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Characterization of β-carotene loaded emulsion gels containing denatured and native whey protein
Journal Pre-proof Characterization of β-carotene loaded emulsion gels containing denatured and native why protein Yao Lu, Like Mao, Hongxia Zheng, Hongqiang Chen, Yanxiang Gao PII:
S0268-005X(19)32160-5
DOI:
https://doi.org/10.1016/j.foodhyd.2019.105600
Reference:
FOOHYD 105600
To appear in:
Food Hydrocolloids
Received Date: 18 September 2019 Revised Date:
22 November 2019
Accepted Date: 16 December 2019
Please cite this article as: Lu, Y., Mao, L., Zheng, H., Chen, H., Gao, Y., Characterization of β-carotene loaded emulsion gels containing denatured and native why protein, Food Hydrocolloids (2020), doi: https://doi.org/10.1016/j.foodhyd.2019.105600. This is a PDF file of an article that has undergone enhancements after acceptance, such as the addition of a cover page and metadata, and formatting for readability, but it is not yet the definitive version of record. This version will undergo additional copyediting, typesetting and review before it is published in its final form, but we are providing this version to give early visibility of the article. Please note that, during the production process, errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain. © 2019 Published by Elsevier Ltd.
Graphical abstract
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Characterization of β-carotene loaded emulsion gels containing
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denatured and native why protein
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Yao Lu, Like Mao*, Hongxia Zheng, Hongqiang Chen, Yanxiang Gao
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Beijing Advanced Innovation Center for Food Nutrition and Human Health, Beijing
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Laboratory for Food Quality and Safety, College of Food Science & Nutritional
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Engineering, China Agricultural University, Beijing, China
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Corresponding author:
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Tel: +86-10-62737034
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Fax: +86-10-62737986
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E-mail: [email protected] (L. Mao)
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Abstract:
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The current study developed whey protein emulsion gels containing β-carotene, and the
25
effects of the content of denatured protein and native protein were investigated. Two
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sets of emulsion gels were obtained by fixing the total protein content or the denature
27
protein content (Cprotein-D). Emulsion properties were mostly affected by the content of
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native protein (Cprotein-N), and higher Cprotein-N resulted in emulsions with smaller
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particle size, higher surface charge and better creaming stability. Emulsions were then
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gelled with the addition of Glucono-δ-lactone. At fixed total protein content, higher
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Cprotein-D contributed to gels with higher mechanical properties, e.g., fracture stress,
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Young’s modulus and storage modulus (G′). At fixed Cprotein-D, the increase in Cprotein-N
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also resulted in stronger gels but at much lower magnitude. The dynamic gelation
34
analysis revealed that the increase in Cprotein-N or Cprotein-D resulted in shorter gelling
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time. All the gels had rather high water holding capacity, and the gels with greater
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mechanical strength had lower swelling ratios. When emulsion gels were applied as
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carriers for β-carotene, both Cprotein-D and Cprotein-N had significant effects on the light
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stability and heat stability of β-carotene.
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Keywords: emulsion gel; denatured protein; native protein; gel structure; β-carotene
40 41 42 43 44 45 46 47
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1. Introduction
49
Emulsion gels are structured emulsion systems, which have dispersed phases entrapped
50
within three-dimensional (3D) network (Farjami & Madadlou, 2019). Yoghurt, cheese,
51
and some processed meat are common food with emulsion gel structures. Emulsion
52
gels are generally prepared through two-stage processes, i.e., emulsification and
53
gelation. The gelation can be originated from proteins, polysaccharides or their
54
mixtures, via heat-induced, salt-induced, acid-induced, or enzyme-induced approaches
55
(Lu, Mao, Hou, Miao, & Gao, 2019). When the gelling agents have surface activity
56
(e.g., whey protein, soy protein, gum Arabic), they may also behave as emulsifiers to
57
stabilize the emulsions. In other cases, emulsifiers and gelling agents can be different
58
ingredients. Emulsion gels are usually applied to structure food systems, offering
59
desirable rheological and textural properties, and they are also widely used in
60
fat-reduced food (Dickinson, 2012). Many recent studies have revealed that emulsion
61
gels are suitable carriers for lipid-soluble food bioactives, as the strong gel network can
62
provide effective protection, and the modulation of gel structures allows controlled
63
release and digestion of the incorporated ingredients (McClements, 2010; Torres,
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Murray, & Sarkar, 2016; Lu, et al., 2019).
65
In emulsion gels, compositions and structures of the interface and continuous phase
66
have great influence on the their functionality. According to the different interactions
67
between the interfacial membrane and the continuous gel, the dispersed oil droplets can
68
behave as active or inactive fillers (Dickinson, 2012; Lu, et al., 2019). With active
69
fillers, the dispersed phase also participates the assembly of the gel network, and it is
70
able to reinforce gel structure. Generally, emulsion gels using proteins to stabilize the
71
interface and gel the continuous phase have active fillers. In these systems, the
72
reduction in oil droplet size contributed to larger interfacial area, and thus led to gels
3
73
with higher strength (Sala, van Vliet, Cohen Stuart, van de Velde, & van Aken, 2009).
74
Literature studies also indicated that droplet coalescence or oil solidification could
75
assist the formation of stronger gels (Oliver, Wieck,
76
Scholten, & van Aken, 2015). Furthermore, the interface can largely influence droplet
77
distribution and emulsion stability, which may also affect the structures of the gels
78
(Guido, van Aken, Cohen Stuart, & van de Velde, 2010). Although different proteins
79
(e.g., whey protein, soy protein, sodium caseinate) have been tested for their roles in the
80
properties of emulsions gels, no detailed information regarding the effects of the
81
content and structures of proteins at the interface were available (Lu, et al., 2019). With
82
inactive fillers, the oil-water interface has minor or no interactions with the continuous
83
gel body, and the oil phase is likely to weaken the gel structure. Generally, the gel
84
systems containing low molecular weight surfactants have inactive fillers (Dickinson,
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2012).
86
The biopolymers (i.e., proteins, polysaccharides) in the continuous phase constitute the
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main structures of the gel network, and their structures and content play essential roles.
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In a typical cold-gelation process, proteins are preheated to unfold their ternary
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structures and expose hydrophobic residues. The denatured protein molecules then
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aggregate to form 3D network with the aid of gelation triggers, e.g., acid, salt or
91
enzymes (Mao, Lu, Cui, Miao, & Gao, 2019). Generally, emulsion systems with higher
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protein content are more favorable for the formation of compact gel network because of
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the presence of larger number of crosslinking sites. Second, with large number of oil
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droplets dispersed in protein dispersion, the protein concentration threshold for gelation
95
can be well reduced, compared to pure gel systems. Mao et al. (2014) reported that a
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system with a protein content of 4% was able to form emulsion gels with
97
self-supporting behaviors. Third, at a fixed protein concentration, protein preheating of
4
& Scholten, 2016; Oliver,
98
higher intensity (e.g., longer heating time, higher heating temperature) could facilitate
99
the formation of denser gel network (Mao, Miao, Yuan, & Gao, 2018). In some
100
emulsion gels, there could be two or more proteins and/or polysaccharides
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(Balakrishnan, Nguyen, Schmitt, Nicolai, & Chassenieux, 2017; Feng, Jia, Zhu, Liu, &
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Yin, 2019). In these systems, the interactions between biopolymers had critical impact
103
on the development and structures of the gels. Depending on the charging properties,
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proteins and/or polysaccharides could form gel systems with single continuous phase,
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double continuous phase, uniform continuous phase, or non-homogeneous chained gel
106
systems (van de Velde, de Hoog, Oosterveld, & Tromp, 2015). Furthermore,
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biopolymer-biopolymer interactions were likely to change during the gelation as
108
affected by pH, ionic strength, etc., which then affected gel structures (Williams,
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Phillips, Matiamerino, & Dickinso, 2004). However, less attention was paid to the gel
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systems containing non-gelling biopolymers.
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In the current study, native whey protein was used mainly as an emulsifier, and
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heat-denatured whey protein was used as a gelling agent. β-Carotene loaded emulsion
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gels were prepared by varying the content of denatured protein and native protein, and
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both emulsion properties and gel properties were characterized, aiming to better
115
understand the roles of oil-water interface and continuous phase in the structure and
116
functionality of the gel systems. To the authors’ knowledge, it is the first time to study
117
emulsion gel systems with one type of protein at both native and denatured states,
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which is meaningful for the innovation of healthy food.
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2. Materials and methods
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2.1. Materials
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Corn oil was the product of Changshouhua Food Company Limited (Shandong, China),
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and used withoug additional purification. Bipro-type whey protein isolate(WPI) was 5
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purchased from Davisco Foods (Le Sueur, MN, USA). Crystalline β-carotene with a
124
purity >99% was a favor of NHU Holding Group Co., Ltd. (Zhejiang, China). Sodium
125
azide, glucono-δ-lactone (GDL), n-hexane were products of Sigma-Aldrich (St. Louis,
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MO, USA).
127
2.2. Preparation of denatured protein powder
128
To induce protein denaturation, WPI dispersion (5 wt%) was incubated in a water bath
129
at 85 °C for 30min, and then cooled rapidly to about 25 °C using ice. The samples were
130
lyophilized using a vacuum freeze dryer (Marin Christ, Germany), and the obtained
131
protein powder was stored in a desiccator for further use.
132
2.3. Determination of interfacial tension
133
Protein powder was hydrated in deionized water and kept overnight. Then interfacial
134
tension between protein solution (1 wt%) and corn oil was measured using a
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Tensiometer K100 (Krüss, Hamburg, Germany) following a classical Wilhelmy plate
136
method. During the measurement (20 °C), a platinum Wilhelmy plate (19.9×10×0.2
137
mm) was immersed in the protein solution (20 mL) to a depth of 3 mm at a surface
138
detection speed of 15 mm/min. The vessel drive speed applied for the tracking of the
139
liquid surface was regarded as the surface detection speed. When the surface was
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determined by the microbalance in the machine, the vessel moved at the selected
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surface detection speed to the position specified by the immersion depth (3 mm).
142
Afterwards, an interface between the protein solution and corn oil was created by
143
carefully inject the corn oil over the protein solution (O'Sullivan, Rellano, Pichot, &
144
Norton, 2014). Evolution of interfacial tension during the measurement of monitored,
145
and the values at equilibrium were reported.
