The main purpose of the present research was to test the ability of nanostructured lipid carriers (NLCs) to efficiently host a hydrophilic polyphenol active with health-promoting activities (caffeic acid (CA)). The caffeic acid-loaded lipid nanocarriers (CA-NLCs) were obtained by high-pressure homogenization technique using a surfactant mixture of Tween 20 and L-α-phosphatidylcholine in association with a lipid mixture of linseed oil, hexadecyl palmitate, and glycerol monostearate. In the first stage, the proportion between surfactant mixture and lipid phase has been varied to obtain appropriate stable nanocarriers. The optimized NLCs have been further loaded with different amounts of caffeic acid and were analyzed in terms of physical stability, size characteristics, and encapsulation efficiency. The antioxidant activity of CA-loaded NLCs and their release behavior have been tested by specific in vitro methods, e.g., ABTS (2,2-azinobis-(3-ethylbenzothiazoline-6-sulfonic acid)) assay and release experiments, by Franz cell diffusion. The ABTS assay highlighted a high antioxidant potential of the caffeic acid in association with linseed oil. The capacity to capture ABTS cationic radicals was superior for the NLC entrapping an initial amount of 1.5% CA, the level of antioxidant capacity being 91.3%. The in vitro release experiments showed a different release behavior, depending on the initial amount of caffeic acid used. NLC loaded with a higher concentration of CA manifests a gradual slow release, e.g., 45% CA after 24 h of in vitro experiments, while the NLC loaded with smaller concentration of CA assured a higher release in time, around 65%.
1. Introduction
During the past decade, lipid nanoparticles have been investigated as platforms for efficient drug encapsulation and sustained release at the specific site of many localized diseases. The solid lipid nanoparticles (SLNs) and nanostructured lipid carriers (NLCs), respectively, are derived from oil/water emulsions, with the remark that the solid lipids or a mixture of solid and liquid lipids, respectively, replace the liquid lipids [1]. Lipid nanoparticles have an average diameter ranging between 50 and 1000 nm, a spherical morphology containing a solid lipid core surrounded by a surfactant shell. One of the most important features of the lipid matrix is its ability to maintain in solid form at both ambient and body temperatures [2]. NLCs are known as improved systems of SLNs, showing a better stability and higher encapsulation efficiency for numerous active compounds. Concomitantly, the NLCs prevent the active substances’ expulsion from the lipid matrix during storage, thus increasing their stability and efficacy during administration [3].
NLCs are considered modified SLNs in which the lipidic phase contains both solid and liquid lipids at ambient temperature, which generate imperfections within the matrix, decreasing its crystallinity and facilitating the accommodation of drug molecules [4, 5]. In this sense, improved drug encapsulation, minimized drug leakage during storage, and controlled drug release kinetics are demonstrated for these delivery systems [1]. Additional advantages of NLCs include high biocompatibility and simple production at large scale [6]. These nanocarriers have been widely developed in the last years aiming at the improvement of the therapeutic index of drugs by means of modifying their pharmacokinetics and biodistribution. Several examples include the encapsulation into SLN and NLC systems of synthetic and/or natural active principles, i.e., anti-UV, anti-inflammatory, antitumor, and antioxidant actives, such as ethylhexyl salicylate, octocrylene, bemotrizinol [7, 8], naringenin [9], tocopherols [10], azelaic acid [11], sodium pemetrexed [6], ivy leaf extract [1], willow bark extract [12], and natural carotenoid extracts from Tagetes patula and Calendula officinalis L. [13]. In the present work, nanostructured lipid carriers (NLCs) based on bioactive linseed oil have been developed in order to test their ability to encapsulate a hydrophilic polyphenol active with potential antioxidant, anti-inflammatory, and antineoplastic activities—caffeic acid (CA)—and to assure an efficient release of this natural active.
Caffeic acid (3,4-dihydroxycinnamic acid, Figure 1) is a hydroxycinnamic acid derivative with potential antioxidant, anti-inflammatory, and antihyperglycemic action and antineoplastic activities [14]. It is a naturally occurring phenolic compound which is produced in many fruits, vegetables, and herbs, including pears, basil, thyme, verbena, tarragon, oregano, wood betony, burning bush, turmeric, dandelion, yarrow, horsetail, rosemary, hawthorn, and coffee [15]. The amount of caffeic acid is strongly dependent on the plant species [16]. Their variety of potential pharmacological effects in in vitro studies and in animal models and the inhibitory effect of caffeic acid on cancer cell proliferation by an oxidative mechanism in the human cell line have recently been established [17]. Caffeic acid is an efficient antioxidant in vitro and also in vivo, e.g., upon administration, it prevents oxidative stress, thereby preventing DNA damage induced by free radicals [18]. Caffeic acid also shows immunomodulatory and anti-inflammatory activity; it reduces the aflatoxin production by more than 90% [19]. Another study showed that oxidative stress that would otherwise trigger or enhance Aspergillus flavus aflatoxin production can be stopped by caffeic acid [20]. Despite the large therapeutic efficiency of caffeic acid, oral administration of high doses of caffeic acid in rats has caused stomach papilloma [21].
