Citation: Binte Abdul Halim, F.N.;

Taheri, A.; Abdol Rahim Yassin, Z.;

Chia, K.F.; Goh, K.K.T.; Goh, S.M.;

Du, J. Effects of Incorporating

Alkaline Hydrogen Peroxide Treated

Sugarcane Fibre on The Physical

Properties and Glycemic Potency of

White Bread. Foods 2023, 12, 1460.

https://doi.org/10.3390/

foods12071460

Received: 8 February 2023

Revised: 24 March 2023

Accepted: 26 March 2023

Published: 29 March 2023

Copyright: © 2023 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://

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4.0/).

foods

Article

Effects of Incorporating Alkaline Hydrogen Peroxide Treated
Sugarcane Fibre on The Physical Properties and Glycemic
Potency of White Bread
Fatin Natasha Binte Abdul Halim 1, Afsaneh Taheri 1 , Zawanah Abdol Rahim Yassin 1, Kai Feng Chia 1,
Kelvin Kim Tha Goh 2 , Suk Meng Goh 1 and Juan Du 1,*

1 Food, Chemical and Biotechnology Cluster, Singapore Institute of Technology, 10 Dover Drive,
Singapore 138683, Singapore

2 School of Food & Advanced Technology, Massey University, Private Bag 11222,
Palmerston North 4410, New Zealand

* Correspondence: du.juan@singaporetech.edu.sg

Abstract: The consumption of dietary fibres can affect glycemic power and control diabetes. Sug-
arcane fibre (SCF) is known as insoluble dietary fibre, the properties of which can be affected by
physical, chemical, and enzymatic treatments. In this study, alkaline hydrogen peroxide (AHP)
treatments were conducted over time (0.5, 1, 3, and 5 h) at 12.6% (w/v) SCF and the effects on the
physicochemical and structural properties of the SCF were evaluated. After making dough and bread
with the SCF, with and without AHP treatments, the glycemic responses of the bread samples were
evaluated. Shorter durations of AHP treatment (0.5 and 1 h) reduced lignin effectively (37.3 and
40.4%, respectively), whereas AHP treatment at 1 and 3 h duration was more effective in increasing
particle sizes (50.9 and 50.1 µm, respectively). The sugar binding capacity, water holding capacity
(from 2.98 to 3.86 g water/g SCF), and oil holding capacity (from 2.47 to 3.66 g oil/g SCF) increased
in all AHP samples. Results from Fourier-transform infrared spectroscopy (FTIR) confirmed the
polymorphism transition of cellulose (cellulose I to cellulose II). The morphology of SCF detected
under scanning electron microscopy (SEM) indicated the conversion of the surface to a more porous,
rough structure due to the AHP treatment. Adding SCF decreased dough extensibility but increased
bread hardness and chewiness. All SCF-incorporated bread samples have reduced glycemic response.
Incorporation of 1, 3, and 5 h AHP-treated SCF was effective in reducing the glycemic potency than
0.5 h AHP-treated SCF, but not significantly different from the untreated SCF. Overall, this study
aims to valorize biomass as AHP is commonly applied to bagasse to produce value-added chemicals
and fuels.

Keywords: alkaline hydrogen peroxide; bread; glycemic potency; in vitro digestion; sugarcane fibre

1. Introduction

Dietary fibres can significantly contribute to physiological processes and maintain
human health. They can lower the incidence of chronic diseases, like type 2 diabetes and
cardiovascular problems. Adding dietary fibres to foods can lower glycemic potency and
contribute to the prevention of diabetes [1]. Since the occurrence of diabetes continues to
increase globally, recent research has attempted to find new ways of preventing diabetes.
Adding dietary fibres to food products, such as white bread, has sparked interest among
researchers and developers in the food industries [2–4]. Fibres are divided into two cate-
gories: soluble and insoluble. Although research has proven the health effects of soluble
fibres to be more pronounced than insoluble fibres, insoluble fibres such as lignocellulosic
materials are more abundant and affordable [5]. Modification of lignocellulosic materials
with diverse methods (enzymatic, physical, and chemical) have the potential to increase its
applications [5].

Foods 2023, 12, 1460. https://doi.org/10.3390/foods12071460 https://www.mdpi.com/journal/foods

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Foods 2023, 12, 1460 2 of 19

Sugarcane is cultivated extensively in Brazil, China, India, and other tropical regions of
the world. In 2017, 1.84 billion tons of sugarcane were produced worldwide [6]. Processing
1 ton of sugarcane can generate approximately 280 kg of sugarcane bagasse. Sugarcane
fibre (SCF) is an insoluble dietary fibre that can be processed from sugarcane bagasse [7].
As a lignocellulosic material, SCF is the major byproduct of sugarcane processing and is
generally regarded as waste material. Finding optimal methods to incorporate SCF into
food products, such as bread, a staple food, can benefit consumers and increase the net
profit of the sugarcane industry [8]. Despite the benefits, adding SCF to bread can cause a
loss in product quality, a decrease in bread loaf volume, inferior sensory characteristics,
and increased hardness and chewiness of bread [3,9]. A study using Alkaline Hydrogen
Peroxide (AHP) treatment was found to enhance such features in SCF-loaded bread [10].

AHP treatment was commonly used to pretreat bagasse to produce value-added
chemicals and fuels [11]. AHP treatments usually involve solubilizing lignin and ex-
posing hydroxyl groups, thereby improving the hydration properties of lignocellulose
compounds [12]. Subjecting SCF to alkaline treatment can significantly affect the morphol-
ogy of SCF as the alkaline environment causes fibres to swell and the cellulose molecules
to detach from each other, thereby disrupting the rigid SCF structure [13]. This results in
higher water absorbing SCF with a more open internal structure, allowing alkali-treated
SCF to hydrate more, resulting in swelled and soft particles [14,15]. A relevant study
by Meng et al. [16] considered the effects of AHP on the physicochemical and structural
properties of buckwheat straw insoluble fibres. The results showed that AHP treatment
caused wrinkled surfaces, due to the disintegration of the lignocellulosic part. Furthermore,
breaking the intermolecular hydrogen bonds of cellulose and hemicelluloses through AHP
treatment enhanced the water holding capacity of fibres. AHP treatment degrades lignin
and does not release chemical wastes into the environment, primarily because hydrogen
peroxide can decompose into oxygen gas and water and is an environmentally friendly
and food-grade reagent. Another advantage of using AHP is that the duration of treatment
is usually short, requires low pressure, and can operate with a low concentration [11,17]
Therefore, AHP SCFs have the potential to be used as functional food ingredients. In a
study done by Sangnark and Noomhorm [18], the water and oil holding capacities of SCF
increased after AHP treatment at 1% hydrogen peroxide for 12 h. However, the incorpo-
ration of AHP SCF into bread caused a decrease in dough expansion, an increase in the
hardness of bread, and a decrease in loaf volume, which reduced product quality [18]. In
comparison, we aim to treat SCF with AHP at a higher concentration and shorter time to
improve scalability, process mass intensity (PMI), and efficiency.

Given the available literature and the knowledge gaps, this study aimed to explore
the physicochemical properties of SCF when treated with 7.7% AHP at different durations
of exposure (0.5, 1, 3, 5 h). Ultimately, the effects of adding SCF were evaluated on the
physical properties and glycemic response of wheat flour-based dough and white bread.

