- Email: [email protected]
Sunflower oil organogels and organogel-in-water emulsions (part I): Microstructure and mechanical properties
Accepted Manuscript Sunflower oil organogels and organogel-in-water emulsions (part I): microstructure and mechanical properties T. Moschakis, E. Panagiotopoulou, E. Katsanidis PII:
S0023-6438(16)30141-4
DOI:
10.1016/j.lwt.2016.03.004
Reference:
YFSTL 5344
To appear in:
LWT - Food Science and Technology
Received Date: 12 November 2015 Revised Date:
24 February 2016
Accepted Date: 4 March 2016
Please cite this article as: Moschakis, T., Panagiotopoulou, E., Katsanidis, E, Sunflower oil organogels and organogel-in-water emulsions (part I): microstructure and mechanical properties, LWT - Food Science and Technology (2016), doi: 10.1016/j.lwt.2016.03.004. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. 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.
ACCEPTED MANUSCRIPT 1
Sunflower oil organogels and organogel-in-water emulsions (part I): microstructure and
2
mechanical properties
3
Moschakis T., Panagiotopoulou, E. and Katsanidis, E*
5
RI PT
4
6
Department of Food Science and Technology, Faculty of Agriculture, Aristotle University of
7
Thessaloniki, P.O. Box 235, Thessaloniki, Greece
* Corresponding author at: Department of Food Science and Technology, Faculty of Agriculture,
M AN U
9
SC
8
10
Aristotle University of Thessaloniki, P.O. Box 235, Thessaloniki, Greece. Tel.: +30 2310991640; fax:
11
+30 2310991632.
12
E-mail address: [email protected] (E. Katsanidis).
TE D
13
Abstract
15
Currently, there is a growing interest for foods with not only sensorial quality, safety and
16
shelf stability but also providing health benefits through certain added ingredients. The aim of
17
the present study was to explore the potential use of vegetable oils structured with γ-oryzanol
18
and phytosterols as an alternative to animal fat with regard to mechanical properties.
19
Polarised microscopy and bulk rheological measurements have been employed to study the
20
microstructure and the mechanical properties of organogels and organogel-in-water
21
emulsions. Sterol ratio, total sterol content, storage duration and temperature were found to
22
substantially affect the properties of the oil structures, both in organogels and organogels-in-
23
water emulsions. However, the behaviour of the organogels structures does not always seem
24
to match with the organogel-in-water emulsions response. Modulating the sterol ratio and
25
total sterol content, the microstructure and mechanical properties of the vegetable oil
AC C
EP
14
1
ACCEPTED MANUSCRIPT 26
organogels and organogels-in-water emulsions could be modified to mimic the mechanical
27
properties of animal fat, without adversely affecting the textural quality and shelf-life of the
28
food products.
29
31
RI PT
30
Highlights
Mechanical properties of oil structures with γ-oryzanol & phytosterols were studied
33
Sterol ratio and sterol content affect the properties of the oil structures
34
Equimolar sterol structurant ratio resulted in stronger organogels
35
Excess phytosterols crystallise and enhance the stability of organogel emulsions
M AN U
SC
32
36 37
Keywords: organogels; organogel-based emulsions; phytosterols; γ-oryzanol; rheology
39 40
EP
TE D
38
1. Introduction
42
Organogels are gels where the liquid (continuous) phase is comprised of oil (M. A. Rogers,
43
2009) that is immobilized within a three-dimensional, cross-linked network. Mixtures of γ-
44
oryzanol and β-sitosterol, among others, are used as gelators to form three-dimensional
45
networked structures (Calligaris, Mirolo, Da Pieve, Arrighetti, & Nicoli, 2014; Nukit,
46
Setwipattanachai, Chaiseri, & Hongsprabhas, 2014; Sawalha et al., 2015). The oil structuring
47
ability of γ-οryzanol and different phytosterols is attributed to the formation of hollow
48
tubules of 7 nm diameter and just under 1 nm wall thickness (Bot, den Adel, Roijers, &
AC C
41
2
ACCEPTED MANUSCRIPT Regkos, 2009). The tubule formation is a synergistic phenomenon between the phytosterols
50
and γ-oryzanol, because individually neither one is capable of entrapping the oil phase (Bot
51
& Agterof, 2006), while the sterol molecules are dynamically transferring from tubules to
52
solution and vice versa (Sawalha et al., 2015). The oil phase is present both inside and
53
outside of the tubule (Bot, den Adel, et al., 2009).
54
The visual and mechanical properties of the organogels, e.g. firmness and transparency,
55
depend on the oryzanol-sitosterol ratio (Bot & Agterof, 2006; Bot, den Adel, & Roijers,
56
2008; Bot, Veldhuizen, den Adel, & Roijers, 2009). The turbidity of a sunflower oil gel
57
decreased with increasing γ-oryzanol concentration and the firmest transparent gel is usually
58
obtained at the ratio of 60:40 w/w oryzanol-sitosterol which corresponds to 1:1 molar ratio
59
(Bot & Agterof, 2006; Bot et al., 2008; Bot, Veldhuizen, et al., 2009). Modifications to the
60
ratio of phytosterols to γ-oryzanol affect not only the opacity of gels but also the aggregation
61
into tubules and the activation energy of nucleation (M. A. Rogers, Bot, Lam, Pedersen, &
62
May, 2010; Sawalha, Venema, Bot, Floter, & van der Linden, 2011).
63
Moreover, γ-oryzanol and phytosterols are capable of structuring o/w and w/o emulsions.
64
According to Duffy et al. (2009), oryzanol and sitosterol, under certain conditions, are
65
capable of forming fibril structures also in aqueous phase. The formation of tubular
66
microstructure in the oil phase of the emulsion can be promoted by reducing the water
67
activity and/or by using oil of low polarity (Sawalha et al., 2012). It has also been reported
68
that a mixture of oryzanol and sitosterol (16% in total, ratio 60:40) forms crystals in water
69
phase that can be related to the crystals of the pure compounds (Bot et al., 2011; den Adel,
70
Heussen, & Bot, 2010; Sawalha et al., 2012). Crystallization of the phytosterols in the
71
aqueous continuous phase takes place during and after the emulsification process (Duffy et
72
al., 2009). Phytosterols have surface activity, which would allow them to migrate to the oil–
73
water interface of the emulsion droplets (Cercaci, Rodriguez-Estrada, Lercker, & Decker,
AC C
EP
TE D
M AN U
SC
RI PT
49
3
ACCEPTED MANUSCRIPT 2007) and then to migrate to the water phase to form crystals. Previous research has shown
75
that the presence of water interferes with the capacity of the phytosterols to structure the
76
emulsion (Bot et al., 2011; Bot, Veldhuizen, et al., 2009; den Adel et al., 2010; Duffy et al.,
77
2009). However, in oil gels a completely different structure is formed which is not related to
78
the structures that are formed by both individual compounds, and which can be identified as a
79
self-assembled tubular structure involving both molecules of sitosterol and oryzanol (den
80
Adel et al., 2010).
81
γ-Oryzanol is extracted from rice bran oil and is derived from a fraction containing ferulate
82
(4-hydroxy-3-methoxycinnamic acid) esters of triterpene alcohols and plant sterols (E. J.
83
Rogers et al., 1993). It is considered to be an antioxidant compound which is associated with
84
decreasing plasma and serum cholesterol levels, cholesterol absorption and platelet
85
aggregation (Patel & Naik, 2004). β-Sitosterol is a phytosterol widespread in plants (Moreau,
86
Whitaker, & Hicks, 2002). Phytosterols are non-caloric compounds that occur naturally in
87
vegetable products (such as fruits and nuts) as well as oils (Brufau, Canela, & Rafecas, 2008).
88
Phytosterols appear to have bioactive properties and moderate dietary doses might have a
89
positive impact on human health, by decreasing cholesterol absorption (Sanclemente et al.,
90
2012). Dietary phytosterol supplementation of as little as 2 g per day has been reported to
91
cause, on average, a 13% LDL-cholesterol reduction, and a 10% total cholesterol reduction
92
(Romer & Garti, 2006).
93
Oleogels and their emulsions could be used as trans- or saturated (animal) fat replacements
94
and therefore, a better understanding of the factors affecting the mechanical properties and
95
their stability is needed. The aim of this study (Part I) was to investigate the microstructure
96
and the rheological properties of sunflower oil organogels and organogel-in-water emulsions
97
in an attempt to characterise the mechanical properties of these systems for their potential to
98
replace trans- or saturated aminal fat in structured food products.
AC C
EP
TE D
M AN U
SC
RI PT
74
4
ACCEPTED MANUSCRIPT 99
2. Materials & Methods
101
2.1 Materials
102
Sunflower oil and olive oil (Minerva SA, Metamorphosi, Greece) were obtained from the
103
local market. γ-Oryzanol was purchased from Jan Dekker Nederland B.V. (Wormerveer, the
104
Netherlands). Tetradecane was purchased from TCI Europe NV (Antwerp, Belgium) and
105
phytosterols (Vegapure 867G) were kindly provided by BASF Group (Ludwigshafen,
106
Germany). Tween® 20 and xanthan gum were obtained from Sigma-Aldrich (Hannover,
107
Germany). All aqueous solutions were prepared with double distilled water. In preliminary
108
experiments, sunflower lecithin (Solec™ SF-10, Solae Europe, S.A., Geneva, Switzerland)
109
was added to sunflower oil prior to heating. All other chemicals used were of analytical
110
grade.
M AN U
SC
RI PT
100
TE D
111
2.2 Preparation of organogels and organogel-based emulsions
113
Organogels. Two different γ-oryzanol:phytosterol weight ratios, 30:70 and 60:40, were used
114
in the preparation of sunflower oil solutions with total sterol content of 5%, 10%, 15% and
115
20% w/w. The 60:40 w/w oryzanol-phytosterol ratio gives the firmest transparent gel which
116
corresponds to 1:1 molar ratio (Bot & Agterof, 2006; Bot et al., 2008; Bot, Veldhuizen, et al.,
117
2009). On the contrary, in the 30:70 ratio, the phytosterols are in excess and thus the effect of
118
crystallization on the physicochemical properties of the organogels was investigated. A given
119
amount of γ-oryzanol and phytosterols was added in oil at ambient temperature. The solutions
120
were heated and maintained at the temperature range of 90-95 οC for 30 min, under constant
121
stirring. Subsequently, the samples were cooled and stored at 4 οC or 25 οC, depending on the
122
experimental procedure.
AC C
EP
112
5
ACCEPTED MANUSCRIPT Organogel-based emulsions. Organogel-in-water emulsions containing sterols at different
124
ratios (10% and 20% w/w total sterol content in the oil phase, 30:70 and 60:40 γ-oryzanol to
125
phytosterol weight ratio) were also prepared by mixing 50% w/w sunflower oil and 50% w/w
126
aqueous phase. The aqueous phase of the emulsions containing Tween 20 (1.7% w/w) and
127
xanthan gum (0.15% w/w) was heated up to 70 οC under stirring. The emulsions were
128
prepared by homogenising the oil containing the structurants (γ-oryzanol and phytosterol)
129
and the water phase using a high shear disperser (Ultra Turrax IKA T18 basic, IKA Works
130
Inc., Wilmington, USA) for 1 min at 14.000 rpm at temperature > 70 οC. The produced
131
emulsions were cooled immediately at ambient temperature and stored at 4 οC until further
132
examination.
M AN U
SC
RI PT
123
133
2.3 Optical Microscopy
135
Micrographs of the organogels and the organogel-in-water emulsions were captured by using
136
an Olympus BX51 (Olympus Optical Co Ltd, Tokyo, Japan) polarising microscope equipped
137
with a microscope digital camera (Olympus DP 70, Japan). The freshly prepared organogels
138
and organogel-based emulsions were placed onto a microscope slide with a cover glass and
139
were observed after 24h at ambient temperature without any further preparation.
EP
AC C
140
TE D
134
141
2.4 Large deformation measurements: Penetration Test
142
Penetration tests were performed in organogel samples on a TA-XT2i Texture Analyser
143
(Godalming, Surrey, UK) using a stainless steel cylindrical probe with a diameter of 6 mm.