146
2.4. Emulsion preparation
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The method for the preparation of emulsions was previously reported by Mao, Roos &
148
Miao (2014). WPI (native) dispersions of different protein content were mixed with
149
corn oil (20 wt%) using a high speed blender (Ultra-Turrax, IKA, Germany) to form
150
coarse emulsions, which were then homogenized at 500 bar for three passes using a
151
high pressure homogenizer (Niro-Soavi, Parma, Italy). The emulsions were rapidly
152
cooled to about 25 °C using ice. The lyophilized denatured protein powder was added
153
to the emulsions, and mixed well for complete hydration of the powder.
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For the preparation of β-carotene emulsions, β-carotene crystals (6 wt%) were first
155
dissolved in the oil phase at 140 °C before mixing with the water phase. Samples
156
containing different content of native protein (Cprotein-N) and denatured protein (Cprotein-D)
157
were listed in Table 1.
158
2.5. Characterization of WPI stabilized emulsions
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Droplet size and surface charge of the emulsions were determined by utilizing a
160
Malvern Zetasizer (Nano-ZS90, Malvern Instrument, UK). RI (refractive index) of
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aqueous and oil phases were set to 1.33 and 1.45, respectively. In order to reduce
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multiple scattering effect, each sample was diluted with deionized water prior to the
163
measurement. Droplet size was described as hydrodynamic diameter (nm) and
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polydispersity index (PDI), and surface charge was described as ζ-potential (mV).
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Viscosity of the emulsions was evaluated via a DHR-2 rheometer (TA Instruments,
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UK) , and the geometry with parallel plates (40 mm diameter and 1 mm gap) was
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selected. The determination was carried out at the shear rate range of 10–400 s−1 at
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25 °C.
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Emulsion stability was determined using a LUMiSizer (L.U.M.GmbH, Berlin,
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Germany), which applied centrifugation force to accelerate the test. The machine used
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near-infrared light (880 nm) to scan the whole samples, and intensity of the transmitted 7
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light was recorded. The measurement (25 °C) was set at a centrifugation speed of 4000
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rpm and the samples were scanned 800 times at an interval of 10 s. The curves of
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integrated intensity of the light transmitted as a function of time were plotted, and
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slopes of the curves were regarded as instability index (Mao, Roos, & Miao, 2015).
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2.6. Preparation of emulsion gels
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Emulsion gels were prepared following the method reported previously (Mao, et al.,
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2014). Briefly, GDL (0.5 wt%) was introduced into emulsions and mixed well with
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stirring bars, and the mixtures were incubated quiescently at 25 °C for 12 h to form the
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gels.
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2.7. Characterization of emulsion gels
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2.6.1. Viscoelastic behaviors
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The same rheometer for viscosity analysis was also applied to the evaluation of
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viscoelastic characteristics of the gels. Emulsion drops were placed onto the plate right
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after the addition of GDL, and the dynamic gelation process was evaluated at a strain of
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0.5% and a frequency of 1 Hz under the oscillation mode (25 °C). The linear
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viscoelastic range of the samples was pre-determined through a strain sweep. The
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evolution of storage modulus (G′) and loss modulus (G′′) in the gelation process were
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recorded (Mao et al., 2018).
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2.6.2. Textural properties
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Textural analysis was performed for all the emulsion gels using a FTC texture analyzer
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(Rockville, Maryland, USA). Samples for the test were specifically formed in plastic
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containers (34 mm id., 50 mm height) following the approach reported earlier. The gels
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received uniaxial compression by a 12 mm cylindrical plunger at a strain of 50%.
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Fracture stress, fracture strain and Young’s modulus of the samples were then
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calculated. All the reported values were means of eight replicates.
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2.6.3. Swelling ratio
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Swelling ratios of the gels were measured according to a study by Carvajal-Millan et al.
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(2015). The gels were cut into cylindrical shape and weighed, and the initial mass was
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recorded as M0. All the samples were immersed in deionized water for 24 h, and then
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the swollen gels were moved out for mass determination (M). The swelling ratio (t) was
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calculated using the following equation: t = (M-M0)/M0 * 100
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2.6.4. Water holding capacity (WHC)
205
WHC of the gels was measured following the method reported by Wang and
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co-workers (2018) with slight adjustments. The emulsions were gelled in 10 mL
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centrifuge tube and weighed (W0). Afterwards, samples were centrifuged at 14,000 rpm
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and 25 °C for 20 min. The water released was removed, and the mass of the remaining
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gels (with centrifuge tube) was weighed and recorded as W. WHC (%) of the emulsion
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gels was calculated using the equation below: WHC=(W0-W)/W0 *100
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2.6.5. Scanning electron microscopy (SEM) observation.
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Microstructural observation of the samples was carried out using a SU-8100 SEM
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(Hitachi, Japan). The gel structures were fixed in a glutaraldehyde-cacodylate buffer,
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followed by ethanol dehydration and critical point drying. The dried samples were then
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placed on a copper stud and sputtered with gold for the observation.
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2.8. Stability of β-carotene
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2.8.1. UV-light stability
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Light stability test was performed in a Q-SUN xenon test chamber (Q-Panel Lab
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Products, USA) at an irradiance of 0.68 W/m2. Fresh emulsion gels were first moved
221
into transparent glass bottles (flushed with nitrogen), and then incubated in the test
222
chamber for 8h at 25 °C (Liu, Wang, Xu, Sun, & Gao, 2016). Sampling was done each
223
2h to determine the remained content of β-carotene.
224
2.8.2. Thermal stability
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Glass bottles (flushed with nitrogen) containing fresh emulsion gels were incubated at
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25 and 55 °C for 15 d at dark. Sampling was done every 3d to determine the remained
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content of β-carotene.
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2.8.3. Determination of the content of β-carotene
229
Emulsion gels from stability test were mashed to destroy the gel structures for the ease
230
of the extraction of β-carotene with n-hexane. β-Carotene content was then determined
231
using a UV 1800 spectrophotometer (Shimadzu, Japan) by recording the absorbance at
232
450 nm, in assistance with a standard curve (Yuan, Gao, Zhao, & Mao, 2008).
233
Retention ratio C/C0 (C: content of β-carotene after storage; C0: initial content of
234
β-carotene before storage) of β-carotene in the gels after the test was applied to describe
235
the stability of β-carotene.
236
By fitting a first-order kinetic model, the degradation kinetics of β-carotene was also
237
evaluated. Reaction rate constant (k) and half-life (t1/2) of β-carotene was calculated
238
following the equations below (Sharma, Kaur, Oberoi, & Sogi, 2008): C / C 0 = exp(−k • t )
239 240
ln C = ln C 0 − kt
241
t1 / 2 = ln 2 / k 242
2.9. Statistical analysis
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Mean values ± standard deviations (SD) were reported for all data points based on three
244
replicates. An analysis of variance (ANOVA) of the data was performed using Origin
245
Pro 8 at a level of significance of 5%.
246
3. Results and discussion
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3.1. Characterization of the emulsions
248
It is known that proteins in the continuous phase or at the interface can largely affect
249
emulsion properties (McClements, 2004). However, there is little information available
250
when a mixture of denatured protein and native protein is used. Table 2 summarizes the
251
droplet characteristics of the emulsions, i.e., droplet size, PDI and surface charge, as
252
affected by the content of proteins at the interface and continuous phase. At fixed total
253
protein content (group A), the increase in Cprotein-N led to smaller particle size and lower
254
PDI of the emulsions, as higher interfacial coverage prevented droplet association via
255
steric hindrance and electrostatic repulsion (McClements, 2015). In fact, the magnitude
256
of zeta-potential was also higher in the emulsions with higher Cprotein-N. At fixed
257
Cprotein-D (group B), similar trends were also observed, and the increase in Cprotein-N
258
contributed to emulsions with smaller particle size. At fixed Cprotein-N, the change in
259
Cprotein-D did not affect particle size significantly (A1 and B1, A3 and B3). Therefore,
260
the content of native protein played a more significant role in emulsion properties. The
261
interfacial tension between protein solution and corn oil was also determined, and the
262
result indicated that the native protein (13.748±0.029 mN/m) was capable to reduce the
263
interfacial tension a lower level than the denatured protein (14.935±0.006 mN/m) at
264
equilibrated state, which was in agreement with literature study (Euston, Finnigan, &
265
Hirst, 2000). Besides, native protein was firstly added to form the emulsions, followed
266
by the addition of denatured protein. Therefore, the native protein was more likely to
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dominate the interface. However, the emulsions with lower Cprotein-D had significantly
268
higher magnitude of surface charge (B1>A1, A3>B3). There could be some
269
interactions between denatured protein and native proteins (Vardhanabhuti, Foegeding,
270
McGuffey, Daubert, & Swaisgood, 2001), and the resultant complex might have
271
decreased amount of charged moieties. For example, the exposed thiol groups in
272
denatured protein can interact with the surface active groups of native protein (Torres,
273
Janhøj, Mikkelsen, & Ipsen, 2010). However, the underlying mechanisms required
274
further investigation.
275
Fig. 1 shows the difference in viscosity between the two groups of emulsions. The
276
results indicated that all the emulsions were shear-thinning fluids, and viscosity of the
277
emulsions decreased gradually with the increase in shear rates (Dybowska, 2004).
278
Shear thinning behavior was a sign of droplet flocculation in emulsions, which
279
presented resistance against shearing at lower force and broke up at high shear rates
280
(Floury, Desrumaux, & Lardières, 2000). Dickinson et al. (1997) believed that
281
reversible depletion flocculation caused by unabsorbed protein present in the
282
continuous phase can cause pseudoplasticity of the emulsion. In the current systems,
283
there was also a high content of denatured protein at the continuous phase, which was
284
possible to induce droplet flocculation (Euston et al., 2000). Second, as protein
285
denaturation had thickening effect, the increase in Cprotein-D contributed to the systems
286
with higher viscosity (Fig. 1A) (Britten, Giroux, Jean, Rodrigue, 1994). At fixed
287
Cprotein-D, the change in Cprotein-N did not affect emulsion viscosity significantly (Fig. 1B).
288
It is known that emulsions with smaller particles generally have higher viscosity
289
(McClements, 2010), which was not observed for the present samples, probably due to
290
the bigger roles of Cprotein-D.
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291
All the emulsions had good creaming stability before gelation, probably due to the high
292
content of protein, and the higher interfacial charge. We performed acceleration tests to
293
observe the differences in emulsion stability by applying a multisample centrifugation
294
technique. Fig. 2 reveals that emulsions with higher Cprotein-N generally had lower
295
instability index, both at fixed total protein content and Cprotein-D.
