Scavenging Effects of FRC001 China
No.1 Tian Xian Liquid on Oxygen Free Radicals
Ba-Lu Zhao1 Ph.D., Wen-Juan Xin 1 Ph.D., Chung-Yu
Kao2 MD, Hong Zhang3 MD. Ph.D.
1. Institute of Biophysics, Academia Sinica, Beijing
2. FRC Free Radical Biology and Medical Research
Center, Taipei
3. Department of Pathology, Univewrsity of Linkoping,
Sweden
ABSTRACT
The transplantation sarcoma S180 and hepatic carcinoma
of mouse are the most popular and important models
in the screening of antineoplastic drugs. This paper
studied the inhibition effects of FRC001 on these
two models. The results showed that on FRC001 had
inhibition effects, to some extent, sarcoma S180
and hepatic carcinoma. Among then, the inhibition
rate of high, middle and low dose of FRC001 on S180
were 59.73%, 52.57%, 41.33% respectively which showed
obvious dose-dependent effects; FRC001 also had
some effects on hepatic carcinoma foci, and the
inhibition rate was 47.81%; after the treatment
of FRC001, the average weight decreased and the
carcinoma foci shrinked apparently compared with
the control group (P<0.05 or P<0.01). FRC001
is an antineoplastic using traditional Chinese medicine
as the main ingredient.
Key Words : FRC001; Transplantation tumor; Sarcoma
S180; Inhibition effect on hepatic carcinoma
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BACKGROUND
Malignant tumor is a series of commonly encountered
diseases which harm the human. The treatment of
it is a difficult problem of today’s world
medical science. Besides operation, radiotherapy,
chemotherapy, the roles of TCM and the combination
of Chinese and Western medicine are widely noted
by medical circles. FC001 is prepared mainly using
traditional Chinese drugs which can eliminate the
pathogenic factor and support healthy energy. The
supporting healthy energy includes invigorating
Qi and enriching the blood, warming Yang and nourishing
Yin; the eliminating the pathogenic factor includes
promoting blood circulation to remove stasis, clearing
away heat and toxic material and softening and resolving
hard mass. These methods have better inhibition
effect on tumors.
This paper studies the effects of FRC001 on transplantation
carcinoma S180 and hepatic carcinoma of mice.
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MATERIALS AND METHODS
Agents : DMPO (5.5-dimethyl-pyrroline-1-oxide)
was purchased from Sigma Chem Co. and purified by
active charcoal before use PMA (phorbol myristate
acetate), linoleic acid, lipoxidase, SOD (6500 U/mg),
xanthine/xanthine oxidase (2.125 U/ml) and luminol
were purchased from Sigma Chem Co., PMA was dissolved
in a little acetone and diluted with 50 mM phosphate
buffer to a proper concentration before use. Other
agents made in China are AR Levels. Measurement
of SOD activity included in FRC001.
BJL-chemiluminescence measurement : The reaction
of xanthine and xanthine oxidase can generate oxygen
free radicals which give a luminol-dependent chemiluminescence.
SOD can scavenge the chemiluminescence generated
from this system, so the SOD activity can be measured
with this system. The measurement system includes
0.2 mM luminol, 0.32 mM xanthine, and 0.09 U/ml
xanthine oxidase. The chemiluminescence was measured
with WDD-1 chemiluminescencemeter.
The scavenging effect of FRC001 on O2 is defined
as :
E = ((ho-hx)/ho) X 100%
Here ho is the Chemiluminescence of xanthine/xanthine
oxidase control system and hx is the chemiluminescence
of xanthine/xanthine oxidase after addition of FRC001
solution.
The measurement system was the same as above except
that different concentrations of FRC001 were added
to the system. First, a standard curve of SOD activity
was developed with this system. Then the scavenging
curve of FRC001 on oxygen free radicals was measured
in this syustem. By using both of these curves,
the SOD activity included in FRC001 solution can
be determined.
Scangenging effect of FRC001 on OH free radicals
generated from Fenton reaction.
A solution of 50 mM DMPO 1% H2O2 and 100 µM
Fe(II) as ferrous ammonium sulfate were mixed and
transferred to a quartz capillary for ESR measurement.
When the scavenging effect of FRC001 was measured,
different concentrations of FRC001 solution were
added to the system. The scavenging effect was calculated
as above but here the height of the second peak
was used for calculation. ESR conditions : All ESR
spectra were recorded at Varian E-109 ESR spectrometer.
The conditions are : microwave power 20 mW. X-band,
100 kHz modulation with amplitude 1G, central magnetic
field 3250 G, scan width 200 G, time constant 0.
128 S, room temperature.
Scavenging effect of FRC001 on . O2 generated from
irradiation of riboflavin/EDTA system.
A mixture containing 0.3 mM riboflavin, 5 mM EDTA
and 0.1 M DMPO was transferred to a quartz capillary
and put into the cavity of ESR spectrometer. After
irradiation of the sample for 20 seconds with a
xenon lamp (500 W, distance 70cm), the ESR spectra
were recorded immediately. When the scavenging effect
of FRC001 was measured, different concentrations
of FRC001 were added to the system. The scavenging
effect was calculated as above but here the height
of the first peak was used for calculation. The
ESR measurement condition was the same as above.