144
Hot solutions of sunflower oil with 5%, 10%, 15% and 20% w/w sterols (30:70 and 60:40 γ-
145
oryzanol to phytosterol weight ratio) were poured into plastic cylindrical containers and
146
stored at 4 οC or 25 οC. After a period of approximately 24 h, in which gelation had taken
147
place, the organogels were removed and cut to self-sustained cylinders of 10 mm height and
6
ACCEPTED MANUSCRIPT 148
19 mm diameter. Penetration experiments were performed at a penetration speed of 0.5 mm s-
149
1
150
distance of 5 mm, corresponding to the 50% of the height of the samples. The parameters
151
extracted were hardness (N) as the maximum force that occurred during penetration and total
152
work for penetration defined as the gel strength (mJ) represented by the surface under the
153
force deformation curve (Vancamp & Huyghebaert, 1995; Verbeken, Bael, Thas, &
154
Dewettinck, 2006). At least five measurements were performed at ambient temperature for
155
each sample and the data were collected by using the software Texture Expert Version 1.22
156
of Stable Micro Systems (Godalming, Surrey, UK).
158 159
M AN U
157
SC
RI PT
(probe speed before and after penetration 1.0 mm s-1 and 5.0 mm s-1, respectively) over a
2.5 Rheological Measurements
161
The rheological properties of the organogel-based emulsions were studied by a rotational
162
Physica MCR 300 rheometer (Physica Messtechnic GmbH, Stuttgart, Germany) using a
163
parallel plate geometry (50 mm diameter and 1 mm gap); the temperature was regulated by a
164
Paar Physica circulating bath and a controlled peltier system (TEZ 150 P/MCR) with an
165
accuracy of ± 0.1 οC. The data of the rheological measurements were analysed with a
166
supporting rheometer software US200 V2.21. Two recordings were made per sample and
167
each measurement was carried out on two separate prepared samples (total four
168
measurements per sample). All tests were performed at 25 οC.
169
Initially, strain sweep tests were performed at 1 Hz for all the samples in order to determine
170
the linear viscoelastic region (LVR). Deviation from the linear viscoelastic region occurs
171
when the sample starts to permanently deform, implying the destruction of the transient
172
network structure. The apparent yield stress τy of the samples was determined as the stress at
AC C
EP
TE D
160
7
ACCEPTED MANUSCRIPT which the G' values begin to show a noticeable deviation of 10% from the LVR where the G'
174
remains constant.
175
A target strain of 0.5% was used in the subsequent experiments, which was within the LVR
176
for each sample examined. Small deformation oscillatory measurements for evaluation of the
177
viscoelastic properties, G' (storage modulus), G'' (loss modulus), and phase angle δ (defined
178
by tanδ= G''/G') were performed over the frequency range 0.1 to 100 Hz at 25 οC. In addition,
179
the flow behaviour of the samples was assessed by measuring steady shear viscosity η (Pa·s)
180
over a range of shear rates 0.001–100 s-1 at 25 οC.
SC
RI PT
173
181
2.2.7 Statistical Analysis
183
All data collected during measurements were analysed by using the General Linear Model.
184
Means were compared using Tukey’s multiple range test. All analyses were performed using
185
the Minitab (Minitab Inc., USA) statistical software.
M AN U
182
TE D
186
3. Results & Discussion
188
3.1 Organogels
189
3.1.1 Polarized microscopy
190
Figure 1 illustrates the microstructure of sunflower oil organogels with 10% and 20% w/w
191
structurants at different sterol weight ratios, 60:40 and 30:70 (γ-oryzanol:phytosterol), after
192
24h at ambient temperature. In the 30:70 samples (Figure 1 a & b), crystal formation of
193
sterols is favoured. The microstructure was studied under polarised light, thus the liquid oil
194
phase, optically isotropic, appears dark, while crystals appear as bright white features. The
195
crystals resemble typical phytosterol crystals observed in phytosterol-saturated oil systems
196
(Vaikousi, Lazaridou, Biliaderis, & Zawistowski, 2007). As can be seen from Figure 1a & b,
AC C
EP
187
8
ACCEPTED MANUSCRIPT a diverse crystal morphology is observed dependent on the sterol content. That is, at 20%
198
w/w sterol content sample (Figure 1 b), the size of the phytosterol crystals appears to be
199
larger and the shape seems to be more blade-shaped in comparison with needle-shaped
200
crystals at 10% w/w sterol content. On the other hand, the 60:40 sterol weight ratio, i.e. 1:1
201
molar ratio, has been characterised as ideal for creating sterol structured organogels (Pernetti,
202
van Malssen, Floter, & Bot, 2007). Indeed, in this ratio, no crystals were observed (Figure 1 c
203
& d), only some feather-like formations. These formations are likely to be the result of the
204
sterol fibrillar network, described by other researchers (Bot et al., 2008).
SC
RI PT
197
205
3.1.2 Mechanical properties
207
Effect of sterol content: Visual observations of olive and sunflower oil organogels at
208
concentrations of 5%, 10% and 20% w/w sterols and 60:40 weight ratio are shown in Figure
209
2.
210
The mixture of γ-oryzanol and plant sterols is capable of structuring a liquid fat of vegetable
211
origin (Pernetti et al., 2007). During preliminary experiments, it was found that dispersions of
212
6% w/w γ-oryzanol and 4% w/w phytosterols also exhibited significant mechanical properties
213
by using tetradecane oil as the liquid lipid phase (results not shown) implying that the
214
structuring effect occurs in non-vegetable origin oils. That is, at the equimolar oryzanol and
215
phytosterol ratio a network can be established in other apolar liquid solvents apart from the
216
polyunsaturated triglyceride oils. However, in this study only sunflower oil was selected as
217
the continuous phase of organogels to be further examined.
218
Organogels produced with 5% w/w sterol content were not free-standing, and thus they could
219
not be subjected to penetration tests even after being stored at ambient temperature for 10
220
days (Figure 2 a&b). On the other hand, the organogels of 10%, 15% and 20% w/w of sterols
221
were strong enough to be subjected to penetration tests 24 h after preparation. These results
AC C
EP
TE D
M AN U
206
9
ACCEPTED MANUSCRIPT indicate that total sterol content of 10%, 15% and 20% w/w developed a well-structured three
223
dimensional network at a very short time period at ambient temperature. Obviously, 5%
224
structurant concentration exhibited a time dependent gelation process, since it did not flow
225
upon container’s inversion 21 days after preparation (Figure 2 c&d). Similar results were
226
obtained in organogels produced with 30:70 weight γ-oryzanol:phytosterol ratio.
227
Hardness and gel strength of the organogels increased statistically significantly with
228
increasing total sterol content after 24 h storage at 25 oC (Figure 3 A).
RI PT
222
SC
229
Effect of sterol mass ratio: As previous research has shown, the sterol mass ratio affects in a
231
large extent the appearance and mechanical properties of organogels (Bot et al., 2008).
232
Modifying the oryzanol and phytosterol amount in the system, results in drastic changes to
233
the kinetics of the tubule self-assembly, as well as the final physical properties of the material
234
(M. A. Rogers et al., 2010). Indeed, the 60:40 ratio resulted in transparent gels while in the
235
case of 30:70 ratio more turbid gels were formed (results not shown). This implies that the
236
gel structuring blocks at 60:40 ratio are considerably smaller than the wavelength of visible
237
light (Pernetti et al., 2007). However, the turbidity at 30:70 gels can be explained by the
238
crystallization of excess phytosterols to large-scale structures, much larger than the fiber
239
structures of γ-oryzanol and phytosterol network (Bot et al., 2008). Moreover, according to
240
macroscopic observation, the 30:70 gels had an oily-greasy surface and were much softer
241
than those of 60:40 ratio at all total sterol contents tested. At high sterol levels, such as 20%
242
w/w, the 30:70 ratio exhibited a waxy-like texture and brittleness, opposed to the elastic
243
behaviour of 60:40 ratio. Indeed, the penetration test confirmed the increased (twofold)
244
hardness and gel strength of 60:40 sterol ratio gels in comparison to 30:70 ones in both sterol
245
contents examined (Figure 3 A). Assuming that both sterols are involved in the fibrillar
246
network at 60:40 ratio which corresponds to 1:1 molar ratio, then in 30:70 gels, the
AC C
EP
TE D
M AN U
230
10
ACCEPTED MANUSCRIPT phytosterols are in excess and therefore crystallize (see also Figure 1 a&b). Apparently, at
248
30:70 ratio there is not enough γ-oryzanol to associate with all the available phytosterols and
249
form the aforementioned fibrillar network. Thus, phytosterols in excess tend to crystallize. In
250
this case, a weaker fibrillar network is formed resulting in lower mechanical responses of the
251
30:70 organogels; i.e., the network formed by oryzanol and phytosterol seems to play the
252
important role in the overall mechanical properties.
RI PT
247
253
Effect of ageing: Hardness increased statistically significantly (p < 0.05) with time for both
255
total sterol concentrations and ratios (Figure 3 B). This implies that the gel network
256
undergoes reorganization, rearrangement and restructuring resulting in firmer gel networks.
257
This becomes more pronounced at longer times (see Figure 2 and total sterol content 5%
258
w/w). Nevertheless, although the absolute values of gel strength increased with time, no
259
statistically significant differences were detected (Figure 3 B).
M AN U
SC
254
TE D
260
Effect of storage temperature: The effect of two temperatures, 4 οC and 25 οC for 48h
262
storage, on hardness and gel strength was studied in 30:70 ratio organogels with 10% and
263
20% w/w total sterol content. Samples showed no differences in the macroscopic
264
examination. However, the penetration test (all the measurements were conducted at 25 oC
265
for uniformity reasons) indicated that by reducing the storage temperature, the hardness of
266
organogels increased statistically significantly for both samples (Figure 3 C). Undoubtedly, at
267
low temperatures (4 οC) crystal growth occurred more extensively and rapidly and thus
268
crystal-structured gels of 30:70 ratio became more resilient. Gel strength increased at 4 οC,
269
and statistically significant differences were detected only for the 20% w/w sample. These
270
results show that apart from its time dependence, gelation process is additionally temperature
271
dependent due to the enhanced interactions between the organogel components at higher
AC C
EP
261
11
ACCEPTED MANUSCRIPT 272
temperatures. Consequently, different sterol concentrations provide different levels of
273
structural organization. An increase in gel stability at low temperatures (5 οC) has been also
274
observed in rapeseed oil organogels with 12-hydroxy-stearic acid (M. A. Rogers, Wright, &
275
Marangoni, 2008).
RI PT
276
3.2 Organogel-based emulsions
278
3.2.1 Polarized microscopy
279
Sterol-structured organogels emulsified in water in the presence of Tween 20 and xanthan
280
gum led to organogel-in-water emulsions. The microstructure was studied under polarised
281
light (Figure 4), thus the liquid oil phase, optically isotropic, appears dark, while crystals
282
appear as bright white spots.
283
Irrespective of sterol weight ratio, 10% w/w organogels (Figure 4 a & c) produced stable
284
emulsions with small-sized oil droplets dispersed in the aqueous phase, where no crystal
285
formation was detected 24 h after storage at 4 οC. However, in 20% w/w organogel-based
286
emulsions of 30:70 ratio (Figure 4 b), numerous crystalline structures were observed. Crystals
287
were larger in the aqueous phase and limited due to the droplet size in the oil phase. Some of
288
the crystals (Fig. 4b) revealed in the micrographs – captured using polarised optical
289
microscopy – were larger than the emulsion droplets with irregular crystal morphology and
290
located in the water phase. In addition, flocculated and crystallised oil droplets that exhibit
291
birefringence were displayed in the micrograph. The presence of a non-adsorbing biopolymer
292
like xanthan leads to the formation of a transient but potentially long-lasting network from
293
emulsion droplets due to attractive depletion flocculation interactions (Thomas Moschakis,
294
2013; T. Moschakis, Murray, & Dickinson, 2006). This flocculation may have resulted in
295
partially crystalline oil droplets (partial coalescence) with marked increase in viscosity (see
296
section 3.2.2). Further experiments are needed to clarify this point.
AC C
EP
TE D
M AN U
SC
277
12
ACCEPTED MANUSCRIPT On the other hand, at the 60:40 ratio, no crystals were noticed even at 20% w/w sterols
298
(Figure 4 d). At 30:70 ratio (Figure 4 a & b), only at high sterol content used, i.e. 20% w/w
299
(Figure 4 b), the crystal formation was extensive. Thus, the γ-oryzanol:phytosterols weight
300
ratio seems to also play an important role in crystal formation in the produced emulsions.
301
Moreover, it has been found that structurants (γ-oryzanol and phytosterols), in the presence of
302
water, crystallise into forms similar to those that each sterol would individually form alone as
303
it has also been reported in other studies (Bot et al., 2011; den Adel et al., 2010; Duffy et al.,
304
2009). Basically, the water appears to inhibit or destabilize the tubular structures of sterols
305
that occur in organogels. The absence of crystalline features in 60:40 weight ratio is probably
306
due to the 1:1 molar ratio of sterols.