296
3.2. Characterization of the emulsion gels
297
3.2.1. Viscoelastic properties of the emulsion gels
298
The gelation process was simulated in a rheometer, and the evolution of the rheological
299
properties of the systems was evaluated (Fig.3). In the current study, all the systems
300
followed similar gelation dynamics, which could be divided into three stages. At the 1st
301
stage, both G' and G'' of the systems were low and increased slowly. In this stage, the
302
hydrolysis of GDL was just initiated, and pH of the systems was still high, and there
303
was little interaction between protein aggregates; At the 2nd stage, both G' and G'' got
304
sharp increase, and G' was increased even faster. In this stage, pH of the systems was
305
lowered to the isoelectric point (pI) of the protein, and the protein molecules tended to
306
form 3D network as a result of hydrophobic attraction, van der Waals forces and
307
hydrogen bonding (Ye & Talor, 2009; Mellema, van Opheusden, & van Vliet, 2002). In
308
some studies, the time point at which the sharp increase started was refered to as gelling
309
time (Ersch et al., 2015); At the 3rd stage, the increase of G' and G'' was well slowed
310
down until levelled off. In this stage, pH of the systems was kept at low level (Mao et al.,
311
2014), and the development of the gel network gradually reached a steady state. At
312
fixed total protein content, the system with the highest Cprotein-D (A1) started all the three
313
stages much earlier than the other two systems, because of the earlier onset of gelation.
314
Furthermore, G' at the steady state was higher in the systems with higher Cprotein-D
315
(A1>A2>A3) (Fig. 3A). These results indicated the big role of denatured protein in the 13
316
development of the gel network. With higher Cprotein-D, there were more binding sites
317
for aggregate association, leading to faster gelation and higher gel strength. At fixed
318
Cprotein-D, the increase in Cprotein-N (with higher total protein content) resulted in faster
319
gelation and bigger G' at the steady state (Fig. 3B). The findings indicated that the
320
native protein took part in the development of the gel network, and higher total protein
321
content promoted gelation. It has been well documented that denatured protein at the
322
interface participate the gelation process with the denatured protein at the continuous
323
phase (Ye & Talor, 2009; Mao et al., 2018). However, there was little information on
324
the roles of native protein in the gelation of denatured protein. In fact, the current
325
systems could be regarded as mixed emulsion gels with two proteins. The native
326
protein in the current systems was not possible to gel individually, because of its folded
327
structures and low concentration. On the other hand, no phase separation was observed
328
when the two proteins coexisted in the dispersions, indicting the two proteins were
329
thermodynamically compatible. Therefore, there were other mechanisms responsible
330
for the participation of the native protein in the gel network: 1) Native protein (either in
331
the continuous phase or at the interface) formed complexes with denatured protein
332
(through electrostatic or hydrogen bonding) (Britten, Giroux, Jean, & Rodrigue, 1994;
333
Zhai, Day, Aguilar, & Wooster, 2015); 2) Native protein behaved as fillers to support
334
the gel network. With higher density of protein deposited at the interface, the oil
335
droplets could have higher density and strengthen the gel structures (Lu, et al., 2019);
336
the native protein could compete for water binding and concentrated the denatured
337
protein (Ersch, ter Laak, van der Linden, Venema, & Martin, 2015). Wu et al. (2018)
338
concluded that non-networking proteins (mainly soy protein peptides) did not affect the
339
G′ of the emulsion gels (heat-induced), because the non-networking proteins were
340
dissolved and located at the pores of gel network. However, in the current study, native
14
341
protein was believed to be mostly distributed at the interface. Second, different gelation
342
methods and protein structures in the two studies could also be responsible for the
343
contradicting results. It was deducted that the oil droplets worked as active fillers in
344
these systems (Dickinson, 2012). However, systems with smaller oil droplets (e.g., A3)
345
did not always had higher G', probably because the size effect was blocked by the big
346
role of protein content.
347
3.2.2. Textural properties
348
Gel food received compression and stretching during oral processing, and the forces
349
received by the brain were largely perceived as texture (Stokes, Boehm, & Baier, 2013).
350
Table 3 represents the textural characteristics of the emulsion gels. It was observed that
351
the content of denatured protein and native protein greatly affected the texture of the
352
gels. At fixed total protein content, the increase in Cprotein-D was accompanied by the rise
353
in fracture stress and Young’s modulus (A1>A2>A3), indicating the big role of the
354
denatured protein in the formation of gel structures of high strength. Similar results
355
were also obtained by Vardhanabhuti and coworkers (2001), who found that the
356
replacement of native whey protein by denatured protein resulted in gels with higher
357
fracture stress and modulus. It was reported that Young’s modulus could reflect
358
molecular rigidity, which for biopolymers, could be a sign of the number of cross-links.
359
With higher Cprotein-D, there were more cross-linking sites in the systems, leading to
360
higher rigidity of the gels (Saavedra Isusi, Karbstein, & van der Schaaf, 2019). At fixed
361
Cprotein-D, only slight increase in Young’s modulus and fracture stress (B3>B2>B1) with
362
the increase in Cprotein-N was observed. In the current study, gelation was originated
363
from the aggregation of protein molecules, which was favorable when the molecules
364
were unfolded (at denatured state). For example, by changing the Cprotein-D from 4% (B1)
365
to 4.5% (A1), the fracture modulus was increased by 18.06% (from 2.99 to 3.53 MPa);
15
366
by changing the Cprotein-N from 1% (B2) to 1.5% (B3), the fracture stress was only
367
increased by 1.31% (from 3.06 to 3.10 MPa). These results also indicated that the
368
current systems were homogeneous, as inhomogeneity usually resulted in a decrease in
369
fracture stress, as result of stress concentration (van Vliet & Walstra, 1995).
370
Interestingly, fracture strain of the gels was independent on Cprotein-D and Cprotein-N,
371
probably because of the soft nature of the gels at the current protein range.
372
3.2.3. Microstructures
373
Figure 4 illustrates the morphology of the emulsion gels through SEM observation,
374
which clearly showed the differences in the microstructures of the samples. At fixed
375
total protein content (group A), the gels with higher Cprotein-D had more compact
376
structures with smaller pores. In sample A1, the gel network was formed by protein
377
aggregates of smaller size and similar shape. In sample A3, the aggregates were rather
378
big with different shapes. The results reconfirmed the bigger roles of denatured protein
379
for the development of compact gel network. At fixed Cprotein-D, the changes in Cprotein-N
380
only resulted in slight changes in the microstructures of the gels. Comparatively, the
381
gels with the highest Cprotein-N had the densest structure and lowest number of pores.
382
Whey protein could develop particulate gels or filamentous gels, which was mainly
383
dependent on the force balance between attraction and repulsion among protein
384
molecules (Lefevr & Subirade, 2000; Ikeda & Li-Chan, 2004). In the current study,
385
lower repulsion force was present as the pH of the gels was lowered to the pI of the
386
protein, and the development of particulate gels was favored. Oil droplets could not be
387
clearly observed in these SEM images, because they were completely surrounded by
388
the particulate protein network. In fact, there were a lot of small-sized protrusion at the
389
surface of the gel network, which could be the oil droplets (Lu et al., 2019).
390
3.2.4. Swelling ratio & WHC
16
391
The three-dimensional network in emulsion gels entrap a certain amount of water, and
392
they are also able to adsorb addition water (Begam, Nagpal, & Singhal, 2003), which
393
are important for the mouth feel of gel food and the release of functional ingredients
394
incorporated (Lu et al., 2019). Swelling properties of gels were highly dependent on the
395
pore size and water-adsorbing capacity of the gelling biopolymers (Feng et al., 2019).
396
Fig. 5A reveals that the gels with higher Cprotein-D (fixed total protein content) had lower
397
swelling ratios. For example, the swelling ratio of A1 was 1.64%, and that of A3 was
398
4.46%. As discussed earlier, higher Cprotein-D contributed to more compact gel network,
399
and there could be only small pores to accommodate additional water. Second,
400
denatured protein had decreased capability to adsorb water (Saffon, Britten, & Pouliot,
401
2011). Third , the gels already had high amount of water adsorbed during the
402
development of gel network. In fact, all the three gels maintained their self-supporting
403
structures after the swelling test. Fig. 5B indicates that gels with lower Cprotein-N (fixed
404
Cprotein-D) had higher swelling ratios. The greater adsorption of water might be resulted
405
from the bigger size of the oil droplets (Feng et al., 2019). Morphological observation
406
showed that the gels with higher swelling ratio became softer and were not able to
407
maintain their intact structures. During food digesting, swelling of gels can facilitate
408
bioactive release (Mao et al., 2019).
409
Water holding capacity (WHC) refers to the ability of the tested samples to immobilize
410
moisture through capillary forces, which is largely dependent on pore size (Wu et al.,
411
2009). Fig. 6 indicates all the samples had quite big WHC (>85%), and there was small
412
difference among samples. At fixed total protein content, the highest WHC (87.29%)
413
was observed in the sample with the highest Cprotein-D. At fixed Cprotein-D, the highest
414
WHC (88.78%) was found in the sample with the highest Cprotein-N. Some studies
415
concluded that WHC and storage modulus of emulsion gels had positive association
17
416
(Sok Line, Remondetto, & Subirade, 2005; Yang, Liu, & Tang, 2013), which was also
417
found in the current study. Emulsion gels with higher storage modulus generally had
418
denser and more uniform microstructures, which allowed the gels to hold water
419
molecules strongly against centrifugation (Hu et al., 2013). In the current systems,
420
water was mostly bound to proteins, and only small amount of water could be present in
421
the pores of the gel network. Vardhanabhuti et al. (2001) suggested there could be a
422
transition in network structures from particulate to a more filamentous structures in gels
423
with more denatured protein, and the latter type of gels had higher ability to hold water.
424
3.3. Emulsion gels as carriers for β-carotene
425
β-carotene has strong antioxidant activity, and it is able to enhance the specific and
426
non-specific immune function. However, β-carotene is extremely sensitive to light,
427
heat and oxygen, and is prone to degradation, which can result in the loss of its
428
bioactivity (Rodriguez-Amaya, 2015). It has been proved that delivery systems,
429
including emulsions, gels, nanoparticles are able to protect β-carotene from
430
degradation (Mao, Wang, Liu, & Gao, 2018).
431
Fig. 7 shows the changes in the retention ratios of β-carotene within emulsion gels of
432
different protein content during the light stability test. At fixed total protein content
433
(Fig. 7A), the emulsion gels with higher Cprotein-D can retain more β-carotene
434
(A1>A2>A3). For example, in the gel with a Cprotein-D of 4.5%, about 56.53±0.03% of
435
the original content of β-carotene was retained after the test. However, only 45.06 ±
436
0.02% β-carotene was retained in the sample with a Cprotein-D of 3.5%. As discussed
437
earlier, gels with higher Cprotein-D had denser structures, which could effectively prevent
438
the contact of the embedded functional ingredients with external environmental stresses.