2. Materials and Methods
2.1. Materials and Reagents

Food grade H2O2 (35% dilution, Raw Essentials, Philippines) was purchased from
www.rawessentials.com.sg (accessed on 17 January 2021). Amyloglucosidase (EC 3.2.1.3 from
A. niger, Megazyme, E-AMGDF, Bray, Wicklow, Ireland; 3260 U/Ml) was purchased from
Megazyme. Absolute ethanol, 37% HCl, and glacial acetic acid were purchased from MERCK.
NaOH pellets, 95–97% H2SO4, 99% ethanol, and sodium bicarbonate were purchased from
AIK MOH, SINGAPORE, SINGAPORE. D-(+)-Glucose, sodium dodecyl sulphate, phenol,
pepsin (pepsin EC 3.4.23.1 from porcine gastric mucosa, P7000, Sigma-Aldrich, Burlington,
MA, USA; USP ≥ 250 U/mg), pancreatin (EC 232-468-9 from porcine pancreas, P7545, Sigma-
Aldrich, Saint Louis, MO, USA; USP × 8 specifications), invertase (EC 3.2.1.26 from S. cerevisiae,
I4504, Sigma-Aldrich, Saint Louis, MO, USA; ≥300 U/mg), maleic acid, sodium azide, calcium
chloride dihydrate, sodium acetate, potassium sodium tartrate, and 3,5-dinitrosalicylic acid
were purchased from Sigma Aldrich, Burlington, MA, USA.

www.rawessentials.com.sg


Foods 2023, 12, 1460 3 of 19

2.2. AHP Modification of SCF

AHP modification of SCF was carried out following a method modified from Zhang
et al. [11]. First, 1400 mL 10.5% H2O2 was prepared, and pH was adjusted to 11.5 with 5 M
NaOH. Then, 240 g of SCF was added to the solution and stirred at 4 different durations
(0.5, 1, 3, and 5 h), with manual titration of 5 M NaOH to maintain pH at 11.5. The final
concentration of H2O2 was 7.7% while SCF in H2O2 was 12.6% (w/v). Subsequently, the
solution was neutralized with 6 M HCl until pH reached 7.0, covered, and left overnight.
Samples were transferred into centrifuge tubes and centrifuged at 4000× g for 10 min.
Supernatant and pellet were collected separately. The pellet was rinsed with 2000 mL
of deionized water with stirring in a beaker overnight. Centrifuging and rinsing were
subsequently repeated twice to ensure thorough washing. Samples were collected into
centrifuge tubes and stored at −80 ◦C for 24 h, and subsequent freeze drying (VirTis
Benchtop Pro, SP Scientific, Warminster, PA, USA) at −80 ◦C for at least 72 h under vacuum
condition. The final product of AHP modification at all 4 different durations (0.5, 1, 3, and
5 h) was a white powder with a yield of above 90%. SCF treated for 0.5, 1, 3, and 5 h were
labelled as 0.5 h AHP SCF, 1 h AHP SCF, 3 h AHP SCF, and 5 h AHP SCF, respectively,
while the untreated SCF was labelled as untreated SCF.

Based on the AHP treatment described above, the PMI value was significantly reduced
from 101–200 [18] to 18.4. Details in the PMI calculation are described in Table S1.

2.3. Characterization of SCF
2.3.1. Acid-Insoluble Lignin Content Determination

Acid-insoluble lignin content was determined following a method modified from
Fang et al. [19]. In a 250 mL round-bottomed flask, 1 g of SCF (m0) in 100 mL ethanol was
stirred and heated at 100 ◦C under reflux for 4 h. The mixture was then cooled to 25 ± 2 ◦C.
Cold 15% H2SO4 was slowly added, and the mixture was stirred vigorously for 2 h at
25 ± 2 ◦C. Then, 560 mL of deionized water was added, and the mixture was stirred and
heated at 100 ◦C for 4 h. The mixture was cooled to 25 ± 2 ◦C and subsequently filtered
under vacuum conditions. The residue was collected and washed until neutral pH before
drying in an air oven at 105 ◦C until dried. Mass (m1) of the residue was recorded, and the
procedure was repeated twice [19].

Acid − insoluble Lignin Content(%) =
m1

m0
× 100% (1)

2.3.2. Sugar Binding Capacity (SBC)

SBC was determined following a method modified from Dubey et al. [20]. First, 0.1 g
of SCF was dispersed in 2.5 mL deionized water. Subsequently, 5 mL 0.01 M glucose was
added, and the mixture was subjected to shaking under incubated conditions at 200 rpm
and 37 ◦C for 6 h (SB-12l, Benchmark Scientific, Sayreville, NJ, USA). The mixture was
centrifuged at 2000× g for 15 min, and the supernatant was filtered through a 0.45 µm
filter. Then, 2 mL of filtrate was collected and subsequently analyzed using the phenol-
sulfuric assay. Absorbance of the mixtures was recorded at 490 nm (Cary 60 UV-Vis
Spectrophotometer, Agilent Technologies, Santa Clara, CA, USA) [20]. To quantify the
glucose content of SCF, absorbance values of the samples were compared against a glucose
standard curve.

2.3.3. Water Holding Capacity (WHC) and Oil Holding Capacity (OHC)

The following method is modified from Zhao et al. [21]. First, 1 g of SCF and 20 mL
of deionized water or canola oil were added to a centrifuge tube and mixed thoroughly
using a vortex mixer for 1 min at highest speed. The sample was left to sit for 2 h at
25 ± 2 ◦C. After which, the sample was centrifuged at 3000× g for 30 min at 25 ◦C for WHC
or 1500× g for 10 min at 25 ◦C for OHC. Without disturbing the pellet, the supernatant
was removed using a 3 mL plastic dropper. After the complete removal of excess water or



Foods 2023, 12, 1460 4 of 19

oil, the centrifuge tube containing the sample was weighed. The procedure was repeated
thrice. WHC or OHC of SCF was determined following the equation below:

WHC or OHC =
wet weight − dry weight

dry weight
(2)

2.3.4. Particle Size Measurement

Particle size was determined following a method modified from Feng et al. [22]. First,
0.1 g of SCF in 10 mL of 1% Sodium Dodecyl Sulphate (SDS) solution was homogenized
using IKA Homogenizer (Ultra TURRAX) at 6000 rpm for 2 min [22]. The particle size of
the sample was then determined using parameters listed in Table S2 by Mastersizer 3000
(Malvern Instruments Ltd., HydroMV, Worcestershire, UK) with laser light scattering and
ultrasonication, using the HydroMV dispersion unit. Results obtained were analyzed with
Mastersizer 3000 software using the Mie scattering model.

2.3.5. Fourier Transform Infrared Spectroscopy (FTIR)

A small amount of freeze-dried SCF sample was analyzed using an ATR FT-IR spectropho-
tometer (Agilent Cary 630 FTIR, Agilent Technologies, Santa Clara, CA, USA). The spectrum
wavelength was recorded from 600–4000 cm−1 at a resolution of 4 cm−1 with 64 scans [14].

2.3.6. Scanning Electron Microscope (SEM)

A small amount of freeze-dried SCF sample was scattered onto a conductive adhesive
tape and subsequently coated with platinum for 60 s at a flow rate of 20 mA. The sample
was then viewed in the vacuumed stage in the microscopic chamber of a scanning electron
microscope (JSM IT800, Jeol Asia, Tokyo, Japan) [14].