307
In general, the crystallization of a structurant spreads rapidly in the continuous phase once
308
initiated (Bot & Agterof, 2006; Bot, Veldhuizen, et al., 2009). However, in the case of an oil-
309
in-water emulsion, the oil phase is dispersed into the aqueous phase and therefore
310
crystallization or extensive crystal structure formation takes place more slowly since it has to
311
be initiated independently in each oil droplet (Bot & Agterof, 2006; Bot, Veldhuizen, et al.,
312
2009). Of course, the absence of large crystals at the time of the microscopic observation of
313
the emulsions, i.e., 24 h after preparation, does not preclude their creation in the future.
314
However, evolution of the emulsion microstructure over time was not further investigated in
315
the present study.
316
Lecithin has been reported as a phytosterol-crystallization inhibitor (Engel & Schubert,
317
2005). During preliminary experiments, sunflower lecithin was added before emulsification
318
to 30:70 organogel (lipid) phase of the emulsion along with sterols prior to heating, with the
319
aim to inhibit crystallization of plant sterols in excess. Surprisingly, in such an organogel-
320
based emulsion, lecithin not only did not inhibit the crystallization of phytosterols in excess
321
in the system, but on the contrary, numerous crystallization nuclei formed even in 10% w/w
AC C
EP
TE D
M AN U
SC
RI PT
297
13
ACCEPTED MANUSCRIPT total sterol content (Figure 5). Lecithin is commonly used as surfactant and crystal modifier.
323
According to Han et al. (2014) the addition of lecithin modifies the crystal morphology of
324
phytosterols. The addition of lecithin in the organogel phase probably interferes in the
325
crystallisation of phytosterols and led to more unstable emulsions and larger crystal structures
326
formation. Therefore, the morphology of phytosterol crystals seems to be related with the
327
stability of the organogel-based emulsions.
328
RI PT
322
3.2.2 Rheological measurements
330
Amplitude sweep. The shear-stress amplitude sweeps for organogel-based emulsions are
331
shown in Figure 6A. It is observed that the 30:70 samples exhibited longer linear viscoelastic
332
region (LVR) for both total sterol contents (10% and 20%). That is, the storage modulus
333
remained relatively constant over a broader range of shear stress applied in the emulsions
334
produced with 30:70 ratio. In addition, the 30:70 emulsion samples exhibited much higher G'
335
values at the LVR than the respective 60:40 samples.
336
The shear stress where a noticeable deviation from the linear viscoelastic region during the
337
strain sweep test occurs could be a rough estimate of the sample’s yield stress (Figure 6B).
338
Deviation from the LVR occurs when the sample starts to permanently deform, implying the
339
destruction of the structure. In this study, the tolerated deviation was defined as 10%.
340
Although the existence of yield stress has been questioned in the literature (Barnes, 1999), it
341
is a good indication of a gel network strength.
342
As can be seen from Figure 6, the 20%-30:70 emulsion gel exhibited the highest level of
343
internal structure against all other samples tested. Consequently, in contrast to organogels, the
344
crystallization of the excess phytosterols resulted in an overall stronger structure. This
345
reinforcement was not observed in organogels (without emulsion droplets) where the
346
equimolar sterol ratio plays the key role in mechanical properties. In emulsions, the increase
AC C
EP
TE D
M AN U
SC
329
14
ACCEPTED MANUSCRIPT in viscosity inside the oil droplets (caused by fibril formation from γ-oryzanol and
348
phytosterol) did not augment substantially the overall viscosity, whereas an enhancement of
349
the mechanical properties in the continuous phase and/or in the interconnected aggregated
350
crystallised (or partially crystallised) oil droplets phase, predominantly determines the
351
rheological behaviour of the overall bulk mechanical properties.
352
RI PT
347
Frequency sweep. Frequency sweep tests show that the elastic behaviour dominates in all the
354
organogel-in-water emulsions (Figure 7) since the G' was always higher than G'' over the
355
entire frequency range explored. However, a weak frequency dependence of the phase angle
356
was observed which is more pronounced for the samples containing 20% structurants
357
indicating a weak gel behaviour.
358
Figure 8 shows the G' and tanδ at 1 Hz of the emulsion gels. A large increase in G' was
359
obtained with increasing total sterol content while higher values were exhibited at 30:70
360
emulsions. The sterol ratio seems to affect the rheological properties of the organogel-in-
361
water emulsions. In addition, all emulsions had a dominant elastic character (tanδ < 1)
362
(Thomas Moschakis, 2013), and no statistical differences were found; i.e., the emulsions
363
exhibited the same elastic character independently of the sterol content and ratio (Figure 8).
M AN U
TE D
EP
AC C
364
SC
353
365
Large deformation steady-state viscometry. During large deformation steady-state
366
viscometry (Figure 9), the curves show pronounced shear-thinning behaviour, irrespectively
367
to sterol ratio and sterol content, and increasingly high viscosities at low-shear rates for
368
increasing sterol content and percentage of phytosterols in the sterol ratio (γ-
369
oryzanol:phytosterols ratio from 60:40 to 30:70) (Figure 9). This behaviour is typical of weak
370
associative interactions and suggests the formation of a weak droplet network structure.
371
Addition of xanthan in stable emulsions causes depletion flocculation, network formation,
15
ACCEPTED MANUSCRIPT and highly non-Newtonian and strongly shear thinning rheological behaviour (Thomas
373
Moschakis, 2013; T. Moschakis, Murray, & Dickinson, 2005; T. Moschakis et al., 2006). In
374
such systems, the rheological behaviour is dependent on the viscoelastic properties of the
375
interconnected depletion-flocculated network and not on the rheology of the aqueous
376
continuous phase (T. Moschakis et al., 2006).
377
At high oil volume fractions (e.g. 50%) the emulsion droplets begin to interact with each
378
other due to hydrodynamic interactions, apart from the colloidal interactions. As a result, the
379
viscosity of the system is modified. The hydrodynamic interactions are the result of the
380
relative motion of neighbouring particles (McClements, 2005), and are important in all types
381
of concentrated emulsions (say oil volume fraction > 0.4) (T. Moschakis et al., 2006). In
382
such systems, shear thinning occurs when the shear stress is large enough to overcome the
383
rotational but mainly translational Brownian motion of the emulsion droplets (McClements,
384
2005). As the shear stress increases, the hydrodynamic forces dominate, and thus
385
rearrangement and reordering of the emulsion droplets along the shearing occurs which cause
386
a decrease in the overall viscosity (shear- thinning behaviour). At low oil volume fractions
387
(20% wt % oil), enhanced shear thinning behaviour was exhibited only on systems that
388
extensive crystallization of phytosterols in the continuous phase was observed (unpublished
389
data).
390
When the phytosterols were added at higher proportions than γ-oryzanol (ratio 30:70),
391
crystals of phytosterols were formed, especially at high sterol content and upon storage (see
392
Figure 4), which enhances the overall viscosity. The low shear rate viscosity measured in
393
10%-30:70 emulsion was found to be ~90 Pa·s while for the 10%-60:40 emulsion was ~70
394
Pa·s illustrating the higher structural organization level in the first sample. At 20% total sterol
395
content, the low shear rate viscosity was an order of magnitude higher indicating that the
AC C
EP
TE D
M AN U
SC
RI PT
372
16
ACCEPTED MANUSCRIPT 396
enhancement in the organogel viscoelastic properties resulted in an substantial increase of the
397
overall bulk viscosity.
398
4. Conclusions
400
Sterol ratio, total sterol content, storage duration and temperature was found to define the
401
properties of the oil structures, both in organogels and organogels-in-water emulsions. In
402
30:70 sterol ratio, phytosterols in excess crystallize and therefore enhance the stability of the
403
system while the 60:40 ratio favours fibril formation. However, fibril formation resulted in
404
stronger gels indicating a remarkable fibril structuring effect on pure oil phase. On the
405
contrary, the 30:70 ratio, having excess amount of phytosterols, produced stronger emulsion
406
gels compared to the 60:40 ratio due to the interconnected aggregated crystallised (or
407
possibly partially crystallised) oil droplets and/or the enhancement of the mechanical
408
properties in the aqueous continuous phase containing phytosteol crystals. An increase in
409
total sterol content reinforced and amplified the structuring potential of both sterol ratios in
410
organogels and emulsions.
411
Vegetable oils structured with γ-oryzanol and phytosterols, undoubtedly, constitute a
412
noteworthy alternative to trans- or saturated (animal) fat. Vegetable oil gels could be utilized
413
in foods containing relatively high amounts of solid fat. Organogel-based emulsions, on the
414
other hand, are more appropriate for foods with emulsion composition such as margarine,
415
yoghurt, spread and processed cheese, mayonnaise and dressings.
SC
M AN U
TE D
EP
AC C
416
RI PT
399
417 418
5. References
419
17
ACCEPTED MANUSCRIPT
EP
TE D
M AN U
SC
RI PT
Barnes, H. A. (1999). The yield stress - a review or 'pi alpha nu tau alpha rho epsilon iota' - everything flows? Journal of Non-Newtonian Fluid Mechanics, 81(1-2), 133-178. doi: 10.1016/s03770257(98)00094-9 Bot, A., & Agterof, W. G. M. (2006). Structuring of edible oils by mixtures of gamma-oryzanol with beta-sitosterol or related phytosterols. Journal of the American Oil Chemists Society, 83(6), 513-521. doi: 10.1007/s11746-006-1234-7 Bot, A., den Adel, R., Regkos, C., Sawalha, H., Venema, P., & Floter, E. (2011). Structuring in betasitosterol plus gamma-oryzanol-based emulsion gels during various stages of a temperature cycle. Food Hydrocolloids, 25(4), 639-646. doi: 10.1016/j.foodhyd.2010.07.026 Bot, A., den Adel, R., & Roijers, E. C. (2008). Fibrils of gamma-oryzanol plus beta-sitosterol in edible oil organogels. Journal of the American Oil Chemists Society, 85(12), 1127-1134. doi: 10.1007/s11746-008-1298-7 Bot, A., den Adel, R., Roijers, E. C., & Regkos, C. (2009). Effect of sterol type on structure of tubules in sterol plus gamma-oryzanol-based organogels. Food Biophysics, 4(4), 266-272. doi: 10.1007/s11483-009-9124-9 Bot, A., Veldhuizen, Y. S. J., den Adel, R., & Roijers, E. C. (2009). Non-TAG structuring of edible oils and emulsions. Food Hydrocolloids, 23(4), 1184-1189. doi: 10.1016/j.foodhyd.2008.06.009 Brufau, G., Canela, M. A., & Rafecas, M. (2008). Phytosterols: physiologic and metabolic aspects related to cholesterol-lowering properties. Nutrition Research, 28(4), 217-225. doi: 10.1016/j.nutres.2008.02.003 Calligaris, S., Mirolo, G., Da Pieve, S., Arrighetti, G., & Nicoli, M. C. (2014). Effect of Oil Type on Formation, Structure and Thermal Properties of gamma-oryzanol and beta-sitosterol-Based Organogels. Food Biophysics, 9(1), 69-75. doi: 10.1007/s11483-013-9318-z Cercaci, L., Rodriguez-Estrada, M. T., Lercker, G., & Decker, E. A. (2007). Phytosterol oxidation in oilin-water emulsions and bulk oil. Food Chemistry, 102(1), 161-167. doi: 10.1016/j.foodchem.2006.05.010 den Adel, R., Heussen, P. C. M., & Bot, A. (2010). Effect of water on self-assembled tubules in betasitosterol plus gamma-oryzanol-based organogels. Xiv International Conference on SmallAngle Scattering (Sas09), 247. doi: 10.1088/1742-6596/247/1/012025 Duffy, N., Blonk, H. C. G., Beindorff, C. M., Cazade, M., Bot, A., & Duchateau, G. S. M. J. E. (2009). Organogel-based emulsion systems, micro-structural features and impact on in vitro digestion. Journal of the American Oil Chemists Society, 86(8), 733-741. doi: 10.1007/s11746009-1405-4 Engel, R., & Schubert, H. (2005). Formulation of phytosterols in emulsions for increased dose response in functional foods. Innovative Food Science & Emerging Technologies, 6(2), 233237. doi: 10.1016/j.ifset.2005.01.004 Han, L., Li, L., Li, B., Zhao, L., Liu, G.-q., Liu, X., & Wang, X. (2014). Structure and Physical Properties of Organogels Developed by Sitosterol and Lecithin with Sunflower Oil. Journal of the American Oil Chemists Society, 91(10), 1783-1792. doi: 10.1007/s11746-014-2526-y McClements, D. J. (2005). Food Emulsions: Principles, Practice, and Techniques (2nd ed.). Florida: CRC Press. Moreau, R. A., Whitaker, B. D., & Hicks, K. B. (2002). Phytosterols, phytostanols, and their conjugates in foods: structural diversity, quantitative analysis, and health-promoting uses. Progress in Lipid Research, 41(6), 457-500. doi: 10.1016/s0163-7827(02)00006-1 Moschakis, T. (2013). Microrheology and particle tracking in food gels and emulsions. Current Opinion in Colloid & Interface Science, 18(4), 311-323. doi: 10.1016/j.cocis.2013.04.011 Moschakis, T., Murray, B. S., & Dickinson, E. (2005). Microstructural evolution of viscoelastic emulsions stabilised by sodium caseinate and xanthan gum. Journal Of Colloid And Interface Science, 284(2), 714-728.