Caffeic acid (3,4-dihydroxycinnamic acid).
In this context, the main objective of the present work is to encapsulate different amounts of caffeic acid and to determine the influence of CA concentrations on the antioxidant properties and CA release under controlled conditions. Firstly, the influence of surfactant concentration was investigated on the most important characteristics of NLCs such as mean diameter particle size and zeta potential. The CA was encapsulated into NLCs with the adequate characteristics. For the CA-loaded NLCs, mean diameter particle size, zeta potential, and entrapment efficiency were evaluated. The efficiency of NLCs as pharmaceutical formulations has been characterized by in vitro analysis of the antioxidant activity and CA in vitro release from NLCs.
The research presented in this study is aimed at providing new insights about the association of two categories of natural active principles—hydrophilic and lipophilic—in a lipid delivery system. Although there are several studies in which caffeic acid has been loaded into solid lipid nanoparticles (SLNs) [22, 23], to our knowledge, its capture in lipid nanocarriers has not been achieved so far. As such, the novelty achieved by performing this work refers to the design of CA-loaded nanocarriers containing linseed oil to obtain a synergic effect between linseed oil and caffeic acid and the enhancement of antioxidant activity of both natural actives (caffeic acid and linseed oil).
2. Materials and Methods2.1. Materials
Polyoxyethylene (20) sorbitan monolaurate (Tween 20) and caffeic acid (CA) were purchased from Merck, while Synperonic PE/F68 (poloxamer 188) and L-α-phosphatidylcholine (~99%, from egg yolk, lyophilized powder) were purchased from Sigma Aldrich Chemie GmbH (Munich, Germany). The solid lipids, n-hexadecyl palmitate (CP) and glycerol monostearate (GMS), were obtained from Acros Organics (New Jersey, USA) and Cognis GmbH (Monheim, Germany), respectively. 2,2-Azinobis-(3-ethylbenzothiazoline-6-sulfonic acid) (ABTS) was obtained from Sigma-Aldrich (Munich, Germany). The linseed oil (LO) was purchased from Hofigal S.A., Bucharest, Romania. The LO composition, evaluated by gas chromatography (Thermo-GC, DSQ P 5000 mass spectrometer, Macrogol 2000 column with Φ=0.25mm and l=30m; helium carrier gas, injection temperature of 25°C, flow rate of 1 mL/min), is 50.59% α-linolenic acid (C18:3, ω-3), 24.33% oleic acid (C18:1, ω-9), 14.34% linoleic acid (C18:2, ω-6), 5.19% palmitic acid, 4.34% stearic acid, 0.8% cis-vaccenic acid, and 0.11% γ-linolenic acid (C18:3, ω-6).
2.2. Synthesis and Characterization of NLCs2.2.1. Preparation of Nanostructured Lipid Carriers
Lipid nanocarriers were prepared using melt emulsification method coupled with high-shear homogenization and high-pressure homogenization [24]. For preparation of NLCs, both the lipid phase (a mixture of CP, GMS, and LO) and the aqueous phase (different concentrations of surfactant mixture, namely, 2%, 2.5%, 3%, and 3.5%) were heated under stirring conditions, at 78°C. The active substance was added into the aqueous phase, in which then was also slowly added the lipid phase under stirring, at 78°C. The obtained preemulsion was exposed to an external mechanical energy by high-shear homogenization with a lab rotor-stator homogenizer by applying 15000 rpm for 1 min and then by high-pressure homogenization by applying 500 bar for 196 s. Furthermore, the formed NLC dispersions were subjected to lyophilization in order to remove the water in excess. Table 1 shows different compositions of the synthesized NLCs.
Composition of nanostructured lipid carriers (NLCs).
NLC formulation∗
Surfactant (% w/w)
Caffeic acid (% w/w)
NLC-LO1
2.0
—
NLC-LO2
2.5
—
NLC-LO3
3.0
—
NLC-LO4
3.5
—
NLC-LO-CA1
2.5
0.5
NLC-LO-CA2
2.5
1.0
NLC-LO-CA3
2.5
1.5
∗All NLCs were prepared with 10% (w/w) lipid mixtures, in a ratio of CP/GMS/LO=1:1:1 and a ratio of Tween 20 : poloxamer : L-α-phosphatidylcholine = 70 : 15 : 15.
2.2.2. Particle Size Analysis
The Dynamic Light Scattering (DLS) technique was used for measuring the mean diameter size (Zave) and the polydispersity index (PdI), at a scattering angle of 90° and 25°C, with a Zetasizer Nano ZS, Malvern Instruments, Malvern, United Kingdom. The aqueous NLC dispersions have been adequately diluted in deionized water to fulfill the sensitivity range of the instrument in terms of an accurate achievement of the light scattering intensity (dilution of NLC dispersion: deionizedwater=0.02:1). The intensity distribution was used to evaluate the particle size data, with Zave and PdI being expressed as an average of three DLS measurements. DLS measurements (Zave and PdI determination) were performed on the day of preparation of free and caffeic acid-loaded NLC.
