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Effects of different stabilizers on colloidal properties and encapsulation efficiency of vitamin D3 loaded nano-niosomes
Journal Pre-proof Effects of different stabilizers on colloidal properties and encapsulation efficiency of vitamin D3 loaded nano-niosomes Vahideh Talebi, Babak Ghanbarzadeh, Hamed Hamishehkar, Akram Pezeshki, Alireza Ostadrahimi PII:
S1773-2247(19)30426-5
DOI:
https://doi.org/10.1016/j.jddst.2019.101284
Reference:
JDDST 101284
To appear in:
Journal of Drug Delivery Science and Technology
Received Date: 26 March 2019 Revised Date:
31 August 2019
Accepted Date: 11 September 2019
Please cite this article as: V. Talebi, B. Ghanbarzadeh, H. Hamishehkar, A. Pezeshki, A. Ostadrahimi, Effects of different stabilizers on colloidal properties and encapsulation efficiency of vitamin D3 loaded nano-niosomes, Journal of Drug Delivery Science and Technology (2019), doi: https://doi.org/10.1016/ j.jddst.2019.101284. This is a PDF file of an article that has undergone enhancements after acceptance, such as the addition of a cover page and metadata, and formatting for readability, but it is not yet the definitive version of record. This version will undergo additional copyediting, typesetting and review before it is published in its final form, but we are providing this version to give early visibility of the article. Please note that, during the production process, errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain. © 2019 Published by Elsevier B.V.
2
Effects of different stabilizers on colloidal properties and encapsulation efficiency of vitamin D3 loaded nano-niosomes
3 4 5
Vahideh Talebi1, Babak Ghanbarzadeh*1,2, Hamed Hamishehkar3,
6
Akram Pezeshki1, Alireza Ostadrahimi 4
1
7 8
1-
9 10
Tabriz, P.O. Box 51666-16471, Tabriz, Iran 2-
11 12 13 14 15
Department of Food Science and Technology, Faculty of Agriculture, University of
Department of Food Engineering, Faculty of Engineering, Near East University P. O. Box 99138, Nicosia, Cyprus, Mersin 10, Turkey
3-
Drug Applied Research Center, Tabriz University of Medical Sciences, Tabriz, Iran 4- Nutrition Research Center, Tabriz University of Medical Sciences, Tabriz, Iran
* Corresponding author: [email protected], [email protected] Tel: 00989123039836, Fax: 00984133356005
16 17 18 19 20 21 22 23 24 1
25
Abstract
26
The vitamin D3 loaded nano-niosomes were prepared by thin layer hydration and sonication
27
methods. Influence of stabilizers (vitamin E acetate, polyethylene glycol and, cholesterol) on
28
the different physicochemical properties of resulted niosomes including particle size
29
distribution, zeta potential, encapsulation efficiency (EE%), antioxidant activities, turbidity,
30
sedimentation, and pH were evaluated. The images of scanning electron microscopy (SEM)
31
confirmed the results of the particle size data which were obtained using dynamic light
32
scattering (DLS). Fourier transform infrared spectroscopy (FT-IR) and differential scanning
33
calorimetry (DSC) analysis demonstrated the incorporation of vitamin D3 into niosomes.
34
Incorporation of vitamin E-acetate and cholesterol to the niosome formulation (N2) caused a
35
significant increase (P<0.5) in niosome size. Addition of vitamin E-acetate caused a
36
significant effect on increasing of encapsulation efficiency.The highest efficiency was
37
observed in the samples containing cholesterol and polyethylene glycol. The niosome
38
formulation containing 0.02 mmole vitamin E acetate with the size of 99 nm was selected as
39
the optimal formulation. This formulation had the highest antioxidant capacity (56%), the
40
lowest pH changes and high encapsulation efficiency (92.9%).
41
Keywords: nano-niosome, vitamin E-acetate, vitamin D3, encapsulation, stabilizer
42
2
43
1. Introduction
44
Nutraceuticals are food ingredients that, in addition to having basic nutritional properties,
45
have valuable biological activities such as enhancing the immune system and inhibitory
46
effects against important disorders such as cancer, cardiovascular diseases, diabetes, macular
47
degeneration, and other age-related diseases. Vitamins are among the most important groups
48
of nutraceutical compounds and are naturally present in foods. Low doses of vitamins are
49
essential for growth, maintaining the normal state of cells and body function. By growing
50
tendency of people to low-fat or non-fat foods due to the changing the lifestyle, and also the
51
destruction of nutraceuticals during the processing and food preservation, concerns about
52
diseases caused by essential hydrophobic nutrients deficiencies have been increased.
53
Therefore, the enrichment of some foods and beverages with these essential nutrients can be
54
an effective way to solve this problem.
55
Vitamin D is a lipid-soluble vitamin with two main chemical forms, vitamin (ergocalciferol)
56
D2 and vitamin D3 (cholecalciferol) [1]. Vitamin D3 (cholecalciferol) is synthesized in the
57
human epidermis after light exposure [2]. Recent studies showed a high prevalence of
58
vitamin
59
diabetes [4], metabolic bone diseases, osteoporosis, hypertension and others [5]. Due to poor
60
food sources containing this vitamin, food fortification with vitamin
61
[6].
62
The role of vitamin E as an important factor and its antioxidant and non-antioxidant
63
biological activities in the normal metabolism of all cells and reduction of cardiovascular
64
disease, diabetes, and cancer has been proven. Because of higher chemical stability of
65
vitamin E acetate (the esterified form of α-tocopherol) compared to the non-esterified form
66
(α-tocopherol), this form is often used in foods and beverages [7].
67
Encapsulation of nutraceutical compounds by lipid or polymer-based carriers is an effective
deficiency, especially in women [3] which causes cardiovascular diseases and
3
is the priority deal
68
way to protect their properties and also increase their solubility and bioavailability and
69
decrease their possible off flavor [2]. Niosome, non-ionic surfactants vesicle (NSV) is one of
70
the nanocarriers that is formed from non-ionic surfactants. It is structurally similar to
71
liposomes and consists of an aqueous core enclosed by a bilayer membrane of non-ionic
72
surfactants [8]. In their vesicular structure, the hydrophobic groups are placed in the interior
73
of the membrane while the hydrophilic ones are exposed to the aqueous core. The niosome
74
and vesicular liposome structures do not form spontaneously, and they need some energy
75
input (e.g., hand-shaking, agitation, ultrasound, heating) and this has led to the development
76
of different preparation methods, during the last two decades. Niosomes, as substitutes of
77
liposomes, [9] are chemically more stable and have lower costs than liposomes. In addition, a
78
more wide range of surfactants is available for the formulation of these vesicular carriers.
79
These vesicles can encapsulate a large amount of different functional components (lipophilic,
80
hydrophilic, and amphiphilic) in their small volumes [10]. Span and Tween, non-ionic
81
surfactants, have some interesting properties such as biodegradability, biocompatibility, and
82
low toxicity, so they are used in some foods and pharmaceuticals [11].
83
In recent years, several types of research have worked on the production of nutriceutical
84
loaded noisomes such as capsaicin [11], resveratrol [12], gallic acid, ascorbic acid, curcumin
85
and quercetin [13], resveratrol/curcumin and alpha-tocopherol/curcumin [14], vitamin D3 and
86
ferrous sulfate [15], α-Tocopherol [16]. However, the comparison of effects of different
87
stabilizers on the noisome systems has not extensively studied.
88
The main objective of the present work was to preparing vitamin D3 loaded nano-niosome by
89
thin layer hydration and sonication method and then study of effects of some food grade
90
stabilizers such as vitamin E acetate, polyethylene glycol and cholesterol on physicochemical
91
properties of developed nano-niosomes.
92 4
93
Materials and Method
94
1.1.
95
Vitamin D was provided by DSM. (Swiss). Vitamin E acetate was obtained from Zahravi.
96
(Iran) and Cholesterol was purchased from Sigma (Germany). Polyethylene glycol 400 was
97
purchased from Sacharlau (Spain). Other chemicals including Span 60, Tween 80, 2,2-
98
diphenyl-1-picrylhydrazyl (DPPH) powder and 2-propanol were analytical grade and were
99
provided from Merck (Germany).
Materials
100
1.2.
Preparation of nano-niosomes
101
Nano-niosomes were prepared according to thin layer hydration- sonication method described
102
by Pando, et al. [17] with some modification. Span 60, a non-ionic surfactant was used as the
103
main component in the formulations. Span 60 and Tween 80 were dissolved in isopropyl
104
alcohol (5ml) at 50 ºC for 20 min. Vitamin
105
isopropyl alcohol (5 ml). Two solutions were mixed and thin layer formation was performed
106
in the rotary evaporator LABOROTA 4002- digital model (Heidolph, Germany) at 60 ºC, 90
107
rpm, 100 mmHg for 60 min. Hydration was done by 10 ml distilled water in rotary at 65 ºC
108
for 30 min. Sonication was performed for 6 min by 1 min intervals at 120 Hz (UP200H
109
model, Hielscher, Germany). Finally, the prepared nano niosomes were filtered through 0.2
110
µm Whatman filter.
111
Due to the increased encapsulation efficiency in the range of HLB = 8.6 [18], two types of
112
surfactants were used to obtain the desired HLB. The percentages of the used amounts of
113
surfactants were obtained from Equation 1 [19]: HLB = =
114
(
and Vitamin E- acetate were dissolved in
)+( +
)
× 100
(1)
=
The formulation used for the preparation of nano-niosomes is shown in 5
115
Table 1.
116 117
1.3.
Mean size, polydispersity index, and zeta potential of niosomes
118
The average diameter, polydispersity index (PDI) and zeta potential of samples was measured
119
using a dynamic laser scattering (DLS) device, the Nanotrac Wave Microtrac (Germany)
120
model. For this purpose, each sample was diluted 20 times with distilled water. All specimens
121
were measured in three replicates. This system determined the particle size by measuring
122
their propulsion and dynamic light diffraction (DLS), and then the size is determined by
123
applying proven theories.
