219219

Dental Journal
(Majalah Kedokteran Gigi)
2019 December; 52(4): 219–223

Research Report

The potency of Andrographis paniculata Nees extract to increase 
the viability of monocytes following exposure to Porphyromonas 
gingivalis

Yani Corvianindya Rahayu,1 Didin Erma Indahyani,2 Sheila Dian Pradipta3 and Anis Irmawati4
1Department of Oral Biology, Faculty of Dentistry, Universitas Jember, Jember – Indonesia
2Department of Biomedical, Faculty of Dentistry, Universitas Jember, Jember – Indonesia
3Undergraduate student, Faculty of Dentistry, Universitas Jember, Jember – Indonesia
4Department of Oral Biology, Faculty of Dental Medicine, Universitas Airlangga, Surabaya – Indonesia

ABSTRACT
Background: Periodontitis is a chronic infectious disease affecting the global population. In Indonesia, the prevalence of periodontal 
disease has reached 57.6% across all age groups. The bacterium considered as the orginator factor of periodontitis is Porphyromonas 
gingivalis (P. gingivalis). Herbal ingredients are currently being promoted as a form of treatment because of the minimal side effects 
they induce. Andrographis paniculata Nees (ApN) extract produces pharmacological effects, including ones immunomodulatory in 
character, rendering possible its application as a preparation for treating periodontitis. Purpose: The purpose of the study was to 
prove the potency of Andrographis paniculata Nees extract in increasing the viability of monocytes following exposure to P. gingivalis. 
Methods: The sample was divided into four groups, namely; Control negative (C-): monocytes in the medium, not exposed to P. 
gingivalis; Control positive (C+): monocytes in the medium, exposed to P. gingivalis; Treatment I (AP25): monocytes with 25% ApN 
extract, exposed to P. gingivalis; Treatment II (AP50): monocytes with 50% ApN extract, exposed with P. gingivalis. The monocytes were 
exposed to 100 uL P. gingivalis for 4.5 hours and stained with trypan blue. Observations were conducted using an inverted microscope 
at 200x magnification. The percentage of viable monocytes was calculated based on the ratio of the number of the cells which absorbed 
trypan blue staining to that which did not. Data was tested using a one-way ANOVA followed by an LSD test. Results:  There were 
significant differences between the treatment groups in the number of viable monocytes (p=0.001) they contained. Monocyte viability 
was higher in the 25% ApN extract group than that exposed to 50% P. gingivalis. Conclusion: Andrographis paniculata Nees extract 
demonstrates the potency to increase monocyte viability following exposure to P. gingivalis.

Keywords: Andrographis paniculata Nees extract; monocytes viability; Porphyromonas gingivalis

Correspondence: Anis Irmawati, Departement of Oral Biology, Faculty of Dental Medicine, Universitas Airlangga. Jl. Mayjend. Prof. 
Dr. Moestopo no. 47 Surabaya 60132, Indonesia. E-mail: anis-m@fkg.unair.ac.id

INTRODUCTION

Periodontitis, a disease potentially causing damage to 
supporting tissues, is triggered by Porphyromonas gingivalis 
(P. gingivalis), a gram-negative anaerobic bacterium which 
can invade periodontal tissues, while evading the host’s 
defences.1,2 During chronic inflammation, P. gingivalis-
mediated periodontal disease constitutes a risk factor in 
several systemic diseases among others; diabetes, pre-term 
birth, strokes, and atherosclerotic cardiovascular disease.3 

It has major virulence factors, namely; lipopolysaccharide, 
capsule, gingipains and fimbriae.4 

During bacterial attack, lipopolysaccharide (LPS) of P. 
gingivalis stimulates an increase in monocyte levels in the 
periodontal tissues and activates monocytes in peripheral 
blood vessels. Monocytes which are not activated will 
produce free radicals through a metabolic process .5 Free 
radical production in activated monocytes increases as 
the result of phagocytosis against infection. Free radical 
production from various biological and environmental 

Dental Journal (Majalah Kedokteran Gigi) p-ISSN: 1978-3728; e-ISSN: 2442-9740. Accredited No. 32a/E/KPT/2017. 
Open access under CC-BY-SA license. Available at http://e-journal.unair.ac.id/index.php/MKG
DOI: 10.20473/j.djmkg.v52.i4.p219–223

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220 Rahayu, et al./Dent. J. (Majalah Kedokteran Gigi) 2019 December; 52(4): 219–223

Table 1. The different monocyte viability test results for all 
groups produced by a one-way ANOVA test

