Analysis of Total Phenolics and Flavonoids from the
R
oot Bark of
Flacourtia rukam
Muharni
*
, Elfita, Julinar, and Heni Yohandini
Department of Chemistry, Faculty of Mathematics and Natural Sciences, University of Sriwijaya, Jl. Raya Palembang-
Prabumulih Km 32, Indralaya, Ogan Ilir, South Sumatera, 30662 Indonesia
Keywords: Phe
nolic, Flavonoid, Flacourtia rukam
Abstract:
Flacourtia rukam have been used in the to folk medicine. The roots was used by women after giving birth
as antiseptic and the stem bark was used to antihypertensive in the Regency of Musi Banyu Asin South
Sumatera Indonesia. Total phenolic and flavonoid content were determined for methanol, ethyl acetate and
n-hexane extracts from the root bark of F. rukam. Each extracts were determined antioxidant activity using
1,1-diphenyl-2-picryl-hydrazyl (DPPH) method. The results of the study showed that phenolic higher in
methanol extract (71.8868 mg GAE/g) compared with ethyl acetate extract (56.6094 mg GAE/g), while n-
hexane extract no detection. For flavonoids content showed, methanol extract (2.3116 mg QE/g) and ethyl
acetate extract (2.3304 mg QE/g) where the flavonoid content is not significantly different, while n-hexane
extract only contained flavonoid 0.8129 mg QE/g. The antioxidant activity the methanol, and ethyl acetate
extracts showed IC
50
52.91µg/mL and 86.92 µg/mL and in categorized as active antioxidant, while n-hexane
extract obtained IC
50
values 268.02 µg/ml in category weak antioxidant.
1 INTRODUCTION
Phenolic compounds is antioxidant properties and
antiradical activities that are beneficial to health.
Phenolic compound also showed activity as anti-
inflammatory, enzyme inhibition and induction,
detoxification and process of skin rejuvenation or
the premature aging process through stimulate
collagen production (Fuad et al., 2016). Antioxidant
activity of phenolic pompounds in small
concentrations can protect, prevent or induction the
level of oxidative damage to biomolecules. One of
the plants used as traditional medicine is Flacourtia
rukam.
This plant in the south of Sumatra the stem bark
is used as an antihypertensive drug. Besides that the
fruit is used to treat diarrhea and dysentery, the
leaves are used to treat swollen eyelids, and the roots
are used by women after giving birth (Yustian et al.,
2012. The biological activity of a plant extract is
closely related to the secondary metabolites it
contains, including flavonoid, phenol, terpenoid,
steroid and alkaloid. Secondary metabolites can be
utilized in the field of pharmacology (Mustarichie et
al., 2013), including as an antioxidant, antibiotic,
anticancer, blood anticoagulant, inhibiting
carcinogenic effects. Besides that secondary
metabolites can also be used as environmentally
friendly pest controllers (Samsudin and Khoiruddin,
2008).
Some information on the chemical content and
biological activity of F. rukam has been reported.
Saree et al., (1998) reported that the Flacourtia
rukam contained stigmastan-3,6-dione and friedelin.
Besides that, Ikram et al., (2009) reported that the
fruit contained phenolic and showed antioxidant
activity with a value of % inhibition of 70.9%. From
the fruit section 5 compounds have been reported,
namely monogalactosyl diacylglycerol, β-sitosterol-
3β-glucopiranoside-6β-fatty acid esters, β-sitosterol,
triacylglycerol, and chlorophyll a (Ragasa et al.,
2016). Monogalaktosildiasilgliserol compound is
active as anti-inflammatory (Imbs et al., 2013).
Meanwhile for the parts of the stem bark of
Flacourtia rukam was reported to contain friedelin,
poliothrysoside, and β-sitosteryl-3β-glucopyranoside
(Muharni et al., 2018). The phytochemical test of the
Flacourtia rukam plant has been shown contain
triterpenoid, steroids, flavonoids and phenolic
compounds (Muharni et al., 2016). In this paper we
will report the analysis of total phenolic and
30
Muharni, ., Elfita, ., Julinar, . and Yohandini, H.
