Abstract

Nicotine, the important component of cigarette products, may have an impact on the oral environment after inhalation. The research of interaction between nicotine and bovine submaxillary mucin (BSM) contributes to understand the binding mechanism of nicotine and BSM, and the effects of nicotine on the structure and function of the mucin. NMR data demonstrated that the interaction between nicotine and BSM did exist, and it was pyrrolidyl ring of nicotine playing the major role in the binding. The quenching mechanisms of nicotine and BSM in different pH were different: for acidic environment, the quenching was dynamic; while it became static in the alkaline circumstance. Synchronous fluorescence spectra indicated that nicotine had effect on the microenvironment of the Trp rather than Tyr residue. Meanwhile, the impact of nicotine on the conformation of BSM was also confirmed by 3D fluorescence and FTIR spectra.

1. Introduction

Mucins are large, abundant, and filamentous glycoproteins and composed of secreted mucins and cell-tethered mucins with polymerizing and nonpolymerizing forms [1, 2]. General structural features of mucins consist of a long central domain rich in proline, threonine, and serine (PTS domain) and are densely grafted with anionic and hydrophilic carbohydrate chains [3]. Mucins can act as a steric barrier, preventing nonspecific interaction of proteins and cells with the underlying cell membrane, protecting underlying tissues against external insult, mechanical stress, and pathogens, transducing cell signal, and so forth [4, 5].

Salivary mucin, a kind of salivary protein, accompanies with the whole digestive process from the oral to gastrointestinal organs and plays a significant role in the protection of oral cavity [6, 7]. Submaxillary mucin is the most associated mucin types in oral processing [5]. For BSM, the glycosylation level of the PTS domain is about 70–85% of the total molecular weight and sialic acid accounts for as much as 30% of the molecular weight [3]. As one of the mucins, BSM contains many charged groups, resulting in its pH-dependent physicochemical properties. Moreover, BSM is amphiphilic and can be linked with each other or interact with other proteins via noncovalent bonds [8, 9]. However, the field of investigating the interaction between BSM and small molecules is still blank.

Tobacco smoking is a major worldwide health problem, which can lead to high morbidity and mortality. As the principal psychoactive agent in tobacco, nicotine (NIC, shown in Figure 1) has been determined to be a highly addictive substance with subjective effects like clear-headedness, feelings of relief, fatigue recovery, and hyperactivity [10, 11]. During cigarette smoking, NIC is absorbed into the body and induces multiple pharmacological and toxicological effects [12]. Thus, NIC may have an effect on the activities of the oral cavity, such as salivary mucin, after its inhalation, which may pose a further threat to animal’s health. However, the interaction between NIC and BSM has not been studied so far.

This study was committed to probe into the interaction of NIC with BSM in vitro by spectral approaches. Nuclear magnetic resonance (NMR) measurements were carried out to investigate whether and how the interaction between BSM and NIC occurred. Fluorescence quenching measurements were used for obtaining the quenching mechanism. Due to the influence of pH on the forms of NIC in the solution, the effects of pH on the binding of NIC to BSM were discussed. Synchronous fluorescence, three-dimensional (3D) fluorescence, and Fourier transform infrared (FTIR) spectra were used to analyze the effect of NIC on the conformation of BSM.

2. Experimental

2.1. Chemicals and Materials

Bovine submaxillary mucin (BSM) was purchased from Dalian Meilun Biological Technology Co., Ltd. (Dalian, China). The contents of protein and carbohydrate were 36.6% and 56.7%, respectively. The BSM stock solution was prepared at a concentration of 4.76 × 10−4 M in 0.05 M phosphate buffer. Nicotine (NIC) (purity > 99%) and deuterium oxide at 99.9% purity were provided by J&K Scientific, Ltd. (Beijing, China). All other reagents were of analytical grade.

2.2. Methods
2.2.1. NMR Measurements

1H NMR spectra experiments were performed on a Bruker Avance 400 MHz NMR spectrometer operating at 400.13 MHz for hydrogen at 298 K. The NMR studies were carried out by fixing the concentration of NIC (9.00 × 10−3 M) while adding different ratios of BSM ( = 0, 1/400, 1/200, 1/100, 1/50).