2.4. Development of Dough and Bread
2.4.1. Hydration of Flour Using DoughLAB

DoughLAB (DoughLAB 2500, Perten Instruments, Stockholm, Sweden) was used
to ensure sufficient volume of water was incorporated into each bread formulation. It
uses a 300 g mixing bowl based on the standard AACC International Approved Methods
54-21.02. [23] method. Two different measurements were conducted, one for 300 g wheat
flour and one for 300 g wheat flour with 15 g of untreated SCF (based on 5% of baker’s
percentage). For each measurement, water was added into the mixing bowl via an automatic
water dripping system, followed by mixing at 30 ± 0.1 ◦C and speed 63 rpm for 20 min,
whereby a maximum torque of 500 ± 25 Farinograph units (FU) indicated optimal dough
development, with Farinograph results indicated in Figure S1. The water absorption values
were recorded, and each analysis was conducted in triplicate.

2.4.2. Bread Making Process

Bread samples were prepared using the straight dough method, AACC International
Method 10-09.01. [24], and the finalized bread formulations, with the respective water
absorption determined in the previous analysis, are shown in Table 1.

Table 1. Formulation of reference and SCF incorporated breads.

Reference SCF

Ingredients Mass (g) w/w (%) Mass (g) w/w (%)

Wheat Flour 300.0 59.6 300.0 56.2
SCF - - 15.0 2.8

Water 193.5 38.5 208.8 39.2
Dry Yeast 3.60 0.7 3.60 0.7

Salt 6.00 1.2 6.00 1.1
Total 503.1 100.0 533.4 100.0



Foods 2023, 12, 1460 5 of 19

Wheat flour was stored in the refrigerator overnight before use to ensure that its
temperature is kept below 10 ◦C before usage. The amount of water was divided into 20%
and 80% parts at 25 ± 2 ◦C and chilled (4 ◦C) conditions, respectively.

Dry yeast was pre-dispersed and hydrated in the 20% room temperature (25 ± 2 ◦C)
portion of water for 10 min before mixing. All dry ingredients were pre-mixed using a
stand mixer (3.3 L Mixer 5, Kitchen Aid, Greenville, OH, USA) with a spiral dough hook at
speed 2 for 1 min before the yeast mixture and chilled water was slowly added in a steady
stream. After the addition of water, mixing was continued at speed 2 for 2 min before
increasing the mixing speed to speed 4 for 9 min. Approximately 20 g of dough was kept
aside after mixing for dough extensibility analysis.

After mixing, 2 portions of dough weighing approximately 195 g each were molded into a
ball, covered in aluminum foil, and left to rest at 25 ± 2 ◦C for 5 min. Dough pieces were placed
in an incubator at 30 ◦C and relative humidity of 85% for 60 min to proof. After 60 min, they
were taken out, knocked, and shaped into loaf pans before undergoing a final proofing at the
same conditions for another 60 min. Finally, loaf pans were baked in an oven (MC28H5015AS,
Samsung, Seoul, South Korea) at 200 ◦C for 30 min. After baking, bread samples were allowed
to rest at ambient temperature (25 ± 2 ◦C) for 2 to 2.5 h before further analysis.

2.5. Characterization of Dough and Bread
2.5.1. Dough Extensibility

The extensibility of dough was measured using the texture analyzer (Stable Micro
Systems, TA.Xtplus Texture Analyzer, Godalming, Surrey, UK) with a Kieffer rig attached [25].
The texture analyzer was first calibrated with a 5 kg load cell before analysis. Immediately
after mixing the ingredients listed in Table 1, the dough was clamped into the oiled Teflon
mold and placed into the refrigerator to set for 30 min before analysis using parameters listed
in Table S3. Subsequently, a thin spatula was used to remove the dough strip from the mold
and carefully place it onto the sample plate. The sample plate was then placed onto the Kieffer
rig, and the measurement was repeated 10 times per formulation. After each analysis, the
software quantifies the resistance to extension and extensibility of the dough sample.

2.5.2. Loaf Specific Volume and Maximum Height of Loaf

Loaf specific volume of the bread samples was measured with the use of a solid
displacement method based on the standard AACC International Method 10-05.01. [26]
(Measurement of Volume by Rapeseed Displacement) with modifications made. In this
analysis, mustard seeds were used in replacement of rapeseed. Mustard seeds were placed
in and levelled in a container, and their volume was measured using a 500 mL graduated
measuring cylinder. The bread sample was weighed before being placed into the same
container, filled, and levelled with mustard seeds. The excess mustard seeds were measured
using a 500 mL graduated measuring cylinder to determine the volume of the bread sample.
The analysis was measured in duplicates, and the specific volume of bread was determined
following the equation below:

Specfic Volume
(

cm3/g
)
=

volume of bread sample
mass of bread sample

(3)

The maximum height of the bread sample was measured using a digital vernier caliper,
measuring from the middle point of the longitudinal side of the bread. The analysis was
done in duplicates per formulation.

2.5.3. Texture Profile Analysis of Bread Crumb

The texture profile of the bread was analyzed using the texture analyzer (TA.Xtplus Tex-
ture Analyzer, Stable Micro Systems, Godalming, Surrey, United Kingdom) with a 36R probe
attached [25]. The texture analyzer was first calibrated with a 5 kg load cell before analysis.
Bread samples were sliced into 25 mm thickness, surface area ranging from 4500–5000 mm2,
and placed onto the stage cross-section flat down for analysis. The texture analyzer then



Foods 2023, 12, 1460 6 of 19

compresses the bread twice to understand how it behaves during chewing. After each analysis,
the software quantifies the hardness and chewiness of the sample, and the test parameters are
listed in Table S4. The analysis was repeated thrice for each bread formulation.

2.5.4. Moisture Analysis and Water Activity of Bread Crumb

The moisture content of bread samples was determined using a halogen moisture
analyzer (HE53, Mettler Toledo, Columbus, OH, USA). Bread samples were sealed in
Ziplock bags and kept in an airtight container at 25 ± 2 ◦C, and moisture content analysis
was conducted the day after baking (Day 1). Approximately 4 g of bread sample was placed
onto the sample pan and analyzed at 105 ◦C under automatic operating conditions. The
analysis was repeated twice for each bread formulation.

The water activity of bread samples was determined using the water activity meter
(Novasina, LabMaster-aw neo, Switzerland) at 25 ◦C. Approximately 1 g of bread sample
was placed into the sample cup and analyzed. The analysis was repeated twice for each
bread formulation.

2.5.5. In Vitro Determination of Glycemic Potency

The glycemic potency of bread samples was determined, with slight modifications,
via in vitro study as described by SRV et al. [27] and Monro et al. [28]. Bread samples were
sliced, sealed in Ziplock bags, and stored at −20 ◦C. Prior to analysis, bread samples were
thawed in ambient conditions (25 ± 2 ◦C) for at least 1 h.

2.5.6. In Vitro Digestion of Bread Samples

First, 5 g of bread, in dry weight based on moisture content, was added to 50 mL of
deionized water and homogenized with an S18N-19G dispersing tool (T18 digital ULTRA-
TURRAX®, IKA®-Werke GmbH & Co.KG, Breisgau, Germany) at 6000 rpm for 2 min in a
250 mL Duran bottle.

The mixture was adjusted to pH 2.5 with 1 M HCl. Subsequently, 2 mL of 10% (w/v)
pepsin dissolved in 0.05 M HCl was added, to stimulate the gastric phase. The mixture
was then subjected to shaking under incubated conditions at 170 rpm and 37 ◦C for 30 min
(SB-12l, Benchmark Scientific, Sayreville, NJ, USA). The mixture was neutralized with 4 mL
1 M sodium bicarbonate and 10 mL 0.1 M sodium maleate buffer (pH 6), to initiate the small
intestinal phase. Then, 500 µL aliquot (T0) of the suspension was transferred into 2 mL
of chilled absolute ethanol and mixed thoroughly using a vortex to stop the enzymatic
reaction. Next, 200 µL amyloglucosidase and 2 mL 5% (w/v) pancreatin dissolved in
0.1 M sodium maleate buffer were added to the neutralized mixture in the Duran bottle.
Following the addition, the volume of the mixture was adjusted to 110 mL with deionized
water. Mixtures were subjected to the same shaking and incubated conditions of 170 rpm
and 37 ◦C, where successive 500 µL aliquots were removed at time points of 10, 20, 30, 40,
60, 120, and 180 min and transferred into 2 mL chilled absolute ethanol. Inactivated aliquots
were kept at 4 ◦C prior to the quantification of glucose release. In vitro digestion of each
bread sample was performed in duplicates, with timed samples removed in duplicates.