Analysis of Total Phenolics and Flavonoid from the Root Bark of Flacourtia rukam.
DOI: 10.5220/0008839200300035
In Proceedings of the 1st International Conference on Chemical Science and Technology Innovation (ICOCSTI 2019), pages 30-35
ISBN: 978-989-758-415-2
Copyright
c
2020 by SCITEPRESS – Science and Technology Publications, Lda. All rights reserved
flavonoids from the root extracts of Flacourtia
rukam
2 MATERIALS AND METHODS
2.1 Chemicals
1,1-diphenyl-2-picryl-hydrazyl (DPPH), quercetin,
gallic acid, Folin-Ciocalteu, dimethylsulfoxide,
sodium carbonat, aluminum chloride, potassium
acetate (reagent were obtained from Sigma Aldrich,
USA), methanol, ethyl acetate, n-hexane, and
aquadest. The solvents is analytical grade and were
destilation before used.
2.2 Preparation of Sampel and
Identification
The root bark of plant of F. rukam was collected at
month of january 2018 2018 from Musi Banyuasin,
South Sumatera, Indonesia. The taxonomic identity
of the plant was confirmed by Dr. Laila Hanum
(number specimen VIC 2702) at of the Botanical
laboratory Departement of Biology University of
Sriwijaya. The plant materials (1Kg) was cleaned
from the pollutants and the materail plants were
cut into smaller sizes and then to air dried at
room temperature until the weight constant. The
dried sample was powdered busing a grinding
machine and obtained (300 g) and used for further
studies.
2.3 Extraction
Powdered of root bark F. rukam (300 g) was place
in bottle and extracted with organic solvents with
step gradien polarity: using n-hexane, ethyl acetate,
and methanol and placed at room temperature.
Maceration was done for 24 h and then were
filtered using paper filter.
The extraction was repeated
three times for each solvent, and extraction has been
complete. The maserate obtained was concentrated
by rotary vacuum evaporator, at temperature 55 ºC
and then air dried so that we obtained eachs crude
extract.
2.3.1 Yield Precentage of Extracts
The extraction yield precentage is the amount of
extract to obtained compared with the amount of
root plant used. Yield precentage (%) was
determined for each solvent with equations:
%Yield= Wa/ Wb 100 %
(1)
Wa = weight of crude extract
Ws = weight of sample
2.4 Analysis of Total Phenolic
Determination of the total phenolic content of each
extracts of obtained used spectrometrically
analysis to the Folin-Ciocalteu method. (Santoso et
al., 2012). The Standard gallic acid solution of
1000 µg/mL was prepared by dissolving 5 mg gallic
acid in 2 mL ethanol and the volume made up to a
volume of 5 mL with aquadest. The standard gallic
acid with a concentration series of 5, 10 , 15, and 20
µg/mL were preparated with multilevel dilution
from a standard solution of 1000 µg/mL . 100 μL of
each standard gallic acid add 1 mL of 5% Na
2
CO
3
solution. The mixture incubated for 5 min, then
added 1 mL Folin-Ciocalteu reagent 50%,
incubation to continued for 1 hour at room
temperature, then measured absorbance at λ
maxs
765
nm. The calibration curve is made through the
relationship between the concentration of gallic acid
(µg/mL) and absorbance.
The total phenolic in the sample was determined
by means of 5 mg of the each extracts were
dissolved in 2 mL ethanol and the volume made up
to a volume 5 mL with distilled water. Then each
sample 1 ml were added 1 mL sodium carbonat
solution (5%) 0.5 mL, and incubated for 5 minutes,
then add folin ciocalteu’s reagent 50%) and
incubated for 1 hour. Absorbance was recorded at
λ
maxs
765 nm used spectrofotometer UV-Vis. The
total phenolics were expressed as gallic acid
equivalents (GAE). Base on the calibration curve
total phenolic calculations used the following
formula:
Total phenolic = x Fp /
(2)
note :
c = equivalent levels of gallic acid (mg GAE / L)
v = volume of extract solution (mL)
m = mass of extract (g)
Fp = Dilution factor
2.5 Determining of Flavonoid Contents
The Determining of flavonoid contents eachs
extracts were according to the method described
(Nugroho et al., 2013). The standard concentration
of quercetin 1000 µg/mL 25 mL was prepared by
means of 0.025 g quercetin dissolved in aquadest in
a 25 mL flask. The quercetin standard was prepared
with a concentration of 50, 100, 150 and 200 µg/mL
by piping 0.5 mL; 1 mL; 1.5 mL; and 2 mL of a
Analysis of Total Phenolics and Flavonoid from the Root Bark of Flacourtia rukam
31
standard solution of quercetin 1000 µg/mL into a
100 ml volumetric flask and added distilled water.
