Utilization of Intestinal Probiotics to Improve the Degradation and
Absorption of Food and Drug Homologous Flavonoids
Zixun Su
Dalian Huamei School, Dalian, Liaoning Province, 116033, China
Keywords:
Flavone, E. Coli, Degradation Rate, PCR, Deamination Tyrosine, FLR.
Abstract:
Under the condition that the slow degradation rate of flavone in food in the gastrointestinal tract of the human
body has long been a problem for researchers, we constructed and justified a protein to improve the
degradation and absorption rate of flavone. The paper, through methods including polymerase chain reaction
and gel electrophoresis, explores the possible solution for increasing degradation rate with a flr gene. The
FLR enzyme produced throughout the experiment would successfully degrade flavonoids into deamination
tyrosine (DAT) to achieve the goal of having anti-inflammatory function. The paper concludes that with E.
Coli carrying Pet28a-flr-chi-enoR-phy, flavonoids tested can be dissolved and decomposed up to 95% within
6 hours.
1 INTRODUCTION
In modern life, people often have poor resistance and
get sick easily. Due to the situation, flavonoids should
be a good choice as flavones in fruits and vegetables
have been found to help fight cancer and bacteria.
They have antioxidant, hypocholesterolemic, and
anti-inflammatory properties, as well as the ability to
modulate cell signaling and gene expression, which
are linked to disease development. (Thilakarathna S
H, 2013) Nevertheless, the low apparent availability
of flavonoids is currently considered as a problem as
the benefits of flavones cannot be expressed fully.
The enzyme in the human intestinal flora was unable
to practice degrading and absorbing flavonoids well.
(Ravishankar D, 2013) Therefore, attempts to
improve their bioavailability in order to improve the
efficacy of flavonoids are always being made and
studied. (Yang, 2021) Research on flavonoid
degradation has been ongoing, but the way to
improve the absorption of flavonoids in the
gastrointestinal tract of the human body is still to be
found. The situation stayed still until 2020, when
Nature Communication reported a key enzyme FLR
that would initialize the degradation of the flavone. In
this case, flavone functions and can help the human
body absorb various types of flavonoids.
Flavones are largely found in plants. (Leonard,
2006) The research on flavonoids in recent years is
extensive, such as Soybeans flavone, Baicalensis
flavone, and Epimedium flavone. (Geng, 2003) They
are pharmacodynamic compounds and have been
widely used in the treatment of cancer and various
diseases. (Yao, 2004) However, it is unfortunately
that some people do not have the ability to digest
certain groups of flavones, which become detrimental
to their health in this way. During this experiment, we
made E. coli carry the flr gene to more efficiently
produce the FLR enzyme. This manufactured bacteria
can now express the FLR gene well, increase the
degradation rate of flavonoids, and furtherly generate
DAT, which would activate the immune system of the
human body so as to achieve anti-inflammatory,
antibacterial, anti-cancer and other purposes, at the
same time helping reduce clinical treatment costs.
(Ashrafizadeh, 2020)
2 CONCEPTS
Flavonoids belong to a large class of significant
secondary metabolites of plants, which have good
pharmacological activities and important nutrition.
The metabolism, absorption, and excretion of it are
accomplished in the gastrointestinal tract of the
human body. (Chen, 2021) It acts as a role in the
gastrointestinal tract in a physiological way, leading
to the functions of antioxidant, anti-inflammatory,
and anti-cancer as shown in Figure 1.
34
Su, Z.
Utilization of Intestinal Probiotics to Improve the Degradation and Absorption of Food and Drug Homologous Flavonoids.
DOI: 10.5220/0012001100003625
In Proceedings of the 1st International Conference on Food Science and Biotechnology (FSB 2022), pages 34-41
ISBN: 978-989-758-638-5
Copyright
c
ξ 2023 by SCITEPRESS β Science and Technology Publications, Lda. Under CC license (CC BY-NC-ND 4.0)
Figure 1: Multiply diagrams to illustrate the benefit brought by flavonoids (Jeon, 2009).
Figure 2: Chemical process of FLR participating in changing flavone into DAT (Jeon, 2009).
In the past ten years, a large number of studies
have been carried out to discover the digestion and
absorption of flavonoids, especially in the digestive
tract of the human body, with the aim of applying the
functions to foods, drugs, or even synthetic products
to treat diseases. Along with this goal, we managed
to build intestinal engineering probiotics to increase
the degradation of food and drug homologous
flavonoids.
Inspired by a paper from Nature Communication
written by Weihong Jiang Research Group, CAS,
which demonstrated the newly discovered alkene
reductase-flavone reductase (FLR), we started our
project. FLR enzyme not only initiates flavonoid
absorption and degradation in the human body, but it
also has similar effects and functions for another type
of flavonoid, flavonol. According to the paper, the
enzyme comes from intestinal bacteria, so this
experiment should have an outcome that is highly
practicable.