Measurement of scavenging effect of FRC001 on conjugated
dienes generated from lipid peroxidation of linoleic
acid by lipoxidase.
0.1 mM linoleic acid in PBS was mixed with 480
U/ml lipoxidase and measured at 232 nm with time.
When inhibition effects of FRC001 on the generation
of conjugated dienes were measured, different concentrations
of FRC001 were added into the sytem. The scavenging
effect was calculated as above, but here the h and
hx was used by reaction rate of control and sample
respectively.
Measurement rate of scavenging effect of FRC001
on TBA reacted materials (TBARM) generated from
lipid peroxidation of liposome initiated by Fe2+.
Liposome made from lecithine (10mg/ml) was peroxidized
by addition of Fe2+ (100 µM), then 95ºC
mixed with 6.7 mg/ml TBA and 0.05 M HCL. The sample
was incubated for 60 minutes at 95 C, then cooled
to room temperature. The TBARM was extracted by
butanol : methanol (85:15) and measured at 532 nm.
When the inhibition effects of FRC001 were measured,
different concentrations of FRC001 were added in
the system. The scavenging effect was calculated
as above.
Scavenging effect of FRC001 on oxygen free radicals
generated from PMA stimulated PMN
Isolation of PMN : Fresh whole blood of healthy
donor was purchased from Red Cross Blood Center
of Beijing. PMN were separated from other cellular
components by using 6% dextran sendimentation, hypersonic
lysis of remained red cells and Ficoll density gradient
centrifugation separation of mononuclear cells.
Production and measurement of active oxygen free
radicals generated from PMN stimulated with PMA
: In a typical experiment, a mixture containing
107 /ml PMN, 0.1 mM DETAPAC (diethylentriaminepentacetic
acid) and 100 ng/ml PMA was incubated for 2 minutes
at 37ºC, then 0.1 M luminal was added and mixed
homogeneously before measurement with BJL-chemiluminescence.
When the scavenging effect of FRC001 was measured,
different concentrations of FRC001 were added into
the system. The scavenging effect was calculated
as above.
Scavenging effect of FRC001 on ONOO
Peroxynitrite synthesis : Peroxynitrite was synthesized
in a quenched flow reactor [12]. Solutions of (i)
0.6 mol/L NaNO2 , and (ii) 0.6 mol/L HCL/0.7 mol/L
H2O2 were pumped at 26 ml/min into a T-junction
and mixed in a 3 mm diamter by 2.5 cm glass tube.
The acid catalyzed reaction of nitrous acid with
H2O2 to form peroxynitrous acid was quenched by
pumping 15 mol/L NaOH at the same rate into a second
T-junction at the end of the glass tube. Excess
H2O2, was removed by passage over a 1 X5 cm column
filled with 4g of granular MnO2. The suolution was
frozen at –20 ºC for as long as a week.
Peroxynitrite can oxidize luminol and give a very
strong chemiluminescence. The scavenging effect
of FRC001 on peroxynitrite was measured by chemiluminescence
method and the scavenging effect was calculated
as above.
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RESULTS AND DISCUSSION
Scavenging effects of FRC001 on oxygen free radicals
generated from xanthine/xanthine oxidase system.
A standard curve of scanvenging effect of SOD on
free radicals generated from xanthine/xanthine oxidase
was shown in Figure 1.
SOD activity (U/ml)
Figure 1. The standard curve of scavenging effect
of SOD on oxygen free radical generated from the
reaction of xanthine/xanthine oxidase system.
The scavenging effect of FRC001 on oxygen free
radicals generated from the reaction of xanthine/xanthine
oxidase system was shown in Figure 2.
Figure 2. The scavenging effect of FRC001 on oxygen
free radicals generated from xanthine/xanthine oxidase
system.
From above two curves, the SOD ACTIVITY INCLUDED
IN 1g FRC001 IS CALCULATED AND EQUAL TO 300.000
U/ml.
2.Scavenging effects of FRC001 on oxygen
free radicals generated from PMN stimulated with
PMA.
When PMN are stimulated or they are in phagocytes.,
there will be a respiratory burst and production
of active oxygen free radicals. The active oxygen
radicals produced in this process play an important
role in microbicidal and tumorcidal processes and
in protecting the healthy body from diseases. But
if there are excess active oxygen radicals in the
body, they will damage the components of cells and
even kill the normal cells and cause aging and very
serious disease, such as heart disease and cancer.
Here it was used to examine effect of FRC001 on
the oxygen free radicals. Figure 3 shows the scavenging
effect of FRC001 on oxygen free radicals generated
from PMA stimulated PMN measured by BJL-chemiluminescence.
It was determined C50=0.62 mg/ml which was smaller
than that of Vitamin C (C50=0.2 mg/ml) and bigger
than that of Vitamin E.
Figure 3. Scavenging effect of FRC001 on oxygen
free radicals generated from PMA stimulated PMN.
