Synthesis of Tetracyclic Spirooxindolepyrrolidine-Engrafted Hydantoin Scaffolds: Crystallographic Analysis, Molecular Docking Studies and Evaluation of Their Antimicrobial, Anti-Inflammatory and Analgesic Activities

In a sustained search for novel potential drug candidates with multispectrum therapeutic application, a series of novel spirooxindoles was designed and synthesized via regioselective three-component reaction between isatin derivatives, 2-phenylglycine and diverse arylidene-imidazolidine-2,4-diones (Hydantoins). The suggested stereochemistry was ascertained by an X-ray diffraction study and NMR spectroscopy. The resulting tetracyclic heterocycles were screened for their in vitro and in vivo anti-inflammatory and analgesic activity and for their in vitro antimicrobial potency. In vitro antibacterial screening revealed that several derivatives exhibited remarkable growth inhibition against different targeted microorganisms. All tested compounds showed excellent activity against the Micrococccus luteus strain (93.75 µg/mL ≤ MIC ≤ 375 µg/mL) as compared to the reference drug tetracycline (MIC = 500 µg/mL). Compound 4e bearing a p-chlorophenyl group on the pyrrolidine ring exhibited the greatest antifungal potential toward Candida albicans and Candida krusei (MIC values of 23.43 µg/mL and 46.87 µg/mL, respectively) as compared to Amphotericin B (MIC = 31.25 and 62.50 µg/mL, respectively). The target compounds were also tested in vitro against the lipoxygenase-5 (LOX-5) enzyme. Compounds 4i and 4l showed significant inhibitory activity with IC50 = 1.09 mg/mL and IC50 = 1.01 mg/mL, respectively, more potent than the parent drug, diclofenac sodium (IC50 = 1.19 mg/mL). In addition, in vivo evaluation of anti-inflammatory and analgesic activity of these spirooxindoles were assessed through carrageenan-induced paw edema and acetic acid-induced writhing assays, respectively, revealing promising results. In silico molecular docking and predictive ADMET studies for the more active spirocompounds were also carried out.


Introduction
Non-steroidal anti-inflammatory drugs (NSAIDs) are the most commonly used drugs in clinical practice to relieve arthritis pain and inflammation [1,2].They generally work by inhibiting cyclooxygenase (COX) and lipoxygenase (LOX) enzymes, thereby preventing the biosynthesis of prostaglandin that protects the gastric mucosa.However, long-term use of these drugs is usually associated with adverse side effects, particularly ulcers and gastrointestinal irritation, but also renal and cardiovascular damage [3][4][5].Over recent decades, an increasing number of new anti-inflammatory agents have been developed to alleviate the acuteness of inflammatory complications.Nevertheless, most of the currently approved NSAIDs exhibit either undesirable side reactions or drug tolerance [6].
On the other side, multidrug-resistant (MDR) pathogens have dramatically expanded all over the globe in recent years and have become a serious public health emergency [7][8][9].Without effective antimicrobials, infectious diseases caused by microorganisms become increasingly difficult, or even impossible, to treat, increasing the risk of severe illness, disability and death.For instance, resistant Pseudomonas aeroginosa and Staphylococcus aureus are among the leading factor of infections and increased healthcare costs [10].The World Health Organization (WHO) estimates that approximately 64% of patients infected with methicillin-resistant Staphylococcus aureus (MRSA) are more likely to die than other patients with drug-sensitive infections [11,12].Therefore, the development of new therapeutic options with a safer profile, greater efficacy and lower side effects remains a challenge for the medicinal chemist.
However, despite the demonstrated therapeutic efficacy inherent in these two specific heterocycles, a limited number of synthetic methods have been reported over the years to access N-spiroheterocycles that merge hydantoin and spiropyrrolidine derivatives [43].Interestingly, the conception of spiropyrrolidines fused to hydantoin and the subsequent exploration of their biological activities as a means to develop novel drug candidates has largely remained untapped.We envisioned that the combination of these distinct heterocycles holds promising potential in the creation of innovative and biologically relevant molecules.The discovery of biologically active compounds embedded in spirooxinole and hydantoin scaffolds prompted us to investigate further modifications within this class of compounds.Similarly, hydantoin derivatives (imidazolidine-2,4-diones) [28,29] emerged as privileged scaffolds in medicinal chemistry due to their various biological and therapeutic applications such as anticancer [30][31][32], anti-inflammatory [33][34][35], antidiabetic [36], anticonvulsant [37,38] and antimicrobial agents [39].With such broad bioactivities, many hydantoin derivatives featured in several clinically used drugs such as phenytoin (anti-epileptic agent) [40], nilutamide (nonsteroidal androgen antagonists) [41] and nitrofurantoin (antibiotic for the treatment of infections caused by multi-drug resistant pathogens) (Figure 1) [42].They are also frequently encountered in natural molecules and have found a diversity of applications in organic synthesis.
However, despite the demonstrated therapeutic efficacy inherent in these two specific heterocycles, a limited number of synthetic methods have been reported over the years to access N-spiroheterocycles that merge hydantoin and spiropyrrolidine derivatives [43].Interestingly, the conception of spiropyrrolidines fused to hydantoin and the subsequent exploration of their biological activities as a means to develop novel drug candidates has largely remained untapped.We envisioned that the combination of these distinct heterocycles holds promising potential in the creation of innovative and biologically relevant molecules.The discovery of biologically active compounds embedded in spirooxinole and hydantoin scaffolds prompted us to investigate further modifications within this class of compounds.
Here, we report the design and synthesis of novel hydantoin-grafted spiroxindoles.The current approach involves one-pot multicomponent reactions (MCRs) of isatin 1 2phenylglycine 2 and (Z)-5-arylidene 2,4-imidazolidinediones 3 (Scheme 1).The newly synthesized compounds were evaluated against four pathogenic Gram-positive and Gram-negative bacteria and two fungal strains using the in vitro micro diffusion technique.The in vitro and in vivo anti-inflammatory and analgesic activity of the new spirocompounds were also evaluated and the results were further supported by molecular modeling studies to provide a deeper understanding of the plausible binding interactions of the most active compounds.Structure-activity relationship (SAR) trends were also explored to better understand the structural modification substrate scope and extension of Here, we report the design and synthesis of novel hydantoin-grafted spiroxindoles.The current approach involves one-pot multicomponent reactions (MCRs) of isatin 1 2phenylglycine 2 and (Z)-5-arylidene 2,4-imidazolidinediones 3 (Scheme 1).The newly synthesized compounds were evaluated against four pathogenic Gram-positive and Gramnegative bacteria and two fungal strains using the in vitro micro diffusion technique.The in vitro and in vivo anti-inflammatory and analgesic activity of the new spirocompounds were also evaluated and the results were further supported by molecular modeling studies to provide a deeper understanding of the plausible binding interactions of the most active compounds.Structure-activity relationship (SAR) trends were also explored to better understand the structural modification substrate scope and extension of the new hybrids.