439
Second, carotenoids can form complexes with protein through hydrophobic
440
interactions (Dufour, &Haertlé, 1991;Wackerbarth, Stoll, Gebken, Pelters, Bindrich, 18
441
2009), and the complexes could be more resistant to oxidation. At fixed Cprotein-D, the
442
stability of β-carotene was improved with the increase in Cprotein-N (B3>B2>B1). This
443
may be due to the fact that β-carotene degradation was initially started at the emulsion
444
interface (Liu et al., 2016). The increase in Cprotein-N can enhance the thickness of the
445
interfacial film and effectively inhibit the initiation and propagation of the oxidation
446
process (Waraho, McClements, & Decker, 2011). Second, there were some
447
antioxidative moieties in protein molecules, e.g., cysteyl residues, disulphide bonds and
448
thiol groups, which also worked to inhibit β-carotene oxidation (Mao et al., 2018).
449
When the emulsion gels were stored at different temperatures (25 °C and 55 °C), the
450
changes in the retention ratios of β-carotene followed similar trends as those observed
451
in the light stability test (Fig. 8). For example, after a 12-day storage test, the retention
452
rate of β-carotene in A1 was 57.61±0.01% (25 °C) and 45.61±5.55% (55 °C), and that
453
of A3 was 52.81±0.02% (25 °C) and 37.81. ±1.92% (55 °C). In general, gels with
454
higher gel strength and denser structures could provide stronger protection for
455
β-carotene against adverse stresses. Similar results were also observed in other studies
456
on different lipophilic bioactives (Lu et al., 2019). Although the increase in the content
457
of native protein and denatured protein were both helpful in retaining higher content of
458
the bioactive, higher Cprotein-D was more effective.
459
In order to get a systematic understanding of β-carotene degradation in these gel
460
systems, degradation kinetics was calculated (Table 4). It was found that β-carotene in
461
the gels containing higher Cprotein-D had smaller k and bigger t1/2 values during light
462
stability and thermal stability test. For example, when the emulsion gel had a Cprotein-D
463
of 4.5% and a Cprotein-N of 0.5% (A1), β-carotene had a k value of 77.4×10-4 h-1, and a t1/2
464
value of 8.95 h during the light stability test; the k value was 2.56×10-4h-1, and the t1/2
465
value was 270.70 h when the gels was stored at 55 °C. The emulsion gels with higher
19
466
Cprotein-D had better protection effect on the embedded ingredient, and the degradation
467
rates were slower. It was also found that the increase in Cprotein-N could reduce the k
468
value of β-carotene in the emulsion gels and enhance its protective effect. The
469
calculation clearly indicated that the increase in Cprotein-D was more effective in slowing
470
the degradation of β-carotene than the increase in Cprotein-N, suggesting that the gel
471
structures provided more protection for β-carotene than the interface.
472
4. Conclusion
473
The present work studied the influence of the content of native protein and denatured
474
protein in the structure and functionality of emulsion gels. With strong self-assembling
475
properties of the denatured protein molecules at pH close to its isoelectric point, the
476
changes in Cprotein-D greatly affected mechanical, water adsorption and holding
477
capacities. Consequently, the gels with higher Cprotein-D retained more β-carotene during
478
stability tests. The native protein also took part in the development of the gel network
479
and the protection for β-carotene, though it played relatively weaker roles. The study
480
revealed the strong influences of the gel structures on the functionality of the emulsion
481
gels, and appropriate structural designs in the gel matrix and at the interface could bring
482
in flexible delivery of bioactives incorporated in the systems. The knowledge obtained
483
in this study would provide novel information for the development of delivery systems
484
for functional food.
485
486
Acknowledgments
487
This research was funded by National Natural Science Foundation of China (No.
488
31701648).
489
20
490
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24
Table 1. Composition of emulsions/emulsion gels with different content of native protein and denatured protein.
Group
A
B
Sample codes
Cprotein-D
Cprotein-N
(w/w)
(w/w)
A1
4.5%
0.5%
A2
4%
1%
A3
3.5%
1.5%
B1
4%
0.5%
B2
4%
1%
B3
4%
1.5%
*A2 and B2 were the same sample. For the ease of understanding, different codes were used.
25
Table 2. Droplet characteristics of emulsions with different content of native protein and
denatured protein. Samples
Size
PDI
Zeta potential (mV)
A1
393.75±7.71
a
0.24±0.05
-43.32±2.56a
A2/B2
326.88±4.23b
0.23±0.04
-51.02±1.88b
A3
276.33±7.19c
0.19±0.07
-56.62±1.30c
B1
400.20±8.51a
-46.90±0.90d
B3
283.47±6.22c
0.24±0.07 0.18±0.01
-46.23±0.21d
Values with different lowercase letters in the same column indicate a significant difference among the values of p < 0.05. A2 and B2 were the same sample. For the ease of understanding, different codes were used.
26
Table 3. Texture properties of emulsion gels with different content of native protein and denatured protein.
Samples
Fracture stress (MPa)
Fracture strain
a
0.52±0.04
Young's modulus (MPa)
a
9.00±0.41a
A1
3.53±0.17
A2/B2
3.06±0.14b
0.47±0.04ab
8.83±0.20a
A3
2.99±0.07c
0.45±0.02b
8.11±0.31b
B1
2.99±0.06c
0.45±0.02b
8.52±0.25c
B3
3.10±0.22b
0.48±0.04ab
9.00±0.41a
Values with different lowercase letters in the same column indicated a significant difference (p < 0.05). A2 and B2 were the same sample. For the ease of understanding, different codes were used.
27
Table 4. Degradation rate constant (k), half-life time (t1/2), regression coefficient of first-order kinetic model (R2) for β-carotene in emulsion gels at different storage conditions. R2
t1/2 (h)
k (10-4h-1) Samples UV-light
25 °C
55 °C
UV-light
25 °C
55 °C
UV-light
25 °C
55 °C
A1
77.41±0.29a
1.85±0.36a
2.56±0.35a
8.95
374.59
270.70
0.8198
0.8865
0.9307
A2/B2
91.83±0.23b
1.85±0.13a
2.71±0.05a
7.55
374.59
255.72
0.9183
0.9793
0.9987
A3
105.60±0.34c
2.24±0.11b
3.21±0.20b
6.56
309.38
215.89
0.8644
0.9913
0.9844
B1
115.82±0.33d
2.05±0.22b
3.23±0.15b
5.98
338.05
214.55
0.8911
0.9547
0.9909
B3
73.21±0.25e
1.47±0.16c
2.64±0.22a
9.47
471.43
262.5
0.8526
0.9511
0.9729
Values with different lowercase letters in the same column indicated a significant difference (p < 0.05). A2 and B2 were the same sample. For the ease of understanding, different codes were used.
28
Figure 1
A
40 A1
Viscosity (mPa.s)
35
A2
30
A3
25 20 15 10 5 0 0
100
200 Shear rate (s-1)
300
B 40
B1
35 Viscosity (mPa.s)
400
B2
30
B3 25 20 15 10 5 0 0
100
200 Shear rate (s-1)
300
400
Fig. 1. Viscosity of the emulsions with different content of native protein and denatured protein (A: fixed total protein content; B: fixed denatured protein content). A2 and B2 were the same sample. For the ease of understanding, different codes were used.
29
Figure 2
A
0.50
Instability index
0.40
0.30
0.20
0.10
0.00
B
A1
A2
A3
B1
B2
B3
0.50
Instability index
0.40
0.30
0.20
0.10
0.00
Fig. 2. Instability index of emulsions with different content of native protein and denatured protein (A: fixed total protein content; B: fixed denatured protein content). A2 and B2 were the same sample. For the ease of understanding, different codes were used.
30
Figure 3
A 100000
G', G'' (Pa)
10000
1000
100 A1,G' A1,G'' A2, G' A2, G'' A3, G' A3, G''
10
1 0
2000
4000 Time (s)
6000
8000
B 100000
G', G'' (Pa)
10000
1000
100 B1,G' B1,G'' B2, G'
10
B2, G'' B3, G' B3, G''
1 0
2000
4000 Time (s)
6000
8000
Fig. 3. Gelation dynamics of the emulsion gels with different content of native protein and denatured protein (A: fixed total protein content; B: fixed denatured protein content). A2 and B2 were the same sample. For the ease of understanding, different codes were used.
31
Figure 4 B1
A1
A2/B2
A3
B3
Fig.4. Microstructures of emulsion gels with different content of native protein and denatured protein. A2 and B2 were the same sample. For the ease of understanding, different codes were used.
32
Figure 5
A
6
Swelling ratio (%)
5 4 3 2 1 0 A1
A2
A3
B1
B2
B3
B6
Swelling ratio (%)
5 4 3 2 1 0
C A1
A2
A3
B1
B2
B3
Fig.5. Swelling properties of emulsion gels with different content of native protein and denatured protein. (A: fixed total protein content; B: fixed denatured protein content; C morphology of the samples after swelling test). A2 and B2 were the same sample. For the ease of understanding, different codes were used.
33
Figure 6
A 100
a
b
c
A1
A2
A3
c
b
B1
B2
80
WHC (%)
60
40
20
0
B 100
a
80
WHC (%)
60
40
20
0 B3
Fig.6. Water holding capacity (WHC) of emulsion gels with different content of native protein and denatured protein (A: fixed total protein content; B: fixed denatured protein content). A2 and B2 were the same sample. For the ease of understanding, different codes were used.
34
Figure 7
A
B
Fig. 7. The retention ratios of β-carotene in emulsions gels with different content of native protein and denatured protein when exposed to light (A: fixed total protein content; B: fixed denatured protein content). A2 and B2 were the same sample. For the ease of understanding, different codes were used.
35
Figure 8
A
B
C
D
Fig. 8. The retention ratios of β-carotene in emulsions gels with different content of native protein and denatured protein when stored at 25 and 55 °C (A&B: fixed total protein content; C&D: fixed denatured protein content). A2 and B2 were the same sample. For the ease of understanding, different codes were used.
36
Emulsion gels were prepared with both denatured protein and native protein. Emulsion properties were mostly affected by the content of native protein. The denatured protein played a leading role in the gelation process and structures of the emulsion gels. Both proteins were responsible for the stability of β-carotene.
We declare that we have no conflict of interest.
Author statement
The work presented in this paper has not been published previously, that it is not under consideration for publication elsewhere, that its publication is approved by all authors and tacitly or explicitly by the responsible authorities where the work was carried out, and that, if accepted, it will not be published elsewhere in the same form, in English or in any other language, including electronically without the written consent of the copyright-holder.