In order to increase the practicability and improve
the feasibility of our experiment, we chose apigenin,
chrysin, luteolin, and diosmetin as four samples for
function tests based on the substrate spectrum
analysis since chronic diseases can be cured or
alleviated by intaking them (see figure 3). (Tang,
2017).
Utilization of Intestinal Probiotics to Improve the Degradation and Absorption of Food and Drug Homologous Flavonoids
35
Figure 3: Demonstration of part of the substrate spectrum of flavonoids.
Figure 4: Flow chart representing the principle of E. coli carrying pET28a-FLR.
3 DESIGN
By starting with the pET28a vector, we constructed
the pET28a-flr plasmid. After that, we insert it into
the carrier, which is the E. coli, to produce the
engineered strain for realization of the concept of our
product. In the ATLATL lab in Shanghai, we
successfully built the pET28a-flr plasmid and proved
it with methods like polymerase chain reaction and
sequencing.
Next, with the aim of determining the
performance of the E. coli carrying pET28a-flr, we
designed and used two experiments with the four
types of common flavonoids mentioned before, which
include apigenin, chrysin, luteolin, and diosmetin.
With the initial concentration set at 10mg/L, we
measured and recorded the concentration of
flavonoids after 2 hours and 6 hours. We repeat the
enzyme activity test for each flavonoid three times, to
guarantee the credibility of the outcome.
4 RESULT
After we purified the protein, which is the FLR
enzyme, an enzyme activity test to evaluate the
functions of the FLR enzyme was carried out by us.
The same four kinds of flavonoids were used as
samples: apigenin, chrysin, luteolin, and diosmetin.
Starting with an initial flavonoids concentration of
100.05 mg per liter, an OD600 as 1.0, and an FLR
enzyme concentration as 1 mM per liter, we
conducted the tests. Every test is repeated three times
to reduce the errors and limit the uncertainty to the
best of our ability.
The results are recorded for 0h, 2h, and 6h to
demonstrate the changes:
Table 1: Data of concentrations of flavonoids.
Concentration (mg/L) 0h 2h 6h
Apigenin 9.96 2.16 0.03
Chrysin 9.97 2.79 0.12
Luteolin 9.96 2.09 0.11
Diosmetin 10.05 5.15 0.53
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36
The results are also shown in the following bar graphs:
Figure 5: Bar graph of the concentration of flavonoids after 2 hours and 6 hours.
Figure 6: Bar graph of the concentration of flavonoids after 2 hours.
As shown in Figure 5, the concentration of the
four types of flavonoids significantly decreased after
6 hours. Although after 6 hours, approximately 0.3-
5% of flavonoids are still left, it can be used to
indicate that the enzyme we made has high activity in
degrading and certain universality in degrading
different flavonoids.
Similarly, in Figure 6, it can be inferred that all
the tested flavonoids have only 1-7% left, which is
near the stage of full degradation. The strong and
undoubtable ability of our E. coli to degrade
flavonoids is shown with the data and visualized
graphs in the way we expected.
To sum up, the E. coli carrying the FLR enzyme
has the ability to degrade various common flavonoids
with certain practicability. In the comparison of the
degradation rates of the tested flavonoids, they should
be ranked from least to greatest: diosmetin < luteolin
< chrysin < apigenin.
5 MODEL
Besides tables and graphs, we also designed models
to represent and forecast the degradation rate of our
FLR enzyme using the data we got from the testing.
In considering about the quantity of our data, we
chose MATLAB as the tool to visualize our results in
the form of model.
Since the data follows a declining trend, we chose
to use the following negative exponential function to
prevent the appearance of negative values in the y-
axis:
ππ¦
ππ₯
ξ΅ποΊπ¦ξ΅π₯ο»
where dy represents the change in y, dx represents
the change in x, and a represents the initial
concentration of the four flavonoids.
In this case, the analytic expression will be:
π¦ξ΅ππ
ξ―ξ―«
ξ΅
π
where a, b, c are constant resulted from the line of
best fit in the models.
According to the modeling results for each
samples showing below, the fitting degrees are the
same.
As shown by Figure 8, these four curves have
pretty similar trends. The functions can be used as a
reference to predict the time needed for our E. coli
carrying pET28a-flr to achieve its efficiency. For
example, it may take 0.8 hours for the bacteria to
degrade half of the apigenin, and it may take 3.9
hours to degrade chrysin to 10% of the original
amount.
Furthermore, the derivative of these curves is also
calculated and visualized by us to directly see their
degradation rate in certain hours:
Utilization of Intestinal Probiotics to Improve the Degradation and Absorption of Food and Drug Homologous Flavonoids
37
Figure 7: Results of apigenin(a), chrysin(b), luteolin(c), diosmetin(d) is used for modeling.
Figure 8: Line of best fit in exponential mode to represent the curves of degradation.
In Figure 9, though the degradation rate of
diosmetin is much slower than the others during the
first 2 hours of degradation, the rate increases and
turns to be the fastest in the next four hours. Because
Figure 9 shows that the lower the concentration of
flavonoids, the faster the degradation rate, we can
conclude that FLR enzyme should be suitable for
degrading flavonoids in large quantities.
