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A hypoxia efficient imidazole-based Ru(II) arene anticancer agent resistant to deactivation by glutathione.
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Cite this: Dalton Trans., 2015, 44,
5969
Received 24th December 2014,
Accepted 15th February 2015
DOI: 10.1039/c4dt03983a
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A hypoxia efficient imidazole-based Ru(II) arene
anticancer agent resistant to deactivation
by glutathione†
Kallol Purkait,‡ Subhendu Karmakar,‡ Sudipta Bhattacharyya, Saptarshi Chatterjee,
Suman Kr Dey and Arindam Mukherjee*
www.rsc.org/dalton
A slow hydrolyzing imidazole-based RuII-arene complex [(L)RuII(η6p-cym)(Cl)](PF6) (1) with excellent stability in the extracellular
chloride concentration shows better activity under hypoxia and
strong resistance to glutathione (GSH) in vitro under hypoxic conditions. 1 arrests the cell cycle in sub G1 and G2/M phases and
leads to apoptosis.
Ruthenium-based anticancer agents have been one of the
most appreciated anticancer drugs after the platinum drugs
for their remarkable activity against cancer, the availability of
different oxidation states at normal physiological conditions
and less risk of side effects.1–3 Several π-bonded arene bound
ruthenium(II) complexes show high potency against various
forms of cancer.4–8 RuIII complexes have also demonstrated
potential as anti-cancer agents. NAMI-A1,9–11 is in clinical
trials due to its potential to stop the metastasis of cancer cells,
especially for solid tumors, although it has relatively poor IC50
values in vitro. In contrast, KP1019 and NKP1339 are active in
primary tumors.1,9–11 In vivo experiments in mice show that
the [RuII(η6-arene)Cl2( pta)] ( pta is 1,3,5-triaza-7-phosphaadamantane) (RAPTA) complex is also a promising candidate
to reduce the growth of lung metastases.7 Binding of Ru anticancer agents with albumin and transferrin in the blood
stream is thought to help their delivery to cells.1,2,12–14 It is
mostly believed that the Ru in oxidation state +II is the active
form. The presence of a reducing agent like glutathione (GSH),
or ascorbic acid in pancreas,1,15,16 causes the reduction of RuIII
to RuII and increases the rate of aquation and binding with
biomolecules.4,9,17 The redox processes however also help to
Department of Chemical Sciences, Indian Institute of Science Education and
Research Kolkata, Mohanpur campus, Mohanpur-741246, India.
E-mail: a.mukherjee@iiserkol.ac.in; Fax: +91-33-25873020
† Electronic supplementary information (ESI) available: General synthetic procedures and characterization data, experimental details of all biological studies,
selected single crystal X-ray data of 1, NMR spectra, hydrolysis and stability
studies, CT DNA binding, IC50 and GSH binding plots, cell cycle analysis, DNA
ladder assay, optical microscopy image. CCDC 1001374. For ESI and crystallographic data in CIF or other electronic format see DOI: 10.1039/c4dt03983a
‡ These authors contributed equally to this work.
This journal is © The Royal Society of Chemistry 2015
generate reactive oxygen species (ROS), which can destroy GSH
pools,1,18 thus destroying the cellular redox balance.19 Yet, the
presence of a higher concentration of glutathione (viz. in
resistant cells) can inhibit the RuII complexes by binding to
the metal center, thus rendering them inactive.20,21 Ru complexes have the potential to be a good alternative to cisplatin
for treating cisplatin-resistant cancers, but they also have
affinity towards the thiolate sulphur of cysteine and glutathione, which inhibits their anticancer activity,20,21,22,23
leading to failure of chemotherapeutics.24–26 In addition, the
situation is more complicated due to hypoxia, viz. in carcinomas, sarcomas, and lymphomas, since many anticancer
agents show less activity in hypoxia, viz. cisplatin.27
The activity of RuII arene complexes has been tuned mostly
by a change of arene,17,28,29 or change of the other
ligands,30–32 including the halide ion.17,33 Several RuII arene
complexes are active against cisplatin-resistant cell lines.34–36
Among the several ways to tune the activity of RuII arene complexes, we planned to introduce steric bulk in the auxiliary
ligand to slow down the hydrolysis. The ligand used for
this purpose was a sterically hindered imidazole based
Schiff base ligand (L = N-((1H-imidazol-2-yl)methylene)-2,6diisopropylaniline).
