2.1. Preparation of AgNPs Functionalized Natural Products Doped PANI (SNPs)

The chemicals used in the present study have been purchased from standard commercial sources. Aniline, silver nitrate, paraphenylenediamine, oxalic acid, adipic acid, and myoinositol were sourced from S.D. Fine Chemicals, ellagic acid and phloroglucinol from Sigma-Aldrich, and gallic acid from Spectrochem. SNPs were synthesized by dissolving 1 g of aniline as monomer and 0.1 equivalent of paraphenylenediamine as an initiator in 100 mL of distilled water containing 0.3 equivalent of natural products. To the above reaction mixture, three equivalents of AgNO₃ dissolved in 50 mL of distilled water were added drop by drop with constant stirring. After complete addition, the reaction mixture was stirred for additional 24 h at room temperature. The product obtained was filtered, washed with water followed by methanol, and vacuum dried at 60°C for 12 h.

2.2. Characterization of SNPs

The analysis of SNPs was performed by Fourier transform infrared (FTIR), X-ray diffraction (XRD), scanning electron microscopy (SEM), and energy-dispersive X-ray spectroscopy (EDX).

2.3. Evaluation of the Antibacterial Activity of SNPs

2.4. Evaluation of the Antifungal Activity of SNPs

3.1. Characterization of SNPs

3.1.1. FTIR spectra

The FTIR spectra of AgNPs functionalized polyaniline nanocomposites (SPs) and SNPs are presented in Figure 1. The spectra of SPs indicate the presence of C-H vibration peaks at 2977 and 2896 cm⁻¹. The C-H bending in SPs can be observed at 1398 and 1060 cm⁻¹. SPs exhibited a C=N bond vibration peak at 1662 cm⁻¹, C-N bond vibration at 1230 cm⁻¹, and C=C bond vibration peaks at 1540 cm⁻¹ [33]. Similar peaks are observed in all SNPs. In addition, ellagic acid doped SNP exhibited phenolic OH group at 3660 cm⁻¹ and C=O stretching at 1719 cm⁻¹ [34]. Adipic acid, gallic acid, and oxalic acid doped SNPs exhibited a broad peak at around 3400 cm⁻¹ corresponding to carboxylic acid. Phloroglucinol and myoinositol doped SNPs showed the presence of −OH groups at 3447 cm⁻¹ and 3362 cm⁻¹, respectively.

Figure 1: FTIR spectra of SNPs (a) control – SPs, (b) adipic acid [ADP], (c) oxalic acid [OA], (d) myoinositol [MI], (e) phloroglucinol [PG], (f) gallic acid [GA], and (g) ellagic acid [EA]. [Click here to view]

3.1.2. XRD analysis

The diffraction pattern was observed in the XRD spectrum of the SNPs, indicating their crystalline nature. The fingerprint diffraction patterns of SNPs are illustrated in Figure 2, which shows three major peaks at 2q = 37.51°, 43.12°, and 63.47° corresponding to the planes (111), (200), and (220), thereby indicating the face-centered cubic patterns of SNPs [35]. Using Scherrer’s formula, the average crystallite size of the SNPs obtained from FWHM of the more intense peak corresponding to the (111) plane located at 37.51º was determined to be ~40 nm.

Figure 2: XRD images of synthesized SNPs. [Click here to view]

3.1.3. SEM and EDX analysis

The SEM images of SNPs are illustrated in Figure 3 and their respective EDX in Figure 4. The SEM images were captured with X 20,000. The surface morphology of SNPs certainly reveals the uniform and good dispersion of nanoparticles. The agglomeration of nanoparticles might have occurred because of the electrostatic interaction of SNPs. The images captured here resemble that of [36], where the morphology was spherical in appearance with aggregation as found in our analysis.

Figure 3: SEM images of SNPs synthesized using (a) control – SPs, (b) adipic acid, (c) ellagic acid, (d) gallic acid, (e) oxalic acid, (f) myoinositol, and (g) phloroglucinol. [Click here to view]

Figure 4: EDX images of synthesized SNPs. [Click here to view]

The qualitative and quantitative profile of elements present in the synthesized SNPs was confirmed by analysis of EDX. The spectral analysis has indicated intense signals relating to the Ag element, which further affirms the incorporation of the natural products into the AgNPs during the synthesis of the SNPs. The EDX profile of Ag at 3 keV is indicated by a strong peak, confirming it as the major elemental component of the SNPs. In addition to Ag, elements such as C and O were observed in SNPs, which can be attributed to carbon and oxygen present in the PANI and dopants.

