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Article
Physicochemical and Functional Properties of 2S, 7S, and 11S
Enriched Hemp Seed Protein Fractions
Comfort F. Ajibola and Rotimi E. Aluko *
Department of Food and Human Nutritional Sciences, University of Manitoba, Winnipeg, MB R3T 2N2, Canada;
cfajibola06@gmail.com
* Correspondence: rotimi.aluko@umanitoba.ca
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Citation: Ajibola, C.F.; Aluko, R.E.
Physicochemical and Functional
Abstract: The hemp seed contains protein fractions that could serve as useful ingredients for food
product development. However, utilization of hemp seed protein fractions in the food industry can
only be successful if there is sufficient information on their levels and functional properties. Therefore,
this work provides a comparative evaluation of the structural and functional properties of hemp seed
protein isolate (HPI) and fractions that contain 2S, 7S, or 11S proteins. HPI and protein fractions were
isolated at pH values of least solubility. Results showed that the dominant protein was 11S, with a
yield of 72.70 ± 2.30%, while 7S and 2S had values of 1.29 ± 0.11% and 3.92 ± 0.15%, respectively.
The 2S contained significantly (p < 0.05) higher contents of sulfhydryl groups at 3.69 µmol/g when
compared to 7S (1.51 µmol/g), 11S (1.55 µmol/g), and HPI (1.97 µmol/g). The in vitro protein
digestibility of the 2S (72.54 ± 0.52%) was significantly (p < 0.05) lower than those of the other isolated
proteins. The intrinsic fluorescence showed that the 11S had a more rigid structure at pH 3.0, which
was lost at higher pH values. We conclude that the 2S fraction has superior solubility, foaming
capacity, and emulsifying activity when compared to the 7S, 11S, and HPI.
Keywords: hemp seed; globulins; albumin; amino acid composition; intrinsic fluorescence; circular
dichroism; functional properties; protein digestibility
Properties of 2S, 7S, and 11S Enriched
Hemp Seed Protein Fractions.
Molecules 2022, 27, 1059. https://
doi.org/10.3390/molecules27031059
Academic Editors: Francesco Bonomi,
Stefania Iametti and
Pasquale Ferranti
Received: 29 December 2021
Accepted: 2 February 2022
Published: 4 February 2022
Publisher’s Note: MDPI stays neutral
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Copyright: © 2022 by the authors.
Licensee MDPI, Basel, Switzerland.
This article is an open access article
distributed under the terms and
conditions of the Creative Commons
Attribution (CC BY) license (https://
creativecommons.org/licenses/by/
4.0/).
1. Introduction
The global demand for food proteins continues to grow and is expected to generate
an estimated $76.48 billion in revenue by 2027 [1]. The reasons for increased demand for
food-derived proteins have been associated with their nutritional and techno-functional
properties and health benefits [2]. Thus, food proteins have become prominent ingredients
in the food industry. Recently, there has been a growing interest in hemp seed proteins
due to their high nutritional properties such as high digestibility and contents of sulfurcontaining amino acids and arginine [3–6]. The main storage protein in hemp seed is edestin
(globulins), which accounts for 60–80% of the total protein, while albumins constitute
approximately 25% [7]. Currently, the available hemp seed proteins in the market are
mainly defatted flours and protein concentrates, which are produced from cold-pressed
seeds to remove the oil. Although hemp seed protein flours and concentrates have been
successfully incorporated into a variety of products such as protein shakes, hemp milk,
energy bars, and defatted meals, their use as ingredients in food applications is still limited
due to poor functional properties [3,4,8].
Previous works have studied the potential use of hemp seed proteins as functional
ingredients in food formulation. For example, Tang et al. [9] examined the functional
properties of hemp seed protein isolate (86.9% protein content) obtained from defatted
meal using alkaline solubilization followed by isoelectric precipitation at pH 5.0. With the
exception of methionine and cysteine, the protein isolate contained levels of essential amino
acids that satisfy human nutrition requirements. The effect of limited enzymatic hydrolysis
on the functional properties of hemp seed protein was carried out by Yin et al. [10]. Malomo
Molecules 2022, 27, 1059. https://doi.org/10.3390/molecules27031059
https://www.mdpi.com/journal/molecules
�Molecules 2022, 27, 1059
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and Aluko [11] compared the functional properties of a protein concentrate obtained by
membrane ultrafiltration (after the digestion of the defatted meal using carbohydrase
and phytase to remove non-protein materials) with those of a protein isolate obtained by
isoelectric precipitation. A comparative study of the structural and functional properties
of hemp seed albumin and globulin protein fractions was carried out by Malomo and
Aluko [12]. Wang et al. [13] studied the physicochemical and nutritional properties of
hemp seed 11S (legumin), which had an isoelectric point at pH 6.4 when compared to the
7S (Vicilin) with least solubility at pH 4.6. The 7S was limited in contents of methionine
and cysteine in contrast to the 11S, which contained sufficient amounts of all the essential
amino acids. Dapcevic-Hadnadev et al. [3] recently reported the effect of protein isolation
method on the emulsifying properties of hemp seed proteins. However, to the best of our
knowledge, information is scant on the comparative structural and functional properties
of a hemp seed fractions enriched in 11S, 7S, and 2S proteins. The present work presents
new information on the physicochemical and functional properties of HPI, 11S, 7S, and
2S hemp seed proteins, which could promote their use as ingredients to formulate novel
food products. Hence, the aim of this study was to determine the structural and functional
properties of hemp seed extracts enriched with 11S, 7S, and 2S proteins in comparison to
the protein isolate.
2. Results
2.1. Proximate Composition
The proximate compositions of HPI, 11S, 7S, and 2S are shown in Table 1. The moisture
content was significantly higher in the 2S protein fraction, which could have contributed to
the reduced fat level when compared to HPI, 11S, and 7S. The HPI and 11S had significantly
higher crude protein content, which indicates greater protein purity when compared to the
2S and 7S protein fractions. Fat content was highest in the 11S followed by the 7S, while the
lowest level was present in the 2S fraction. The 11S had the significantly lowest ash content,
which indicates the presence of lower amounts of mineral compounds when compared to
the HPI, 2S, and 7S proteins. In general, all the proteins had very low (<1.5%) fiber contents
and the 2S was almost devoid of this non-nutrient polysaccharide.
Table 1. Proximate composition of hemp seed protein isolate (HPI) and fractions (2S, 7S, 11S).
Sample
Moisture (%)
Protein (%)
Fat (%)
Ash (%)
Fibre (%)
HPI
11S
7S
2S
4.11 ± 0.01 d
4.84 ± 0.03 c
5.18 ± 0.06 b
8.45 ± 0.03 a
87.14 ± 0.08 a
87.23 ± 0.04 a
57.70 ± 0.19 c
66.34 ± 0.01 b
2.14 ± 0.01 c
6.46 ± 0.06 a
5.33 ± 0.42 b
0.67 ± 0.09 d
8.63 ± 0.01 a
1.50 ± 0.17 c
8.66 ± 0.04 a
6.31 ± 0.06 b
0.11 ± 0.13 b
1.12 ± 0.47 a
1.04 ± 0.12 a
0.01 ± 0.01 c
Each value is the mean and standard deviation of duplicate determinations. Within the same column, mean
values with different letters are significantly different (p < 0.05).
2.2. Yield, Digestibility, Sulfhydryl Group, and Bound Carbohydrate
Table 2 shows that the 11S globulin is the predominant protein in hemp seed, accounting for approx. 73% of the total proteins while the 7S and 2S can be considered as
minor proteins. In the present study, a combination of proteases was used to simulate
the gastrointestinal enzymatic process that occurs in the normal human digestion of food
proteins. Results show that the 2S protein had significantly lower digestibility than the HPI,
11S, and 7S proteins (Table 2). HPI and 11S had similar protein digestibility, though higher
than that of 7S. However, the 2S protein had significantly higher levels of exposed and total
sulfhydryl groups when compared to the HPI, 11S, and 7S. The 11S had the lowest number
of exposed sulfhydryl groups as well as bound carbohydrates, but the 2S and 7S contained
similar contents of bound carbohydrates, which were higher than that of the HPI.
�Molecules 2022, 27, 1059
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Table 2. Yield, in vitro protein digestibility (IVPD), sulfhydryl groups (SH), and bound carbohydrates
(CHO) of hemp seed protein isolate (HPI) and fractions (2S, 7S, 11S).