Our attempt provided us a p-cymene ( p-cym)-bound ruthenium(II) complex of L (1) (Fig. 1). The compound is slow to
hydrolyze and has excellent stability in saline solution. The
compound shows promising anticancer activity as per our
initial studies using three different carcinoma cell lines
(MCF-7, A549, HeLa). We found that in hypoxic conditions the
activity of 1 is enhanced and the complex is strongly resistant
to deactivation by the cellular reductant L-glutathione.
Complex 1 crystallizes in the monoclinic space group, P21/n
(see ESI, Table S1†). Each unit cell contains four complexes. In
each molecule, one vertex of the tetrahedral structure is occupied by a chloride, two with ligand L and another one by the
p-cymene with a η6 bonding, but all the distances between
carbons of p-cymene and metal atoms are not the same (see
ESI, Table S2†). This may be due to the steric hindrance of the
isopropyl group of p-cymene with the closest isopropyl group
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Dalton Transactions
Fig. 1 ORTEP diagram of complex 1. Thermal ellipsoids are drawn at
the 30% probability level. Hydrogen atoms and counter anion have been
omitted for clarity.
of the other ligand (L). The NMR spectra also support the
above fact that the two methyl groups of the isopropyl in
p-cymene are no longer equivalent (see ESI, Fig. S1, S2†). One
PF6 group is present in the lattice per molecule of the
complex, since the RuII is in the +2 oxidation state.
The hydrolysis of the labile halide group in such complexes
in general renders the complex active towards DNA
binding.4,17 The 1H NMR study of complex 1 shows that the
complex is ca. 32% hydrolyzed after 28 h (see ESI, Fig. S4†) in
a 3 : 7 v/v DMSO-d6–D2O mixture, and initially up to 2.5 h, we
could not see any peak for the hydrolyzed product. This slow
hydrolysis may be associated with the steric hindrance rendered by the ligand due to the presence of isopropyl groups.
The hydrolysis rate in 20 mM phosphate buffer solution at pH
7.4 containing 4 mM NaCl and 1% acetonitrile is 0.0115(5) h−1
and hence the t1/2 is ca. 60(3) h (Table 1, see ESI, Fig. S5†). In
water containing 1% acetonitrile, the t1/2 of 1 is 4.5(1) h. 1 is
stable up to 10 days in 110 mM saline solution as per the 1H
NMR data (see ESI, Fig. S6†), which is encouraging for an
active anticancer agent and relatively less commonly found.
The properties of 1 and the available data in literature on this
type of RuII complexes bearing the general formulation,
RuII(arene)(ligand)-(halide), suggests that in general, there
does not appear to be a strong correlation between the rate of
hydrolysis and cytotoxicity (see ESI, Table S3†). However, when
Table 1 Rate of hydrolysis and half lives of 1 at pH 7.4 and 6.7 measured
by UV-vis spectroscopy in 20 mM phosphate buffer solution in the presence of 40 mM or 4 mM salinea
Half-life (t1/2) h
Dissociation
rate (k) h−1
pH 7.4 NaCl (mM)
pH 6.7 NaCl (mM)
40
4
40
4
Waterb
110(6)
0.0063(3)
60(3)
0.0115(5)
28(3)
0.025(2)
6.0(2)
0.115(3)
4.5(1)
0.154(4)
a
Data presented are the mean of three independent experiments. b Data
presented are average of two experiments instead of three.
5970 | Dalton Trans., 2015, 44, 5969–5973
t1/2 is less than an hour, the complexes are more cytotoxic (see
ESI, Table S3†) with a few exceptions.32,37–39 In the case of 1, in
99% water the t1/2 is 4.5(1) h, and in 4 mM NaCl the t1/2
increases drastically to 60(3) h showing that 1 is relatively slow
to hydrolyze when compared with rates in the literature. Complexes with half-lives range of 1 < t1/2 < 12 h in water are in
general not significantly cytotoxic (see ESI, Table S3†).
