Hye-Jung Park1, Moon-Moo Kim2. 1. Department of Chemistry and Biology, Dong-Eui University, Busan, Republic of Korea. 2. Department of Applied Chemistry, Dong-Eui University, Busan, Republic of Korea. Electronic Address:mmkim@deu.ac.kr.
Amentoflavone used in the study is mainly contained
in Selaginella tamariscina to have a hemostatic effect,
anti-inflammatory and anti-cancer effect (1). Selaginella
tamariscina has been used as an anti-cancer agent and
contains many different compounds such as biflavonoids
(2) which are widely present in vascular plants and have
a variety of physiological activities (3, 4). Amentoflavone
is a dimer composed of apigenin that has the capability to
promote the cell cycle arrest and induction of apoptosis
through the p53-related pathway as well as the induction
of autophagy in several human cancer cell lines (5).
However, the role of amentoflavone in the mechanism of
the induction of autophagy remains unclear.Anti-aging studies have focused on manipulation of
genes involved in histone acetylation, Insulin-like growth
factor-1 (IGF-1) pathway, and p53 system to suppress
the senescence as a mean to extend the lifespan of the
mammalian model (6, 7). However, the efforts increasing
longevity in complex animal models do not have a
sufficient understanding of the life mechanism. On the
other hand, p53, a tumor suppressor protein, is closely
related to aging as well as the induction of autophagy
and apoptosis. In particular, the activated IGF-1 signaling
is involved in the senescence and cell growth via p53
protein dependently. The short-term of IGF-1 treatment
promotes the cell growth by up-regulating PI3K/AKT
pathway through IGF1R against p53 protein. In contrast,
the long-term IGF-1 treatment induces the senescence and
is also very closely related to the development of cancer,
depending on the concentration of the p53 protein that is
as a substrate for SIRT1, a histone deacetylase, resulting
in the inhibition of cell aging caused by long-term IGF-1
treatment (8, 9).In recent years, resveratrol or spermidine, calorie
restriction, and rapamycin have been reported to
induce autophagy associated with longevity (10).
Therefore, it is important to study the relationship and
the mechanism of senescence related to IGF-1, p53,
and HAT/SIRT1 pathway associated with the induction
of autophagy to remove the cellular wastes such as
organelles and macromolecules damaged by internal
and external stimuli. In addition, the previous study
reported that there is substantial evidence supporting
the roles of autophagy in megakaryopoiesis. The
engagement of transcription factors, cytokines,
and extracellular stress synergically promotes the
maturation of megakaryocytes (11). Transcription
factors, such as SCL, GATA1, GATA2, and NF-E2
allow the development of megakaryocyte/erythroid
progenitor cells (12). The abrogation of autophagy
from stem cell stage by hematopoietic knockout
of ATG7 leads to impaired megakaryopoiesis, the
loss of autophagy caused mitochondrial and cell
cycle dysfunction, impeding megakaryopoiesis, and
megakaryocyte differentiation (13).While the active autophagy process prolongs the cell
survival and lifespan, the over-activated autophagy
leads to autophagic cell death (14). In the autophagic
process, Beclin1 (Atg6) in the initial formation of
autophagosome acts as a partner of Bcl-2 as an antiapoptosis
factor that exerts an anti-autophagic effect
as well as anti-apoptosis (15). Recently, some studies
in breast cancer cell line confirmed that the expression
level of Beclin1 is remarkably low and induces the
tumor activity of cells (16).Accordingly, in this study, we investigated whether
amentoflavone could modulate autophagy related to cell
aging through the modulation of p53 and SIRT1.
Materials and Methods
This experimental study was conducted at the
Department of Applied Chemistry at Dong-Eui
University (Republic of Korea). In this study,
Amentoflavone was obtained from Sigma-Aldrich
(St. Louis, MO, USA). Dulbecco’s modified Eagle’s
medium (DMEM), trypsin-EDTA, penicillin/
streptomycin/ amphotericin (10000 U/ml, 10000 g/
ml, and 2500 g/ml, respectively), and fetal bovine
serum (FBS) were obtained from Gibco BRL, Life
Technologies (NY, USA). A549 (ATCC # CRL-6323)
and WI38 (ATCC # CRL-75) cells were purchased from
ATCC. 3-(4,5-dimethyl-2-yl)-2,5- diphenyl tetrazolium
bromide (MTT) reagent, agarose, and other materials
were purchased from Sigma Chemical Co. (St. Louis,
MO, USA).