Sample
Protein Yield
(%)
IVPD
(%)
Exposed SH
(µmol/g)
Total SH
(µmol/g)
CHO
(%)
HPI
11S
7S
2S
82.72 ± 4.36 a
72.70 ± 2.30 b
1.29 ± 0.11 d
3.92 ± 0.15 c
88.10 ± 0.26 a
88.28 ± 0.17 a
84.48 ± 0.30 b
72.54 ± 0.52 c
1.16 ± 0.02 c
0.57 ± 0.04 d
1.32 ± 0.07 b
2.39 ± 0.14 a
1.97 ± 0.07 b
1.55 ± 0.22 c
1.51 ± 0.12 c
3.69 ± 0.05 a
5.16 ± 0.95 b
2.07 ± 0.09 c
10.36 ± 0.53 a
10.05 ± 0.49 c
Each value is the mean and standard deviation of duplicate determinations. Within the same column, mean
values with different letters are significantly different (p < 0.05).
2.3. Amino Acid Composition
Table 3 shows that the amino composition of the 2S protein (albumins) differs from those
of 7S, 11S, and HPI (mainly globulins). The 2S had lower contents of aspartic + asparagine
(Asx), phenylalanine, tyrosine, and branched-chain amino acids (valine, leucine, isoleucine)
but higher contents of glutamic + glutamine (Glx) and cysteine. Except for a slightly higher
level of sulfur-containing amino acids (SCAAs), the amino acid composition of the 11S was
similar to that of the HPI. The 11S and HPI also had higher levels of Arg/Lys ratios when
compared to the 2S and 7S protein fractions. The total level of aromatic amino acids (AAA),
hydrophobic amino acids (HAA), and essential amino acids (EAA) were lower in the 2S
than the 7S, 11S, and HPI. With the exception of threonine, histidine, and lysine, the 2S had
essential amino acid levels that do not satisfy the minimum requirement for children. In
contrast, the 11S and HPI were deficient only in lysine, while the 7S had levels of essential
amino acids that meet the FAO-suggested levels for children.
2.4. Gel Electrophoresis (SDS-PAGE)
The SDS-PAGE profiles of the polypeptide components of HPI, 11S, 7S, and 2S in
the presence (reduced) and absence (non-reduced) of mercaptoethanol are presented in
Figure 1A,B, respectively. The 2S profile under non-reduced conditions had five major
polypeptides that are <30 kDa while the 7S, 11S, and HPI consisted of additional polypeptides with up to 150 kDa in size. The 7S profile under non-reduced conditions confirmed
the presence of four major polypeptides (150, 100, 49, and 15 kDa). The non-reduced 11S
and HPI had a similar five polypeptide bands with a basic subunit (18 to 20 kDa) and an
acidic subunit (30 to 40 kDa) and other polypeptides showing MW values of 47, 80, 120,
and 160 kDa. The similarity of the polypeptide composition of 11S and HPI is consistent
with the dominant role of 11S as the major (approx. 73%) hemp seed protein (Table 2).
Moreover, the 7S, 11S, and HPI all contained polymeric proteins that could not enter the gel
(PP) under non-reduced conditions (Figure 1B), which indicates protein aggregation and a
hydrophobic character. In contrast, the 2S did not contain the polymeric aggregates (PP)
and is an indication of a hydrophilic protein. Under the reduced condition, the 2S fraction
had two major polypeptides (20 and 25 kDa) along with three minor bands, which present
a different pattern when compared to the non-reducing condition and is an indication of
the presence of disulfide bonds in the native protein. Similarly, the polypeptide profiles
of 7S, 11S, and HPI under reduced conditions were different from those of non-reducing
conditions, which also confirm the presence of disulfide bonds in the native forms of these
proteins. The protein aggregates (PP) observed for 7S, 11S, and HPI under non-reduced
conditions disappeared under reduced conditions, which indicate conversion into smaller
monomeric polypeptides after the disruption of the disulfide bonds.
�Molecules 2022, 27, x FOR PEER REVIEW
Molecules 2022, 27, 1059
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4 of 19
SCAA
7.05
4.77
4.04
2.93
2.5
EAA
26.56
35.19
33.13
33.89
32.8
BCAA
9.08
14.91
15.16
16.58
Arg/Lys
ratio amino
1.96acid composition
1.67
Table
3. Percent
of3.94
hemp seed4.04
protein isolate (HPI) and fractions (2S, 7S, and 11S).
Asx = aspartic acid + asparagine; Glx = glutamic acid + glutamine; AAA = aromatic amino acids;
BCAA
= branched-chain
amino acids;
amino acids;FAO-/WHO-Suggested
NCAA = negatively
Amino
Acids
2S
7S HAA = hydrophobic
11S
HPI
(2–5amino
Years)
charged amino acids; PCAA = positively charged amino acids; SCAA =Requirements
sulfur-containing
acids; EAA
Asx= essential amino
7.50 acids.9.15
11.04
11.60
Thr
4.14
3.79
3.44
3.49
3.4
5.04
5.61
5.36
2.4. Gel Ser
Electrophoresis5.01
(SDS-PAGE)
Glx
25.63
20.95
18.44
18.13
The SDS-PAGE profiles of the polypeptide components of HPI, 11S, 7S, and 2S in the
Pro
3.93
3.87
3.74
3.64
presence
(reduced) and
(non-reduced)
are presented in FigGly
5.75absence
4.17
4.06 of mercaptoethanol
4.18
ure 1A,B,
respectively.
The
2S
profile
under
non-reduced
conditions
had five major polyAla
5.86
5.46
5.18
5.19
Cys
1.56
1.22
peptides
that are <30 4.88
kDa while2.24
the 7S, 11S,
and HPI consisted
of additional polypeptides
3.07
5.32
with upVal
to 150 kDa in
size. The4.87
7S profile4.74
under non-reduced
conditions3.5
confirmed the
Met
2.17
2.53
2.48
1.71
presence of four major polypeptides (150, 100, 49, and 15 kDa). The non-reduced 11S and
Ile
1.99
3.70
3.81
4.36
2.8
HPI had a similar five polypeptide bands with a basic subunit (18 to 20 kDa) and an acidic
Leu
4.02
6.34
6.61
6.90
6.6
subunitTyr
(30 to 40 kDa)2.46
and other3.14
polypeptides
MW values of 47, 80, 120, and 160
3.70 showing
3.53
kDa. The
the polypeptide
composition
of4.78
11S and HPI is consistent with the
Phesimilarity of1.43
3.67
4.49
Hisrole of 11S 3.20
3.14(approx.
2.93
2.91
1.92). Moreover,
dominant
as the major
73%) hemp
seed protein (Table
6.45 polymeric
3.44 proteins
3.28
5.8 the gel (PP)
the 7S, Lys
11S, and HPI6.36
all contained
that could not enter
Arg
12.45
10.79
13.55
13.24 protein aggregation and a hyunder non-reduced
conditions
(Figure 1B),
which indicates
Trp
0.18
0.70
1.19
1.14
1.1
drophobic
character.30.86
In contrast,
the 2S did
not contain
the polymeric aggregates (PP) and
HAA
38.45
40.00
40.80
is an indication
of a hydrophilic
protein. Under
2S fraction had
AAA
4.07
7.51
9.38 the reduced
9.45 condition, the6.3
two major
polypeptides
25 kDa) 29.04
along with 29.73
three minor bands, which present a
NCAA
33.13(20 and
30.1
PCAA
22.01
20.38to the non-reducing
19.92
19.43
different
pattern when
compared
condition and is an indication of
SCAA of disulfide
7.05 bonds4.77
4.04 protein.2.93
2.5
the presence
in the native
Similarly, the polypeptide
profiles
EAA
26.56
35.19
33.13
33.89
32.8
of 7S, 11S, and HPI under reduced conditions were different from those of non-reducing
BCAA
9.08
14.91
15.16
16.58
conditions, which also confirm the presence of disulfide bonds in the native forms of these
Arg/LysThe
ratio
1.67
3.94 for 7S,
4.04
proteins.
protein1.96
aggregates
(PP) observed
11S, and HPI under non-reduced
Asx
=
aspartic
acid
+
asparagine;
Glx
=
glutamic
acid
+
glutamine;
AAA
= aromatic into
amino
acids;
conditions disappeared under reduced conditions, which indicate
conversion
smaller
BCAA = branched-chain amino acids; HAA = hydrophobic amino acids; NCAA = negatively charged amino acids;
monomeric
polypeptides
after
the
disruption
of the disulfide
bonds.