2.2.2. Fluorescence Measurements

Fluorescence quenching measurements were conducted via a Cary Eclipse Fluorescence Spectrophotometer (Varian, USA) equipped with 1.0 cm quartz cells. Fluorescence quenching spectra were recorded by fixing the concentration of BSM (1.10 × 10−4 M) while varying the NIC concentration from 0.00 to 19.15 × 10−3 M at three pH (5.0, 6.9, and 8.0). Prior to fluorescence measurements, the solutions were mixed and maintained for 1 h in a thermostat water bath at 288, 298, and 310 K.

Synchronous fluorescence spectra of BSM (1.10 × 10−4 M) with different NIC concentrations (0–19.15 × 10−3 M) were measured at  nm and  nm, respectively.

Three-dimensional (3D) fluorescence spectra of BSM (1.10 × 10−4 M) and NIC-BSM complex (molar ratio, 1 : 1) were obtained at an excitation wavelength range of 200–400 nm with an increment of 5 nm. Emission spectra were also monitored between 200 and 500 nm.

2.2.3. FTIR Measurements

FTIR spectra were recorded on a Nicolet–6700 FTIR (Thermo, USA) spectrometer with a smart OMNI-sampler accessory. The spectra of BSM (9.52 × 10−5 M) in the absence and presence of NIC (2.49 × 10−4 M) were recorded over the spectral range 4000–600 cm−1 with a resolution of 4 cm−1 and 64 scans at 298 K. Background spectra were collected before each measurement. The spectrum of the buffer solution was subtracted from the spectra of the BSM and the BSM-NIC complexes.

3. Results and Discussion

3.1. Characterization of Interaction between BSM and NIC
3.1.1. NMR Spectra Analysis

NMR spectrum, an effective method for evaluating the interaction between a ligand and its target molecule [13, 14], was conducted to study whether and how NIC bound to BSM. The changes of NMR parameters of ligands, such as absolute peak positions and linewidth, can reflect the binding activity between protein and ligand [15]. As displayed in Figure 2, different degrees of changes in peak position as well as the overlapping of split peaks were noticed with increasing BSM, indicating that the molecular interaction of NIC with BSM occurred.

To present the changes in chemical shift of different protons for NIC more intuitively, the changes of the chemical shift (Δδ) were calculated and plotted versus the molar ratio of BSM to NIC (Figure 3). Compared with the protons on the pyridine ring of NIC, the changes of chemical shifts for protons (H5, H6, H7, H8, and H9) on the pyrrolidyl ring of NIC were much more obvious under the same condition, illustrating the pyrrolidyl ring of NIC played a more important role in the NIC-BSM complex formation. In conclusion, NIC, pyrrolidyl ring of NIC more particular, was capable of interacting with BSM.

3.1.2. Fluorescence Quenching and Quenching Mechanism

On the basis of NMR studies, the fluorescence quenching of BSM-NIC system was studied. In order to simulate the oral environment of animal, fluorescence quenching experiments were carried out at 310 K and pH 6.9, and the results were displayed in Figure 4(b2). As seen in Figure 4(b2), BSM can emit strong fluorescence after being excited with wavelengths of 280 nm. The fluorescence intensity decreased significantly with the addition of NIC, which suggested that NIC could interact with BSM [16]. In addition to the change in intensity, the maximum emission wavelength was slightly red shifted, suggesting that the conformational changes in BSM were induced by NIC [17, 18].

Generally, fluorescence quenching may be either dynamic, which is caused by the collision of fluorophore with quencher, or static, which is caused by the formation of ground-state complex [19, 20]. As temperature rising, dynamic quenching constants are expected to increase because higher temperature results in larger diffusion coefficients. Reversely, the static quenching constants are supposed to decrease because the complex stability decreases with increasing temperature [21]. Thus, these two mechanisms could be distinguished by comparing the changes of quenching constants with temperature rising. The quenching constants could be estimated by the following well-known Stern-Volmer equation [22, 23]:where and denote the fluorescence intensities of BSM in the absence and presence of NIC, respectively. is the concentration of the quencher, and is the quenching constant. is the fluorescence lifetime of the molecule without any quencher and the fluorescence lifetime of the biopolymer is about 10−8 s [24]. is the quenching rate constant of the biological macromolecule.