Groups Mean ± SD one-way ANOVA (p)

C- 73.5 ± 2.38

0.0001
C+ 64.25 ± 2.36

AP25 82.75 ± 2.62

AP50 96 ± 2.16

Table 2. The different monocyte viability results for groups 
produced by a LSD test

Treatment groups C- C+ AP25 AP50

C- .004 .003 .000

C+ .000 .000

AP25 .000

AP50

sources is caused by an imbalance of natural antioxidants 
which leads to various disease-associated inflammation.6 

The effect of oxidative stress and its associated factors are 
an important problem within human health. Endogenous 
enzymatic and non-enzymatic antioxidant substances are 
incapable of coping with the overload of reactive oxygen 
species (ROS) which leads to imbalances within the 
process, cell damage, and health problems.7 Therefore, in 
this case, the body requires external antioxidants, referred 
to as exogenous antioxidants, to increase monocytes 
viability.8

Andrographis paniculata Nees (ApN), commonly 
known as the “king of bitters,” is an herbaceous plant 
which includes the Acanthaceae family found in all 
regions of tropical and subtropical Asia and Southeast 
Asia. In Indonesia, most people refer to it as sambiloto 
(Java) to. The Andrographolide contained in ApN 
exhibits immunostimulatory, antiviral, and antibacterial 
pharmacological properties.9,10 The purpose of this research 
was to prove the potency of ApN extract to increase 
monocytes viability after exposure to P. gingivalis.

MATERIALS AND METHODS

This study was approved by the Ethical Committee, 
University of Jember (Permit Number: 000651/KKEP/
FKG-UGM/EC/2016). P. gingivalis strain ATCC 33277 
was supplied by the Department of Microbiology, Faculty 
of Dental Medicine, Universitas Jember (Identification 
number: 0970Mikro/S. Ket/2016). 

ApN powder was obtained from Materia Medica, Batu, 
East Java, Indonesia which had utilized the following 
extraction process. First, n 400 g of ApN leaf powder 
was moistened with 96% ethanol solvent until 2,000 ml 
of solution was obtained. The jar containing it was closed 
for 48 hours and agitated in a digital shaker at 50 rpm. The 
liquid extract was subsequently filtered and placed in an 
erlenmeyer flask. Remaseration was performed twice with 
1,000 ml of 96% ethanol before being soaked overnight 
in a shaker. Finally, the liquid extract was evaporated in a 
rotary evaporator for 2.5 hours.

Monocytes were isolated by collecting 9cc of blood 
using 1 mM ethylene diamine tetraacetic acid (EDTA) as an 
anticoagulant. The blood, all solutions, and equipment were 
conditioned at 4°C prior to use and agitated gently before 

extraction of an aliquot. Iodixanol working solution (WS) 
at 40% (w/v) concentration was prepared with OptiPrep 4 
vol of diluted with 2 vol of diluent (Axis-Shield Density 
Gradient Media, USA). This solution had a density of 
approximately 1.217 g/ml. 1.072 g/ml-1.074 g/ml density 
barrier solution was prepared by WS diluted with 2.14 
ml + 5 ml and 2.27 + 5 ml diluent, respectively. 4.24 ml 
of WS was mixed with 10 ml of whole blood (WB) in a 
15 ml centrifuge tube; 5 ml of one of the density barrier 
solutions over 5 ml of the blood, and then layered with 
0.5 ml of diluents (WS mix WB) on top. The solution was 
centrifuged at 700g in a swinging-bucket rotator for 30 
minutes at 4°C. 100 µl of mononuclear cells was pipetted 
onto the microplate, suspended again with 1000 µl RPMI 
media, and then added to 20 µl fungizon.11 The P. gingivalis 
used was P. gingivalis ATCC 33277 at a concentration of 
106 which was measured by densicheck until a density of 
0.5 McFarland was achieved.

In the subsequent stage, monocytes were divided into 
four groups. Control negative (C-): monocytes not exposed 
to P. gingivalis; Control positive (C+): monocytes exposed 
to P. gingivalis; Treatment I (AP25): monocytes with 25% 
ApN extract and exposed to P. gingivalis; and, Treatment 
II (AP50): monocytes with 50% ApN extract and exposed 
to P. gingivalis.

A 0.4% trypan blue exclusion test was conducted 
to determine monocyte viability. Monocytes that did 
not absorb trypan blue staining were counted as viable. 
The percentage of monocytes viability was calculated 
by dividing the number of viable monocyte cells by the 
total number of monocyte cells and multiplying the result 
by 100%. The data produced was subsequently tested 
statistically using IBM with SPSS 20.0 software. A one-
way analysis of variance (ANOVA) and a LSD test were 
administered for pairwise comparison with a significance 
of 0.05. 

