Fluorescence Spectroscopy and Molecular Docking Approach to Probe the Interaction between Dehydroeburicoic Acid and Human Serum Albumin ()
1. Introduction
Dehydroeburicoic acid (DeEA) is a triterpene purified from medicinal fungi such as Taiwanofungus camphoratus, Fomitopsis officinalis, Fomitopsis pinicola and Wolfiporia cocos [1] [2] . The molecular structure of DeEA was presented in Figure 1. It can protect the liver from CCl4-induced oxidative stress and tissue injuries [3] . It possesses analgesic and anti-inflammatory effects [4] . It exhibits antitumor activity against the human glioblastoma U87MG [2] [5] . It has an excellent therapeutic potential for the treatment of type 1 diabetes and type 2 diabetes [6] [7] . Human serum albumin (HSA) is significant in the blood circulatory system. It contains 585 amino acid residues [8] [9] . It is stabilized by 17 disulfide bridges [10] . It consists of three homologous domains (domain I-III). And each domain contains two subdomains (IA, IB, IIA, IIB, IIIA and IIIB). It has two high-affinity binding sites (site I and site II) [11] [12] . The site I is located in the subdomain IIA. The site II is located in the subdomain IIIA. The interaction between biologically active substances (drugs or natural products) and HSA affects the bioavailability, distribution, free state concentration and metabolism of biologically active compounds in the bloodstream [13] [14] . In addition, the interaction between biologically active compounds and HSA changes the structure and function of HSA [15] . Therefore, probing the interaction between DeEA with HSA is significant to deeply understand the pharmacodynamics and pharmacokinetics properties of DeEA.
In summary, we characterized the interaction between DeEA and HSA by fluorescence spectroscopy, synchronous fluorescence spectroscopy, three-dimensional fluorescence spectroscopy and molecular docking approach. The quenching mechanism, the binding constant, the number of binding site, the thermodynamic parameters and the acting force were estimated according to the fluorescence spectroscopy data. Synchronous fluorescence spectroscopy and three-dimensional fluorescence spectroscopy were performed to probe the conformational and microenvironmental changes of HSA during the binding process. Molecular docking was performed to show the interaction between
Figure 1. The molecular structure of dehydroeburicoic acid.
DeEA and amino acid residues of HSA.
2. Materials and Methods
2.1. Reagents and Materials
HSA (A1887; fatty acid and globulin free) was purchased from Sigma-Aldrich. DeEA was purchased from Aikon Biopharmaceutical R&D Co. Ltd. (Jiangsu, China). Site probes (Warfarin and Ibuprofen) were purchased from Shanghai Xiyuan biological technology Co. Ltd. (Shanghai, China). The concentration of HSA stock solution is 1.0 × 10−4 M in 1.0 × 10−2 M phosphate buffer solution (pH 7.40). The concentration of DeEA stock solution is 1.0 × 10−4 M. The concentration of site probes stock solution is 1.0 × 10−4 M. All reagents used are of analytical grade. The water used for the experiment was ultrapure water. Stock solutions were prepared weekly and stored in the dark at 4˚C.
2.2. Fluorescence Spectroscopy Measurements
Fluorescence spectroscopy measurements were performed on the Thermo Scientific Lumina fluorescence spectrophotometer. The excitation wavelength was 280 nm. The emission wavelength was recorded from 285 to 500 nm. The fixed concentration of 3.0 μM HSA (3.5 mL) was continuously titrated with the addition of DeEA. The photomultiplier tube (PMT) voltage, the excitation slit, the emission slit, the response time, the integration time and the scan speed were set at 500 V, 2.5 nm, 2.5 nm, 1.0 s, 20 ms and 1200 nm/min, respectively. The experiments were performed at 288, 298 and 308 K.