Cell line and culture
This project was approved by the Ethics Committee
of Dong-Eui University of Applied Chemistry, Busan,
Republic of Korea. Cell lines were separately grown
as monolayers at 5% CO2 at 37°C in the humidified
atmosphere using appropriate media supplemented
with 5% FBS, 2 mM glutamine, and 100 g/ml penicillin-
streptomycin. DMEM was used as the culture medium
for A549 cells. Cells were passaged 3 times a week by
treating with trypsin-EDTA.
MTT assay
Cytotoxic levels of amentoflavone were measured
using MTT method as described previously by Hansen
et al. (17). The viability of cells was quantified as a
percentage compared to the control (optical density
of treated cells/optical density of blank×100) and
dose-response curves were developed. The data were
expressed as the mean from at least three independent
experiments and P<0.05 was considered significant.
Autophagosome detection assay
Autophagy activity was detected using a
commercially available autophagy/cytotoxicity
dual staining kit from Cayman Chemical Company
(Item No. 600140). Autophagy assay was performed
according to the manufacturer’s protocol. In brief,
A549 cells were seeded in a 96-well plate at a density
of 5×104 cells/well in DMEM culture medium and
incubated overnight at 37°C. Then, cells were treated
with different concentrations of amentoflavone
and tamoxifen as a positive control and incubated
overnight. On the third day, cells were stained with
propidium iodide (PI) and monodansylcadaverine
(MDC) according to the manufacturer’s protocol.
Autophagic vacuole staining intensity can be detected
using an excitation wavelength of 335 nm and an
emission wavelength of 512 nm using microplate
reader (Tecan Austria GmbH, Austria). The cells were
also analyzed by fluorescent microscopy according to
the manufacturer’s protocol. Dead cells are stained by
propidium iodide and can be detected with a rhodamine
filter (excitation/emission=540/570 nm).
Analyses of proteins expression using western blot
Western blotting was performed according to the
standard procedures. Cells treated with different
concentrations of amentoflavone were lysed with
RIPA lysis buffer (Sigma Chemical Co., St. Louis,
MO, USA). The cell lysates were resolved on a
4-20% Novex®gradient gel (Invitrogen, USA),
electrotransferred onto a nitrocellulose membrane
and blocked with 10% skim milk. The primary
antibodies (1:1,000) including p-p21(sc-12902, Santa
Cruz Biotechnology., CA, USA), p53(sc-126X),
p-p53(9286S, Sell Signaling Technology, MA, USA),
ac-p53(06-758, Upstate Biotechnology Inc., NY 12946
USA), Atg3 (sc-393623), Atg7 (2631S, Sell Signaling),
Beclin1 (3738, Sell Signaling), LC-3 (sc-292354), Bcl2
(sc-492-G), ß-actin (sc-1616), and their secondary
antibodies (1:5,000) (sc-1616, sc-2354, sc-2005, Santa
Cruz Biotechnology, CA, USA) were used to detect
the respective proteins using a chemiluminescent ECL
assay kit (Amersham Pharmacia Biosciences, NJ,
USA) according to the manufacturer’s instructions.
Protein bands were visualized using AlphaEase®gel
image analysis software (Alpha Innotech, CA, USA)
and protein expression was quantified by Multi Gauge
V3.0 software (Fujifilm Life Science, Japan).
Analysis of protein expression using immunofluorescence
staining
Cells were seeded onto a slide chamber and were
incubated overnight at 37°C. Then, the cells were
treated with different concentrations of amentoflavone.
After 24 hours of incubation, cells were fixed with 10%
formalin for 15 minutes at room temperature followed
by the permeabilization with phosphate buffer solution
(PBS) containing 0.5% tween 20 (0.5% PBS T-20)
and washed three times by 0.1% PBS T-20. The cells
had preconditioning process with 5% Donkey normal
serum and immunofluorescence staining with primary
antibodies (anti-Atg7, anti-p53, anti-p-p21, anti-pmTOR)
(1:500) for 24 hours at room temperature.
