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Cytotoxic cis-ruthenium(III) bis(amidine) complexes.
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An international journal of inorganic chemistry
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Wen-Xiu Ni, Wai-Lun Man et al.
Cytotoxic cis-ruthenium(III) bis(amidine) complexes
Volume 52
Number 25
7 July 2023
Pages 8491-8820
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Cite this: Dalton Trans., 2023, 52,
8540
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Cytotoxic cis-ruthenium(III) bis(amidine)
complexes†
Tao Liu,a Chen Pan,a Huatian Shi,b Tao Huang,a Yong-Liang Huang,
Yang-Yang Deng,a Wen-Xiu Ni *a and Wai-Lun Man *b
a
In chemotherapy, the search for ruthenium compounds as alternatives to platinum compounds is proposed because of their unique properties. However, the geometry effect of ruthenium complexes is
sparely investigated. In this paper, we report the synthesis of a series of bis(acetylacetonato)ruthenium(III)
complexes bearing two amidines (1−) in a cis configuration. These complexes are highly cytotoxic against
various cancer cell lines, including a cisplatin-resistant cell line. In vitro studies suggested that the representative complex can induce cell cycle G0/G1 phase arrest, decrease the mitochondrial membrane
potential, elevate the intracellular reactive oxygen species level, and cause DNA damage and caspaseReceived 2nd February 2023,
Accepted 20th March 2023
mediated mitochondrial pathway apoptosis in NCI-H460 cells. In vivo, it can effectively inhibit tumor
DOI: 10.1039/d3dt00328k
xenograft growth in nude mouse models with no body weight loss. In combination with the reported
trans-bis(amidine)ruthenium(III) complexes, we found that ruthenium(III) bis(amidine) complexes could be
rsc.li/dalton
cytotoxic in both trans and cis geometries, which is in contrast to platinum-based compounds.
Introduction
In chemotherapy, the undesired side effects and acquired resistance to platinum-based compounds have motivated the
search for other metal-based anticancer agents.1–3 Ruthenium
complexes are the best alternative with unique properties,
including a good binding ability to biological molecules, low
toxicity, and high selectivity.4,5 So far, many ruthenium-based
anticancer agents have been reported with promising in vitro
and in vivo activities; they are well-designed with precious
ancillary ligands that could be systematically tuned with steric
and electronic effects.6–9 Surprisingly, the geometry effect of
these ruthenium complexes is less explored. For example,
Glazer et al. reported the biological properties of the polypyridyl ruthenium(II) diamine complex.10 To the tested HL-60 and
A549 cell lines, the trans isomer is cytotoxic, while its cis
analog is intrinsically inactive (Fig. 1). This result contrasts
with the well-known platinum-based anticancer drugs, of
which cisplatin is highly active, but transplatin is ineffective in
cancer treatment.
a
Department of Medicinal Chemistry, Shantou University Medical College, Shantou,
Guangdong, 515041, P.R. China. E-mail: wxni@stu.edu.hk
b
Department of Chemistry, Hong Kong Baptist University, Kowloon Tong, Hong Kong,
P.R. China. E-mail: wlman118@hkbu.edu.hk
† Electronic supplementary information (ESI) available. CCDC 2223820. For ESI
and crystallographic data in CIF or other electronic format see DOI: https://doi.
org/10.1039/d3dt00328k
8540 | Dalton Trans., 2023, 52, 8540–8548
Inspired by the recent work reported by Zhu et al., the axial
ligands on (salen)ruthenium(III) complexes have shown a profound effect on the mechanism of killing cancer cells. In the
trans-configuration, the two amidine ligands coordinated to
the planar (salen)ruthenium(III) complexes can induce cancer
cell death via the para-apoptosis mechanism.11 These bis
(amidine) complexes are easily accessed by nucleophilic attack
of appropriate amines to the acetonitrile coordinated onto the
ruthenium(III) center. In this work, we prepared the complex
cis-[RuIII(acac)2(NCCH3)2]+ [acac = acetylacetonate(1−)] and synthesized a series of bis(amidine)ruthenium(III) complexes in
the cis-configuration. These complexes are highly active toward
the tested cancer cell lines. The possible anti-cancer mecha-
Fig. 1 The drawings of the cis/trans-isomers of ( polypyridyl)ruthenium
(II) and diamminedichloroplatinum(II).