However, 1 is found to be a potent RuII anticancer agent.
Hence, our results indicate that the role of the ligand is important not only in restricting the hydrolysis, but the ligand acts
synergistically with RuII to increase cytotoxicity. A few exceptions of non-hydrolyzing or slow hydrolyzing RuII(arene)(ligand)(halide) type complexes being toxic again emphasize
the importance of the ligand to act in synergism with the
metal center to render cytotoxicity.32,37 The hydrolysis studies
of complex 1 show that t1/2 values may show drastic changes
with pH and ionic strength/common ion effect (Table 1).
However, hydrolytic data in the intracellular type chloride concentration range (3–5 mM) are available only for a very few
complexes, and hence, the correlation cannot be made.32,37
The correlation of t1/2 values in water shows that our complex
is also an exception to the generally observed trend. Recently a
TiIV isopropoxide complex reported by Tshuva et al. shows that
complexes stable towards hydrolysis in aqueous medium may
be active as per the in vitro studies.40 From the above results,
it appears that the hydrolysis of a complex in a biological
environment may not be a simple phenomenon as predicted
through hydrolysis studies in buffer.
To gain more insight about the pathway of action, CT DNA
binding titration was carried in 1 : 9 v/v DMF:50 mM Tris-HCl/
NaCl ( pH = 7.4). The binding constant (Kb) of 2.31(3) × 103
M−1 (see ESI, Fig. S7†) shows that the interaction is moderate.
Although the interaction with CT DNA is not too high, literature data suggest that the cytotoxicity of a similar family of
complexes is due to the formation of adducts with DNA bases
especially N7 of guanine.41 This interaction was in spite of
50 mM NaCl being present in the buffer, which would render
the hydrolysis of 1 very slow. Hence, we may say that either the
complex is able to interact with DNA even without undergoing
hydrolysis or the presence of DNA may assist the hydrolysis,
leading to more complex–DNA interaction. The lipophilicity of
1 showed that it is more lipophilic, based on the partition
coefficient (log D), as compared to the ligand L (2.0(1)). The
log D value for 1 is 3.2(1), which is predicted to be within the
optimum range for a molecule to be a good drug.42 Hence,
the slow hydrolysis and the log D value are encouraging for
good cytotoxicity. When we probed 1 for cytotoxicity against
HeLa (human cervical carcinoma), MCF-7 (human breast
adenocarcinoma) and A549 (human lung adenocarcinoma)
cell lines, we found that 1 is significantly active in all the
above (Table 2, ESI, Fig. S8†). Since L is not cytotoxic up
to 500 μM, the toxicity is due to formation of the complex
[RuII(η6-p-cym)L(Cl)](PF6). It is known that having a good
in vitro cytotoxicity profile in normoxia may be a good indication, but cytotoxicity may worsen under hypoxic conditions
due to hypoxia-induced resistance.27,43 Hence, we probed the
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Table 2
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Cytotoxicity of the ligand (L) and complex 1 in comparison to that of [Ru(en)(η6-p-cym)Cl]PF6 (C1) and cisplatin (CDDP)
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IC50 (µM) ± S.D.a
Hypoxiab
Normoxia
1
L
C1
CDDP
Hypoxia + glutathioned
MCF-7
A549
HeLa
MCF-7
A549
MCF-7
A549
13.8 ± 1.2
>500
43.9 ± 2.6
15 ± 1
23.2 ± 0.4
>500
36.7 ± 2.3
24 ± 1
7.4 ± 1.1
N.D.c
N.D.c
7±1
9.1 ± 0.3
N.D.c
31.7 ± 1.7
19 ± 2
15.6 ± 1.4
N.D.c
31.2 ± 1.5
27 ± 1
10.8 ± 1.2
N.D.c
49.3 ± 1.8
29 ± 2e
16.7 ± 0.5
N.D.c
31.7 ± 2.6
40 ± 2e
a
IC50 values were calculated by non linear curve fitting in dose response inhibition—variable slope model using graph pad prism. S.D. =
standard deviation. The data presented are mean of three independent experiments, in a single experiment each concentration was assayed in
triplicate. The statistical significance (p) of the data is <0.05 or better. b Hypoxia (1.5% O2). c Not determined. d With 1 mM of reduced
e
L-glutathione. 20 molar equivalent of reduced L-glutathione used with respect to IC50 dosage of the respective cell line in hypoxia.
