Investigating binding dynamics of trans resveratrol to HSA for an efficient displacement of aflatoxin B1 using spectroscopy and molecular simulation

Resveratrol is a polyphenol belonging to the class stilbenes. The active and stable form of resveratrol is trans-resveratrol. This polyphenol is bestowed with numerous biological properties. Aflatoxin B1 is a hepato-carcinogen and mutagen that is produced by Aspergillus species. In this study, the interaction of trans-resveratrol with HSA followed by competitive dislodging of AFB1 from HSA by trans-resveratrol has been investigated using spectroscopic studies. The UV-absorption studies revealed ground state complex formation between HSA and trans-resveratrol. Trans-resveratrol binds strongly to HSA with the binding constant of ~ 107 M−1 to a single binding site (n = 1.58), at 298.15 K. The Stern–Volmer quenching constant was calculated as 7.83 × 104 M−1 at 298.15 K, suggesting strong fluorescence quenching ability of trans-resveratrol. Site markers displacement assay projected subdomain IIA as the binding site of trans-resveratrol to HSA. The molecular docking approach envisages the amino acid residues involved in the formation of the binding pocket. As confirmed from the site marker displacement assays, both trans-resveratrol and AFB1 binds to HSA in the same binding site, subdomain IIA. The study explores the ability of trans-resveratrol to displace AFB1 from the HSA-AFB1 complex, thereby affecting the toxicokinetic behavior of AFB1 associated with AFB1 exposure.

HSA is a major transport protein in humans, having a molecular weight of 66.5 kDa comprising 585 amino acid residues, with single tryptophan viz Trp-214 15 . The presence of aromatic amino acid residues like Trp, Tyr, and Phe imparts HSA its fluorescent property. Nevertheless, the significant contribution is due to tryptophan residues. It is a model protein that has been explored to investigate ligand-protein interactions.
Pharmacokinetics and pharmacodynamics studies of molecules using biophysical tools are prerequisites in determining its efficacy, toxicity, and elimination process from the body. There are a number of studies exploring the hepatocellular toxicity of AFB 1 using in vitro and in vivo approaches. Though, studies aiming at the fate of this hepato-carcinogen in the presence of serum albumin and vice versa are fewer. Recently few studies focused on the binding behavior of AFB 1 with BSA, HSA, and chicken egg albumin [16][17][18] , provided information about its binding constant, site of binding, and thermodynamic parameters. Still, these studies have gaps that need to be filled by an approach that could unload the mycotoxin from the precise binding location in serum albumin, leading to its biotransformation followed by its elimination from the body. This study focuses on the very same approach using a polyphenol trans-resveratrol that could effectively dislodge the AFB 1 from serum albumin using fluorescence spectroscopic tools. In the present study, UV-absorption spectroscopy is used to investigate the structural alterations and ground-state complex formation between HSA and trans-resveratrol, the fluorescence spectroscopy was used to calculate the binding constant of the polyphenol and HSA, thermodynamic parameters (ΔG, ΔH, and ΔS), followed by site marker displacement assay to examine the binding site of trans-resveratrol on HSA. The Circular dichroism study was performed to investigate secondary structure changes induced by trans-resveratrol in HSA, followed by the calculation of melting temperature (Tm). Temperature-dependent heat denaturation and unfolding profile of HSA in the presence of trans-resveratrol were also determined. Molecular docking analysis visualized the amino acid residues involved in the binding of trans-resveratrol with HSA along with major binding forces stabilizing the interacting entities. In silico amino acid substitution study was performed to ascertain the role of Trp-214 in the binding process of the ligand to the protein molecule. After confirming the binding location of the polyphenol, a comparative analysis of the fluorescence quenching strength of trans-resveratrol versus AFB 1 was established for HSA. Later on, the displacement assays were performed to analyze the dislodging potential of trans-resveratrol to displace AFB 1 from the HSA and vice versa. The outcome of this study will help the researchers to understand the kinetics and dynamics of the binding process of trans-resveratrol and AFB 1 .