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nisms, which included colony formation, cell cycle arrest,
induction of apoptosis, mitochondrial membrane potential
(MMP) change, reactive oxygen species (ROS) elevation, and
the protein expression level, were explored using various
methods. Moreover, the in vivo antitumor potency of the representative complex was evaluated using a xenograft mouse
model.
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Fig. 2
The structures of 1–6.
Results and discussion
Synthesis and characterization
The amidine complexes can be readily accessed by nucleophilic
attack of the amines onto the nitriles coordinated to the ruthenium(III) ion (Scheme 1). The purple complex cis[RuIII(acac)2(NCCH3)2]+ was prepared according to the literature
method.12 Treatment of RuIII(acac)3 with 1.2 equiv. of HX (X =
ClO4− or CF3SO3−) in CH3CN at room temperature afforded the
corresponding compound cis-[RuIII(acac)2(NCCH3)2](X) in high
yield. These compounds were used without further purification.
Addition of 10 equiv. of primary amines (RNH2) to cis[RuIII(acac)2(NCCH3)2]+ in CH3CN at room temperature afforded
a deep red solution in 10 min. After evaporation of the volatiles
and recrystallization from CH3CN/Et2O, a series of cis-ruthenium(III) bis(amidine) complexes, with the general formula of
cis-[RuIII(acac)2(NHvC(CH3)NHR]+ (1–6), were isolated (Fig. 2).
Mass spectrometry shows the dominant peaks corresponding to their parent ions. Fig. 3A shows the representative
ESI-MS of complex 6. The dominant peak at a mass-to-charge
ratio (m/z) of 584 is assigned to the parent ion with the
formula [Ru(acac)2(NHvC(CH3)NH(CH2)5CH3)2]+. This assignment is supported by the excellent agreement between the
experimental and simulated patterns of the peak (insets). The
MALDI-TOF mass spectra ( positive mode) of other complexes
are shown in Fig. S1–S5.†
We have also done the cyclic voltammetry (CV) of complexes
5 and 6 in CH3CN using 0.1 M [NnBu4](PF6) as the supporting
electrolyte. All potentials are reported in volts (V) with referFig. 3 Characterization of 6(CF3SO3). (A) ESI mass spectrum ( positive
mode) in CH3CN. Insets show the peak’s experimental (top) and simulated (bottom) patterns. (B) CV in CH3CN. (C) X-ray structure of the
cation. The solvent molecule and hydrogen atoms are omitted for
clarity.
Scheme 1 The synthesis of trans- and cis-ruthenium(III) bis(amidine)
complexes.
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ence to ferrocenium/ferrocene (Cp2Fe+/0). In Fig. 3B, the two
reversible couples at +0.62 V (ΔEp = 71 mV) and −1.02 V (ΔEp =
77 mV) are assigned to the metal-centered RuIV/III and RuIII/II
couples of 6, respectively. The reduction potentials of both
RuIV/III and RuIII/II couples are insensitive to the length of the
alkyl chain. In complex 5, these couples occurred at E1/2 =
+0.62 and −1.01 V (Fig. S6†). Both complexes 5 and 6 are
stable in CH3CN in air, similar to the trans-[RuIII(salen)(NHvC
(CH3)NH(CH2)5CH3)2]+ with an E1/2 of RuIV/III and RuIII/II =
+0.36 and −1.13 V respectively in CH3CN.
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The molecular structure of complex 6 has been determined
by X-ray crystallography (Fig. 3C and Tables S1–S2†). The structure clearly shows that two amidines are bonded to the ruthenium center, cis to each other. The bond distances of Ru(1)–N
(1) and Ru(1)–N(3) are 2.034(3) Å and 2.038(4) Å, respectively,
which are slightly shorter (Ru–Namidine = 2.070(3) Å) than that
in trans-[RuIII(salen)(NHvC(CH3)NH(CH2)5CH3)2]+.