After, the cells were then washed with 0.1% PBS T-20
three times for 5 minutes, respectively and treated with
the secondary antibodies (donkey anti-rabbit conjugated
CY3, donkey anti-goat conjugated CY3, donkey anti-goat
conjugated FITC, donkey anti-rabbit conjugated CY3,
donkey anti-goat conjugated FITC, donkey anti-mouse
conjugated FITC, donkey anti-rabbit conjugated CY3)
(CY3 1:400, FITC 1:200) at room temperature for 1 hour.
The cells were then washed with 0.1% PBS T-20 three
times and PB once for 5 minutes, respectively. Finally,
the slide was spread using DAPI solution and examined
using iRiS™ Digital Cell Imaging System (Logos
Biosystems, Annandale, US).
SA-ß-galactosidase staining
According to the method of Tran (8), WI38 and A549
cells were incubated in a 24-well plate format under a
serum starvation state for 4 days, then exposed to 5
ng/mL of IGF-1 treatment for 6 days as a long-term
treatment or 10 µM H2O2 treatment for 24 hours. After
the treatment for 24 hours with a proper concentration
of amentoflavone, the cell culture medium was
aspirated and the cells were twice washed with PBS.
After the last rinse, PBS was replaced with 250 µl of
4% paraformaldehyde (PFA) for the fixation. The cells
were incubated for 5 minutes at room temperature.
The 4% PFA was aspirated and the cells were washed
two times for 5 minutes each at room temperature with
gentle shaking with 500 µl of PBS. Each well was
exposed to 250 µl of SA-ß-gal staining solution. The
cells were incubated in the dark in a 37°C incubator.
The reaction was terminated when the cells were
stained as blue-green. To terminate the reaction, the
staining solution was aspirated and replaced with
distilled water. The cells were washed for the second
time with distilled water. After the last wash, 500 µl
of distilled water was added to each well and the plate
was observed under the microscope.
Statistical analysis
Data were analyzed using Student’s t test for paired data
(comparison with the control group) and MEGFL. Data
are represented as the mean of values ± S.D and obtained
from three independent experiments (*P<0.05, **P<0.01,
***P<0.001).
Results
Effect of amentoflavone on the cytotoxicity
The cytotoxic effect of amentoflavone was investigated
using MTT assay. Amentoflavone above 8 µM exhibited
Park and Kim
the cytotoxicity in cancerous human lung fibroblasts (A549
cells) as shown in Figure 1A. In addition, amentoflavone
above 1 µM showed the cytotoxicity in normal human
lung fibroblasts (WI38 cells) as shown in Figure 1B.Effect of amentoflavone on cell viability. A. Amentoflavone was
treated to A549 cells and B. Amentoflavone was treated to WI38 cells. The
cells were treated with amentoflavone at the indicated concentration and
the cell viability was determined by MTT assay after 48 hours. Data are
presented as the mean of values ± SD obtained from three independent
experiments. The level of significance was identified statistically (*;
P<0.05, **; P<0.01, ***; P<0.001) using Student’s t test.
Effect of amentoflavone on the formation of
autophagosome
The effect of amentoflavone on the formation of
autophagosome was investigated by the degree of MDC
absorbed into autophagosome by the action of autophagy.
Amentoflavone above 2 µM displayed a remarkable
fluorescence image in A549 cells as shown in Figure 2A.
It was observed that it induced autophagy by 1.7-fold
increase compared with tamoxifen treatment group used
as a positive control in Figure 2B. In order to examine its
cytotoxicity at the same time, the cells were stained with
PI. Amentoflavone above 2 µM showed PI staining
that means the cell death as shown in Figure 2C.Effect of amentoflavone on formation of autophagosome in A549 cells. The cells (1×105 cells) were treated with amentoflavone at the indicated
concentration. The level of autophagosome formation was evaluated in the presence of amentoflavone or tamoxifen. A. The autophagosome was
stained by MDC and the damaged cells or dying cells were stained by PI, B. The effect of amentoflavone on autophagy was analyzed by the fluorescence
measurement of autophagic vacuole. The cells showing autophagic vacuoles were quantified by fold increase in green detection reagent signal, and C. The
effect of amentoflavone on the cell viability was analyzed by the fluorescence measurement of dead cells stained by propidium iodide. Data are shown
as the mean of values ± SD obtained from three independent experiments. The level of significance was identified statistically (**; P<0.01, ***; P<0.001)
using Student’s t test. MDC; Monodansylcadaverine and PI; propidium iodide.