Results and discussion
Spectroscopic studies. The binding and interactive mode of flavonoid trans-resveratrol with HSA was investigated before its use as a dislodging agent for HSA bound AFB 1 . The binding behavior was studied using spectroscopic tools like fluorescence spectroscopy and UV-visible spectroscopy. UV-absorption spectroscopy was used to ascertain the structural changes induced by trans-resveratrol upon binding with HSA. The UVabsorption property of HSA is by virtue of its aromatic amino acids (Trp, Tyr, and Phe) that impart a strong UV absorption signal at 280 nm 19 . Nevertheless, trans-resveratrol shows the absorption signal at 319 nm, as shown in Fig. 2a. From the Fig. 2a, it is clear that in the presence of an increasing concentration of trans-resveratrol, the hyperchromic effect was observed at absorption maxima (λ max ) of HSA, coupled with bathochromic shift, suggesting structural alterations in the native structure of HSA and a ground state complex formation between trans-resveratrol and HSA 20 . The absorption spectrum also gives a clue about the existence of static quenching between trans-resveratrol and HSA, since in static type of quenching, the absorption spectra of native protein changes in the presence of a ligand molecule, however in dynamic quenching, it remains unaffected 21,22 . Fluorescence spectroscopy was performed to get insight into the binding and thermodynamics parameters associated with the interaction of trans-resveratrol with HSA. When excited at 280 nm, a strong fluorescence quenching was observed in the fluorescence emission spectrum of HSA in the presence of an increasing concentration of trans-resveratrol (0-14 µM) as shown in Fig. 2b. HSA consists of fluorophores, critical for the fluorescent property of the protein viz, Trp, Tyr, and Phe, where the major contribution is from Trp-214 residue 23 . Quenching is accompanied by redshift suggesting structural and conformational alterations in the native structure of HSA in the presence of trans-resveratrol. Bathochromic shift is the result of the increase in the polarity around fluorophores in HSA in the presence of trans-resveratrol 24 .
Stern-Volmer quenching constant (K SV ) for binding trans-resveratrol with HSA was calculated according to Eq. (1) 25 . There is linearity between the concentration of T-res (Q) and F 0 /F, as shown in Fig. 3a, at 298.15, 303.15, and 308.15 K. With the rise in temperature, a decrease in the slope of the Stern-Volmer plot is observed, the binding between HSA and trans-resveratrol also destabilizes with the increase in the temperature, suggesting a static mode of fluorescence quenching and quashing the existence of dynamic quenching mechanism operating between HSA and trans-resveratrol 26 . Nevertheless, from Fig. 3a, if we look at the F 0 /F vs Q plot at 298.15 K, at a higher concentration of trans-resveratrol, the F 0 /F vs Q plot is shifted towards y axis, envisaging a mixed    Table 1, is greater than the maximum scattering collision constant whose value is 2 × 10 10 M −1 s −1 , thus confirming the existence of static quenching and groundstate complex formation between HSA and trans-resveratrol 24,27 . In a protein and ligand interaction, three different natures of fluorescence quenching can be observed, static, dynamic, and mixed (both static and dynamic) quenching. These different kinds of quenching patterns can be differentiated based on the K SV values obtained at different temperatures. Static quenching is marked by ground-state complex formation between ligand molecule and protein 28 , followed by decreases in the K SV values with an increase in the temperature. The decrease in the K SV is the result of a decrease in the ligand and protein stability with the rise in the temperature. However, in the dynamic nature of fluorescence quenching, the K SV value increases with the rise in the temperature 29,30 . Dynamic quenching results from the collision of the fluorophore and the ligand molecule. The mixed nature of fluorescence quenching displays both the properties of static and dynamic quenching 31 . The binding constant (K b ) was calculated at three different temperatures, viz 298.15, 303.15, and 308.15 K using Eq. (4) 25,32 , mentioned in the "Methods" section. The plot of log (F 0 − F)/F versus log (Q) is shown in Fig. 3b. The plot is a straight line, and the value of K b was calculated to be 6.36 ± 0.32 × 10 7 M −1 at 298.15 K. Such a high binding constant is an indication of strong binding affinity between HSA and trans-resveratrol. The values of K b and number of binding sites (n) at three different temperatures are reported in Table 2.