Synthetic Chemistry
At the outset of our studies, we performed the three-component reaction between an equivalent amount of chloro-isatin 1b, 2-phenylglycine 2 with (Z)-5-(p-methoxybenzylidene) imidazolidine-2,4-dione 3a as model substrates to optimize the reaction parameters (Scheme 1).The reaction was explored in different solvents and the results were summarized in Table 1.The spirooxindolepyrrolidine 4a was formed in 70 and 60% yields by performing the reaction in EtOH and CH 3 CN, respectively (Table 1, entries 1 and 5).The yields of the isolated spiroadduct were inferior in 1,4-dioxane, THF, EtOH/H 2 O and toluene (Table 1, entries 2-4 and 6).Gratifyingly, the reaction proceeded smoothly in refluxing the MeOH to furnish the desired N-spiroheterocycle 4a in 85% yield as a single regioisomer (Table 1, entry 5).Subsequently, the generality of the one pot reaction was examined using several substituted dipolarophiles 3a-f and isatins 1a-d, resulting in the synthesis of diversely substituted products 4a-m in good yields and with high regio-and stereoselectivity (Scheme 2).As shown in Scheme 2, the multicomponent reaction appears to be tolerant towards both electron-donating and electron-withdrawing groups at the para position of the aromatic ring of arylidene hydantoins 3, thereby affording the corresponding products 4a-m in 80-91% yield range (Scheme 2).The system also proceeded well with halogen substituents at the aromatic ring of isatin such as chloro (1b) and bromo (1c), providing the desired dispiro[imidazolidine-4,3 -pyrrolidine-2 ,3 -indoline]-2,2 ,5-triones 4 in 76−91% isolated yields (Scheme 2).Furthermore, N-protected isatin 1d was compatible with the reaction.

Spectroscopic and Crystallographic Characterization of the Cycloadducts 4
The structure, the purity and the relative configuration of all products were elucidated from their 1D and 2D NMR spectroscopic data and were unequivocally confirmed by an X-ray data analysis performed on cycloadduct 4i.Relevant 1 H and 13 C chemical shifts of dispiropyrrolidine 4i are shown in Figure 2.
The 1 H NMR spectrum of the cycloadduct 4i shows a doublet at δ H 3.75 (J = 9.6 Hz) corresponding to H-4 proton of the pyrrolidine ring which showed 1 H- 13 C HSQC correlation (Figure S20) with the doublet of a doublets at δ 5.40 ppm (J = 9.6 Hz and J = 4.8 Hz), attributed to the pyrrolidine proton H-5.The multiplicity and the coupling constant values of these protons confirm the formation of the regioisomer 4i as in the case of hypothetical regioisomer 4i (Scheme 1), pyrrolidinyl protons should exhibit a singlet instead of a doublet in the 1 H NMR spectrum.Furthermore, the carbonyl group at 179.1 ppm is attributed to the isatin carbonyl C-2 based on its heteronuclear multiple-bond correlation (HMBC) (Figure S21) with the H-1 hydrogen of pyrrolidine ring.The two downfield singlets resonating at 10.60 and 7.80 ppm can be attributed to the NH-1 and NH-1 hydrogens of the oxindole and hydantoin moieties on the basis of their HMBCs with C-2 and C-3 spirocarbons at 73.3 and 75.9 ppm, respectively, providing further evidence for the proposed structure.

Spectroscopic and Crystallographic Characterization of the Cycloadducts 4
The structure, the purity and the relative configuration of all products were elucidated from their 1D and 2D NMR spectroscopic data and were unequivocally confirmed by an X-ray data analysis performed on cycloadduct 4i.Relevant 1 H and 13 C chemical shifts of dispiropyrrolidine 4i are shown in Figure 2. The 1 H NMR spectrum of the cycloadduct 4i shows a doublet at δ H 3.75 (J = 9.6 Hz) corresponding to H-4 proton of the pyrrolidine ring which showed 1 H- 13 C HSQC correlation (Figure S20) with the doublet of a doublets at δ 5.40 ppm (J = 9.6 Hz and J = 4.8 Hz), attributed to the pyrrolidine proton H-5.The multiplicity and the coupling constant values of these protons confirm the formation of the regioisomer 4i as in the case of

Spectroscopic and Crystallographic Characterization of the Cycloadducts 4
The structure, the purity and the relative configuration of all products were eluci dated from their 1D and 2D NMR spectroscopic data and were unequivocally confirmed by an X-ray data analysis performed on cycloadduct 4i.Relevant 1 H and 13 C chemica shifts of dispiropyrrolidine 4i are shown in Figure 2. The 1 H NMR spectrum of the cycloadduct 4i shows a doublet at δ H 3.75 (J = 9.6 Hz corresponding to H-4 proton of the pyrrolidine ring which showed 1 H- 13 C HSQC correla tion (Figure S20) with the doublet of a doublets at δ 5.40 ppm (J = 9.6 Hz and J = 4.8 Hz) attributed to the pyrrolidine proton H-5.The multiplicity and the coupling constant val ues of these protons confirm the formation of the regioisomer 4i as in the case o The regio-and stereochemistry of the 1,3-dipolar cycloaddition was further corroborated by a single-crystal X-ray analysis of spiropyrrolidine 4i, whose molecular structure is depicted in Figure 3.It reveals that the carbonyl carbon of the oxindole component and (i) carbonyl group of hydantoin part (C-10 in the crystal structure) are in trans-relationship, and (ii) a cis -relationship with H-5 pyrrolidinyl proton bonded to C-5 (C-19 in the crystal structure).
the proposed structure.
The asymmetric unit of 4i shown in Figure S30 contains two independent molecules (with slightly different bond lengths and angles), crystallizing in the triclinic space group P-1, along with H 2 O molecules.The stereochemistry of the tetracyclic core bearing two additional aryl groups at C19 and C12 is in the solid state in line with the NMR data in solution and establishes the transoid arrangement of two the hydrogen atoms of the pyrrolidine-type five-membered cycle.As visualized in Figure S30 49 Å) completes the supramolecular interactions occurring in this highly organized network (Figure 4).

