Vol 20 No 2 Page 56-61 July 2020 

Mutiara Medika: Jurnal Kedokteran dan Kesehatan 
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Suweg Flour (Amorphophallus campanulatus) Potential 
Reducing TNF-α Levels in Model Diabetic Rats 

 
Ika Setyawati1* 
1 Department of Biochemistry, School of Medicine, Faculty of Medicine and Health Sciences, Universitas Muhammadiyah 
Yogyakarta, Jl Brawijaya, Tamantirto, Kasihan, Bantul, Yogyakarta, Indonesia 

 
DATA OF ARTICLE: Abstract: Diabetes mellitus is a disease characterized by hyperglycemia. Chronic 

Received: 05 Feb 2020 hyperglycemia increases reactive oxygen species (ROS) synthesis. Oxidative stress on 

Reviewed: 10 Mar 2020 fat, muscle, and liver tissue leading to insulin resistance. Insulin resistance produces 
Revised: 24 May 2020 several oxidative stress mediators such as tumor necrosis factor-alpha (TNF-α). This 
Accepted: 03 Jun 2020 

 
*CORRESPONDENCE: 
ikasetyawati.dr@umy.ac.id  

study aims to determine the effect of suweg flour (Amorphophallus campanulatus) on 

TNF-α levels in diabetic rats. This type of research is a laboratory experimental design 
with a pre-post test control group. The research subjects were 25 Rattus norvegicus 

Wistar strains divided into 5 groups, namely normal control, positive control 

DOI: 
10.18196/mm.200246 

(untreated), standard (Glibenclamide 0.09 mg/200 KgBW/day), and treatment 

groups (Suweg Flour 1.25 and 2.50 g/day). The treatment was given for 28 days. Data 

were obtained by measuring TNF-α levels using ELISA and then analyzed using 
TYPE OF ARTICLE: Paired t-test, Anova and Tuckey Post Hoc Test. The result showed that there were 

Research significant differences before and after treatment (p <0.001); there were significant 

 differences between all groups (p<0.001); P Suweg Flour 2.50 - 1.25 < 0.001; P Suweg Flour 2.50 – standard 

= 0.002. It can be concluded that Suweg flour can reduce TNF-α in diabetic mice but 

 it is still lower than standard treatment. 

Keywords: Amorphophallus campanulatus; TNF-; Diabetes mellitus 

 
Abstrak: Diabetes melitus merupakan penyakit yang ditandai dengan hiperglikemia. 

 Hiperglikemia kronis meningkatkan sintesis spesies oksigen reaktif (ROS). Stres oksidatif pada 

 lemak, otot, dan jaringan hati yang menyebabkan resistensi insulin. Resistensi insulin 

menghasilkan beberapa mediator stres oksidatif seperti tumor necrosis factor -alpha (TNF-α). 

 Penelitian ini bertujuan untuk mengetahui pengaruh tepung suweg (Amorphophallus 

campanulatus)   terhadap   kadar   TNF-α   pada   tikus   diabetes.   Jenis   penelitian   adalah 
 eksperimental laboratoris dengan pre-post control group. Subjek penelitian adalah 25 strain 
 Rattus norvegicus Wistar yang terbagi dalam 5 kelompok yaitu kontrol normal, kontrol positif 
 (tanpa  perlakuan),  standar  (Glibenclamide  0.09  mg/200  KgBB/hari),  dan  kelompok 
 perlakuan (Tepung Suweg 1.25 dan 2.50 g/hari). Perlakuan diberikan selama 28 hari. Data 

 diperoleh  dengan  mengukur   kadar  TNF-α   menggunakan  ELISA  kemudian  dianalisis 
 menggunakan   sample   paired   t-test   Anova   dan   Post   Hoc   Tuckey.   Hasil   penelitian 
 menunjukkan ada perbedaan bermakna sebelum dan sesudah perlakuan (p <0,001); ada 
 perbedaan signifikan antara semua kelompok (p <0.001). Nilai P tepung Suweg 2.50 - 1.25 <0.001; P 

 tepung Suweg 2,50 - standar = 0.002. Dapat disimpulkan bahwa tepung suweg dapat menurunkan TNF- 

α pada mencit diabetes namun masih lebih rendah daripada perlakuan standar. 
Kata Kunci: Amorphophallus campanulatus; TNF-α; Diabetes mellitus 

 
 

INTRODUCTION 
 

Diabetes mellitus (DM) is a group of non- 
communicable and chronic diseases. This disease is 