500 µL each standard solution were added 1.5 mL
of methanol, 0.1 mL of AlCl
3
10%, 1 mL of NaNO
2
0.5 M and 2.8 mL of aquadest, then homogenized
the mixture by means of the vortex, and incubation
to continued until 30 min and followed the
addition of 1 mL of NaOH (1 M). After that
absorbance was measured at at the λ
maxs
415 nm.
The flavonoid content in the extract is
determined by means of the sample 1000 µg/mL
was prepared by means of 5 mg dissolved in
aquadest in a 5 mL flask. Sample solution (500 µL)
of different extract wereadded 1.5 ml of methanol,
0.1 mL of AlCl
3
10%, 1 mL of NaNO
2
1M and 2.8
mL of aquadest, incubating for 30 min at room
temperature and then to continued with addition of
1 mL of NaOH (1 M). As the blank using test tube
containing 2.5 mL of aquadest. The sample
containing of flavonoid was show by pink color to
the read with UV-spectrophotometrically at λ
maxs
415 nm. For the determining quantification of
flavonoid content of sampel used Quercetin
compound as the standard. This experiment with
with triplicates and the results were determined in
quercetin equivalents (QE). Flavonoid content
calculations use the following formula
Flavonoid content = x Fp /
(3)
note :
c = equivalent levels of quercetin (mg QE / L)
v = volume of extract solution (mL)
m = mass of extract (g)
Fp = Dilution factor
2.6 In vitro Antioxidant with DPPH
Method
The radical DPPH methd was used to measure
antioxidant activity ( Nataraj et al., 2013). 200 µL
the samples at various concentrations (62.5, 125,
250, 500, and 1000 µg/mL of extracts with
respective organic solvents) were taken and added
3.8 mL of a 0.05 mM. As a negative control used .
200 µL of methanol in 3.8 ml of DPPH solution.
The reaction mixtures were incubated for 30 min at
room temperature. Antioxidant activity determined
as inhibition of DPPH by the samples with reduced
content of DPPH radical characterized by decreased
absorbance. against the blank (methanol) and was
measured at λ
maxs
517 nm.
3 RESULT AND DISCUSISON
3.1 Yield Percentage
The dry powder of plant roots F. rukam (300 g) were
extracted successively using solvent with increased
polarity of n-hexane, ethyl acetate and methanol and after
concentrating the extracts of each extract were obtained.
T
he choice of maceration method has many
advantages compared to other methods. such as
procedures and tools that are used simply, do not use
heating so that the compounds contained therein will
not be damaged or decomposed, the solvents used
are also less than the other cold methods of
percolation.
The yield percentage showed in Table 1.
Each extracts after concentrating to obtained n-hexane
extract (1.101 g), ethyl acetate fraction (3.221 g) and
methanol fraction (17.701 g).
Extract yield percentage
of methanol (5.90%)
higher compared ethyl acetate
(1.07%) and n-hexane extract (0.36%).
Among the
different solvent extractions, methanol solvent found to
have higher ecovery over other.
Table 1: Yield percentage of extracts
Solvent
weight of crude
extract (g)
yield
percentage (%)
n-Hexane 1.101 0.36
Ethyl acetate 3.221 1.07
Methanol 17.701 5.90
3.2 Determining of Total Phenolic, and
Flavonoid Contents
The total phenolic contents of different extracts were
analyzed with used curva standard gallic acid. The
gallic acid standard curve with 4 series of standard
quercetin solutions in ethanol with folin ciocalteu
and sodium carbonate solution. The results are
shown in Table 2.