To study the effect of SNPs on bacterial cells, overnight grown bacterial cells were treated with different concentrations of the SNPs and a change in surface morphology was observed using SEM analysis. Figure 5 illustrates the images of E. coli cells treated with SNPs doped with adipic acid and gallic acid. Loss of integrity of the cells is indicated by the uneven shapes of cells, indicating the development of cracks or ruptures on the cell wall in SNPs treated cells when compared to control. The disruption of cells was observed among SNPs treated cells of E. faecalis and S. mutans. The same is depicted in Figure 5.

Figure 5: SEM images of I) E. coli treated with SNPs (a) control – SPs, (b) adipic acid and (c) gallic acid; II) E. faecalis treated with SNPs (a) gallic acid and (b) myoinositol; III) S. mutans treated with SNP a) oxalic acid; and IV) E. faecalis treated with SNPs (a) gallic acid and (b) myoinositol. [Click here to view]

3.2. Evaluation of the Antimicrobial Activity of SNPs

Bacterial infections are a significant cause of morbidity and mortality in humans [37]. In traditional medicine, crude drugs formulated from extracts of plants in combination with other natural products are used for treating bacterial infections, which impart dual benefits, inhibiting bacterial proliferation along with enhancing general immunity of the body [38]. Therefore, traditional medicines provide long-term protection against a broad spectrum of infections [39]. Contrary to this approach, modern medicine relies on isolated active compounds, synthesized or produced on a large scale, to address the issue of meeting the higher demand. This trend has led to the phenomenon of antibiotic resistance among pathogenic [40]. Recently, nanoparticles conjugated with active drug molecules have emerged as novel tools for developing antibacterial formulations [41]. A combination of natural products with green synthesized nanoparticles would be an ideal choice for drug development. This idea has prompted us to synthesize SNPs, which have both AgNPs and the natural antimicrobial qualities of organic dopants.

The microbial growth inhibition induced by SNPs has been demonstrated in selected bacterial and fungal strains. Easy methods of synthesis and enhanced efficacy demonstrated by the nanoparticles in damaging microorganisms have made them acceptable for antimicrobial applications. The reason for such an enhanced effect is the release of cations from nanoparticles while entering the cell, which causes a transformation in their normal functioning and hence kills the bacterium. Gram-negative bacteria, which possess a thin peptidoglycan layer in their cell walls when compared to Gram-positive bacteria, allow better penetration of nanoparticles and hence exhibit a larger zone of inhibition [42] in well/disk diffusion assays and the same observation was found in our present study as well.

3.3. Evaluation of the Antimicrobial Efficacy of SNPs on Dental/Oral Pathogens

3.3.1. Bacteriostatic activity of SNPs on S. mutans

Subsequently, we have evaluated the antibacterial effect on Gram-positive dental pathogens like S. mutans. The bacteriostatic effect along with standard deviation on S. mutans due to the treatment with SNPs, SPs, and control is presented in Table 1, and it can be observed that all the SNPs have demonstrated good antibacterial activity. The MIC and MBC values of SNPs in S. mutans are illustrated in Table 2. All the samples tested on S. mutans have emerged as equally potent bacteriostatic candidates. Multivariate ANOVA of the data of myoinositol-doped SNP yielded a high F-static of 114.778 and a P-value of 1.653. This shows that the hypothesis was true and the null hypothesis was rejected. Gallic acid-doped SNP showed no effect on hypothesis testing, and phloroglucinol-doped SNP showed significant true hypothesis testing. The zone of inhibition and MBC test results for myoinositol doped SNP on S. mutans are presented in Figure 6.