Biological Activity 2.3.1. In Vitro Lipoxygenase Inhibitory Assay and Structure-Activity Relationship (SAR) Study
Lipoxygenases are a family of monomeric proteins that catalyze oxidation of polyunsaturated fatty acids (PUFA) (linoleic, linolenic and arachidonic acid) to produce hydroperoxides [44,45].Fractions' anti-LOX activity was also measured as inhibition of linoleic acid's peroxidation to hydroperoxylinoleic acid [46].
To evaluate the prospects of the newly synthesized spirooxindoles as promising drug candidates, we first studied their inhibitory potency against the Lipoxygenase-5 (LOX-5) enzyme.The IC 50 values (concentration causing 50% enzyme inhibition) of the tested compounds and the reference drug diclofenac sodium are recorded in Table 2.  Lipoxygenases are a family of monomeric proteins that catalyze oxidation of polyunsaturated fatty acids (PUFA) (linoleic, linolenic and arachidonic acid) to produce hydroperoxides [44,45].Fractions' anti-LOX activity was also measured as inhibition of linoleic acid's peroxidation to hydroperoxylinoleic acid [46].
To evaluate the prospects of the newly synthesized spirooxindoles as promising drug candidates, we first studied their inhibitory potency against the Lipoxygenase-5 (LOX-5) enzyme.The IC50 values (concentration causing 50% enzyme inhibition) of the tested compounds and the reference drug diclofenac sodium are recorded in Table 2.As shown in Table 2, all tested spirooxindoles exhibited modest to potent inhibitory activity (IC 50 = 1.01-4.96mg/mL) against LOX-5 enzyme.Interestingly, spirooxindoles 4i and 4l (IC 50 = 1.09 mg/mL and IC 50 = 1.01 mg/mL, respectively) showed improved LOX-5 inhibition profile better that of diclofenac sodium (IC 50 = 1.19 mg/mL) (Table 2).
A brief analysis of the SAR of the newly spirooxindole-hydantoin derivatives revealed the following: compounds 4f (IC 50 = 4.92 mg/mL) and 4g (IC 50 = 4.96 mg/mL) bearing the N-benzyl substituent, were comparably less active than the other tested heterocycles.This result could be explained by means of the steric effect of the benzyl group resisted the binding ability with the LOX-5 enzyme.The introduction of halogen substituents (4e, 4h-k) or hydroxyl group (4l-m) at the para position of the aromatic ring of the hydantoin, caused a remarkably increase of the in vitro LOX-5 inhibitory activity.This could be due to the lipophilicity of these groups improving the bioavailability.In addition, compound 4i and 4l featuring an unsubstituted isatin ring expressed the highest inhibitory potency.

Carrageenan-Induced Paw Edema Test
Compounds 4i and 4l, which showed the more potent in vitro lipoxygenase inhibitory, were accessed for their in vivo anti-inflammatory activity using carrageenan-induced rat paw edema method as reported by Lopes et al. [47].Diclofenac sodium was used as a reference drug.This method is used to assess the ability of the tested compounds to reduce the edema produced in the rat paw after being injected with carrageenan (https://en.wikipedia.org/wiki/Carrageenan(accessed on 16 October 2023).Results recorded in Table 3 shows that the injection of carrageenan produced a local edema that increased progressively to reach its maximum after 4h.However, the ingestion of 4i and 4l reduced the edema volume by 33% and 32%, respectively, 4 h after the administration of these compounds.Compounds 4i and 4l were tested in comparison of reference drug diclofenac sodium in dose of 10 mg/kg [48].Drugs were administrated orally 1 h before carrageenan injection.Data are mean ± SEM (n = 5 each).

In Vivo Analgesic Assay
The in vivo analgesic activity of the candidate drugs 4i and 4l was assessed by the acetic acid-induced writhing test using diclofenac sodium as positive controls as reported previously [49][50][51][52].
Acetic acid injection induces peritoneal inflammation in mice which reacts with a characteristic stretching behavior, called writhing.Any writhing was considered a positive response.The efficacy and potency of analgesic activity of the test compounds is inferred from the reduction in the frequency of writhings [53].
As can be seen in Table 4, the administration of the candidate drugs 4i and 4l to acetic acid-induced pain in rats exert good analgesic activity.In fact, the administration by injection of acetic acid to control rats provoked 63 instances of writhing (Table 4).Pretreatment of rats with 4l, 4i, and diclofenac sodium at 100 mg/kg reduced the instances of writhing to 36, 29 and 23, respectively (42, 53, and 63% inhibition, respectively).

