Effect of Interaction Phenolic Compounds with Milk Proteins on Cell Line ()
1. Introduction
Phenolic compounds with anti-inflammatory and antioxidant activities play an important role in antitumor activity. Oxidative stress may cause damage to DNA, thus inducing mutations that may contribute to progressive tumor growth [1] . Several reports have demonstrated the anti-proliferative effects of herbal polyphenols, such as quercetin, in various human cancer cell lines [2] [3] .
Phytochemicals are defined as bioactive nonessential nutrients from plants (phyto is derived from the Greek word phyto, which means plant). They have a variety of human health effects such as possessing putative chemoreventive properties (anticarcinogenic and antimutagenic) and interfering with tumor promotion and progression [4] .
Natural phenolic compounds play an important role in cancer prevention and treatment. Phenolic compounds from medicinal herbs and dietary plants include phenolic acids, flavonoids, tannins, stilbenes, curcuminoids, coumarins, lignans, quinones, and others. Various bioactivities of phenolic compounds are responsible for their chemopreventive properties (e.g., antioxidant, anticarcinogenic, or antimutagenic and anti-inflammatory effects) and also contribute to their inducing apoptosis by arresting cell cycle, regulating carcinogen metabolism and ontogenesis expression, inhibiting DNA binding and cell adhesion, migration, proliferation or differentiation, and blocking signaling pathways. This review covers the most recent literature to summarize structural categories and molecular anticancer mechanisms of phenolic compounds from medicinal herbs and dietary plants [5] .
Fourier Transform Infrared Spectroscopy FTIR is a technique that measures the infrared intensity versus wavenumber of light, by shining infrared radiation on sample protein, polypeptide backbone absorbs light and cause the vibration spectral band at different frequencies depended on wavelengths of radiation in the infrared region of the spectrum [6] . FTIR spectroscopy gives the information of protein conformation in the secondary structure. It is the technique capable of quantitative and qualitative analysis of chemical characteristics on the surfaces [7] .
The objective of the study was to further our understanding of the interaction between some phenolics (Rosmarinic acid, Chlorogenic acid, Quercetin, Vanillin, Gallic acid, Caffic acid, Catechin and some Tannins), and milk proteins (casein and whey proteins isolate), because this interaction reduces the nutritional value of the milk proteins and phenolic compounds as anticancer so the aim of this study is to know effect these interactions of phenolic compounds as anticancer on human cells line.
2. Materials and Methods
2.1. Materials
Fresh cow’s skim milk was obtained from faculty of agriculture, Cairo University. Whey proteins isolate (WPI) was obtained from Davisco Foods International Inc. (Minnesota, USA). Sodium di basic from Egyptian Co., Sodium mono basic from MERCK (Darmstadt-Germany), Ethanol from sd. fine-Chem. Limited, Catechin was purchased from Fluka Chemical Co., Gallic and Rosemarinic acids were obtained from MP Biomedical LLC. Caffic acid was purchased from Bio Basic INC. Vanillin and Chlorogenic acid, from Roth GmbH Co. Qurecetin, from ALDRICH. Sephadex LH-20 and tannic acid from Sigma, Chinese green tea leaves, walnut, lentil from Poland-Olsztyn,
2.2. Methods
2.2.1. Preparation of Casein Powder
Casein powder was prepared from fresh cow’s skim milk according to Morr [8] .
2.2.2. Preparation of Standard Phenolic Compounds Solution
Phenolic compounds (Catechin, Gallic acid, Qurecetin, Caffic acid and Vanillin) were dissolved separately in 0.1 M sodium phosphate buffer pH 7 (0.1% w/v) while Chlorogenic acid and Rosemarinic acid were dissolved separately in ethanol (0.1% w/v).
Extraction of tannins: Extraction of tannins from walnut, green tea and lentil were attained according Kosi?ska [9] .