124
The average particle diameter was reported in terms of the volumetric average. The mean
125
particle diameter or DeBroukere mean was calculated from Equation 2 [20]:
!" !
∑ 4,3 = ∑
(2)
126
1.4.
127
Morphology of nano-niosomes was investigated by scanning electron microscopy (SEM).
128
The sample was diluted 20 times with water and observed under KYKY-EM3200 at an
129
accelerating voltage of 26 kV [21].
130
Morphological analysis (scanning electron microscopy)
1.5. Differential scanning calorimetry (DSC)
131
Differential scanning calorimetry of blank sample and nanoniosome containing vitamin D3
132
(N1) and vitamin D3 was performed on a DSC device (PerkinElmer, Jade DSC model, US
133
manufacturing). The device was calibrated with indium, and an empty aluminum container
134
was used as a reference. Samples with a mass of approximately 4 milligrams were scanned at
135
20 °C/min at a temperature range of 30 to 300 °C, and the melting point of the compounds
136
was determined [22].
137
1.6.
Fourier transform infrared spectroscopy (FTIR) 6
138
Infrared spectroscopy was performed using an FTIR device TENSOR 27, in the range of 400-
139
4000 cm-1. The samples (Span 60, Tween 80, Vitamin D3, Vitamin E-acetate, blank nano-
140
niosome and nano-niosome containing vitamin D3) were separately mixed with pure
141
potassium bromide (KBr) in a ratio of 1 to 100 and this mixture was used in
142
spectrophotometry [23].
143
1.7.
144
The antioxidant capacity (AOC) was determined using the 2,2-diphenyl-1-picrylhydrazyl
145
(DPPH) method. DPPH is a free radical widely used to determine the ability of antioxidant
146
molecules to react as free radical scavengers [11]. First, nano-niosomes were broken down
147
using chloroform. For this purpose, 2 ml of nano-niosome solution was mixed with 2 ml of
148
chloroform and stirred for 20 minutes. Then the white upper liquid (water) was discarded. A
149
chloroform solution containing DPPH (0.01mM) was prepared and mixed with samples in the
150
ratio of 1:1, then the adsorption changes were read after 2 hours of incubation in darkness at
151
517 nm with UV-vis Ultrospec 2000 (UK) spectrophotometer. The antioxidant capacity with
152
the DPPH inhibitory content was determined according to Equation 3 [24]:
Antioxidant capacity
Inhibition% =
+, − +. × 100 +,
(3)
153
where A0 is absorbance of control sample at 517 nm and A1 is sample absorbance at 517 nm.
154
1.8.
155
To obtain a qualitative amount of oxidation and hydrolysis of niosomes over a month, the pH
156
of the nano-niosome solutions was measured. The pH was measured by direct injection of a
157
pH meter (Metrohm, Switzerland) into a new mass solution, and setting the sample
158
temperature.
159
1.9.
160
To obtain a qualitative dimension of variation in the size and release rate of nano-niosomes
pH
Turbidity
7
161
during a month, the turbidity was measured. First, 1 ml of the sample was diluted with 2 ml
162
of distilled water and stored at room temperature for 30 minutes. Then, the turbidity of the
163
sample was measured in a spectrophotometer of the Ultrospec 2000 produced by the UK in
164
quartz tubes at a wavelength of 600 nm [25].
165 166
1.10.
Sedimentation
167
In order to determine the stability of nano-niosome solutions, their sediment was measured. 5
168
ml of each formulation was stored for 60 days and 30 days at 2 °C and room temperature and
169
their sedimentation height was measured. Sediment volume was obtained using Equation 4
170
[26]: S% =
V1 2V × 100 ,
(4)
171
where Vu is sediment volume at a specified time and V0 is Total volum of nano-niosome
172
solution.
173
1.11.
174
To determine encapsulation efficiency (EE%), 3 ml of nano-niosome solution was mixed
175
with 3 ml of isopropyl 50% solution (to dissolve only soluble vitamins). Amicon filter was
176
used by centrifugation at 4000 rpm for 2 minutes [27] to isolate free and encapsulated
177
vitamins. From each of the upper and lower sections of the filter, 1 ml samples were
178
removed, and 500 µl of chloroform was added to each. The test tube containing nano-
179
niosome was shaken for 20 minutes to degrade the nano-niosome and free the vitamin.
180
Sample containing free vitamin was also shaken for several minutes. The chloroform phase of
181
the solutions was separated, and the samples were dried under nitrogen gas. EE was
182
calculated using Equation 5:
Loading parameters
8
Encapsulation efficiency% =
Capsulated vitamin (mg) × 100 Free + encapsulated vitamin (mg)
(5)
183
The loading capacity (LC) calculated as the ratio of the active ingredient to the whole lipid
184
(stabilizing agent + surfactant + vitamin E-acetate).
185
1.11.1. High-Performance liquid chromatography (HPLC)
186
HPLC (Waters 1525 Binary, USA) was used to determine the free and encapsulated vitamin
187
in nano-niosomes. The optimal condition of the column and the HPLC device to determine
188
the encapsulation efficiency was as follows: C18 silica gel column (5 µm, 250mm × 4.6mm),
189
room temperature, flow rate 1 ml/min, wavelength 270 nm, injection valium 20 µl, and
190
mobile phase chloroform + 0.5% amyl alcohol (95 ml), ethyl acetate (5 ml).
191
In order to plot the calibration curve, 100 mg of a standard solution of 1 million units was
192
transferred to a 50-caliber balloon and chloroform was added to reach the specified valium
193
(2000 IU / ml); 20 µl of the standard solution was injected to the device, and the sub-curved
194
surface was calculated.
195
The concentration of vitamin D3 was determined using Equation 6: CD =
AD × CF AF
(6)
196
where At is the area below the vitamin D3 curve in the sample solution, As is the area under
197
the curve of vitamin D3 in the standard solution, Cs is standard concentration and Ct is sample
198
concentration
199
1.12.
200
Physical and chemical tests were performed on a completely randomized design with three
201
replications. Data were analyzed by one-way ANOVA and Duncan's comparison test at 5%
202
level. The statistical software of SPSS 23 was used for data analysis.
203
2.
Results and discussion
204
2.1.
Determination of niosome mean size, PDI and zeta potential
Statistical analyses
9
205
The particle size in a colloidal carrier system plays an important role in determining its
206
stability, bioavailability, solubility, turbidity and rheological properties. Decreasing particle
207
size can lead to lower gravitational separation and turbidity, and higher solubility and
208
bioavailability. The results of particle size, PDI and the zeta potential measurements of blank
209
niosome and vitamin D3 loaded nano-niosomes with or without stabilizing agents (vitamin E
210
acetate, cholesterol and polyethylene glycol 400) are presented in Figure 1.
211
In the first day, the particle sizes of different niosome samples were 74-197 nm. The particle
212
size of vitamin D3-loaded noisome (N2) did not show a significant difference with the control
213
sample (without vitamin, N0) (74 vs 76 nm). Incorporation of vitamin E-acetate to the
214
niosome formulation (N2) caused a significant increase (P<0.5) in niosome size (93 nm) and
215
increasing of vitamin E concentration enhanced particle size nonsignificantly (93 to 99 nm).
216
According to Figure 1 (a), the particle sizes of niosomes containing cholesterol (G" ) and
217
polyethylene glycol (GH ) were larger compared to other formulations and G" sample had the
218
largest size (197±5 nm).
219
Presence of cholesterol increased particle size probably due to the spacing in surfactant
220
molecule in the hydrophobic layer. Similar results were reported for α-tocopherol-loaded
221
niosomes [16] and ascorbic acid and α-tocopherol niosomes [28].
222
The vesicle size depends on the concentration and nature of surfactant (HLB value),
223
stabilizer, bioactive component (hydrophobicity) and method of preparation.
224
After 40 days, the change in the size of G" and GH was significant and their size increased
225
(P<0.05); however, the size of G. and GI samples were reduced which could be due to the
226
separation of the particles interconnected during storage time. Beugin, et al. [29] in a study of
227
nano-niosomes containing cholesterol and polyethylene glycol observed the reduction of
228
particle size after one week. The size of their nano-niosomes was between 63-141 nm
229
depending on the formulation. 10
230
The polydispersity index of samples is shown in Figure 1 (b). The PDI value of samples was
231
in the range of 0.32-0.51, implying a relatively broad size distribution. N0 showed the
232
minimum PDI and N2 had the widest size distributions. At the first day, the PDI of nano-
233
niosome was significantly increased by incorporation of vitamin D3 and vitamin E. However;
234
Adding cholesterol and polyethylene glycol (G and G" ) caused a significant decrease on
235
polydispersity. During the 40 days of storage, the increase of PDI could be observed in the
236
samples containing stabilizer agents except for N2.
237
One of the factors affecting the physical stability and surface features of vesicles is the
238
surface charge which is usually evaluated by zeta potential [30]. The ionic atmosphere around
239
the charged particle causes an electrostatic repulsion between the particles, and when two
240
particles approach each other with the same load; it creates a repulsive force that prevents the
241
flocculation of particles. Therefore, by measuring zeta potential, the physical stability of the
242
colloidal systems could be estimated. On the other hand, the surface charge of vesicles is
243
important in adhering to active encapsulated compounds and cellular membrane.
244
According to Figure 1 (c), the zeta potential of samples except for the control sample (N0)
245
and the sample containing vitamin D3 (N1) were negative. This positive or negative zeta
246
potential is probably due to the different nature of the stabilizer agents. The highest zeta
247
potential (+29 mV) was related to the sample containing vitamin D3 (N1) and the lowest zeta
248
potential (-15mV) was observed in the sample contains vitamin D3 and vitamin E-acetate
249
(N3). All samples showed a decrease in zeta potential for 40 days, which was high in sample
250
GH and less in control samples (P<0.05). Among the various formulations, after 40 days, the
251
zeta potential of the sample containing vitamin D3 (N1) was higher than the rest (+19 mV).