The binding affinity of AFB 1 towards HSA has already been reported earlier by Tan et al. 33 . AFB 1 binds to HSA in subdomain IIA with a binding constant ~ 10 4 M −1 . The binding constant (K b ) for AFB 1 -HSA system is lower than the HSA-T-res system.
The Gibbs free energy (ΔG), enthalpy change (ΔH), and entropy change (ΔS) are the essential thermodynamic parameters that portray the spontaneity and favorability of a chemical reaction. These thermodynamic values are calculated using Eqs. (6) and (7) of the "Methods" section. Figure 3c shows the lnK versus 1/T (K) plot, the intercept and slope of the plot were used in the calculation of ΔS and ΔH, which was calculated to be −257.67 cal mol −1 K -1 and −87.60 kcal mol −1 , respectively. The magnitude of both ΔS and ΔH is negative, signifying hydrogen bonding and van der Waals interaction as the major forces acting in HSA and trans-resveratrol complex stabilization. The principal forces acting between the protein and ligand molecule are hydrogen bonding and van der Waals interaction when ΔS < 0 > ΔH 34 . We also calculated the value of ΔG for the HSA-T-res system that was found to be negative, suggesting a favorable and spontaneous process of trans-resveratrol binding with HSA. All the thermodynamic parameters are reported in Table 2.
Location of the binding site of trans-resveratrol in HSA using site markers displacement assay. Our molecule of interest, trans-resveratrol, binds to HSA with a much higher affinity as compared to AFB 1 , hence possessing the potential to compete with AFB 1 . We further explored the binding site of transresveratrol on HSA using site markers, warfarin, and ibuprofen. These two site markers are routinely used probe molecules to locate the binding site of a small molecule on protein 35 . Most of the ligand binds to the protein at Sudlow's site I (subdomain IIA) and Sudlow's site 2 (subdomain IIIA). Warfarin binds to subdomain IIA, and ibuprofen binds to subdomain IIIA. The binding location of AFB 1 on HSA has already been studied by Tan et al. and Poor et al. 17,33 , confirming Sudlow's site 1 as the binding pocket of AFB 1 on HSA. If trans-resveratrol and AFB 1 share the same binding site on the protein molecule, trans-resveratrol, by virtue of its higher binding constant (K b ) for HSA than AFB 1, could easily displace the mycotoxin from the HSA and increase its availability in the body in free form rather than bound form. The percentage displacement was calculated from the plot of F 2 / F 1 × 100 versus probe/HSA, obtained using Eq. (7) of the "Methods" section 36,37 . From Fig. 4, it is inferred that Circular dichroism measurement. Circular dichroism is a valuable tool for deciphering the conformational or secondary structure change in the protein induced by a ligand 40 . It is a routinely used technique involved in ligand and protein interaction to investigate the nature of the binding between protein and molecules 41 . Interaction of chromophores in the protein molecule, in an asymmetric milieu, with the polarized light results in CD signals 42 . Peptide bonds absorb polarized light in the far UV-region 43 . The far UV-CD signal of HSA with predominant alpha helix exhibits two negative ellipticity at 208 and 222 nm as a consequence of n → π* and π → π* transition 44 . From Fig. 5a, it is observed that the native HSA exhibited two peaks at 208 and 222 nm, suggesting the predominance of the alpha helix. The MRE value at 208 nm and percentage alpha helix was calculated using Eqs. (8) and (9) of the "Methods" section 38,45 .   Figure 5b shows the CD values at 208 and 222 nm for HSA in the absence and presence of trans-resveratrol, which depicts a clear picture of the increase in CD (mdeg) values corresponding to increase in an alpha helix at 10 and 20 µM trans-resveratrol. Some phytochemicals and drug molecules, on interaction with albumins, have shown to increase the alpha helix and thereby its stability, and it is due to an increase in the extent of hydrogen bonding in the protein molecules [46][47][48] .