Cell culture: Cytotoxic effect on human cell line (HePG2: Human hepatocellular carcinoma cell line), (MCF7: Human Caucasian breast adenocarcinoma) and (HCT116: Colon cell line): Cell viability was assessed by the mitochondrial dependent reduction of yellow MTT (3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyl tetrazolium bromide) to purple formazan [10] . All procedures were done in a sterile area using a Laminar flow cabinet biosafety class II level (Baker, SG403INT, Sanford, ME, USA). Cells were suspended in RPMI 1640 medium for HePG2-MCF7 and HCT116-DMEM for A549. The absorbance was then measured using a microplate multi- well reader (Bio-Rad Laboratories Inc., model 3350, Hercules, California, USA) at 595 nm and a reference wavelength of 620 nm. A statistical significance was tested between samples and negative control (cells with vehicle) using independent t-test by SPSS 11 program.
2.2.3. Preparation Sample for Fourier Transform Infrared Spectroscopy (FTIR)
10 mg Milk proteins (10% W/V) samples were dissolved in 50 µl 0.1 M Sodium phosphate buffer at pH 7 and mixed with Phenolic compounds (1 mg/1µl buffer) solutions to give a final protein concentration of 10% containing 1% Phenolic compounds. The solution was initially freeze dried, SUBLIMATOR, VaCo5, ZIRBUS technology, Germany. FTIR (JASCO FT/IR 6100 using KBr Wafer technique Kim and Kim [11] was performed on Milk proteins and Phenolic compounds.
3. Results and Discussion
Casein and WPI are contributes to beneficial therapeutic effects, including anti-cancer; casein and WPI directly targets both tumor cells and tumor vasculature, thereby inhibiting tumor growth, proliferation, and angiogenesis of HePG2 and MCF7 but without any effect on HCT116, Table 1.
3.1. FTIR Spectra
The spectra were recorded under conditions generally applied in quantitative work. IR spectra were recorded in the region from 4000 - 250 cm−1, but the bands in the region 4000 - 1400 cm−1 were analyzed in detail, since they are characteristic of OH groups while NH groups were appeared at (3000 - 4000 cm−1) of various protonic species that undergo hydrogen bonding interaction. Another region of interest was the region from 1800 - 1400 cm−1, characteristic of the bending vibrations of the same group. Since the bands in this region are wide and complex.
Interaction of casein and whey protein with phenolic compounds was determined by FTIR; it was found that some complexes exhibit hydrogen bonding. Also, electrostatic interaction plays a dominant role in the stabilization of the peptide by phenolic compounds. Phenolic molecules have been placed appropriately near the side chain groups of the peptide. The functional groups para-OH (ρ-OH) meta-OH (m-OH) and COOH of Phenolics have been assumed to act as a hydrogen bond donor/acceptor for different side chain groups of amino acid [12] .
The FTIR spectrum of pure casein and whey protein surface displays two characteristic bands at (1648 - 1649) cm−1 respectively, (amide-I) band arises predominantly from the protein amide C=O stretching vibrations, and (1536 - 1547) cm−1, respectively, (amide-II) band is due to the amide N-H bending vibrations and C-N stretching vibrations as mentioned by Huang [5] .
Fourier transform infrared spectroscopy (FTIR) spectrum of pure WPI displays two characteristic bands of amide Ι (1649 cm−1) which associated with C=O stretching vibration, and amide Π (1547 cm−1) which resultant from N-H bending vibration. But the FTIR spectrum of casein revealed that amid Ι and Π were at 1648 and 1563 cm−1 respectively. The significant peak position shifts absorbed in amide Ι and Π bands attributed to hydrogen bonding between all phenolics and milk whey proteins. The interactions between WPI and some mono-, di- and polyphenolic compounds were illustrated in Figures 1(a)-(j). on the other hand the interactions between casein and some mono-, di- and polyphenolic compounds were illustrated in Figures 1(k)-(t).
3.2. Interactions with Mono-Phenolic Compounds
Chloroginic acid has anticancer effect on all tumor cells but this effect more significance on (HePG2). This result agree with Takahama [13] where showed that chlorogenic acid could also inhibit the formation of DNA single strand breaks and prevent the formation of dinitrogen trioxide by scavenging nitrogen dioxide generated in the human oral cavity.
On the other hand complex chloroginic-WPI appears against effect on (MCF7), but this complex has significant effect on (HePG2); while the complex chloroginic-casein appeared against effect on (HCT116). The interaction
Table 1. Cytotoxic activity of phenolic compounds against the human tumor cell line.