Table 2: Effect of concentration on the absorbance value
of gallic acid
Concentration ( µg/mL) Absorbance
0 0
5 0.226
10 0.445
15 0.739
20 1.003
The coefficient correlation of the gallic acid
standard curve based on the regression equation y
= 0,050x - 0,021 R² = 0.996, is greater than 0.98,
this shows that the curve linearity obtained is very
good. The total phenol content of each extract was
determined with standard gallic acid calibration
ICOCSTI 2019 - International Conference on Chemical Science and Technology Innovation
32
curve, were stated in mg gallic acid in each g of
extract (Mg QE/g) and presented in Table 3. In this
study, methanol extract (71.8868 mg/g) shows
higher total phenolic content compared ethyl acetate
extract (56.6094) and n-hexane extract phenolic
compound was no detection. The methanol solvent
was more effective in extracting phenolic
constituents.
Table 3: Total phenolic contents of the root of F. rukam
Extract Total phenolics (mg GAE/g
n-hexane -
Ethyl acetate 56,6094
Methanol 71,8868
Analysis of flavonoid content was determined
based on the quercetin standard curve. Standard
curve was done by reacting 4 series of standard
quercetin solutions in ethanol and the results are
shown in Table 4.
Table 4: Effect of concentration on the absorbance
valueof quercetin
Concentration ( µg/mL) Absorbance
0 0
0.5 0,032
1 0.063
2 0.138
5 0.346
Based on the regression equation, y = 0,069x -
0,002, R² = 0,999 the correlation coefficient value is
approaching 1. This shows that the curve has a good
linearity value. The flavonoid content of each
extract was determined based on the quercetin
standard curve regression equation. Flavonoid
content is expressed in mg qercetin in each gram of
extract (Mg QE/g) as shown in Table 5. This data
show, methanol extract (2.3116 mg QE/g) and
ethyl acetate extract ( 2.3304 mg QE/g) shows The
flavonoid content is not significantly different,
Meanwhile n-hexane extract shows lower
flavonoid content than other extracts. Base on this
data methanol and ethyl acetate solvent having the
same effectiveness were used to isolate flavonoid
constituents.
Phenolic and flavonoids compounds have been
know to have multiple biological effects oxidative
stress related disorders such as antioxidant,
anticancer, antidiabetic, anticholesterol, hypertence,
and anti-inflammatory properties (Amarowicz,
2007). Phenolic and flavonoid constituents of root
bark of F. rukam allegedly plays a role in the
used of this plant traditionally for the treatment of
diseases related to oxidative stress related disorders.
Table 5: Flavonoid contents of the root bark of F. rukam
Extract Flavonoid content (mg QE/g)
n-hexane 0.8129
Ethyl acetate 2.3304
Methanol 2.3116
3.3 In vitro Antioxidant Activity by
DPPH Method
The DPPH method, has been widely used for
determining the antioxidant activity of plant extracts.
The results of all extract show decrease Inhibition
percentage with decrease concentration test (Table
6) .
Table 6: The effect of concentration on % inhibition
values each extracts
concentration
(µg/ml)
Percentage Inhibition extrcts
n-hexane Ethyl
acetate
Metanol
1000 71.96 98.20 93.53
500 68.94 78.71 72.86
250 53.30 69.06 68.10
125 44.42 59.08 57.57
62.5 25.76 39.28 39.33
To determine the IC
50
value of each extracts, base
on a linear regression equation between the %
inhibition value eachs extracts and the concentration
variation. Based on the regression equation
obtained IC
50
values for n-hexane, ethyl acetate, and
methanol extract 268.02, 86.92, and 52.91 µg/mL
respectively. The IC
50
value which is getting lower,
the extract is stated to be more active. Based on this
data, the methanol extract showed higher antioxidant
activity compared to other extracts (Table 7).