2.2.3. Zeta Potential Analysis
The Helmholtz-Smoluchowski equation [25, 26] was used to calculate the zeta potential (ZP) after determining the electrophoretic mobility of the NLC dispersion. Prior to analysis, each NLC dispersion was diluted with ultrapurified water (in a ratio of NLC aqueous dispersion : ultrapurified water = 1 : 0.01, v/v) and was adjusted by adding a minimum volume of sodium chloride 0.9% solution (e.g., to 20 mL of NLC aqueous dispersion was added 65 μL NaCl solution, 0.9%) in order to reach a conductivity of 50 μS/cm (a value required in the electrophoretic light scattering technique). The zeta potential measurements were performed on Zetasizer Nano ZS; zeta potential values were determined on the day of NLC preparation. The ZP was expressed as an average of three ZP measurements.
2.2.4. Entrapment Efficiency of Caffeic Acid into NLC Systems
The entrapment efficiency of caffeic acid into NLCs was determined by UV-VIS spectroscopy, an amount of 0.05 g of lyophilized NLC-LO-CA being dispersed into 1.0 mL ethanol, mixed, and centrifuged at 15000 rpm, for 15 min. Then, the unloaded CA from the obtained supernatant was analyzed by a spectrophotometric system Jasco V-670, at 325 nm. Before analysis, 50 μL of supernatant was dispersed into 10 mL ethanol. The blank sample consisted of ethanol. The following equation was used for calculating the percent of EE:
(1)%EE=Wa−WsWa×100,where Wa is the weight of total CA used for the preparation of NLC-LO-CA and Ws is the analyzed weight of CA in the supernatant.
Equation (2) was used to calculate the percentage of loading capacity (%LC):
(2)%LC=Wa−WsWa−Ws+WL×100,where Wa is the weight of CA added in the NLC, Ws is the analyzed weight of CA in the supernatant, and WL is the weight of lipid added in the NLC.
2.2.5. In Vitro Antioxidant Activity Measurements
The in vitro determination of antioxidant activity was conducted using a UV-VIS Spectrophotometer Type V670 (Jasco, Japan), according to ABTS assay [27], at 734 nm. The blank sample consisted of normalized ABTS solution and ethanol. Each analyzed sample was prepared with ABTS solution and ethanol.
Firstly, an aqueous 7 mM solution of ABTS was prepared. The cationic radical ABTS⋅+ was generated after 16 hours of reaction between 7 mM ABTS solution and 2.45 mM potassium persulfate solution, in the dark conditions, at 25°C. The ABTS⋅+ solution was normalized with ethanol to an absorbance of 0.700 (±0.02) at 734 nm. Each sample was prepared by adding 3.0 mL of normalized ABTS⋅+ solution to 1 mL NLC solution (prepared with 0.05 g lyophilized nanocarriers into 10 mL ethanol) and 2.0 mL ethanol into a 5 mL flask.
The absorbance of samples was determined after 4 min of reaction of initial mixture, with ethanol being used as reference. Each absorbance of sample was determined in duplicate, the average of absorbance values being used for calculating the percentage inhibition of the sample on ABTS⋅+ according to
(3)%InhibitionABTS+⋅=A0−AsA0×100,where A0 is the absorbance of the blank and As is the absorbance after the addition of the antioxidant.
The antioxidant capacity of NLC systems was also highlighted by TEAC (Trolox Equivalent Antioxidant Capacity) method, with the Trolox solution concentrations ranging between 2 and 60 μM (R2=0.999).
2.2.6. In Vitro Release of Caffeic Acid from NLC
The release of caffeic acid from loaded lipid nanocarriers in dispersion was evaluated using Franz diffusion [28]. The Franz system has two chambers—a donor chamber and a receptor chamber. Between the chambers, a Tuffryn membrane filter was placed.
The receptor chamber contains a release medium of ethanol with a volume of 6 mL. In the donor chamber, an amount of 150 μL of each formulation NLC-LO-CA was placed onto the Tuffryn membrane which was initially hydrated in ethanol for 1 h. The receptor phase consisted of ethanol and phosphate buffer, at a ratio of 50 : 50 (v/v), maintained at 37°C. At 1, 2, 3, 4, 5, 6, 7, 8, and 24 hours, aliquots of 500 μL of sample were collected from the receptor chamber and discharged. The sample was then diluted with ethanol. During the study, the volume of release medium was maintained constant. Finally, the collected samples were measured using the UV-VIS Spectrophotometer Jasco V670. All the measurements were performed in duplicate at 325 nm.
3. Results and Discussion3.1. Optimization of NLC and Physical Stability
Lipid nanocarriers were firstly characterized in terms of mean diameter, polydispersity index, and zeta potential (ξ) by DLS technique. To identify the optimized surfactant composition, the NLCs with different concentrations (2%, 2.5%, 3%, and 3.5%) of surfactants have been synthesized (Table 1). The variation of Zave and PdI of NLCs is shown in Figure 2.
Mean diameter (columns) and PdI (circles) of NLCs prepared with variable content of surfactants.