2.5.7. Quantification of Glucose Release

The release of reducing sugars during the digestion process was quantified using
the dinitrosalicylic acid (DNS) colorimetric method [27,28]. Inactivated aliquots were
centrifuged at 1000× g at 25 ◦C for 10 min. Then, 500 µL of the supernatant was transferred
to 250 µL of enzyme solution containing 1% (v/v) amyloglucosidase (and 0.05% (w/v)
invertase dissolved in 0.1 M sodium acetate buffer (pH 5.2). The mixture was incubated at
37 ◦C for 15 min (SB-12l, Benchmark Scientific, Sayreville, NJ, USA). Subsequently, 750 µL
of DNS mixture (comprising of a 1:1:5 mixture of 0.5 mg/mL of glucose solution, 4 M
NaOH, and DNS reagent respectively) was added, and the contents were heated in a water
bath at 95 ◦C for 15 min. Samples were cooled in ice water and 4 mL of deionized water
was added and thoroughly mixed. Absorbance of the mixtures was recorded at 530 nm



Foods 2023, 12, 1460 7 of 19

(Cary 60, Agilent Technologies, Santa Clara, CA, USA). To quantify the glucose content of
SCF, absorbance values of the samples were compared against a glucose standard curve.

2.6. Data Analysis for In Vitro Glycemic Potency Determination

The release of glucose through in vitro digestion was quantified via the dinitrosalicylic
acid (DNS) colorimetric method [27,28]. The glucose content of bread samples was derived
from a glucose standard curve (y = 0.0965x + 0.2459) and subsequently used in the calculations
of Glycemic Glucose Equivalent (GGE) values per 100 g of bread. The GGE release curves
were depicted by plotting the GGE values against the in vitro digestion time. Equation (4) was
used for deriving an apparent glucose disposal rate (GD). The GD values were subsequently
used for deriving the GGE disposal per time point (GD × time point = GGE disposal), which
was then plotted against the in vitro digestion time. Subsequently, to account for blood glucose
clearance, the GGE disposal values were subtracted from the GGE release to generate net GGE
values (Net GGE = GGE−GD). To account for the in vivo delay in the onset of the glycemic
response, the in vitro digestion time was extended for an additional 10 min. These values were
then plotted against the net GGE values. The incremental area under the curve (iAUC) was
calculated based on the net GGE curve using the 45 triangle/trapezoid summation method
described by the World Health Organization (WHO) [28], as presented in Table S5. The relative
glycemic potency of bread samples was determined on an equal weight basis of 100 g of bread
in comparison with the iAUC of a white bread reference of known GGE. The glycemic index
(GI) of bread samples was then estimated by comparing the calculated iAUC of bread samples
with the iAUC of reference bread.

Glucose Disposal (GD) = 0.0135x + 0.02232 (4)

where x = GGE released by 100 g of bread at 40 min of in vitro digestion.

GIbread sample =
iAUC of bread sample

iAUC of reference
× GIreference (5)

2.7. Statistical Analysis

Statistical analyses were performed with the one-way analysis of variance (ANOVA)
test using Minitab software (Minitab®19, MiniTab Inc., State College, PA, USA). The means
and standard deviation were compared using Tukey’s honest significance test at 95%
confidence level, where a significant difference is observed when p < 0.05. Analytical values
of experiments are shown as mean ± standard deviation.

3. Results and Discussion

The acid-insoluble lignin content, sugar binding capacity (SBC), and particle size
presented as D(4,3) and D(3,2) of the untreated SCF and AHP-treated SCF samples are listed
in Table 2.

Table 2. Acid-insoluble lignin content, sugar binding capacity (SBC), particle size of untreated SCF
and AHP SCF samples.

Sample Acid-Insoluble Lignin
(%)

SBC
(g/g SCF)

Particle Size (µm)

D(4,3) D(3,2)

Untreated SCF 88.7 ± 0.15 a 3.8 × 10−5 ± 2.3 × 10−6 b 46.1 ± 0.47 d 27.8 ± 0.48 c

0.5 h AHP SCF 55.6 ± 0.29 c 4.2 × 10−5 ± 3.0 × 10−7 a 49.3 ± 0.62 c 28.0 ± 0.18 c

1 h AHP SCF 52.8 ± 0.32 c 4.3 × 10−5 ± 1.7 × 10−6 a 50.9 ± 0.50 a 29.9 ± 0.12 a

3 h AHP SCF 65.0 ± 0.70 b 4.1 × 10−5 ± 3.7 × 10−8 ab 50.1 ± 0.72 b 29.9 ± 0.11 a

5 h AHP SCF 65.7 ± 4.03 b 4.2 × 10−7 ± 2.5 × 10−7 a 49.7 ± 0.37 bc 29.4 ± 0.25 b

Different letter represents a significant difference (p < 0.05) in the same column, where n = 3.



Foods 2023, 12, 1460 8 of 19

Accordingly, the acid-insoluble lignin content of SCF decreased after the AHP
treatment at 0.5 h but increased again at 3 h (Table 2). Similar decreases in the lignin
content of fibres were reported after applying AHP treatments to lignocellulosic materials
in previous cases of relevant research [5,11,29]. Hydrogen peroxide is known as a
strong oxidizing agent that can cause delignification and solubilization of hemicellulose.
According to Gould [15], an alkaline medium (pH = 11.5) can hasten the decomposition
of hydrogen peroxide. During the decomposition of hydrogen peroxide, hydroperoxide
ions are released, thereby contributing to the removal of chromophoric groups of lignin
by attacking carboxyl groups and ethylene groups. Hydrogen peroxide then reacts
with hydroperoxide ions to generate hydroxyl radicals which, in turn, are regarded as
the strongest oxidizers for having an important role in the oxidation process [15]. The
delignification and solubilization of hemicellulose in sugarcane fibres usually result
from the activity of hydroxyl radicals [30]. In our study, AHP treatment reduced the
lignin content in all samples. The acid-insoluble lignin content decreased significantly
in the 0.5 h and 1 h AHP SCF samples. However, as the AHP treatment time increased
from 1 h to 5 h, a slight increase occurred in the acid-insoluble lignin content, which was
noticeable when comparing the 0.5 h and 1 h AHP SCF samples to the 3 h and 5 h AHP
SCF samples. Our results agree with another study, which showed that AHP treatments
caused a significant decrease in lignin content in the first 30 min, although an increase in
the treatment time caused no further declines in the lignin content [31]. However, the
acid-insoluble lignin content increases to 65% and 65.7% for 3 h and 5 h, suggesting that
hemicellulose has been reduced as indicated in the FTIR spectra. As seen in Table 2, there
was an increase in the SBC of SCF samples treated with AHP. Fibres usually have the
capacity to bind to glucose and, thus, can potentially lower postprandial blood glucose
concentrations [32,33]. As shown in Table 2, particle sizes of AHP SCF samples were
larger than those of untreated-SCF samples. The particle size of AHP SCF samples
increased from 0.5 h to 1 h but then decreased slightly as the treatment time increased
to 5 h. This agrees with a study done by Gu et al. [34], which indicated that reduction
in particle size was due to the delignification effect of AHP on corn stover and wheat
straw. Additionally, this correlated with its WHC since a positive correlation usually
exists between the particle size and the WHC of SCF [35]. As the WHC increased, there
is an increase in hydrodynamic diameter, which is indicated by D(3,2) value due to its
swelling capacity and, thus, led to a greater amount of water absorption.