The linear regressions of the plot of against at different temperatures were shown in Figure 4(b2), and the corresponding values of and were listed in Table 1. increased as the temperature rising, illustrating that the interaction was dynamic and driven by collision.

3.1.3. Binding Constants and Thermodynamic Parameters

The binding constants () and number of binding sites () could be calculated by the following equation [25]:where and demonstrate the fluorescence intensities in the absence and presence of BSM, respectively, and refers to the concentration of BSM. and , determined by the linear regression of the plot of against , are the binding constants and number of binding sites, respectively. The results were listed in Table 2. The binding constants and number of binding sites increase with the temperature rising, which indicated that temperature had an impact on the binding of NIC to BSM.

Thermodynamic parameters (, , and ) can be calculated using the data of the fluorescence quenching measurements and by the van’t Hoff equation as follows [26]:where is the associative binding constant at the corresponding temperature and is the gas constant.

As shown in Table 2, ΔG was negative, suggesting that the binding was spontaneous. Meanwhile, according to the theory of Ross and Subramanian [27], the positive values of ΔH and ΔS illustrated that the hydrophobic force played a major role in the binding process.

3.1.4. The Effects of pH on the Fluorescence Quenching of BSM by NIC

NIC is a weak base with different forms in different pH [28], which may cause differences in the binding of NIC to BSM under the conditions of different pH. Besides, there are differences in pH of individual oral environment. Therefore, the effects of pH on the interaction of NIC to BSM are valuable to be investigated. In addition to the above pH (pH 6.9), the fluorescence quenching in pH 5.0 and pH 8.0 was also investigated. All the results were summarized in Figure 4 and Table 1.

As shown in Table 1, the quenching mechanism in pH 5.0 was similar to that in pH 6.9; namely, it was dynamic under the condition of acidity. While it was opposite under alkaline condition (pH 8.0), decreased with increasing of the temperature; that is to say, the quenching was static along with the formation of ground-state complex. Besides, the larger in alkaline condition showed that the binding of NIC to BSM was stronger in alkaline environment. Putting it another way, the content of NIC in the cigarettes for people who are in more alkaline oral environment should be lower.

The different mechanisms and quenching ability may be due to the different forms of NIC and BSM in different values of pH. As mentioned above, NIC which is a binary organic weak base satisfied the following equilibrium (, ) [28].

The forms of NIC in the acid and alkaline condition are different: C10H14N2 in acid, and C10H14N2 as well as C10H14N2H+ in alkaline, as shown in Figure 5. Thus, when pH reaches to 5, NIC is in the form of C10H14N2, while BSM is near to its isoelectric point with relatively tight structure and the aromatic amino acid residues which contributed to the fluorescence are mainly in hydrophobic region. NIC with a strong positive charge is equivalent to the molecular ion, which will limit its access to the hydrophobic region; thereby the opportunity to interact with the aromatic amino acid residues in the hydrophobic region will be reduced. However, when pH > 7, more amino acid residues are exposed to the surface of BSM and the solution, and the positive charges of NIC are decreased to be more neutral, which will strengthen the interaction between NIC and BSM, as well as the formation of complex.

3.2. Conformation Investigations
3.2.1. Synchronous Fluorescence Measurements

Synchronous fluorescence spectroscopy is a very simple, sensitive, and effective technique to probe into the microenvironment of amino acids residues of protein, and it can be obtained by setting a fixed interval (Δλ) between the excitation and emission monochromator [29]. Specifically, when the scanning interval (Δλ) is set to 15 nm and 60 nm, the synchronous fluorescence gives the characteristic information of tyrosine (Tyr) and tryptophan (Trp) residues, respectively [30]. There was a slight emission wavelength at  nm (data not show), indicating the emission of BSM is primarily attributed to the Trp residues. The effect of NIC on BSM synchronous fluorescence ( nm) was displayed in Figure 6. The maximum emission wavelength shows a gradual red shift with the addition of NIC, which demonstrated the polarity around the Trp residue was slightly changed to be more polar in the presence of NIC [31]. Besides, the decrease of fluorescence intensity could also be observed in Figure 6, which further indicates the occurrence of fluorescence quenching during the binding process. Moreover, the decrease of fluorescence intensity might due to the reduction of energy transfer between aromatic amino acid residues, resulting from the stretch of BSM caused by high concentration of NIC.