PCAA
= positively
charged amino
acids;
SCAA
= sulfur-containing
amino acids;
EAA = essential amino acids.
(A)
(B)
Figure 1.
1. SDS-PAGE
SDS-PAGEof
ofhemp
hempseed
seedprotein
proteinisolate
isolate(HPI)
(HPI)and
andfractions
fractions
(2S,
and
11S)
under
reducFigure
(2S,
7S,7S,
and
11S)
under
reducing
ing (A) and non-reducing (B) conditions.
(A) and non-reducing (B) conditions.
2.5. Intrinsic Fluorescence Emission
The fluorescence intensity (FI) of the hemp seed proteins was maximal (λmax) at
338–344 nm at all the pH values (Figure 2). At pH 3.0, the 11S fraction exhibited a more
�Molecules 2022, 27, 1059
5 of 19
compact structure, which is reflected in the higher FI when compared to the 2S, 7S, and
HPI. At pH 5.0 and 7.0, the 11S and HPI assumed disorganized structures, which increased
interactions with the hydrophilic environment, as evident in their low FI values (indicative
of fluorescence quenching), while there was a slight increase at pH 9.0. In contrast, the
2S
Molecules 2022, 27, x FOR PEER REVIEW
5 of 19
and 7S had less compact structures (lower FI) at pH 3.0 but were significantly enhanced
(higher FI) at pH 5.0, 7.0, and 9.0.
2.5.Secondary
Intrinsic Fluorescence
2.6.
and Tertiary Emission
Structure Conformations
Theeffect
fluorescence
intensity
(FI) of thestructure
hemp seed
proteins wasof
maximal
(λmax)
at 338The
of pH on
the secondary
conformations
hemp seed
proteins
are
in ellipticity
3) and
of eacha structural
344shown
nm at as
all changes
the pH values
(Figurevalues
2). At (Figure
pH 3.0, the
11Sproportions
fraction exhibited
more comtype
4). At
pH 3.0,
the 2S had
a secondary
structure
dominated
by
pact(Table
structure,
which
is reflected
in the
higher FI when
compared
to themostly
2S, 7S,(80%)
and HPI.
the
(Table
is also evident
in the intense
ellipticity
At α-helix
pH 5.0 conformation
and 7.0, the 11S
and 2),
HPIasassumed
disorganized
structures,
which between
increased
200
and 220 nm
3) when compared
to 7S,
11S, and
increased,
interactions
with(Figure
the hydrophilic
environment,
as evident
inHPI.
theirAs
lowthe
FI pH
values
(indicathe
most of the
α-helix conformation
by high at
levels
of the
β-sheet
tive2Soflost
fluorescence
quenching),
while there accompanied
was a slight increase
pH 9.0.
In contrast,
and
conformations.
contrast,(lower
the secondary
of 7S,
11S, and HPI
the unordered
2S and 7S had
less compactIn
structures
FI) at pHstructure
3.0 but were
significantly
enproteins
was dominated
β-sheet
hanced (higher
FI) at pHmainly
5.0, 7.0,by
and
9.0. and unordered conformations at all the pH
values (Table 2).
Figure 2. Intrinsic fluorescence intensity of hemp seed protein isolate (HPI) and fractions (2S, 7S, and 11S).
Figure 2. Intrinsic fluorescence intensity of hemp seed protein isolate (HPI) and fractions (2S, 7S,
and The
11S). pH-dependent tertiary structure conformations of the hemp seed proteins, as
analyzed by near-UV CD spectroscopy, are shown in Figure 4. At pH 3.0, the 2S and 7S had
Secondary
andtertiary
Tertiarystructure
Structure (increased
Conformations
a2.6.
more
organized
ellipticity between 260 and 290 nm) when
compared
to 11Sofand
Atsecondary
pH 5.0, there
was a slight
increase in
compactness
of the
The effect
pHHPI.
on the
structure
conformations
of the
hemp
seed proteins
are
2S
protein,
as evident
the increased
the 7S lost
significant
parttype
of
shown
as changes
in in
ellipticity
valuesellipticity,
(Figure 3)whereas
and proportions
of aeach
structural
the
compact
and2S
hence
reduced structure
ellipticity dominated
values when
compared
pH
(Table
4). Atstructure
pH 3.0, the
had had
a secondary
mostly
(80%)toby
the3.0.
αAt
pH
7.0,
there
was
a
significant
increase
in
the
ellipticity
values
of
HPI,
which
reflects
a
helix conformation (Table 2), as is also evident in the intense ellipticity between 200 and
more
compact
structure
when
compared
to
2S,
7S,
and
11S.
220 nm (Figure 3) when compared to 7S, 11S, and HPI. As the pH increased, the 2S lost
most of the α-helix conformation accompanied by high levels of the β-sheet and unordered conformations. In contrast, the secondary structure of 7S, 11S, and HPI proteins was
dominated mainly by β-sheet and unordered conformations at all the pH values (Table 2).
�Molecules 2022, 27, x FOR PEER REVIEW
6 of 19
Molecules 2022, 27, 1059
6 of 19
Figure 3. Far-UV spectra of hemp seed protein isolate (HPI) and fractions (2S, 7S, and 11S) at different
Figure
3. Far-UV spectra of hemp seed protein isolate (HPI) and fractions (2S, 7S, and 11S) at differpH values.
ent pH values.
Table 4. Circular dichroism-derived protein secondary structure composition of hemp seed protein
isolate
(HPI) anddichroism-derived
fractions (2S, 7S, andprotein
11S) at different
pHstructure
values. composition of hemp seed protein
Table
4. Circular
secondary
isolate (HPI) and fractions (2S, 7S, and 11S) at different pH values.