Figure 1 shows the WHC and OHC of both AHP and untreated-SCF samples. The
WHC values for untreated SCF, 0.5 h AHP SCF, 1 h AHP SCF, 3 h AHP SCF, and 5 h AHP
SCF were 2.98, 3.18, 3.86, 3.59, 3.38 g of water per g of SCF, respectively. As compared to
the untreated SCF, the WHC of SCF increased after the AHP treatment, rising through time,
from 0.5 to 1 h, but then decreased thereafter until the fifth hour. An increase in WHC
values reportedly occurred in previous research on ginseng fibre [29], okra fibre [5], and
sugarcane fibre [18,36]. The increase in the WHC of AHP-treated SCF could be due to the
changes in morphological structure of the fibres via the breakage of bonds and a greater
exposure of hydroxyl groups [29,37].

The OHC values for untreated SCF, 0.5 h AHP SCF, 1 h AHP SCF, 3 h AHP SCF, and
5 h AHP SCF were 2.47, 3.66, 3.50, 3.18, and 2.96 g of oil per g of SCF, respectively. As
compared to untreated SCF, the OHC of SCF increased after the AHP treatment. While the
OHC values of AHP SCF samples were higher than that of the untreated SCF, it decreased
over time, from 0.5 h to 5 h. Similar studies reported an increase in OHC after subjecting
SCF to AHP treatments [29,38]. Additionally, the observed trend in OHC values could be
attributed to the increased porosity of SCF after the AHP treatment.



Foods 2023, 12, 1460 9 of 19

Foods 2023, 12, x FOR PEER REVIEW 9 of 21 
 

 

time, from 0.5 to 1 h, but then decreased thereafter until the fifth hour. An increase in 
WHC values reportedly occurred in previous research on ginseng fibre [29], okra fibre [5], 
and sugarcane fibre [18,36]. The increase in the WHC of AHP-treated SCF could be due to 
the changes in morphological structure of the fibres via the breakage of bonds and a 
greater exposure of hydroxyl groups [29,37]. 

 
Figure 1. WHC and OHC of untreated and AHP SCF, different letters represent a significant differ-
ence within the same functional test (p < 0.05), where n = 3. 

The OHC values for untreated SCF, 0.5 h AHP SCF, 1 h AHP SCF, 3 h AHP SCF, and 
5 h AHP SCF were 2.47, 3.66, 3.50, 3.18, and 2.96 g of oil per g of SCF, respectively. As 
compared to untreated SCF, the OHC of SCF increased after the AHP treatment. While 
the OHC values of AHP SCF samples were higher than that of the untreated SCF, it de-
creased over time, from 0.5 h to 5 h. Similar studies reported an increase in OHC after 
subjecting SCF to AHP treatments [29,38]. Additionally, the observed trend in OHC values 
could be attributed to the increased porosity of SCF after the AHP treatment. 

FTIR analysis was conducted to identify the functional organic groups in SCF and to 
monitor their alterations before and after AHP treatments. Figure 2a depicts the FTIR 
spectra of SCF samples, where absorbance peaks appeared at 3200–3500 cm−1 (OH groups 
in cellulose), 2892 cm−1 (C-H vibration in cellulose and hemicellulose), 1633 cm−1 (vibration 
of water molecules absorb in cellulose), 1426 cm−1 (-CH2 group of cellulose), 1367 cm−1 (-
CH group of cellulose), 1158 cm−1 (hydroxyl bending of cellulose), 1028 cm−1 (O-H vibra-
tion in cellulose), and 895 cm−1 (C-O stretching in cellulose). The broadening of the OH 
band (3200–3500 cm−1) in IR spectra resulted from a mixture of intermolecular (3230–3310 
cm−1) and intramolecular (3340–3375 cm−1) hydrogen bonds [39,40]. These bands have 
higher intensities in the spectra of AHP-treated SCF, thereby confirming the variation in 
the hydrogen bond structure of SCF. The -CH region (2870–2900 cm−1) was used as an 

0.0

0.5

1.0

1.5

2.0

2.5

3.0

3.5

4.0

WHC  OHC

g/
g 

SC
F

Untreated SCF 0.5h AHP SCF 1h AHP SCF 3h AHP SCF 5h AHP SCF

d
cd

a
ab

bc

c

a
a

b
b

Figure 1. WHC and OHC of untreated and AHP SCF, different letters represent a significant difference
within the same functional test (p < 0.05), where n = 3.

FTIR analysis was conducted to identify the functional organic groups in SCF and to
monitor their alterations before and after AHP treatments. Figure 2a depicts the FTIR spec-
tra of SCF samples, where absorbance peaks appeared at 3200–3500 cm−1 (OH groups in
cellulose), 2892 cm−1 (C-H vibration in cellulose and hemicellulose), 1633 cm−1 (vibration
of water molecules absorb in cellulose), 1426 cm−1 (–CH2 group of cellulose), 1367 cm−1

(–CH group of cellulose), 1158 cm−1 (hydroxyl bending of cellulose), 1028 cm−1 (O–H
vibration in cellulose), and 895 cm−1 (C–O stretching in cellulose). The broadening of
the OH band (3200–3500 cm−1) in IR spectra resulted from a mixture of intermolecular
(3230–3310 cm−1) and intramolecular (3340–3375 cm−1) hydrogen bonds [39,40]. These
bands have higher intensities in the spectra of AHP-treated SCF, thereby confirming the
variation in the hydrogen bond structure of SCF. The –CH region (2870–2900 cm−1) was
used as an indicator of polymorphic transformation within the crystalline parts of cellu-
lose [41] In this study, after 0.5 and 5 AHP treatments, the peak values of the CH region
shifted from 2884 to 2890 and 2893 cm−1 (Figure 2b), respectively, which indicated the poly-
morphism transition from cellulose I to cellulose II [42]. The peak at 1633 cm−1 emanated
from absorbed water molecules via hydrogen bonds in the amorphous region of cellulose
macromolecules. AHP caused a higher intensity of the peak (1633 cm−1), which amplified
the decrease in the amorphous part of the SCF during the AHP treatments (Figure 2c).
Some specific peaks at 1426 and 895 cm−1 were relevant to the spectrum of the treated SCF,
which relate to the CH bending of amorphous and crystalline cellulose I. The empirical
crystallinity index (CI) can be calculated using the ratios of peaks at 1426 and 895 cm−1 [43].
The AHP treatment increased the CI index (from 0.452 of untreated SCF to 0.490, 0.491,
0.499, and 0.525 of 0.5 h to 5 h AHP SCF), revealing that the samples mainly comprised
crystalline cellulose II. The peak at 1277 cm−1 indicated C-H bending and O-H bending
in plain deformation, representing an overwhelming existence of crystalline cellulose
II (Figure 2c). As the absorbance at 895 increased with 0.5 h AHP SCF, showing the
transformation from cellulose I (natural cellulose) to cellulose II (because cellulose II is
more stable than cellulose I), the results confirmed the polymorphism transformation
peaks, shifting at 2800 cm−1.



