole-Based 4-Thiazolidinones

4-Thiazolidinones: Novel inhibitors of the bacterial enzyme MurB

Kinetic characterization of wild-type and S229A mutant MurB: Evidence for the role of Ser 229 as a general acid

Nitro-Group-Containing Drugs

Effects of the nitro-group on the mutagenicity and toxicity of some benzamines

Mechanism of toxicity of nitro compounds used in the chemotherapy of trichomoniasis

Halogen atoms in the modern medicinal chemistry: Hints for the drug design

Effect of bromine and chlorine positioning in the induction of renal and testicular toxicity by halogenated propanes

Design, synthesis and antimicrobial activity of usnic acid derivatives

Chemical, nutritive composition and a wide range of bioactive properties of honey mushroom Armillariamellea (Vahl: Fr.) Kummer. Food Funct

Rapid detection, differentiation and typing of methicillin-resistant Staphylococcus aureus harbouring either mecA or the new mecA homologue mecA(LGA251)

Inhibition of biofilm formation, quorum sensing and infection in Pseudomonas aeruginosa by natural products-inspired organosulfur compounds

Novel Hit Compounds as Putative Antifungals: The Case of Aspergillus fumigatus

Pyrimethanil: Between efficient fungicide against Aspergillus rot on cherry tomato and cytotoxic agent on human cell lines

The authors declare no conflict of interest.