RESULTS

The results of data analysis can be observed in Table 
1 indicated that significant differences existed in all 
experimental groups. The results of data analysis contained 
in Table 2 revealed that 25% of the ApN extract group 
(AP25) had a significant difference compared to the 
negative control group (C-), positive control group (C+), 

Dental Journal (Majalah Kedokteran Gigi) p-ISSN: 1978-3728; e-ISSN: 2442-9740. Accredited No. 32a/E/KPT/2017. 
Open access under CC-BY-SA license. Available at http://e-journal.unair.ac.id/index.php/MKG
DOI: 10.20473/j.djmkg.v52.i3.p219–223

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221Rahayu, et al./Dent. J. (Majalah Kedokteran Gigi) 2019 December; 52(4): 219–223

 

 

 

         

          

A       B  

C       D 
Figure 1. Monocytes viability counted using an inverted microscope (200x) and trypan blue staining. Viable monocytes are light-colored 

(red arrows), while unviable monocytes are dark-colored (purple arrows). Monocytes viability in C- group (A), C+ group 
(B), AP25 group (C), and AP50 group (D). In the AP50 group, monocyte viability was higher than in the other groups.

and 50% ApN extract group (AP50). The 50% ApN extract 
group (AP50) had a significant difference compared to the 
negative control group (C-), positive control group (C+), 
and 25% ApN extract (AP25) group.

Figure 1 contains images of monocyte viability counted 
by means of an inverted microscope (200x) and trypan blue 
staining. Viable monocytes were light-colored (red arrows), 
while unviable monocytes were dark-colored (purple 
arrows). Monocyte viability was highest in the AP50 group 
compared to the other groups (light-colored).

DISCUSSION

The overall results of this research indicated that the presence 
of ApN leaf extract induced a higher increase in monocyte 
viability in the treatment group compared to the control 
group. Based on the contents of Table 1, the results of this 
study showed that there were significant differences in all 
experimental groups. ApN is an effective antiinflammatory 
and a correlation existed between increasing the extract 
dose and a more potent anti-inflammatory effect. The 
positive control group had the lowest average monocyte 
viability of all the groups due to the virulence factors of P. 
gingivalis, i.e. LPS, fimbria, and gingipain.4

The LPS in P. gingivalis induced an increase in the 
superoxide and nitric oxides contained in monocytes. Nitric 
oxide in the form of gas molecules constitutes another 
reactive species of ROS which is toxic.12 The imbalance 
between free radical production and antioxidant defenses 
leads to an oxidative stress causing lipid peroxidation of cell 

membranes. The presence of excessive lipid peroxidation 
causes damage to cell membranes precipitating lysis in the 
monocytes. LPS acts as protypical endotoxin which binds 
CD14/TLR-4, a complex receptor in different types of cells, 
especially monocytes. Binding of CD14 by LPS results in 
the release of proinflammatory cytokines, namely; IL-1α, 
IL-1β, IL-16, TNF-α and lipid inflammatory prostalglandins 
E2 (PGE2) mediators. 

13

During the inflamatory process, inflammatory cells 
produce inflammatory mediators such as arachidonic acid 
and chemokines that demonstrate higher solubility. Both 
of these inflammatory mediators will work by activating 
inflammatory cells in the   infection site and releasing more 
reactive species. Certain markers, in addition to being 
capable of stimulating signal transduction cascade, can also 
cause changes in transcription factors, including; nuclear 
factor kappa B (NF-κB), signal transducers and activators 
in transcription 3, NF-E2 related factor-2, nuclear factor in 
activated T cells (NFAT), and hypoxia-inducible factor-
1α (HIF1-α), which mediate cellular stress reactions. The 
subsequent stage is the initiation of cyclooxygenase-2 
(COX-2), inducing of nitric oxide synthase (iNOS), and 
high expression of inflammatory cytokines, including tumor 
necrosis factor-α (TNF-α), interleukin-1β (IL-1β), IL-6, and 
chemokines.14–16 However, if the number of inflammatory 
mediators in monocytes is excessive, tissue damage may 
ensue commencing with cell lysis.17

Gingipain in P. gingivalis degrades CD14 receptors 
which causes the hyper-responsiveness of monocytes to 
bacterial infection.18 Gingipain in P. gingivalis manipulates 
host molecules proactively by intervening in cross-talk 