Foods 2023, 12, 1460 10 of 19
Foods 2023, 12, x FOR PEER REVIEW 11 of 21 
 

 

 

 

 

 
Figure 2. FTIR spectra of untreated SCF, 0.5 h, 1 h, 3 h, and 5 h AHP SCF (a) at the wavelength of 
500–4000 cm−1, (b) The -CH region (2870–2900 cm−1) shifting, and (c) Variations of peak intensity at 

Figure 2. FTIR spectra of untreated SCF, 0.5 h, 1 h, 3 h, and 5 h AHP SCF (a) at the wavelength of
500–4000 cm−1, (b) The –CH region (2870–2900 cm−1) shifting, and (c) Variations of peak intensity at
wavelength 1633 (cm−1) and indicator peaks in transformation cellulose I to cellulose II (1426 and
1277 cm−1).

As seen in Figure 3a,b, the untreated-SCF samples appeared larger lengthwise and
had a smoother surface, probably due to the presence of intact lignin and hemicellulose. In
comparison, AHP SCF samples were more fragmented and had a rougher, wrinkled, more
porous surface (as indicated by the yellow arrows). Subjecting SCF to sodium hydroxide



Foods 2023, 12, 1460 11 of 19

can significantly affect the morphology of SCF as the alkaline environment causes fibres to
swell and the cellulose molecules to detach from each other, thereby disrupting the rigid
SCF structure [13].

Foods 2023, 12, x FOR PEER REVIEW 13 of 21 
 

 

 
Figure 3. Morphological images of untreated and AHP SCF detected by SEM at (a–e) 500× magnifi-
cation and (f–j) 2000× magnification. Yellow arrows indicate surface differences. 

AHP treatment could have caused shorter fragments and rough surfaces in SCF (Fig-
ure 3b–e and Figure 3g–j). With extended hours of AHP treatment, FTIR results indicated 
that amorphous cellulose, lignin, and hemicellulose content decreased from 0.5 to 5 h, 
which caused the SCF to be more porous, fragmented, and wrinkled, and it agrees with 
the SEM results. In a relevant study, AHP treatment with the effect of reducing 

Figure 3. Morphological images of untreated and AHP SCF detected by SEM at (a–e) 500× magnifi-
cation and (f–j) 2000× magnification. Yellow arrows indicate surface differences.



Foods 2023, 12, 1460 12 of 19

AHP treatment could have caused shorter fragments and rough surfaces in SCF
(Figures 3b–e and 3g–j). With extended hours of AHP treatment, FTIR results indicated that
amorphous cellulose, lignin, and hemicellulose content decreased from 0.5 to 5 h, which
caused the SCF to be more porous, fragmented, and wrinkled, and it agrees with the SEM
results. In a relevant study, AHP treatment with the effect of reducing hemicellulose in
the fibres caused a rougher surface in kenaf fibre [44]. The non-uniformity of fibre surface,
increasing porosity, and wrinkle structure were observed in citrus fruit fibre [38], white
turnip fibre [45], and ginseng fibre [29]. The wrinkled, porous surface of the AHP-treated
SCF samples meant a larger surface area and a greater level of exposure to hydrophilic
groups, thereby increasing the WHC, as discussed previously [29,46]. The particle size of
SCF increased and then decreased from 0.5 to 5 h as indicated in Table 2, which suggests
the size of SCF swelled first and then dissembled, from Figure 3a–e.

In Table 3, the reference sample refers to a typical white bread sample with no SCF
incorporation, while the untreated-SCF bread sample refers to that incorporated with
untreated SCF. Bread samples of 0.5 h AHP SCF, 1 h AHP SCF, 3 h AHP SCF, and 5 h
AHP SCF refer to samples with the corresponding AHP SCF samples. Table 3 lists the
resistance to extension of dough samples collected after mixing, maximum height, and
specific volume of bread samples.

Table 3. Extensibility of dough samples, maximum height, and specific volume of bread samples
without SCF incorporated (reference), incorporated with 5% untreated SCF, and 0.5 to 5 h AHP SCF.

Samples Resistance to
Extension (g)

Maximum Height
(mm)

Specific Volume
(cm3/g)

Reference 20.08 ± 0.45 c 61.7 ± 1.9 a 2.24 ± 0.05 a

Untreated SCF 26.62 ± 1.87 b 61.6 ± 1.5 a 2.20 ± 0.05 ab

0.5 h AHP SCF 30.41 ± 1.04 a 57.6 ± 3.2 b 2.13 ± 0.04 ab

1 h AHP SCF 13.10 ± 1.05 d 54.1 ± 0.7 b 2.00 ± 0.15 b

3 h AHP SCF 20.56 ± 2.71 c 54.2 ± 0.4 b 2.14 ±0.09 ab

5 h AHP SCF 11.72 ± 0.88 d 54.7 ± 0.9 b 2.05 ± 0.18 ab

Different letter represents a significant difference (p < 0.05) in the same column, where n = 6.

According to Table 3, a greater level of resistance to the extension of dough samples
was observed in the untreated group and the 0.5 h AHP SCF incorporated bread, compared
to that of the reference sample. Even though 1 h and 5 h AHP SCF dough samples had
lower resistance to extension values compared to the reference, the samples were observed
to break off immediately during the analysis, when stretched by the texture analyzer.
This observation was in agreement with a previous study on the incorporation of wheat
bran dietary fibre on steamed bread, showing that the incorporation of fibre resulted in
a decrease in dough extensibility [47]. Another study conducted by Gomez et al. [48]
suggested that the incorporation of dietary fibres increased the resistance to extension but
decreased the dough extensibility. The decrease in dough extensibility and the increase
in stiffness of the dough resulted from disruptions in the gluten network structure and
reduced gas retention ability through the process of dough and bread making because
SCF was incorporated [48]. This could negatively affect the height and loaf volume of
bread in the production line [47,49]. As shown in Table 3, the maximum height of AHP
SCF-incorporated bread samples significantly decreased, compared to the reference sample.

The decrease in maximum height can be seen in Figure 4a. Similar studies on the
incorporation of SCF [10] and hazelnut fibre [50] showed a decrease in height and loaf
volume, most probably due to lower gas retention during proofing resulting from the
disruption of the gluten network. Figure 4b demonstrates the average hardness and
chewiness of bread samples. The average hardness values for the reference sample, control
sample, 0.5 h, 1 h, 3 h, and 5 h AHP SCF were 2398, 2892, 4058, 4185, 3878, and 3794 g,
respectively; while the average chewiness values were 2187, 2218, 2604, 2960, 2444, and



Foods 2023, 12, 1460 13 of 19

2567. By adding SCF, the average hardness and chewiness increased compared to the
reference sample. In addition, all AHP samples are significantly harder and chewier than
the untreated-SCF sample, but no significant difference was found among all AHP samples.
Previous studies done by was found that incorporating dietary fibre from wheat bran and
inulin [51] and fenugreek [9] have increased the hardness of bread. The hardness and
chewiness trends correspond to the WHC values of SCF samples due to the amount of
water in the formulation of all SCF-incorporated bread samples, which were kept constant
despite having an increase in WHC. The increase in the hardness of AHP SCF incorporated
bread samples was due to the SCF, which competed with gluten over the absorption of
water, as the AHP SCF had a higher WHC and therefore resulted in a weak gluten network,
which was unable to retain large gas bubbles produced during proofing [52].