252
Ionic strength and pH are two factors that can have the most profound impact on the zeta
253
potential values [31]. The zeta potential is decreased by leakage of active substances from the
254
inside of the niosomes and decreasing of medium’pH. 11
255
In general, in all of the formulations, the zeta potential was not high which is similar to the
256
previous reports [16, 32]. Zeta potential of particles in the colloidal system depends on type
257
and concentration of surfactants, active material, and stabilizer. Also, environmental and
258
process condition such as temperature, ionic strength of solvent and mechanical treatment can
259
be effective. Low zeta potential indicating the low electrostatic force of the vesicles which
260
can be attributed to the use of non-ionic and neutral surfactants [33]. Also, the observed zeta
261
potential can be due to the vitamin D3, stabilizers, pH of the hydration water, application of
262
heat and subsequent sonication. In general, the important parameter in long term stability of
263
the nano-niosomes could be related to repulsive steric between the vesicles. Also, vitamin D3
264
could induce relatively good positive charge density and selected stabilizers decreased this
265
stabilizing effect.
266
2.2.
267
Scanning electron microscopy (SEM) is used to provide more accurate information with
268
respect to size, size distribution, particle aggregation and shape of nano-niosomes.
269
Figure 1 (d) shows SEM images of nano-niosomes containing vitamin D3 (N1) which was
270
determined by size distribution analysis as the best niosome. These images showed spherical
271
and elliptical nanometer-sized particles in the vesicular carriers, which was almost
272
ascertained by the results of the particle size measurements. In some parts, vesicles had been
273
stuck together and reduction in the size of particles over time can be attributed to the
274
separation of these masses.
275
2.3.
276
An important application of DSC in delivery system researches is the study of the changes in
277
thermal behavior and phase transition (melting, crystallization and glass transition) of carriers
278
by an encapsulant, stabilizer, and other ingredients. These changes, by incorporation of
279
bioactive compounds, may relate to interactions between surfactants and encapsulant that
Morphological analysis by SEM
Differential scanning calorimetry (DSC)
12
280
affect bioavailability. Thermodynamic parameters, such as enthalpy and melting temperature,
281
are very important because they are not only indicating the complexation and kinetics of the
282
active material release but also potentially show the stability of the nano-niosomes during
283
storage.
284
DSC analysis was performed to evaluate the entry of vitamin D3 to the nano-niosome
285
structure and its encapsulation. Figure 2 (a) shows the DSC curve of vitamin D3, the control
286
sample (N0), and nano-niosome containing vitamin D3 (N1). Also, the melting temperature
287
and enthalpy of them are presented in
288
Table 2.
289
Analyses of all three samples were carried out at a temperature of 30-300 °C. As seen in
290
Figure 2 (a), there was only one melting peak in the vitamin D3 loaded nano-niosome (N1)
291
graph, and there was no peak of vitamin melting peak; This is in accordance with a previous
292
study [34]. The absence of vitamin D3 melting peak and observing only one melting peak in
293
the curve of nano-niosomes containing vitamin D3 can indicate that the two compounds are
294
co-crystallized and their compatibility is good.
295
Also, by incorporation of vitamin D3 enthalpy and the melting temperature of nano-niosome
296
increased slightly (5 °C) compared to the control sample. According to this evidence, it can
297
be said that vitamin D3 can create hydrogen (by the free hydroxyl group in the structure of
298
vitamin D3) and hydrophobic interactions with surfactant compounds and which in turn
299
changes the thermal properties of niosomes and gives higher stability. Also, the increase in
300
melting temperature of nano-niosome containing vitamin D3 indicates an increase in
301
crystallite size and crystalline order than the control sample (blank).
302
The colorimetric studies of Sezgin-Bayindir, et al. [26], on the niosomes containing
303
Candesartan, showed that Candesartan melting peak was removed from the DSC curves of
304
loaded niosomes, indicate that the active agent was encapsulated into the niosome and has the 13
305
amorphous state. Adversely, Varshosaz, et al. [35] reported that insulin loading had no
306
significant effect on the melting point of niosomes.
307
2.4.
308
In Figure 2 (b), the IR spectra of the nano-niosome components are presented. As shown in
309
the figure, vitamin D3 has a peak in 3300-3600 cm-1, which is related to stretching vibrations
310
of OH groups. Also, vitamin D3, blank nano-niosome and nano-niosome containing vitamin
311
D3 have a peak in 2900-3000 cm-1, which is related to stretching vibrations of CH groups.
312
As Figure 2 (b) shows all peaks regarding niosomes and vitamin D3 are present with a slight
313
displacement and intensity. In nano-niosome containing vitamin D3, the intensity of the
314
hydroxyl group peak has been declined in comparison to blank niosome, indicating hydrogen
315
bond formation. The intensity of the ester, ether and Alkanes group peaks have increased.
316
The increase in the intensity of these peaks is indicative of the formation of the interaction
317
among the components. Mehta, et al. [36] examined the IR spectra of blank and drug
318
(rifampicin, isoniazid, pyrazinamide) encapsulated niosomes. Their results did not show
319
significant differences between the control sample and the drugs containing samples.
320
2.5.
321
DPPH is a free radical widely used to measure the ability of antioxidant molecules to react as
322
a free radical scavenger or hydrogen donor [13]. The aim of this study was to evaluate the
323
antioxidant properties of nano-niosomes. Therefore, the DPPH test was performed in equal
324
volume from different formulations of nano-niosomes. The inhibitory concentration of 1 ml
325
of the samples is shown in Error! Reference source not found. (a).
326
The potential role of vitamin
327
work [37]; So all samples, although in a little amount, have anti-oxidant properties.
328
According to Error! Reference source not found. (a), the highest inhibitory effect in 1 ml of
329
nano-niosome solution belonged to nano-niosomes containing vitamin E-acetate (N3: 56%
Fourier transform infrared spectroscopy (FTIR)
Antioxidant properties
as a membrane antioxidant has been reported in previous
14
330
and N2: 42%) and lowest inhibitory belonged to blank sample (N0: 15%) due to the lack of
331
vitamin D3. The higher antioxidant properties in vitamin E-acetate samples compared to those
332
without it could be due to the break-up of the ester bond in vitamin E-acetate and the retrieval
333
of antioxidant properties at very low levels. Yang, et al. [7] studied vitamin E-acetate-
334
enriched nanoemulsions. Their results showed that approximately 35% of vitamin E-acetate
335
was converted to a free form (vitamin E) in the simulated intestine. Also, Di Mambro, et al.
336
[38] showed that Vitamin E acetate had almost no antioxidant activity (7% in 200 µg/ml) in
337
vitro, whereas for vitamin E at the same concentration the inhibitory concentration was 72%.
338
After 30 days the inhibitory effect of N0, N1 and N5 samples did not change significantly.
339
However, in samples containing vitamin E-acetate (N2 and N3) and a sample containing
340
cholesterol (N4), after 30 days the antioxidant properties decreased. Probably, vitamin E-
341
acetate and cholesterol was oxidized after a long period of time, which reduced the
342
antioxidant properties of these samples.
343
2.6.
344
Due to the exposure of binary bands to light and oxygen in nano-niosomes, lipid oxidation
345
may be easily accomplished by free radicals. In addition, with the presence of water,
346
hydrolysis may also occur and with releasing of free fatty acids, the pH is reduced [39]. Since
347
pH is one of the instability factors in these nano niosomes, it is possible to estimate the
348
chemical and physical instability in a qualitative way by measuring pH.
349
Error! Reference source not found. (b) shows the pH variations of different nano-niosome
350
formulations during one-month storage. The pH of the hydration water for all samples was
351
about 7.5, which was changed after the preparation of nano-niosomes.
352
The pH was decreased by incorporation of vitamin D3 and stabilizer agents. After a month,
353
the pH of nano-niosomes containing stabilizers was much lower. The pH of N4 and N5 was
354
almost identical on the first day, but over time, the nano-niosome containing polyethylene
pH
15
355
glycol decreased further. Probably the stabilizing effect of cholesterol is more, and prevents
356
the active substance leakage; So it causes less decrease in pH.
357
Considering that pH reduction is one of the instability factors in these samples, decreasing pH
358
can effect on physical and chemical stability. Soto-Jover, et al. [40] showed that the low pH
359
significantly reduced the physical and chemical stability of the nano-niosomes containing
360
canthaxanthin prepared by Tween 80 and Span 60.
361
2.7.
362
Turbidity refers to the light scattering properties by the particles in suspension. It depends on
363
nature, number, and size of colloidal particles in the liquid phase, on the difference in
364
refractive index between the particles and the medium, and on the particle size distribution.
365
To obtain a qualitative measure of particle size variations during 30 days, the turbidity of a nano-
366
niosome solution was measured [25]. The results of the optical properties of nano-niosomes
367
are illustrated in Error! Reference source not found. (c). Blank and N1 samples showed the
368
least turbidity and sample N4 had the highest turbidity.
369
The difference in turbidity among the samples of the first day can be due to the nature of the
370
stabilizers and correlated well with the size of nano-niosome particles. Cui, et al. [41]
371
reported that turbidity increases with increasing particle size.
372
Particle migration (i.e. creaming or sedimentation), and particle size variation or aggregation
373
(i.e. coalescence and flocculation) are the two major destabilization phenomena which affect
374
the homogeneity of dispersions [42]. As expected, the turbidity of all samples decreased over
375
a month. The decrease in turbidity could be due to the degradation of the active substance,
376
particle size variation, and flotation of particles to the surface of the solution [43].
377
Turbidity
2.8. Sedimentation
378
The effect of temperature on the amount of sediment during the storage period was
379
investigated. (70 days for samples in the refrigerator and 30 days for samples outside of the 16
380
refrigerator). Due to the higher instability of samples outside of the refrigerator, their
381
sediment percentage was measured on the 30th day. According to Error! Reference source
382
not found. (d), the results showed that the storage temperature was effective in the
383
sedimentation of the nano-niosomes. Sun, et al. [44] reported the effect of increasing the
384
temperature on aggregation in nanostructured lipid carriers. Also, Ravaghi, et al. [45] showed
385
that the high temperature significantly reduced the physical and chemical stability of the
386
nano-niosomes containing canthaxanthin.