AC C
420 421 422 423 424 425 426 427 428 429 430 431 432 433 434 435 436 437 438 439 440 441 442 443 444 445 446 447 448 449 450 451 452 453 454 455 456 457 458 459 460 461 462 463 464 465 466 467 468
18
ACCEPTED MANUSCRIPT
EP
TE D
M AN U
SC
RI PT
Moschakis, T., Murray, B. S., & Dickinson, E. (2006). Particle tracking using confocal microscopy to probe the microrheology in a phase-separating emulsion containing nonadsorbing polysaccharide. Langmuir, 22(10), 4710-4719. doi: 10.1021/la0533258 Nukit, N., Setwipattanachai, P., Chaiseri, S., & Hongsprabhas, P. (2014). Effects of Surfactants and Aging Time on Solidification of Rice Bran Oil at Room Temperature. Journal of Oleo Science, 63(11), 1099-1107. doi: 10.5650/jos.ess14099 Patel, M., & Naik, S. N. (2004). Gamma-oryzanol from rice bran oil - A review. Journal of Scientific & Industrial Research, 63(7), 569-578. Pernetti, M., van Malssen, K. F., Floter, E., & Bot, A. (2007). Structuring of edible oils by alternatives to crystalline fat. Current Opinion in Colloid & Interface Science, 12(4-5), 221-231. doi: 10.1016/j.cocis.2007.07.002 Rogers, E. J., Rice, S. M., Nicolosi, R. J., Carpenter, D. R., McClelland, C. A., & Romanczyk, L. J. (1993). Identification and quantitation of gamma-oryzanol components and simultaneous assessment of tocols in rice bran oil. Journal of the American Oil Chemists Society, 70(3), 301-307. doi: 10.1007/bf02545312 Rogers, M. A. (2009). Novel structuring strategies for unsaturated fats - Meeting the zero-trans, zerosaturated fat challenge: A review. Food Research International, 42(7), 747-753. doi: 10.1016/j.foodres.2009.02.024 Rogers, M. A., Bot, A., Lam, R. S. H., Pedersen, T., & May, T. (2010). Multicomponent hollow tubules formed using phytosterol and gamma-oryzanol-based compounds: an understanding of their molecular embrace. Journal of Physical Chemistry A, 114(32), 8278-8285. doi: 10.1021/jp104101k Rogers, M. A., Wright, A. J., & Marangoni, A. G. (2008). Crystalline stability of self-assembled fibrillar networks of 12-hydroxystearic acid in edible oils. Food Research International, 41(10), 10261034. doi: 10.1016/j.foodres.2008.07.012 Romer, S., & Garti, N. (2006). The activity and absorption relationship of cholesterol and phytosterols. Colloids and Surfaces a-Physicochemical and Engineering Aspects, 282, 435456. doi: 10.1016/j.colsurfa.2005.12.032 Sanclemente, T., Marques-Lopes, I., Fajo-Pascual, M., Cofan, M., Jarauta, E., Ros, E., . . . Garcia-Otin, A. L. (2012). Naturally-occurring phytosterols in the usual diet influence cholesterol metabolism in healthy subjects. Nutrition Metabolism and Cardiovascular Diseases, 22(10), 849-855. doi: 10.1016/j.numecd.2011.01.010 Sawalha, H., den Adel, R., Venema, P., Bot, A., Floter, E., & van der Linden, E. (2012). Organogelemulsions with mixtures of beta-sitosterol and gamma-oryzanol: influence of water activity and type of oil phase on gelling capability. Journal of Agricultural and Food Chemistry, 60(13), 3462-3470. doi: 10.1021/jf300313f Sawalha, H., Venema, P., Bot, A., Floter, E., den Adel, R., & van der Linden, E. (2015). The Phase Behavior of gamma-Oryzanol and beta-Sitosterol in Edible Oil. Journal of the American Oil Chemists Society, 92(11-12), 1651-1659. doi: 10.1007/s11746-015-2731-3 Sawalha, H., Venema, P., Bot, A., Floter, E., & van der Linden, E. (2011). The influence of concentration and temperature on the formation of gamma-oryzanol + i-2-sitosterol tubules in edible oil organogels. Food Biophysics, 6(1), 20-25. doi: 10.1007/s11483-010-9169-9 Vaikousi, H., Lazaridou, A., Biliaderis, C. G., & Zawistowski, J. (2007). Phase transitions, solubility, and crystallization kinetics of phytosterols and phytosterol-oil blends. Journal of Agricultural and Food Chemistry, 55(5), 1790-1798. doi: 10.1021/jf0624289 Vancamp, J., & Huyghebaert, A. (1995). High pressure-induced gel formation of a whey-protein and hemoglobin protein-concentrate. Food Science and Technology-Lebensmittel-Wissenschaft & Technologie, 28(1), 111-117. Verbeken, D., Bael, K., Thas, O., & Dewettinck, K. (2006). Interactions between kappa-carrageenan, milk proteins and modified starch in sterilized dairy desserts. International Dairy Journal, 16(5), 482-488. doi: 10.1016/j.idairyj.2005.06.006
AC C
469 470 471 472 473 474 475 476 477 478 479 480 481 482 483 484 485 486 487 488 489 490 491 492 493 494 495 496 497 498 499 500 501 502 503 504 505 506 507 508 509 510 511 512 513 514 515 516 517 518 519
19
b
c
d
M AN U
SC
a
RI PT
ACCEPTED MANUSCRIPT
200 μm
Figure 1. Polarized micrographs of organogels, after storage at ambient temperature for 24 h; (a) 10% w/w sterol content 30:70 weight γ-oryzanol:phytosterol ratio, (b) 20% w/w - 30:70 γ-oryzanol:phytosterol, (c) 10% w/w - 60:40 γ-oryzanol:phytosterol and (d) 20%
AC C
EP
TE D
w/w - 60:40 γ-oryzanol:phytosterol.
ACCEPTED MANUSCRIPT
b
c
d
TE D
M AN U
SC
RI PT
a
EP
Figure 2. Vegetable oil organogels of 60:40 weight γ-oryzanol:phytosterol ratio in various total concentrations at ambient temperature; after 10 days storage (a) olive oil and
AC C
(b) sunflower oil, and after 21 days storage (c) olive oil and (d) sunflower oil. Total sterol concentration from left to right: 5%, 10%, 15%, 20% w/w.
ACCEPTED MANUSCRIPT
A
d
Hardness
Gel Strength
80 c 60 b D
40 a 20
C
B
A
0 10% - 30:70
RI PT
100
SC
Hardness (N), Gel Strength (mJ)
120
10% - 60:40
20% - 30:70
20% - 60:40
M AN U
Total sterol content (% w/w) - Oryzanol:phytosterol ratio
B
2d Hardness 10d Hardness 2d Gel Strength 10d Gel Strength
120
80 60
a
40 20
a
a
TE D
100
a
a
A B
A B
A B
EP
Hardness (N), Gel Strenth (mJ)
140
0
10%
15%
20%
AC C
Total sterol concentration (% w/w)
C
a
60
Hardness at 4 °C Hardness at 25 °C Gel Strength at 4 °C Gel strength at 25 °C
50 40
a b
a
30
a A
20 A
10
B
B
0 10%
20%
RI PT
Hardness (N), Gel strength (mJ)
ACCEPTED MANUSCRIPT
M AN U
SC
Total sterol content (% w/w)
Figure 3. Mechanical properties, hardness (N) and gel strength (mJ), of sunflower organogels with different total sterol contents (10% and 20% w/w). A) Effect of oryzanol-phytosterol weight ratio, 30:70 and 60:40, after 24 h storage at 25 °C.
°C.
TE D
B) Effect of storage time, 2 and 10 days at 60:40 oryzanol:phytosterol weight ratio at 25
C) Effect of temperature after 48h storage at 4 οC and 25 οC for the 30:70
EP
oryzanol:phytosterol weight ratio. Texture measurements were conducted at 25 °C. Means with different superscript letters are different (p < 0.05). The superscript letters for
AC C
Hardness are in capital (upper case) while in gel strength is in small (lower case)
b
c
d
200 μm
M AN U
SC
a
RI PT
ACCEPTED MANUSCRIPT
200 μm
Figure 4. Polarized micrographs of emulsions, after storage at 4 οC for 24 h. The emulsions contain 50% w/w aqueous phase and 50% w/w organogel; (a) 10% w/w sterol content 30:70 weight ratio, (b) 20% w/w - 30:70, (c) 10% w/w - 60:40 and (d) 20% w/w -
AC C
EP
TE D
60:40.
ACCEPTED MANUSCRIPT
b
SC
RI PT
a
Figure 5. Polarized micrographs of 30:70 organogel-based emulsions, after storage at 4 ο
C for 24 h. The emulsions contain 50% w/w aqueous phase and 50% w/w organogel: (a)
AC C
EP
TE D
M AN U
10% w/w sterol content and 1% w/w lecithin, (b) 20% w/w and 2% w/w lecithin.
ACCEPTED MANUSCRIPT
A
100
RI PT
10%-30:70 10%-60:40 20%-30:70 20%-60:40
SC
10
1 0.001
0.01
M AN U
Storage Modulus G' (Pa)
1000
0.1
1
10
100
Shear stress (Pa)
B
1.5 1.0
c
b
EP
2.0
a
AC C
Yield Stress τy (Pa)
2.5
TE D
3.0
0.5
a
0.0
10% 30:70
10% 60:40
20% 30:70
20% 60:40
Figure 6. Α) Strain sweep tests of organogel-based emulsions, after storage at 4 οC for 24 h. The emulsions contain 50% w/w aqueous phase and 50% w/w organogel
ACCEPTED MANUSCRIPT
Β) Yield stress τy (Pa) of organogel-based emulsions after storage at 4 οC for 24 h.
EP
TE D
M AN U
SC
RI PT
Means with different superscript letters are statistically different (p < 0.05)
AC C
ab
ACCEPTED MANUSCRIPT
B
10 1
0.1 0.1
1
Frequency (Hz)
1
tan δ
100 10
G' G'' tan δ
1
10
0.1
Frequency (Hz)
1.0
G' G'' tan δ
100
10
1
0.1
0.1
1
Frequency (Hz)
1000
100
M AN U
tan δ
G', G'' (Pa)
1000
10
10
SC
D
G', G'' (Pa)
C
0.1
1
10
1.0
tan δ
100
1000
G', G'' (Pa)
1
G' G'' tan δ
tan δ
G', G'' (Pa)
1000
RI PT
A
G' G'' tan δ
1
0.1
0.1 1
Frequency (Hz)
10
AC C
EP
TE D
Figure 7. Variation of G', G'' and tan δ as a function of frequency of organogel-in-water emulsions after storage at 4 οC for 24 h: (A) 10% w/w, 30:70 sterol ratio; (B) 20% w/w, 30:70 sterol ratio; (C) 10% w/w, 60:40 sterol ratio; (D) 20% w/w, 60:40 sterol ratio
ACCEPTED MANUSCRIPT
0,7
d
103 G' (1Hz) tanδ (1Hz)
c
0,5
a
b
10
a
a
a
0,4
0,3
10% 30:70
10% 60:40
20% 30:70
20% 60:40
M AN U
100
a
SC
1
tanδ
G' (Pa)
102
RI PT
0,6
Figure 8. Variation of G' and tanδ at 1 Hz among different organogel composition (30:70 and 60:40 γ-oryzanol:phytosterol weight ratio, 10% and 20% w/w total sterol content) of emulsion gels, after storage at 4 οC for 24 h.
EP
TE D
Means with different superscript letters are different (p < 0.05)
AC C
abc
ACCEPTED MANUSCRIPT 1 10000
10% 30:70 10% 60:40 20% 30:70 20% 60:40
100
10
1
0.1 0.001
0.01
0.1
Shear rate
2
1
10
(s-1)
SC
3
100
RI PT
Viscosity η (Pa·s)
1000
Figure 9. Shear rate (s-1) dependence of the viscosity η (Pa·s) of organogel-based emulsions
5
(30:70 and 60:40 sterol weight ratio, 10% and 20% w/w total sterol content), after storage at
6
4 οC for 24 h.