Foods 2023, 12, x FOR PEER REVIEW 15 of 21 
 

 

inulin [51] and fenugreek [9] have increased the hardness of bread. The hardness and 
chewiness trends correspond to the WHC values of SCF samples due to the amount of 
water in the formulation of all SCF-incorporated bread samples, which were kept constant 
despite having an increase in WHC. The increase in the hardness of AHP SCF incorpo-
rated bread samples was due to the SCF, which competed with gluten over the absorption 
of water, as the AHP SCF had a higher WHC and therefore resulted in a weak gluten 
network, which was unable to retain large gas bubbles produced during proofing [52]. 

 

 
Figure 4. (a) Cross-sectional photographs illustrating the crumb appearance of bread samples. (b) 
Texture profile analysis (hardness and chewiness) of bread samples without SCF (reference), incor-
porated with 5% untreated SCF, and 0.5 to 5 h AHP SCF. Different letter represents a significant 
difference within the same texture attributes (p < 0.05), where n = 6. 

0

1000

2000

3000

4000

5000

6000

Reference Untreated
SCF

0.5h AHP
SCF

1h AHP
SCF

3h AHP
SCF

5h AHP
SCF

Hardness Chewiness

b c

a

a
b

b

a

a

a
a

a a

(b)

Figure 4. (a) Cross-sectional photographs illustrating the crumb appearance of bread samples.
(b) Texture profile analysis (hardness and chewiness) of bread samples without SCF (reference),
incorporated with 5% untreated SCF, and 0.5 to 5 h AHP SCF. Different letter represents a significant
difference within the same texture attributes (p < 0.05), where n = 6.



Foods 2023, 12, 1460 14 of 19

Figure 5 shows the respective glycemic glucose equivalent (GGE) disposal, GGE release,
and net GGE curves of the bread samples. GI values are categorized as low (≤55), medium
(55 < GI < 70), and high (≥70) [53]. White bread had a high GI value of 70–100, which can be
used as a reference to calculate the estimated GI values of SCF-incorporated bread samples.
In this study, the reference sample was taken to have an estimated GI of 100.

Foods 2023, 12, x FOR PEER REVIEW 16 of 21 
 

 

Figure 5 shows the respective glycemic glucose equivalent (GGE) disposal, GGE re-
lease, and net GGE curves of the bread samples. GI values are categorized as low (≤55), 
medium (55 < GI < 70), and high (≥70) [53]. White bread had a high GI value of 70–100, 
which can be used as a reference to calculate the estimated GI values of SCF-incorporated 
bread samples. In this study, the reference sample was taken to have an estimated GI of 
100. 

 

 

0

10

20

30

40

50

60

70

0 20 40 60 80 100 120 140 160 180

G
G

E 
R

el
ea

se
 (g

)

Time (min)

Reference Untreated SCF 0.5h AHP SCF

1h AHP SCF 3h AHP SCF 5h AHP SCF

(a)

0

20

40

60

80

100

120

140

0 20 40 60 80 100 120 140 160 180

G
G

E 
D

isp
os

al
 (g

)

Time (min)

Reference Untreated SCF 0.5h AHP SCF
1h AHP SCF 3h AHP SCF 5h AHP SCF

(b)

Figure 5. Cont.



Foods 2023, 12, 1460 15 of 19Foods 2023, 12, x FOR PEER REVIEW 17 of 21 
 

 

 
Figure 5. (a) GGE release curves illustrating overall glucose release. (b) GGE disposal curves. (c) Net 
GGE curves. Error bars represent mean ± standard deviation (n = 2). All data were calculated based 
on the fresh weight of the bread samples without SCF incorporated (reference), incorporated with 
5% untreated SCF, and 0.5 to 5 h AHP SCF. 

Table 4 lists the incremental area under the curve (iAUC), relative glycemic potency 
(RGP), and rapid, digestible starch (RDS) values of the respective bread samples. There 
was a significant decrease in iAUC values, associated with the incorporation of SCF, com-
pared to the reference sample. A similar trend was also observed in both RGP and RDS 
values of the SCF-incorporated bread samples. Additionally, the 0.5 h AHP SCF incorpo-
rated sample has significantly higher iAUC, RCP, and RDS values than untreated SCF and 
the rest of the AHP SCFs, but there is no significant difference found among untreated 
SCF and AHP SCF samples. As shown in Table 4, the estimated GI values of SCF-incorpo-
rated samples were lower than that of the reference, making them fall under the “me-
dium” or “low” GI category. However, there was a slight increase in the respective values 
of the 0.5 h AHP SCF samples, compared to the other AHP SCF samples. This could sug-
gest that a short duration of AHP treatment at 0.5 h increased the digestion rate, but a 
longer duration of the AHP treatment (1 h and above) decelerates the digestion rate. In a 
study by Dhital et al. [54], starch hydrolysis can be inhibited by a high concentration of 
cellulose during digestion. Cellulose can bind to α-amylase via a noncompetitive mecha-
nism, which can effectively inhibit its activity on starch. A similar study by Seki et al. [55] 
demonstrated that postprandial blood glucose concentrations were lowered by insoluble 
dietary fibre. We did observe that the 0.5 h AHP SCF sample has a lower glycemic re-
sponse reduction effect. This suggests that SCF treated at shorter AHP durations were 
unable to modulate the degree of starch gelatinization. However, at 0.5 h AHP treatment, 
lignin was removed, indicating that hemicellulose reduction might be able to further in-
fluence starch digestibility as further reduction of hemicellulose would cause a disinte-
grated fibre structure, therefore increasing surface area. Nsor-Atindana et al. [56] demon-
strated that particle size and surface area influenced the interaction of cellulose with α-
amylase and as a result, the digestion of potato starch in both oral and gastric digestion, 
with the inhabitation effect of cellulose against α-amylase becoming more pronounced as 
particle size was reduced while surface area increased. Although in our study, significant 

0

5

10

15

20

25

30

35

40

0 10 20 30 40 50 60 70 80 90 100

N
et

 G
G

E 
(g

)

Time (min)

Reference Untreated SCF 0.5h AHP SCF

1h AHP SCF 3h AHP SCF 5h AHP SCF

(c)

Figure 5. (a) GGE release curves illustrating overall glucose release. (b) GGE disposal curves. (c) Net
GGE curves. Error bars represent mean ± standard deviation (n = 2). All data were calculated based
on the fresh weight of the bread samples without SCF incorporated (reference), incorporated with 5%
untreated SCF, and 0.5 to 5 h AHP SCF.

Table 4 lists the incremental area under the curve (iAUC), relative glycemic potency
(RGP), and rapid, digestible starch (RDS) values of the respective bread samples. There was
a significant decrease in iAUC values, associated with the incorporation of SCF, compared
to the reference sample. A similar trend was also observed in both RGP and RDS values of
the SCF-incorporated bread samples. Additionally, the 0.5 h AHP SCF incorporated sample
has significantly higher iAUC, RCP, and RDS values than untreated SCF and the rest of
the AHP SCFs, but there is no significant difference found among untreated SCF and AHP
SCF samples. As shown in Table 4, the estimated GI values of SCF-incorporated samples
were lower than that of the reference, making them fall under the “medium” or “low” GI
category. However, there was a slight increase in the respective values of the 0.5 h AHP
SCF samples, compared to the other AHP SCF samples. This could suggest that a short
duration of AHP treatment at 0.5 h increased the digestion rate, but a longer duration of
the AHP treatment (1 h and above) decelerates the digestion rate. In a study by Dhital
et al. [54], starch hydrolysis can be inhibited by a high concentration of cellulose during
digestion. Cellulose can bind to α-amylase via a noncompetitive mechanism, which can
effectively inhibit its activity on starch. A similar study by Seki et al. [55] demonstrated that
postprandial blood glucose concentrations were lowered by insoluble dietary fibre. We did
observe that the 0.5 h AHP SCF sample has a lower glycemic response reduction effect. This
suggests that SCF treated at shorter AHP durations were unable to modulate the degree of
starch gelatinization. However, at 0.5 h AHP treatment, lignin was removed, indicating that
hemicellulose reduction might be able to further influence starch digestibility as further
reduction of hemicellulose would cause a disintegrated fibre structure, therefore increasing
surface area. Nsor-Atindana et al. [56] demonstrated that particle size and surface area
influenced the interaction of cellulose with α-amylase and as a result, the digestion of
potato starch in both oral and gastric digestion, with the inhabitation effect of cellulose
against α-amylase becoming more pronounced as particle size was reduced while surface
area increased. Although in our study, significant reduction of GI was not observed in
the AHP SCF incorporated breads in comparison to the untreated one, which could be