Stability
UV-vis spectroscopy was used to investigate the stability of 1–6
in various solvents (Fig. S7 and S8†). All complexes are stable
in neat DMSO at room temperature with no notable spectral
changes for 24 h. They are also stable (except for 3 and 4) in
phosphate-buffered saline (PBS, with 1% DMSO) solution. The
decline of the UV-vis spectra of 3 and 4 in the PBS solution
was presumably due to the decreasing solubility in the
aqueous solution when the alkyl chain length increased in the
amidine moiety. Notable precipitates were observed after
standing the PBS solutions of 3 and 4 for 24 h.
Cytotoxicity
MTT assay ([3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide]) evaluated the in vitro cytotoxicity of complexes
1–6 against a panel of human cancer cell lines, including liver
hepatocellular (HepG2), cervical epithelioid (HeLa), breast
(MCF-7), ovarian (A2780), and lung (NCI-H460, A549, A549/
DDP). IC50 values are summarized in Table 1. The IC50 value is
the dose required to inhibit 50% cellular growth for 48 h.
Cisplatin (used as a positive control) exhibits micromolar IC50
values toward the tested cancer cell lines (except for A549/
DPP), which aligned with the results found in other research
groups. Generally, 1–6 exhibit similar or slightly higher cytotoxicity than cisplatin. The cytotoxicity of these complexes
varies with the length of the alkyl chain. Increasing the
number of CH2 groups in the amidine moieties decreases the
IC50 value and reaches the minimum when n = 8 (complex 3,
Fig. 2). However, further increasing the chain length to n = 10
(complex 4) lowers the cytotoxicity. On the other hand, the
cytotoxicity of these ruthenium(III) complexes is insensitive to
the counterions. The IC50 values are the same for the ClO4− or
CF3SO3− complexes. It is known that cisplatin is less cytotoxic
Table 1
to the cisplatin-resistant cell line (A549/DDP). A large resistance factor (RF) value of 14.4 is observed. RF value is defined
as IC50 in (A549/DDP)/IC50 in A549. In contrast, complexes 1–6
are highly active toward the A549/DDP cell line, with low RF
values ranging from 0.8 to 1.2. This result suggested that complexes 1–6 are potential drugs to overcome the resistance to
platinum-based anticancer drugs. Considering the stability,
solubility, and cytotoxicity, we have selected complex 6 as the
representative candidate for further in vitro and in vivo studies
using NCI-H460 cells. Apart from the MTT assay, the colony
formation assay is a well-established method to evaluate the
antiproliferative activity of anticancer agents.13 Fig. 4A shows
the dose-dependent suppression of colony formation in 6treated NCI-H460 cells. For the NCI-H460 cells treated with
0.5 μM 6, 75% of colonies were observed. When the concentration of 6 was increased to 1, 2, and 4 μM, the colonies significantly dropped to 55, 8, and 2%, respectively. No colony
formation was observed for the NCI-H460 cells when treated
with 8 μM 6. This result agrees with the IC50 value adapted in
the above MTT assay. We have also performed the EdU incorporation assay to examine the rate of DNA replication. EdU
(5-ethynyl-2′-deoxyuridine) can substitute thymidine by incorporating newly synthesized DNA during DNA synthesis. The
proportion of EdU-positive cells significantly decreased dosedependently after treatment with complex 6 (Fig. 4B).
Cell cycle progression
Cell proliferation inhibition by hindering cell cycle progression
is known to many anticancer agents.14 Hence, we have investigated the cell cycle distribution of 6-treated NCI-H460 cells by
flow cytometry using propidium iodide (PI) staining (Fig. 5A).
The G0/G1 phase population of the untreated group was
43.0%. After treatment with 8 μM complex 6, the G0/G1 phase
population increased to 52.3 and 61.6% at 12 and 24 h,
respectively, indicating a G0/G1 phase arrest. Furthermore, a
concentration-dependent G0/G1 phase arrest was also found
in 6-treated cells (Fig. S9†). To further elucidate 6-induced cell
cycle arrest, we examined the level of proteins in cell cycle distribution by western blotting. The transcription factor E2F-1
plays a vital role in the G1/S transition of cell cycle progression.