2.3. Synchronous Fluorescence Spectroscopy
Synchronous fluorescence spectroscopy measurements were performed on the Thermo Scientific Lumina fluorescence spectrophotometer. Synchronous fluorescence spectroscopy was recorded from 200 to 500 nm. The scanning interval between the excitation and emission wavelength (Δλ) was set at 15 and 60 nm, respectively. Other parameters are the same as the fluorescence spectroscopy measurements. The experiments were performed at 298 K.
2.4. Three-Dimensional Fluorescence Spectroscopy
Three-dimensional fluorescence spectroscopy measurements were performed on the Thermo Scientific Lumina fluorescence spectrophotometer. The excitation wavelength ranged from 200 to 360 nm. The emission wavelength ranged from 200 to 660 nm. Other parameters are the same as the fluorescence spectroscopy measurements. The experiments were performed at 298 K.
2.5. Site Marker Competitive Experiments
The site marker competitive experiments were performed on the Thermo Scientific Lumina fluorescence spectrophotometer. Warfarin is marker for site I. Ibuprofen is marker for site II [12] [16] . The warfarin-HSA system was continuously titrated with the addition of DeEA. The ibuprofen-HSA system was continuously titrated with the addition of DeEA. Other parameters are the same as the fluorescence spectroscopy measurements. The experiments were performed at 298 K.
2.6. UV-Visible Absorption Spectroscopy Experiments
The UV-visible absorption spectroscopy experiments were performed on the Shimadzu UV-2550 spectrophotometer. The UV-visible absorption spectroscopy was recorded from 200 to 500 nm. The experiments were performed at room temperature.
2.7. Molecular Docking
Molecular docking was performed using the AutoDock [17] . The 3D structure of DeEA was optimized using Gaussian 09 before docking simulations [18] . The binding site was defined using one grid of 120 × 120 × 120 points at the subdomain IIIA [19] . Lamarckian genetic algorithm was used with a total of 100 runs. The DeEA-HSA complex was visualized and analyzed using Chimera [20] .
3. Results and Discussion
3.1. Quenching Mechanism
Fluorescence spectroscopy was performed to probe quenching mechanism of the interaction between DeEA and HSA. The fluorescence spectroscopy of HSA in the absence and presence of DeEA were presented in Figure 2. The fluorescence intensity of HSA obviously decreased with increasing the concentration of
Figure 2. The effect of DeEA on the fluorescence of HSA, c (HSA) = 3.0 μM. Lines 1 - 10: c (DeEA) = 0, 0.143, 0.286, 0.429, 0.572, 0.715, 0.858, 1.001, 1.144, 1.287 μM, respectively; λex = 280 nm; λem = 345 nm; pH = 7.4; T = 298 K. Curve x shows the emission spectrum of DeEA only, c (DeEA) = 0.143 μM.
DeEA. However, the fluorescence intensity of DeEA was almost equal to 0. In general, for dynamic quenching, the quenching constant increases with increasing the temperature [13] . For static quenching, the quenching constant decreases with increasing the temperature [13] . The Stern-Volmer equation was used to estimate the possible quenching mechanism [21] [22] .
(1)
where F0 is the fluorescence intensity of free HSA, F is the fluorescence intensity of the HSA-DeEA system, KSV is the Stern-Volmer quenching constant, [Q] is the concentration of DeEA, Kq is the biomolecule quenching rate constant,
is the lifetime of the fluorophore in the absence of DeEA and the fluorescence lifetime of the biopolymer is 10−8 s [23] .
The Stern-Volmer plots for fluorescence quenching of the DeEA-HSA system at different temperatures were presented in Figure 3. The KSV and Kq value were collected in Table 1. The value of KSV obviously increased with increasing the temperature, which indicated that the quenching mechanism was dynamic quenching [24] . However, the value of Kq was much greater than the maximum scatter collision quenching constant (2.0 × 1010 M−1・S−1), which showed that the quenching mechanism was static quenching [25] . The results demonstrated that DeEA quenched the fluorescence of HSA through the combination of static and dynamic quenching mechanism.