By tracking the behavior of the four types of NLCs, it was shown that all the synthesized formulations have an appropriate distribution of particle size, e.g., between 110.9 and 131.4 nm. These results could be correlated with the efficiency of the surfactant mixture but also with the presence of the linseed oil which contributes to the viscosity decrease of the lipid mixture, which reduces the surface tension to form smaller and smoother surface particles [29].
Different values of Zave and PdI are influenced by the different molecular weights of surfactants [30]. The best experimental data were obtained for NLCs with a surfactant concentration of 2.5%: Zave=110.9±2.3nm and PdI=0.156±0.004. According to literature data, it is known that the NLCs with a PdI lower than 0.25 show a minimum tendency to aggregation [31].
It was observed that the extreme concentrations selected for the surfactant mixture, e.g., 2% and 3.5%, lead to higher values of Zave. This result can be attributed on the basis of two considerations: (1) a high amount of phosphatidylcholine and poloxamer favors the formation of liposomes, which would lead to higher mean values of Zave; (2) too small amounts of surfactants do not ensure full coverage of the lipid core.
NLCs prepared with the highest amount of surfactant mixture exhibit higher values of Zave (Zave=131.4±1.1nm) and PdI (PdI=0.222±0.005), while by using lower surfactant concentrations (NLC-LO2 and NLC-LO3), the average diameter has been drastically decreased (Figure 2). According to the literature data, compared with a single surfactant, the surfactant mixture could decrease the interfacial tension [32].
3.2. Physical Stability of NLC Dispersions
The zeta potential (ZP) (ξ) is one of the main characteristics that defines the behavior of nanoparticles in aqueous solution, which highlights the physical stability of NLCs. The zeta potential is the electrostatic potential at the shear plane and reflects the electric charge on the particle surface, being a measure of surface charge. It can influence particle stability as well as cellular uptake and intracellular trafficking [33]. The ZP data of the synthesized NLCs are shown in Figure 3. All the developed NLCs are stable, with the zeta potential distribution being between −52.8 mV and −47.6 mV. The negative charges of NLCs are due to surfactant mixture, with the best ZP result being obtained with 2.5% surfactant mixture, ξ=−52.8mV±0.56 (Figure 3), which reveals a high stability of NLC and a low potential of aggregation of solid lipid nanocarriers suspended in aqueous media.
Evaluation of NLC stability by zeta potential.
3.3. Size Characteristics and Physical Stability of CA-NLCs
The NLC-LO2, having a reduced mean diameter and appropriate physical stability, was used for encapsulating the natural antioxidant. The DLS results showed that CA-NLCs present a unimodal profile of size distribution, with a Zave value of 145.5±0.8nm for NLC-LO-CA1, 119.7±0.9nm for NLC-LO-CA2, and 195.1±5.3nm for NLC-LO-CA3 (Figure 4(a)). One example of size distribution is included in Figure 4(b).
(a) Evaluation of loaded NLC stability by mean diameter and PdI. (b) Exemplification of particle size distribution for NLC-LO-CA2.
After CA encapsulation in the NLC, a significant increase of the mean diameter compared to that of the free NLC is observed (ZaveNLC‐LO=110.9±2.3nm). This increase mainly denotes trapping of caffeic acid in the coating created by the surfactant mixture, most probably by hydrogen bonds between the OH groups of caffeic acid, the OH groups of Tween 20, and the polar groups of phosphatidylcholines. If there was a capture of caffeic acid in the voids/imperfections in the lipid core, it would have resulted in an insignificant change in the average diameter. This result was not observed, but on the contrary, a Zave increase was detected which confirms a preferential distribution of caffeic acid in the surfactant layer. These results are predictable having in view the greater affinity and solubility of caffeic acid in surfactant coating than in solid lipids.
A drastic increase of Zave was observed for NLCs loaded with a high amount of CA, e.g., 195.1±5.3nm for NLC loaded with 1.5% CA versus 119.7±0.9nm for NLC loaded with 1% CA. This could be attributed to the hydrophilic character of CA; the surfactant coating can capture a limited concentration of CA, with the remainder being trapped outside the nanocarrier system, thus leading to the appearance of larger mean diameters of lipid nanocarriers.
The results obtained after determination of electrokinetic potential showed that the NLC formulations loaded with CA are negatively charged (Figure 5). As compared to the free NLC, there is a significant perturbation of electric surface after retention of caffeic acid. The addition of caffeic acid resulted in an increase in zeta potential, e.g., from -52.8 mV in free NLC to -48.2 mV and -34.9 mV in NLC-LO-CA1 and NLC-LO-CA2 (loaded with 0.5% and 1% CA, respectively). The presence of anionic active ingredient (CA) has led to a notable modification in zeta potential values because of surface charge rearrangements. A potential explanation may be related to masking of negative charges from phosphate groups (from phosphatidylcholine), due to the caffeic acid trapped by weak bonds in the surfactant coating or attached to the surfactant layer. These aspects justify a certain compensation of surface charges or a covering of negative charges from phosphatidylcholine.
(a) Zeta potential values of empty and CA-loaded NLCs. (b) Exemplification of zeta potential distribution for NLC-LO-CA2.