M AN U
4
7
AC C
EP
TE D
8
1
S0023-6438(16)30141-4
DOI:
10.1016/j.lwt.2016.03.004
Reference:
YFSTL 5344
To appear in:
LWT - Food Science and Technology
Received Date: 12 November 2015 Revised Date:
24 February 2016
Accepted Date: 4 March 2016
Please cite this article as: Moschakis, T., Panagiotopoulou, E., Katsanidis, E, Sunflower oil organogels and organogel-in-water emulsions (part I): microstructure and mechanical properties, LWT - Food Science and Technology (2016), doi: 10.1016/j.lwt.2016.03.004. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. 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.
ACCEPTED MANUSCRIPT 1
Sunflower oil organogels and organogel-in-water emulsions (part I): microstructure and
2
mechanical properties
3
Moschakis T., Panagiotopoulou, E. and Katsanidis, E*
5
RI PT
4
6
Department of Food Science and Technology, Faculty of Agriculture, Aristotle University of
7
Thessaloniki, P.O. Box 235, Thessaloniki, Greece
* Corresponding author at: Department of Food Science and Technology, Faculty of Agriculture,
M AN U
9
SC
8
10
Aristotle University of Thessaloniki, P.O. Box 235, Thessaloniki, Greece. Tel.: +30 2310991640; fax:
11
+30 2310991632.
12
E-mail address: [email protected] (E. Katsanidis).
TE D
13
Abstract
15
Currently, there is a growing interest for foods with not only sensorial quality, safety and
16
shelf stability but also providing health benefits through certain added ingredients. The aim of
17
the present study was to explore the potential use of vegetable oils structured with γ-oryzanol
18
and phytosterols as an alternative to animal fat with regard to mechanical properties.
19
Polarised microscopy and bulk rheological measurements have been employed to study the
20
microstructure and the mechanical properties of organogels and organogel-in-water
21
emulsions. Sterol ratio, total sterol content, storage duration and temperature were found to
22
substantially affect the properties of the oil structures, both in organogels and organogels-in-
23
water emulsions. However, the behaviour of the organogels structures does not always seem
24
to match with the organogel-in-water emulsions response. Modulating the sterol ratio and
25
total sterol content, the microstructure and mechanical properties of the vegetable oil
AC C
EP
14
1
ACCEPTED MANUSCRIPT 26
organogels and organogels-in-water emulsions could be modified to mimic the mechanical
27
properties of animal fat, without adversely affecting the textural quality and shelf-life of the
28
food products.
29
31
RI PT
30
Highlights
Mechanical properties of oil structures with γ-oryzanol & phytosterols were studied
33
Sterol ratio and sterol content affect the properties of the oil structures
34
Equimolar sterol structurant ratio resulted in stronger organogels
35
Excess phytosterols crystallise and enhance the stability of organogel emulsions
M AN U
SC
32
36 37
Keywords: organogels; organogel-based emulsions; phytosterols; γ-oryzanol; rheology
39 40
EP
TE D
38
1. Introduction
42
Organogels are gels where the liquid (continuous) phase is comprised of oil (M. A. Rogers,
43
2009) that is immobilized within a three-dimensional, cross-linked network. Mixtures of γ-
44
oryzanol and β-sitosterol, among others, are used as gelators to form three-dimensional
45
networked structures (Calligaris, Mirolo, Da Pieve, Arrighetti, & Nicoli, 2014; Nukit,
46
Setwipattanachai, Chaiseri, & Hongsprabhas, 2014; Sawalha et al., 2015). The oil structuring
47
ability of γ-οryzanol and different phytosterols is attributed to the formation of hollow
48
tubules of 7 nm diameter and just under 1 nm wall thickness (Bot, den Adel, Roijers, &
AC C
41
2
ACCEPTED MANUSCRIPT Regkos, 2009). The tubule formation is a synergistic phenomenon between the phytosterols
50
and γ-oryzanol, because individually neither one is capable of entrapping the oil phase (Bot
51
& Agterof, 2006), while the sterol molecules are dynamically transferring from tubules to
52
solution and vice versa (Sawalha et al., 2015). The oil phase is present both inside and
53
outside of the tubule (Bot, den Adel, et al., 2009).
54
The visual and mechanical properties of the organogels, e.g. firmness and transparency,
55
depend on the oryzanol-sitosterol ratio (Bot & Agterof, 2006; Bot, den Adel, & Roijers,
56
2008; Bot, Veldhuizen, den Adel, & Roijers, 2009). The turbidity of a sunflower oil gel
57
decreased with increasing γ-oryzanol concentration and the firmest transparent gel is usually
58
obtained at the ratio of 60:40 w/w oryzanol-sitosterol which corresponds to 1:1 molar ratio
59
(Bot & Agterof, 2006; Bot et al., 2008; Bot, Veldhuizen, et al., 2009). Modifications to the
60
ratio of phytosterols to γ-oryzanol affect not only the opacity of gels but also the aggregation
61
into tubules and the activation energy of nucleation (M. A. Rogers, Bot, Lam, Pedersen, &
62
May, 2010; Sawalha, Venema, Bot, Floter, & van der Linden, 2011).
63
Moreover, γ-oryzanol and phytosterols are capable of structuring o/w and w/o emulsions.
64
According to Duffy et al. (2009), oryzanol and sitosterol, under certain conditions, are
65
capable of forming fibril structures also in aqueous phase. The formation of tubular
66
microstructure in the oil phase of the emulsion can be promoted by reducing the water
67
activity and/or by using oil of low polarity (Sawalha et al., 2012). It has also been reported
68
that a mixture of oryzanol and sitosterol (16% in total, ratio 60:40) forms crystals in water
69
phase that can be related to the crystals of the pure compounds (Bot et al., 2011; den Adel,
70
Heussen, & Bot, 2010; Sawalha et al., 2012). Crystallization of the phytosterols in the
71
aqueous continuous phase takes place during and after the emulsification process (Duffy et
72
al., 2009). Phytosterols have surface activity, which would allow them to migrate to the oil–
73
water interface of the emulsion droplets (Cercaci, Rodriguez-Estrada, Lercker, & Decker,
AC C
EP
TE D
M AN U
SC
RI PT
49
3
ACCEPTED MANUSCRIPT 2007) and then to migrate to the water phase to form crystals. Previous research has shown
75
that the presence of water interferes with the capacity of the phytosterols to structure the
76
emulsion (Bot et al., 2011; Bot, Veldhuizen, et al., 2009; den Adel et al., 2010; Duffy et al.,
77
2009). However, in oil gels a completely different structure is formed which is not related to
78
the structures that are formed by both individual compounds, and which can be identified as a
79
self-assembled tubular structure involving both molecules of sitosterol and oryzanol (den
80
Adel et al., 2010).
81
γ-Oryzanol is extracted from rice bran oil and is derived from a fraction containing ferulate
82
(4-hydroxy-3-methoxycinnamic acid) esters of triterpene alcohols and plant sterols (E. J.
83
Rogers et al., 1993). It is considered to be an antioxidant compound which is associated with
84
decreasing plasma and serum cholesterol levels, cholesterol absorption and platelet
85
aggregation (Patel & Naik, 2004). β-Sitosterol is a phytosterol widespread in plants (Moreau,
86
Whitaker, & Hicks, 2002). Phytosterols are non-caloric compounds that occur naturally in
87
vegetable products (such as fruits and nuts) as well as oils (Brufau, Canela, & Rafecas, 2008).
88
Phytosterols appear to have bioactive properties and moderate dietary doses might have a
89
positive impact on human health, by decreasing cholesterol absorption (Sanclemente et al.,
90
2012). Dietary phytosterol supplementation of as little as 2 g per day has been reported to
91
cause, on average, a 13% LDL-cholesterol reduction, and a 10% total cholesterol reduction
92
(Romer & Garti, 2006).
93
Oleogels and their emulsions could be used as trans- or saturated (animal) fat replacements
94
and therefore, a better understanding of the factors affecting the mechanical properties and
95
their stability is needed. The aim of this study (Part I) was to investigate the microstructure
96
and the rheological properties of sunflower oil organogels and organogel-in-water emulsions
97
in an attempt to characterise the mechanical properties of these systems for their potential to
98
replace trans- or saturated aminal fat in structured food products.
AC C
EP
TE D
M AN U
SC
RI PT
74
4
ACCEPTED MANUSCRIPT 99
2. Materials & Methods
101
2.1 Materials
102
Sunflower oil and olive oil (Minerva SA, Metamorphosi, Greece) were obtained from the
103
local market. γ-Oryzanol was purchased from Jan Dekker Nederland B.V. (Wormerveer, the
104
Netherlands). Tetradecane was purchased from TCI Europe NV (Antwerp, Belgium) and
105
phytosterols (Vegapure 867G) were kindly provided by BASF Group (Ludwigshafen,
106
Germany). Tween® 20 and xanthan gum were obtained from Sigma-Aldrich (Hannover,
107
Germany). All aqueous solutions were prepared with double distilled water. In preliminary
108
experiments, sunflower lecithin (Solec™ SF-10, Solae Europe, S.A., Geneva, Switzerland)
109
was added to sunflower oil prior to heating. All other chemicals used were of analytical
110
grade.
M AN U
SC
RI PT
100
TE D
111
2.2 Preparation of organogels and organogel-based emulsions
113
Organogels. Two different γ-oryzanol:phytosterol weight ratios, 30:70 and 60:40, were used
114
in the preparation of sunflower oil solutions with total sterol content of 5%, 10%, 15% and
115
20% w/w. The 60:40 w/w oryzanol-phytosterol ratio gives the firmest transparent gel which
116
corresponds to 1:1 molar ratio (Bot & Agterof, 2006; Bot et al., 2008; Bot, Veldhuizen, et al.,
117
2009). On the contrary, in the 30:70 ratio, the phytosterols are in excess and thus the effect of
118
crystallization on the physicochemical properties of the organogels was investigated. A given
119
amount of γ-oryzanol and phytosterols was added in oil at ambient temperature. The solutions
120
were heated and maintained at the temperature range of 90-95 οC for 30 min, under constant
121
stirring. Subsequently, the samples were cooled and stored at 4 οC or 25 οC, depending on the
122
experimental procedure.
AC C
EP
112
5
ACCEPTED MANUSCRIPT Organogel-based emulsions. Organogel-in-water emulsions containing sterols at different
124
ratios (10% and 20% w/w total sterol content in the oil phase, 30:70 and 60:40 γ-oryzanol to
125
phytosterol weight ratio) were also prepared by mixing 50% w/w sunflower oil and 50% w/w
126
aqueous phase. The aqueous phase of the emulsions containing Tween 20 (1.7% w/w) and
127
xanthan gum (0.15% w/w) was heated up to 70 οC under stirring. The emulsions were
128
prepared by homogenising the oil containing the structurants (γ-oryzanol and phytosterol)
129
and the water phase using a high shear disperser (Ultra Turrax IKA T18 basic, IKA Works
130
Inc., Wilmington, USA) for 1 min at 14.000 rpm at temperature > 70 οC. The produced
131
emulsions were cooled immediately at ambient temperature and stored at 4 οC until further
132
examination.
M AN U
SC
RI PT
123
133
2.3 Optical Microscopy
135
Micrographs of the organogels and the organogel-in-water emulsions were captured by using
136
an Olympus BX51 (Olympus Optical Co Ltd, Tokyo, Japan) polarising microscope equipped
137
with a microscope digital camera (Olympus DP 70, Japan). The freshly prepared organogels
138
and organogel-based emulsions were placed onto a microscope slide with a cover glass and
139
were observed after 24h at ambient temperature without any further preparation.
EP
AC C
140
TE D
134
141
2.4 Large deformation measurements: Penetration Test
142
Penetration tests were performed in organogel samples on a TA-XT2i Texture Analyser
143
(Godalming, Surrey, UK) using a stainless steel cylindrical probe with a diameter of 6 mm.
144
Hot solutions of sunflower oil with 5%, 10%, 15% and 20% w/w sterols (30:70 and 60:40 γ-
145
oryzanol to phytosterol weight ratio) were poured into plastic cylindrical containers and
146
stored at 4 οC or 25 οC. After a period of approximately 24 h, in which gelation had taken
147
place, the organogels were removed and cut to self-sustained cylinders of 10 mm height and
6
ACCEPTED MANUSCRIPT 148
19 mm diameter. Penetration experiments were performed at a penetration speed of 0.5 mm s-
149
1
150
distance of 5 mm, corresponding to the 50% of the height of the samples. The parameters
151
extracted were hardness (N) as the maximum force that occurred during penetration and total
152
work for penetration defined as the gel strength (mJ) represented by the surface under the
153
force deformation curve (Vancamp & Huyghebaert, 1995; Verbeken, Bael, Thas, &
154
Dewettinck, 2006). At least five measurements were performed at ambient temperature for
155
each sample and the data were collected by using the software Texture Expert Version 1.22
156
of Stable Micro Systems (Godalming, Surrey, UK).