Table 7.: IC
50
value eachs extracts
Extracts
IC
50
(µg/ml)
n-hexane 268.02
Ethyl acetate 86.92
Methanol 52.91
According to Molyneux (2004) extract is
categorized as active as an antioxidant if it has an
IC
50
of less than 200 µg/mL. If the IC
50
value is
found at around 200 to 1000 µg/mL in category
weak antioxidant and if above 1000 µg/mL is
categorized as in active. Base on data we conclusion
that methanol and ethyl acetate extract in category
active antioxidant and n-hexane extract category
weak antioxidant. Based on this study, the search
for antioxidant compounds from root bark of F.
Analysis of Total Phenolics and Flavonoid from the Root Bark of Flacourtia rukam
33
rukam plants can be carried out on ethyl acetate and
methanol extracts. This data also proves that the
used of F. rukam as traditional medicine for the
treatment of diseases related to degenerative
diseases can be explained by the presence contained
of antioxidant compounds found in F. rukam.
Antioxidant compounds are generally phenolic
groups which are soluble in semi-polar solvents or
polar solvents. However, the discovery of the
antioxidant properties of non-polar n-hexane fraction
is thought to be due to the presence of flavonoid
compounds extracted into n-hexane solvents.
according to the results of previous studies where in
the n-hexane extract was found to contain flavonoid
compounds. Fidrianny et al., (2014) also found
flavonoid compounds as antioxidant from n-hexane
extract Tamarindus indica L. Atioxidant activity
was also reported from the n-hexane fraction
Euphorbia tirucalli (Mawadah et al., 2016).
Antioxidant activity is proportional to the total
phenolic content and flavonoids of the extract
(Esmaeilli et al., 2015). At the tested extracts found
the significant correlation between the antioxidant
activity of extracts with value total phenolic and
flavonoid content. According to the findings, the
extract of methanol possesses a comparable
antioxidant activity to the total phenolic and
flavonoid content.
4 CONCLUSIONS
The result of the study showed that phenolic higher
in methanol extract compared with ethyl acetate
extract while n-hexane extract no detection. For
flavonoids content showed, methanol extract and
ethyl acetate extract, the flavonoid content was not
significantly different, while n-hexane extract only
contained flavonoid very less. The antioxidant
activity the methanol, and ethyl acetate extractin
category active antioxidant, while n-hexane extract
in category in weak antioxidant.
ACKNOWLEDGMENTS
The authors are thankful to ministry Ristekdikti
Republic of Indonesia, who have funded this
research through grant Basic Research superior
university periode of 2019. Thank you also to the
department of chemistry University of Sriwijaya
and Basic Laboratory of University on providing
facilities for the research work
.
REFERENCES
Crozier A, Clifford M.N., and Ashihara H., 2006. Plant
secondary metabolites: Occurrence, Structure, and
Role in the Human Diet. Lowa, Blackwell Publishing
Ltd.
Esmaeili, A.K., Rosna, M.T., Sadegh, M., and Behrooz,
B., 2015. Antioxidant activity and total phenolic and
flavonoid content of various solvent extracts from
invivo and in vitro grown Trifolium pratense L (red
clover). Biomed Research International, 643285.
Fidrianny, I., Ellis, S.T., and Rika, H., 2014. Antioxidant
compound from n-hexane extract leaves asam jawa
(Tamarindus indica L.) from Banyuresmi, Garut –
Indonesia. Acta pharmaceutica Indonesia, 39(3&4),
45-50.
Fuad, A.R., Suzi, A. Sharehan, H.A., Mahmoud, F.K.W.,
and Ismail, S., 2016. Anticancer Activity, Antioxidant
Activity, and Phenolic and Flavonoids Content of
Wild Tragopogon porrifolius Plant Extracts, Evid
Based complement Alternat Med, 9612490.
Ikram, E.H.K., Eng, K. H., Jalil, A.M.M., Islail, M., Idris,
S., Azlan, A., Nasri, H. S. M., Ditom, N.K.M., and
Mokhtar, R. A.M., 2009. Antioxidant capacity and
total phenolic content of Malaysian underutilized
fruits. Journal of Food Composition and Analysis, 22,
388–393.