387
Instability of samples at high temperatures may be due to the breakdown of hydrogen bonds
388
of surfactants. As seen in Error! Reference source not found. (d), sedimentation was observed
389
in all formulations (room and refrigerator temperature) except control sample in refrigerator
390
temperature. With increasing temperature and increasing time, the amount of sediment
391
increased. The samples in the refrigerator were flocculated on the 50-55th day and returned to
392
their original state with a little shaking, but after the 65-70th day, the phenomenon of
393
coalescence happened. Also in the cholesterol-containing sample, a cake after the 60th day
394
was formed, and flocculation phenomenon was not observed. In the samples outside the
395
refrigerator, after 12-20 days, the flocculation phenomenon occurred, and after the 25th day,
396
the coalescence and sedimentation occurred. The main factor for aggregation in the vesicular
397
systems can be attributed to the van der Waals attractions. Also, this aggregation in niosomes
398
may be due to the reduction of electrostatic repulsion between niosomes, the ion charge
399
density of the dispersion medium, high input energy (sonication, etc.), widespread
400
distribution of particles, reduction of water-binding sites in the membrane, etc., which causes
401
thermodynamic instability [26].
402
In some formulations, despite the higher zeta potential, more sediment was observed than the
403
other samples. Chemical instability may be affected by physical instability over time. The
404
results of Bozó, et al. [30] showed that the amount of surface charge was unaffected by 17
405
sedimentation.
406
2.9.
407
One of the most important parameters in the evaluation of niosomal formulations is
408
entrapment efficiency. Figure 4 (a) shows the encapsulation efficiency (EE%) of the samples
409
which varies from 75.3% to 94.3%. Addition of vitamin E-acetate caused a significant effect
410
on increasing of encapsulation efficiency (75.3% vs 82.4%). Also, increasing the amount of
411
vitamin E-acetate caused the increase of EE (2%). The highest efficiency was observed in the
412
samples containing cholesterol and polyethylene glycol. Cholesterol can decrease the
413
permeability of the bilayer with a better chain order and stability. The encapsulation
414
efficiency of vitamin D3 containing cholesterol was 94.2%. This is in accordance with a
415
previous study [15]. In a sample containing PEG, the EE% could be increased by entrapping
416
some molecules in the PEG chains [45]. These results show that the EE was strongly
417
dependent on the type and amount of the stabilizer agent (p < 0.05). Overall, a stabilizer can
418
increase EE% by changing hydrophobicity (HLB), rigidity, chain order and spacing between
419
tails of the lipid membrane.
420
The results of Wagner [46] showed higher EE of vitamin
421
sulfate (25.1%) in nano-niosomes. Palozza, et al. [47], in the study of nano-niosomes
422
containing beta-carotene, showed that the addition of cholesterol increased the encapsulation
423
efficiency.
424
Figure 4 (b) shows the loading capacity of the nano-niosomes. In general, the LC of all
425
samples was low which could be due to the initial degradation of vitamin
426
sonication and hydration). The highest LC is related to the sample containing cholesterol
427
(7%) and a sample containing polyethylene glycol (6.2%). The lowest LC is assigned to
428
sample N1` (2.4%). Considering that there was no significant difference in the LC of samples
429
containing vitamin E-acetate (N2 and N3).
Loading parameters
18
(95.9%) compared to iron
(during
430
3.
Conclusion
431
Niosomes provide a non-toxic and inexpensive vehicle for encapsulation of different
432
functional components (lipophilic, hydrophilic, and amphiphilic). In this study, the vitamin
433
D3 loaded nano-niosomes were produced by using a thin layer hydration method. The
434
resulted niosomes had nanometric size (<200 nm) and high encapsulation efficiency (>75%).
435
The different stabilizers were effective in enhancing of encapsulation efficiency and vitamin
436
E-acetate was the best stabilizer for this system due to the highest increasing effects on
437
encapsulation efficiency and antioxidant capacity.
438
4.
439
The authors gratefully acknowledge the support of the University of Tabriz and the support of
440
the Drug Applied Research Center of the Tabriz University of Medical Science.
441
5.
442
We wish to confirm that there are no known conflicts of interest associated with this
443
publication and there has been no significant financial support for this work that could have
444
influenced its outcome.
Acknowledgments
Conflict of Interest
445 446
6.
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562
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563
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564
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565
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567
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568
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569 570
24
571
Figure Captions
572
Figure 1. Effect of formulation on a) size; b) PDI; and c) zeta potential of nano-niosomes by
573
calculating standard deviation in three replicates (different letters indicate a significant
574
difference at the 5% probability level of Duncan test); d) Scanning electron microscopy of
575
nano-niosomes containing vitamin D3 (N1).
576
Figure 2. a) DSC curve of the control sample, the sample containing vitamin D3 and vitamin
577
D3;
578
containing Vitamin D3 (N1).
579
Figure 3. a) Percentage of inhibition of one ml of nano-niosome specimens on day one and
580
on day 30 after production; by calculating the mean and standard deviation in three replicates
581
(different letters indicate a significant difference at the 5% probability level according to
582
Duncan test); b) Changes in pH of formulations over a month; c) Turbidity of nano-niosomes
583
in the first and 30th days (similar letters indicate no significant difference at the 5% Duncan
584
test); d) The percentage of deposition of formulations at room temperature and inside the
585
refrigerator after 70 days.
586
Figure 4. Encapsulation efficiency and loading capacity of the formulation by calculating the
587
mean and standard deviation with three repetitions (different letters representing a significant
588
difference at the 5% probability level of Duncan's test).
b) FTIR spectrum for vitamin D3, blank nano-niosome (N0) and nano-niosome
589
25
b
a a
300
0.6
b
a a
0.5 d
200
0.4
150 gh gh
100
a
bc
f
gh h
d
ef e 0.2
g
50
0.1
0
0 N1
N2
N3
1st day
N4
N0
N5
40th day
d
cd
cd e
10 0
-20
f
f
f
-10
f
e bc
-30 N0
N1
N2
1st day
30 20
N1
N2
N3
d
b
N4
N5
Formulation 1st day
N3
N4
Formulation
c
a
b
cd
cd
0.3
Formulation
Zeta potential ( mV)
a
d
N0
590 591 592
b bc
c
PDI
Particle size (nm)
250
40th day
Figure 1
26
40th day
N5
593 594 595
Figure 2
596 597
27
a
60
a 6.8
50 40
6.6
c cd
fe
6.2
g
fg
30
6.4
cde def pH
Inhibition%
b
20
b
7
h
6 5.8
h h
5.6 5.4
10
5.2 0
5 N0
N1
N2
N3
N4
N5
0
5
10
N0 N3
30th day
b
d
0.7
e
0.6
e f
0.5 0.4 0.3 0.2 0.1
g h
N1 N4
N2 N5
d
25 20 15 10 5
g h
0
0 N0
N1
N2
N3
N4
N0
N5
1st day
N1
N2
N3
N4
N5
Formulation
Formulation
T=4 - 70th day
30th day
598 599
30
30
sedinantation%
Absorbance
35
b c
0.9 0.8
25
a
c
1
20
Day
Formulation 1st day
15
Figure 3
600 601 602 603 604 28
T=25 - 30th day
605 606 607 608 609 610 611 612
100 90 80 70 60 50 40 30 20 10 0
b a
e
d
c
b
Loading capacity %
Encapsulation efficiency%
a
N1
N2
N3
N4
a b
d
N1
N5
Formulation
613 614
10 9 8 7 6 5 4 3 2 1 0
c
c
N2
N3 Formulation
Figure 4
615 616 617 618 619 620 621 622 623 29
N4
N5
624
Table 1. The formulation used for the preparation of nano-niosomes Formulation JKL 60⁄NOPP 80 (mole ratio) Vitamin D3 (mmole) Vitamin E- acetate (mmole) Cholesterol (mmole) Polyethylene Glycol 400 (mmole)
N0
N1
N2
N3
N4
N5
3:2
3:2
3:2
3:2
3:2
3:2
-
0.02 -
0.02 0.01 -
0.02 0.02 -
0.02 0.06 -
0.02 0.06
625 626 627 628 629 630 631 632 633 634 635 636 637 638 639 640 641 642 643 644 645 646 647 648
30
649
Table 2. Melting and enthalpy temperature of the control sample, sample G. and vitamin Sample
Melting peak (oC)
Onset temperature (oC)
Endset temperature (oC)
Enthalpy (J/g)
N1
53
33.6
62.8
-36.4
Control (N0)
48
30.16
56.3
-10.7
Vitamin D3
91
82.98
98
-35.47
650 651 652 653 654 655 656 657 658 659 660 661 662 663 664 665 666 667 668 669 670 671 672 673 674 675 676 677 678 679 680 681 682 683 684 685 686 687 688 689
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JDDST 101284
To appear in:
Journal of Drug Delivery Science and Technology
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Please cite this article as: V. Talebi, B. Ghanbarzadeh, H. Hamishehkar, A. Pezeshki, A. Ostadrahimi, Effects of different stabilizers on colloidal properties and encapsulation efficiency of vitamin D3 loaded nano-niosomes, Journal of Drug Delivery Science and Technology (2019), doi: https://doi.org/10.1016/ j.jddst.2019.101284. This is a PDF file of an article that has undergone enhancements after acceptance, such as the addition of a cover page and metadata, and formatting for readability, but it is not yet the definitive version of record. This version will undergo additional copyediting, typesetting and review before it is published in its final form, but we are providing this version to give early visibility of the article. Please note that, during the production process, errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain. © 2019 Published by Elsevier B.V.