Acute Toxicity
The acute toxicity test (Table 5) showed that administration of compounds 4i and 4l up to a dose of 16.25 mg/kg to rats did not cause any toxicity or physiological or biochemicals changes in the liver (AST and ALT activities) and -kidneys (Albulin, urea and ceat rates) functions.In this part, the spiropyrrolidines 4a-m were selected to be screening for their antimicrobial activities, using in vitro micro diffusion method, against multiple bacterial strains (Staphylocoocus aureus ATCC 25923, Escherichia coli ATCC 25922, Pseudomonas aeruginosa ATCC 27950, Micrococcus luteus NCIMB 8166), and two pathogenic reference yeasts namely Candida albicans ATCC 90028 and Candida kreusei ATCC 6258.
The results showed that all synthesized compounds 4a-m exhibited excellent antibacterial activity against M. luteus strain with MIC values ranging from 93.75 to 375 µg/mL.The spiropyrrolidines 4c, 4h, 4g, and 4m were the most potent derivatives with MIC values of 93.75 µg/mL, as compared to the reference antibiotic Tetracycline (MIC value of 500 µg/mL) (Figure 5).The best activity against S. aureus pathogen was obtained for compound 4g (MIC = 23.34µg/mL) followed by 4b, 4e, and 4l with MIC value of 46.87 µg/mL.We also noticed a moderate growth inhibition of the tested compounds towards E. coli (187.50 µg/mL ≤ MIC ≤ 750 µg/mL) and P. Aeroginosa (93.75 µg/mL ≤ MIC ≤ 187.50 µg/mL).Notably, compounds 4c and 4m exhibited significant antibacterial activity towards E. coli (187.50 µg/mL in MIC), higher than that of Tetracycline (MIC = 256 µg/mL).It is worth noting that compound 4e demonstrated strong antifungal activity against both the antifungal strains C. albicans and C. krusei with MIC values of 23.43 and 46.87 µg/mL, in comparison with Amphotericin B (MIC = 31.25 and 62.50 µg/mL, respectively).
To further determine the killing efficiency of the synthesized spiropyrrolidines against selected strains, the minimum bactericidal concentration (MBC) and the minimum fungicidal concentration (MFC) were assessed by the agar method [54].The results of MBC and MFC assays are summarized in Table 6.To further determine the killing efficiency of the synthesized spiropyrrolidines against selected strains, the minimum bactericidal concentration (MBC) and the minimum fungicidal concentration (MFC) were assessed by the agar method [54].The results of MBC and MFC assays are summarized in Table 6.Interestingly, most of the synthesized molecules exhibited good MBCs results versus Gram-negative pathogen E. coli, and compounds 4b, 4d, 4f, 4g, 4h, and 4m revealed better efficacy (MBC values in the range of 187.50-374 µg/mL) than the standard tetracycline reference drug (MBC of 512 µg/mL).
Tetracycline was used as reference drug for the antibacterial assay while Amphotericin B was used as a standard antifungal drug.The results are summarized in the histograms presented in Figure 6.
Notably, compounds 4b and 4c were effective against the bacterial strain P. aeruginosa, while 4h and 4m were active against M. luteus (MBC = 187.50µg/mL).However, no significant antibacterial activity was observed towards the Gram-positive bacteria S. aureus.The MFC results of the tested fungal strains showed that C. albicans is more sensitive to all spiropyrrolidines (except for 4d and 4h).The MFC values ranged from 23.43 to 187.50 µg/mL, while for Amphotericin B, it was recorded as 500 µg/mL.Compound 4e also showed a good killing efficacy against the C. krusei strain, with an MBC value of 46.87 µg/mL.Notably, compounds 4b and 4c were effective against the bacterial strain P. aeruginosa, while 4h and 4m were active against M. luteus (MBC = 187.50µg/mL).However, no significant antibacterial activity was observed towards the Gram-positive bacteria S. aureus.The MFC results of the tested fungal strains showed that C. albicans is more sensitive to all spiropyrrolidines (except for 4d and 4h).The MFC values ranged from 23.43 to 187.50 µg/mL, while for Amphotericin B, it was recorded as 500 µg/mL.Compound 4e also showed a good killing efficacy against the C. krusei strain, with an MBC value of 46.87 µg/mL.

Evaluating the Bactericidal and Bacteriostatic Effects: MBC/MIC Ratio of the Spiropyrrolidines against Microbial Strains
The bactericidal and bacteriostatic action of the spiropyrrolidines 4a-m on selected organisms was determined using their MBC/MIC ratio.The compounds are considered as bactericidal or fungicidal agents when the MBC/MIC or MFC/MIC ratios ≤ 4 and as bacteriostatic or fungistatic if these ratios are >4.All the tested spiropyrrolidines exhibited a bactericidal effect (MBC/MIC ≤ 4) against gram positive and Gram-negative bacteria, except derivatives 4c, 4g, and 4h that demonstrated a bacteriostatic effect (MBC/MIC = 8 > 4) against M. luteus pathogen and 4b showing a bacteriostatic action towards S. aureus strain (MBC/MIC = 16).For the fungal strains, the majority of the synthesized heterocycles can be classified as fungicidal agents, especially compounds 4a, 4b, 4e, 4g, 4i, 4k, 4l, and 4m which showed MFC/MIC ratios ≤ 4 on both strains C. Albicans and C. Krusei.The bactericidal and bacteriostatic action of the spiropyrrolidines 4a-m on selected organisms was determined using their MBC/MIC ratio.The compounds are considered as bactericidal or fungicidal agents when the MBC/MIC or MFC/MIC ratios ≤ 4 and as bacteriostatic or fungistatic if these ratios are >4.All the tested spiropyrrolidines exhibited a bactericidal effect (MBC/MIC ≤ 4) against gram positive and Gram-negative bacteria, except derivatives 4c, 4g, and 4h that demonstrated a bacteriostatic effect (MBC/MIC = 8 > 4) against M. luteus pathogen and 4b showing a bacteriostatic action towards S. aureus strain (MBC/MIC = 16).For the fungal strains, the majority of the synthesized heterocycles can be classified as fungicidal agents, especially compounds 4a, 4b, 4e, 4g, 4i, 4k, 4l, and 4m which showed MFC/MIC ratios ≤ 4 on both strains C. Albicans and C. Krusei.

SAR Study
The SAR was established to unravel the important features responsible for the antimicrobial activity of the tested compounds.The influence of different substituents on the isatin nucleus as well as on the aromatic cycle of the dipolarophile was therefore explored.Biological assays results indicated that compounds 4b and 4d with electron-donating groups (CH 3 and OCH 3 ) at the para-position of phenyl ring exhibit better inhibition against S. aureus than derivatives 4e and 4h containing chloro substituent attached to the same phenyl ring.Moreover, compounds with electron-donor substituents attached to the phenyl ring of the dipolarophile part generally displayed a higher inhibitory potency than derivatives incorporating electron-withdrawing groups bonded to the identical phenyl ring.
Derivatives that had an electron-donating groups (CH 3 , OCH 3 and OH) at the para and ortho positions of the phenyl ring are more effective against Gram-negative bacteria P. aeroginosa.For instance, spiropyrrolidines 4b, 4c, and 4d feature electron-donating substituents (CH 3 and OCH 3 ) at the para-position of the phenyl ring exhibited better inhibition compared to compounds containing halogen groups (Cl, Br, and F) attached to the same phenyl ring.
For the Gram-negative strain E. coli, compounds 4c and 4m displayed significant inhibition potency owing to their chloro-substituted isatin nucleus and electron-donating groups (OCH 3 and OH).Notably, the inhibitory activity is linked to both the substitutions on the dipolarophile and isatin core.
All compounds are more active against M. luteus compared to tetracycline, regardless of the nature of the substituents present on both the isatin and the dipolarophiles unit.However, a noteworthy observation is that the activity generally increases by an electronwithdrawing group attached to the isatin core and decreases in the case of unsubstituted isatin-derivatives (4e, 4i, and 4l).

Computational Approach
In an attempt to rationalize the observed bioactivity for the newly synthesized derivatives, molecular docking studies were performed.The most antibacterial spirooxindolehydantoins, i.e., 4c, 4g, and 4h were docked into the active site of three bacterial targets: Thymidylate Kinase (TMK) (PDB ID 4QGG) from S. aureus, (3-oxoacyl-[acyl-carrier-protein) synthase 3 (PDB ID 4EWP) from M. luteus, DNA gyrase (PDB ID 4DUH) from E. coli.The ligand 4e was docked to the target secreted aspartic protease (PDB ID 3Q70) from C. albicans and C. krusei.The Ligands 4i and 4l with the most promising ant-inflammatory potential were docked into the active sites of LOX-5 (PDB ID: 3V99).The PDB binding structures of different target enzymes are presented in Figures S31-S42 of the Supplementary Material.