Figure 6: Zone of inhibition and MBC of myoinositol SNP by Streptococcus mutans. [Click here to view]

3.3.2. Bacteriostatic activity of SNPs on E. faecalis

E. faecalis is another dental pathogen on which the efficacy of SNPs has been tested. The bacteriostatic efficacy of the SNPs on this pathogen is presented in Table 1. We performed the multivariate ANOVA for the results of MIC and MBC tests on this pathogen for different SNPs using Roy’s method and the results are presented in Table 2. Myoinositol-doped SNP has yielded 13.182 under F-static and 0.006372 as P value defined for intercept, while MIC showed 11.636 for F-static and 0.008612 for P-value. This indicates that the null hypothesis was tested and found to be true. The parallel evaluation was also obtained for adipic acid and gallic acid doped SNPs. The images of MIC and MBC treatment of gallic acid-doped SNP are presented in Figure 7.

Figure 7: Zone of inhibition and MBC of gallic acid by Enterococcus faecalis. [Click here to view]

The above results indicate that SNPs showed better antimicrobial activity than SPs and can also perform on par with the commercially available antibiotics. Nanoparticles are known to possess the tendency to react with sulfur and phosphorus predominantly present in the outer membrane of bacteria, leading to the formation of pores in the bacterial cell wall. The interaction of nanoparticles to the bacterial membrane leads to the outflow of intracellular substances which causes shrinkage and finally lysis of the cell [43]. Different mechanisms are being proposed for the mode of action of nanoparticles on bacterial cells, such as cell wall and membrane damage, intracellular penetration and damage, and oxidative stress [44]. Our attempt to control the antibiotic-resistant bacterial phenotype was found to be successful as discussed in Section 3.1.3. SNPs have been shown to break the bacterial cell wall [Figure 5], indicating that they could be used as pro-drug antibiotic candidates.

3.4. Antifungal Activity of SNPs

Fungi are found all over the world, and their pathogenic varieties are highly resistant which makes them tough to combat. Therefore, it is important to study the fungistatic activity of the SNPs, as well. A. niger is known to cause critical diseases such as aspergillosis and otomycosis, F. oxysporum can cause mycotoxicosis and skin-related infections, while E. floccosum is recognized for triggering septicity such as tinea pedis, tinea cruris, tinea corporis, and onychomycosis, and T. rubrum is noted for athlete’s foot, infections such as jock itch and ringworm. We have evaluated the effect of our SNPs against predominant pathogenic fungi A. niger, F. oxysporum, E. floccosum, and T. rubrum. The fungal virulence factor, encrypting gene rearrangements, and other similar observed behaviors are attributed to the adaptation to any stress environment [45]. It was observed from Table 3 that oxalic acid- and phloroglucinol-doped SNP exhibited better antifungal effects compared to the other SNPs. The gallic ­acid-, adipic acid-, and myoinositol-doped SNPs have hardly exhibited any mycostatic activity. These data are supported by Figures S4-S7 signifying the zone of inhibition exhibited by SNPs and control against individual fungal strains. Oxalic acid-doped SNP was effective against A. niger and F. oxysporum with 7.33 mm of inhibition at 5 mg/mL and 20 mm at 10 mg/mL, respectively. Ellagic acid-doped SNP inhibited the growth of E. floccosum by 12 mm at a 10 mg/mL concentration. When the fungal strains were dosed with 5 mg/mL of phloroglucinol-doped SNP, the growth inhibition of 11 mm and 9.67 mm was observed in E. floccosum and T. rubrum organisms, justifying their fungistatic activity.

Table 3: The fungistatic activity of SNPs in terms of zone of inhibition.

Organic acids can be efficiently used as antifungal agents due to their properties relating to bioactivity, polarity, and high solubility in many solvents including water [46]. There is evidence for the fact that commercial antifungals have limited utilization and also related medicinal values because of side effects and slow recovery [47], and hence, there is an urgent need to design and develop nanoparticles with better antifungal activities. Therefore, we opted to incorporate selected natural products with AgNPs and PANI to enhance their antifungal activity, which has been proved in our study through the significant difference in the antifungal activities of SNPs with those of the control samples [Table 3]. Similar observation on enhanced antifungal activity of nanomaterial reported earlier by Xia et al. [48]. Our study has demonstrated interesting results by inhibiting human and animal pathogenic fungi, indicating their potential as alternatives to commercial antifungal products.

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