Thermal stability of HSA in the presence of trans-resveratrol was also investigated using CD spectroscopy, by measuring changes in CD signal at 222 nm by sigmoidal fitting, as a function of temperature (20-90 °C). Hydrophobic interactions are the major contributors to the folding mechanism of protein. However, other factors like hydrogen bonding and electrostatic interactions also play significant roles in stabilizing protein structure 49 . T m is the midpoint transition temperature at which the equilibrium is maintained between folded and unfolded form 50 . The thermal stability of the protein is directly proportional to its T m value. In other words higher the T m value more is the thermal stability of the protein 51 . The native HSA exhibited T m values of 63.75 °C. However, in the presence of trans-resveratrol, it was increased to 66.25 °C. The increase in the T m value from 63.75 °C to 66.25 °C confirms the trans-resveratrol-assisted folding of HSA. The thermal unfolding experiment further explores that the thermal stability of HSA is increased in the presence of trans-resveratrol. Certain drugs which bind to subdomain IIA, like warfarin and virstatin have been known to increase the T m of HSA, as reported in earlier studies 52,53 . Figure 6 shows the melting profile of HSA in the presence of trans-resveratrol.
Far UV-three dimensional CD spectra of HSA in the absence and presence of trans-resveratrol as a function of temperature were also plotted to envisage the ligand-induced structural and conformational perturbation of HSA at each temperature ranging from 20 to 90 °C. From Fig. 7, it is clear that with each rise in temperature from 20 to 90 °C, the negative ellipticity at 208 and 222 nm decreases, suggesting the unfolding of HSA as a function of temperature. In the presence of 20 µM trans-resveratrol, the alpha-helical content of HSA is protected at each rise in temperature, suggesting the trans-resveratrol mediated stabilization of the secondary structure of native HSA. From Table 3, it is evident that at 20 °C, native HSA showed 61.30% alpha-helix, and at 90 °C, it was reduced to 27.69% as a result of unfolding and temperature-induced denaturation. However, trans-resveratrol bound HSA at 20 °C exhibited 67.58%, higher than the HSA alone, at each increment in the temperature; HSA bound transresveratrol showed higher alpha-helix as compared to HSA alone at the same temperature. The drastic decrease in the alpha helix in HSA as a function of temperature is attributed to the reduction in the hydrogen bonding in the amino acids. Nevertheless, trans-resveratrol proved to be effective in protecting the unfolding of HSA, thereby restoring hydrogen bonding in the amino acid residues at a given temperature range. Figure 7 reflects the far UV-CD spectra of HSA in the presence of trans-resveratrol from 20 to 90 °C.

Displacement of AFB 1 from HSA by trans-resveratrol.
After confirming that AFB 1 and trans-resveratrol shares the same binding site, subdomain IIA in HSA, displacement assay was followed to check the dislodging potential of trans-resveratrol against AFB 1 competing for the same binding pocket. In Fig. 8a, it is shown that each increasing concentration of trans-resveratrol (0-20 µM), displaces the AFB 1 bound to HSA from the HSA-AFB 1 system. However, when the displacing potential of AFB 1 against trans-resveratrol was studied for the HSA-Tres system, as shown in Fig. 8b, AFB 1 failed to dislodge trans-resveratrol from HSA, indicating the inability of AFB 1 to compete for albumin sharing the same binding site with trans-resveratrol. From Fig. 8b, it is clear that the increasing concentration of AFB 1 (0-20 µM) has no effect on the percentage displacement of trans-resveratrol bound to HSA. www.nature.com/scientificreports/ Comparative analysis of the binding potentials of trans-resveratrol and AFB 1 to HSA. We also performed the comparative analysis of the effect of AFB 1 and trans-resveratrol on HSA, as depicted in Fig. 9. From the figure, based on the values of the fluorescence intensities, the emission spectrum of HSA underwent more quenching in the presence of trans-resveratrol than AFB 1 . The decrease in the fluorescence intensity is more in HSA + T-res as compared to HSA + AFB 1 . To further gain insights into the dislodging potential of trans-resveratrol, competing for HSA, equal concentrations of AFB 1 and trans-resveratrol were used for displacing trans-resveratrol bound HSA and AFB 1 bound HSA, respectively. From Table 4, it is evident that HSA alone (5 µM) showed fluorescence intensity of 47,776.6, the fluorescence intensity in the presence of AFB 1 and trans-resveratrol was decreased to 37,322.6 and 24,784.8, respectively. The fluorescence intensity of HSA for the HSA + T-res + AFB 1 system (Table 4) insignificantly differed from the fluorescence intensity of the HSA + T-res system, thereby confirming the inability of AFB 1 to displace trans-resveratrol from HSA-T-res. Nevertheless, the fluorescence emission intensity of HSA for the HSA + AFB 1 + T-res system (Table 4) significantly changed from  www.nature.com/scientificreports/ the fluorescence emission intensity of the HSA + AFB 1 system, elucidating the potentiality of trans-resveratrol to dislodge the AFB 1 bound to albumin and apprehending its binding site.