2
Effects of different stabilizers on colloidal properties and encapsulation efficiency of vitamin D3 loaded nano-niosomes
3 4 5
Vahideh Talebi1, Babak Ghanbarzadeh*1,2, Hamed Hamishehkar3,
6
Akram Pezeshki1, Alireza Ostadrahimi 4
1
7 8
1-
9 10
Tabriz, P.O. Box 51666-16471, Tabriz, Iran 2-
11 12 13 14 15
Department of Food Science and Technology, Faculty of Agriculture, University of
Department of Food Engineering, Faculty of Engineering, Near East University P. O. Box 99138, Nicosia, Cyprus, Mersin 10, Turkey
3-
Drug Applied Research Center, Tabriz University of Medical Sciences, Tabriz, Iran 4- Nutrition Research Center, Tabriz University of Medical Sciences, Tabriz, Iran
* Corresponding author: [email protected], [email protected] Tel: 00989123039836, Fax: 00984133356005
16 17 18 19 20 21 22 23 24 1
25
Abstract
26
The vitamin D3 loaded nano-niosomes were prepared by thin layer hydration and sonication
27
methods. Influence of stabilizers (vitamin E acetate, polyethylene glycol and, cholesterol) on
28
the different physicochemical properties of resulted niosomes including particle size
29
distribution, zeta potential, encapsulation efficiency (EE%), antioxidant activities, turbidity,
30
sedimentation, and pH were evaluated. The images of scanning electron microscopy (SEM)
31
confirmed the results of the particle size data which were obtained using dynamic light
32
scattering (DLS). Fourier transform infrared spectroscopy (FT-IR) and differential scanning
33
calorimetry (DSC) analysis demonstrated the incorporation of vitamin D3 into niosomes.
34
Incorporation of vitamin E-acetate and cholesterol to the niosome formulation (N2) caused a
35
significant increase (P<0.5) in niosome size. Addition of vitamin E-acetate caused a
36
significant effect on increasing of encapsulation efficiency.The highest efficiency was
37
observed in the samples containing cholesterol and polyethylene glycol. The niosome
38
formulation containing 0.02 mmole vitamin E acetate with the size of 99 nm was selected as
39
the optimal formulation. This formulation had the highest antioxidant capacity (56%), the
40
lowest pH changes and high encapsulation efficiency (92.9%).
41
Keywords: nano-niosome, vitamin E-acetate, vitamin D3, encapsulation, stabilizer
42
2
43
1. Introduction
44
Nutraceuticals are food ingredients that, in addition to having basic nutritional properties,
45
have valuable biological activities such as enhancing the immune system and inhibitory
46
effects against important disorders such as cancer, cardiovascular diseases, diabetes, macular
47
degeneration, and other age-related diseases. Vitamins are among the most important groups
48
of nutraceutical compounds and are naturally present in foods. Low doses of vitamins are
49
essential for growth, maintaining the normal state of cells and body function. By growing
50
tendency of people to low-fat or non-fat foods due to the changing the lifestyle, and also the
51
destruction of nutraceuticals during the processing and food preservation, concerns about
52
diseases caused by essential hydrophobic nutrients deficiencies have been increased.
53
Therefore, the enrichment of some foods and beverages with these essential nutrients can be
54
an effective way to solve this problem.
55
Vitamin D is a lipid-soluble vitamin with two main chemical forms, vitamin (ergocalciferol)
56
D2 and vitamin D3 (cholecalciferol) [1]. Vitamin D3 (cholecalciferol) is synthesized in the
57
human epidermis after light exposure [2]. Recent studies showed a high prevalence of
58
vitamin
59
diabetes [4], metabolic bone diseases, osteoporosis, hypertension and others [5]. Due to poor
60
food sources containing this vitamin, food fortification with vitamin
61
[6].
62
The role of vitamin E as an important factor and its antioxidant and non-antioxidant
63
biological activities in the normal metabolism of all cells and reduction of cardiovascular
64
disease, diabetes, and cancer has been proven. Because of higher chemical stability of
65
vitamin E acetate (the esterified form of α-tocopherol) compared to the non-esterified form
66
(α-tocopherol), this form is often used in foods and beverages [7].
67
Encapsulation of nutraceutical compounds by lipid or polymer-based carriers is an effective
deficiency, especially in women [3] which causes cardiovascular diseases and
3
is the priority deal
68
way to protect their properties and also increase their solubility and bioavailability and
69
decrease their possible off flavor [2]. Niosome, non-ionic surfactants vesicle (NSV) is one of
70
the nanocarriers that is formed from non-ionic surfactants. It is structurally similar to
71
liposomes and consists of an aqueous core enclosed by a bilayer membrane of non-ionic
72
surfactants [8]. In their vesicular structure, the hydrophobic groups are placed in the interior
73
of the membrane while the hydrophilic ones are exposed to the aqueous core. The niosome
74
and vesicular liposome structures do not form spontaneously, and they need some energy
75
input (e.g., hand-shaking, agitation, ultrasound, heating) and this has led to the development
76
of different preparation methods, during the last two decades. Niosomes, as substitutes of
77
liposomes, [9] are chemically more stable and have lower costs than liposomes. In addition, a
78
more wide range of surfactants is available for the formulation of these vesicular carriers.
79
These vesicles can encapsulate a large amount of different functional components (lipophilic,
80
hydrophilic, and amphiphilic) in their small volumes [10]. Span and Tween, non-ionic
81
surfactants, have some interesting properties such as biodegradability, biocompatibility, and
82
low toxicity, so they are used in some foods and pharmaceuticals [11].
83
In recent years, several types of research have worked on the production of nutriceutical
84
loaded noisomes such as capsaicin [11], resveratrol [12], gallic acid, ascorbic acid, curcumin
85
and quercetin [13], resveratrol/curcumin and alpha-tocopherol/curcumin [14], vitamin D3 and
86
ferrous sulfate [15], α-Tocopherol [16]. However, the comparison of effects of different
87
stabilizers on the noisome systems has not extensively studied.
88
The main objective of the present work was to preparing vitamin D3 loaded nano-niosome by
89
thin layer hydration and sonication method and then study of effects of some food grade
90
stabilizers such as vitamin E acetate, polyethylene glycol and cholesterol on physicochemical
91
properties of developed nano-niosomes.
92 4
93
Materials and Method
94
1.1.
95
Vitamin D was provided by DSM. (Swiss). Vitamin E acetate was obtained from Zahravi.
96
(Iran) and Cholesterol was purchased from Sigma (Germany). Polyethylene glycol 400 was
97
purchased from Sacharlau (Spain). Other chemicals including Span 60, Tween 80, 2,2-
98
diphenyl-1-picrylhydrazyl (DPPH) powder and 2-propanol were analytical grade and were
99
provided from Merck (Germany).
Materials
100
1.2.
Preparation of nano-niosomes
101
Nano-niosomes were prepared according to thin layer hydration- sonication method described
102
by Pando, et al. [17] with some modification. Span 60, a non-ionic surfactant was used as the
103
main component in the formulations. Span 60 and Tween 80 were dissolved in isopropyl
104
alcohol (5ml) at 50 ºC for 20 min. Vitamin
105
isopropyl alcohol (5 ml). Two solutions were mixed and thin layer formation was performed
106
in the rotary evaporator LABOROTA 4002- digital model (Heidolph, Germany) at 60 ºC, 90
107
rpm, 100 mmHg for 60 min. Hydration was done by 10 ml distilled water in rotary at 65 ºC
108
for 30 min. Sonication was performed for 6 min by 1 min intervals at 120 Hz (UP200H
109
model, Hielscher, Germany). Finally, the prepared nano niosomes were filtered through 0.2
110
µm Whatman filter.
111
Due to the increased encapsulation efficiency in the range of HLB = 8.6 [18], two types of
112
surfactants were used to obtain the desired HLB. The percentages of the used amounts of
113
surfactants were obtained from Equation 1 [19]: HLB = =
114
(
and Vitamin E- acetate were dissolved in
)+( +
)
× 100
(1)
=
The formulation used for the preparation of nano-niosomes is shown in 5
115
Table 1.
116 117
1.3.
Mean size, polydispersity index, and zeta potential of niosomes
118
The average diameter, polydispersity index (PDI) and zeta potential of samples was measured
119
using a dynamic laser scattering (DLS) device, the Nanotrac Wave Microtrac (Germany)
120
model. For this purpose, each sample was diluted 20 times with distilled water. All specimens
121
were measured in three replicates. This system determined the particle size by measuring
122
their propulsion and dynamic light diffraction (DLS), and then the size is determined by
123
applying proven theories.
124
The average particle diameter was reported in terms of the volumetric average. The mean
125
particle diameter or DeBroukere mean was calculated from Equation 2 [20]:
!" !
∑ 4,3 = ∑
(2)
126
1.4.
127
Morphology of nano-niosomes was investigated by scanning electron microscopy (SEM).
128
The sample was diluted 20 times with water and observed under KYKY-EM3200 at an
129
accelerating voltage of 26 kV [21].
130
Morphological analysis (scanning electron microscopy)
1.5. Differential scanning calorimetry (DSC)
131
Differential scanning calorimetry of blank sample and nanoniosome containing vitamin D3
132
(N1) and vitamin D3 was performed on a DSC device (PerkinElmer, Jade DSC model, US
133
manufacturing). The device was calibrated with indium, and an empty aluminum container
134
was used as a reference. Samples with a mass of approximately 4 milligrams were scanned at
135
20 °C/min at a temperature range of 30 to 300 °C, and the melting point of the compounds
136
was determined [22].
137
1.6.
Fourier transform infrared spectroscopy (FTIR) 6
138
Infrared spectroscopy was performed using an FTIR device TENSOR 27, in the range of 400-
139
4000 cm-1. The samples (Span 60, Tween 80, Vitamin D3, Vitamin E-acetate, blank nano-
140
niosome and nano-niosome containing vitamin D3) were separately mixed with pure
141
potassium bromide (KBr) in a ratio of 1 to 100 and this mixture was used in
142
spectrophotometry [23].
143
1.7.