Retinoblastoma protein (Rb) is a typical tumoral suppressor
Cytotoxicity of cis-ruthenium(III) bis(amidine) complexes 1–6
IC50 a (μM)
Compound
HepG2
HeLa
MCF-7
A2780
NCI-H460
A549
A549/DDP
RFb
1
2
3
4
5
6
Cisplatin
11.0 ± 2.4
2.66 ± 0.36
0.85 ± 0.18
4.30 ± 0.35
13.5 ± 1.77
3.00 ± 0.85
3.58 ± 0.72
1.82 ± 0.92
1.15 ± 0.52
0.19 ± 0.01
1.85 ± 0.41
1.87 ± 0.46
0.64 ± 0.02
5.12 ± 0.22
1.32 ± 0.13
0.83 ± 0.27
0.24 ± 0.06
2.67 ± 0.48
1.58 ± 0.07
0.51 ± 0.01
4.24 ± 0.40
2.09 ± 1.01
0.55 ± 0.10
0.23 ± 0.01
2.24 ± 0.48
1.78 ± 0.45
0.72 ± 0.01
11.6 ± 0.04
1.83 ± 0.07
0.92 ± 0.06
0.18 ± 0.01
2.13 ± 0.28
1.63 ± 0.19
0.77 ± 0.02
3.02 ± 0.03
2.40 ± 0.40
1.62 ± 0.28
0.22 ± 0.05
2.30 ± 0.52
1.76 ± 0.36
0.71 ± 0.01
10.6 ± 0.71
1.88 ± 0.42
1.25 ± 0.16
0.27 ± 0.01
1.97 ± 0.18
1.81 ± 0.49
0.66 ± 0.07
153.8 ± 5.0
0.8
0.8
1.2
0.8
1.0
0.9
14.4
a
50% inhibitory concentration after exposure for 48 h in the MTT assay. b Resistance factor calculated from the ratio of IC50(A549/DPP) to
IC50(A549).
8542 | Dalton Trans., 2023, 52, 8540–8548
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same time, it significantly uplifted the levels of p27 and p16 in
NCI-H460 cells. These results indicated that 6 could induce
G0/G1 phase cell cycle arrest in both time- and dose-dependent manners.
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Cell death pathway
Fig. 4 (A) Inhibitory effect of 6 on colony formation in NCI-H460 cells.
(B) NCI-H460 cell proliferation determined by EdU staining. Typical
images of EdU-stained proliferating cell nuclei (green) and Hoechststained cell nuclei (blue) and merged images are shown (scale bar:
100 mm).
Calcein-AM/PI double staining assay was conducted to distinguish between the live cells (green fluorescence) and dead
cells (red fluorescence). As shown in Fig. 6, the number of
dead cells increased significantly after treatment with different
concentrations of complex 6. To understand the cell death
mechanism, we initially investigated whether complex 6
induced cell apoptosis in NCI-H460 cells by flow cytometry.
Annexin V-FITC/PI double staining cells are shown in the flow
chart, which contains four typical quadrants including normal
cells (lower left quadrant), necrotic cells (upper left quadrant),
early apoptotic cells (lower right quadrant), and late apoptotic
cells (upper right quadrant). Compared with the control cells,
the low dose of 6 (1 μM) resulted in insignificant apoptotic
cells (early and late stage) of only 2.7%. When the concentration of 6 was increased to 8 and 10 μM, the apoptotic cells
were uplifted to 28.4 and 51.5%, respectively (Fig. 7). In
addition, the apoptotic rate was also increased from 16.4%
(12 h) to 56.5% (48 h) when treated with 8 μM complex 6
(Fig. S11†).