The colloidal systems are considered stable when the zeta potential values of particles are integrated in the -30 mV and -60 mV potential ranges [34]. All the zeta potential values determined for NLC loaded with CA were below the critical value. Moreover, according to the values lower than <40 mV (reported for NLC-LO-CA1 and NLC-LO-CA3), the obtained NLC systems are expected to manifest a long-term physical stability, which involves the existence of desired electrostatic and steric repulsions between the lipid nanocarriers suspended in aqueous dispersion. This last aspect avoids the aggregation of lipid particles dispersed in water over time.
3.4. Entrapment Efficiency of Caffeic Acid into NLC Systems
The entrapment efficiency (EE%) of LO-based CA-NLCs is shown in Figure 6. There was no relevant difference between EE values, when variable content of CA was included in the NLC formulations. All synthesized NLC-CA showed high EE values, exceeding 95% CA. These results revealed that CA was efficiently entrapped into the NLC, mainly captured in the layer formed by the mixture of surfactants and cosurfactant, showing a high compatibility with the surfactant mixture.
Entrapment efficiency of CA into lipid nanocarriers based on linseed oil.
3.5. The In Vitro Determination of Antioxidant Activity
Oxidative processes are represented by a lost balance between the oxidative and antioxidative systems of the cells and tissues, with the production of oxidative free radicals and reactive oxygen species (ROS). Excessive ROS generated could attack the cellular proteins, lipids, and nucleic acids leading to cellular disorders including loss of energy metabolism, altered cell signaling and cell cycle control, genetic mutations, altered cellular transport mechanisms and overall decreased biological activity, immune activation, and inflammation [35].
The ABTS method highlights the antioxidant activity of complex biological systems [36] and was used in our study to determine the scavenging activity of developed NLC-LO-CA 1/2/3 on ABTS+∗ radical. The experimental data highlighted the high antioxidant capacity of the CA in association with linseed oil. Figure 7 reveals that ABTS+∗ inhibition depends on CA concentration. The obtained data showed a higher antioxidant capacity for the CA-NLCs compared to native CA. The smaller concentration of the native CA (0.5%) shows a 21.5%±0.15 antioxidant capacity, while the encapsulation of CA into NLC revealed a radical ABTS+∗ inhibition activity of 47.2%±0.5.
Comparative assessment of antioxidant activity of native CA, NLC-LO, and NLC-LO-CA.
The incorporation of higher CA concentration into NLC has led to stronger antioxidant properties, an improved antioxidant activity of 91.3%±0.3 being determined for NLC-LO-CA3. Figure 7 shows an inhibition of 79.2%±0.8 for NLC loaded with 1% CA and an inhibition of 47.2%±0.5 for NLC loaded with 0.5% CA.
The improved results of ABTS+∗ inhibition of NLC-LO-CA compared to CA can be explained by the size effect produced by trapping the CA into NLC. The free radical scavenging activity is a surface reaction since only the surface meets the free radicals [37]. According to several studies, the radical scavenging potential is dependent on various factors such as particle size, morphology, and network defects [38, 39]. An enhancement in free radical scavenging which coincided with a decreasing of nanofiber diameters has been underlined in a study of Kumar et al. This has been associated with the increase in the surface reaction sites with the size reduction [40].
Similar to other nanomaterials, NLCs exhibit unique properties attributed to their high surface to volume ratio. The average diameters of NLC lower than 200 nm offer more reactive sites for capturing the ABTS+∗ cationic radicals, determining an enhancement of antioxidant activity.
In conclusion, the in vitro assays evidenced that NLC-LO-CA has an important role in reducing the cellular oxide species [41]. It is also known that the physical and biological properties of CA-NLCs are influenced by a reduced size of bioactive [22].
3.6. In Vitro Release of Caffeic Acid from NLC
The series of release profiles of CA from different NLCs loaded with 0.5%, 1%, and 1.5% CA showed a different behavior. Despite the similar sustained release pattern encountered for all NLC formulations in the first hours of release experiments, significant delimitation has been noted after 5 h as a function of the initial percent of CA loaded into NLC. Regarding the CA-NLCs, it was not evidenced a burst release, with a minimum CA release being found after the first hour of experiment (with about 8-10% of total CA released); a sustained release with a maximum degree of about 65% CA was followed. It is interesting to note that during the entire release period, the amount of CA released from NLC loaded with 0.5 and 1% CA was almost similar (Figure 8).
Influence of the lipid nanocarrier type on the release of caffeic acid.
The evolution of caffeic acid release could be illustrated as follows: the initial release (during 8 h of experiments) might be related to the release of CA slightly bonded to the surface of NLC. After 8 h, the release trend has been maintained almost constant. NLC-LO-CA3 assures a gradual slow release of CA, e.g., 45.1% CA after 24 h of in vitro experiments, while from the NLC-LO-CA2 and NLC-LO-CA1 the amount of CA released was significantly higher, 64.7% and 65.6%, respectively. The slowest release percent obtained for NLC-LO-CA3 containing a higher amount of CA could be potentially assigned to the size characteristics of developed NLC. According to DLS measurements, an increase of CA percent into nanostructured formulation has led to higher Zave value (e.g., from 119 nm for NLC loaded with 1% to about 195 nm for NLC loaded with 1.5% CA). This higher loading resulted in a delay in the diffusion process of CA in the receptor medium.