158 159
M AN U
157
SC
RI PT
(probe speed before and after penetration 1.0 mm s-1 and 5.0 mm s-1, respectively) over a
2.5 Rheological Measurements
161
The rheological properties of the organogel-based emulsions were studied by a rotational
162
Physica MCR 300 rheometer (Physica Messtechnic GmbH, Stuttgart, Germany) using a
163
parallel plate geometry (50 mm diameter and 1 mm gap); the temperature was regulated by a
164
Paar Physica circulating bath and a controlled peltier system (TEZ 150 P/MCR) with an
165
accuracy of ± 0.1 οC. The data of the rheological measurements were analysed with a
166
supporting rheometer software US200 V2.21. Two recordings were made per sample and
167
each measurement was carried out on two separate prepared samples (total four
168
measurements per sample). All tests were performed at 25 οC.
169
Initially, strain sweep tests were performed at 1 Hz for all the samples in order to determine
170
the linear viscoelastic region (LVR). Deviation from the linear viscoelastic region occurs
171
when the sample starts to permanently deform, implying the destruction of the transient
172
network structure. The apparent yield stress τy of the samples was determined as the stress at
AC C
EP
TE D
160
7
ACCEPTED MANUSCRIPT which the G' values begin to show a noticeable deviation of 10% from the LVR where the G'
174
remains constant.
175
A target strain of 0.5% was used in the subsequent experiments, which was within the LVR
176
for each sample examined. Small deformation oscillatory measurements for evaluation of the
177
viscoelastic properties, G' (storage modulus), G'' (loss modulus), and phase angle δ (defined
178
by tanδ= G''/G') were performed over the frequency range 0.1 to 100 Hz at 25 οC. In addition,
179
the flow behaviour of the samples was assessed by measuring steady shear viscosity η (Pa·s)
180
over a range of shear rates 0.001–100 s-1 at 25 οC.
SC
RI PT
173
181
2.2.7 Statistical Analysis
183
All data collected during measurements were analysed by using the General Linear Model.
184
Means were compared using Tukey’s multiple range test. All analyses were performed using
185
the Minitab (Minitab Inc., USA) statistical software.
M AN U
182
TE D
186
3. Results & Discussion
188
3.1 Organogels
189
3.1.1 Polarized microscopy
190
Figure 1 illustrates the microstructure of sunflower oil organogels with 10% and 20% w/w
191
structurants at different sterol weight ratios, 60:40 and 30:70 (γ-oryzanol:phytosterol), after
192
24h at ambient temperature. In the 30:70 samples (Figure 1 a & b), crystal formation of
193
sterols is favoured. The microstructure was studied under polarised light, thus the liquid oil
194
phase, optically isotropic, appears dark, while crystals appear as bright white features. The
195
crystals resemble typical phytosterol crystals observed in phytosterol-saturated oil systems
196
(Vaikousi, Lazaridou, Biliaderis, & Zawistowski, 2007). As can be seen from Figure 1a & b,
AC C
EP
187
8
ACCEPTED MANUSCRIPT a diverse crystal morphology is observed dependent on the sterol content. That is, at 20%
198
w/w sterol content sample (Figure 1 b), the size of the phytosterol crystals appears to be
199
larger and the shape seems to be more blade-shaped in comparison with needle-shaped
200
crystals at 10% w/w sterol content. On the other hand, the 60:40 sterol weight ratio, i.e. 1:1
201
molar ratio, has been characterised as ideal for creating sterol structured organogels (Pernetti,
202
van Malssen, Floter, & Bot, 2007). Indeed, in this ratio, no crystals were observed (Figure 1 c
203
& d), only some feather-like formations. These formations are likely to be the result of the
204
sterol fibrillar network, described by other researchers (Bot et al., 2008).
SC
RI PT
197
205
3.1.2 Mechanical properties
207
Effect of sterol content: Visual observations of olive and sunflower oil organogels at
208
concentrations of 5%, 10% and 20% w/w sterols and 60:40 weight ratio are shown in Figure
209
2.
210
The mixture of γ-oryzanol and plant sterols is capable of structuring a liquid fat of vegetable
211
origin (Pernetti et al., 2007). During preliminary experiments, it was found that dispersions of
212
6% w/w γ-oryzanol and 4% w/w phytosterols also exhibited significant mechanical properties
213
by using tetradecane oil as the liquid lipid phase (results not shown) implying that the
214
structuring effect occurs in non-vegetable origin oils. That is, at the equimolar oryzanol and
215
phytosterol ratio a network can be established in other apolar liquid solvents apart from the
216
polyunsaturated triglyceride oils. However, in this study only sunflower oil was selected as
217
the continuous phase of organogels to be further examined.
218
Organogels produced with 5% w/w sterol content were not free-standing, and thus they could
219
not be subjected to penetration tests even after being stored at ambient temperature for 10
220
days (Figure 2 a&b). On the other hand, the organogels of 10%, 15% and 20% w/w of sterols
221
were strong enough to be subjected to penetration tests 24 h after preparation. These results
AC C
EP
TE D
M AN U
206
9
ACCEPTED MANUSCRIPT indicate that total sterol content of 10%, 15% and 20% w/w developed a well-structured three
223
dimensional network at a very short time period at ambient temperature. Obviously, 5%
224
structurant concentration exhibited a time dependent gelation process, since it did not flow
225
upon container’s inversion 21 days after preparation (Figure 2 c&d). Similar results were
226
obtained in organogels produced with 30:70 weight γ-oryzanol:phytosterol ratio.
227
Hardness and gel strength of the organogels increased statistically significantly with
228
increasing total sterol content after 24 h storage at 25 oC (Figure 3 A).
RI PT
222
SC
229
Effect of sterol mass ratio: As previous research has shown, the sterol mass ratio affects in a
231
large extent the appearance and mechanical properties of organogels (Bot et al., 2008).
232
Modifying the oryzanol and phytosterol amount in the system, results in drastic changes to
233
the kinetics of the tubule self-assembly, as well as the final physical properties of the material
234
(M. A. Rogers et al., 2010). Indeed, the 60:40 ratio resulted in transparent gels while in the
235
case of 30:70 ratio more turbid gels were formed (results not shown). This implies that the
236
gel structuring blocks at 60:40 ratio are considerably smaller than the wavelength of visible
237
light (Pernetti et al., 2007). However, the turbidity at 30:70 gels can be explained by the
238
crystallization of excess phytosterols to large-scale structures, much larger than the fiber
239
structures of γ-oryzanol and phytosterol network (Bot et al., 2008). Moreover, according to
240
macroscopic observation, the 30:70 gels had an oily-greasy surface and were much softer
241
than those of 60:40 ratio at all total sterol contents tested. At high sterol levels, such as 20%
242
w/w, the 30:70 ratio exhibited a waxy-like texture and brittleness, opposed to the elastic
243
behaviour of 60:40 ratio. Indeed, the penetration test confirmed the increased (twofold)
244
hardness and gel strength of 60:40 sterol ratio gels in comparison to 30:70 ones in both sterol
245
contents examined (Figure 3 A). Assuming that both sterols are involved in the fibrillar
246
network at 60:40 ratio which corresponds to 1:1 molar ratio, then in 30:70 gels, the
AC C
EP
TE D
M AN U
230
10
ACCEPTED MANUSCRIPT phytosterols are in excess and therefore crystallize (see also Figure 1 a&b). Apparently, at
248
30:70 ratio there is not enough γ-oryzanol to associate with all the available phytosterols and
249
form the aforementioned fibrillar network. Thus, phytosterols in excess tend to crystallize. In
250
this case, a weaker fibrillar network is formed resulting in lower mechanical responses of the
251
30:70 organogels; i.e., the network formed by oryzanol and phytosterol seems to play the
252
important role in the overall mechanical properties.
RI PT
247
253
Effect of ageing: Hardness increased statistically significantly (p < 0.05) with time for both
255
total sterol concentrations and ratios (Figure 3 B). This implies that the gel network
256
undergoes reorganization, rearrangement and restructuring resulting in firmer gel networks.
257
This becomes more pronounced at longer times (see Figure 2 and total sterol content 5%
258
w/w). Nevertheless, although the absolute values of gel strength increased with time, no
259
statistically significant differences were detected (Figure 3 B).
M AN U
SC
254
TE D
260
Effect of storage temperature: The effect of two temperatures, 4 οC and 25 οC for 48h
262
storage, on hardness and gel strength was studied in 30:70 ratio organogels with 10% and
263
20% w/w total sterol content. Samples showed no differences in the macroscopic
264
examination. However, the penetration test (all the measurements were conducted at 25 oC
265
for uniformity reasons) indicated that by reducing the storage temperature, the hardness of
266
organogels increased statistically significantly for both samples (Figure 3 C). Undoubtedly, at
267
low temperatures (4 οC) crystal growth occurred more extensively and rapidly and thus
268
crystal-structured gels of 30:70 ratio became more resilient. Gel strength increased at 4 οC,
269
and statistically significant differences were detected only for the 20% w/w sample. These
270
results show that apart from its time dependence, gelation process is additionally temperature
271
dependent due to the enhanced interactions between the organogel components at higher
AC C
EP
261
11
ACCEPTED MANUSCRIPT 272
temperatures. Consequently, different sterol concentrations provide different levels of
273
structural organization. An increase in gel stability at low temperatures (5 οC) has been also
274
observed in rapeseed oil organogels with 12-hydroxy-stearic acid (M. A. Rogers, Wright, &
275
Marangoni, 2008).
RI PT
276
3.2 Organogel-based emulsions
278
3.2.1 Polarized microscopy
279
Sterol-structured organogels emulsified in water in the presence of Tween 20 and xanthan
280
gum led to organogel-in-water emulsions. The microstructure was studied under polarised
281
light (Figure 4), thus the liquid oil phase, optically isotropic, appears dark, while crystals
282
appear as bright white spots.
283
Irrespective of sterol weight ratio, 10% w/w organogels (Figure 4 a & c) produced stable
284
emulsions with small-sized oil droplets dispersed in the aqueous phase, where no crystal
285
formation was detected 24 h after storage at 4 οC. However, in 20% w/w organogel-based
286
emulsions of 30:70 ratio (Figure 4 b), numerous crystalline structures were observed. Crystals
287
were larger in the aqueous phase and limited due to the droplet size in the oil phase. Some of
288
the crystals (Fig. 4b) revealed in the micrographs – captured using polarised optical
289
microscopy – were larger than the emulsion droplets with irregular crystal morphology and
290
located in the water phase. In addition, flocculated and crystallised oil droplets that exhibit
291
birefringence were displayed in the micrograph. The presence of a non-adsorbing biopolymer
292
like xanthan leads to the formation of a transient but potentially long-lasting network from
293
emulsion droplets due to attractive depletion flocculation interactions (Thomas Moschakis,
294
2013; T. Moschakis, Murray, & Dickinson, 2006). This flocculation may have resulted in
295
partially crystalline oil droplets (partial coalescence) with marked increase in viscosity (see
296
section 3.2.2). Further experiments are needed to clarify this point.
AC C
EP
TE D
M AN U
SC
277
12
ACCEPTED MANUSCRIPT On the other hand, at the 60:40 ratio, no crystals were noticed even at 20% w/w sterols
298
(Figure 4 d). At 30:70 ratio (Figure 4 a & b), only at high sterol content used, i.e. 20% w/w
299
(Figure 4 b), the crystal formation was extensive. Thus, the γ-oryzanol:phytosterols weight
300
ratio seems to also play an important role in crystal formation in the produced emulsions.
301
Moreover, it has been found that structurants (γ-oryzanol and phytosterols), in the presence of
302
water, crystallise into forms similar to those that each sterol would individually form alone as
303
it has also been reported in other studies (Bot et al., 2011; den Adel et al., 2010; Duffy et al.,
304
2009). Basically, the water appears to inhibit or destabilize the tubular structures of sterols
305
that occur in organogels. The absence of crystalline features in 60:40 weight ratio is probably
306
due to the 1:1 molar ratio of sterols.