Molecular docking and amino acid substitution studies. Molecular docking is a powerful computational approach to investigate ligand binding to the protein molecule at the atomic level 54 . These in silico tools   www.nature.com/scientificreports/ were used to explore and recognize the binding site of trans-resveratrol in HSA, corroborate the findings of spectroscopic studies, and get insight into the amino acid residues involved in the binding of trans-resveratrol with HSA. Figure 10 shows the best-docked pose and Sudlow's site 1 as the binding pocket for the binding of trans-resveratrol with HSA. The binding energy for the interaction as calculated from the docking is −7.76 kcal mol −1 . If we look at Fig. 10, Trp-214 is present in the binding pocket, and it has a role in the stabilization of HSA trans-resveratrol complex. The amino acid residues surrounding the trans-resveratrol molecule are shown in Table 5. Figure 11 depicts the 2D picture of the amino acid residues in the vicinity of the trans-resveratrol and the nature of bonds formed between them. The hydrogen bonding and van der Waals interactions are best illustrated by the 2D pot of the HSA and trans-resveratrol interaction. Previous studies on the interaction of AFB 1 with HSA also confirmed Sudlow's site 1 as the binding pocket for AFB 1 using in silico approach 17 , and the amino acids residues involved in the binding are in very close proximity to that involved in HSA and trans-resveratrol binding in the same Sudlow's site 1. The van der Waals + hydrogen bonding + desolvation energy for HSA and trans-resveratrol complex was −9.07 kcal/mol, much higher than their electrostatic energy of −0.19 kcal/mol, thus proposing hydrogen bonding and van der Waals interaction as the major forces stabilizing the HSA and trans-resveratrol complex. This further corroborates our thermodynamic findings. Since the binding affinity of trans-resveratrol is much higher than the AFB 1 , trans-resveratrol is able to displace bound AFB 1 to HSA for com- www.nature.com/scientificreports/ peting the binding site. Similar binding sites (subdomain IIA) have also been reported in a study of the binding of oxyresveratrol to HSA 39 . We further explored the binding of mutated HSA with trans-resveratrol. In mutated HSA, Trp-214 was substituted with neutral amino acid glycine to elucidate the changes in the binding fashion of trans-resveratrol with mutant HSA as compared to non-mutated HSA. Glycine was substituted in place of Trp-214 because glycine, the simplest amino acid, is also neutral. The molecular docking study revealed that the complex of trans-resveratrol with mutant HSA was less stabilized than the non-mutated complex because the binding energy of the mutated HSA complex was less negative compared to the non-mutated complex. The binding energy of the complex and the amino acid residues involved in the stabilization of the mutated HSA-trans-resveratrol complex is shown in Table 5. Interestingly, the binding site of trans-resveratrol was located at the same subdomain IIA as it was with non-mutated HSA. However, the number of hydrogen bonds was reduced to 2 only, as shown in Fig. 12. Gly-214 was not involved in any kind of bonding with trans-resveratrol. A mutation study was also performed by substituting the hydrophobic amino acid valine in Trp-214. Surprisingly, the binding site of trans-resveratrol on HSA was different as compared to native non-mutated HSA, and HSA with Trp-214 substituted with Gly. The binding energy of the complex was also less negative. The study with mutated HSA was significant since it investigates the role of Trp-214 during the stabilized complex formation between HSA and trans-resveratrol. The substitution of Trp-214 with either Gly or Val did not result in the highly stabilized complex formation as compared to the non-mutated HSA. The binding of the mutated HSA complex with trans-resveratrol was less negative as compared to the native HSA. The amino acid residues that form the binding pocket for mutant HSA and trans-resveratrol interaction are shown in Table 5. Figure 12 shows the best-docked pose of binding of transresveratrol with mutated HSA. Table 5 represents the amino acid residues involved and binding energies in the formation of mutated HSA-trans-resveratrol complex.