S0268-005X(19)32160-5
DOI:
https://doi.org/10.1016/j.foodhyd.2019.105600
Reference:
FOOHYD 105600
To appear in:
Food Hydrocolloids
Received Date: 18 September 2019 Revised Date:
22 November 2019
Accepted Date: 16 December 2019
Please cite this article as: Lu, Y., Mao, L., Zheng, H., Chen, H., Gao, Y., Characterization of β-carotene loaded emulsion gels containing denatured and native why protein, Food Hydrocolloids (2020), doi: https://doi.org/10.1016/j.foodhyd.2019.105600. This is a PDF file of an article that has undergone enhancements after acceptance, such as the addition of a cover page and metadata, and formatting for readability, but it is not yet the definitive version of record. This version will undergo additional copyediting, typesetting and review before it is published in its final form, but we are providing this version to give early visibility of the article. Please note that, during the production process, errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain. © 2019 Published by Elsevier Ltd.
Graphical abstract
1
Characterization of β-carotene loaded emulsion gels containing
2
denatured and native why protein
3
Yao Lu, Like Mao*, Hongxia Zheng, Hongqiang Chen, Yanxiang Gao
4 5
Beijing Advanced Innovation Center for Food Nutrition and Human Health, Beijing
6
Laboratory for Food Quality and Safety, College of Food Science & Nutritional
7
Engineering, China Agricultural University, Beijing, China
8 9 10 11 12 13 14 15 16 17 18
Corresponding author:
19
Tel: +86-10-62737034
20
Fax: +86-10-62737986
21
E-mail: [email protected] (L. Mao)
22
1
23
Abstract:
24
The current study developed whey protein emulsion gels containing β-carotene, and the
25
effects of the content of denatured protein and native protein were investigated. Two
26
sets of emulsion gels were obtained by fixing the total protein content or the denature
27
protein content (Cprotein-D). Emulsion properties were mostly affected by the content of
28
native protein (Cprotein-N), and higher Cprotein-N resulted in emulsions with smaller
29
particle size, higher surface charge and better creaming stability. Emulsions were then
30
gelled with the addition of Glucono-δ-lactone. At fixed total protein content, higher
31
Cprotein-D contributed to gels with higher mechanical properties, e.g., fracture stress,
32
Young’s modulus and storage modulus (G′). At fixed Cprotein-D, the increase in Cprotein-N
33
also resulted in stronger gels but at much lower magnitude. The dynamic gelation
34
analysis revealed that the increase in Cprotein-N or Cprotein-D resulted in shorter gelling
35
time. All the gels had rather high water holding capacity, and the gels with greater
36
mechanical strength had lower swelling ratios. When emulsion gels were applied as
37
carriers for β-carotene, both Cprotein-D and Cprotein-N had significant effects on the light
38
stability and heat stability of β-carotene.
39
Keywords: emulsion gel; denatured protein; native protein; gel structure; β-carotene
40 41 42 43 44 45 46 47
2
48
1. Introduction
49
Emulsion gels are structured emulsion systems, which have dispersed phases entrapped
50
within three-dimensional (3D) network (Farjami & Madadlou, 2019). Yoghurt, cheese,
51
and some processed meat are common food with emulsion gel structures. Emulsion
52
gels are generally prepared through two-stage processes, i.e., emulsification and
53
gelation. The gelation can be originated from proteins, polysaccharides or their
54
mixtures, via heat-induced, salt-induced, acid-induced, or enzyme-induced approaches
55
(Lu, Mao, Hou, Miao, & Gao, 2019). When the gelling agents have surface activity
56
(e.g., whey protein, soy protein, gum Arabic), they may also behave as emulsifiers to
57
stabilize the emulsions. In other cases, emulsifiers and gelling agents can be different
58
ingredients. Emulsion gels are usually applied to structure food systems, offering
59
desirable rheological and textural properties, and they are also widely used in
60
fat-reduced food (Dickinson, 2012). Many recent studies have revealed that emulsion
61
gels are suitable carriers for lipid-soluble food bioactives, as the strong gel network can
62
provide effective protection, and the modulation of gel structures allows controlled
63
release and digestion of the incorporated ingredients (McClements, 2010; Torres,
64
Murray, & Sarkar, 2016; Lu, et al., 2019).
65
In emulsion gels, compositions and structures of the interface and continuous phase
66
have great influence on the their functionality. According to the different interactions
67
between the interfacial membrane and the continuous gel, the dispersed oil droplets can
68
behave as active or inactive fillers (Dickinson, 2012; Lu, et al., 2019). With active
69
fillers, the dispersed phase also participates the assembly of the gel network, and it is
70
able to reinforce gel structure. Generally, emulsion gels using proteins to stabilize the
71
interface and gel the continuous phase have active fillers. In these systems, the
72
reduction in oil droplet size contributed to larger interfacial area, and thus led to gels
3
73
with higher strength (Sala, van Vliet, Cohen Stuart, van de Velde, & van Aken, 2009).
74
Literature studies also indicated that droplet coalescence or oil solidification could
75
assist the formation of stronger gels (Oliver, Wieck,
76
Scholten, & van Aken, 2015). Furthermore, the interface can largely influence droplet
77
distribution and emulsion stability, which may also affect the structures of the gels
78
(Guido, van Aken, Cohen Stuart, & van de Velde, 2010). Although different proteins
79
(e.g., whey protein, soy protein, sodium caseinate) have been tested for their roles in the
80
properties of emulsions gels, no detailed information regarding the effects of the
81
content and structures of proteins at the interface were available (Lu, et al., 2019). With
82
inactive fillers, the oil-water interface has minor or no interactions with the continuous
83
gel body, and the oil phase is likely to weaken the gel structure. Generally, the gel
84
systems containing low molecular weight surfactants have inactive fillers (Dickinson,
85
2012).
86
The biopolymers (i.e., proteins, polysaccharides) in the continuous phase constitute the
87
main structures of the gel network, and their structures and content play essential roles.
88
In a typical cold-gelation process, proteins are preheated to unfold their ternary
89
structures and expose hydrophobic residues. The denatured protein molecules then
90
aggregate to form 3D network with the aid of gelation triggers, e.g., acid, salt or
91
enzymes (Mao, Lu, Cui, Miao, & Gao, 2019). Generally, emulsion systems with higher
92
protein content are more favorable for the formation of compact gel network because of
93
the presence of larger number of crosslinking sites. Second, with large number of oil
94
droplets dispersed in protein dispersion, the protein concentration threshold for gelation
95
can be well reduced, compared to pure gel systems. Mao et al. (2014) reported that a
96
system with a protein content of 4% was able to form emulsion gels with
97
self-supporting behaviors. Third, at a fixed protein concentration, protein preheating of
4
& Scholten, 2016; Oliver,
98
higher intensity (e.g., longer heating time, higher heating temperature) could facilitate
99
the formation of denser gel network (Mao, Miao, Yuan, & Gao, 2018). In some
100
emulsion gels, there could be two or more proteins and/or polysaccharides
101
(Balakrishnan, Nguyen, Schmitt, Nicolai, & Chassenieux, 2017; Feng, Jia, Zhu, Liu, &
102
Yin, 2019). In these systems, the interactions between biopolymers had critical impact
103
on the development and structures of the gels. Depending on the charging properties,
104
proteins and/or polysaccharides could form gel systems with single continuous phase,
105
double continuous phase, uniform continuous phase, or non-homogeneous chained gel
106
systems (van de Velde, de Hoog, Oosterveld, & Tromp, 2015). Furthermore,
107
biopolymer-biopolymer interactions were likely to change during the gelation as
108
affected by pH, ionic strength, etc., which then affected gel structures (Williams,
109
Phillips, Matiamerino, & Dickinso, 2004). However, less attention was paid to the gel
110
systems containing non-gelling biopolymers.
111
In the current study, native whey protein was used mainly as an emulsifier, and
112
heat-denatured whey protein was used as a gelling agent. β-Carotene loaded emulsion
113
gels were prepared by varying the content of denatured protein and native protein, and
114
both emulsion properties and gel properties were characterized, aiming to better
115
understand the roles of oil-water interface and continuous phase in the structure and
116
functionality of the gel systems. To the authors’ knowledge, it is the first time to study
117
emulsion gel systems with one type of protein at both native and denatured states,
118
which is meaningful for the innovation of healthy food.
119
2. Materials and methods
120
2.1. Materials
121
Corn oil was the product of Changshouhua Food Company Limited (Shandong, China),
122
and used withoug additional purification. Bipro-type whey protein isolate(WPI) was 5
123
purchased from Davisco Foods (Le Sueur, MN, USA). Crystalline β-carotene with a
124
purity >99% was a favor of NHU Holding Group Co., Ltd. (Zhejiang, China). Sodium
125
azide, glucono-δ-lactone (GDL), n-hexane were products of Sigma-Aldrich (St. Louis,
126
MO, USA).
127
2.2. Preparation of denatured protein powder
128
To induce protein denaturation, WPI dispersion (5 wt%) was incubated in a water bath
129
at 85 °C for 30min, and then cooled rapidly to about 25 °C using ice. The samples were
130
lyophilized using a vacuum freeze dryer (Marin Christ, Germany), and the obtained
131
protein powder was stored in a desiccator for further use.
132
2.3. Determination of interfacial tension
133
Protein powder was hydrated in deionized water and kept overnight. Then interfacial
134
tension between protein solution (1 wt%) and corn oil was measured using a
135
Tensiometer K100 (Krüss, Hamburg, Germany) following a classical Wilhelmy plate
136
method. During the measurement (20 °C), a platinum Wilhelmy plate (19.9×10×0.2
137
mm) was immersed in the protein solution (20 mL) to a depth of 3 mm at a surface
138
detection speed of 15 mm/min. The vessel drive speed applied for the tracking of the
139
liquid surface was regarded as the surface detection speed. When the surface was
140
determined by the microbalance in the machine, the vessel moved at the selected
141
surface detection speed to the position specified by the immersion depth (3 mm).
142
Afterwards, an interface between the protein solution and corn oil was created by
143
carefully inject the corn oil over the protein solution (O'Sullivan, Rellano, Pichot, &
144
Norton, 2014). Evolution of interfacial tension during the measurement of monitored,
145
and the values at equilibrium were reported.
146
2.4. Emulsion preparation
6
147
The method for the preparation of emulsions was previously reported by Mao, Roos &
148
Miao (2014). WPI (native) dispersions of different protein content were mixed with
149
corn oil (20 wt%) using a high speed blender (Ultra-Turrax, IKA, Germany) to form
150
coarse emulsions, which were then homogenized at 500 bar for three passes using a
151
high pressure homogenizer (Niro-Soavi, Parma, Italy). The emulsions were rapidly
152
cooled to about 25 °C using ice. The lyophilized denatured protein powder was added
153
to the emulsions, and mixed well for complete hydration of the powder.