144
The antioxidant capacity (AOC) was determined using the 2,2-diphenyl-1-picrylhydrazyl
145
(DPPH) method. DPPH is a free radical widely used to determine the ability of antioxidant
146
molecules to react as free radical scavengers [11]. First, nano-niosomes were broken down
147
using chloroform. For this purpose, 2 ml of nano-niosome solution was mixed with 2 ml of
148
chloroform and stirred for 20 minutes. Then the white upper liquid (water) was discarded. A
149
chloroform solution containing DPPH (0.01mM) was prepared and mixed with samples in the
150
ratio of 1:1, then the adsorption changes were read after 2 hours of incubation in darkness at
151
517 nm with UV-vis Ultrospec 2000 (UK) spectrophotometer. The antioxidant capacity with
152
the DPPH inhibitory content was determined according to Equation 3 [24]:
Antioxidant capacity
Inhibition% =
+, − +. × 100 +,
(3)
153
where A0 is absorbance of control sample at 517 nm and A1 is sample absorbance at 517 nm.
154
1.8.
155
To obtain a qualitative amount of oxidation and hydrolysis of niosomes over a month, the pH
156
of the nano-niosome solutions was measured. The pH was measured by direct injection of a
157
pH meter (Metrohm, Switzerland) into a new mass solution, and setting the sample
158
temperature.
159
1.9.
160
To obtain a qualitative dimension of variation in the size and release rate of nano-niosomes
pH
Turbidity
7
161
during a month, the turbidity was measured. First, 1 ml of the sample was diluted with 2 ml
162
of distilled water and stored at room temperature for 30 minutes. Then, the turbidity of the
163
sample was measured in a spectrophotometer of the Ultrospec 2000 produced by the UK in
164
quartz tubes at a wavelength of 600 nm [25].
165 166
1.10.
Sedimentation
167
In order to determine the stability of nano-niosome solutions, their sediment was measured. 5
168
ml of each formulation was stored for 60 days and 30 days at 2 °C and room temperature and
169
their sedimentation height was measured. Sediment volume was obtained using Equation 4
170
[26]: S% =
V1 2V × 100 ,
(4)
171
where Vu is sediment volume at a specified time and V0 is Total volum of nano-niosome
172
solution.
173
1.11.
174
To determine encapsulation efficiency (EE%), 3 ml of nano-niosome solution was mixed
175
with 3 ml of isopropyl 50% solution (to dissolve only soluble vitamins). Amicon filter was
176
used by centrifugation at 4000 rpm for 2 minutes [27] to isolate free and encapsulated
177
vitamins. From each of the upper and lower sections of the filter, 1 ml samples were
178
removed, and 500 µl of chloroform was added to each. The test tube containing nano-
179
niosome was shaken for 20 minutes to degrade the nano-niosome and free the vitamin.
180
Sample containing free vitamin was also shaken for several minutes. The chloroform phase of
181
the solutions was separated, and the samples were dried under nitrogen gas. EE was
182
calculated using Equation 5:
Loading parameters
8
Encapsulation efficiency% =
Capsulated vitamin (mg) × 100 Free + encapsulated vitamin (mg)
(5)
183
The loading capacity (LC) calculated as the ratio of the active ingredient to the whole lipid
184
(stabilizing agent + surfactant + vitamin E-acetate).
185
1.11.1. High-Performance liquid chromatography (HPLC)
186
HPLC (Waters 1525 Binary, USA) was used to determine the free and encapsulated vitamin
187
in nano-niosomes. The optimal condition of the column and the HPLC device to determine
188
the encapsulation efficiency was as follows: C18 silica gel column (5 µm, 250mm × 4.6mm),
189
room temperature, flow rate 1 ml/min, wavelength 270 nm, injection valium 20 µl, and
190
mobile phase chloroform + 0.5% amyl alcohol (95 ml), ethyl acetate (5 ml).
191
In order to plot the calibration curve, 100 mg of a standard solution of 1 million units was
192
transferred to a 50-caliber balloon and chloroform was added to reach the specified valium
193
(2000 IU / ml); 20 µl of the standard solution was injected to the device, and the sub-curved
194
surface was calculated.
195
The concentration of vitamin D3 was determined using Equation 6: CD =
AD × CF AF
(6)
196
where At is the area below the vitamin D3 curve in the sample solution, As is the area under
197
the curve of vitamin D3 in the standard solution, Cs is standard concentration and Ct is sample
198
concentration
199
1.12.
200
Physical and chemical tests were performed on a completely randomized design with three
201
replications. Data were analyzed by one-way ANOVA and Duncan's comparison test at 5%
202
level. The statistical software of SPSS 23 was used for data analysis.
203
2.
Results and discussion
204
2.1.
Determination of niosome mean size, PDI and zeta potential
Statistical analyses
9
205
The particle size in a colloidal carrier system plays an important role in determining its
206
stability, bioavailability, solubility, turbidity and rheological properties. Decreasing particle
207
size can lead to lower gravitational separation and turbidity, and higher solubility and
208
bioavailability. The results of particle size, PDI and the zeta potential measurements of blank
209
niosome and vitamin D3 loaded nano-niosomes with or without stabilizing agents (vitamin E
210
acetate, cholesterol and polyethylene glycol 400) are presented in Figure 1.
211
In the first day, the particle sizes of different niosome samples were 74-197 nm. The particle
212
size of vitamin D3-loaded noisome (N2) did not show a significant difference with the control
213
sample (without vitamin, N0) (74 vs 76 nm). Incorporation of vitamin E-acetate to the
214
niosome formulation (N2) caused a significant increase (P<0.5) in niosome size (93 nm) and
215
increasing of vitamin E concentration enhanced particle size nonsignificantly (93 to 99 nm).
216
According to Figure 1 (a), the particle sizes of niosomes containing cholesterol (G" ) and
217
polyethylene glycol (GH ) were larger compared to other formulations and G" sample had the
218
largest size (197±5 nm).
219
Presence of cholesterol increased particle size probably due to the spacing in surfactant
220
molecule in the hydrophobic layer. Similar results were reported for α-tocopherol-loaded
221
niosomes [16] and ascorbic acid and α-tocopherol niosomes [28].
222
The vesicle size depends on the concentration and nature of surfactant (HLB value),
223
stabilizer, bioactive component (hydrophobicity) and method of preparation.
224
After 40 days, the change in the size of G" and GH was significant and their size increased
225
(P<0.05); however, the size of G. and GI samples were reduced which could be due to the
226
separation of the particles interconnected during storage time. Beugin, et al. [29] in a study of
227
nano-niosomes containing cholesterol and polyethylene glycol observed the reduction of
228
particle size after one week. The size of their nano-niosomes was between 63-141 nm
229
depending on the formulation. 10
230
The polydispersity index of samples is shown in Figure 1 (b). The PDI value of samples was
231
in the range of 0.32-0.51, implying a relatively broad size distribution. N0 showed the
232
minimum PDI and N2 had the widest size distributions. At the first day, the PDI of nano-
233
niosome was significantly increased by incorporation of vitamin D3 and vitamin E. However;
234
Adding cholesterol and polyethylene glycol (G and G" ) caused a significant decrease on
235
polydispersity. During the 40 days of storage, the increase of PDI could be observed in the
236
samples containing stabilizer agents except for N2.
237
One of the factors affecting the physical stability and surface features of vesicles is the
238
surface charge which is usually evaluated by zeta potential [30]. The ionic atmosphere around
239
the charged particle causes an electrostatic repulsion between the particles, and when two
240
particles approach each other with the same load; it creates a repulsive force that prevents the
241
flocculation of particles. Therefore, by measuring zeta potential, the physical stability of the
242
colloidal systems could be estimated. On the other hand, the surface charge of vesicles is
243
important in adhering to active encapsulated compounds and cellular membrane.
244
According to Figure 1 (c), the zeta potential of samples except for the control sample (N0)
245
and the sample containing vitamin D3 (N1) were negative. This positive or negative zeta
246
potential is probably due to the different nature of the stabilizer agents. The highest zeta
247
potential (+29 mV) was related to the sample containing vitamin D3 (N1) and the lowest zeta
248
potential (-15mV) was observed in the sample contains vitamin D3 and vitamin E-acetate
249
(N3). All samples showed a decrease in zeta potential for 40 days, which was high in sample
250
GH and less in control samples (P<0.05). Among the various formulations, after 40 days, the
251
zeta potential of the sample containing vitamin D3 (N1) was higher than the rest (+19 mV).
252
Ionic strength and pH are two factors that can have the most profound impact on the zeta
253
potential values [31]. The zeta potential is decreased by leakage of active substances from the
254
inside of the niosomes and decreasing of medium’pH. 11
255
In general, in all of the formulations, the zeta potential was not high which is similar to the
256
previous reports [16, 32]. Zeta potential of particles in the colloidal system depends on type
257
and concentration of surfactants, active material, and stabilizer. Also, environmental and
258
process condition such as temperature, ionic strength of solvent and mechanical treatment can
259
be effective. Low zeta potential indicating the low electrostatic force of the vesicles which
260
can be attributed to the use of non-ionic and neutral surfactants [33]. Also, the observed zeta
261
potential can be due to the vitamin D3, stabilizers, pH of the hydration water, application of
262
heat and subsequent sonication. In general, the important parameter in long term stability of
263
the nano-niosomes could be related to repulsive steric between the vesicles. Also, vitamin D3
264
could induce relatively good positive charge density and selected stabilizers decreased this
265
stabilizing effect.
266
2.2.
267
Scanning electron microscopy (SEM) is used to provide more accurate information with
268
respect to size, size distribution, particle aggregation and shape of nano-niosomes.
269
Figure 1 (d) shows SEM images of nano-niosomes containing vitamin D3 (N1) which was
270
determined by size distribution analysis as the best niosome. These images showed spherical
271
and elliptical nanometer-sized particles in the vesicular carriers, which was almost
272
ascertained by the results of the particle size measurements. In some parts, vesicles had been
273
stuck together and reduction in the size of particles over time can be attributed to the
274
separation of these masses.
275
2.3.
276
An important application of DSC in delivery system researches is the study of the changes in
277
thermal behavior and phase transition (melting, crystallization and glass transition) of carriers
278
by an encapsulant, stabilizer, and other ingredients. These changes, by incorporation of
279
bioactive compounds, may relate to interactions between surfactants and encapsulant that
Morphological analysis by SEM
Differential scanning calorimetry (DSC)
12
280
affect bioavailability. Thermodynamic parameters, such as enthalpy and melting temperature,
281
are very important because they are not only indicating the complexation and kinetics of the
282
active material release but also potentially show the stability of the nano-niosomes during
283
storage.