Molecular dynamic simulation studies. Molecular dynamic (MD) simulation studies were carried out to get insights into the dynamic nature of trans-resveratrol binding to HSA over the simulated period up to 100 ns. For the investigation of the system stability, root mean square deviations (RMSD) values of HSA backbone (C-Cα-N) and HSA-T-res complex were calculated, and the graph was plotted from 0 to 100 ns. From  Fig. 13a, it is clear that the RMSD value of HSA alone was stable from 0 to 40 ns, and it was increased from 40 to 60 ns and later became stable again from 60 to 100 ns. For HSA-T-res complex, the RMSD value steadily increases from 0 to 20 ns. From 40 to 100 ns, the system becomes stabilized, and no significant increase or decrease in the RMSD value is obtained, and the system reaches the equilibrium suggesting HSA and transresveratrol is steadily bound to HSA at subdomain IIA. During the simulated time of 100 ns, the RMSD value of HSA and trans-resveratrol complex was lesser than the RMSD value of HSA alone, this also suggests the stability of the HSA system after binding with trans-resveratrol molecule. The RMSD values of HSA obtained in the present study are in good agreement with the previously reported studies 55 .
Root mean square fluctuation (RMSF) values for HSA alone and HSA-trans-resveratrol complex were also evaluated to explore the protein flexibility 56 . Figure 13b shows the plot of RMSF values versus amino acid residues in HSA. It is inferred that the amino acid residues in subdomain IIA are more rigid than other regions due to the complex formation between HSA and trans-resveratrol. Owing to the presence of random coils at the end of helix, flexibility is observed at the end residues, as shown in Fig. 13b.
Radius of gyration (R g ) value for HSA alone and HSA-trans-resveratrol complex was calculated to investigate the compactness of the protein and structural dynamics of the system over the simulated period of 100 ns. From  Fig. 14, it is evident that the R g value of HSA alone initially fluctuates at around 2.80 nm and reaches a maximum fluctuation value of 2.85 nm at around 50 ns. After that, it decreases continuously up to 90 ns, and after that, it remains constant up to 100 ns. The R g values of HSA obtained are in accordance with the previously reported studies 55,57 . On the other hand, the R g value of HSA-trans-resveratrol complex initially decreases from 0 to 20 ns. Then it increases up to 30 ns, becomes stable, and reaches equilibrium from 30 to 100 ns. Figure 15 shows the   www.nature.com/scientificreports/

Conclusion
The study describes the interacting potential of polyphenol, trans-resveratrol with HSA explored by UV-absorption spectroscopy, fluorescence spectroscopy, and molecular docking. The study also investigated the dislodging potential of trans-resveratrol competing for the binding site on HSA by displacing AFB 1 bound to HSA using fluorescence spectroscopic tools. The fluorescence quenching study was used to calculate the Stern-Volmer quenching constant (K SV ), binding constant (K b ), and various thermodynamic parameters (ΔG, ΔH, and ΔS). The K SV and K b values obtained suggested high fluorescence quenching potential and strong binding constant, respectively, for trans-resveratrol and HSA. Circular dichroism studies confirmed an increase in the alpha-helix content in HSA in the presence of trans-resveratrol. MD simulation studies confirmed the dynamic nature of trans-resveratrol binding at the subdomain IIA of HSA over the simulated time of 0 to 100 ns. In silico amino www.nature.com/scientificreports/ acid substitution studies using Trp-214 mutated HSA provided the role of Trp-214 residue in the binding of transresveratrol to HSA.The thermal stability or melting temperature (Tm) of the HSA also increased in the presence of trans-resveratrol. The binding constant of AFB 1 for serum albumin was lower than trans-resveratrol, signifying the displacing potential of the polyphenol for competing AFB 1 acquiring the same binding site i.e. subdomain IIA or Sudlow's site 1. This is the first investigation on the use of trans-resveratrol to remove AFB 1 from serum albumin and thereby to decrease the bound form of AFB 1 . This is a spectroscopy-based study; however, an in vivo study is required to elucidate the effect of trans-resveratrol and AFB 1 competition in animal models. The findings of this study will aid in the understanding of the pharmacokinetics and pharmacodynamics of phytochemical efficacy to compete with bound toxin and quick biotransformation leading to mycotoxin clearance from the body. The study will help explore more phytochemicals and their use in the unloading of the toxic substances from serum albumin, thus reducing the risk of pathological conditions in the human and animal body.

Material and methods
Materials. Aflatoxin B 1 , trans-resveratrol, human serum albumin, warfarin, and ibuprofen were procured from Sigma Aldrich (USA). The reagents used for making buffer solutions like sodium phosphate monobasic and sodium phosphate dibasic were obtained from SRL, India. All the chemicals were high purity grade and used as such without any further purification. Binding parameters like Stern-Volmer quenching constant (K SV ), binding constant (K b ), and bimolecular quenching constant (K q ) were calculated using the following Eq. (2) and (3).

Methods.
where F 0 is the fluorescence intensity of HSA alone; F is the fluorescence intensity of HSA in the presence of ligand; Q is the concentration of the ligand; K q is the bimolecular quenching constant, and τ 0 is the average integral lifetime of the tryptophan residue in HSA (~ 10 -9 s).The binding constant (K b ) for the interaction of trans-resveratrol with HSA was calculated using Eq. (4) The calculations of thermodynamic parameters were based on Eqs. (5) and (6). In Eq. (5), ΔG is the Gibbs free energy, R is the universal gas constant (1.987 cal mol −1 K −1 ), T denotes temperature in kelvin, ΔS is the entropy change, and ΔH represents enthalpy change of the HSA and trans-resveratrol system. www.nature.com/scientificreports/ Investigation of the binding site of trans-resveratrol on HSA using site markers. Most of the small molecule binds to HSA at Sudlow's site 1 (subdomain IIA) or Sudlow's site 2 (subdomain IIIA). To confirm the binding location of trans-resveratrol on HSA, a competitive site markers displacement assay was followed using warfarin and ibuprofen. Initially, 5 micro molar concentration of HSA was saturated with an excess of trans-resveratrol (14 µM) followed by titrations with increasing concentration of warfarin and ibuprofen (0-80 µM). The HSA and trans-resveratrol complex was excited at 280 nm, and the emission was recorded in the wavelength range of 300-400 nm. The percentage of trans-resveratrol displaced by the site markers is calculated according to Eq. (7) as follows where F 1 and F 2 are the fluorescence intensities of HSA bound trans-resveratrol in the absence and presence of warfarin and ibuprofen site markers. The fluorescence spectrum was recorded using Shimadzu RF-6000 spectrofluorometer with fixed emission and excitation bandwidth of 5 nm each.