pH
Samples
α-Helix (%)
pH
Samples
2S
7S
2S
11S
7S
HPI
11S
2S
HPI
7S
2S
11S
HPI
7S
11S
2S
7S
HPI
11S
2S
HPI
7S
2S
11S
7S
HPI
11S
HPI
2S
7S
11S
HPI
α-Helix
(%)1.53 ±
Unordered
(%)
80.40
± 0.00(%) 0.70β-Sheet
±0.00 (%)5.95 ±β-Turns
0.01
0.03
4.40
±
0.00
31.18
±
0.00
17.30
±
0.00
46.66
±
0.00
80.40 ± 0.00
0.70 ±0.00
5.95 ± 0.01
1.53 ± 0.03
3.10 ± 0.01
37.45 ± 0.02
17.45 ± 0.01
43.65 ± 0.00
4.40 ± 0.00
31.18 ± 0.00
17.30 ± 0.00
46.66 ± 0.00
2.20 ± 0.01
43.45 ± 0.03
19.45 ± 0.01
34.95 ± 0.00
pH 3
pH 3
pH 5
pH 5
pH 7
pH 7
pH 9
pH 9
3.10 ± 0.01
β-Sheet (%)
β-Turns (%)
37.45 ± 0.02
Unordered (%)
17.45 ± 0.01
43.65 ± 0.00
18.60 ± 0.00
3.90 ± 0.01
12.50 ± 0.03
65.05 ± 0.04
2.20 ± 0.01 39.5043.45
± 0.0320.35 ±19.45
± 0.0139.05 ± 34.95
± 0.00
1.40 ± 0.00
± 0.00
0.00
0.00
18.60
± 0.00 43.253.90
± 0.01 21.30 ±12.50
1.55
± 0.00
± 0.02
0.01 ± 0.03
35.50 ± 65.05
0.00 ± 0.04
1.85
± 0.00
± 0.01
0.00 ± 0.00
36.35 ± 39.05
0.01 ± 0.00
1.40
± 0.00 41.5039.50
± 0.0020.30 ±20.35
1.55
± 0.00
1.35
± 0.01
2.20
±
0.00
1.85 ± 0.00
3.45 ± 0.00
1.35 ± 0.01
17.40 ± 0.01
± 0.0217.55 ±21.30
37.5543.25
± 0.02
0.00 ± 0.01
47.05 ± 35.50
0.01 ± 0.00
40.8041.50
± 0.02
19.05
±
0.03
38.85
±
0.03 ± 0.01
± 0.01
20.30 ± 0.00
36.35
44.25 ± 0.00
20.30 ± 0.00
32.20 ± 0.00
37.55 ± 0.02
17.55 ± 0.00
47.05 ± 0.01
26.05 ± 0.01
20.20 ± 0.04
36.15 ± 0.04
4.55 ± 0.02
3.45 ± 0.00
3.30 ± 0.00
17.40
± 0.01
0.00
± 0.00
0.00
± 0.00
4.55
± 0.02
34.30 ± 0.00
17.30 ± 0.00
46.90 ± 0.00
44.25 ± 0.0017.05 ±20.30
± 0.0046.60 ± 32.20
± 0.00
37.10 ± 0.00
0.00
0.00
± 0.0123.60 ±20.20
55.4526.05
± 0.02
0.01 ± 0.04
24.15 ± 36.15
0.00 ± 0.04
45.9534.30
± 0.01
0.00 ± 0.00
39.99 ± 46.90
0.03 ± 0.00
± 0.0013.70 ±17.30
2.20 ± 0.00
3.30 ± 0.00
0.00 ± 0.00
0.00 ± 0.00
40.80 ± 0.02
19.05 ± 0.03
38.85 ± 0.03
37.10 ± 0.00
55.45 ± 0.02
45.95 ± 0.01
17.05 ± 0.00
23.60 ± 0.01
13.70 ± 0.00
46.60 ± 0.00
24.15 ± 0.00
39.99 ± 0.03
The pH-dependent tertiary structure conformations of the hemp seed proteins, as
analyzed by near-UV CD spectroscopy, are shown in Figure 4. At pH 3.0, the 2S and 7S
had a more organized tertiary structure (increased ellipticity between 260 and 290 nm)
when compared to 11S and HPI. At pH 5.0, there was a slight increase in the compactness
of the 2S protein, as evident in the increased ellipticity, whereas the 7S lost a significant
�Molecules 2022, 27, x FOR PEER REVIEW
Molecules 2022, 27, 1059
7 of 19
part of the compact structure and hence had reduced ellipticity values when compared to
pH 3.0. At pH 7.0, there was a significant increase in the ellipticity values of HPI, which
7 of 19
reflects a more compact structure when compared to 2S, 7S, and 11S.
Figure 4. Near-UV spectra of hemp seed protein isolate (HPI) and fractions (2S, 7S, and 11S) at
Figure 4.pH
Near-UV
different
values.spectra of hemp seed protein isolate (HPI) and fractions (2S, 7S, and 11S) at different pH values.
2.7. Protein Solubility Profiles
2.7. Protein
Profiles
Figure Solubility
5 shows the
pH-dependent solubility of 11S, 7S, 2S, and HPI. The results indi-
Protein solubility (%)
Figure
shows
pH-dependent
solubility
of in
11S,
7S, 2S,
HPI. The
results
indicate that
HPI5 and
11Sthe
had
similar solubility
profiles
which
theand
proteins
have
moderate
(30–60%)
at pH
whichsolubility
decreasedprofiles
significantly
(p <the
0.05)
at pH 5.0–9.0.
The PS
cate that solubility
HPI and 11S
had3.0,
similar
in which
proteins
have moderate
profile
of 7S
shows that
the 3.0,
protein
is fairly
soluble
at pH 3.0 and
characterized
(30–60%)
solubility
at pH
which
decreased
significantly
(p <4.0,
0.05)
at pH 5.0–9.0.
The
Molecules 2022, 27, x FOR PEER REVIEW
8by
of min19
imal
solubility
point,
and higher
pH4.0,
5.0–9.0.
The 2S fracPS profile
of 7Saround
showsthe
thatisoelectric
the protein
is fairly
solublesolubility
at pH 3.0atand
characterized
by
tion
was highly
soluble
overthe
a wide
pH range,
at pH 5.0–9.0.
minimal
solubility
around
isoelectric
point,with
and values
higher reaching
solubility97–99%
at pH 5.0–9.0.
The 2S
fraction was highly soluble over a wide pH range, with values reaching 97–99% at pH 5.0–
9.0. 1 10
1 00
90
80
70
60
50
40
30
20
10
0
2
3
4
2S
5
6
pH
7S
7
8
11S
9
10
HPI
Figure 5. pH-dependent changes in the solubility of hemp seed protein isolate (HPI) and fractions
Figure 5. pH-dependent changes in the solubility of hemp seed protein isolate (HPI) and fractions
(2S,
and
11S).
(2S, 7S,7S,
and
11S).
2.8. Water Holding Capacity (WHC), Oil Holding Capacity (OHC), and Least Gelation Concentration
The WHC of HPI was significantly (p < 0.05) higher than the values obtained for 7S
and 11S (Table 5). The WHC of 2S was not reported due to complete solubility in water.
�Molecules 2022, 27, 1059
8 of 19
2.8. Water Holding Capacity (WHC), Oil Holding Capacity (OHC), and Least Gelation Concentration
The WHC of HPI was significantly (p < 0.05) higher than the values obtained for 7S
and 11S (Table 5). The WHC of 2S was not reported due to complete solubility in water.
The OHC is the ability of non-polar side chains of protein to interact with aliphatic chains
of oil/fat and is usually expressed as the amount of fat/oil that can be absorbed per gram
of protein. The 2S and HPI had similar OHCs, which were significantly higher (p < 0.05)
than the values obtained for 7S and 11S. The LGC results show that the 7S has a higher
ability to form a gel, hence a smaller amount of the protein is required when compared to
2S, 11S, and HPI (Table 5).
Table 5. Water holding capacity (WHC), oil holding capacity (OHC), and least gelation concentration
(LGC) of hemp seed protein isolate (HPI) and fractions (2S, 7S, and 11S) *.
Sample
WHC (g/g)
OHC (g/g)
LGC (%)
HPI
11S
7S
2S
5.81 ± 0.01 a
10.32 ± 0.01 a
3.63 ± 0.03 c
5.97 ± 0.08 b
4.09 ± 0.21 b
4.93 ± 0.51 b
11.04 ± 0.01 a
22.00 ± 0.00 c
30.00 ± 0.00 d
10.00 ± 0.00 a
14.00 ± 0.00 b
* For each column, values with different letters are significantly different (p < 0.05).
2.9. Foaming Capacity (FC) and Foam Stability (FS) of Hemp Seed Proteins
The FCs of hemp seed proteins at different pH values indicate that the 2S fraction
produced significantly (p < 0.05) larger volumes of foam than those of 7S, 11S, and HPI at
all the pH values (Table 6). In general, the FCs of HPI, 11S, and 7S were minimal at pH
5.0, which is within the pH 4.5–5.0 isoelectric point range for the proteins. In contrast, the
2S had high FC in the acidic pH 3.0 and 5.0 with a slight reduction at pH 7.0. Figure 6
shows that the 2S has lower FS when compared to the 7S, 11S, and HPI, especially at pH 3.0
and 5.0. Generally, all the proteins produced stable foams (85% stability) over the 30 min
measurement duration.
Table 6. Foaming capacity of hemp seed protein isolate (HPI) and fractions (2S, 7S, and 11S) *.
Sample
pH 3.0 (%)
pH 5.0 (%)
pH 7.0 (%)
HPI
11S
7S
2S
75.00 ± 7.07 c
55.00 ± 7.07 c
60.00 ± 0.00 d
60.00 ± 0.00 b
95.00 ± 7.07 b
195.00 ± 7.07 a
60.00 ± 0.00 b
185.00 ± 7.07 a
75.00 ± 7.07 c
90.00 ± 0.00 b
60.00 ± 0.00 d
150.00 ± 0.00 a
* For each column, values with different letters are significantly different (p < 0.05).
2.10. Emulsion Formation (Oil Droplet Size) and Stability
The emulsifying capacities of 2S, 7S, 11S, and HPI were analyzed by measuring the
mean oil droplet size (d3,2 ) of emulsions formed by these proteins at different pH values.