 

often found throughout the world and the number 
of this case is predicted to increase over time. 
According to the International Diabetes Federation 
(IDF) in 2019, the diabetics were estimated at 9.3% 

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Vol 20 No 2 
July 2020 

58 | 

 

 

 
(463 million people) increased to 10.2% (578 million 

people) in 2030 and 10.9% (700 million people) in 
2045.1,2 The prevalence of Diabetes Mellitus in the 
world in 2014 was 8.5% with 424 million survivors and 
it was expected to increase over time.3 

Diabetes Mellitus is a metabolic disease 
characterized by hyperglycemia (increased blood 
glucose levels) due to abnormal insulin secretion, 
insulin action, or both. Diabetes Mellitus can cause 
complications such as microvascular and 
macrovascular complications including coronary 
artery disease and peripheral arterial disease.4,5 

Diabetes Mellitus is an inflammatory disease 
caused by the increase of serum cytokine levels such 
as IL-6 IL-18, IL-1, and TNF-α.6 Additionally, 
Hyperglycaemia leads to induct oxidative stress of 
increase the production of ROS, promote lipid 
peroxidation, loss of function of different cell types 
such as renal cells.7 Hyperglycaemia and Oxidative 
stress activate the immune system and create an 
inflammatory medium by the activation of the 
nuclear transcription factors-kappa B (NF-kB), and 
release of inflammatory cytokines (TNF-α).8 

Hyperglycemia causes an increase of Reactive 
Oxygen Species (ROS) synthesis.9 It causes oxidative 
stress, which imbalance between the oxidative and 
antioxidative systems of cells and tissues. Oxidative 
stress is a major damaging factor as a cause of Insulin 
Resistance, Dyslipidemia, Pancreatic β-cell 
dysfunction, impaired glucose tolerance and triggers 
type 2 Diabetes Mellitus.10 

Insulin resistance due to the compensatory 
work function of excessive pancreatic beta cells 
correlates significantly with elevated levels of TNF-α. 
Tumor necrosis factor-α is an adipocytokine which 
involved in systemic inflammation secreted by 
macrophages and the other cells include adipocytes. 
Moreover, tumor necrosis factor-α inhibits Insulin 
transduction and affects glucose metabolism. It will 
affect the emergence of DM if TNF-α metabolism is 
disturbed.11,12,13 

Many compounds can react to ROS that 
occurs in cells and reduce levels of these 
compounds. One molecule that is considered as an 
effective reduction of ROS levels is antioxidants such 
as suweg.14 Therefore, food intake management is a 
key factor that can be modified for caring for the 
DM. 

 

MATERIALS AND METHOD 
 

The subjects and materials were 25 wistars, 
gloves, scales, microtube, test tube racks, 
microhematocrit pipettes, timers, labels, and 
spectrophotometers. Suweg is mixed into the flour 
with a disk mill machine and grinding at 1500 rpm 

with 80 mesh filter. One kilogram of suweg can 
produce 300-350 grams of flour.15,16 

Blood samples from orbital veins are put into 
a tube to be processed into the serum. The tube 
containing the complete blood samples was placed 
on the tube rack and let stand for approximately one 
hour at room temperature until the blood clots. The 
blood must be clotted before it was centrifuged to 
avoid hemolysis and the tubes must be centrifuged 
at 3000 rpm for 10 minutes to obtain the serum. 
These samples used for estimating the TNF-α levels 
of estimation was measured by a biochemical 
analyzer using an enzyme-linked immunosorbent 
assay (ELISA) at the pretest and posttest of the 
study with Fine Test ELISA kit (Catalog number: 
ER1393). Blood glucose levels were measured using 
the GOD-PAP (Glucose Oxidase-Peroxidase 
Aminoantypirin) method with Dyasis Kit reagen. 

This study used 25 male white rats (Rattus 
norvegicus) aged between 2 - 3 months with ± 150- 
200 g of weight and physical health as the sample. 
The exclusion criteria were rats that showed a 
decrease in the physical condition during the 
adaptation phase. The rats were adapted for 7 days 
at Gedung Pusat Antar Universitas (PAU) 
Laboratorium Pusat Studi Pangan dan Gizi 
Universitas Gajah Mada with adequate feeding with 
standard pellet rats diet, drinking, and lighting at 
room temperature. 

This research used experimental laboratory 
design by using a pre-post test control group. The 
subjects were 25 white male rats (Rattus norvegicus) 
taken by stratified random sampling and observed in 
28 days. The independent variable in this research 
was suweg flour of various concentrations. The 
dependent variable was the TNF-α level. The 
controlled variable was a trial animal with the same 
strain, sex, weight, age, feed, and individual cage. 

