135135

Research Report

Dental Journal
(Majalah Kedokteran Gigi)
2015 September; 48(3): 135–138

Apoptosis of Rattus novergicus gingival fibroblasts caused by 
silver nano-particles gel exposure

Kharinna Widowati,1 Titiek Berniyanti,2 and Retno Pudji Rahayu3
1 Department of Oral Medicine, Faculty of Dentistry, Universitas Hangtuah 
2 Department of Dental Public Health, Faculty of Dental Medicine, Universitas Airlangga
3 Department of Oral Pathology and Maxillofacial, Faculty of Dental Medicine, Universitas Airlangga
Surabaya – Indonesia

abstract

Background: The use of silver nanoparticle are growing, especially in medical science. It’s used in many concentration. In dentistry, 
it’s used to decrease halitosis, periodontal diseases, and wound healing. It can affect the viability of the cells, give bad effects to the 
human’s health and environment if used in a long duration and in certain concentration. Purpose: The purpose of this study was to 
learn the apoptosis of gingival fibroblasts in Rattus novergicus which is exposed with 15 µg/ml silver nano-particle gel by the expression 
of caspase-3. Method: This study used 9 male wistar rats and were divided into 3 groups. Sample in group A were cut (hurt) in the 
oral gingiva and exposed to Ag-Np gel 15 µg/ml for 3 days. After 3 days, they were sacrificed and cut the gingival fibroblasts off 3x4 
cm size with scalpel. Samples in group B were cut in the oral gingiva and exposed to Ag-Np Gel 15 µg/ml for 5 days. After 5 days they 
were sacrificed and the gingival fibroblasts off 3 x 4 cm with a scalpel. Samples in group C were cut in the oral gingiva and exposed 
to none for 3 days then cut the gingival fibroblasts off 3 x 4 cm size with scalpel. The expressions of caspase-3 in the apoptotic and 
wound healing process were analyzed by Immunohistochemical test. This data was analyzed by using the t-test method. Result: Mean 
expression numbers of caspase-3 in the group A=5.67; group B=11.33; and group C (control)=18.67. T-test sign.number of group 
A and C=0.009; group B & C=0.000. Conclusion: The exposure of 15 µg/ml silver gel nanoparticle to gingival fibroblasts of Rattus 
novergicus reduces the expressions of caspase-3 in the day-3 and day-5 post exposure. The amounts of cell death through the apoptotic 
pathway which were analyzed by the expressions of caspase-3 will decrease too.

Keywords: apoptotic; silver; nano-particles; caspase-3

Correspondence: Kharinna Widowati, c/o: Departemen Ilmu Penyakit Mulut, Fakultas Kedokteran Gigi Universitas Hangtuah. Jl. Arif 
Rahman Hakim 150 Surabaya 60111, Indonesia. e-mail: kharinna.widowati@gmail.com

introduction

The use of silver reminds us of the luxury culture in 
Greek, Roman, and egyptian. Silver is well-known type 
of metal and ranks number third after gold and silver 
copper in those nations.1 Silvers are generally used for 
water containers and the other liquid materials to keep the 
cleanliness and sterility.2

Silver use has developed very fast for health purpose. 
The Macedonians use silver to prevent infection after 
surgery. Aside from being antiseptic, Hippocrates used the 
preparation of silver nitrate for ulcer treatments, compound 
fractures, and a good wound healing supporting material.1 

Avicenna use silver nitrate to purify blood, to prevent 
heart palpitation, and to handle respiratory diseases. In 
1880, Doctor Carl Siegmund Franz Crede, a German 
obstetrician, became the first person to use eye drops made 
from 1% silver nitrate to prevent ophthalmia neonatorium 
(gonorrheal ophthalmia) on babies.3 Anti-bacterial function 
of silver nano-particles are also utilized by the dentists as 
mouthwash therapy for periodontal diseases, to reduce 
bad breath, to help wound healing process and to prevent 
infection in tooth extraction and surgery.4

The use of silver nano-particles progresses rapidly in the 
field of nanobiotechnology; however, silver nano-particles 
also have negative consequences to human and environment 

Dental Journal (Majalah Kedokteran Gigi) p-ISSN: 1978-3728; e-ISSN: 2442-9740. Accredited No. 56/DIKTI/Kep./2012.
Open access under CC-BY-SA license. Available at http://e-journal.unair.ac.id/index.php/MKG
DOI: 10.20473/j.djmkg.v48.i3.p135-138

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136 Widowati, et al/Dent. J. (Majalah Kedokteran Gigi) 2015 September; 48(3): 135–138

for prolonged use or in uncontrollable concentration.5 

Silver particels have a nano size because they can easily 
fit into cells. Therefore, if silver nano-particles are used 
continuously with uncontrollable concentrations, they can 
lead to cells death and affect human biological system.6

Several studies have been conducted to examine the 
effect of silver nano-particles use on rats liver cells. The 
result showed that the use of silver nano-particles with 5-10 
µg/ml concentration can affect the decline of mitochondrial 
function and the integrity of liver cell membranes after 
24 hours incubation.7 The other in vitro studies, 24-48 
hours exposure of silver nano-particles with 10-25 µg/ml 
concentration on human lung cells fibroblasts can stimulate 
the release of pro-inflammatory cytokines as the oxidative 
stress level and reactive oxygen species (ROS) production 
are proliferated that can potentially damage DNA cells.8 
This implies that some information about the other effects 
caused by the use of silver nano-particles with concentration 
circulated in the market are needed so that people will be 
more vigilant in using silver nano-particles.