Dental Journal (Majalah Kedokteran Gigi) p-ISSN: 1978-3728; e-ISSN: 2442-9740. Accredited No. 32a/E/KPT/2017. 
Open access under CC-BY-SA license. Available at http://e-journal.unair.ac.id/index.php/MKG
DOI: 10.20473/j.djmkg.v52.i4.p219–223

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222 Rahayu, et al./Dent. J. (Majalah Kedokteran Gigi) 2019 December; 52(4): 219–223

between C5a receptors and TLR signaling to avoid bacterial 
clearance. In-vitro studies have indicated that gingipain 
plays a role in the regulation of inflammatory mediators in a 
number host cells, including IL-1α, IL-1β, and IL-18.19 The 
excessive amount of inflammatory mediators in monocytes 
causes tissue damage which leads to lysis.20

Anti-inflammatory activity of andrographolide has 
been studied using a number of in vivo and in vitro 
experimental paradigms, including human whole genome 
DNA microarrays. The most common anti-inflammatory 
and immunomodulatoy activities of andrographolide are 
barriers to mitogen-activated protein kinase/extracellular 
signal (MAPK/ERK) or regulated kinase signalling 
(specifically p38 MAPK/ERK1/2) and final transcription 
factors such as nuclear factor kappa B (NF-κB) and nuclear 
factor of activated T cells (NFAT).21 Inflammation is a 
complex interaction between organisms and pathogens 
which induces macrophage activation and secretion of pro-
inflammatory cytokines, such as TNF-α, IL-1β, and IL-6, as 
the body’s immune system response. Research previously 
conducted confirmed that LPS is a powerful inflammatory 
trigger capable of stimulating macrophages to synthesize 
TNF-α, IL-1β, and IL-6.22

As indicated by the contents of Table 2, this study showed 
that the AP25 and AP50 groups had a significant difference 
to C- and C+ group, while AP25 also demonstrated a 
significant difference to AP50. It was suspected that the 
active ingredients in ApN leaves are andrographolide 
and flavonoids capable of suppressing the inflammatory 
process. Flavonoids contained in the ApN leaves extract act 
as antioxidants which inhibit the formation of free radical 
reactions (peroxide) during lipid oxidation by donating one 
or more electrons to free radicals causing them to become 
muted. Antioxidants delay or prevent the formation of 
free radical reactions (peroxide) in the lipid oxidation.23 
In vitro studies have confirmed that flavonoids are strong 
inhibitors of lipid peroxidation, as traps of ROS or reactive 
nitrogen, and are also able to inhibit cyclooxygenase and 
lipooxygenase enzyme activity.24 Flavonoids derived from 
polyphenols can inhibit the oxidation reaction through a 
radical arrest mechanism (radical scavenging) by donating 
an electron to the unpaired electrons in free radicals causing a 
reduction in their number.23 Flavonoids significantly inhibit 
the protease activity of Porphyromonas gingivalis gingipain 
depending on the size of the dose administered.24

Monocyte viability of the AP25 group was higher 
compared to the C- and C+ groups. The AP50 group 
demonstrated the highest level of monocyte viability. 
The results of this study are compatible with those of the 
research conducted by Chandrasekaran (2011) which found 
that andrographolide is the main active component of 
Andrographis paniculate which provides anti-inflammatory 
effects by inhibiting the activation of the NF-κB/MAPK 
signaling pathway and inducing pro-inflammatory 
cytokines. Andrographolide can inhibit the expression of 
iNOS through LPS, which is activated by macrophages and 
prostaglandin E2 (PGE2) production.25

ApN can suppress isoform iNOS and COX-2 and 
decrease nitric oxide and the production of PGE2.14 

Andrographolide reduces the expression and production of 
pro-inflammatory cytokines (IL-1α, IL-6, TNF-α) and pro-
inflammatory mediators PGE2-stimulated by LPS, while 
also reducing the production of superoxide anion radicals 
and hydrogen peroxide.13 It was concluded that ApN extract 
is highly effective in increasing monocyte viability after 
exposure to P. gingivalis. 

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Dental Journal (Majalah Kedokteran Gigi) p-ISSN: 1978-3728; e-ISSN: 2442-9740. Accredited No. 32a/E/KPT/2017. 
Open access under CC-BY-SA license. Available at http://e-journal.unair.ac.id/index.php/MKG
DOI: 10.20473/j.djmkg.v52.i4.p219–223

http://e-journal.unair.ac.id/index.php/MKG
http://dx.doi.org/10.20473/j.djmkg.v52.i4.p219-223