Circular dichroism. Jasco J-1500 spectropolarimeter was employed to investigate the secondary structure alterations in HSA in the presence of trans-resveratrol. The spectropolarimeter was equipped with a temperature control Peltier system. Quartz cuvette of path length 0.1 cm was used for taking the reading of the sample and for correcting the baseline. Far-UV CD spectra of HSA (5 µM) in the presence of trans-resveratrol (10 and 20 µM) were taken in the wavelength range of 190-250 nm with a data pitch of 1 nm. The scanning speed was fixed to 200 nm/min, and the bandwidth of 1 nm was set. Each spectrum was an average value of 3 spectra. MRE 208 value and percentage alpha helix was calculated using Eqs. (8) and (9), respectively. The thermal melting profile of HSA in the presence of trans-resveratrol was studied by measuring the CD (mdeg) values at 222 nm at a temperature range of 20-90 °C, to investigate the melting temperature (T m ) of HSA.
In Eq. (8), C p represents the concentration of the HSA, n is the number of amino acid residues in HSA, and l is the path length of the quartz cuvette in cm. in Eq. (9), MRE 208 is the mean residual ellipticity value at 208 nm.
Competitive displacement of HSA bound AFB 1 by trans-resveratrol. In the first set of experiments, the dislodging potential of trans-resveratrol was investigated to displace AFB 1 from HSA bound to AFB 1 , employing the fluorescence spectroscopic tool. Five micromolar concentration of HSA was added to 14 µM AFB 1 and subsequently titrated with the increasing concentration of trans-resveratrol (0-20 µM). The HSA-AFB 1 complex was excited at 280 nm, and emission was recorded between 300 and 400 nm.
In the second set of experiments, the dislodging ability of AFB 1 was explored by probing AFB 1 ability to displace trans-resveratrol from HSA bound trans-resveratrol. The percentage displacement of the AFB or transresveratrol was studied by plotting F 2 /F 1 × 100 versus the concentration of trans-resveratrol or AFB 1 .The experiment was performed using Shimadzu RF-6000 spectrofluorometer having xenon flash lamp, with excitation and emission bandwidth of 5 nm each. Sodium phosphate buffer of strength 20 mM and pH 7.4 was used to construct the desired concentration of the sample.
Molecular docking and in silico amino acid substitution studies. Autodock 4.2 tools were employed for performing molecular docking to explore the binding sites of trans-resveratrol on HSA. The chemical structure of trans-resveratrol was obtained from Pubchem (CID: 445154). The crystal structure of HSA was obtained from the RCSB protein data bank (PDB ID: 1AO6). The energy optimization of ligand was performed using Avogadro software, whereas Swiss PDB viewer was used for energy minimization of the protein molecule. PDBQT files were created for both ligand and protein after adding polar hydrogen and removing water molecules. Grid files were created with the grid dimension of 68 × 68 × 44 in xyz axis with grid point spacing of 0.375 Å, and all other parameters were used as default set values. Total 100 GA runs were processed for docking analysis, and Lamarckian genetic algorithm 4.2 with a maximum of 2,500,000 energy evaluations were used for docking calculations. In silico amino acid substitution studies were performed by substituting the desired amino acid in place of Trp-214 followed by saving the mutated HSA molecule in .pdb format. Molecular docking of the mutated HSA with trans-resveratrol was performed using the above-mentioned protocol for native HSA. The final docked complex was visualized using Discovery studio visualizer and PyMOL.
Molecular dynamic simulation studies. The MD simulation studies were carried out to explore the binding mode of trans-resveratrol to HSA. MD simulations were performed by Desmond v4.1 applied in Schrodinger-Maestro v11. The side-chain bumps and steric clashes were fixed. The PDB structure of HSA (1AO6) and transresveratrol (CID: 445154) were optimized for GROMOS96 54a7 force field. These prepared structures were then optimized by GROMOS96 54a7 force field 58 . Simple point charge water model was employed for adding the solvent molecules in the dodecahedron box with 1 Å distance from the protein surface, followed by the addition of four Na + ions for the system neutralization. MD runs were set for 100 ns in three replicas with a time steps of (7) Probe displacement (% ) = F 2 F 1 × 100% www.nature.com/scientificreports/