284
DSC analysis was performed to evaluate the entry of vitamin D3 to the nano-niosome
285
structure and its encapsulation. Figure 2 (a) shows the DSC curve of vitamin D3, the control
286
sample (N0), and nano-niosome containing vitamin D3 (N1). Also, the melting temperature
287
and enthalpy of them are presented in
288
Table 2.
289
Analyses of all three samples were carried out at a temperature of 30-300 °C. As seen in
290
Figure 2 (a), there was only one melting peak in the vitamin D3 loaded nano-niosome (N1)
291
graph, and there was no peak of vitamin melting peak; This is in accordance with a previous
292
study [34]. The absence of vitamin D3 melting peak and observing only one melting peak in
293
the curve of nano-niosomes containing vitamin D3 can indicate that the two compounds are
294
co-crystallized and their compatibility is good.
295
Also, by incorporation of vitamin D3 enthalpy and the melting temperature of nano-niosome
296
increased slightly (5 °C) compared to the control sample. According to this evidence, it can
297
be said that vitamin D3 can create hydrogen (by the free hydroxyl group in the structure of
298
vitamin D3) and hydrophobic interactions with surfactant compounds and which in turn
299
changes the thermal properties of niosomes and gives higher stability. Also, the increase in
300
melting temperature of nano-niosome containing vitamin D3 indicates an increase in
301
crystallite size and crystalline order than the control sample (blank).
302
The colorimetric studies of Sezgin-Bayindir, et al. [26], on the niosomes containing
303
Candesartan, showed that Candesartan melting peak was removed from the DSC curves of
304
loaded niosomes, indicate that the active agent was encapsulated into the niosome and has the 13
305
amorphous state. Adversely, Varshosaz, et al. [35] reported that insulin loading had no
306
significant effect on the melting point of niosomes.
307
2.4.
308
In Figure 2 (b), the IR spectra of the nano-niosome components are presented. As shown in
309
the figure, vitamin D3 has a peak in 3300-3600 cm-1, which is related to stretching vibrations
310
of OH groups. Also, vitamin D3, blank nano-niosome and nano-niosome containing vitamin
311
D3 have a peak in 2900-3000 cm-1, which is related to stretching vibrations of CH groups.
312
As Figure 2 (b) shows all peaks regarding niosomes and vitamin D3 are present with a slight
313
displacement and intensity. In nano-niosome containing vitamin D3, the intensity of the
314
hydroxyl group peak has been declined in comparison to blank niosome, indicating hydrogen
315
bond formation. The intensity of the ester, ether and Alkanes group peaks have increased.
316
The increase in the intensity of these peaks is indicative of the formation of the interaction
317
among the components. Mehta, et al. [36] examined the IR spectra of blank and drug
318
(rifampicin, isoniazid, pyrazinamide) encapsulated niosomes. Their results did not show
319
significant differences between the control sample and the drugs containing samples.
320
2.5.
321
DPPH is a free radical widely used to measure the ability of antioxidant molecules to react as
322
a free radical scavenger or hydrogen donor [13]. The aim of this study was to evaluate the
323
antioxidant properties of nano-niosomes. Therefore, the DPPH test was performed in equal
324
volume from different formulations of nano-niosomes. The inhibitory concentration of 1 ml
325
of the samples is shown in Error! Reference source not found. (a).
326
The potential role of vitamin
327
work [37]; So all samples, although in a little amount, have anti-oxidant properties.
328
According to Error! Reference source not found. (a), the highest inhibitory effect in 1 ml of
329
nano-niosome solution belonged to nano-niosomes containing vitamin E-acetate (N3: 56%
Fourier transform infrared spectroscopy (FTIR)
Antioxidant properties
as a membrane antioxidant has been reported in previous
14
330
and N2: 42%) and lowest inhibitory belonged to blank sample (N0: 15%) due to the lack of
331
vitamin D3. The higher antioxidant properties in vitamin E-acetate samples compared to those
332
without it could be due to the break-up of the ester bond in vitamin E-acetate and the retrieval
333
of antioxidant properties at very low levels. Yang, et al. [7] studied vitamin E-acetate-
334
enriched nanoemulsions. Their results showed that approximately 35% of vitamin E-acetate
335
was converted to a free form (vitamin E) in the simulated intestine. Also, Di Mambro, et al.
336
[38] showed that Vitamin E acetate had almost no antioxidant activity (7% in 200 µg/ml) in
337
vitro, whereas for vitamin E at the same concentration the inhibitory concentration was 72%.
338
After 30 days the inhibitory effect of N0, N1 and N5 samples did not change significantly.
339
However, in samples containing vitamin E-acetate (N2 and N3) and a sample containing
340
cholesterol (N4), after 30 days the antioxidant properties decreased. Probably, vitamin E-
341
acetate and cholesterol was oxidized after a long period of time, which reduced the
342
antioxidant properties of these samples.
343
2.6.
344
Due to the exposure of binary bands to light and oxygen in nano-niosomes, lipid oxidation
345
may be easily accomplished by free radicals. In addition, with the presence of water,
346
hydrolysis may also occur and with releasing of free fatty acids, the pH is reduced [39]. Since
347
pH is one of the instability factors in these nano niosomes, it is possible to estimate the
348
chemical and physical instability in a qualitative way by measuring pH.
349
Error! Reference source not found. (b) shows the pH variations of different nano-niosome
350
formulations during one-month storage. The pH of the hydration water for all samples was
351
about 7.5, which was changed after the preparation of nano-niosomes.
352
The pH was decreased by incorporation of vitamin D3 and stabilizer agents. After a month,
353
the pH of nano-niosomes containing stabilizers was much lower. The pH of N4 and N5 was
354
almost identical on the first day, but over time, the nano-niosome containing polyethylene
pH
15
355
glycol decreased further. Probably the stabilizing effect of cholesterol is more, and prevents
356
the active substance leakage; So it causes less decrease in pH.
357
Considering that pH reduction is one of the instability factors in these samples, decreasing pH
358
can effect on physical and chemical stability. Soto-Jover, et al. [40] showed that the low pH
359
significantly reduced the physical and chemical stability of the nano-niosomes containing
360
canthaxanthin prepared by Tween 80 and Span 60.
361
2.7.
362
Turbidity refers to the light scattering properties by the particles in suspension. It depends on
363
nature, number, and size of colloidal particles in the liquid phase, on the difference in
364
refractive index between the particles and the medium, and on the particle size distribution.
365
To obtain a qualitative measure of particle size variations during 30 days, the turbidity of a nano-
366
niosome solution was measured [25]. The results of the optical properties of nano-niosomes
367
are illustrated in Error! Reference source not found. (c). Blank and N1 samples showed the
368
least turbidity and sample N4 had the highest turbidity.
369
The difference in turbidity among the samples of the first day can be due to the nature of the
370
stabilizers and correlated well with the size of nano-niosome particles. Cui, et al. [41]
371
reported that turbidity increases with increasing particle size.
372
Particle migration (i.e. creaming or sedimentation), and particle size variation or aggregation
373
(i.e. coalescence and flocculation) are the two major destabilization phenomena which affect
374
the homogeneity of dispersions [42]. As expected, the turbidity of all samples decreased over
375
a month. The decrease in turbidity could be due to the degradation of the active substance,
376
particle size variation, and flotation of particles to the surface of the solution [43].
377
Turbidity
2.8. Sedimentation
378
The effect of temperature on the amount of sediment during the storage period was
379
investigated. (70 days for samples in the refrigerator and 30 days for samples outside of the 16
380
refrigerator). Due to the higher instability of samples outside of the refrigerator, their
381
sediment percentage was measured on the 30th day. According to Error! Reference source
382
not found. (d), the results showed that the storage temperature was effective in the
383
sedimentation of the nano-niosomes. Sun, et al. [44] reported the effect of increasing the
384
temperature on aggregation in nanostructured lipid carriers. Also, Ravaghi, et al. [45] showed
385
that the high temperature significantly reduced the physical and chemical stability of the
386
nano-niosomes containing canthaxanthin.
387
Instability of samples at high temperatures may be due to the breakdown of hydrogen bonds
388
of surfactants. As seen in Error! Reference source not found. (d), sedimentation was observed
389
in all formulations (room and refrigerator temperature) except control sample in refrigerator
390
temperature. With increasing temperature and increasing time, the amount of sediment
391
increased. The samples in the refrigerator were flocculated on the 50-55th day and returned to
392
their original state with a little shaking, but after the 65-70th day, the phenomenon of
393
coalescence happened. Also in the cholesterol-containing sample, a cake after the 60th day
394
was formed, and flocculation phenomenon was not observed. In the samples outside the
395
refrigerator, after 12-20 days, the flocculation phenomenon occurred, and after the 25th day,
396
the coalescence and sedimentation occurred. The main factor for aggregation in the vesicular
397
systems can be attributed to the van der Waals attractions. Also, this aggregation in niosomes
398
may be due to the reduction of electrostatic repulsion between niosomes, the ion charge
399
density of the dispersion medium, high input energy (sonication, etc.), widespread
400
distribution of particles, reduction of water-binding sites in the membrane, etc., which causes
401
thermodynamic instability [26].
402
In some formulations, despite the higher zeta potential, more sediment was observed than the
403
other samples. Chemical instability may be affected by physical instability over time. The
404
results of Bozó, et al. [30] showed that the amount of surface charge was unaffected by 17
405
sedimentation.
406
2.9.