The 2S fraction consistently formed smaller oil droplets when compared to the 7S, 11S, and
HPI proteins at all pH values (Table 7). The results show that the 2S protein has better
emulsifying properties (smaller oil droplet sizes) when compared to 7S, 11S, and HPI,
which formed bigger oil droplet sizes. At pH 3.0 and 5.0, the 11S had a better emulsifying
capacity (smaller d3,2 values) when compared to 7S and HPI, whereas at pH 7.0, the 7S was
better. The emulsions formed with 2S, 7S, and 11S proteins exhibited better stability at all
pH values when compared to those formed with HPI (Figure 7).
�Molecules 2022, 27, 1059
11S
60.00 ± 0.00 d
60.00 ± 0.00 b
90.00 ± 0.00 b
b
b
7S
95.00 ± 7.07
60.00 ± 0.00
60.00 ± 0.00 d
a
a
2S
195.00 ± 7.07
185.00 ± 7.07
150.00 ± 0.00 a9 of 19
* For each column, values with different letters are significantly different (p < 0.05).
Figure 6. Foam stability of hemp seed protein isolate (HPI) and fractions (2S, 7S, and 11S) at different
Figure 6. Foam stability of hemp seed protein isolate (HPI) and fractions (2S, 7S, and 11S) at different
pH
values.Bars
Barswith
withdifferent
differentletters
lettershave
havesignificantly
significantlydifferent
differentvalues
values(p
(p<<0.05).
0.05).
pH values.
Table 7. Oil droplet sizes (d3,2 ) of emulsions formed with hemp seed protein isolate (HPI) and
fractions (2S, 7S, and 11S) *.
2.10. Emulsion Formation (Oil Droplet Size) and Stability
The emulsifying capacities of 2S, 7S, 11S, and HPI were analyzed by measuring the
3.0 (µm) formed by pH
5.0 proteins
(µm)
pH 7.0
(µm)
emulsions
these
at different
pH
values.
mean oilSample
droplet size (d3,2) ofpH
a
d
The 2S fraction
consistently
formed
smaller
oil
droplets
when
compared
to
the
7S,
HPI
6.23 ± 0.36
4.90 ± 0.07 c 11S,
12.65 ± 0.88
a
b
d
and HPI proteins
at
all
pH
values
(Table
7).
The
results
show
that
the
2S
protein
11S
6.06 ± 0.43
5.50 ± 0.13
5.66 ± has
0.27 better
Molecules 2022, 27, x FOR PEER REVIEW
10bof 19
c
a
7S
7.62
±
0.14
6.79
±
0.22
± 0.23
emulsifying properties (smaller oil droplet sizes) when compared to 7S,4.45
11S,
and HPI,
a
b
2S bigger oil droplet
4.19 sizes.
± 0.17At
2.25 emulsifying
± 0.01 a
4.29
± the
0.2011S
which formed
pH 3.0 and
5.0,
had a better
* For each (smaller
column, values
with different
are significantly
different
< 0.05). at pH 7.0, the 7S was
capacity
d3,2 values)
whenletters
compared
to 7S and
HPI,(pwhereas
better. The emulsions formed with 2S, 7S, and 11S proteins exhibited better stability at all
pH values when compared to those formed with HPI (Figure 7).
Table 7. Oil droplet sizes (d3,2) of emulsions formed with hemp seed protein isolate (HPI) and fractions (2S, 7S, and 11S) *.
Sample
pH 3.0 (µm)
pH 5.0 (µm)
pH 7.0 (µm)
HPI
12.65 ± 0.88 d
6.23 ± 0.36 a
4.90 ± 0.07 c
11S
5.50 ± 0.13 b
6.06 ± 0.43 a
5.66 ± 0.27 d
6.79 ± 0.22 a
4.45 ± 0.23 b
7S
7.62 ± 0.14 c
2S
4.19 ± 0.17 a
4.29 ± 0.20 b
2.25 ± 0.01 a
* For each column, values with different letters are significantly different (p < 0.05).
Figure 7. Emulsion stability of hemp seed protein isolate (HPI) and fractions (2S, 7S, and 11S) at
Figure 7. Emulsion stability of hemp seed protein isolate (HPI) and fractions (2S, 7S, and 11S) at
differentpH
pHvalues.
values.Bars
Barswith
withdifferent
differentletters
lettershave
havesignificantly
significantlydifferent
differentvalues
values(p(p<<0.05).
0.05).
different
3. Discussion
3. Discussion
Knowledge of the physicochemical properties of food proteins is very important
Knowledge
of the physicochemical
properties
foodmay
proteins
is very
important inin
in providing
a mechanistic
understanding
of howofthey
function
as ingredients
providing
a
mechanistic
understanding
of
how
they
may
function
as
ingredients
food
food product formulations. In this work, we have provided new informationinon
the
product
formulations.
In
this
work,
we
have
provided
new
information
on
the
chemical
chemical composition and structural properties of hemp seed protein fractions as a means
composition and structural properties of hemp seed protein fractions as a means of enhancing their utilization as food ingredients. The higher moisture content of the 2S, when
compared to other fractions (Table 1), could be associated with the lower fat, which favors
interactions with water molecules. The presence of attached carbohydrate molecules may
�Molecules 2022, 27, 1059
10 of 19
of enhancing their utilization as food ingredients. The higher moisture content of the 2S,
when compared to other fractions (Table 1), could be associated with the lower fat, which
favors interactions with water molecules. The presence of attached carbohydrate molecules
may have also enhanced the interactions with water molecules, as evident in the higher
moisture content of 2S and 7S proteins, both of which have higher carbohydrate contents
when compared to HPI and 11S (Table 2). The 87% protein content obtained for HPI is
the same as the value reported by Tang et al. [9]. Wang et al. [13] had reported 90% and
93% protein contents for HPI and 11S, which are slightly higher than the 87% obtained in
the present study. In contrast, the ~58% protein content of the 7S is lower than the ~88%
reported by Wang et al. [13], which may be due to differences in the raw materials used for
the protein extraction. The lower protein contents observed in 7S and 2S may be due to
the presence of higher levels of attached carbohydrate molecules (Table 2) when compared
to the 11S and HPI proteins. The results are consistent with previous works that have
reported that the 2S [14,15] and 7S [16] proteins of different legume seeds are glycoproteins
with covalently bound carbohydrate moieties. The 11S had the lowest ash content, which
suggests the presence of lower amounts of mineral compounds when compared to the HPI,
2S, and 7S proteins. The ash contents of the HPI and 7S are higher than the <0.4% values
reported by Wang et al. [13].
Table 2 shows that the 11S globulin is the predominant protein in hemp seed, accounting for approx. 73% of the total proteins while the 7S and 2S can be considered as minor
proteins. This is in contrast to some legume seeds where the 7S is more abundant than the
11S [17,18]. Using a similar isoelectric protein precipitation method, Tang et al. [9] reported
approx. 73% while Hadnadev et al. [4] and Shen et al. [6] obtained ~51% and ~47% protein
yields, respectively, for HPI, which are lower than the ~83% obtained in the current work.
The higher HPI yield obtained in this work may be due to the lab-scale defatting at room
temperature, which would have produced a meal with reduced protein denaturation when
compared to the 40 ◦ C meal used by Tang et al. [9]. The effect of raw material quality is
further demonstrated by the approx. 38% HPI yield reported by Malomo et al. [8], which
was produced from a meal obtained by mechanical press-defatted hemp seed meal.
In the present study, in vitro protein digestibility was determined to estimate susceptibility to gastrointestinal proteases and hence amino acid bioavailability during dietary
consumption. The 2S had lower digestibility, which could be associated with its high
content of total sulfhydryl groups (Table 2) when compared to HPI, 11S, and 7S proteins.
The 2S (albumins) contains proteins with a conserved skeleton of cysteine residues, which
form several rigid intermolecular disulfide bonds that enhance stability to proteolytic
attack [19]. House et al. [5] reported protein digestibility that ranged from 83.50 to 97.50%
for hemp products, which are consistent with the values obtained for HPI, 11S, and 7S in
this work. HPI and 11S had similar protein digestibility, though higher than that of 7S,
which is consistent with the work of Wang et al. [13].