Effect of amentoflavone on the expression of Atg7 and
autophagy-related proteins
In order to confirm the effect of amentoflavone on
the induction of autophagy, the expression of Atg7,
an autophagic marker, was examined in A549 cells
using immunofluorescence analysis. Cell nuclei were
labeled with blue DAPI fluorescence dye and the target
protein Atg7 was stained with a red CY3 fluorescence
dye as shown in Figure 3A. It was confirmed that
amentoflavone at 4 µM exhibited a higher red image
than tamoxifen at 20 µM used as a positive control,
indicating that amentoflavone could induce a higher
expression of Atg7 protein related to induction of
autophagy. Western blotting was also carried out to
examine the level of autophagy-related proteins by
amentoflavone. Amentoflavone at 8 µM remarkably
increased the levels of LC3, Becline1, and Atg7
involved in the formation of autophagosome in A549
cells as shown in Figure 3B and 3C. Moreover, it was
found that it can increase the levels of above-mentioned
proteins at a higher level than the tamoxifen group.
However, amentoflavone decreased the level of Bcl-2
protein, an anti-autophagy marker, and did not affect
the level of Atg3.
Effect of amentoflavone on the expression of proteins
related to p53 signaling pathway
In order to investigate the effect of amentoflavone
on p53 signaling pathway involved in the senescence
mechanism, immunofluorescence for p53 and p21
proteins were performed in this study. The nucleus of
A549 cells was stained with DAPI, and the p-p21 and
p53 proteins were labeled with green FITC and red
CY3 fluorescence dyes, respectively. Amentoflavone
treatment above 2 µM or 4 µM remarkably increased
the levels of p53 protein and p-p21 proteins,
respectively, as shown in Figure 4A. The effect on the
level of proteins related to p53 signaling pathway was
examined using western blot analysis. Amentoflavone
above 2 µM increased the level of p53 as shown in
Figure 4B and C. Similarly, the level of p-p21 protein
was enhanced in the presence of amentoflavone above
2 µM. However, amentoflavone above 2 µM decreased
the level of acetyl-p53.Effect of amentoflavone on the expression of Atg7 and autophagy-
related proteins. A. The images of Atg7 immunofluorescence-stainedA549 cells were shown by the red color. The arrows show Atg7 hasbeen localized to the cell cytosol (scale bar: 100 µm), B. The effect
of amentoflavone on protein expressions of LC3, Bcl-2, Beclin1, Atg3,
Atg7, and ß-actin was analyzed by western blot, and C. The level of
proteins expression was quantified by Multi Gauge V3.0 software. Dataare presented as the mean of values ± SD from three independentexperiments. The level of significance was identified statistically (***;
P<0.001) using Student’s t test.Effect of amentoflavone on the expression of proteins related
to p53 signaling pathway. A. The images of p53 (FITC) and p-p21 (CY3)
immunofluorescence-stained A549 cells were shown by the green
and red color, respectively. Arrows show p53 and p-p21 have been
localized to the cell cytosol or nuclear (scale bar: 100 µm), B. The
effect of amentoflavone on protein expressions of p-p21, p53, ac-p53,
and p-p53 was analyzed by western blot, and C. The level of protein
expressions was quantified by Multi Gauge V3.0 software.
Immunofluorescence analysis for the effect of
amentoflavone on expression of SIRT1
The anti-aging effect of amentoflavone was investigated
by the analysis of SIRT1 protein expression involved in
the senescence mechanism using immunofluorescence
staining. The nucleus of the cell was stained with DAPI,
and the SIRT1 protein was labeled with a red CY3
fluorescence dye, respectively. Resveratrol treatment
used as a positive control showed the highest level of
SIRT1 protein in the treatment groups as shown in Figure
5. Although the effect of amentoflavone on the level of
SIRT1 was lower than that of the resveratrol treatment
group, it remarkably increased the level of SIRT1
compared with the blank group.Immunofluorescence analysis of the effect of amentoflavone on
expression of SIRT1. The images of SIRT1 (CY3) immunofluorescencestained
A549 cells were shown by the red color. The cells were cultured
in the presence of amentoflavone and detected with a rabbit polyclonal
antibody against SIRT1. Arrows show SIRT1 has been localized to the cell
cytosol. Res stands for resveratrol used as a positive control in this study
(scale bar: 100 µm).