Intracellular ROS detection
Intracellular reactive oxygen species (ROS) oxidative stress can
induce cell apoptosis.18,19 We determined the ROS levels in 6treated cells by inverted fluorescence microscopy and flow
cytometry after staining with 2′,7′-dichlorodihydrofluorescein
diacetate (DCFH-DA). In the presence of cellular ROS,
DCFH-DA can be converted to DCF, which displays green fluo-
Fig. 5 (A) NCI-H460 cell cycle distribution for 0–24 h after treatment
with 6 (8 μM) as determined by flow cytometry. (B) Protein expression
levels of 6-treated (8 μM) NCI-H460 cells assessed by western blotting.
which can be hyper-phosphorylated to its inactivated form by
cyclins and CDKs, such as CyclinD1-CDK4/6 and
CyclinE-CDK2 and allow E2F-1 releases. CDKs can be inhibited
by specific cyclin-dependent kinase inhibitors (CKIs) such as
p27 and p16, resulting in G1 phase arrest.15–17 As clearly
shown in Fig. 5B and Fig. S10,† complex 6 suppressed the
levels of relevant cell cycle regulatory proteins, including
CDK2, CDK4, CyclinE1, CyclinD1, p-Rb, and E2F-1. At the
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Fig. 6 Fluorescence images of Calcein-AM and PI co-stained 6-treated
NCI-H460 cells (the scale bar is 100 mm).
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rescence probe, JC-1 (5,5′,6,6′-tetrachloro-1,1′,3,3′-tetraethylimidacarbocyanine iodide). JC-1 forms J-aggregates with red
fluorescence at high MMP. In contrast, it exists as a
J-monomer and displays green fluorescence at low MMP.
Complex 6 resulted in a dose-dependent increase in the green/
red fluorescence intensity ratio. Compared to the control
group (1.02), the ratio was increased to 3.34 (8 µM) and 3.36
(10 µM) (*P < 0.05), suggesting that 6 could induce mitochondrial dysfunction, particularly the loss of MMP (Fig. 8C).
Western blot analysis of the apoptosis pathway
Fig. 7 Apoptosis detection in NCI-H460 cells using AnnexinV-FITC/PI
double staining after 24 h treatment with various concentrations of 6.
rescence.20 The microscopy images (Fig. 8A) showed an apparent dose-dependent increase in green fluorescence. Compared
to the control group, the mean fluorescence intensity of
NCI-H460 cells incubated with 10 μM 6 increased by ca. 3 fold
(Fig. 8B). These results indicated that 6 could induce ROS
elevation.
Mitochondrial membrane potential detection
The reduced mitochondrial membrane potential (MMP) is a
sign of early cell apoptosis.21,22 To investigate the effect of
complex 6 on cell MMP, we carried out flow cytometry to
analyze 6-treated NCI-H460 cells using a mitochondria fluo-
Fig. 8 Analysis of cellular ROS levels in NCI-H460 cells treated with
compound 6 (1, 4, 8, and 10 μM) for 6 h and stained with DCFH-DA.
Rosup was used as a positive control. (A) Cells were measured by flow
cytometry. (B) Fluorescence microscopy images of cells, scale bar:
100 μm. (C) MMP analysis by flow cytometry. Cells were treated for 24 h
and then stained with JC-1.
8544 | Dalton Trans., 2023, 52, 8540–8548
Cell apoptosis is known to undergo an extrinsic death receptor
or intrinsic mitochondrial and endoplasmic reticulum (ER)
pathway.23–25 The caspase and Bcl-2 family proteins play essential roles in apoptosis. For example, the activation of Caspase 3
by Caspases-8 and -9 is one of the best-recognized signs of
apoptosis. The Bcl-2 family acts as the regulator, which
involves pro-apoptosis (Bax or Bad) and anti-apoptosis proteins
(Bcl-2 or Bcl-xl).26,27 We detected the expression of apoptosisrelevant proteins in 6-treated NCI-H460 cells by western blotting (Fig. 9). We found that the Cleaved-Caspase 9 was activated to increase in a dose- and time-dependent manner. In
addition, the downregulation of Bcl-2 and the up-regulation of
Bax and Cleaved-Caspase 3 were detected in 6-treated
NCI-H460 cells (Fig. 9 and S12†). Therefore, we concluded that
complex 6 could induce caspase-mediated apoptosis in
NCI-H460 cells via the intrinsic mitochondrial pathway.