154
For the preparation of β-carotene emulsions, β-carotene crystals (6 wt%) were first
155
dissolved in the oil phase at 140 °C before mixing with the water phase. Samples
156
containing different content of native protein (Cprotein-N) and denatured protein (Cprotein-D)
157
were listed in Table 1.
158
2.5. Characterization of WPI stabilized emulsions
159
Droplet size and surface charge of the emulsions were determined by utilizing a
160
Malvern Zetasizer (Nano-ZS90, Malvern Instrument, UK). RI (refractive index) of
161
aqueous and oil phases were set to 1.33 and 1.45, respectively. In order to reduce
162
multiple scattering effect, each sample was diluted with deionized water prior to the
163
measurement. Droplet size was described as hydrodynamic diameter (nm) and
164
polydispersity index (PDI), and surface charge was described as ζ-potential (mV).
165
Viscosity of the emulsions was evaluated via a DHR-2 rheometer (TA Instruments,
166
UK) , and the geometry with parallel plates (40 mm diameter and 1 mm gap) was
167
selected. The determination was carried out at the shear rate range of 10–400 s−1 at
168
25 °C.
169
Emulsion stability was determined using a LUMiSizer (L.U.M.GmbH, Berlin,
170
Germany), which applied centrifugation force to accelerate the test. The machine used
171
near-infrared light (880 nm) to scan the whole samples, and intensity of the transmitted 7
172
light was recorded. The measurement (25 °C) was set at a centrifugation speed of 4000
173
rpm and the samples were scanned 800 times at an interval of 10 s. The curves of
174
integrated intensity of the light transmitted as a function of time were plotted, and
175
slopes of the curves were regarded as instability index (Mao, Roos, & Miao, 2015).
176
2.6. Preparation of emulsion gels
177
Emulsion gels were prepared following the method reported previously (Mao, et al.,
178
2014). Briefly, GDL (0.5 wt%) was introduced into emulsions and mixed well with
179
stirring bars, and the mixtures were incubated quiescently at 25 °C for 12 h to form the
180
gels.
181
2.7. Characterization of emulsion gels
182
2.6.1. Viscoelastic behaviors
183
The same rheometer for viscosity analysis was also applied to the evaluation of
184
viscoelastic characteristics of the gels. Emulsion drops were placed onto the plate right
185
after the addition of GDL, and the dynamic gelation process was evaluated at a strain of
186
0.5% and a frequency of 1 Hz under the oscillation mode (25 °C). The linear
187
viscoelastic range of the samples was pre-determined through a strain sweep. The
188
evolution of storage modulus (G′) and loss modulus (G′′) in the gelation process were
189
recorded (Mao et al., 2018).
190
2.6.2. Textural properties
191
Textural analysis was performed for all the emulsion gels using a FTC texture analyzer
192
(Rockville, Maryland, USA). Samples for the test were specifically formed in plastic
193
containers (34 mm id., 50 mm height) following the approach reported earlier. The gels
194
received uniaxial compression by a 12 mm cylindrical plunger at a strain of 50%.
8
195
Fracture stress, fracture strain and Young’s modulus of the samples were then
196
calculated. All the reported values were means of eight replicates.
197
2.6.3. Swelling ratio
198
Swelling ratios of the gels were measured according to a study by Carvajal-Millan et al.
199
(2015). The gels were cut into cylindrical shape and weighed, and the initial mass was
200
recorded as M0. All the samples were immersed in deionized water for 24 h, and then
201
the swollen gels were moved out for mass determination (M). The swelling ratio (t) was
202
calculated using the following equation: t = (M-M0)/M0 * 100
203 204
2.6.4. Water holding capacity (WHC)
205
WHC of the gels was measured following the method reported by Wang and
206
co-workers (2018) with slight adjustments. The emulsions were gelled in 10 mL
207
centrifuge tube and weighed (W0). Afterwards, samples were centrifuged at 14,000 rpm
208
and 25 °C for 20 min. The water released was removed, and the mass of the remaining
209
gels (with centrifuge tube) was weighed and recorded as W. WHC (%) of the emulsion
210
gels was calculated using the equation below: WHC=(W0-W)/W0 *100
211 212
2.6.5. Scanning electron microscopy (SEM) observation.
213
Microstructural observation of the samples was carried out using a SU-8100 SEM
214
(Hitachi, Japan). The gel structures were fixed in a glutaraldehyde-cacodylate buffer,
215
followed by ethanol dehydration and critical point drying. The dried samples were then
216
placed on a copper stud and sputtered with gold for the observation.
217
2.8. Stability of β-carotene
218
2.8.1. UV-light stability
9
219
Light stability test was performed in a Q-SUN xenon test chamber (Q-Panel Lab
220
Products, USA) at an irradiance of 0.68 W/m2. Fresh emulsion gels were first moved
221
into transparent glass bottles (flushed with nitrogen), and then incubated in the test
222
chamber for 8h at 25 °C (Liu, Wang, Xu, Sun, & Gao, 2016). Sampling was done each
223
2h to determine the remained content of β-carotene.
224
2.8.2. Thermal stability
225
Glass bottles (flushed with nitrogen) containing fresh emulsion gels were incubated at
226
25 and 55 °C for 15 d at dark. Sampling was done every 3d to determine the remained
227
content of β-carotene.
228
2.8.3. Determination of the content of β-carotene
229
Emulsion gels from stability test were mashed to destroy the gel structures for the ease
230
of the extraction of β-carotene with n-hexane. β-Carotene content was then determined
231
using a UV 1800 spectrophotometer (Shimadzu, Japan) by recording the absorbance at
232
450 nm, in assistance with a standard curve (Yuan, Gao, Zhao, & Mao, 2008).
233
Retention ratio C/C0 (C: content of β-carotene after storage; C0: initial content of
234
β-carotene before storage) of β-carotene in the gels after the test was applied to describe
235
the stability of β-carotene.
236
By fitting a first-order kinetic model, the degradation kinetics of β-carotene was also
237
evaluated. Reaction rate constant (k) and half-life (t1/2) of β-carotene was calculated
238
following the equations below (Sharma, Kaur, Oberoi, & Sogi, 2008): C / C 0 = exp(−k • t )
239 240
ln C = ln C 0 − kt
241
t1 / 2 = ln 2 / k 242
2.9. Statistical analysis
10
243
Mean values ± standard deviations (SD) were reported for all data points based on three
244
replicates. An analysis of variance (ANOVA) of the data was performed using Origin
245
Pro 8 at a level of significance of 5%.
246
3. Results and discussion
247
3.1. Characterization of the emulsions
248
It is known that proteins in the continuous phase or at the interface can largely affect
249
emulsion properties (McClements, 2004). However, there is little information available
250
when a mixture of denatured protein and native protein is used. Table 2 summarizes the
251
droplet characteristics of the emulsions, i.e., droplet size, PDI and surface charge, as
252
affected by the content of proteins at the interface and continuous phase. At fixed total
253
protein content (group A), the increase in Cprotein-N led to smaller particle size and lower
254
PDI of the emulsions, as higher interfacial coverage prevented droplet association via
255
steric hindrance and electrostatic repulsion (McClements, 2015). In fact, the magnitude
256
of zeta-potential was also higher in the emulsions with higher Cprotein-N. At fixed
257
Cprotein-D (group B), similar trends were also observed, and the increase in Cprotein-N
258
contributed to emulsions with smaller particle size. At fixed Cprotein-N, the change in
259
Cprotein-D did not affect particle size significantly (A1 and B1, A3 and B3). Therefore,
260
the content of native protein played a more significant role in emulsion properties. The
261
interfacial tension between protein solution and corn oil was also determined, and the
262
result indicated that the native protein (13.748±0.029 mN/m) was capable to reduce the
263
interfacial tension a lower level than the denatured protein (14.935±0.006 mN/m) at
264
equilibrated state, which was in agreement with literature study (Euston, Finnigan, &
265
Hirst, 2000). Besides, native protein was firstly added to form the emulsions, followed
266
by the addition of denatured protein. Therefore, the native protein was more likely to
11
267
dominate the interface. However, the emulsions with lower Cprotein-D had significantly
268
higher magnitude of surface charge (B1>A1, A3>B3). There could be some
269
interactions between denatured protein and native proteins (Vardhanabhuti, Foegeding,
270
McGuffey, Daubert, & Swaisgood, 2001), and the resultant complex might have
271
decreased amount of charged moieties. For example, the exposed thiol groups in
272
denatured protein can interact with the surface active groups of native protein (Torres,
273
Janhøj, Mikkelsen, & Ipsen, 2010). However, the underlying mechanisms required
274
further investigation.
275
Fig. 1 shows the difference in viscosity between the two groups of emulsions. The
276
results indicated that all the emulsions were shear-thinning fluids, and viscosity of the
277
emulsions decreased gradually with the increase in shear rates (Dybowska, 2004).
278
Shear thinning behavior was a sign of droplet flocculation in emulsions, which
279
presented resistance against shearing at lower force and broke up at high shear rates
280
(Floury, Desrumaux, & Lardières, 2000). Dickinson et al. (1997) believed that
281
reversible depletion flocculation caused by unabsorbed protein present in the
282
continuous phase can cause pseudoplasticity of the emulsion. In the current systems,
283
there was also a high content of denatured protein at the continuous phase, which was
284
possible to induce droplet flocculation (Euston et al., 2000). Second, as protein
285
denaturation had thickening effect, the increase in Cprotein-D contributed to the systems
286
with higher viscosity (Fig. 1A) (Britten, Giroux, Jean, Rodrigue, 1994). At fixed
287
Cprotein-D, the change in Cprotein-N did not affect emulsion viscosity significantly (Fig. 1B).
288
It is known that emulsions with smaller particles generally have higher viscosity
289
(McClements, 2010), which was not observed for the present samples, probably due to
290
the bigger roles of Cprotein-D.
12
291
All the emulsions had good creaming stability before gelation, probably due to the high
292
content of protein, and the higher interfacial charge. We performed acceleration tests to
293
observe the differences in emulsion stability by applying a multisample centrifugation
294
technique. Fig. 2 reveals that emulsions with higher Cprotein-N generally had lower
295
instability index, both at fixed total protein content and Cprotein-D.