407
One of the most important parameters in the evaluation of niosomal formulations is
408
entrapment efficiency. Figure 4 (a) shows the encapsulation efficiency (EE%) of the samples
409
which varies from 75.3% to 94.3%. Addition of vitamin E-acetate caused a significant effect
410
on increasing of encapsulation efficiency (75.3% vs 82.4%). Also, increasing the amount of
411
vitamin E-acetate caused the increase of EE (2%). The highest efficiency was observed in the
412
samples containing cholesterol and polyethylene glycol. Cholesterol can decrease the
413
permeability of the bilayer with a better chain order and stability. The encapsulation
414
efficiency of vitamin D3 containing cholesterol was 94.2%. This is in accordance with a
415
previous study [15]. In a sample containing PEG, the EE% could be increased by entrapping
416
some molecules in the PEG chains [45]. These results show that the EE was strongly
417
dependent on the type and amount of the stabilizer agent (p < 0.05). Overall, a stabilizer can
418
increase EE% by changing hydrophobicity (HLB), rigidity, chain order and spacing between
419
tails of the lipid membrane.
420
The results of Wagner [46] showed higher EE of vitamin
421
sulfate (25.1%) in nano-niosomes. Palozza, et al. [47], in the study of nano-niosomes
422
containing beta-carotene, showed that the addition of cholesterol increased the encapsulation
423
efficiency.
424
Figure 4 (b) shows the loading capacity of the nano-niosomes. In general, the LC of all
425
samples was low which could be due to the initial degradation of vitamin
426
sonication and hydration). The highest LC is related to the sample containing cholesterol
427
(7%) and a sample containing polyethylene glycol (6.2%). The lowest LC is assigned to
428
sample N1` (2.4%). Considering that there was no significant difference in the LC of samples
429
containing vitamin E-acetate (N2 and N3).
Loading parameters
18
(95.9%) compared to iron
(during
430
3.
Conclusion
431
Niosomes provide a non-toxic and inexpensive vehicle for encapsulation of different
432
functional components (lipophilic, hydrophilic, and amphiphilic). In this study, the vitamin
433
D3 loaded nano-niosomes were produced by using a thin layer hydration method. The
434
resulted niosomes had nanometric size (<200 nm) and high encapsulation efficiency (>75%).
435
The different stabilizers were effective in enhancing of encapsulation efficiency and vitamin
436
E-acetate was the best stabilizer for this system due to the highest increasing effects on
437
encapsulation efficiency and antioxidant capacity.
438
4.
439
The authors gratefully acknowledge the support of the University of Tabriz and the support of
440
the Drug Applied Research Center of the Tabriz University of Medical Science.
441
5.
442
We wish to confirm that there are no known conflicts of interest associated with this
443
publication and there has been no significant financial support for this work that could have
444
influenced its outcome.
Acknowledgments
Conflict of Interest
445 446
6.
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Deliv. 10 (2003) 251-262.
537
[35] S.K. Mehta, N. Jindal, G. Kaur, Quantitative investigation, stability and in vitro release
538
studies of anti-TB drugs in Triton niosomes, Colloids Surf., B. 87 (2011) 173-179.
539
[36] A.A. Moghadamnia, S. Hakiminia, M. Baradaran, S. Kazemi, M. Ashraf-pour, Vitamin
540
D Improves Learning and Memory Impairment in Streptozotocin-Induced Diabetic Mice,
541
Arch. Iran. Med. 18 (2015).
542
[37] V.M. Di Mambro, A.E. Azzolini, Y.M. Valim, M.J. Fonseca, Comparison of antioxidant
543
activities of tocopherols alone and in pharmaceutical formulations, Int. J. Pharm. 262 (2003)
544
93-99.
545
[38] O. Krasodomska, P. Paolicelli, S. Cesa, M.A. Casadei, C. Jungnickel, Protection and
546
viability of fruit seeds oils by nanostructured lipid carrier (NLC) nanosuspensions, J. Colloid
547
Interface Sci. 479 (2016) 25-33.
548
[39] S. Soto-Jover, M. Boluda-Aguilar, A. López-Gómez, Influence of heating on stability of 23
549
γ-oryzanol in gluten-free ready meals, LWT-Food Sci. Technol. 65 (2016) 25-31.
550
[40] H. Cui, C. Zhao, L. Lin, The specific antibacterial activity of liposome-encapsulated
551
Clove oil and its application in tofu, Food Control. 56 (2015) 128-134.
552
[41] J. Araújo, S. Nikolic, M.A. Egea, E.B. Souto, M.L. Garcia, Nanostructured lipid carriers
553
for triamcinolone acetonide delivery to the posterior segment of the eye, Colloids Surf., B. 88
554
(2011) 150-157.
555
[42] F.K. Nahr, B. Ghanbarzadeh, H. Hamishehkar, H.S. Kafil, Food grade nanostructured
556
lipid carrier for cardamom essential oil: Preparation, characterization and antimicrobial
557
activity, J. Funct. Foods. 40 (2018) 1-8.
558
[43] M. Sun, S. Nie, X. Pan, R. Zhang, Z. Fan, S. Wang, Quercetin-nanostructured lipid
559
carriers: characteristics and anti-breast cancer activities in vitro, Colloids Surf., B 113 (2014)
560
15-24.
561
[44] M. Ravaghi, S.H. Razavi, S.M. Mousavi, C. Sinico, A.M. Fadda, Stabilization of natural
562
canthaxanthin produced by Dietzia natronolimnaea HS-1 by encapsulation in niosomes,
563
LWT-Food Sci. Technol. 73 (2016) 498-504.
564
[45] M. Wagner, Application Of Supercritical Carbon Dioxide In Lipid Vesicle Design And
565
Extraction Of Oil From Potato Chips, (2015).
566
[46] P. Palozza, R. Muzzalupo, S. Trombino, A. Valdannini, N. Picci, Solubilization and
567
stabilization of β-carotene in niosomes: delivery to cultured cells, Chem. Phys. Lipids. 139
568
(2006) 32-42.
569 570
24
571
Figure Captions
572
Figure 1. Effect of formulation on a) size; b) PDI; and c) zeta potential of nano-niosomes by
573
calculating standard deviation in three replicates (different letters indicate a significant
574
difference at the 5% probability level of Duncan test); d) Scanning electron microscopy of
575
nano-niosomes containing vitamin D3 (N1).
576
Figure 2. a) DSC curve of the control sample, the sample containing vitamin D3 and vitamin
577
D3;
578
containing Vitamin D3 (N1).
579
Figure 3. a) Percentage of inhibition of one ml of nano-niosome specimens on day one and
580
on day 30 after production; by calculating the mean and standard deviation in three replicates
581
(different letters indicate a significant difference at the 5% probability level according to
582
Duncan test); b) Changes in pH of formulations over a month; c) Turbidity of nano-niosomes
583
in the first and 30th days (similar letters indicate no significant difference at the 5% Duncan
584
test); d) The percentage of deposition of formulations at room temperature and inside the
585
refrigerator after 70 days.
586
Figure 4. Encapsulation efficiency and loading capacity of the formulation by calculating the
587
mean and standard deviation with three repetitions (different letters representing a significant
588
difference at the 5% probability level of Duncan's test).
b) FTIR spectrum for vitamin D3, blank nano-niosome (N0) and nano-niosome
589
25
b
a a
300
0.6
b
a a
0.5 d
200
0.4
150 gh gh
100
a
bc
f
gh h
d
ef e 0.2
g
50
0.1
0
0 N1
N2
N3
1st day
N4
N0
N5
40th day
d
cd
cd e
10 0
-20
f
f
f
-10
f
e bc
-30 N0
N1
N2
1st day
30 20
N1
N2
N3
d
b
N4
N5
Formulation 1st day
N3
N4
Formulation
c
a
b
cd
cd
0.3
Formulation
Zeta potential ( mV)
a
d
N0
590 591 592
b bc
c
PDI
Particle size (nm)
250
40th day
Figure 1
26
40th day
N5
593 594 595
Figure 2
596 597
27
a
60
a 6.8
50 40
6.6
c cd
fe
6.2
g
fg
30
6.4
cde def pH
Inhibition%
b
20
b
7
h
6 5.8
h h
5.6 5.4
10
5.2 0
5 N0
N1
N2
N3
N4
N5
0
5
10
N0 N3
30th day
b
d
0.7
e
0.6
e f
0.5 0.4 0.3 0.2 0.1
g h
N1 N4
N2 N5
d
25 20 15 10 5
g h
0
0 N0
N1
N2
N3
N4
N0
N5
1st day
N1
N2
N3
N4
N5
Formulation
Formulation
T=4 - 70th day
30th day
598 599
30
30
sedinantation%
Absorbance
35
b c
0.9 0.8
25
a
c
1
20
Day
Formulation 1st day
15
Figure 3
600 601 602 603 604 28
T=25 - 30th day
605 606 607 608 609 610 611 612
100 90 80 70 60 50 40 30 20 10 0
b a
e
d
c
b
Loading capacity %
Encapsulation efficiency%
a
N1
N2
N3
N4
a b
d
N1
N5
Formulation
613 614
10 9 8 7 6 5 4 3 2 1 0
c
c
N2
N3 Formulation
Figure 4
615 616 617 618 619 620 621 622 623 29
N4
N5
624
Table 1. The formulation used for the preparation of nano-niosomes Formulation JKL 60⁄NOPP 80 (mole ratio) Vitamin D3 (mmole) Vitamin E- acetate (mmole) Cholesterol (mmole) Polyethylene Glycol 400 (mmole)
N0
N1
N2
N3
N4
N5
3:2
3:2
3:2
3:2
3:2
3:2
-
0.02 -
0.02 0.01 -
0.02 0.02 -
0.02 0.06 -
0.02 0.06
625 626 627 628 629 630 631 632 633 634 635 636 637 638 639 640 641 642 643 644 645 646 647 648
30
649
Table 2. Melting and enthalpy temperature of the control sample, sample G. and vitamin Sample
Melting peak (oC)
Onset temperature (oC)
Endset temperature (oC)
Enthalpy (J/g)
N1
53
33.6
62.8
-36.4
Control (N0)
48
30.16
56.3
-10.7
Vitamin D3
91
82.98
98
-35.47
650 651 652 653 654 655 656 657 658 659 660 661 662 663 664 665 666 667 668 669 670 671 672 673 674 675 676 677 678 679 680 681 682 683 684 685 686 687 688 689
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33
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