MolDock Score and Poses Analysis
The potencies of the most bioactive compounds: 4c, 4g, 4h, 4e, 4i and 4l were measured computationally in terms of their MolDock Score.MolDock Score is actually the strength of the intra-molecular interactions among multiple molecules within the binding pockets of selected targets.After having the molecular docking calculation for all 4c, 4g, 4h, 4e, 4i and 4l compounds with their selected enzymes, the results obtained were analyzed based on the different parameters such as: Affinity (S-score), Interactions (types and distances).First, if an E-L formed complex gives a low energy score it means that this complex is the most stable also we have high affinity between the compound and target.Second, hydrogen bonds are the most important in the formation of E-L complexes and they can be classified according to the following intervals: If the distance belongs to the interval between 2.5 Å and 3.1 Å, we are considered to be strong interactions.If the distance belongs to the interval between 3.1 Å and 3.55 Å, we are assumed to be weak [55][56][57].Third, According to C. Janiak et al. [58] who suggested that the optimal range of hydrophobic interactions is between: 3.3-3.8Å.While other researchers have suggested a relatively higher range [59,60].

Molecular Docking Study of the Antibacterial Targets
The results obtained after the docking calculations and the best pose received for the compounds 4c, 4g, and 4h with the bacterial targets have been grouped in Table 7.

Orientation and Bonding Interaction Compound 4g in the Active Site Cavity of Thymidylate Kinase (PDB: 4QGG)
The molecular docking results shows that the compound 4g is the most potent antibacterial agent against TMK (ID: 4QGG) from S. aurues, revealing the highest negative score of −153.700kcal/mol, comparable to the standard drug Tetracycline with the score of −112.465kcal/mol (Table 7).Comparatively, compound 4g being the most active against the antibacterial agent against TMK (ID: 4QGG) from S. aurues which showed that was formed almost the same number of interactions with the TMK protein of S. aureus compared to the Tetracycline with a small difference in the type of residue (Table 7).Compound 4g displayed five strong hydrogen bonds (two Conventional H-Bond types and three Carbon H-Bond types) with crucial residues: ARG36 (1.74 Å), GLU37 (2.26 Å), PRO38 (2.12 Å) and ARG48 (2.73 and 3.05 Å) of TMK protein from S. aureus (Table 7 and Figure 6).As illustrated in Figure 6, two 6-rings of the compound 4g displayed two hydrophobic interactions (Pi-Pi T-shaped) with the residues PHE66 and TYR100.In addition, two other hydrophobic interactions (Pi-Pi Stacked) were formed between compound 4g and residue PHE66.While four hydrophobic interactions (Pi-Alkyl) with active site residues: ARG36, ILE47, ARG48 and VAL51 (Table 7 and Figure 6).We note that these results confirmed by previous studies [61][62][63] which concluded that inhibition of the both amino groups: ARG48, PHE66 and GLU37 of TMK protein might be responsible for their potent antibacterial activity.
Orientation and Bonding Interaction Compound 4h in the Active Site Cavity of (3-Oxoacyl-[acyl-carrier-protein) Synthase (PDB: 4EWP) Due to the existence of only one crystal structure of the M. luteus receptor in the RCSB Protein Data Bank.Initially, we faced a great challenge to identify the active site of the receptor (PDB ID 4EWP) for molecular docking analysis.After solving that problem, we launched molecular docking simulation and as presented in Table 7, the compound 4h fits well in the binding pocket of M. luteus receptor (PDB ID 4EWP) with highest negative score of −147.875 kcal/mol, which is comparable of Tetracycline with a score of −96.245 kcal/mol.Moreover, the docking conformation of compound 4h showed that this compound established three hydrogen bonds and five hydrophobic interactions with active site residues of the target protein (Figure 7).The hydrogen bonds were observed between the compound and active site residues SER120(2.58Å), TRP197(1.70Å) and SER120(2.41Å) of the target protein, (3-oxoacyl-[acyl-carrier-protein) synthase (Figure 7).While five hydrophobic interactions with active site residues: two with TRP197, two with VAL92 and one with ALA338 were observed (Table 7 and Figure 7).On the other hand, the results of the docking thus indicated a slight difference in the binding of the compound 4h to the (3-oxoacyl-[acyl-carrier-protein) synthase enzyme vs. the Tetracycline.Furthermore, previous papers [64,65] confirmed that the residues Val92 and ALA338 are responsible for the formation of complex: 4EWP-compounds.
Molecules 2023, 28, x FOR PEER REVIEW 16 of 29 receptor (PDB ID 4EWP) for molecular docking analysis.After solving that problem, we launched molecular docking simulation and as presented in Table 7, the compound 4h fits well in the binding pocket of M. luteus receptor (PDB ID 4EWP) with highest negative score of −147.875 kcal/mol, which is comparable of Tetracycline with a score of −96.245 kcal/mol.Moreover, the docking conformation of compound 4h showed that this compound established three hydrogen bonds and five hydrophobic interactions with active site residues of the target protein (Figure 7).The hydrogen bonds were observed between the compound and active site residues SER120(2.58Å), TRP197(1.70Å) and SER120(2.41Å) of the target protein, (3-oxoacyl-[acyl-carrier-protein) synthase (Figure 7).While five hydrophobic interactions with active site residues: two with TRP197, two with VAL92 and one with ALA338 were observed (Table 7 and Figure 7).On the other hand, the results of the docking thus indicated a slight difference in the binding of the compound 4h to the (3-oxoacyl-[acyl-carrier-protein) synthase enzyme vs. the Tetracycline.Furthermore, previous papers [64,65] confirmed that the residues Val92 and ALA338 are responsible for the formation of complex: 4EWP-compounds.Orientation and Bonding Interaction Compound 4c in the Active Site Cavity of DNA Gyrase (PDB: 4DUH) The obtained results revealed that the compound 4c binds into the DNA Gyrease enzyme.The MolDock Score energy and types of possible interactions in addition to, the interacting moiety of our docked compound is represented in Table 7 and Figure 8.The obtained results revealed that the compound 4c binds into the DNA Gyrease enzyme.The MolDock Score energy and types of possible interactions in addition to, the interacting moiety of our docked compound is represented in Table 7 and Figure 8.
Furthermore, the compound 4c proved a good ability to the binding into DNA Gyrase binding site and this is confirmed by forming 6 strong hydrogen bonding interactions with Gly 101(1.43Å), Arg 136(2.63Å and 2.23 Å), Gly 77(2.26Å), and Lys 103(1.86Å).As shown from the obtained data compound, 4c was able to form 6 hydrophobic interactions with different amino acids in the DNA Gyrase binding pocket which are ARG76, LYS103, ILE94, PRO79, ILE78, and GLY77.In addition, the compound 4c showed two electrostatic interactions (Pi-Anion and Pi-Cation) with GLU50 and LYS103, as displayed by orange dotted lines in Figure 9 for compound 4c (Table 7 and Figure 8).
Asp 73(2.54 Å) (Table 2 and Figure 8).Also, molecular docking studies revealed that the compound 4c has many binding modes with a high affinity to DNA gyrase binding site, showing a lowest MolDock Score −139.692kcal/mol compared to Tetracycline with the MolDock Score of −108.370kcal/mol (Table 7).However, the results of the docking thus indicated a slight difference in the binding of the compound 4c to the DNA gyrease enzyme vs. the tetracycline.There are four important amino acids that are common between them, which are mentioned in recent studies [66][67][68].Furthermore, the compound 4c proved a good ability to the binding into DNA Gyrase binding site and this is confirmed by forming 6 strong hydrogen bonding interactions with Gly 101(1.43Å), Arg 136(2.63Å and 2.23 Å), Gly 77(2.26Å), and Lys 103(1.86Å).As shown from the obtained data compound, 4c was able to form 6 hydrophobic interactions with different amino acids in the DNA Gyrase binding pocket which are ARG76, LYS103, ILE94, PRO79, ILE78, and GLY77.In addition, the compound 4c showed two electrostatic interactions (Pi-Anion and Pi-Cation) with GLU50 and LYS103, as displayed by orange dotted lines in Figure 9 for compound 4c (Table 7 and Figure 8).Asp 73(2.54 Å) (Table 2 and Figure 8).Also, molecular docking studies revealed that the compound 4c has many binding modes with a high affinity to DNA gyrase binding site, showing a lowest MolDock Score −139.692kcal/mol compared to Tetracycline with  Furthermore, the compound 4c proved a good ability to the binding into DNA Gyrase binding site and this is confirmed by forming 6 strong hydrogen bonding interactions with Gly 101(1.43Å), Arg 136(2.63Å and 2.23 Å), Gly 77(2.26Å), and Lys 103(1.86Å).As shown from the obtained data compound, 4c was able to form 6 hydrophobic interactions with different amino acids in the DNA Gyrase binding pocket which are ARG76, LYS103, ILE94, PRO79, ILE78, and GLY77.In addition, the compound 4c showed two electrostatic interactions (Pi-Anion and Pi-Cation) with GLU50 and LYS103, as displayed by orange dotted lines in Figure 9 for compound 4c (Table 7 and Figure 8).Asp 73(2.54 Å) (Table 2 and Figure 8).Also, molecular docking studies revealed that the compound 4c has many binding modes with a high affinity to DNA gyrase binding site, showing a lowest MolDock Score −139.692kcal/mol compared to Tetracycline with