Effect of amentoflavone on cell aging in A549 cells and
WI38 cells
The effect of amentoflavone on aging of A549 cells was
investigated using SA-ß-galactosidase staining assay as
a senescence marker. In this study, the aging of cells was
induced by the short-term of treatment with H2O2 at 10 µM.
H2O2 treatment showed a higher blue staining image than
the blank group, indicating that H2O2 can induce the cell
aging as shown in Figure 6A. However, amentoflavone
treatment remarkably decreased the blue staining image
induced by H2O2, indicating that the cell aging induced
by H2O2 is inhibited by amentoflavone. The effect of
amentoflavone on senescence was also examined using
SA-ß-galactosidase staining assay normal lung fibroblasts
(WI38 cells). The senescence of WI38 cells was induced
by the long-term treatment of 5 ng/mL of IGF-1 or the
treatment with H2O2 at 10 µM. The IGF-1 treated group
exhibited a good phenotype of the cellular senescence
showing a strong blue staining with a wide flattened shape,
a typical shape of the aged cell as shown in Figure 6B.
H2O2treated group showed the phenotype of the cellular
senescence but the shape of the aged cell was slightly
less than the IGF-1 treated group. It was observed that
the amentoflavone treatment group above 2 µM reduced
the degree of blue staining and increased the cell size into
the wide flattened shape, indicating that amentoflavone
reduces the senescence.Effect of amentoflavone on senescence-associated (SA)-ß-galactosidase staining in A549 cells and in human lung fibroblast cells (WI38). A.
After the cells were treated with amentoflavone and H2O2 (10 µM) for 24hours, SA-ß-gal staining was carried out (scale bar: 100 µm). The senescentcells were stained by the blue color and B. After the cells were treated with
amentoflavone and IGF-1 (5 ng/mL) for 6 days or H2O2 (10 µM) for 24 hours,
SA-ß-gal staining assay was carried out (scale bar: 100 µm).
Discussion
As various studies on longevity have progressed, a
variety of pathways associated with aging have been found
and some gene manipulations succeed the life extension
of the simple model such as the nematode (18) .In recent
years, autophagy is closely related to the aging. Fasting
related to IGF-1 pathway and rapamycin associated
with mTOR mechanism necessarily require autophagy
process for the life extension (19). Therefore, this study
focused on the investigation whether the inductive effect
of amentoflavone, a biflavonoid compound contained in
Selaginella tamariscina, on autophagy could modulate the
senescence induced by the long-term of IGF-1 treatment
via p53 and SIRT1 signaling pathway.In the first place, the effect of amentoflavone on the
induction of autophagy was determined by the formation of
autophagosome that is the first step in autophagy process.
Beclin1 (Atg6) and class .
phosphatidylinositol 3-kinase
(PI3 kinase) form a complex with Vps34, creating inactive
form of the autophagosome (20). Amentoflavone increased
the formation of such autophagosome and, remarkably, also
enhanced the level of Beclin1 in A549 cells. Amentoflavone
exhibited a higher effect than tamoxifen used as a positive
control in forming autophagosome. Amentoflavone is believed
to promote the formation of the initial autophagosome by
increasing not only the extension of the phagophore and the
expression of LC3 (Atg8) protein promoting the formation
of autophagosome but also the expression of Atg7 activating
its ubiquitination. Ubiquitin-like protein of Atg8 exists in a
complex form (Atg8-PE) with phosphatidylethanolamine
(PE) in autophagic membranes (or phagophore) and
mediates the fusion portion of liposomes containing Atg8PE
and tethering in in vitro system (21). Therefore, the
positive effect of amentoflavone on the expression of LC3
and Atg7 proteins could affect even after the formation
autophagosome, and the effect of amentoflavone on a later
stage of autophagy should be further studied.These findings confirm that amentoflavone strongly
promotes the autophagy process in the early stage, in
particular by increasing the formation of autophagosome
than tamoxifen by increasing the level of the Beclin1,
Atg7, and LC3 proteins. Moreover, a previous study
reported that the crosstalk between autophagy and
apoptosis can be modulated by the interaction between
Bcl-2 family proteins and Beclin1, a Bcl-2 interacting
protein that promotes autophagy (22).On the other hand, it was previously reported that
apigenin. The monomer of amentoflavone, inhibits
mTOR, an autophagy repressor, and its downstream target
p70S6K, but does not alter the level of Beclin1, (23). In
addition, it was found that the induction of autophagy by
apigenin-mediated AMPK activation is accompanied by
the inhibition of the mTOR signaling pathway as a potent
chemopreventive agent (24).In this study, amentoflavone inhibited the protein
expression of Bcl-2, which is consistent with the previous
report that Bcl-2 not only acts as an anti-apoptosis factor
but also functions as an anti-autophagy factor (25),
indicating that amentoflavone could induce apoptosis.