Streptozotocin and NA induction were 
conducted by injecting the intraperitoneal STZ 45 
mg/KGB and NA 110 mg/KGB in 7 or 8 days after the 
adaptation phase to induct the male rats (Rattus 
norvegicus) that damaged the pancreatic cell-β. The 
main characteristic of diabetic rats was the 
extension of hyperglycemia with blood glucose >160 
mg/dL rate. The rats were tested for hyperglycemia 
by measuring their blood glucose concentration in 3 
and 7 days following the STZ and NA injections.17,18 

This research involved 25 rats were divided 
into 5 groups (n = 5) consisting of P1= normal control, 
P2 = positive control, P3 = standard (diabetic rats + 
glibenclamide 0.09 mg/200 KgBW/day), P4 = 
treatment 1 (diabetic rats + suweg flour 1.25 g/day), 
and P5 = treatment 2 (diabetic rats + suweg flour 2.50 
g/day). The treatment is given orally in a daily dose 
for 28 days. Previous research with dosage of boiled 



| 59 

 

 

 
and raw suweg tubers is 10 mg/180 g BW/day (1800 
mg/day) 19 and suspension of suweg tuber powder 
(360, 729 and 1440 mg/KgBW).20 

The data was analyzed using SPSS 15 for 
Windows. Data distribution was priorly determined 
using the Shapiro-Wilk test. Tumor necrosis factor-α 
(TNF-α) level was analyzed by paired sample t-test. 

This study was approved by the Health 
Research Ethics Committee with number of 148/EC- 
KEPK FKIK UMY/V/2019. 

 

RESULT 
 

Research subjects were diabetic rats induced 
by STZ and NA. Diabetic rats can be identified by 
testing blood glucose levels on 3rd day after 
induction (Table 1). 

This research showed a significant difference 
of TNF-α level between pre-treatment and post- 
treatment by Suweg flour in rats diabetic model 
(Table 2). The average of TNF-α decrease is shown in 
Table 3. Table 3 shows an increase in TNF-α in the 
Normal control and Positive control groups, while 
the Standard and Treatment groups with Suweg 
flour showed a decrease in TNF-α. 

 
Table I. The Average of Blood Glucose Levels Pre 

  Treatment  
 

 
Group 

Average Level of Blood 
Glucose (mg/dL) 

 Normal control 63.89* 
 Positive control 265.03# 
 Standard 261.61# 

 Suweg flour 1.25 260.00# 
 Suweg flour 2.50 258.59# 

*Normal rats 
#Diabetic rats 

 

Table 2 Paired T-test for TNF-α Levels in Diabetic 
  Rats in All Study Groups  

 
Group 

Average level of TNF- 

  (pg/mL)  SD  
 

P value 
 Pretest Posttest  

Normal control 6.07 ± 0.22 6.33 ± 0.16 0.025 

Positive control 14.89 ± 0.52 15.17 ± 0.47 0.010 

Standard 15.06 ± 0.59 7.81 ± 0.47 <0.001 

Suweg flour 1.25 14.58 ± 0.51 11.54 ± 0.40 <0.001 

Suweg flour 2.5 14.85 ± 

                                     0.69  

8.86 ± 0.22 <0.001 

Table 3. The Average of TNF-α Decrease Post 
  Treatment in All Study Group  

Group 
Decrease in TNF- 

(pg/mL) 

Normal control -0.26 
Positive control -0.28 
Standard 7.25 
Suweg flour 1.25 2.96 
Suweg flour 2.50 5.99 

 

This study also tested the significance of the 
differences between P3 (Standard), P4 (1.25 g / day), 
and P5 (2.50 g / day) groups using One Way ANOVA. 
Previously, the data abnormality test using Saphiro 
Wilk showing that the data were normally 
distributed (Table 4). One Way ANOVA test showed 
that there were significant differences among the 
three groups (p <0.001). Furthermore, the Post Hoc 
of Tuckey Test was conducted to determine how 
significant the differences between groups were. 
The test results are shown in Table 5. 