The 2S had the highest level of SCAAs (Table 3), which suggests a potentially better
antioxidative effect than 7S, 11S, and HPI because of the suggested role of the sulfhydryl
group in enhanced iron-reducing and hydrogen peroxide scavenging [20]. The levels of
SCAAs obtained in this work are higher than the values reported by Wang et al. [13], which
may be attributed to differences in the source of the defatted meal used for protein extraction. HPI and 11S had arginine/lysine ratios of 4.0 and 3.9, respectively, which are higher
than those of 7S (1.7) and 2S (1.9). A high ratio has been reported to have a beneficial effect
in lowering blood cholesterol and thereby contributing to overall cardiovascular health [21].
Therefore, the HPI and 11S may have better cardiovascular health benefits than the 2S and
7S proteins. The arginine/lysine ratios obtained in this work are consistent with the 1.74
and 4.37 reported for hemp seed albumin and globulin, respectively [12]. The HPI, 11S,
and 7S (globulins) have higher contents of branched-chain amino acids (BCAAs) than the
2S (albumin), which has implications for human health. This is because BCAAs are part of
indispensable amino acids and play remarkable metabolic and regulatory roles since about
40% of the total protein required by mammals and 35% of muscle protein essential amino
�Molecules 2022, 27, 1059
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acids are BCAAs [22]. BCAAs enhance protein synthesis, improve metabolic processes,
improve immune functions, reduce oxidative stress, and improve gut health [23], which
further emphasizes the higher nutritional value of HPI, 11S, and 7S when compared to the
2S. The total amount of essential amino acids (EAA) in HPI, 11S, and 7S are similar to the
~33% level suggested by the FAO/WHO for children’s health maintenance. In contrast, the
2S content of EAA is slightly below the minimum recommended level.
The polypeptide composition, as shown in Figure 1A,B, indicates similarities between
11S and HPI. The 49 kDa polypeptide in the present study is similar to the 47 kDa reported
for the 7S of hemp protein by Wang et al. [13]. A previous work has also shown similar HPI
polypeptides as obtained in this work under reducing and non-reducing conditions [4].
The lack of polymeric forms (PP) of the 2S could be due to the presence of a high number
of sulfhydryl groups (Table 2), which enhances the greater formation of disulfide bonds
and confers a more rigid structure to make the protein more resistant to protein–protein
interactions when compared to the 7S, 11S, and HPI proteins.
The intrinsic fluorescence properties of a protein are determined by the location of its
aromatic amino acid residues [24]. The 338–344 nm λmax obtained in this work is similar
to the 344 and 340 nm reported for the 7S and 11S of soybean proteins [25]. The higher FI
of the 11S protein at pH 3.0 indicates a more hydrophilic surface, which led to the packing
of aromatic residues into the interior while the opposite was the case with the other protein
fractions. However, at higher pH values, the presence of greater numbers of attached
carbohydrate residues may have enhanced the surface hydrophilic properties of the 2S and
7S proteins, which influenced structural rearrangements that moved the aromatic residues
into the non-polar interior, hence giving a higher FI when compared to the 11S and HPI.
The intrinsic fluorescence data obtained for 11S and HPI in this study are in agreement
with those reported for HPI by Malomo et al. [8], who observed the quenching of the FI of
HPI at pH 5.0 and an increase in the FI at both acidic and alkaline pH values.
The far-UV data for 7S, 11S, and HPI show pH-dependent variations in secondary
conformation, which are in agreement with the work of Choi and Ma [26], who reported
that buckwheat globulins possess higher contents of β-sheet strands than α-helix at pH
3–11. This is important because high levels of β-sheet strands have been reported to be
directly related to the ability of the protein to make strong gels [27]. The actual shape
and magnitude of the near-UV spectrum of a protein in the region of 250 nm to 320 nm
depend on the number of each type of aromatic amino acid residues, their mobility, and
the nature of their environment, as well as their spatial disposition in the protein [28]. At
pH 3.0, the more organized tertiary structure of 2S and 7S may be due to the presence of
attached carbohydrates, which are not ionized and hence have fewer repulsions within
the proteins. In contrast, the lack of a defined tertiary structure (almost zero ellipticity) for
the 11S and HPI could indicate the presence of charged groups within the protein, hence
strong protein–protein repulsions. At pH 7.0, the HPI had higher ellipticity values, which
reflect increased interactions of the protein surface with the hydrophilic environment and
the movement of the aromatic groups into the inner core of the protein when compared to
the 2S, 7S, and 11S with looser structures. The 11S and HPI also had significant increases
in a compact tertiary conformation at pH 9.0, which reflects increased protein surface
interactions with the hydrophilic environment. An increase in negative charges as the pH
moves towards alkaline pH would produce a more hydrophilic environment, which favors
structural rearrangements that relocate aromatic residues into hydrophobic environments
away from the protein surface.
The similar solubility profile of the HPI and 11S is consistent with their comparable
polypeptide profiles and amino acid composition, which further confirms that the major
proteins in hemp seed are the 11S globulins. The low solubility of 11S and HPI could
be attributed to the high contents of hydrophobic amino acids, which enhance protein–
protein interactions and result in protein aggregation and weak interactions with the water
environment. The results are consistent with the detection of protein aggregates under
non-reducing gel electrophoresis (Figure 1B), as well as previous reports that showed that
�Molecules 2022, 27, 1059
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hemp seed proteins exhibited poor solubility [8,9]. However, Hadnadev et al. [4] and
Shen et al. [6] reported higher HPI solubility values than obtained in this work, which
may be due to differences in the source of the defatted meal used for the protein isolate
preparation. Moreover, the HPI used in this work was prepared through precipitation
at pH 4.2, which may have led to greater protein aggregation (reduced solubility) than
the pH 5.0 used in previous reports [4,6]. The improved solubility of 7S at alkaline pH
may be associated with its smaller polypeptide sizes and the high content of attached
carbohydrate residues, which could enhance net charge density. These structural features
of the 7S protein will increase flexibility and interactions with the water environment when
compared to the 11S and HPI proteins with bigger polypeptides and smaller numbers of
attached carbohydrate residues. The high solubility of the 2S fraction over a wide pH range
is consistent with previous reports for albumin fractions of other plant proteins [12,29].
The presence of a high level of attached carbohydrate residues (Table 2), the low molecular
weight of polypeptides (Figure 1), and the low level of hydrophobic amino acids coupled
with high levels of positively and negatively charged amino acids (Table 3) may have
contributed to the high solubility of the 2S protein. It has also been shown that the exposure
of the SH group could enhance protein interactions with water [15,30]. Hence, the higher
content of exposed SH (Table 2) in the 2S could have contributed to the observed superior
protein solubility when compared to the 7S, 11S, and HPI.
The higher WHC of HPI suggests a higher degree of protein aggregation (enhances
trapping of water molecules) than the 7S and 11S proteins, as previously reported for
aggregated soybean proteins [31]. Ajibola et al. [14] also obtained no value for the albumin
fraction of African yam bean protein because of its complete solubility in water, a result
that is similar to the 2S in the present work. This is consistent with a previous report stating
that proteins with high solubility exhibit minimal WHC [32]. The OHC obtained for HPI
in this study is comparable to the 13.7 g/g value reported by Malomo et al. [8] but higher
than the 5.27 g/g reported by Tang et al. [9] for hemp seed protein isolate. The OHC of
a protein has been reported to be a function of several parameters, such as the physical
entrapment of oil, protein surface area, size, charge, and hydrophobicity [14]. The high
OHC of HPI and 2S suggest potential use in the food industry for the formulation of meat
substitutes, ground meat, baked goods, extenders, and soups.
A protein’s ability to form gels is traditionally measured by the LGC, which may be
defined as the lowest protein concentration required to form a self-supporting gel that does
not slide along the test tube walls in the inverted position [33]. The ability of the 7S and
2S to form gels at lower protein concentrations of 10 and 14% (w/v), respectively, could
be associated with their higher solubility, smaller polypeptide sizes, increased structural
flexibility, and a high percentage of attached carbohydrate residues [34]. In contrast, the
poor gelling ability of 11S and HPI may be due to their poor solubility, which limits the
ability of the proteins to unfold and form the required network. The results are consistent
with a recent work, which showed that increased levels of the 7S pea protein (low 11S/7S
ratio) produced gels at lower protein concentrations than the extract with a high 11S/7S
ratio [18]. Therefore, the presence of 7S in the HPI could be responsible for the better gelling
property when compared to the 11S. Likewise, the better gelling ability of the 2S may have
been due to higher contents of sulfur groups, which have been shown to contribute to the
formation of strong gels that are stabilized by disulfide bonds [27].