To describe the in vitro release study, different kinetic mathematic models were used, and the kinetic parameters, the rate constant (k), the release coefficient (n), and the correlation coefficient (R2), have been determined. Table 2 shows the kinetic parameters of caffeic acid release from CA-NLCs for different mathematical models: zero order, first order, Higuchi, Korsmeyer–Peppas, and Hixson–Crowell [42, 43].
Kinetic data obtained after release of caffeic acid from NLC prepared with linseed oil.
NLC formulations
Zero order
First order
Higuchi
Hixson–Crowell
Peppas–Korsmeyer
R2
k0
R2
k1
R2
k2
R2
k3
R2
k4
n
NLC-LO-CA1
0.9966
8.1046
0.9938
0.1353
0.9928
31.528
0.9897
0.0175
0.9967
2.0321
0.4754
NLC-LO-CA2
0.9946
7.5755
0.9972
0.1247
0.9946
29.528
0.9948
0.0161
0.9972
1.8555
0.4462
NLC-LO-CA3
0.9701
5.0423
0.9812
0.0667
0.9905
19.859
0.9823
0.0083
0.9941
2.1039
0.5973
It is observed that the CA release from NLC is best reflected by the Korsmeyer–Peppas kinetics (R2>0.994 in all cases studied). According to the release coefficient value (n=0.5973, Table 2), NLC-LO-CA3 assures a release of CA following a non-Fickian diffusion model, while the release of CA% from NLC-LO-CA1 and NLC-LO-CA2 unfolds after a Fick diffusion mechanism (n<0.5, Table 2) [44]. The almost constant trend of CA released remained constant over a period of 24 h, with a percentage of release of about 65% CA (from NLC-LO-CA1 and NLC-LO-CA2) and 45% in the case of NLC-LO-CA3. All experimental results demonstrate that LO from NLC influenced the controlled release of CA; this is a desired purpose in order to avoid the irritant effect of CA and to reach an effective plasmatic concentration of CA (after one hour). Indeed, the controlled release of CA, during a period of 24 h, could maintain an effective plasmatic concentration of CA.
4. Conclusions
The experimental results obtained by this study indicate that lipid nanocarriers prepared by the association of two solid lipids with a bioactive vegetable oil (linseed oil) are appropriate delivery systems for a hydrophilic active compound—caffeic acid. The DLS measurements showed that the CA loaded-NLCs have mean diameters less than 200 nm, with polydispersity index lower than 0.25. Developed lipid nanocarriers that capture caffeic acid are covered by a strong negative charge on the surface (zeta potential values more electronegatively than −35 mV). Despite the hydrophilic feature of caffeic acid, the entrapment efficiency has reached 95%.
CA-NLCs manifested a high antioxidant activity; the capacity to scavenge the ABTS+⁎ cationic radicals was significantly improved as compared to native caffeic acid. The in vitro capacity to capture ABTS cationic radicals was superior for the NLC entrapping an initial amount of 1.5% CA, with the level of antioxidant capacity being 91.3%.
The in vitro release and kinetic modeling of lipid nanocarriers containing caffeic acid were also pursued. CA-NLCs have shown a desired sustained release behavior of caffeic acid during release experiments. After 24 h of in vitro experiments, NLC-LO-CA3 assured a gradual slow release of CA with a percent of 45% CA released, while from NLC-LO-CA2 and NLC-LO-CA1 the amount of CA released was significantly higher, about 65%.
These results showed that the NLCs based on linseed oil and loaded with caffeic acid may be promising delivery systems which could be exploited in several interest area such as antioxidant cosmetic formulations or to produce functional food with improved antioxidant properties.
Data Availability
The data used to support the findings of this study are available from the corresponding author upon request.
Conflicts of Interest
The authors declare that there is no conflict of interest regarding the publication of this paper.