Sample concentration ranged between (100 to 0.78 ppm) using MTT assay. HEPG2: (Human hepatocellular liver carcinoma cell line). HCT116: (Colon cell line). MCF7: (Human Caucasian breast adenocarcinoma).
chloroginic acid with milk proteins lost effect on all cells, Table 1; this may be due to interaction between chloroginic acid and WPI was weak. The results in Figure 1(a) elucidated that amid Ι and Π of chloroginic-WPI acid complex appeared at 1648, 1541 cm−1 respectively and NH2 group in complex appeared near control, Figure 1(b) showed that amid Ι and Π for casein-chloroginic acid complex appeared at 1654 and 1543 cm−1 respectively, also ester group at 1740 cm−1 was formed, while NH2 group in complex was near control (casein only).
Caffeic acid has positive effect on HePG2 and MCF7 but without effect on HCT116, Table 1; this agree with Surh [4] . Han [14] showed that caffeic acids, (an analog of phenolic acids) modulate the ceramide-induced signal transduction pathway, suppress the activation of nuclear factor kappa-lightchain-enhancer of activated cells, and inhibit protein tyrosine kinase activity. caffeic acids could also inhibit tumor promotion, epidermal growth factor and tumor necrosis factor-alpha production [4] . Moreover, some phenolic acids (caffeic acid, ferulic acid, gallic acid, protocatechuic acid, etc.) in grape extracts and wine contribute to their activity against various types of cancer such as breast, lung, and gastric cancer [15] .
While complex caffeic-WPI and caffeic-casein were appeared negative affect on (HCT116), but positive effect on (MCF7), while caffeic-casein has negative effect on (HEPG2), but caffeic-WPI has positive effect on (HEPG2). The interaction caffeic acid with milk proteins has lost effect on all tumor cells. Table 1 these due to the strong interaction between them in Figure 1(c); the function groups of WPI-caffic acid complex as comparison with WPI, amid Ι and Π appeared at 1638 cm−1 respectively and NH2 group was disappeared, this means that interaction between caffic acid and WPI was strong and this agree with the pervious results Hassan [16] . Amid Ι for the casein-caffic acid complex appeared at 1649 cm−1 while amid Π disappeared, but NH2 group was near control (Figure 1(d)).
The inhibitory effect of caffeic acid was greater than that of chlorogenic acid with treatments at the same concentration; Caffeic acid is one of the major metabolites produced by the hydrolyzation of chlorogenic acid, Because a large amount of chlorogenic acid is absorbed in the metabolized form, considerable attention has been focused on the biological effects of metabolites such as caffeic acid in order to evaluate possible in vivo effects of chlorogenic acid-containing diets [17] .
Table 1 elucidated that gallic acid has significant inhibitory effect on all tumor cell proliferation. Gallic acid as a natural antioxidant had significant inhibitory effects on cell proliferation, induced apoptosis in a series of cancer cell lines, and showed selective cytotoxicity against tumor cells with higher sensitivity than normal cells [18] .
While complex gallic-WPI and gallic-casein were appeared negative effect on (HCT116), but positive effect on (HePG2) and (MCF7) The interaction gallic acid with milk proteins has lost effect on all cells, Table 1; these interaction appeared in Figure 1(e) showed that amid Ι and Π for WPI-gallic acid complex appeared at 1646 and 1544 cm−1 respectively and NH2 group disappeared. In Figure 1(f), amid Ι and Π for a complex of casein-gallic acid appeared at 1647 - 1536 cm−1 respectively, NH2 group disappeared, this indicated that interaction between casein and gallic acid was strong. The present findings indicate that these peptidases are strongly inhibited by low concentrations of gallic acid, which is a common constituent of edible foods Thus; the intake of such compounds as dietary constituents may interfere with the absorption of amino acids from intestine [19] . The present data support the contention that gallic acid, a constituent of dietary polyphenols may interfere in the digestion and absorption of proteins in rat intestine.