DNA damage and repair mechanisms are related to cell
apoptosis.28 H2A.X, a member of the histone H2A family, is
involved in checkpoint-mediated cell cycle arrest and DNA
damage repair. When cell DNA double bonds are broken, H2A.
X can be phosphorylated to phospho-H2A.X (γ-H2A.X), so
γ-H2A.X is regarded as a double-strand DNA-broken biomarker. PARP ( poly ADP-ribose polymerase) is a DNA repair
enzyme, which can be activated to be Cleaved-PARP (Cl-PARP)
by recognizing damaged DNA fragments. Cleavage of PARP is
an important indicator of apoptosis.29,30 The expression level
of Cl-PARP and γ-H2A.X in 6-treated NCI-H460 cells was
detected by western blotting. 6 induced time-and concen-
Fig. 9 Western blot analysis of DNA damage and apoptosis-related
proteins in 6-treated NCI-H460 cells at various time intervals.
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have been prepared and characterized, including X-ray analysis. All complexes show promising cytotoxicity against the
tested cancer cell lines, including the cisplatin-resistance
A549/DDP cell line. The representative complex 6 can inhibit
colony formation and induce cell cycle arrest. It works as a
cytostatic and induces cell apoptosis through the caspasemediated mitochondrial pathway. In addition, 6 also increases
intracellular ROS levels, decreases MMP, and causes DNA
damage in vitro. In vivo, complex 6 shows promising antitumor
efficacy with no body weight loss in nude mice. In combination with the work done by Zhu et al., we demonstrated that
both the cis and trans configurations of bis(amidine)ruthenium(III) complexes are promising alternatives as anticancer
agents.
Fig. 10 In vivo anticancer activity of 6 in mice bearing the NCI-H460
tumor xenograft. (A) Effect of 6, cisplatin, and the vehicle control on the
tumor volume. Tumor growth was tracked using the mean tumor
volume (mm3) ± SD (n = 3). (B) Effect of 6, cisplatin, and the vehicle
control on the body weight. (C) The final tumor weight with values
reported as means ± S.D. (n = 3). (*P < 0.05, **P < 0.01 represent significant difference compared with the vehicle control). (D) Photographs of
tumors from the sacrificed mice at the end of the experiment.
tration-dependent up-regulation of their expression levels
(Fig. 9 and S12†). Furthermore, it indicated that 6 could cause
DNA damage in NCI-H460 cells, which is compatible with the
result of the EdU incorporation assay.
In vivo anti-tumor activity
To evaluate the in vivo antitumor efficacy of 6, we have applied
an NCI-H460-bearing nude mouse tumor xenograft model. The
mice were randomly divided into three groups and treated
with the vehicle, complex 6 (12.5 mg kg−1 of mice), and cisplatin (3 mg kg−1 of mice) every 4 d via intravenous tail injection.
The therapeutic effect was monitored by measuring mice’s
tumor volumes and body weights every 2 d (Fig. 10A and B).
Remarkably, the tumor growth of the treated groups (red line
for complex 6 and green line for cisplatin) was significantly
inhibited compared to the control group (blue line). At the end
of the experiment, the tumor sizes were determined from the
sacrificed mice. Consistent with the real-time measurement,
the tumor weight of the treated groups (complex 6 and cisplatin) was much lower than that of the control group (Fig. 10C).
Complex 6 possessed anti-tumoral activity with an inhibitory
rate of 51.0%, which is only slightly lower than 63.9% for cisplatin (*P < 0.05 **P < 0.01) (Fig. 10D). Weight loss in patients
is one of the common side effects of cisplatin. In this animal
test, the mice from the cisplatin-treated group resulted in
steady weight loss after day 13. In contrast, the 6-treated group
exhibited unobvious weight loss throughout the experiment.