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Figure 9: Hours vs. degradation rate graph for four tested flavonoids.
Figure 10: Illustration of pET28a-flr-chi-enoR-phy enzyme.
6 PROTEIN CONSTRUCTION
The target fragment for protein expression,
BBa_K3998004, is built into the vector of pET28a.
This fragment, transcribed by the T7 promoter and
ended by the T7 terminator, contains a His tag for
protein purification. Molecular biology experiments
have been carried out by us, in which we successfully
made the fragment in the vector of E. coli BL21.
Detailed descriptions of all component parts are
listed:
6.1 BBa_K3998000
The flr gene, a 6275bp long gene that increases the
rate of flavonoid degradation, is used to create a strain
that secretes enzyme more efficiently. It can assist in
better producing DAT, activate the immune system
of the human body, and achieve the functions of
flavonoids, including anti-inflammatory, anti-cancer,
and antibacterial. Also, treatment costs would be
largely reduced with the participation of this gene.
6.2 BBa_K3998001
Chi, a 510bp long gene used to improve the rate of
flavonoid degradation, is used to create a strain
capable of secreting enzyme more efficiently. With
chi geneβs function of converting dihydroflavone into
chalcone, it can improve degradation rate, DAT
production, and activate the human immune system
to protect the human body from serious diseases like
cancer, inflammation, and tumors. Improving
immunity of the human body would also make
clinical treatment cost less.
6.3 BBa_K3998002
EnoR, a 948bp long gene that increases the
degradation rate of flavonoids, is used to create a
strain that secretes enzyme more efficiently. It has
almost the same function as the chi gene does. With
the enoR geneβs function of converting
dihydroflavone into chalcone, it can improve
degradation rate, DAT production, and activate the
human immune system to protect the human body
from serious diseases like cancer, inflammation, and
tumors. Improving immunity of the human body
would also make clinical treatment cost less.
Utilization of Intestinal Probiotics to Improve the Degradation and Absorption of Food and Drug Homologous Flavonoids
39
Figure 11: DNA map of plasmids expressing FLR.
Figure 12: DNA map of pET28a and location of flr/chi/enoR/phy on plasmids.
6.4 BBa_K3998003
Phy, a 1068bp long gene that improves flavonoid
absorption, is used to create a strain that secretes
enzyme more efficiently. It has similar functions to
the chi gene and the enoR gene. With phy geneβs
function of converting dihydroflavone into certain
degradation products, it can improve degradation
rate, DAT production, and activate the human
immune system to protect the human body from
serious diseases like cancer, inflammation, and
tumors. Improving immunity of the human body
would also make clinical treatment cost less.
7 EXPERIMENTAL APPROACH
During the experiment, we managed to build the
plasmid and prove it with methods like polymerase
chain reaction and gel electrophoresis.
FSB 2022 - The International Conference on Food Science and Biotechnology
40
The pET28a vector is already in the plasmid
library, so we just needed to obtain it from there.
Acquisition of Inserts: introduce homologous
sequences of pET28a vector into the 5β-end of
forward and reverse primers, to make the ends
identical to each other.
Table 2: Acquisition of inserts.
Primer Sequence
Catalase-F-Nhel: atggctagcatgagttcaaataaactgacaact
Catalase-R-XhoI: gtgctcgagttaagaatcttttttaatcggcaa
Recombination: use formula to calculate the
amount of DNA needed for recombination and
diluted pET28a vector and inserts earlier to ensure the
accuracy of loading.
Table 3: Recombination.
Components Recombination
p
ET28a 107.3ng, convert to volume
flr/chi/enoR/phy 37.3-42.72ng, convert to
volume
Buffe
r
4ul
Exnase II 2ul
ddH2O To 20ul
8 CONCLUSION
In conclusion, by introducing the pET28a-flr-chi-
enoR-phy into the E. coli BL21, we successfully
increased the degradation rate of the medicine and
food homologous flavonoids. As results showed that
more than 95% of the tested flavonoids were
degraded after 6 hours of time. In this case, the
targeted anti-inflammatory, antibacterial, and anti-
cancer functions of flavonoids would work as
intended. When we were doing the experiment, the
bacteria in the culture medium did not grow at a fast
rate, which limited us to repeating it for 3 times.
Possible errors that may be accidentally included in
the data are not totally eliminated. In the future, since
the FLR enzyme appears to have an incredible
capacity to break down flavonoids, we are looking
forward to testing how the human body would
perform with and without the E. coli with pET28a-flr.
Whatβs more, in the event that the further experiment
succeeds, we are going to likely attempt to include the
FLR-built microscopic organisms into yogurt. Yogurt
contains a huge number of lactic-corrosive
microscopic organisms. By including E. coli with
pET28a-flr, we may make a health-care yogurt to be
consumed after meals, which is beneficial for human
well-being advancement.
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