Table 1 showed that vanillin had significant inhibitory effects on cell proliferation MCF7 and HePG. Vanillin, a food flavoring agent, has been reported to show anti-cancer activity and to inhibit chemical carcinogenesis; vanillin has anti-cancer potential by decreasing invasiveness of cancer cells. Since vanillin is generally regarded as safe, it may be of value in the development of anti-cancer drugs for cancer treatment [20] .
The complex vanillin-casein has significant effect on HePG2, and positive effect MCF7 and HCT116 the same effect for vanillin-WPI on all tumor cells; Table 1. Also showed the effect vanillin on tumor cells was higher sensitivity than complex. These interactions were appeared in Figure 1(g). Amid Ι and Π resulting from the interaction between WPI and vanillin appeared at 1651 - 1546 cm−1 respectively and NH2 group appeared near control (WPI), this indicated that the interaction between WPI and Vanillin was weak, Figure 1(h) showed interaction between casein and vanillin, amid Ι and ester group for the complex appeared at 1646 - 1739 cm−1 respectively, amid Π and NH2 group disappeared. The hydrogen bonding/ionic interaction or hydrophobic interaction was envisaged in the interaction of chloroginic acid with proteins [21] .
3.3. Interactions with Di-Phenolic Compound
Rosmarinic acid is an antioxidant phenolic compound, which is found in many dietary spices such as mint, sweet basil, oregano, rosemary, sage, and thyme [22] . So rosmarinic acids was appeared positive effect on all tumor cells and significant effect of HePG2.
The complex rosmarinic acid-casein has negative effect on HCT116, and positive effect on MCF7 and HePG2 while rosmarinic acid-WPI without effect on HCT116 and positive effect on MCF7 and HePG2. The interaction rosmarinic acid has lost effect on all cells, Table 1. Figure 1(i) showed the function group for WPI-rosmarinic acid complex amid Ι and Π appeared 1648 - 1542 cm−1 respectively and NH2 group decreased in complex. Amid Ι and Π of the casein-rosemarinic acid complex appeared at 1650 and 1524 cm−1 respectively (Figure 1(j)), while NH2 group disappeared in complex. The changes in tryptophan microenvironment polarity are probably related to chemical structure of each rosmarinic acid, namely to the number and position of hydroxyl groups. Hydrophobicity around tryptophan residues rose with increasing number of hydroxyl groups in the molecule of rosmarinic acid. However, the position of hydroxyl groups on the benzene ring seemed to be also important, [23] .
Catechins from green tea belong to the family of flavonoids that are powerful antioxidants and free iron scavengers. Many botanical flavonoids possess strong antioxidant activities in the cardiovascular system [24] . Effects of catechins on cancer chemoprevention have been attributed to its antioxidant activities [25] [26] .
Table 1 showed that catechins as well as their inhibition of the proliferation of human tumor cell lines, this effect was significant with HePG2, the results agree with Gu [27] , them show that catechin is contributes to beneficial therapeutic effects, including anti-oxidant, antiinflammatory, anti-cancer, and immunomodulatory effects; catechin directly targets both tumor cells and tumor vasculature, thereby inhibiting tumor growth, proliferation, migration, and angiogenesis of breast cancer.
Where catechin content prompted the evaluation of their in vitro inhibitory effects on cyclooxygenase enzymes and on the proliferation of human cancer cell lines; the cyclooxygenase inhibitory activities of anthocyanidins and catechins as well as their inhibition of the proliferation of human tumor cell lines suggest that these compounds can be further investigated for their health benefits. The use of these bioflavonoids as potential phytoceuticals could be significant in the prevention of fatal diseases such as cancer and crippling inflammatory conditions such as arthritis and gout [28] .
The complex catechin-casein has effect on HCT116 and HePG2, but negative effect on MCF7, while catechin-WPI has effect on MCF7and HCT116 but significant effect on HePG2, interaction between catechin and milk protein lost effect on all cells was lower effect that catechin as free phenolic compound. Table 1; Figure 1(k) showed that amid Ι and Π for WPI-catechin complex was appeared at 1644 and 1543 cm−1 respectively and NH2 group decreased, this means that there was interaction between catechin and WPI. Moreover, amid Ι and Π for casein-catechin complex appeared at 1648 - 1527 cm−1 respectively, ester group was formed at 1739 cm−1 NH2 group disappeared, this means that the interaction between casein and catechin was very strong (Figure 1(l)).