296
3.2. Characterization of the emulsion gels
297
3.2.1. Viscoelastic properties of the emulsion gels
298
The gelation process was simulated in a rheometer, and the evolution of the rheological
299
properties of the systems was evaluated (Fig.3). In the current study, all the systems
300
followed similar gelation dynamics, which could be divided into three stages. At the 1st
301
stage, both G' and G'' of the systems were low and increased slowly. In this stage, the
302
hydrolysis of GDL was just initiated, and pH of the systems was still high, and there
303
was little interaction between protein aggregates; At the 2nd stage, both G' and G'' got
304
sharp increase, and G' was increased even faster. In this stage, pH of the systems was
305
lowered to the isoelectric point (pI) of the protein, and the protein molecules tended to
306
form 3D network as a result of hydrophobic attraction, van der Waals forces and
307
hydrogen bonding (Ye & Talor, 2009; Mellema, van Opheusden, & van Vliet, 2002). In
308
some studies, the time point at which the sharp increase started was refered to as gelling
309
time (Ersch et al., 2015); At the 3rd stage, the increase of G' and G'' was well slowed
310
down until levelled off. In this stage, pH of the systems was kept at low level (Mao et al.,
311
2014), and the development of the gel network gradually reached a steady state. At
312
fixed total protein content, the system with the highest Cprotein-D (A1) started all the three
313
stages much earlier than the other two systems, because of the earlier onset of gelation.
314
Furthermore, G' at the steady state was higher in the systems with higher Cprotein-D
315
(A1>A2>A3) (Fig. 3A). These results indicated the big role of denatured protein in the 13
316
development of the gel network. With higher Cprotein-D, there were more binding sites
317
for aggregate association, leading to faster gelation and higher gel strength. At fixed
318
Cprotein-D, the increase in Cprotein-N (with higher total protein content) resulted in faster
319
gelation and bigger G' at the steady state (Fig. 3B). The findings indicated that the
320
native protein took part in the development of the gel network, and higher total protein
321
content promoted gelation. It has been well documented that denatured protein at the
322
interface participate the gelation process with the denatured protein at the continuous
323
phase (Ye & Talor, 2009; Mao et al., 2018). However, there was little information on
324
the roles of native protein in the gelation of denatured protein. In fact, the current
325
systems could be regarded as mixed emulsion gels with two proteins. The native
326
protein in the current systems was not possible to gel individually, because of its folded
327
structures and low concentration. On the other hand, no phase separation was observed
328
when the two proteins coexisted in the dispersions, indicting the two proteins were
329
thermodynamically compatible. Therefore, there were other mechanisms responsible
330
for the participation of the native protein in the gel network: 1) Native protein (either in
331
the continuous phase or at the interface) formed complexes with denatured protein
332
(through electrostatic or hydrogen bonding) (Britten, Giroux, Jean, & Rodrigue, 1994;
333
Zhai, Day, Aguilar, & Wooster, 2015); 2) Native protein behaved as fillers to support
334
the gel network. With higher density of protein deposited at the interface, the oil
335
droplets could have higher density and strengthen the gel structures (Lu, et al., 2019);
336
the native protein could compete for water binding and concentrated the denatured
337
protein (Ersch, ter Laak, van der Linden, Venema, & Martin, 2015). Wu et al. (2018)
338
concluded that non-networking proteins (mainly soy protein peptides) did not affect the
339
G′ of the emulsion gels (heat-induced), because the non-networking proteins were
340
dissolved and located at the pores of gel network. However, in the current study, native
14
341
protein was believed to be mostly distributed at the interface. Second, different gelation
342
methods and protein structures in the two studies could also be responsible for the
343
contradicting results. It was deducted that the oil droplets worked as active fillers in
344
these systems (Dickinson, 2012). However, systems with smaller oil droplets (e.g., A3)
345
did not always had higher G', probably because the size effect was blocked by the big
346
role of protein content.
347
3.2.2. Textural properties
348
Gel food received compression and stretching during oral processing, and the forces
349
received by the brain were largely perceived as texture (Stokes, Boehm, & Baier, 2013).
350
Table 3 represents the textural characteristics of the emulsion gels. It was observed that
351
the content of denatured protein and native protein greatly affected the texture of the
352
gels. At fixed total protein content, the increase in Cprotein-D was accompanied by the rise
353
in fracture stress and Young’s modulus (A1>A2>A3), indicating the big role of the
354
denatured protein in the formation of gel structures of high strength. Similar results
355
were also obtained by Vardhanabhuti and coworkers (2001), who found that the
356
replacement of native whey protein by denatured protein resulted in gels with higher
357
fracture stress and modulus. It was reported that Young’s modulus could reflect
358
molecular rigidity, which for biopolymers, could be a sign of the number of cross-links.
359
With higher Cprotein-D, there were more cross-linking sites in the systems, leading to
360
higher rigidity of the gels (Saavedra Isusi, Karbstein, & van der Schaaf, 2019). At fixed
361
Cprotein-D, only slight increase in Young’s modulus and fracture stress (B3>B2>B1) with
362
the increase in Cprotein-N was observed. In the current study, gelation was originated
363
from the aggregation of protein molecules, which was favorable when the molecules
364
were unfolded (at denatured state). For example, by changing the Cprotein-D from 4% (B1)
365
to 4.5% (A1), the fracture modulus was increased by 18.06% (from 2.99 to 3.53 MPa);
15
366
by changing the Cprotein-N from 1% (B2) to 1.5% (B3), the fracture stress was only
367
increased by 1.31% (from 3.06 to 3.10 MPa). These results also indicated that the
368
current systems were homogeneous, as inhomogeneity usually resulted in a decrease in
369
fracture stress, as result of stress concentration (van Vliet & Walstra, 1995).
370
Interestingly, fracture strain of the gels was independent on Cprotein-D and Cprotein-N,
371
probably because of the soft nature of the gels at the current protein range.
372
3.2.3. Microstructures
373
Figure 4 illustrates the morphology of the emulsion gels through SEM observation,
374
which clearly showed the differences in the microstructures of the samples. At fixed
375
total protein content (group A), the gels with higher Cprotein-D had more compact
376
structures with smaller pores. In sample A1, the gel network was formed by protein
377
aggregates of smaller size and similar shape. In sample A3, the aggregates were rather
378
big with different shapes. The results reconfirmed the bigger roles of denatured protein
379
for the development of compact gel network. At fixed Cprotein-D, the changes in Cprotein-N
380
only resulted in slight changes in the microstructures of the gels. Comparatively, the
381
gels with the highest Cprotein-N had the densest structure and lowest number of pores.
382
Whey protein could develop particulate gels or filamentous gels, which was mainly
383
dependent on the force balance between attraction and repulsion among protein
384
molecules (Lefevr & Subirade, 2000; Ikeda & Li-Chan, 2004). In the current study,
385
lower repulsion force was present as the pH of the gels was lowered to the pI of the
386
protein, and the development of particulate gels was favored. Oil droplets could not be
387
clearly observed in these SEM images, because they were completely surrounded by
388
the particulate protein network. In fact, there were a lot of small-sized protrusion at the
389
surface of the gel network, which could be the oil droplets (Lu et al., 2019).
390
3.2.4. Swelling ratio & WHC
16
391
The three-dimensional network in emulsion gels entrap a certain amount of water, and
392
they are also able to adsorb addition water (Begam, Nagpal, & Singhal, 2003), which
393
are important for the mouth feel of gel food and the release of functional ingredients
394
incorporated (Lu et al., 2019). Swelling properties of gels were highly dependent on the
395
pore size and water-adsorbing capacity of the gelling biopolymers (Feng et al., 2019).
396
Fig. 5A reveals that the gels with higher Cprotein-D (fixed total protein content) had lower
397
swelling ratios. For example, the swelling ratio of A1 was 1.64%, and that of A3 was
398
4.46%. As discussed earlier, higher Cprotein-D contributed to more compact gel network,
399
and there could be only small pores to accommodate additional water. Second,
400
denatured protein had decreased capability to adsorb water (Saffon, Britten, & Pouliot,
401
2011). Third , the gels already had high amount of water adsorbed during the
402
development of gel network. In fact, all the three gels maintained their self-supporting
403
structures after the swelling test. Fig. 5B indicates that gels with lower Cprotein-N (fixed
404
Cprotein-D) had higher swelling ratios. The greater adsorption of water might be resulted
405
from the bigger size of the oil droplets (Feng et al., 2019). Morphological observation
406
showed that the gels with higher swelling ratio became softer and were not able to
407
maintain their intact structures. During food digesting, swelling of gels can facilitate
408
bioactive release (Mao et al., 2019).
409
Water holding capacity (WHC) refers to the ability of the tested samples to immobilize
410
moisture through capillary forces, which is largely dependent on pore size (Wu et al.,
411
2009). Fig. 6 indicates all the samples had quite big WHC (>85%), and there was small
412
difference among samples. At fixed total protein content, the highest WHC (87.29%)
413
was observed in the sample with the highest Cprotein-D. At fixed Cprotein-D, the highest
414
WHC (88.78%) was found in the sample with the highest Cprotein-N. Some studies
415
concluded that WHC and storage modulus of emulsion gels had positive association
17
416
(Sok Line, Remondetto, & Subirade, 2005; Yang, Liu, & Tang, 2013), which was also
417
found in the current study. Emulsion gels with higher storage modulus generally had
418
denser and more uniform microstructures, which allowed the gels to hold water
419
molecules strongly against centrifugation (Hu et al., 2013). In the current systems,
420
water was mostly bound to proteins, and only small amount of water could be present in
421
the pores of the gel network. Vardhanabhuti et al. (2001) suggested there could be a
422
transition in network structures from particulate to a more filamentous structures in gels
423
with more denatured protein, and the latter type of gels had higher ability to hold water.
424
3.3. Emulsion gels as carriers for β-carotene
425
β-carotene has strong antioxidant activity, and it is able to enhance the specific and
426
non-specific immune function. However, β-carotene is extremely sensitive to light,
427
heat and oxygen, and is prone to degradation, which can result in the loss of its
428
bioactivity (Rodriguez-Amaya, 2015). It has been proved that delivery systems,
429
including emulsions, gels, nanoparticles are able to protect β-carotene from
430
degradation (Mao, Wang, Liu, & Gao, 2018).
431
Fig. 7 shows the changes in the retention ratios of β-carotene within emulsion gels of
432
different protein content during the light stability test. At fixed total protein content
433
(Fig. 7A), the emulsion gels with higher Cprotein-D can retain more β-carotene
434
(A1>A2>A3). For example, in the gel with a Cprotein-D of 4.5%, about 56.53±0.03% of
435
the original content of β-carotene was retained after the test. However, only 45.06 ±
436
0.02% β-carotene was retained in the sample with a Cprotein-D of 3.5%. As discussed
437
earlier, gels with higher Cprotein-D had denser structures, which could effectively prevent
438
the contact of the embedded functional ingredients with external environmental stresses.