activity of 1 under hypoxic conditions in MCF-7 and A549
cells. We found that the IC50 values were 9.1 ± 0.3 μM ( p <
0.01) and 15.6 ± 1.4 μM ( p < 0.05) against MCF-7 and A549
cells, respectively (Table 2, see ESI, Fig. S9†), showing that
there is ca. 35% increase in activity in hypoxia (Table 2). Carcinomas may have a interstitial pH of ca. 6.7;44 hence, the hydrolysis of 1 was also studied at pH 6.7 using UV-Vis spectroscopy,
which showed that the rate of hydrolysis at pH 6.7 was significantly more than the rate at pH 7.4 (Table 1). The results
suggest that a change in pH really affects the rate of hydrolysis
and the increase in the rate of hydrolysis may be one of the
reasons for the enhancement of activity under hypoxia.45 In
contrast, cisplatin shows a decrease in activity (ca. 15–30%)
using the same hypoxic conditions (Table 2), which is well supported by the literature.43 In order to understand if it is a
rather general property of RuII complexes to be equally or
better active in hypoxia, based on the suggestion of a Reviewer,
we synthesized and characterized the [RuII(en)(η6-p-cym)Cl](PF6)
(en = ethylenediamine) of Sadler et al. and then probed its
activity against MCF-7 and A549 cells (Table 2). The results
show that the complex may be considered to be almost equally
active (in A549 cells) or better (in MCF-7 cells) under hypoxic
conditions. The deactivation by glutathione appears to be cell
dependent, since it is not deactivated in A549 cells under
hypoxic conditions in the presence of glutathione but is deactivated in MCF-7 cells. The difference in activity is statistically
significant under normoxic and hypoxic conditions. A recent
study also suggests that having similar activity in normoxia
and hypoxia itself is an appreciable quality for an anticancer
agent,27 since many anticancer agents show a decrease in
activity43 in hypoxia. Hence, 1 may be considered as a potent
anticancer agent with more activity in hypoxia.
Complex 1 exhibits strong resistance to deactivation by
L-glutathione, which is a major deactivating agent for most Pt
and Ru anticancer agents or Pt-based clinical drugs.21,37,46 In
hypoxic conditions, 1 in the presence of 1 mM of reduced
L-glutathione (ca. 60–100 molar equivalent with respect to the
IC50 in hypoxia) exhibits IC50 values of 10.8 ± 1.2 μM ( p < 0.03)
against MCF-7 cells and 16.7 ± 0.5 μM ( p < 0.01) against A549
cells (see ESI, Fig. S10†). It shows that the deactivation by
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glutathione is up to ca. 19% for 1 using such a huge excess of
glutathione, whereas under the same conditions with only
20 molar equivalents of L-glutathione cisplatin is deactivated
by ca. 50% in the MCF-7 and A549 cell lines (Table 2). It
should be noted here that even in the presence of a large
excess of reduced L-glutathione in hypoxia, the IC50 value is
still better than that observed in normoxia for complex 1. The
electronic and steric effects of the ligand in 1 and the kinetic
nature of RuII may be making the hydrolysis rate slow and the
approach by glutathione difficult, leading to no binding with
glutathione. The study on the [RuII(en)(η6-p-cym)Cl](PF6)
complex by us also suggests that RuII may have the potential to
be used in the development of hypoxia-active anticancer
agents.