Molecular Docking Study of the Antifungal Target
The results obtained after the docking simulations and the best pose received for the compound 4e with the fungal target are given in Table 8.
The docking results reveal that compound 4e being the most potent antifungal agent displaying a good docking MolDock Score of −129.886kcal/mol and many molecular interactions with secreted aspartic protease (SAPs) enzyme from C. Albicans vs. of the standard drug Amphotericin B with the score of −112.504kcal/mol.Also, we note that this compound fits well in the binding pocket of the secreted aspartic protease (SAPs) (fungal), which showed good interactions.In fact, compound 4e established four strong hydrogen bonds, two hydrophobic interactions and one electrostatic interaction with active site residues of the target protein (Table 8 and Figure 9).The hydrogen bonds were observed between the compound 4e and active site residues ASP86(2.36Å), THR222(2.02Å) and THR221(2.11Å, 2.61 Å) of the target protein, the secreted aspartic protease (SAPs) (Figure 9).While two hydrophobic interactions with active site residues TYR225, and one electrostatic interaction (Pi-Anion) with ASP218 was observed (Figure 9).Nevertheless, the results of the docking thus indicate a slight difference in the type of residues involve the formation of the binding of the compound 4e with the secreted aspartic protease (SAPs) vs. the Amphotericin B, which are confirmed in previous research [69,70].