439
Second, carotenoids can form complexes with protein through hydrophobic
440
interactions (Dufour, &Haertlé, 1991;Wackerbarth, Stoll, Gebken, Pelters, Bindrich, 18
441
2009), and the complexes could be more resistant to oxidation. At fixed Cprotein-D, the
442
stability of β-carotene was improved with the increase in Cprotein-N (B3>B2>B1). This
443
may be due to the fact that β-carotene degradation was initially started at the emulsion
444
interface (Liu et al., 2016). The increase in Cprotein-N can enhance the thickness of the
445
interfacial film and effectively inhibit the initiation and propagation of the oxidation
446
process (Waraho, McClements, & Decker, 2011). Second, there were some
447
antioxidative moieties in protein molecules, e.g., cysteyl residues, disulphide bonds and
448
thiol groups, which also worked to inhibit β-carotene oxidation (Mao et al., 2018).
449
When the emulsion gels were stored at different temperatures (25 °C and 55 °C), the
450
changes in the retention ratios of β-carotene followed similar trends as those observed
451
in the light stability test (Fig. 8). For example, after a 12-day storage test, the retention
452
rate of β-carotene in A1 was 57.61±0.01% (25 °C) and 45.61±5.55% (55 °C), and that
453
of A3 was 52.81±0.02% (25 °C) and 37.81. ±1.92% (55 °C). In general, gels with
454
higher gel strength and denser structures could provide stronger protection for
455
β-carotene against adverse stresses. Similar results were also observed in other studies
456
on different lipophilic bioactives (Lu et al., 2019). Although the increase in the content
457
of native protein and denatured protein were both helpful in retaining higher content of
458
the bioactive, higher Cprotein-D was more effective.
459
In order to get a systematic understanding of β-carotene degradation in these gel
460
systems, degradation kinetics was calculated (Table 4). It was found that β-carotene in
461
the gels containing higher Cprotein-D had smaller k and bigger t1/2 values during light
462
stability and thermal stability test. For example, when the emulsion gel had a Cprotein-D
463
of 4.5% and a Cprotein-N of 0.5% (A1), β-carotene had a k value of 77.4×10-4 h-1, and a t1/2
464
value of 8.95 h during the light stability test; the k value was 2.56×10-4h-1, and the t1/2
465
value was 270.70 h when the gels was stored at 55 °C. The emulsion gels with higher
19
466
Cprotein-D had better protection effect on the embedded ingredient, and the degradation
467
rates were slower. It was also found that the increase in Cprotein-N could reduce the k
468
value of β-carotene in the emulsion gels and enhance its protective effect. The
469
calculation clearly indicated that the increase in Cprotein-D was more effective in slowing
470
the degradation of β-carotene than the increase in Cprotein-N, suggesting that the gel
471
structures provided more protection for β-carotene than the interface.
472
4. Conclusion
473
The present work studied the influence of the content of native protein and denatured
474
protein in the structure and functionality of emulsion gels. With strong self-assembling
475
properties of the denatured protein molecules at pH close to its isoelectric point, the
476
changes in Cprotein-D greatly affected mechanical, water adsorption and holding
477
capacities. Consequently, the gels with higher Cprotein-D retained more β-carotene during
478
stability tests. The native protein also took part in the development of the gel network
479
and the protection for β-carotene, though it played relatively weaker roles. The study
480
revealed the strong influences of the gel structures on the functionality of the emulsion
481
gels, and appropriate structural designs in the gel matrix and at the interface could bring
482
in flexible delivery of bioactives incorporated in the systems. The knowledge obtained
483
in this study would provide novel information for the development of delivery systems
484
for functional food.
485
486
Acknowledgments
487
This research was funded by National Natural Science Foundation of China (No.
488
31701648).
489
20
490
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24
Table 1. Composition of emulsions/emulsion gels with different content of native protein and denatured protein.
Group
A
B
Sample codes
Cprotein-D
Cprotein-N
(w/w)
(w/w)
A1
4.5%
0.5%
A2
4%
1%
A3
3.5%
1.5%
B1
4%
0.5%
B2
4%
1%
B3
4%
1.5%
*A2 and B2 were the same sample. For the ease of understanding, different codes were used.
25
Table 2. Droplet characteristics of emulsions with different content of native protein and
denatured protein. Samples
Size
PDI
Zeta potential (mV)
A1
393.75±7.71
a
0.24±0.05
-43.32±2.56a
A2/B2
326.88±4.23b
0.23±0.04
-51.02±1.88b
A3
276.33±7.19c
0.19±0.07
-56.62±1.30c
B1
400.20±8.51a
-46.90±0.90d
B3
283.47±6.22c
0.24±0.07 0.18±0.01
-46.23±0.21d
Values with different lowercase letters in the same column indicate a significant difference among the values of p < 0.05. A2 and B2 were the same sample. For the ease of understanding, different codes were used.
26
Table 3. Texture properties of emulsion gels with different content of native protein and denatured protein.
Samples
Fracture stress (MPa)
Fracture strain
a
0.52±0.04
Young's modulus (MPa)
a
9.00±0.41a
A1
3.53±0.17
A2/B2
3.06±0.14b
0.47±0.04ab
8.83±0.20a
A3
2.99±0.07c
0.45±0.02b
8.11±0.31b
B1
2.99±0.06c
0.45±0.02b
8.52±0.25c
B3
3.10±0.22b
0.48±0.04ab
9.00±0.41a
Values with different lowercase letters in the same column indicated a significant difference (p < 0.05). A2 and B2 were the same sample. For the ease of understanding, different codes were used.
27
Table 4. Degradation rate constant (k), half-life time (t1/2), regression coefficient of first-order kinetic model (R2) for β-carotene in emulsion gels at different storage conditions. R2
t1/2 (h)
k (10-4h-1) Samples UV-light
25 °C
55 °C
UV-light
25 °C
55 °C
UV-light
25 °C
55 °C
A1
77.41±0.29a
1.85±0.36a
2.56±0.35a
8.95
374.59
270.70
0.8198
0.8865
0.9307
A2/B2
91.83±0.23b
1.85±0.13a
2.71±0.05a
7.55
374.59
255.72
0.9183
0.9793
0.9987
A3
105.60±0.34c
2.24±0.11b
3.21±0.20b
6.56
309.38
215.89
0.8644
0.9913
0.9844
B1
115.82±0.33d
2.05±0.22b
3.23±0.15b
5.98
338.05
214.55
0.8911
0.9547
0.9909
B3
73.21±0.25e
1.47±0.16c
2.64±0.22a
9.47
471.43
262.5
0.8526
0.9511
0.9729
Values with different lowercase letters in the same column indicated a significant difference (p < 0.05). A2 and B2 were the same sample. For the ease of understanding, different codes were used.
28
Figure 1
A
40 A1
Viscosity (mPa.s)
35
A2
30
A3
25 20 15 10 5 0 0
100
200 Shear rate (s-1)
300
B 40
B1
35 Viscosity (mPa.s)
400
B2
30
B3 25 20 15 10 5 0 0
100
200 Shear rate (s-1)
300
400
Fig. 1. Viscosity of the emulsions with different content of native protein and denatured protein (A: fixed total protein content; B: fixed denatured protein content). A2 and B2 were the same sample. For the ease of understanding, different codes were used.
29
Figure 2
A
0.50
Instability index
0.40
0.30
0.20
0.10
0.00
B
A1
A2
A3
B1
B2
B3
0.50
Instability index
0.40
0.30
0.20
0.10
0.00
Fig. 2. Instability index of emulsions with different content of native protein and denatured protein (A: fixed total protein content; B: fixed denatured protein content). A2 and B2 were the same sample. For the ease of understanding, different codes were used.
30
Figure 3
A 100000
G', G'' (Pa)
10000
1000
100 A1,G' A1,G'' A2, G' A2, G'' A3, G' A3, G''
10
1 0
2000
4000 Time (s)
6000
8000
B 100000
G', G'' (Pa)
10000
1000
100 B1,G' B1,G'' B2, G'
10
B2, G'' B3, G' B3, G''
1 0
2000
4000 Time (s)
6000
8000
Fig. 3. Gelation dynamics of the emulsion gels with different content of native protein and denatured protein (A: fixed total protein content; B: fixed denatured protein content). A2 and B2 were the same sample. For the ease of understanding, different codes were used.
31
Figure 4 B1
A1
A2/B2
A3
B3
Fig.4. Microstructures of emulsion gels with different content of native protein and denatured protein. A2 and B2 were the same sample. For the ease of understanding, different codes were used.
32
Figure 5
A
6
Swelling ratio (%)
5 4 3 2 1 0 A1
A2
A3
B1
B2
B3
B6
Swelling ratio (%)
5 4 3 2 1 0
C A1
A2
A3
B1
B2
B3
Fig.5. Swelling properties of emulsion gels with different content of native protein and denatured protein. (A: fixed total protein content; B: fixed denatured protein content; C morphology of the samples after swelling test). A2 and B2 were the same sample. For the ease of understanding, different codes were used.
33
Figure 6
A 100
a
b
c
A1
A2
A3
c
b
B1
B2
80
WHC (%)
60
40
20
0
B 100
a
80
WHC (%)
60
40
20
0 B3
Fig.6. Water holding capacity (WHC) of emulsion gels with different content of native protein and denatured protein (A: fixed total protein content; B: fixed denatured protein content). A2 and B2 were the same sample. For the ease of understanding, different codes were used.
34
Figure 7
A
B
Fig. 7. The retention ratios of β-carotene in emulsions gels with different content of native protein and denatured protein when exposed to light (A: fixed total protein content; B: fixed denatured protein content). A2 and B2 were the same sample. For the ease of understanding, different codes were used.
35
Figure 8
A
B
C
D
Fig. 8. The retention ratios of β-carotene in emulsions gels with different content of native protein and denatured protein when stored at 25 and 55 °C (A&B: fixed total protein content; C&D: fixed denatured protein content). A2 and B2 were the same sample. For the ease of understanding, different codes were used.
36
Emulsion gels were prepared with both denatured protein and native protein. Emulsion properties were mostly affected by the content of native protein. The denatured protein played a leading role in the gelation process and structures of the emulsion gels. Both proteins were responsible for the stability of β-carotene.
We declare that we have no conflict of interest.
Author statement
The work presented in this paper has not been published previously, that it is not under consideration for publication elsewhere, that its publication is approved by all authors and tacitly or explicitly by the responsible authorities where the work was carried out, and that, if accepted, it will not be published elsewhere in the same form, in English or in any other language, including electronically without the written consent of the copyright-holder.