Quercetin is one of the most potent antioxidants, anti-inflammatory, antiproliferative, and has effect on all tumor cells but significant effect on (HePG2) Table 1, quercetin acts as an anticancer agent through modulation of cell cycle, protein, oncogenes, and antioncogenes [29] . Quercetin is a flavonoid present in many vegetables, fruits and beverages.
The complex quercetin-casein has negative effect on HePG2 and HCT116, but positive effect on MCF7, while quercetin-WPI has effect on MCF7 and without effect on HCT116 but has significant effect on HePG2. Interaction between quercetin and milk proteins was the lowest effect from quercetin as control, Table 1. On the other hand amid Ι and Π for WPI-qurecetin complex (Figure 1(m)) appeared at 1648 and 1544 cm−1 respectively and NH2 group was greatly decreased, consequently the interaction was strong. In Figure 1(n) functional groups for complex of casein-qurecetin, amid Ι and Π at 1653 - 1545 cm−1 respectively, also ester group appeared at 1741 cm−1 and NH2 group decreased, this means that interaction between qurecetin and casein was strong. The interaction between molecules including hydrogen bonding, ionic and van der Waals interactions; Protein-qurecetin interactions play an important role in a variety of biological processes [30] .
3.4. Interaction with Poly-Phenolic Compound
Table 1 elucidated that tannic acid and fractions tannins as antiproliferative has positive effect of all tumor cells, but this effect was significant on HePG2. Tannins are a large class of polyphenolics in dietary plants and medicinal herbs. Oligomeric proanthocyanidins, which are widely distributed in grape seed and skin and pine bark, are considered to be the most potent antioxidants and frequently used in health care and cancer treatment. It is also known that many plants containing tannins are effective against cancer and tumors [31] . Tannins are natural, water-soluble, polyphenolic compounds with molecular weight ranging from 500 to 4000, usually classified into 2 classes: hydrolysable tannins (gallo- and ellagi-tannins) and condensed tannins (proanthocyanidins) [32] .
Hydrolysable tannins and condensed tannins are powerful antioxidant agents because they havemany hydroxyl groups, especially many ortho-dihydroxyl or galloyl groups. Bigger tannin molecules possess more galloy and ortho-dihydroxyl groups, and their activities are stronger [33] . In addition, these tannins also exhibit strong antibacterial, antiulcer, anti-inflammatory, antileishmanial, antimutagenic, enzyme regulating, signal transduction pathways blocking, and apoptotic activities; thus, they have attracted wide attention for cancer treatment [34] - [37] .
The Table 1 showed that complex tannic acid-casein and tannic acid-WPI were positive effect on MCF7 and significant effect on HePG2; but this complex have negative effect on HCT116. The complex tannins (walnut and green tea)-casein and WPI were positive effect of all tumor cells, but tannins (green tea)-WPI was significant effect on HePG2. On the other hand complex tannins (lentil)-casein and WPI have effect on MCF7 and HCT116 but negative effect on HePG2. However interaction between tannins and milk protein lost effect on cell line and this may be due to the strong interaction between them and it’s appeared in Figures 1(o)-(q) illustrated interaction between WPI and plyphenolics (tannins), amid Ι for WPI-tannic acid complex appeared at 1631 cm−1, ester group for complex appeared at 1745 cm−1 while NH2 group was disappeared, this means that the interactions between WPI and tannic acid was strong as comparably with the tannins from green tea and walnut in Figure 1(p) and Figure 1(q) respectively. On the other hand the interaction between WPI and tannins in green tea was stronger than tannins in walnut. Figures 1(r)-(t) illustrated the interaction between casein and polyphenolics (tannins). Amid Ι for casein-tanninc acid complex appeared at 1641 cm−1, also ester group appeared at 1739 cm−1 while amid Π disappeared, this indicated that the interaction between casein and tannic acid was very strong as comparably with the tannins from green tea and walnut, hence, ester group did not form. As shown in Figure 1(s) and Figure 1(t) amid Ι appeared at 1646 - 1627 cm−1 respectively, while amid Π disappeared for all tannins. Tannins, in general have been reported to bind to a variety of proteins by interacting with free NH2 or SH groups [19] .