Based on the data above, we conducted a deeper 
research by using gingival fibroblasts cells of Rattus 
novergicus as the subject test because their tissues are 
similar to human gingival fibroblasts cells that potentially 
get exposed directly when the application process of silver 
nano-particles was done topically. The purpose of this study 
was to examine the death of Rattus novergicus gingival 
fibroblasts cells through apoptosis by analyzing caspase-3 
expression. 

materials and mthods

This study is experimental laboratory with post test 
only control group design. This study was conducted in 
the laboratory of Biochemistry and Pathology, Faculty of 
Medicine Universitas Airlangga, and Institute of Tropical 
Disease (ITD) Universitas Airlangga Surabaya.

This study used male Rattus novergicus, age 3–4 months, 
weight ± 200 grams, and declared healthy on physical 
examination by veterinarian. Materials tested were silver 
nano-particles from Aquasil brand produced by Nanonasb 
Pars Company in gel form with 15 µg/ml concentration. 
Nine Rattus novergicus were divided into three groups. 
The incision was made on each group in the anterior 

mandibular gingiva, extending from interdental gingiva of 
the mandibular central insisiv downwardly along for ≥ 5 mm 
in length and 2 mm in depth. After the incision, 15 µg/ml 
silver nano-particles gel was topically applied into group 
A as much as ± 1 ml and then was followed by suturing 
process on the wound to prevent silver nano-particles gel 
leaked out from the wound area, and decapitation on the 
day 3 after exposure process of silver nano-particles gel 
application. The same steps including slicing process, 
gel application, and suturing process are also performed 
in group B, followed by decapitation on the day 5 after 
exposure process of silver nano-particles gel application. 
The incision of group C was made without followed by the 
application process of silver nano-particles gel 15 µg/ml, 
and then continued by suturing process and decapitation on 
the day 3 after the slicing process and suturing (control). 
Decapitation control group was only given on the day 
3 because in the normal condition of healing process 
(without any supporting materials for healing process), is 
estimated that the cells death through apoptosis will appear 
24-72 hours after the incident lesion.10 For the treatment 
groups, in addition to decapitation on day 3, they were 
also given decapitation on day 5 as the healing process 
could occur faster or slower than in normal condition due 
to the silver nano-particles exposure. The examination of 
caspase-3 was conducted by using immunohistochemistry 
test, and then was observed by using light microscope with 
400x magnification. Comparative test independent t-test 
was used to examine the significant difference between 
treatment groups and control groups. 

results

Table 1 shows the results of 15 µg/ml silver nano-
particles gel exposure on caspase-3 expression of fibroblasts 
research (Table 1). The highest average of caspase-3 
expressions were found in control group. The following 
bar chart shows the mean value of caspase-3 expressions 
of fibroblasts in treatment group on the day-3, day-5 
(Figure 1).

Figure 2 shows the result of immunohistochemical 
examination. Thick and long brown colour lines pointed 
by the small arrows depict the form of fibroblast cells 
indicating caspase-3 expression. On the day-3, caspase-3 

Table 1. The mean and standard deviation of caspase-3 expression in fibroblasts on day-3 and day-5

Day-3 Day-5

Group
Group name

Mean
(x)

+ Standard 
Deviation

(SD)

p Group name
Mean

(x)

+ Standard 
Deviation

(SD)

p

Treatment A 5.67 + 0.577 0.009 B 11.33 + 0.577 0.000

Control C 18.67 + 1.155

Notes: * There are significant difference (p<0,05).

Dental Journal (Majalah Kedokteran Gigi) p-ISSN: 1978-3728; e-ISSN: 2442-9740. Accredited No. 56/DIKTI/Kep./2012.
Open access under CC-BY-SA license. Available at http://e-journal.unair.ac.id/index.php/MKG
DOI: 10.20473/j.djmkg.v48.i3.p135-138

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137137Widowati, et al/Dent. J. (Majalah Kedokteran Gigi) 2015 September; 48(3): 135–138

expression on fibroblasts of control group (C) appeared to 
be denser than of treatment group (A). Caspase-3 expression 
on fibroblasts of treatment group B (day-5) appeared to be 
denser than of treatment group A (day-3).