3.2. Binding Constant and Binding Site
For the binding process, the binding constant (KA) and the number of binding sites (n) were estimated according to the following equation [26] .
Figure 3. The Stern-Volmer plots for fluorescence quenching of the DeEA-HSA system at different temperatures, c (HSA) = 3.0 μM; c (DeEA) = 0.143 - 1.287 μM; λex = 280 nm; λem = 345 nm; pH = 7.4; T = 288, 298 and 308 K.
Table 1. The biomolecule quenching rate constant and the Stern-Volmer quenching constant for the DeEA-HSA system at different temperatures.
(2)
where the meanings of F0, F and [Q] are the same as for Equation (1). The double-logarithm plots for fluorescence quenching of the DeEA-HSA system at different temperatures were presented in Figure 4. The KA and n value were collected in Table 2. The KA value obviously decreased with increasing the temperature, which revealed that the stability of the DeEA-HSA complex was reduced during the binding process [27] [28] [29] . Moreover, the number of binding sites approximated to 1 at 288 K, which suggested that there was almost one site for the interaction between DeEA and HSA at this temperature. And the n value obviously decreased with increasing the temperature, which showed that DeEA could not bind to HSA at higher temperature. Since the stability of the DeEA-HSA complex significantly reduced and the value of n was much less than 1 with increasing the temperature during the binding process. Therefore, DeEA could bind to HSA at 288 K. However, DeEA could not be stored and carried by HSA in the body at higher temperature [30] .
3.3. Thermodynamic Parameters and Acting Forces
In order to estimate the acting forces, the thermodynamic parameters enthalpy change (∆H), entropy change (∆S) and free energy change (∆G) of the binding process were calculated according to the Van’t Hoff equation [31] [32] .
(3)
(4)
where KA is the binding constant at the corresponding temperature, R is the molar gas constant and T is the thermodynamic temperature.
The thermodynamic parameters were collected in Table 3. The negative value of ∆G indicated that the binding process was spontaneous. The negative value of ∆H revealed that the binding process was exothermic. According to the theory of Ross and Subramanian, we concluded that the hydrogen bonding and the van der Waals force were major acting forces for the interaction between DeEA and HSA [31] . Therefore, the hydrogen bonding and the van der Waals force were major acting forces. And the binding process were spontaneous and exothermic.
Figure 4. The double-logarithm plots plot for fluorescence quenching of the DeEA-HSA system at different temperatures, c (HSA) = 3.0 μM; c (DeEA) = 0.143 - 1.287 μM, respectively; λex = 280 nm; λem = 345 nm; pH = 7.4; T = 288, 298 and 308 K.
Table 2. The binding constant and the number of binding site for the DeEA-HSA system.
Table 3. The thermodynamic parameters for the interaction between DeEA and HSA.
3.4. Site Marker Competitive Experiments
The site marker competitive experiments were performed to locate the major binding site for the interaction between DeEA and HSA. HSA has two principal sites located in hydrophobic pocket. The sites are located in the hydrophobic cavities in subdomains IIA and IIIA, which exhibit similar chemical properties [33] . The binding cavities associated with subdomains IIA and IIIA are also referred to as site I and site II. Warfarin is marker for the site I. Ibuprofen is marker for the site II [34] [35] . The warfarin-HSA system and ibuprofen-HSA system were continuously titrated with the addition of DeEA, respectively. Then, the experiment data were analyzed by Equation (2). The binding constant of the DeEA-HSA system before and after addition of site markers were presented in Table 4. The binding constant obviously decreased with the addition of ibuprofen, which revealed that warfarin displaced DeEA from the binding site. Therefore, we concluded that site II might be the major binding site for the interaction between DeEA and HSA.