The most crucial requirement for foam formation during whipping is the ability of
a surfactant to rapidly reduce the free energy (interfacial tension) and form a continuous
and highly viscous film at foam interfaces [35]. The higher FC of the 2S fraction (albumin),
when compared to the globulins (7S, 11S, and HPI), is consistent with previous reports
for soy proteins [35] and African yam bean albumin [14]. The better FC observed in the
2S fraction might be due to its smaller polypeptides, flexibility, and high solubility index,
when compared to the more globular and larger 7S, 11S, and HPI proteins. It has been
reported that the higher the hydrophobicity of a protein fraction, the more stable the film
that forms at the air/water interface [35]. Therefore, the high hydrophobic amino acid
�Molecules 2022, 27, 1059
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contents of 7S, 11S, and HPI (Table 3) may have improved protein–protein interactions to
form strong interfacial membranes that reduced the coalescence rate of air bubbles (higher
FS) better than the more hydrophilic 2S.
The results of the emulsion oil droplet size are in agreement with Tay et al. [35],
who showed that the 2S fraction of soybean protein exhibited better emulsifying capacity
when compared to 7S and 11S. The high emulsifying properties observed in 2S could be
attributed to its smaller polypeptide sizes, which may have enabled rapid or more efficient
rearrangement at the oil and water interface when compared to the larger 7S, 11S, and HPI
polypeptides. The higher level of sulfhydryl groups could have also contributed through
increased disulfide bonding to form strong interfacial membranes that enhanced oil droplet
encapsulation. This is supported by a previous work, which showed that electrochemical
modification of a soybean protein isolate led to an increased number of sulfhydryl groups
and better emulsion formation ability [36]. Wang et al. [37] also reported that a soybean
protein isolate with a higher level of free sulfhydryl groups formed smaller emulsions than
the avocado protein. Since the 2S has a lower content of hydrophobic amino acids than
7S, 11S, and HPI, the results obtained in this work contrast with those previously reported
for Camellia oleifera proteins, where protein hydrophobicity was a strong contributor to
the emulsion-forming ability [38]. The better emulsifying capacity observed for the 7S
protein at pH 7.0 indicates the increased ability of the protein to unfold and encapsulate oil
droplet particles in a neutral environment. On the other hand, the 11S fraction has a higher
ability at acidic pH values to unfold and encapsulate oil droplets. The results are consistent
with the higher protein solubility of 11S at pH 3.0, which could have enhanced protein
unfolding and encapsulation of the oil droplets when compared to HPI and 7S with lower
solubility values. The better stability of emulsions formed at pH 3.0 and 5.0 with 2S and 7S
proteins indicates the greater ability of the proteins to form stronger interfacial membranes
that reduced oil droplet coalescence better than the 11S and HPI. The presence of higher
numbers of exposed sulfhydryl groups in 2S and 7S proteins may also have enabled the
formation of proteins with more disulfide bonds and, hence, stronger interfacial membrane
integrity than those formed by the 11S and HPI.
4. Materials and Methods
4.1. Materials
Hemp seed hearts (dehulled) were purchased from Manitoba Harvest Fresh Hemp
Foods Ltd. (Winnipeg, MB, Canada) and stored at −20 ◦ C. Other analytical-grade chemicals
and reagents were procured from Fisher Scientific (Oakville, ON, Canada) or Sigma Aldrich
(Sigma Chemicals, St. Louis, MO, USA).
4.2. Preparation of Defatted Hemp Seed Flour (DHF)
Hemp seed flour was obtained by grinding the hemp seed hearts in a laboratory
blender, which was followed by defatting using acetone extraction at 1:10 (w/v) for 1 h at
room temperature [39]. The mixture was allowed to settle, after which the acetone was
decanted. The defatting process was repeated once, after which the residual flour was
air-dried in a fume hood at room temperature (23 ◦ C) for 16 h. The resultant defatted meal
was milled using a laboratory blender to obtain DHF, which was stored at −20 ◦ C.
4.3. Preparation of Hemp Seed Protein Isolate (HPI)
HPI was produced from the DHF as described by Tang et al. [9], with slight modifications. The DHF was dispersed in deionized water (1:20, w/v), adjusted to pH 10.0 using
2 M NaOH, and mixed at 37 ◦ C for 2 h; the mixture was then centrifuged (7000× g; 30 min,
4 ◦ C). The supernatant was collected, adjusted to pH 4.2 with 2 M HCl to precipitate the
proteins, and thereafter centrifuged (7000× g; 60 min; 4 ◦ C). The resultant precipitate was
washed with water, adjusted to pH 7.0 with 2 M NaOH, freeze-dried to obtain the HPI, and
stored at −20 ◦ C.
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4.4. Preparation of 11S, 7S, and 2S Protein-Enriched Fractions
Fractions rich in 11S, 7S, and 2S proteins were prepared according to the protocols
developed by Wang et al. [13]. DHF (100 g) was dispersed in distilled water (1:20, w/v) and
adjusted to pH 10.0 with 2 M NaOH to solubilize the proteins at 37 ◦ C for 2 h, followed
by centrifugation (7000× g; 30 min; 4 ◦ C) to obtain supernatant A. Then, NaHSO3 was
added (0.98 g/L) to supernatant A, adjusted to pH 6.4 with 1 M HCl (to precipitate the 11S
fraction), and kept overnight at 4 ◦ C. The resultant dispersion was centrifuged (7000× g;
30 min; 4 ◦ C) and the supernatant (B) saved while the precipitate (A) was adjusted to pH
7.0 with 2 M NaOH followed by dialysis against water for 3 days at 4 ◦ C (3 water changes
daily) using a 6–8 kDa molecular weight cut-off membrane. After dialysis, the precipitate
A was freeze-dried as the 11S protein. The saved supernatant B was further adjusted to
pH 4.6 with 2 M HCl (to precipitate the 7S fraction) and thereafter centrifuged (6500× g;
20 min; 4 ◦ C) to obtain precipitate B and supernatant C. Precipitate B was adjusted to pH
7.0 with 2 M NaOH, and then dialyzed, as above, followed by freeze-drying to obtain the
7S protein. Supernatant C was also dialyzed, as above, and freeze-dried as the 2S protein.
The dried 2S, 7S, and 11S enriched protein fractions were stored at −20 ◦ C.
4.5. Proximate and Amino Acid Composition Analysis
The moisture, crude protein, and ash were analyzed using the relevant AOAC [40]
methods. The fat and fiber contents were determined using AOCS methods [41]. The
protein-bound carbohydrate content was determined as described by Mundi and Aluko [15],
while the amino acid profiles were determined using previously described methods [42].
4.6. Determination of In Vitro Protein Digestibility
The in vitro digestibility of the proteins was determined according to the method of
Hsu et al. [43], with slight modifications, using an enzyme system consisting of trypsin and
chymotrypsin. A 10 mL aliquot of aqueous protein suspension (6.25 mg protein/mL) in
double-distilled water was adjusted to pH 8.0 with 0.1 M NaOH while stirring at 37 ◦ C.
The enzyme solution (containing 1.6 mg/mL trypsin and 3.1 mg/mL chymotrypsin) was
maintained in an ice bath and 1 mL of the solution was added to the protein suspension.
The pH drop was recorded over a 10 min period and the protein digestibility of each protein
sample was calculated as follows:
Protein digestibility (%) = 210.46 − 18.10Xf
(1)
where Xf is the final pH value of each sample after a 10 min digestion.
4.7. Sodium Dodecyl Sulfate-Polyacrylamide Gel Electrophoresis (SDS-PAGE)
SDS-PAGE was performed according to the method of Ijarotimi et al. [42] using 8–25%
gradient gel for polypeptide separation and development on a Phastsystem Separation
and Development unit according to the manufacturer’s instructions (GE Health Sciences,
Montréal, QC, Canada).
4.8. Total and Exposed Sulfhydryl Contents
Sulfhydryl and total cysteine contents were determined, as fully described [15]. The
sulfhydryl concentration (total and exposed) in µmol/g of protein was calculated by using
the extinction coefficient of 2-nitro-5-thiobenzoate at 412 nm (13,600 mol L−1 cm−1 ):
µmol SH/g protein = 73.53A × D/C
(2)
where A = the absorbance at 412 nm; C = the sample concentration in mg solids/mL;
D = dilution factor; and 73.53 is derived from 106 /(1.36 × 104 ). The molar absorptivity is
1.36 × 104 and 106 is for conversions from the molar basis to the µM/mL basis and from
mg solids to g solids.