T-test examination was performed after the data were 
normally distributed by using Kolmogorov-Smirnov test 
and homogeneous by using Levene test. The result of the 
comparative test by using t-test on A-C groups showed 
that the number of expressions of caspase-3 in fibroblasts 
have significant difference with significance value p=0.009. 
While the result of comparative test by using t-test on B-C 
groups also have significant difference with significance 
value p=0.000 (p<0.05).

discussion

The research of 15 µg/ml silver nano-particles gel 
exposure on the expression number of caspase-3 in 
fibroblasts showed the significant difference of the 
mean value between treatment group and control group. 
Caspase-3 expressions in fibroblasts of treatment group 

and macrophage are natural immune cells triggered the 
supression of pro-inflammatory cytokines release and 
various systems such as the complement system and acute 
phase response as the increased oxidative. Macrophage 
cells as antigen presenting cell (APC) has MHC class II 
molecules. Through MHC class II, B cells will receive 
antigen, the antigen is presented to the cells surface 
to activate T helper cells which then will secrete pro-
inflammatory cytokines. The declination of mitochondrial 
function resulted by cells stress also triggers the activation 
of gene p-53 as pro-apoptosis gene in mitochondria.11 
The activation of gene p-53 followed by the inactivation 
of protein Bcl-2 and the increased production of Bax will 
affect the permeability of mitochondrial membrane that 
can release cytocrom c. The released cytocrom c will be 
bound by apoptosis activating factor (Apaf-1) and then 
will form apoptosom. Apoptosom will activate caspase 
9 (initial caspase activated by the released cytocrom C), 
caspase-9 will activate caspase-3 which acts as apoptosis 
executioner.12 The number of expressed caspase-3 indicates 
the number of cells undergoing apoptosis. Caspase 

7 
 

 

 

 

Figure 1. Bar chart of mean value of caspase-3 expressions in fibroblasts on the day-3 and day-5.  
Notes: A) treatment group on the day-3; B) treatment group on the day-5; C) control group. 

 

 

   

Figure 2. Overview of caspase 3 expression in fibroblasts of each group. Fibroblasts are shown by 
the small arrows.  

Notes: A) treatment group onthe day-3; B) treatment group on the day-5; C) control group. 
 

A B C 

Mean 

Figure 1. Bar chart of mean value of caspase-3 expressions 
in fibroblasts on the day-3 (A) and day-5 (B), and  
control (C) 

7 
 

 

 

 

Figure 1. Bar chart of mean value of caspase-3 expressions in fibroblasts on the day-3 and day-5.  
Notes: A) treatment group on the day-3; B) treatment group on the day-5; C) control group. 

 

 

   

Figure 2. Overview of caspase 3 expression in fibroblasts of each group. Fibroblasts are shown by 
the small arrows.  

Notes: A) treatment group onthe day-3; B) treatment group on the day-5; C) control group. 
 

A B C 

Mean 

Figure 2. Overview of caspase 3 expression in fibroblasts of each group. Fibroblasts are shown by the small arrows. 

Notes: A) treatment group onthe day-3; B) treatment group on the day-5; C) control group.

are lesser than of control group (0 µg/ml). The significant 
difference of caspase-3 expressions were also found 
between treatment group A (on the day-3) and B (on the 
day-5). This suggests that the exposure of 15 µg/ml silver 
nano-particles gel is able to supress the expression of 
caspase-3 in gingival fibroblasts cells that suffered injury 
of incision. Typical sign of cells undergoing apoptosis is 
the expression of caspase-3 (caspase executioner) of the 
cells. The supression of caspase-3 expression on gingival 
fibroblasts cells indicates the reduced number of cells 
undergoing apoptosis. 

exposure to 15 µg/ml silver nano-particles gel on 
injury (cuts) were able to suppress the activation of 
the innate immune response which is the beginning 
of an inflammatory mechanism in the immune cells 
activation, the complement system, the identification 
and the removal of foreign substances, as well as the 
activation of the adaptive immune system. Phagocytes 
cells such as polymorphonuclear neutrophils, monocytes, 

Dental Journal (Majalah Kedokteran Gigi) p-ISSN: 1978-3728; e-ISSN: 2442-9740. Accredited No. 56/DIKTI/Kep./2012.
Open access under CC-BY-SA license. Available at http://e-journal.unair.ac.id/index.php/MKG
DOI: 10.20473/j.djmkg.v48.i3.p135-138

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138 Widowati, et al/Dent. J. (Majalah Kedokteran Gigi) 2015 September; 48(3): 135–138

expression will appear in the next 6–9 hours ao that the 
estimated death of cells will appear 24–72 hours after 
incident lesion.10

It is concluded that the exposure of 15 µg/ml silver nano-
particles gel to gel Rattus novergicus gingival fibroblasts 
decline caspase-3 expression. This suggests that apoptosis 
of the observed cells through caspase-3 expression is also 
decreasing.

acknowledgement

Gratitude and appreciations are addressed to all staffs of 
the Laboratory of Pathology Anatomy - Faculty of Dentistry 
Airlangga University, the Laboratory of Biochemistry - 
Faculty of Medicine Airlangga University, and Institute 
of Tropical Disease Airlangga University.

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Dental Journal (Majalah Kedokteran Gigi) p-ISSN: 1978-3728; e-ISSN: 2442-9740. Accredited No. 56/DIKTI/Kep./2012.
Open access under CC-BY-SA license. Available at http://e-journal.unair.ac.id/index.php/MKG
DOI: 10.20473/j.djmkg.v48.i3.p135-138

http://e-journal.unair.ac.id/index.php/MKG
http://dx.doi.org/10.20473/j.djmkg.v48.i3.p135-138