3.2.2. 3D Fluorescence Spectra

3D fluorescence spectrometry, a new method for the study of protein conformation, was also used to investigate the structural changes in BSM caused by interaction with NIC. The 3D fluorescence spectra of BSM in the absence and presence of NIC were shown in Figure 7, and the corresponding data were summarized in Table 3. Peak 1 refers to the spectral characteristic of Trp and Tyr residues, and peak 2 presents the fluorescence characteristics of the polypeptide backbone structures and is relevant to the secondary structure of protein [32, 33]. When NIC was added, a decrease in intensity along with a slight red shift of the maximum emission wavelength in peaks 1 and 2 occurred. Moreover, a new fluorescence peak, named peak a, appeared, which was considered as the fluorescence peak of free NIC with high concentration. Owing to the intensity changes and peak shifts, the conclusions could be drawn that the binding of NIC to BSM induced conformational and microenvironmental changes of BSM [34]. And these findings were basically in agreement with the results of synchronous fluorescence measurements.

3.2.3. FTIR Spectra

FTIR has emerged as a widely used and efficient method to analyze the structural and conformational changes of protein after interacting with small molecules [35]. The stability of protein secondary structure is closely related to the formation of hydrogen bonds. Once the hydrogen bonds in the protein molecules are influenced by the external factors, the vibration frequency or the absorption intensity of these characteristic absorption peaks will be changed, which could demonstrate the ligand interacts with protein and induces conformational changes in the secondary structure of protein [36]. There are three typical absorption bands in the midinfrared region for protein: the first region (~3300 cm−1) refers to the stretching resonance of NH [37, 38]; the second one (1700~1600 cm−1) is caused by C=O stretching vibration of amide I band [36]; the last region (1600~1500 cm−1) involves N–H bending vibration and C–N stretching vibration of the amide II band [39]. Due to the superior sensitivity of amide I band, it has been more widely selected to study the changes in the protein secondary structure [40].

As shown in Figure 8, the stretching resonance of NH (3368.55 cm−1) and C=O stretching vibration of amide I band (1645.49 cm−1) in BSM are clear to be observed. After adding NIC, blue shifts of wavenumbers occurred in both of the above bands: the stretching resonance of NH shifted to 3374.59 cm−1 and C=O stretching vibration of amide I band shifted to 1647.79 cm−1. Therefore, the addition of NIC changed the original network of hydrogen bonds, namely, affected the spatial structure of BSM, which could explain the interaction between NIC and BSM from another perspective.

4. Conclusions

The binding of NIC to BSM was confirmed by NMR, fluorescence, and FT–IR approaches. NMR spectra disclosed the existence of interaction between NIC and BSM and demonstrated that it was mainly contributed by the pyrrolidyl ring of NIC with the molecule of BSM. Fluorescence spectra also proved the interaction from another perspective; namely, the fluorescence of BSM could be quenched by NIC. The influence of pH on the interaction of NIC with BSM was explored to show that different values of pH corresponded to different interactional strength and quenching mechanisms. When pH < 7, the dynamic quenching was performed; while pH > 7, the quenching was static with larger quenching constants than those of the former. Synchronous fluorescence, 3D fluorescence, and FTIR spectra indicated that nicotine had effect on the microenvironment of BSM and could lead the polarity around the Trp residue increase. This study can not only help to fill the gaps of research in the interaction between NIC and salivary mucin but also contribute to cognize the impact of NIC on the oral environment and provide theoretical basis for limiting smoking.

Conflict of Interests

The authors declare that there is no conflict of interests regarding the publication of this paper.

Acknowledgment

The authors gratefully acknowledge the financial support from China Tobacco Yunnan Industrial Co., Ltd. (Grant no. 2014H1069).