Imbs T.I., Ermakova S.P., Fedoreyev S.A., Anastyuk S.D.,
and Zvyagintseva T.N., 2013. Isolationof fucoxanthin
and highly unsaturated monogalactosyldiacylglycerol
from brown alga Fucus evanescens C Agardh and in
vitro investigation of their antitumor activity, Mar
Biotechnol, 15, 606–612.
Mawadah, E.V, Arsyik, Ilizma, F.and Rolan, R., 2016.
Antioxidant activity n-heksana fraction patah tulang
(Euphorbia tirucalli), Proceedings of the 4
th
National
Pharmacy Seminar, Samarinda.
Molyneux, P., 2004. The use of the stable free radicals
diphenyl-picryl-hydrazyl (DPPH) for estimating
antioxidant activity. Songklanakarin J. Sci. Technol,
26(2), 211-219.
Mustarichie, R., Musfiroh, I., dan Levita, J., 2013.
Metode Penelitian Tanaman Obat, Teori dan
Implementasi Penelitian Tanaman untuk Pengobatan,
Widya Padjajaran, Bandung.
Muharni, Fitrya, dan Farida,S., 2016. Skrining fitokimia
aktifitas antioksidan dan antibakteri dari tumbuhan
obat tradisional etnis Musi, Balai besar obat dan jamu
kementrian kesehatan Republik Indonesia, Palembang,
Indonesia.
Muharni, elfita, Adillah, R., Yohandini, H., and Julinar.,
2018. Flavon Compound from The Ethyl Acetate
Extract of The Stem of Supit (Tetracera indica Merr.).
Molekul, 13 (1), 38 – 47.
Nataraj, L., Siddhuraju, P., and Manian,S., 2013.
Antioxidant activity and free radical scavenging
capacity of phenolic extracts from Helicteres isora L.
and Ceiba pentandra L., Journal Food Science
Technology, 50 (4), 687–695.
ICOCSTI 2019 - International Conference on Chemical Science and Technology Innovation
34
Nugroho, A E., Malik, A. and Pramono, S., 2013. Total
Phenolic and Flavonoid contents, and in vitro anti-
hypertension activity of purified extract of Indonesian
cashew leaves (Anacardium occidentale L.),
International Food Research Jounal, 20 (1), 299-305
Ragasa C.Y., Jo M.A.Y., Theresa J.T., Maria C.S., Irving
D., Robert B. and Sylvia U., 2016. Chemical
Constituents of Flacourtia rukam Zoli. & Moritzi
Fruit. International Journal of Pharmaceutical and
Clinical Research, 8(12), 1625-1628.
Sharma, G.N., 2011. Phytochemical Screening and
Estimation Total Phenolic Content in Aegle marmelos
Seeds. International Journal of Pharmaceutical and
Clinical Reseach, 2(3), 27-29.
Samsudin, M.A. dan Khoirudin., 2008. Ekstraksi, filtrasi
dan uji stabilitas zat warna dari kulit manggis
(Garcinia mangostana). Jurnal Teknik Kimia,
Fakultas Teknik, Universitas Diponegoro, Semarang,
Indonesia, Hal: (1):1-8.
Santoso, J., Anwariyah, S., Rumiantin, R.O., Putri,
A.P., Ukhty, N., and Yoshie, Y., 2012. Phenol
Content, Antioxidant Activity and Fibers profile of
Four Tropical Seagrasses from Indonesia. Journal of
Coastal Development 15 (2), 189-196.
Saree, Osman, Prince of Songkla Univ.,1998. Pattani
Campus, Pattani (Thailand). Faculty of Education.
Domonstration Schoo.l
Yustian I., Muharni, Sukarmi S., Zulaicha, and Arbi M..,
2012. Special research on the exploration of
ethnomedicine and local community medicinal plants
in Indonesia (ethnic Musi II). Palembang.
Analysis of Total Phenolics and Flavonoid from the Root Bark of Flacourtia rukam
35