Molecular Docking Study of the Anti-Inflammatory Targets
Molecular docking of the compounds 4i, 4l and Diclofinac sodium was carried out (Table 9).Regarding the docking score values, we found that the compounds: 4i and 4l fit well in the binding active site of the LOX-5 target.As can be observed, the complexes formed by these compounds have a low score energy values of −60.838 and −116.487kcal/mol, respectively (Table 9).Additionally, docking results revealed that the 3V99-A12 complex shows a good docking MolDock score of −116.487kcal/mol compared to the standard drug Diclofinac sodium with a score of −102.441kcal/mol.On the other hand, the two compounds 4i and 4l establish interactions of almost the same type as that formed by the standard drug Diclofinac sodium (Table 9).The docked conformation of the compounds 4i and 4l are illustrated in Figure 10.Regarding the obtained results, it is apparent that compound 4i formed three strong hydrogen bonds with active site residue of 5-LOX target, two conventional H-bonds types, F/TYR558(A)-NH/bond distance = 2.79 Å and H/ASN554(A)-OD1/bond distance = 2.47 Å, another one carbon H-bonds H/ASN554(A)-OD1/bond distance = 2.54 Å (Table 9 and Figure 10).A halogen bond occurs between the fluorine atom of compound A7 and ASN554(A).During which, this compound formed binding with the Fe 2+ ion of the enzyme's active site.In addition, the same compound established five hydrophobic interactions (π-alkyl interactions) with the following residues: ILE406 (A), ALA410 (A), LEU607 (A), VAL175 (A) and ALA672(A) (Table 9 and Figure 10a).In this regards, several studies [71][72][73] have revealed that that ASN554(A) and TYR558(A) play a central role in the inhibition of LOX-5 target.Moreover, we note clearly that the compound 4l establishes more binding interactions with active site residues of 5-LOX target compared to compound 4i.Five strong hydrogen bonds were formed between compound 4l and the pocket site of 5-LOX target, three conventional H-bonds, O/GLN557(A)-HE22/bond length = 1.67 Å, H/VAL175(A)-O/bond length = 1.91 Å and H/ASN554(A)-OD1/bond length = 2.23 Å.Additionally, another two carbon H-bonds, O/HIS367(A)-HE1/bond distance = 2.33 Å, and H/ASN554(A)-OD1/bond length = 2.57 Å.This compound indicates direct binding with the Fe 2+ ion of the enzyme's active site, and a metal-ligand interaction was observed in this case.
Finally, compound 4l exhibits four hydrophobic interactions (π-alkyl interactions) with the following residues: ILE406(A), ALA410(A), LEU607(A), LEU607(A) and ALA672(A) (Table 9 and Figure 10b).These results are supported by a number of studies [74,75], which have indicated that the residues: ALA410(A), ILE406(A) and LEU607(A) represent the major key for the formation of the hydrophobic interactions with the candidates.ADME-T and drug-likeness parameters were calculated using both online servers Swis-sADME server (http://www.swissadme.ch/,accessed on 20 May 2023) and the pkCSM server (http://biosig.unimelb.edu.au/pkcsm/prediction,accessed on 20 May 2023), and all results are given in Table 10.It can be seen from Table 10 that the number of hydrogen bond donors of the all compounds (4c, 4g, 4h, 4e, 4i and 4l) is: <5 (n-HD: (0~7)) and the number of hydrogen bond acceptors is <10 (n-HA: (0~10).Furthermore, all these compounds have molecular weights ranging from 100 to 500 g/mol except compounds 4g and 4h, and MLogP and WLogP values are <5.In addition, we found nROTB values <11, indicating that these compounds are flexible.Also, all TPSA values obtained were below 140 Å.Finally, these results show that all compounds satisfy all criteria of drug-likeness without presenting any violation of the Lipinski, Veber and Egan rules.Evidently, no problems are caused in oral bioavailability and pharmacokinetic parameters of either compound.
In addition, the analysis in Table 10 shows that all compounds (4c, 4g, 4h, 4e, 4i and 4l) have good Caco-2 permeability (Caco-2 values greater than −5.15 cm/s).Furthermore, it was evidenced that all compounds had HIA values greater than 30%, indicating that these compounds were administered orally, and that they are strongly absorbed by the gastrointestinal system into the bloodstream of the human body.
According to data from this table, we can see that logPS values for both compounds 4g and 4h are >−2 which means that these compounds are able to penetrate the CNS.On the other hand, we note that the other compounds (4c, 4e, 4i and 4l) are not able because of their weak logPS values (Table 10).Additionally, the logBB values of the compounds 4h and 4c are −1.09and −1.08, respectively, which are less than −1 (<−1), this indicates that both compounds are poorly distributed to the brain, comparable to other compounds (4g and 4e, 4i and 4l) which are poorly distributed.
Data from this table indicate that all compounds are inhibitors of CYP2C19 isoform and CYP3A4 substrate.Furthermore, neither compound is a CYP1A2 inhibitor nor is it a CYP2D6 substrate (Table 10).Further analysis of this Table showed that all compounds were unlikely OCT2 substrates, and they have a low excretion clearance (<5 mL/min/kg).Finally, we found that all compounds are not likely to be hERG (I and II) Inhibitors and they show no AMES toxicity (Table 10).

Crystal Structure Determination
Data collection was performed on a Bruker D8 Venture four-circle diffractometer from Bruker AXS GmbH (Karlsruhe, Germany).CPAD detectors used were Photon II from Bruker AXS GmbH; X-ray sources: Microfocus source IµS; and microfocus source IµS Mo and Cu, respectively, from Incoatec GmbH with mirror opticsHELIOS and a singlehole collimator from Bruker AXS GmbH.Programs used for data collection were APEX4 Suite [76] (v2021.10-0)and integrated programs SAINT (V8.40A; integration) and SADABS (2018/7; absorption correction) from Bruker AXS GmbH [76].The SHELX programs were used for further processing [77].The solution of the crystal structures was done with the help of the program SHELXT [78], the structure refinement with SHELXL [79].The processing and finalization of the crystal structure data was done with program OLEX2 v1.5 [80].All non-hydrogen atoms were refined anisotropically.For the hydrogen atoms, the standard values of the SHELXL program were used with U iso (H) = −1.2U eq (C) for CH 2 and CH and with U iso (H) = −1.5 U eq (C) for CH 3 .All H atoms were refined freely using independent values for each U iso (H).

Anti-Inflammatory and Analgesic Bioassays
Lipoxygenase (sigma-437996-500U) activity was determined by the protocol of by Choudhary et al. [81].Analgesic activity in rats was determined by the protocol described by Tiss et al. [82].In vivo anti-inflammatory activity was determined by the carrageenaninduced paw edema method as described by Cordaro et al. [83].The indices of hepatic toxicity (the activities of AST and ALT) and the level of albumin, urea and creatinine were calculated according to the protocol described by the supplier (Kits Biolabo, Maizy, France).

Ligands and Targets Preparations
The 3D structures of four most active compounds: 4c, 4g, 4h, 4e, 4i and 4l were preoptimized by means of the Molecular Mechanics using Force Field MM+.After that, all compounds optimized using the semi-empirical method AM1 [84] which implemented in the Hyperchem 8.0.8 software [85].
The X-ray crystallography structures of four different drug target proteins were downloaded from the RCSB Protein Databank (https://www.rcsb.org/,accessed on 20 May 2023), accessed on 10 May 2023 that is, Thymidylate Kinase (TMK) (PDB ID 4QGG) from S. aureus [86], (3-oxoacyl-[acyl-carrier-protein) synthase 3 (PDB ID 4EWP) from M. luteus [65], DNA gyrase (PDB ID 4DUH) from E. coli [87] were selected as antibacterial targets, and secreted aspartic protease (PDB ID 3Q70) from C. albicans and C. krusei [88] was selected as the antifungal targets.The crystal structure of the human 5-LOX enzyme in complex with its substrate, Arachidonic acid PDB (PDB ID: 3V99) [89], was also downloaded from the same Protein Data Bank.Some information related to the selected targets was reported in Table S1 in the Supplementary Materials).According to Table S1, we note X-ray crystals of the targets selected have resolution between 1.5 and 2.5 Å [90], confirming that these structures can be considered of good quality.