Foods 2023, 12, 1460 16 of 19

limited by the low amount of SCF incorporated (5%) or a higher amount of water added
as compared to the reference, which was determined by farinograph analysis. In future
studies, we suggest incorporating dough improvers, such as ascorbic acid, to reduce the
dilution and destruction effect of SCF in the gluten network while incorporating a higher
amount of SCF to amplify its effect on reducing starch digestibility. However, this study
offers guides for future researchers to use optimized AHP duration (3 h) with improved
PMI to treat SCF, to increase its WHC while not to impact the starch digestion reduction
ability of SCF.

Table 4. Estimated glycemic index (GI) values of bread samples with no SCF incorporated (reference),
incorporated with 5% untreated SCF, and 0.5 to 5 h AHP SCF based on fresh weight basis.

Samples
Estimated GI

iAUC RGP RDS

Reference 100 100 100

Untreated SCF 56 60 65

0.5 h AHP SCF 63 58 70

1 h AHP SCF 53 50 56

3 h AHP SCF 49 50 54

5 h AHP SCF 51 52 54

4. Conclusions

To improve the physicochemical properties of SCF fibre, a high hydrogen peroxide
concentration (7.7%) and shorter time (0.5, 1, 3, and 5 h) were used in this study to increase
the productivity and scalability of the alkaline hydrogen peroxide (AHP) treatment. The
AHP treatment affected the composition, structure, and physicochemical properties of SCF.
The acid-insoluble lignin content of the SCF decreased in response to the AHP treatment
from 0.5 h to 5 h under the condition of 7.7% H2O2 at pH 11.5. With the AHP treatment,
the SCF exhibited higher WHC and OHC values, compared to the untreated SCF. This
could result from the exposure of hydrophilic groups and cause an increase in the surface
area as well as the porosity of SCF. The greater surface area and porosity of the SCF after
AHP treatment were found and apparent in the SEM images. Although the AHP treatment
positively affected the physiochemical properties, its incorporation into wheat flour-based
dough and white bread had a negative effect on textural properties. Dough and bread
samples incorporated with AHP SCF exhibited a reduction in dough extensibility and
maximum height, associated with an increase in the hardness and chewiness of bread. This
resulted from the disruption in the gluten network structure and reduced gas retention
ability in the process of dough and bread making, as the incorporation of SCF resulted
in competition with gluten for the absorption of water, especially the AHP SCF which
had higher WHC. Despite its impact on textural properties, the incorporation of SCF
successfully lowered the estimated GI values of bread. Incorporation of 1, 3, and 5 h
AHP SCF was effective in reducing the glycemic index than 0.5 h AHP SCF. We need
further studies to explain the mechanism of AHP treatment on the glucose release rate of
SCF-incorporated bread.

Supplementary Materials: The following supporting information can be downloaded at: https://
www.mdpi.com/article/10.3390/foods12071460/s1. Table S1. PMI for different methods used in
different paper; Table S2. Parameters to determine particle size of samples; Figure S1. Farinograph
analysis indicating the dough development of flour samples over a 20 min mixing regime; Table S3.
Dough extensibility test parameters on texture analyzer; Table S4. Double compression test parameters
on texture analyzer; Table S5. Total iAUC, relative glycemic potency (RGP), and rapidly digestible starch
(RDS) values of bread samples. References [57–59] are cited in the supplementary materials.

https://www.mdpi.com/article/10.3390/foods12071460/s1
https://www.mdpi.com/article/10.3390/foods12071460/s1


Foods 2023, 12, 1460 17 of 19

Author Contributions: Conceptualization, K.F.C., F.N.B.A.H. and J.D.; Methodology, K.F.C., F.N.B.A.H.,
Z.A.R.Y., K.K.T.G. and J.D.; Software, F.N.B.A.H. and A.T.; Validation, F.N.B.A.H., A.T. and J.D.;
Formal Analysis, F.N.B.A.H., A.T. and J.D.; Investigation, F.N.B.A.H., Z.A.R.Y. and J.D.; Resources,
J.D.; Data Curation, F.N.B.A.H. and J.D.; Writing—Original Draft Preparation, F.N.B.A.H. and A.T.;
Writing—Review and Editing, F.N.B.A.H., A.T. and J.D; Visualization, F.N.B.A.H. and A.T.; Supervi-
sion, K.K.T.G., S.M.G. and J.D.; Project Administration, J.D.; Funding Acquisition, K.K.T.G., S.M.G.
and J.D. All authors have read and agreed to the published version of the manuscript.

Funding: This study was funded by Singapore Institute of Technology Ignition Grant (R-MOE-
E103-F019), and ACP was funded by Singapore Food Story Theme 2—1st Alternative Protein Seed
Challenge Grant (W20W2D0013 and W20W2D0019) and Singapore Food Story R&D Programme
Industry Alignment Fund Pre-positioning (IAF-PP) Theme 2—Advanced Biotech-based Protein
Production Grant (A21H7a0131 and H21H8a0005).

Data Availability Statement: Data is contained within the article.

Acknowledgments: This study was funded by Singapore Institute of Technology Ignition Grant
(R-MOE-E103-F019) and supported by Tamu Group Pte Ltd. We would like to thank Enyi Ye, Michelle
Yew Pek Yin, and Dan Kai from Institute of Materials Research and Engineering (IMRE), Agency for
Science, Technology and Research; the previous and present lab mates from Singapore Institute of
Technology, Shanice Lim, Vernice Seah, Cedric Sow Wee Jian, Cheryl Ng Kwoek Zhen, and Jeremy
Chin Tak Gun, for their kindness and assistance.

Conflicts of Interest: The authors declare no conflict of interest.

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	Introduction 
	Materials and Methods 
	Materials and Reagents 
	AHP Modification of SCF 
	Characterization of SCF 
	Acid-Insoluble Lignin Content Determination 
	Sugar Binding Capacity (SBC) 
	Water Holding Capacity (WHC) and Oil Holding Capacity (OHC) 
	Particle Size Measurement 
	Fourier Transform Infrared Spectroscopy (FTIR) 
	Scanning Electron Microscope (SEM) 

	Development of Dough and Bread 
	Hydration of Flour Using DoughLAB 
	Bread Making Process 

	Characterization of Dough and Bread 
	Dough Extensibility 
	Loaf Specific Volume and Maximum Height of Loaf 
	Texture Profile Analysis of Bread Crumb 
	Moisture Analysis and Water Activity of Bread Crumb 
	In Vitro Determination of Glycemic Potency 
	In Vitro Digestion of Bread Samples 
	Quantification of Glucose Release 

	Data Analysis for In Vitro Glycemic Potency Determination 
	Statistical Analysis 

	Results and Discussion 
	Conclusions 
	References