LacatusuI.BadeaN.BadeaG.BrasoveanuL.StanR.OttC.OpreaO.MegheaA.Ivy leaves extract based – lipid nanocarriers and their bioefficacy on antioxidant and antitumor activities2016681772437725510.1039/C6RA12016D2-s2.0-85010049860IstratiD.LacatusuI.BordeiN.BadeaG.OpreaO.StefanL. M.StanR.BadeaN.MegheaA.Phyto-mediated nanostructured carriers based on dual vegetable actives involved in the prevention of cellular damage20166424925910.1016/j.msec.2016.03.0872-s2.0-8496233985227127051NiculaeG.LacatusuI.BadeaN.OpreaO.MegheaA.Optimization of lipid nanoparticles composition for sunscreen encapsulation20137537992TamjidiF.ShahediM.VarshosazJ.NasirpourA.Nanostructured lipid carriers (NLC): a potential delivery system for bioactive food molecules201319294310.1016/j.ifset.2013.03.0022-s2.0-84880056549LiuC. H.WuC. T.Optimization of nanostructured lipid carriers for lutein delivery20103532-314915610.1016/j.colsurfa.2009.11.0062-s2.0-71649087412OttC.LacatusuI.BadeaG.GrafuI. A.IstratiD.BabeanuN.StanR.BadeaN.MegheaA.Exploitation of amaranth oil fractions enriched in squalene for dual delivery of hydrophilic and lipophilic actives20157734235210.1016/j.indcrop.2015.08.0572-s2.0-84942057180LacatusuI.BadeaN.MurariuA.BojinD.MegheaA.Effect of UV sunscreens loaded in solid lipid nanoparticles: a combinated SPF assay and photostability201052324725910.1080/154214010037199282-s2.0-77952971351LacatusuI.ArsenieL. V.BadeaG.PopaO.OpreaO.BadeaN.New cosmetic formulations with broad photoprotective and antioxidative activities designed by amaranth and pumpkin seed oils nanocarriers201812342443310.1016/j.indcrop.2018.06.0832-s2.0-85049857491BadeaG.BadeaN.BrasoveanuL. I.MihailaM.StanR.IstratiD.BalaciT.LacatusuI.Naringenin improves the sunscreen performance of vegetable nanocarriers201741248049210.1039/C6NJ02318E2-s2.0-85010465872NiculaeG.LacatusuI.BorsA.StanR.Photostability enhancement by encapsulation of α-tocopherol into lipid-based nanoparticles loaded with a UV filter201417101028103310.1016/j.crci.2013.12.0072-s2.0-84907552085LacatusuI.BadeaN.BadeaG.MihailaM.OttC.StanR.MegheaA.Advanced bioactive lipid nanocarriers loaded with natural and synthetic anti-inflammatory actives201920011312610.1016/j.ces.2019.01.0442-s2.0-85062152437MitreaE.LacatusuI.BadeaN.OttC.OpreaO.MegheaA.New approach to prepare willow bark extract-lipid based nanosystems with enhanced antioxidant activity20151564080408910.1166/jnn.2015.91622-s2.0-84920681777LacatusuI.BadeaN.NiculaeG.BordeiN.StanR.MegheaA.Lipid nanocarriers based on natural compounds: an evolving role in plant extract delivery2014116121708171710.1002/ejlt.2013004882-s2.0-84919647946KimE. O.MinK. J.KwonT. K.Anti-inflammatory activity of hydroxycinnamic acid derivatives isolated from corn bran in lipopolysaccharide-stimulated Raw 264.7 macrophages20125051309131610.1016/j.fct.2012.02.0112-s2.0-8486279642022366099WuZ.LiZ.XueZ.LuX.WangX.Optimization of extraction technology for determination of caffeic and chlorogenic acid in dandelion2020XI21263710.7904/2068-4738-xi(21)-26MedinaI.UndelandI.LarssonK.StorrøI.RustadT.JacobsenC.KristinováV.GallardoJ. M.Activity of caffeic acid in different fish lipid matrices: a review2012131373074010.1016/j.foodchem.2011.09.0322-s2.0-80755168883PrasadN. R.KarthikeyanA.KarthikeyanS.ReddyB.Inhibitory effect of caffeic acid on cancer cell proliferation by oxidative mechanism in human HT-1080 fibrosarcoma cell line20113491-2111910.1007/s11010-010-0655-72-s2.0-7995228060321116690KiokiasS.ProestosC.OreopoulouV.Effect of natural food antioxidants against LDL and DNA oxidative changes201871010.3390/antiox71001332-s2.0-85055017676EspíndolaK. M.FerreiraR. G.NarvaezL. E.Silva RosarioA. C.da SilvaA. H.SilvaA. G.VieiraA. P.MonteiroM. C.Chemical and pharmacological aspects of caffeic acid and its activity in hepatocarcinoma2019954110.3389/fonc.2019.005412-s2.0-85068963648FountainJ. C.BajajP.NayakS. N.YangL.PandeyM. K.KumarV.JayaleA. S.ChitikineniA.LeeR. D.KemeraitR. C.VarshneyR. K.GuoB.Responses of Aspergillus flavus to oxidative stress are related to fungal development regulator, antioxidant enzyme, and secondary metabolite biosynthetic gene expression20167204810.3389/fmicb.2016.020482-s2.0-85009373471ChandraS. A.NolanM. W.MalarkeyD. E.Chemical carcinogenesis of the gastrointestinal tract in rodents: an overview with emphasis on NTP carcinogenesis bioassays200938118819710.1177/01926233093564522-s2.0-77952306457FathiM.MirlohiM.VarshosazJ.MadaniG.Novel caffeic