 

Table 4. Shapiro Wilk Test on the Average of TNF-α 
  Level of All Study Groups  

 

Group 
P value 

Pre-test Post-test 

Normal control 0.988 0.794 

Positive control 0.914 0.354 
Standard 0.287 0.855 
Suweg flour 1.25 0.301 0.373 
Suweg flour 2.5 0.095 0.894 

 
Table 5. Post Hoc Test Results on TNF-α Post 

Treatment   between   Group   of   Standart, 
  Suweg Flour 1.25 and Suweg Flour 2.50  

 

 

Group 
 

Group 
Mean 

Difference 
p value 

Standart Suweg 
Flour 1.25 

-3.72400* <0.001 

 Suweg 
                                       Flour 2.50  

-1.05000* 0.002 

Suweg 
Flour 1.25 

Standart 3.72400* <0.001 

 Suweg 
                                       Flour 2.50  

2.67400* <0.001 

Suweg 
Flour 2.50 

Standart 1.05000* 0.002 

 Suweg 
                                        Flour 1.25  

-2.67400* <0.001 

* significant (p<0.05) 
 

Table 5 shows that among the three groups, 
namely standard, suweg flour 1.25 and suweg flour 
2.50, there was a significant difference in the 
decrease in TNF-α post treatment. However, it 
appears that the P value between standard - suweg 
flour 2.5 groups is greater (0.002) than between 



Vol 20 No 2 
July 2020 

60 | 

 

 

 
standard - suweg flour 1.25 (<0.001). Meanwhile, the 
p value between Suweg flour 1.25 - Suweg flour 2.5 
was the same as the p value between standard - 
Suweg flour 1.25 (p <0.001). This means that suweg 
flour 2.5 has the ability to reduce TNF-α significantly 
greater than Suweg flour 1.25, although it is still 
below the ability of standard treatment (p = 0.002). 

 

DISCUSSION 
 

The average score of decrease in TNF-α 
between the pre-test and post-test of the tested 
group was showed by P5. It means this test showed 
a good effect in reducing levels more than the P4 
group. Also, this test showed that the more total of 
flour supplied, the lower the TNF-α level (Table 3). 
Then, the P3 group showed that the use of 
glibenclamide was better than the suweg flour in the 
treatment group. Moreover, the glibenclamide was 
one of the choices of the antidiabetic drugs used for 
people with DM. This P3 is tested as a reference and 
comparison of the standardized research method. 

The average of post-test TNF-α levels was 
significantly different (p<0.001) with the One Way 
ANOVA test. Post Hoc test showed that Suweg Flour 
2.50 reduced TNF-α significantly greater than Suweg 
Flour 1.25 but still below the standard significantly. 

The previous research showed that suweg 
has antioxidants that can reduce oxidative stress in 
in-vitro studies and has radical scavenging activity 
which is associated with high phenolic and flavonoid 
antioxidants.18 This potential activity is shown by 
the ability of potential protein donors to inhibit free 
radicals or scavengers. Both phenolic and flavonoid 
have antidiabetic properties and inhibit the fat 
peroxidation chain and preventing secondary 
complications of DM.21,22 

The Phenolics control DM by inhibiting the 
enzymes α-amylase and α-glucosidase which are 
involved in hyperglycemia.21 The enzyme inhibition 
caused the decrease of blood glucose level and 
affected ROS decrease. Whereas, Flavonoids can 
regenerate pancreatic β cells and stimulate insulin 
secretion.23 Therefore, the blood glucose level can be 
decreased by regenerated pancreatic cells of insulin 
secretion. 

Based on other studies related to the 
antioxidant activity test of methanol extract suweg 
which was conducted by in vitro test, methanol 
extract suweg showed potent antioxidant activity.24 
Besides, Antioxidants can protect biomolecules from 
the ROS effect by reducing oxidative stress 
conditions in cells characterized by one of TNF-α 
decreasing levels.25 Antioxidants will downregulate 
NF-kB as a master regulator of inflammation so the 
level of TNF-α will be decreased. 

Tumor necrosis factor-alpha post-test level in 
P2 was increased compared to TNF-α pre-test level. 
It caused by P2 of diabetes mellitus group without 
suweg flour treatment where insulin deficiency or 
insulin resistance occurs in DM conditions. Thus, the 
first proinflammatory cytokine production is TNF-α 
which is reported as reducing insulin-regulated 
glucose transporter type 4 (GLUT4). It was found in 
adipocytes, skeletal muscle and heart muscle.24, 26 

 

Acknowledgement 
This research was supported by Research, 

Publication and Community Service Institute of 
Universitas Muhammadiyah Yogyakarta. 

 

CONCLUSION 
It can be concluded that suweg flour 

(Amorphophallus campanulatus) can reduce TNF-α in 
diabetic mice but it is still lower than standard 
treatment. 

 
 

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