Conclusions
In summary, a series of cis-bis(amidine)ruthenium(III) complexes bearing two bidentate acetylacetonato(1−) ligands 1–6
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Materials and methods
Materials
Cisplatin (CDDP) and 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazoliumbromide (MTT) were purchased from Alfa. Cell
Cycle Analysis Kit, ROS Assay Kit, BCA protein assay kit, MMP
assay kit with JC-1, Calcein AM/PI Cell Viability/Cytotoxicity
Assay Kit, and EdU Cell Proliferation Kit were obtained from
Beyotime Biotechnology (Shanghai, China). FITC Annexin V
Apoptosis Detection Kit I was purchased from BD
Pharmingen™. The primary antibodies β-actin, GAPDH, p27,
p16, CDK4, CDK2, E2F-1, p-Rb, CyclinD1, CyclinE1, PhosphoHistone H2A.X, Bax, and Bcl-2 were afforded by Cell Signaling
Technology (Beverly, MA, USA). Cleaved PARP, Cleaved
Caspase-3, and -9 were obtained from Abcam.
Instrumentation
Elemental analysis was performed on a Vario EL cube CHNs
analyzer (Elementar, Germany). A Matrix-Assisted Laser
Desorption/Ionization Time-of-Flight Mass spectrometer
(Bruker, Germany) was used. UV-vis spectra were recorded on
the Shimadzu UV2450-2550 spectrophotometer. Cell morphology and fluorescence imaging were observed using a
ZEISS Axio Observer A1 inverted fluorescence microscope.
Synthesis. General procedure for synthesizing ruthenium(III)
bis(amidine) complexes
An appropriate primary amine (2.1 mmol) was added to a solution of [RuIII(acac)2(NCCH3)2]2+ (0.21 mmol) in CH3CN
(50 mL), and the mixture was stirred for 5 h at room temperature. After the removal of the volatiles, the red solid was
washed with Et2O and recrystallized from CH3CN/Et2O at room
temperature.
cis-{RuIII(acac)2[NH(CH3)NH(CH2)3(CH3)2](ClO4)} [1](ClO4).
Yield (85%). Anal. calcd for C22H42ClN4O8Ru: C, 42.14; H, 6.75;
N, 8.93; found: C, 42.33; H, 6.93; N, 8.65. MALDI-TOF MS: (M+)
528.
cis-{RuIII(acac)2[NH(CH3)NH(CH2)5(CH3)2](ClO4)} [2](ClO4).
Yield (87%). Anal. calcd for C26H50ClN4O8Ru: C, 45.71; H, 7.38;
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N, 8.20; found: C, 45.57; H, 7.09; N, 7.91. MALDI-TOF MS: (M+)
584.
cis-{RuIII(acac)2[NH(CH3)NH(CH2)9(CH3)2](ClO4)} [3](ClO4).
Yield (82%). Anal. calcd for C34H66ClN4O8Ru: C, 51.34; H, 8.36;
N, 7.04; found: C, 51.04; H, 8.66; N, 7.16. MALDI-TOF MS: (M+)
696.
cis-{RuIII(acac)2[NH(CH3)NH(CH2)11(CH3)2](ClO4)} [4](ClO4).
Yield (80%). Anal. calcd for C38H74ClN4O8Ru: C, 53.60; H, 8.76;
N, 6.58; found: C, 53.63; H, 8.76; N, 6.38. MALDI-TOF MS: (M+)
752.
cis-{RuIII(acac)2[NH(CH3)NH(CH2)3(CH3)2](CF3SO3)}
[5]
(CF3SO3). Yield (81%). Anal. calcd for C23H42F3N4O7RuS: C,
40.82; H, 6.26; N, 8.28; found: C, 40.70; H, 6.06; N, 8.51.
MALDI-TOF MS: (M+) 528.
cis-{RuIII(acac)2[NH(CH3)NH(CH2)5(CH3)2](CF3SO3)}
[6]
(CF3SO3). Yield (84%). Anal. calcd for C27H50F3N4O7RuS: C,
44.25; H, 6.88; N, 7.65; found: C, 44.50; H, 6.92; N, 7.54.