307
In general, the crystallization of a structurant spreads rapidly in the continuous phase once
308
initiated (Bot & Agterof, 2006; Bot, Veldhuizen, et al., 2009). However, in the case of an oil-
309
in-water emulsion, the oil phase is dispersed into the aqueous phase and therefore
310
crystallization or extensive crystal structure formation takes place more slowly since it has to
311
be initiated independently in each oil droplet (Bot & Agterof, 2006; Bot, Veldhuizen, et al.,
312
2009). Of course, the absence of large crystals at the time of the microscopic observation of
313
the emulsions, i.e., 24 h after preparation, does not preclude their creation in the future.
314
However, evolution of the emulsion microstructure over time was not further investigated in
315
the present study.
316
Lecithin has been reported as a phytosterol-crystallization inhibitor (Engel & Schubert,
317
2005). During preliminary experiments, sunflower lecithin was added before emulsification
318
to 30:70 organogel (lipid) phase of the emulsion along with sterols prior to heating, with the
319
aim to inhibit crystallization of plant sterols in excess. Surprisingly, in such an organogel-
320
based emulsion, lecithin not only did not inhibit the crystallization of phytosterols in excess
321
in the system, but on the contrary, numerous crystallization nuclei formed even in 10% w/w
AC C
EP
TE D
M AN U
SC
RI PT
297
13
ACCEPTED MANUSCRIPT total sterol content (Figure 5). Lecithin is commonly used as surfactant and crystal modifier.
323
According to Han et al. (2014) the addition of lecithin modifies the crystal morphology of
324
phytosterols. The addition of lecithin in the organogel phase probably interferes in the
325
crystallisation of phytosterols and led to more unstable emulsions and larger crystal structures
326
formation. Therefore, the morphology of phytosterol crystals seems to be related with the
327
stability of the organogel-based emulsions.
328
RI PT
322
3.2.2 Rheological measurements
330
Amplitude sweep. The shear-stress amplitude sweeps for organogel-based emulsions are
331
shown in Figure 6A. It is observed that the 30:70 samples exhibited longer linear viscoelastic
332
region (LVR) for both total sterol contents (10% and 20%). That is, the storage modulus
333
remained relatively constant over a broader range of shear stress applied in the emulsions
334
produced with 30:70 ratio. In addition, the 30:70 emulsion samples exhibited much higher G'
335
values at the LVR than the respective 60:40 samples.
336
The shear stress where a noticeable deviation from the linear viscoelastic region during the
337
strain sweep test occurs could be a rough estimate of the sample’s yield stress (Figure 6B).
338
Deviation from the LVR occurs when the sample starts to permanently deform, implying the
339
destruction of the structure. In this study, the tolerated deviation was defined as 10%.
340
Although the existence of yield stress has been questioned in the literature (Barnes, 1999), it
341
is a good indication of a gel network strength.
342
As can be seen from Figure 6, the 20%-30:70 emulsion gel exhibited the highest level of
343
internal structure against all other samples tested. Consequently, in contrast to organogels, the
344
crystallization of the excess phytosterols resulted in an overall stronger structure. This
345
reinforcement was not observed in organogels (without emulsion droplets) where the
346
equimolar sterol ratio plays the key role in mechanical properties. In emulsions, the increase
AC C
EP
TE D
M AN U
SC
329
14
ACCEPTED MANUSCRIPT in viscosity inside the oil droplets (caused by fibril formation from γ-oryzanol and
348
phytosterol) did not augment substantially the overall viscosity, whereas an enhancement of
349
the mechanical properties in the continuous phase and/or in the interconnected aggregated
350
crystallised (or partially crystallised) oil droplets phase, predominantly determines the
351
rheological behaviour of the overall bulk mechanical properties.
352
RI PT
347
Frequency sweep. Frequency sweep tests show that the elastic behaviour dominates in all the
354
organogel-in-water emulsions (Figure 7) since the G' was always higher than G'' over the
355
entire frequency range explored. However, a weak frequency dependence of the phase angle
356
was observed which is more pronounced for the samples containing 20% structurants
357
indicating a weak gel behaviour.
358
Figure 8 shows the G' and tanδ at 1 Hz of the emulsion gels. A large increase in G' was
359
obtained with increasing total sterol content while higher values were exhibited at 30:70
360
emulsions. The sterol ratio seems to affect the rheological properties of the organogel-in-
361
water emulsions. In addition, all emulsions had a dominant elastic character (tanδ < 1)
362
(Thomas Moschakis, 2013), and no statistical differences were found; i.e., the emulsions
363
exhibited the same elastic character independently of the sterol content and ratio (Figure 8).
M AN U
TE D
EP
AC C
364
SC
353
365
Large deformation steady-state viscometry. During large deformation steady-state
366
viscometry (Figure 9), the curves show pronounced shear-thinning behaviour, irrespectively
367
to sterol ratio and sterol content, and increasingly high viscosities at low-shear rates for
368
increasing sterol content and percentage of phytosterols in the sterol ratio (γ-
369
oryzanol:phytosterols ratio from 60:40 to 30:70) (Figure 9). This behaviour is typical of weak
370
associative interactions and suggests the formation of a weak droplet network structure.
371
Addition of xanthan in stable emulsions causes depletion flocculation, network formation,
15
ACCEPTED MANUSCRIPT and highly non-Newtonian and strongly shear thinning rheological behaviour (Thomas
373
Moschakis, 2013; T. Moschakis, Murray, & Dickinson, 2005; T. Moschakis et al., 2006). In
374
such systems, the rheological behaviour is dependent on the viscoelastic properties of the
375
interconnected depletion-flocculated network and not on the rheology of the aqueous
376
continuous phase (T. Moschakis et al., 2006).
377
At high oil volume fractions (e.g. 50%) the emulsion droplets begin to interact with each
378
other due to hydrodynamic interactions, apart from the colloidal interactions. As a result, the
379
viscosity of the system is modified. The hydrodynamic interactions are the result of the
380
relative motion of neighbouring particles (McClements, 2005), and are important in all types
381
of concentrated emulsions (say oil volume fraction > 0.4) (T. Moschakis et al., 2006). In
382
such systems, shear thinning occurs when the shear stress is large enough to overcome the
383
rotational but mainly translational Brownian motion of the emulsion droplets (McClements,
384
2005). As the shear stress increases, the hydrodynamic forces dominate, and thus
385
rearrangement and reordering of the emulsion droplets along the shearing occurs which cause
386
a decrease in the overall viscosity (shear- thinning behaviour). At low oil volume fractions
387
(20% wt % oil), enhanced shear thinning behaviour was exhibited only on systems that
388
extensive crystallization of phytosterols in the continuous phase was observed (unpublished
389
data).
390
When the phytosterols were added at higher proportions than γ-oryzanol (ratio 30:70),
391
crystals of phytosterols were formed, especially at high sterol content and upon storage (see
392
Figure 4), which enhances the overall viscosity. The low shear rate viscosity measured in
393
10%-30:70 emulsion was found to be ~90 Pa·s while for the 10%-60:40 emulsion was ~70
394
Pa·s illustrating the higher structural organization level in the first sample. At 20% total sterol
395
content, the low shear rate viscosity was an order of magnitude higher indicating that the
AC C
EP
TE D
M AN U
SC
RI PT
372
16
ACCEPTED MANUSCRIPT 396
enhancement in the organogel viscoelastic properties resulted in an substantial increase of the
397
overall bulk viscosity.
398
4. Conclusions
400
Sterol ratio, total sterol content, storage duration and temperature was found to define the
401
properties of the oil structures, both in organogels and organogels-in-water emulsions. In
402
30:70 sterol ratio, phytosterols in excess crystallize and therefore enhance the stability of the
403
system while the 60:40 ratio favours fibril formation. However, fibril formation resulted in
404
stronger gels indicating a remarkable fibril structuring effect on pure oil phase. On the
405
contrary, the 30:70 ratio, having excess amount of phytosterols, produced stronger emulsion
406
gels compared to the 60:40 ratio due to the interconnected aggregated crystallised (or
407
possibly partially crystallised) oil droplets and/or the enhancement of the mechanical
408
properties in the aqueous continuous phase containing phytosteol crystals. An increase in
409
total sterol content reinforced and amplified the structuring potential of both sterol ratios in
410
organogels and emulsions.
411
Vegetable oils structured with γ-oryzanol and phytosterols, undoubtedly, constitute a
412
noteworthy alternative to trans- or saturated (animal) fat. Vegetable oil gels could be utilized
413
in foods containing relatively high amounts of solid fat. Organogel-based emulsions, on the
414
other hand, are more appropriate for foods with emulsion composition such as margarine,
415
yoghurt, spread and processed cheese, mayonnaise and dressings.
SC
M AN U
TE D
EP
AC C
416
RI PT
399
417 418
5. References
419
17
ACCEPTED MANUSCRIPT
EP
TE D
M AN U
SC
RI PT
Barnes, H. A. (1999). The yield stress - a review or 'pi alpha nu tau alpha rho epsilon iota' - everything flows? Journal of Non-Newtonian Fluid Mechanics, 81(1-2), 133-178. doi: 10.1016/s03770257(98)00094-9 Bot, A., & Agterof, W. G. M. (2006). Structuring of edible oils by mixtures of gamma-oryzanol with beta-sitosterol or related phytosterols. Journal of the American Oil Chemists Society, 83(6), 513-521. doi: 10.1007/s11746-006-1234-7 Bot, A., den Adel, R., Regkos, C., Sawalha, H., Venema, P., & Floter, E. (2011). Structuring in betasitosterol plus gamma-oryzanol-based emulsion gels during various stages of a temperature cycle. Food Hydrocolloids, 25(4), 639-646. doi: 10.1016/j.foodhyd.2010.07.026 Bot, A., den Adel, R., & Roijers, E. C. (2008). Fibrils of gamma-oryzanol plus beta-sitosterol in edible oil organogels. Journal of the American Oil Chemists Society, 85(12), 1127-1134. doi: 10.1007/s11746-008-1298-7 Bot, A., den Adel, R., Roijers, E. C., & Regkos, C. (2009). Effect of sterol type on structure of tubules in sterol plus gamma-oryzanol-based organogels. Food Biophysics, 4(4), 266-272. doi: 10.1007/s11483-009-9124-9 Bot, A., Veldhuizen, Y. S. J., den Adel, R., & Roijers, E. C. (2009). Non-TAG structuring of edible oils and emulsions. Food Hydrocolloids, 23(4), 1184-1189. doi: 10.1016/j.foodhyd.2008.06.009 Brufau, G., Canela, M. A., & Rafecas, M. (2008). Phytosterols: physiologic and metabolic aspects related to cholesterol-lowering properties. Nutrition Research, 28(4), 217-225. doi: 10.1016/j.nutres.2008.02.003 Calligaris, S., Mirolo, G., Da Pieve, S., Arrighetti, G., & Nicoli, M. C. (2014). Effect of Oil Type on Formation, Structure and Thermal Properties of gamma-oryzanol and beta-sitosterol-Based Organogels. Food Biophysics, 9(1), 69-75. doi: 10.1007/s11483-013-9318-z Cercaci, L., Rodriguez-Estrada, M. T., Lercker, G., & Decker, E. A. (2007). Phytosterol oxidation in oilin-water emulsions and bulk oil. Food Chemistry, 102(1), 161-167. doi: 10.1016/j.foodchem.2006.05.010 den Adel, R., Heussen, P. C. M., & Bot, A. (2010). Effect of water on self-assembled tubules in betasitosterol plus gamma-oryzanol-based organogels. Xiv International Conference on SmallAngle Scattering (Sas09), 247. doi: 10.1088/1742-6596/247/1/012025 Duffy, N., Blonk, H. C. G., Beindorff, C. M., Cazade, M., Bot, A., & Duchateau, G. S. M. J. E. (2009). Organogel-based emulsion systems, micro-structural features and impact on in vitro digestion. Journal of the American Oil Chemists Society, 86(8), 733-741. doi: 10.1007/s11746009-1405-4 Engel, R., & Schubert, H. (2005). Formulation of phytosterols in emulsions for increased dose response in functional foods. Innovative Food Science & Emerging Technologies, 6(2), 233237. doi: 10.1016/j.ifset.2005.01.004 Han, L., Li, L., Li, B., Zhao, L., Liu, G.-q., Liu, X., & Wang, X. (2014). Structure and Physical Properties of Organogels Developed by Sitosterol and Lecithin with Sunflower Oil. Journal of the American Oil Chemists Society, 91(10), 1783-1792. doi: 10.1007/s11746-014-2526-y McClements, D. J. (2005). Food Emulsions: Principles, Practice, and Techniques (2nd ed.). Florida: CRC Press. Moreau, R. A., Whitaker, B. D., & Hicks, K. B. (2002). Phytosterols, phytostanols, and their conjugates in foods: structural diversity, quantitative analysis, and health-promoting uses. Progress in Lipid Research, 41(6), 457-500. doi: 10.1016/s0163-7827(02)00006-1 Moschakis, T. (2013). Microrheology and particle tracking in food gels and emulsions. Current Opinion in Colloid & Interface Science, 18(4), 311-323. doi: 10.1016/j.cocis.2013.04.011 Moschakis, T., Murray, B. S., & Dickinson, E. (2005). Microstructural evolution of viscoelastic emulsions stabilised by sodium caseinate and xanthan gum. Journal Of Colloid And Interface Science, 284(2), 714-728.