3.5. Fluorescence Resonance Energy Transfer and Binding Distance
There was obvious overlap between the fluorescence spectrum of HSA and the absorption spectrum of DeEA in Figure 5. According to the fluorescence resonance energy transfer theory, the binding distance (r) between HSA (donor) to DeEA (acceptor) was calculated [36] . The efficiency of energy transfer (E) depends on r and the extent of spectral overlap (J). The value of E can be calculated by the following equation:
(5)
where F0 is the fluorescence intensity of free HSA, F is the fluorescence intensity of the HSA-DeEA system, R0 is the critical energy transfer distance when E = 50% and r is the binding distance between DeEA and HSA. The value of R0 can be calculated according to the Forster’s equation.
Table 4. The binding constant of the DeEA-HSA system before and after addition of site probes (warfarin and ibuprofen).
Figure 5. The overlap between the fluorescence spectrum of HSA (a) and the absorption spectrum of DeEA (b), λex = 280 nm; λem = 345 nm; pH = 7.4; c (HSA) = c (DeEA) = 3.0 μM.
(6)
where k2 is spatial orientation factor of the dipole, N is refractive index of the medium and Ф is the fluorescence quantum yield of HSA. In the present case, k2 = 2/3, N = 1.336 and Ф = 0.118 [37] [38] . The value of J can be calculated by the following equation:
(7)
where
is the fluorescence intensity of HSA at wavelength
and
is the molar absorption coefficient of DeEA at wavelength
.
In view of the above, we calculated that E = 0.15, R0 = 2.45 nm and r = 3.29 nm, r < 7 nm. The value of R0 and r were on the 2 - 8 nm scale and
, which indicated that DeEA could interact with HSA [39] . The results revealed that DeEA could interact with HSA and the energy transfer could occur with high probability.
3.6. Conformational Investigation
3.6.1. Synchronous Fluorescence Spectroscopy
Synchronous fluorescence spectroscopy was performed to probe the conformational and microenvironmental changes of HSA during the binding process. The effect of DeEA on the synchronous fluorescence of HSA was presented in Figure 6. When Δλ = 15 nm, the shift of λmax was minor from 300.6 to 301.4 nm, which showed that the change of microenvironment around tyrosine residues were trivial [40] [41] . When Δλ = 60 nm, the shift of λmax remained unchanged, which indicated that the microenvironment around tryptophan residues remained the same [40] . However, the stronger fluorescence quenching of tyrosine residues than tryptophan residues was observed with increasing the concentration of DeEA, which revealed that the binding site was nearer tyrosine residues. The tyrosine residues were mainly located in the subdomain IIIA. Therefore, we concluded that the major binding site was located in the subdomain IIIA (site II). These results were consistent with the site marker competitive experiments.
3.6.2. Three-Dimensional Fluorescence Spectroscopy
Three-dimensional fluorescence spectroscopy was performed to explore the conformational and microenvironmental changes of HSA during the binding process. Three-dimensional fluorescence spectroscopy of free HSA and the DeEA-HSA system were presented in Figure 7. The corresponding parameters were collected in Table 5. Peak a (λex = λem) is the Rayleigh scattering peak [42] . Peak b (2λex = λem) is the second-order scattering peak [42] . Peak 1 (λex = 280 nm and λem = 331 nm) mainly exhibits the spectrum characteristic of tyrosine and tryptophan residues, which can reflect conformational changes of HSA [19] [43] . In this study, the fluorescence intensity of peak a and peak b obviously decreased with the addition of DeEA due to the formation of the DeEA-HSA complex. The fluorescence intensity of peak 1 increased with the addition of DeEA, which
Figure 6. The effect of DeEA on the synchronous fluorescence of HSA: (a) ∆λ = 15 nm; (b) ∆λ = 60 nm. c (HSA) = 3.0 μM. Lines 1 - 10: c (DeEA) = 0, 0.143, 0.286, 0.429, 0.572, 0.715, 0.858, 1.001, 1.144, 1.287 μM, respectively; pH = 7.4; T = 298 K.
revealed that the hydrophobic microenvironment near tyrosine residues has been changed [44] . The results showed that DeEA have interacted with HSA and slightly changed the conformation and microenvironment of HSA.