The NMR studies support that although the complex 1
slowly hydrolyzes, it does not bind to glutathione when reacted
with 20 molar equivalent of reduced L-glutathione (see ESI,
Fig. S14†). Instead, the formation of the glutathione dimer
slowly takes place over 8–10 h, which may be due to the presence of a trace amount of oxygen, since we find the same
dimer formation even in the absence of any complex in the
solution (although the N2 purging times were quite longer,
ca. 30–45 min) (see ESI, Fig. S14†). The results support that
glutathione hardly affects the cytotoxicity of 1.
Initial studies with MCF-7 cells show that 1 arrested cells at
the sub G1 phase as well as in the G2/M phase (Table 3, see
ESI, Fig. S15†), unlike cisplatin, which arrests MCF-7 cells only
in the G2/M phase.47 The accumulation of a significant popu-
Table 3
Cell cycle analysis in MCF-7 cells treated with the complexa
DMSO control
1, 4 μM
1, 6 μM
Sub G1
G0/G1
S
G2/M
4.5
10.4
14.0
42.7
34.4
26.2
27.5
23.7
16.9
25.3
31.5
42.9
a
Cells were treated for 24 h with 1. Cells were treated with propidium
iodide and analyzed by FACS. Cell populations were analyzed and
expressed as the percentage of cells in each phase. The data presented
are an average of two independent experiments.
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lation of cells in the sub G1 phase indicates that 1 may follow
the apoptotic pathway. The cleavage of chromatin DNA into
internucleosomal fragments is one of the important biochemical characteristics of apoptotic cells.48,49 The ladder assay of 1
against MCF-7 cells shows that the DNA is cleaved to form
nucleosome-sized fragments of approximately 180–2000 base
pairs (see ESI, Fig. S16†), confirming that 1 induces apoptosis
in the MCF-7 cells. The optical microscopy images of MCF-7
cells treated with 1 for 24 h show chromatin condensation and
nucleus swelling as shown with bright arrows in DAPI images
and with dark arrows in merged images (see ESI, Fig. S17†).
The data are supportive of apoptotic killing of cancer cells by
complex 1.
Conclusions
To summarize, [(L)RuII(η6-p-cym)(Cl)](PF6) (1) of the sterically
hindered Schiff base L is highly stable in 110 mM NaCl solution, emphasizing its stability in the extracellular space. 1 is
slow to hydrolyze at the normal physiological pH of 7.4 in
4 mM NaCl with a t1/2 of 60(3) h. The complex shows an
encouraging in vitro cytotoxicity profile and may be a potent
anticancer agent because it is more active under hypoxic conditions and resists deactivation by glutathione in both of the
probed carcinoma cell lines, MCF-7 and A549. The enhancement of activity under hypoxia may be related to the increased
rate of hydrolysis at pH 6.7. The presence of L renders 1 resistant to hydrolysis and deactivation by reduced L-glutathione.
The resistance to deactivation is further supported by the in
vitro activity of 1 in the presence of an excess (60–100 equivalent of IC50) of glutathione for both MCF-7 and A549 cells.
The hypoxia activity of [RuII(en)(η6-p-cym)Cl](PF6) of Sadler
et al. also shows a promising trend as per our studies on
MCF-7 and A549 cells. Therefore, this work shows that RuII may
be exploited to design hypoxia-active anticancer agents, and
steric hindrance may be exploited to improve the cytotoxicity
profile of RuII arene complexes in high concentrations of glutathione. In fact, the resistance to glutathione, steric hindrance
and slow hydrolysis may play a synergistic role. These results are
highly encouraging and warrant more work with L and its
analogues to generate RuII complexes by changing the halide
and the arene to understand the effect of steric hindrance on
the rate of hydrolysis and its dependence on pH, better activity
in hypoxia and resistance to deactivation by L-glutathione.
We sincerely acknowledge DST for financial support via
project no SB/S1/IC-02/2014. We also thank IISER Kolkata for
infra-structural support, including NMR, single crystal X-ray,
microscopy and FACS facilities. K.P. and S.K. thanks UGC, S.B.
and S.K.D. thank CSIR-India and S.C. thanks IISER Kolkata for
providing post-doctoral research fellowship.
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