AC C
420 421 422 423 424 425 426 427 428 429 430 431 432 433 434 435 436 437 438 439 440 441 442 443 444 445 446 447 448 449 450 451 452 453 454 455 456 457 458 459 460 461 462 463 464 465 466 467 468
18
ACCEPTED MANUSCRIPT
EP
TE D
M AN U
SC
RI PT
Moschakis, T., Murray, B. S., & Dickinson, E. (2006). Particle tracking using confocal microscopy to probe the microrheology in a phase-separating emulsion containing nonadsorbing polysaccharide. Langmuir, 22(10), 4710-4719. doi: 10.1021/la0533258 Nukit, N., Setwipattanachai, P., Chaiseri, S., & Hongsprabhas, P. (2014). Effects of Surfactants and Aging Time on Solidification of Rice Bran Oil at Room Temperature. Journal of Oleo Science, 63(11), 1099-1107. doi: 10.5650/jos.ess14099 Patel, M., & Naik, S. N. (2004). Gamma-oryzanol from rice bran oil - A review. Journal of Scientific & Industrial Research, 63(7), 569-578. Pernetti, M., van Malssen, K. F., Floter, E., & Bot, A. (2007). Structuring of edible oils by alternatives to crystalline fat. Current Opinion in Colloid & Interface Science, 12(4-5), 221-231. doi: 10.1016/j.cocis.2007.07.002 Rogers, E. J., Rice, S. M., Nicolosi, R. J., Carpenter, D. R., McClelland, C. A., & Romanczyk, L. J. (1993). Identification and quantitation of gamma-oryzanol components and simultaneous assessment of tocols in rice bran oil. Journal of the American Oil Chemists Society, 70(3), 301-307. doi: 10.1007/bf02545312 Rogers, M. A. (2009). Novel structuring strategies for unsaturated fats - Meeting the zero-trans, zerosaturated fat challenge: A review. Food Research International, 42(7), 747-753. doi: 10.1016/j.foodres.2009.02.024 Rogers, M. A., Bot, A., Lam, R. S. H., Pedersen, T., & May, T. (2010). Multicomponent hollow tubules formed using phytosterol and gamma-oryzanol-based compounds: an understanding of their molecular embrace. Journal of Physical Chemistry A, 114(32), 8278-8285. doi: 10.1021/jp104101k Rogers, M. A., Wright, A. J., & Marangoni, A. G. (2008). Crystalline stability of self-assembled fibrillar networks of 12-hydroxystearic acid in edible oils. Food Research International, 41(10), 10261034. doi: 10.1016/j.foodres.2008.07.012 Romer, S., & Garti, N. (2006). The activity and absorption relationship of cholesterol and phytosterols. Colloids and Surfaces a-Physicochemical and Engineering Aspects, 282, 435456. doi: 10.1016/j.colsurfa.2005.12.032 Sanclemente, T., Marques-Lopes, I., Fajo-Pascual, M., Cofan, M., Jarauta, E., Ros, E., . . . Garcia-Otin, A. L. (2012). Naturally-occurring phytosterols in the usual diet influence cholesterol metabolism in healthy subjects. Nutrition Metabolism and Cardiovascular Diseases, 22(10), 849-855. doi: 10.1016/j.numecd.2011.01.010 Sawalha, H., den Adel, R., Venema, P., Bot, A., Floter, E., & van der Linden, E. (2012). Organogelemulsions with mixtures of beta-sitosterol and gamma-oryzanol: influence of water activity and type of oil phase on gelling capability. Journal of Agricultural and Food Chemistry, 60(13), 3462-3470. doi: 10.1021/jf300313f Sawalha, H., Venema, P., Bot, A., Floter, E., den Adel, R., & van der Linden, E. (2015). The Phase Behavior of gamma-Oryzanol and beta-Sitosterol in Edible Oil. Journal of the American Oil Chemists Society, 92(11-12), 1651-1659. doi: 10.1007/s11746-015-2731-3 Sawalha, H., Venema, P., Bot, A., Floter, E., & van der Linden, E. (2011). The influence of concentration and temperature on the formation of gamma-oryzanol + i-2-sitosterol tubules in edible oil organogels. Food Biophysics, 6(1), 20-25. doi: 10.1007/s11483-010-9169-9 Vaikousi, H., Lazaridou, A., Biliaderis, C. G., & Zawistowski, J. (2007). Phase transitions, solubility, and crystallization kinetics of phytosterols and phytosterol-oil blends. Journal of Agricultural and Food Chemistry, 55(5), 1790-1798. doi: 10.1021/jf0624289 Vancamp, J., & Huyghebaert, A. (1995). High pressure-induced gel formation of a whey-protein and hemoglobin protein-concentrate. Food Science and Technology-Lebensmittel-Wissenschaft & Technologie, 28(1), 111-117. Verbeken, D., Bael, K., Thas, O., & Dewettinck, K. (2006). Interactions between kappa-carrageenan, milk proteins and modified starch in sterilized dairy desserts. International Dairy Journal, 16(5), 482-488. doi: 10.1016/j.idairyj.2005.06.006
AC C
469 470 471 472 473 474 475 476 477 478 479 480 481 482 483 484 485 486 487 488 489 490 491 492 493 494 495 496 497 498 499 500 501 502 503 504 505 506 507 508 509 510 511 512 513 514 515 516 517 518 519
19
b
c
d
M AN U
SC
a
RI PT
ACCEPTED MANUSCRIPT
200 μm
Figure 1. Polarized micrographs of organogels, after storage at ambient temperature for 24 h; (a) 10% w/w sterol content 30:70 weight γ-oryzanol:phytosterol ratio, (b) 20% w/w - 30:70 γ-oryzanol:phytosterol, (c) 10% w/w - 60:40 γ-oryzanol:phytosterol and (d) 20%
AC C
EP
TE D
w/w - 60:40 γ-oryzanol:phytosterol.
ACCEPTED MANUSCRIPT
b
c
d
TE D
M AN U
SC
RI PT
a
EP
Figure 2. Vegetable oil organogels of 60:40 weight γ-oryzanol:phytosterol ratio in various total concentrations at ambient temperature; after 10 days storage (a) olive oil and
AC C
(b) sunflower oil, and after 21 days storage (c) olive oil and (d) sunflower oil. Total sterol concentration from left to right: 5%, 10%, 15%, 20% w/w.
ACCEPTED MANUSCRIPT
A
d
Hardness
Gel Strength
80 c 60 b D
40 a 20
C
B
A
0 10% - 30:70
RI PT
100
SC
Hardness (N), Gel Strength (mJ)
120
10% - 60:40
20% - 30:70
20% - 60:40
M AN U
Total sterol content (% w/w) - Oryzanol:phytosterol ratio
B
2d Hardness 10d Hardness 2d Gel Strength 10d Gel Strength
120
80 60
a
40 20
a
a
TE D
100
a
a
A B
A B
A B
EP
Hardness (N), Gel Strenth (mJ)
140
0
10%
15%
20%
AC C
Total sterol concentration (% w/w)
C
a
60
Hardness at 4 °C Hardness at 25 °C Gel Strength at 4 °C Gel strength at 25 °C
50 40
a b
a
30
a A
20 A
10
B
B
0 10%
20%
RI PT
Hardness (N), Gel strength (mJ)
ACCEPTED MANUSCRIPT
M AN U
SC
Total sterol content (% w/w)
Figure 3. Mechanical properties, hardness (N) and gel strength (mJ), of sunflower organogels with different total sterol contents (10% and 20% w/w). A) Effect of oryzanol-phytosterol weight ratio, 30:70 and 60:40, after 24 h storage at 25 °C.
°C.
TE D
B) Effect of storage time, 2 and 10 days at 60:40 oryzanol:phytosterol weight ratio at 25
C) Effect of temperature after 48h storage at 4 οC and 25 οC for the 30:70
EP
oryzanol:phytosterol weight ratio. Texture measurements were conducted at 25 °C. Means with different superscript letters are different (p < 0.05). The superscript letters for
AC C
Hardness are in capital (upper case) while in gel strength is in small (lower case)
b
c
d
200 μm
M AN U
SC
a
RI PT
ACCEPTED MANUSCRIPT
200 μm
Figure 4. Polarized micrographs of emulsions, after storage at 4 οC for 24 h. The emulsions contain 50% w/w aqueous phase and 50% w/w organogel; (a) 10% w/w sterol content 30:70 weight ratio, (b) 20% w/w - 30:70, (c) 10% w/w - 60:40 and (d) 20% w/w -
AC C
EP
TE D
60:40.
ACCEPTED MANUSCRIPT
b
SC
RI PT
a
Figure 5. Polarized micrographs of 30:70 organogel-based emulsions, after storage at 4 ο
C for 24 h. The emulsions contain 50% w/w aqueous phase and 50% w/w organogel: (a)
AC C
EP
TE D
M AN U
10% w/w sterol content and 1% w/w lecithin, (b) 20% w/w and 2% w/w lecithin.
ACCEPTED MANUSCRIPT
A
100
RI PT
10%-30:70 10%-60:40 20%-30:70 20%-60:40
SC
10
1 0.001
0.01
M AN U
Storage Modulus G' (Pa)
1000
0.1
1
10
100
Shear stress (Pa)
B
1.5 1.0
c
b
EP
2.0
a
AC C
Yield Stress τy (Pa)
2.5
TE D
3.0
0.5
a
0.0
10% 30:70
10% 60:40
20% 30:70
20% 60:40
Figure 6. Α) Strain sweep tests of organogel-based emulsions, after storage at 4 οC for 24 h. The emulsions contain 50% w/w aqueous phase and 50% w/w organogel
ACCEPTED MANUSCRIPT
Β) Yield stress τy (Pa) of organogel-based emulsions after storage at 4 οC for 24 h.
EP
TE D
M AN U
SC
RI PT
Means with different superscript letters are statistically different (p < 0.05)
AC C
ab
ACCEPTED MANUSCRIPT
B
10 1
0.1 0.1
1
Frequency (Hz)
1
tan δ
100 10
G' G'' tan δ
1
10
0.1
Frequency (Hz)
1.0
G' G'' tan δ
100
10
1
0.1
0.1
1
Frequency (Hz)
1000
100
M AN U
tan δ
G', G'' (Pa)
1000
10
10
SC
D
G', G'' (Pa)
C
0.1
1
10
1.0
tan δ
100
1000
G', G'' (Pa)
1
G' G'' tan δ
tan δ
G', G'' (Pa)
1000
RI PT
A
G' G'' tan δ
1
0.1
0.1 1
Frequency (Hz)
10
AC C
EP
TE D
Figure 7. Variation of G', G'' and tan δ as a function of frequency of organogel-in-water emulsions after storage at 4 οC for 24 h: (A) 10% w/w, 30:70 sterol ratio; (B) 20% w/w, 30:70 sterol ratio; (C) 10% w/w, 60:40 sterol ratio; (D) 20% w/w, 60:40 sterol ratio
ACCEPTED MANUSCRIPT
0,7
d
103 G' (1Hz) tanδ (1Hz)
c
0,5
a
b
10
a
a
a
0,4
0,3
10% 30:70
10% 60:40
20% 30:70
20% 60:40
M AN U
100
a
SC
1
tanδ
G' (Pa)
102
RI PT
0,6
Figure 8. Variation of G' and tanδ at 1 Hz among different organogel composition (30:70 and 60:40 γ-oryzanol:phytosterol weight ratio, 10% and 20% w/w total sterol content) of emulsion gels, after storage at 4 οC for 24 h.
EP
TE D
Means with different superscript letters are different (p < 0.05)
AC C
abc
ACCEPTED MANUSCRIPT 1 10000
10% 30:70 10% 60:40 20% 30:70 20% 60:40
100
10
1
0.1 0.001
0.01
0.1
Shear rate
2
1
10
(s-1)
SC
3
100
RI PT
Viscosity η (Pa·s)
1000
Figure 9. Shear rate (s-1) dependence of the viscosity η (Pa·s) of organogel-based emulsions
5
(30:70 and 60:40 sterol weight ratio, 10% and 20% w/w total sterol content), after storage at
6
4 οC for 24 h.
M AN U
4
7
AC C
EP
TE D
8
1