3.7. Molecular Docking
In order to show the interaction between DeEA with amino acid residues of HSA, molecular docking was performed. The binding mode of the DeEA-HSA system was presented in Figure 8. The results revealed that the DeEA molecular
Figure 7. The three-dimensional fluorescence of free HSA (A) and the DeEA-HSA system (B); pH = 7.4; T = 298 K.
located in the cavity surrounded by the following amino acid residues: Asn-405, Val-409, Arg-410, Lys-413, Lys-414, Glu-492, Val-493, Leu-529, Thr-540, Leu-544, Lys-545 and Met-548. The Glu-492 formed hydrogen bonding with the hydrogen atom of the hydroxyl group of DeEA at the distance of 2.571 Å. In
Figure 8. The binding mode of the binding DeEA to HSA, the secondary structure of the protein is shown and the important neighboring amino acid residues are labeled. The ligand structure is represented in the ball-and-stick model and hydrogen bond is indicated by a green dashed line.
Table 5. The three-dimensional fluorescence spectral characteristic parameters of free HSA and the DeEA-HSA system.
*The concentration of HSA was 3.0 μM for each system.
addition, the Lys-545 formed the hydrogen bonding with the oxygen atom of the hydroxyl group of DeEA at the distance of 1.970 Å. Hydrophobicity surface of amino acid residues within 5 Å around DeEA was presented in Figure 9. As color changes from blue to red, surface alters from hydrophilic to hydrophobic gradually. The hydroxyl groups of DeEA were in hydrophilic surface and the hydrophobic portion was in hydrophobic surface, which decided the reasonable interaction between DeEA and HSA. The molecular docking results revealed that the hydrogen bonding and hydrophobic force were significant for the interaction between DeEA and HSA, which were consistent with the thermodynamic analysis. The hydroxyl groups of DeEA were important groups during the binding process. The Lys-545 and Glu-492 were important amino acid residues for the interaction between DeEA and HSA.
Figure 9. Hydrophobicity surface of amino acid residues within 5 Å around DeEA.
4. Conclusion
The interaction between DeEA and HSA was systematically investigated by fluorescence spectroscopy, synchronous fluorescence spectroscopy, three-dimensional fluorescence spectroscopy and molecular docking approach. The fluorescence spectroscopy results suggested that DeEA quenched the intrinsic fluorescence of HSA through the combination of static and dynamic quenching mechanism. The thermodynamic parameters and molecular docking results indicated that the hydrogen bonding, hydrophobic force and van der Waals force were major acting forces during the binding process. DeEA could bind to HSA at 288 K. However, DeEA could not be stored and carried by HSA in the body at higher temperature. The site marker competitive experiments and synchronous fluorescence spectroscopy revealed that the site II was the major binding site. According to the fluorescence resonance energy transfer theory, the energy transfer could occur with high probability and the binding distance was 3.29 nm. The synchronous fluorescence spectroscopy and three-dimensional fluorescence spectroscopy results demonstrated that the binding process slightly changed conformation and microenvironment of HSA. The hydroxyl groups of DeEA were important groups during the binding process. The Glu-492 and Lys-545 were important amino acid residues for the interaction between DeEA and HSA. The interaction between DeEA and HSA was not characterized so far. Therefore, it was of vital significance to study on the interaction between DeEA and HSA. These experimental results will provide theoretical support for understanding the pharmacodynamics and pharmacokinetics properties of DeEA.
Acknowledgements
This work was supported by the National Natural Science Foundation of China (31270088); the program of introducing talents to universities on “creation and utilization of germplasm of mushroom crops” discipline innovation initiative (No. D17014) and the major project for agricultural application technology innovation of Shandong province (2017). Thanks to Mr. Xiangming Chen, Binzhou Medical University, for assisting the fluorescence spectroscopy studies.