Amentoflavone decreased the level of Bcl-2 protein
which inhibits the formation of Bcl-2-Beclin1, complex
and promotes the dissociation of Beclin1, leading to the
induction of autophagy as well as apoptosis which is
promoted by the inhibition of Bcl-2 protein (26). At this
point, the action mechanism of amentoflavone on the
induction of autophagy is distinct from that of apigenin.The previous studies have suggested that amentoflavone
has a great development potential as an anti-cancer drug
on apoptosis in this inductive effect (25, 27). Our findings
also suggest that amentoflavone could be developed
as a potential anti-cancer drug. Although p53 induces
apoptosis, it is a tumor suppressor protein which is closely
involved in the development of cancer (28). Moreover,
p53 protein is closely related to the aging mechanism
(29). SIRT1 and p53 proteins have been reported to play
a key role in the senescence induced by the insulin-like
growth factor-1 (8). The activity of SIRT1, suppressed
by the treatment of IGF-1 in the long-term, reduces
the deacetylation of p53, resulting in the induction of
senescence. In another report, SIRT1 suppresses the
senescence in normal cells such as HDF, but it induces
the senescence in some cancer cells such as MCF-7 and
H1299 by inhibiting their growth and proliferation (30,
31). Thus, SIRT1 is an important factor in determining
the activity of p53 (8). The activation of p53 protein is
made by the SIRT1, as a histone deacetylase, that directly
deacetylates p53 protein (32). In this study, amentoflavone
increased the level of p53 protein, matching the increase
of p-p21 expression activated by the p53 transcription
factor. However, the level of acetyl-p53 protein was
decreased by amentoflavone.Although the expression of p53 is increased by
amentoflavone, the activation of the p53 protein by the
increased SIRT1 is believed to be offset. Therefore, this
result is explained to be caused by the increased expression
of SIRT1. The previous studies on the interaction of SIRT1
with p53 protein support that amentoflavone increases
the level of p53 protein, but rather its increase in SIRT1
level explains very well our result that it could induce
autophagy higher than apoptosis (8, 33). Moreover, most
of aging studies have reported that the accumulation of
p53 protein causes the aging of cells, but the explanation
on the aging of an organism is not sufficient yet by the
accumulation of p53 protein alone. In fact, p53 protein
inhibits the aging of cells, and the inhibitory effect of the
cell aging by p53 protein disappears by nutrin3a, a p53
inhibitor (34). Finally, the study on the premature aging
of WI38 cells induced by H2O2 and the long-term of IGF1
confirmed that amentoflavone could inhibit the aging
of these cells. In this study, we investigated to observe
the effect of amentoflavone on the induction of autophagy
at the protein level, and how the induction of autophagy
affects the aging of the cell.
Conclusion
Amentoflavone increases the expression of Beclin1,
Atg7, Atg8, and LC3 proteins but decreases the expression
of Bcl-2, leading to the promotion of initial autophagy
by contributing to the formation of autophagosome.
Furthermore, the inductive effect of autophagy by
amentoflavone reduced the senescence. In addition, the
levels of p53 and SIRT1 proteins were increased in the
presence of amentoflavone. Therefore, these results
suggest that amentoflavone increases the survival rate of
cells by the induction of autophagy, which is expected as
a potential candidate inhibiting various diseases related to
autophagy and cell aging.
Authors: Alejo Efeyan; Ana Ortega-Molina; Susana Velasco-Miguel; Daniel Herranz; Lyubomir T Vassilev; Manuel Serrano Journal: Cancer Res Date: 2007-08-01 Impact factor: 12.701