Molecular Docking Simulations
Docking simulations were carried out on the five targets selected by using Molegro Virtual Docker v. 6.0.1(MVD)[91] software package knowing that the algorithm keeping the macromolecule rigid while allowing ligand flexibility.All X-ray crystals of the targets selected were simplified by removing water molecules, ions, cofactors and co-crystal ligands from their PDB structure and molecular docking protocol were followed and used in our previous studies [92,93].In the first, The MolDock score [GRID] algorithm was used as the score function, and the MolDock was used as search algorithm.In the second, default parameter settings in the same software package (Score function: MolDock Score; Ligand evaluation: Internal ES, Internal HBond, Sp2-Sp2 Torsions, all checked; Number of runs: 10 runs; Algorithm: MolDock SE; Maximum Interactions: 1500; Max.population size: 50; Max.steps: 300; Neighbor distance factor: 1.00; Max.number of poses returned: 5).The docking procedure was performed using a GRID of 15_A in radius and 0.30 in resolution to cover the ligand-biding site of all targets selected [94].

Method Validation
Re-docking of the co-crystal ligands was performed to validate the applied molecular docking approach.We found that the root mean square deviation (RMSD) values variation are between 1 and 2 Å [95] for all complexes Enzyme-co-crystal which means that the docking method is accuracy and successful.

Conclusions
In summary, a novel series of spirooxindole-hydantoins was successfully synthesized as potent anti-inflammatory, analgesic, and antimicrobial agents.Antimicrobial screening revealed that (i) compounds 4c, 4h, 4g, and 4m (MIC value of 93.75 µg/mL) were more potent than the reference antibiotic tetracycline (MIC value of 500 µg/mL), against M. luteus (ii) compounds 4c and 4m showed highest antibacterial activity with a MIC value of 187.50 µg/mL against E. coli, and (iii) heterocycle 4e showed the greatest antifungal potential toward C. albicans and C. krusei (MIC values of 23.43 µg/mL and 46.87 µg/mL, respectively) as compared to amphotericin B (MIC= 31.25 and 62.50 µg/mL, respectively).On the other hand, all tested spirooxindoles exhibited modest to potent inhibitory activity (IC 50 = 1.01-4.96mg/mL) against LOX-5 enzyme.Among them, spirooxindoles 4i and 4l (IC 50 = 1.09 mg/mL and IC 50 = 1.01 mg/mL, respectively) showed improved LOX-5 inhibition profile better that of diclofenac sodium (IC 50 = 1.19 mg/mL).Moreover, 4i and 4i showed a good anti-inflammatory activity (inhibition: 33 and 32%; respectively) which was comparable to the reference standard diclofenac sodium (inhibition: 46%) in carrageenaninduced rat paw edema assay.In addition, they displayed acceptable in vivo analgesic activity in acetic acid-induced writhing response (inhibition: 42 and 53%; respectively) compared to reference drug (63%).Finally, molecular docking simulation and ADME-T prediction revealed that compounds 4g, 4h, 4c, and 4e have high affinities with the pocket of bacterial and fungal targets, also compounds 4i and 4l have high affinities with the binding site of LOX-5 target, which was confirmed by a lowvalue MolDock score and the appearance of several types of interactions which formed between these compounds and residues of the active site of the target selected.Moreover, ADMET predictions and physicochemical properties proved that all rules: Lipinski, Veber and Egan rules were compiled by all compounds tested.Thus, some of newly synthetized spirooxindoles could act as a platform for further evaluation.

Figure 4 .
Figure 4. Association of the two independent molecules in the packing through intermolecular N-H•••O hydrogen bonding forming a supramolecular 1D array 2.3.Biological Activity 2.3.1.In Vitro Lipoxygenase Inhibitory Assay and Structure-Activity Relationship (SAR) Study

Figure 4 .
Figure 4. Association of the two independent molecules in the packing through intermolecular N-H•••O hydrogen bonding forming a supramolecular 1D array.

Figure 6 .
Figure 6.2D and 3D representation of interactions of the compound 4g occurring within the active site cavity of Thymidylate Kinase (PDB: 4QGG).

Figure 6 .
Figure 6.2D and 3D representation of interactions of the compound 4g occurring within the active site cavity of Thymidylate Kinase (PDB: 4QGG).2.3.6.Evaluating the Bactericidal and Bacteriostatic Effects: MBC/MIC Ratio of the Spiropyrrolidines against Microbial Strains

Figure 7 .
Figure 7. 2D and 3D representation of interactions of the compound 4h occurring within the active site cavity of (3-oxoacyl-[acyl-carrier-protein) synthase (PDB: 4EWP).Orientation and Bonding Interaction Compound 4c in the Active Site Cavity of DNA Gyrase (PDB: 4DUH)

Figure 8 .
Figure 8. 2D and 3D representation of interactions of the compound 4c occurring within the active site cavity of DNA gyrase (PDB: 4DUH).

Figure 9 .
Figure 9. 2D and 3D representation of interactions of the compound 4e occurring within the active site cavity of SAPs (PDB: 3Q70).

Figure 8 .
Figure 8. 2D and 3D representation of interactions of the compound 4c occurring within the active site cavity of DNA gyrase (PDB: 4DUH).

Figure 8 .
Figure 8. 2D and 3D representation of interactions of the compound 4c occurring within the active site cavity of DNA gyrase (PDB: 4DUH).

Figure 9 .
Figure 9. 2D and 3D representation of interactions of the compound 4e occurring within the active site cavity of SAPs (PDB: 3Q70).

Figure 9 .
Figure 9. 2D and 3D representation of interactions of the compound 4e occurring within the active site cavity of SAPs (PDB: 3Q70).

Table 1 .
Optimization of the three component 1,3-dipolar cycloaddition reaction a .

Table 2 .
LOX-5 inhibition results of the synthesized compounds and theirs LogP values.

Table 2 .
LOX -5 inhibition results of the synthesized compounds and theirs LogP values.Comp.

Table 3 .
Effect of the compounds 4i and 4l on λ-carrageenan-induced paw edema in rats.

Table 4 .
Analgesic activity of 4l and 4i on acetic acid-induced writhing test.
a Values are given as mean ± SE.

Table 5 .
Evaluation of the toxicity of compounds 4i and 4l to a dose of 16.25 mg/kg in rats.

Table 8 .
MolDock Score and interactions between the compounds 4e with fungal target.

Table 9 .
Molecular docking results for the compounds 4i, 4l and diclofenac sodium involved in 5-LOX target.

Table 10 .
ADME and drug-likeness properties of the compounds 4c