acid nanocarrier: production, characterization, and release modeling20132013910.1155/2013/4346322-s2.0-84890057479KutluH.GençL.GüneyG.The impact of caffeic acid loaded solid lipid nanoparticles on cancer treatment20139669870310.2174/157341371130999900772-s2.0-84894068394PugliaC.BlasiP.RizzaL.SchoubbenA.BoninaF.RossiC.RicciM.Lipid nanoparticles for prolonged topical delivery: an in vitro and in vivo investigation20083571-229530410.1016/j.ijpharm.2008.01.0452-s2.0-4274908644618343059SzeA.EricksonD.RenL.LiD.Zeta-potential measurement using the Smoluchowski equation and the slope of the current–time relationship in electroosmotic flow2003261240241010.1016/S0021-9797(03)00142-52-s2.0-003773138716256549Barbinta-PatrascuM. E.BadeaN.PirvuC.BacalumM.UngureanuC.NadejdeP. L.IonC.RauI.Multifunctional soft hybrid bio-platforms based on nano-silver and natural compounds20166992293210.1016/j.msec.2016.07.0772-s2.0-8498274044131029305OpitzS. E. W.SmrkeS.GoodmanB. A.YeretzianC.Methodology for the measurement of antioxidant capacity of coffee: a validated platform composed of three complementary antioxidant assays20142625326410.1016/B978-0-12-404738-9.00026-X2-s2.0-84902224444GokceE. H.DelleraE. K. E.SandriG.BonferoniM. C.OzerO.Resveratrol-loaded solid lipid nanoparticles versus nanostructured lipid carriers: evaluation of antioxidant potential for dermal applications201271841185010.2147/IJN.S297102-s2.0-8487036835322605933HuF.-Q.JiangS.-P.DuY.-Z.YuanH.YeY.-Q.ZengS.Preparation and characterization of stearic acid nanostructured lipid carriers by solvent diffusion method in an aqueous system2005453-46717310.1016/j.colsurfb.2005.08.0052-s2.0-26244444984WuG.MajewskiJ.EgeC.KjaerK.WeygandM. J.LeeK. Y. C.Interaction between lipid monolayers and poloxamer 188: an X-ray reflectivity and diffraction study20058953159317310.1529/biophysj.104.0522902-s2.0-2774459728516100276MitriK.ShegokarR.GohlaS.AnselmiC.MüllerR. H.Lipid nanocarriers for dermal delivery of lutein: preparation, characterization, stability and performance20114141-226727510.1016/j.ijpharm.2011.05.0082-s2.0-7995973949121596122PorterM. R.Speciality surfactants1994Boston, MA, USASpringer20320810.1007/978-94-011-1332-8LuG. W.GaoP.2010Oxford, UKEd. Elsevier Inc.LacatusuI.BadeaN.BojinD.IosubS.MegheaA.Novel fluorescence nano-structured materials obtained by entrapment of an ornamental bush extract in hybrid silica glass2009511849110.1007/s10971-009-1925-22-s2.0-66649135571RaniV.DeepG.SinghR. K.PalleK.YadavU. C. S.Oxidative stress and metabolic disorders: pathogenesis and therapeutic strategies201614818319310.1016/j.lfs.2016.02.0022-s2.0-8495901882526851532HassanM. H.EdfawyM.MansourA.HamedA.-A.Antioxidant and antiapoptotic effects of capsaicin against carbon tetrachloride-induced hepatotoxicity in rats20112842843810.1177/07482337114138012-s2.0-84861548350VidhuV. K.PhilipD.Biogenic synthesis of SnO2 nanoparticles: evaluation of antibacterial and antioxidant activities201513437237910.1016/j.saa.2014.06.1312-s2.0-84904286083Barbinta-PatrascuM. E.BadeaN.BacalumM.UngureanuC.Suica-BunghezI. R.IordacheS. M.PirvuC.ZguraI.MaraloiuV. A.3D hybrid structures based on biomimetic membranes and Caryophyllus aromaticus - “green” synthesized nano-silver with improved bioperformances201910112013710.1016/j.msec.2019.03.0692-s2.0-8506345597531029305NavyaP. N.DaimaH. K.Rational engineering of physicochemical properties of nanomaterials for biomedical applications with nanotoxicological perspectives20163111410.1186/s40580-016-0064-z28191411KumarA.BanerjeeS.GargA. B.MittalR.MukhopadhyayR.Size dependent antioxidant activity of polypyrrole nanofibers2011134939910.1063/1.36059032-s2.0-80052434979ShiozawaR.InoueY.MurataI.KanamotoI.Effect of antioxidant activity of caffeic acid with cyclodextrins using ground mixture method2018131243310.1016/j.ajps.2017.08.0062-s2.0-8503234641532104375SiepmannJ.PeppasN. A.Higuchi equation: derivation, applications, use and misuse2011418161210.1016/j.ijpharm.2011.03.0512-s2.0-8005285327621458553PanotopoulosG. P.HaidarZ. S.Mathematical Modeling for Pharmaco-Kinetic and -Dynamic Predictions from Controlled Drug Release NanoSystems: A Comparative Parametric Study20192019510.1155/2019/91538762-s2.0-85060448191915387630723572NagaichU.GulatiN.Nanostructured lipid carriers (NLC) based controlled release topical gel of clobetasol propionate: design and in vivo characterization20166328929810.1007/s13346-016-0291-12-s2.0-8496493328627072979