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3. Scavenging effect of FRC001 on ·
OH free radicals generated from Fenton’s Reaction
Fenton’s Reaction can generate · OH
and has been used for examination of scavengers
of . OH free radicals
H2O2 + Fe²+ -> · OH+OH- + Fe3+
Here it was used for examination of the scavenging
effect of FRC001 on · OH free radicals. The
ESR spectrum of DMPO-OH was shown in Figure 4b (aN=aH=14.9G).
The scavenging effect on FRC001 on · OH was
shown in Figure 5.
Figure 4. ESR spectra of DMPO spin trapped . O2
generated from irradiated riboflavin/EDTA system
(a) and . OH free radicals generated from Fenton
reaction (b).
4.The scavenging effect of FRC001 was shown in
Figure 5 FRC001 can effectively scavenge the hydroxyl
free radicals generated from Fenton Reaction but
Vitamin C just has a little scavenging effect on
the hydroxyl free radical Vitamin E only give a
scavenging effect of 37.5% at the concentration
of 5mg/ml.
Figure 5. Scavenging effect of FRC001 on ·
OH free radicals generated from Fenton reaction.
4.Scavenging effect of FRC001 on · O2 generated
from irradiated riboflavin/EDTA system.
Irradiated riboflavin/EDTA has been used for generation
of · O2- and examination of scavenger of
· O2- in photo system. Here it was used for
examining the scavenging effect of FRC001 on . O2-.
The ESR spectrum of · O2- spin adducts DMPO-OOH
generated from irradiated riboflavin was shown in
Figure 4a (aN=14.3, aHß=11.3G,aHy =1.25G).
According to the definition of the scavenging effect,
the curve of scavenging effect of FRC001 on O2-
generated from irradiated riboflavin/EDTA system
was shown in Fig 6. The concentration of FRC001
for 50% scavenging is about 17 mg/ml. It’s
scavenging effect is smaller than that of Vitamin
C (C50 = 0.0009 mg/ml) but stronger than that of
Vitamin E.
Figure 6. Scavenging effects of FRC001 on . O2 generated
from irradiated ribolfavin/EDTA system.
5.Inhibition effect of FRC001
on conjugated dienes generated from lipid peroxidation
of Linoleic acid by lipoxidase.
Conjugated dienes were generated at the
first step of lipid peroxidation, which has an absorbance
at 233nm. The inhibition effect of FRC001 on the
generation of conjugated dienes from lipid peroxidation
of linoleic acid catalyzed by lipoxidase were shown
in Figure 7. From the curves, it could be found
that the inhibition effects were increased with
the concentrations of FRC001 added in the system.
When the concentrations of FRC001 was 0.35mg/ml,
about 20% of conjuugated dienes was scavenged. When
the concentration was increased, the absorbance
at 233 nm would increase, which disturbed the determination
at high concentration.
Figure 7. Inhibition effects of FRC001 on TBARM generated from lipid peroxidation of liposome initated by Fe2+.
7.Scavenging effect of FRC001 on peroxynitrite.
Nitric oxide has many biological functions, such
as the endothelium-derived relaxing factor (EDRF),
which can relax vascular smooth cell and inhibit
platelet coagulation, and reverse messenger in neuron
transmission. Biosynthesis of nitric oxide from
L-arginine may be a pathway for the regulation of
cell function and communication. Macrophages produce
nitric oxide as part of their cytotoxic armamentarium.
On the other hand, nitric oxide, which contains
an unpaired electron, is a paramagnetic and active
frree radical, it can react with ·O2 to form
peroxynitrite anion (ONOO-). In alkaline solutions,
ONOO- is stable but has a pKa of 6.6 at 0°C
and decays rapidly once protonated, to give a species
with hydroxyl radical-like and NO2 free radicals
respectively, according to the following reaction.
O2 + NO -> ONOO- + H+ -> ONOOH -> ·
OH +NO2
Recently, it is proposed that nitric oxide reacts
with . 02- in many pathological cases to yield cytotoxic
species. The investigation of peroxynitrite has
been given much attention. Its oxidation of sulfhydryls
and membrane lipid, which cause cell toxicity and
some diseases. Here the scavenging effect of FRC001
on ONOO- was measured and it was showed in Figure
8. It can be found that FRC001 could effectively
scavenge ONOO- (C50 = 0.03 mg/ml). Its scavenging
effect on peroxynitrite is smaller than that of
Vitamin C (C50= 0.00003 mg/ml) but stronger than
that of vitamin E.
FRC001 is a drug designed on the basis of the theory of scavenging free radicals. From above experiment results, it can be found that FRC001 can effectively scavenge the oxygen free radicals generated from PMN stimulated with PMA xanthine/xanthine oxidase, irradiation riboflavin/EDTA and Fenton’s Reaction. It was also found that it could inhibit the conjugated dienes and TBA reacted materials (TBARM) formed during lipid peroxidation of linoleic acid and liposome respectively and scavenge ONOO-. These results suggest that the therapy effect of FRC001 on diseases maybe pass through the pathway of scavenging toxic oxygen free radicals in human body.
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