The amide I, II, and III are the most noticeable, easily measured, and are sensitive to conformational of backbone that links the amino acids. Amide I band represent stretching vibration of the C=O bond while amide II band provides primarily to bending vibrations of the N-H bond. Amide I band share with in-plane NH bending and C-N stretching, so the frequency of this vibration depends on the hydrogen bonding between the C=O and NH which varies for the different secondary structure of polypeptides. Since amide III band is relatively weak and is affected by other vibration, most studies have focused on amide I and II band [38] [39] .
The positions of amide bands I and II in phenolics transmission with milk protein surface show a remarkable shift from 1636 cm−1 to 1649 cm−1 and from 1536 to 1547 cm−1 respectively. The significant peak position shifts observed in the amide I and amide II bands may be attributed to hydrogen bonding between all phenolics and milk protein, suggesting that the hydrogen bonding may occur between the phenolic carboxyl groups in phenolic compounds and the functional groups (i.e. amide groups) of the milk protein [7] . The positions of ester in phenolics (vanillin, tannic acid, catechin, qurecetin and choloroginic acid) transmission with milk protein surface show a remarkable shift from 1739 cm−1 to 1741 cm−1. Its form hydrogen bonding may occur between the phenolic hydroxyl groups in phenolic compounds and the functional groups (i.e. carboxyl groups) of the milk protein.
It can be distinguished from nitro and cyano by their IR spectra. Amides exhibit a moderately intense V band near 1650 cm−1.
Amide linkages constitute a defining molecular feature of proteins, the secondary structure of which is due in part to hydrogen bonding abilities of amides.
Because of the greater electronegativity of oxygen, the carbonyl (C=O) is a stronger dipole than the N-C dipole. The presence of a C=O dipole and, to a lesser extent a N-C dipole, allows amides to act as H-bond acceptors. In primary and secondary amides, the presence of N-H dipoles allows amides to function as H-bond donors as well. Thus amides can participate in hydrogen bonding with water and other protic solvents; the oxygen atom can accept hydrogen bonds from water and the N-H hydrogen atoms can donate H-bonds. As a result of interactions such as these, the water solubility of amides is greater than that of corresponding hydrocarbons.
4. Conclusions
The aim of the present study was to investigate the binding type between phenolics compounds and casein or whey protein isolate, using different approaches. It may be assumed that the initial binding between phenolics and milk proteins yields soluble complexes which upon subsequent cross-linking are transformed into insoluble precipitates.
Cross-linking of milk proteins is an important fact because of potential effects on textural properties of milk products, e.g., yogurt and cheese. The cross-linking effect of vanillin phenolic on milk proteins can be used for manufacturing of milk products (ice cream) with desired textural properties.
Phenolic compunds act as anticancer and anti-proliferative but after interaction with milk proteins, they form complexes which become less effective than these compounds alone.
Fourier transform infrared spectroscopy (FTIR) spectrum of pure WPI displays two characteristic bands of amide Ι (1649 cm−1) which associated with C=O stretching vibration, and amide Π (1547 cm−1) which resultant from N-H bending vibration. But the FTIR spectrum of casein revealed that amid Ι and Π were at 1648 and 1563 cm−1 respectively. The significant peak position shifts absorbed in amide Ι and Π bands attributed to hydrogen bonding between all phenolics and milk proteins.
Therefore, interactions of vanillin phenolic with milk proteins must be considered in this regard. Nevertheless, they may be acceptable food additives because of their antioxidant and anticarcinogenic activities; so they also contribute to the functionality of the products. Displaying the interactions of phenolic compounds with milk proteins is a necessary subject, as they may be potential food additives.
Acknowledgements
The authors express their gratitude to Dr. Wael S. I. Abou-Elmagd Associate Professor of Organic Chemistry, Chemistry Department, Faculty of Science, Ain Shams University, Cairo, Egypt.
NOTES
*Corresponding author.