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4.9. Intrinsic Fluorescence Emission
The method described by Ijarotimi et al. [42] was used to record intrinsic fluorescence
spectra on the FP-6300 spectrofluorimeter (Jasco Corp., Tokyo, Japan) at 25 ◦ C with a
1 cm path length cuvette. Protein stock solution (10 mg/mL) was prepared in 0.1 M
sodium phosphate buffer (pH 3.0, 5.0, 7.0, and 9.0), followed by centrifugation and the
determination of the protein content of the supernatant. The supernatant was then diluted
to 0.002% (w/v) and fluorescence spectra were recorded at an excitation wavelength of
275 nm (tyrosine and tryptophan) with emission recorded from 280 to 450 nm. The emission
of the buffer was subtracted from that of the respective samples to obtain the reported
fluorescence intensity (FI) spectra.
4.10. Measurements of Circular Dichroism (CD) Spectra
Far and near-UV CD spectra were measured as previously described by Ijarotimi et al. [42],
using a J-815 spectropolarimeter (Jasco Corp., Tokyo, Japan) at 25 ◦ C. Briefly, protein stock
solution (10 mg/mL) was prepared in 0.1 M sodium phosphate buffer (pH 3.0, 5.0, 7.0,
and 9.0), followed by centrifugation and the determination of the protein content of the
supernatant. The stock solutions were each diluted to 2 and 4.0 mg/mL for far-UV and
near-UV CD spectra measurement at 190–240 nm (0.5 mm quartz cell path length) and
250–320 nm (1 mm quartz cell path length), respectively. All the CD spectra were obtained
as the average of three consecutive scans with the automatic subtraction of the respective
buffer spectra. Secondary structure fractions were calculated from the far-UV data using
the SELCON3 (optimized for 190–240 nm) secondary structure determination algorithm, as
previously described [42].
4.11. Protein Solubility (PS)
PS was determined according to the method described by Ajibola et al. [14]. Briefly,
1 mg/mL protein dispersions were prepared in 0.1 M phosphate buffers, pH 3.0–9.0. The
dispersions were vortexed for 2 min and then centrifuged (7000× g; 30 min; 25 ◦ C). Protein
contents in the supernatants were determined using the modified Lowry method [44]
with bovine serum albumin as the standard. PS was expressed as a percentage ratio of
supernatant protein content to the total protein content.
4.12. Water (WHC) and Oil (OHC) Holding Capacity
The WHC and OHC were determined using the method of Mundi and Aluko [15],
with some modifications. The protein sample (3 g) was dispersed in 25 mL distilled water
(or pure canola oil) in a 50 mL pre-weighed centrifuge tube. The dispersions were vortexed
for 1 min, allowed to stand for 30 min, and then centrifuged (7000× g; 30 min; 25 ◦ C). The
supernatant was decanted, excess water (or oil) in the upper phase was drained for 15 min,
and the tube containing the protein residue was weighed again to determine the amount of
water or oil retained per gram of sample.
4.13. Least Gelation Concentration
The least gelation concentration was determined as previously described [45], by
suspending the protein samples in water at different concentrations. The mixtures were
vortexed, placed in a water bath at 95 ◦ C for 1 h, cooled under tap water, and left in the
refrigerator (4 ◦ C) for 14 h. The sample concentration at which the gel did not slip when
the tube was inverted was taken as the LGC.
4.14. Foaming Capacity (FC)
Foams were formed as previously described [45], using 60 mg/mL samples prepared
in 5 mL of 0.01 M phosphate buffer pH 3.0, 5.0, 7.0, and 9.0, followed by homogenization
at 20,000 rpm for 1 min using a 20 mm generator on the Polytron PT 3100 homogenizer
(Kinematica AG, Lucerne, Switzerland). The foam was formed in a 50 mL graduated
centrifuge tube, which enabled the determination of the foam volume (mL). The volume of
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foam remaining after standing for 30 min at room temperature was expressed as a percent
value of the original foam volume to obtain the foam stability (FS).
4.15. Emulsion Formation and Oil Droplet Size Measurement
The oil-in-water emulsions were prepared and determined according to the method
of Aluko et al. [45]. Briefly, protein samples at 50 mg/mL concentrations were prepared
in 5 mL of 0.1 M phosphate buffer pH 7.0 followed by the addition of 1 mL of pure
canola oil. The oil/water mixture was homogenized at 20,000 rpm for 1 min, using the
20 mm shaft on a Polytron PT 3100 homogenizer. The mean oil droplet size (d3,2 ) of the
emulsions was determined in a Mastersizer 2000 (Malvern Instruments Ltd., Malvern,
UK) with distilled water as a dispersant. Emulsions were kept at room temperature for
30 min without agitation and the increase in oil droplet size was used to determine the
emulsion stability (ES).
4.16. Statistical Analysis
Duplicate or triplicate determinations were used to obtain mean values and standard
deviations. Statistical analysis was performed with SAS (Statistical Analysis Software
9.1) using one-way ANOVA and significant differences (p < 0.05) were determined using
Duncan’s multiple range test.
5. Conclusions
Hemp seed proteins were fractionated into the major globulins (7S and 11S) and
albumins (2S) enriched fractions, followed by a comparison with the protein isolate (HPI).
The 11S was the major fraction in hemp seed, accounting for almost 73% of the total proteins,
which is responsible for the similarities to HPI with respect to the polypeptide and amino
acid compositions, as well as solubility and in vitro protein digestibility. Gel electrophoresis
showed that the 2S protein had polypeptides of small sizes, which could have favored
better interactions with water, in addition to stronger foaming capacity and emulsifying
activities. Overall, the 2S protein had the best potential as an efficient ingredient that can
be used in the formulation of various food products, such as beverages, emulsions, and
foams. However, the nutritional quality of the 2S is inferior to those of the 7S, 11S, and
HPI. In contrast, the 7S had the highest nutritional quality and provides the best hemp seed
protein choice as an ingredient to produce food gels.
Author Contributions: Conceptualization, R.E.A.; methodology, C.F.A. and R.E.A.; formal analysis,
C.F.A.; investigation, C.F.A.; resources, R.E.A.; data curation, C.F.A. and R.E.A.; writing—original
draft preparation, C.F.A.; writing—review and editing, R.E.A.; visualization, C.F.A. and R.E.A.;
supervision, R.E.A.; project administration, R.E.A.; funding acquisition, R.E.A. All authors have read
and agreed to the published version of the manuscript.
Funding: We acknowledge the support of the Natural Sciences and Engineering Council of Canada
(NSERC), funding reference number RGPIN 2018-06019. Cettere chercheaété financée par le Conseil
de recherchesen sciences naturelles et engénie du Canada (CRSNG), numéro de référence RGPIN
2018-06019.
Institutional Review Board Statement: Not applicable.
Informed Consent Statement: Not applicable.
Data Availability Statement: Data are available from the corresponding author.
Acknowledgments: Authors acknowledge the technical support of Adeola M. Alashi.
Conflicts of Interest: The authors declare no conflict of interest. The funders had no role in the design
of the study; in the collection, analyses, or interpretation of data; in the writing of the manuscript; or
in the decision to publish the results.
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Abbreviations
ANOVA
Analysis of variance
BCAA
Branched-chain amino acids
DHF
Defatted hemp seed flour
EAA
Essential amino acids
HPI
Hemp seed protein isolate
IVPD
In vitro protein digestibility
Sulfhydryl groups SH
SCAA
Sulfur-containing amino acids
AAA
Aromatic amino acids
NCAA
Negatively charged amino acids
PCAA
Positively charged amino acids
HAA
Hydrophobic amino acids
Carbohydrates
CHO
FC
Foaming capacity
FS
Foam stability
ES
Emulsion stability
LGC
Least gelation concentration
WHC
Water holding capacity
OHC
Oil holding capacity
PS
Protein solubility
CD
Circular dichroism
FI
Fluorescence intensity
SDS-PAGE
Sodium dodecyl sulfate-polyacrylamide gel electrophoresis
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