ESI-MS: (M+) 584. Single crystals suitable for X-ray analysis
were obtained by slow diffusion of Et2O into a CH3CN solution
containing [6](CF3SO3) under ambient conditions.
X-ray crystallography
X-ray diffraction data of [6](CF3SO3) were collected on a ROD,
Synergy Custom system and HyPix Diffractometer (Rigaku,
Japan, Cu Kα, λ = 1.54184 Å) under 100 K. Data reductions were
performed on CrysAlisPro 1.171.41.123a (Rigaku Oxford
Diffraction, 2022). The structure solution was performed using
SHELXT and refinement with SHELXL within the
OLEX2 graphical interface.31–33 Restraints (SADI, DELU, and
SIMU) were applied for the disordered part. All non-hydrogen
atoms were refined first isotropically and then anisotropically.
All hydrogen atoms of the ligands were placed in calculated
positions with fixed isotropic thermal parameters and included
in the structure factor calculations in the final stage of fullmatrix least-squares refinement. CCDC no. 2223820† contains
the supplementary crystallographic data for this paper.
Cell culture
Cell culture media and supplements were purchased from
Gibco. Cells were cultured in Roswell Park Memorial Institute
(RPMI, 1640) or Dulbecco’s modified Eagle’s medium (DMEM)
supplemented with 10% FBS (fetal bovine serum), 1% penicillin–streptomycin, and 1% Glutamax at 37 °C, under an atmosphere of 5% CO2 and 95% air.
UV-Visible spectroscopy
The solvent stability of compounds 1–6 in DMSO and PBS was
investigated by UV-vis spectroscopy. The complexes were dissolved in DMSO or PBS (1% DMSO) and measured using a
UV2450-2550 spectrophotometer for 24 h. The data were
curved by GraphPad Prism 8 software.
Cytotoxicity MTT assay
Cells were cultured in 96-well plates at 6000 cells per well, followed by incubation at 37 °C for 24 h to allow attachment,
then the addition of dilutions of the test compounds, which
8546 | Dalton Trans., 2023, 52, 8540–8548
Dalton Transactions
were dissolved in DMSO while cisplatin was dissolved in water,
and incubation for 48 h. Cisplatin was introduced as a control.
The compound-containing medium was replaced by fresh
medium with 0.5 mg mL−1 MTT and incubated for 1.5 h. After
incubating, DMSO was added to each well when the medium
containing MTT was removed. The absorbance was measured
at 570 nm using Infinite M200 (Swiss, Tecan). IC50 values were
calculated from concentration-effect curves by logarithmic
interpolation using Origin 8. Each assay was carried out three
times, and the results are expressed as the mean ± SEM.
Plate colony formation assay
The NCI-H460 cells were seeded in 6-well plates (1000 cells per
well). After 24 h attachment, the cells were exposed to different
concentrations of compound 6 for 48 h. Then, after drug
washout and incubation for 7 d, the cells were fixed with 4%
paraformaldehyde for 20 min and stained with 1% crystal
violet solution for 30 min to observe colonies.
EdU incorporation assay
The EdU incorporation assay was performed using the EdU
Cell Proliferation Kit to test DNA synthesis. NCI-H460 cells
were inoculated in 12-well plates. After the cells were treated
with different concentrations of complex 6 for 24 h, the cells
were cultured with 20 µM EdU for 2 h. Hydroxyurea was used
as a positive control. After EdU labeling of the cells, 500 µL of
Click reaction solution was added to each well and incubated
at room temperature for 30 min in the dark. Then, the cells
were incubated with Hoechst 33342 to stain the cell nuclei.
Subsequently, the stained cells were washed with PBS and
observed with a ZEISS Observer A1 inverted fluorescence
microscope.
Calcein AM/PI staining
The living and dead cells were detected using the Calcein AM/
PI Cell Viability/Cytotoxicity Assay Kit. NCI-H460 cells were
seeded in 12-well plates and treated with complex 6 for 24 h.
Then the cells were washed with PBS and stained with Calcein
AM/PI working solution (1000×) for 30 min in the dark at
37 °C. Finally, the cells were washed with PBS twice and
observed under a ZEISS Observer A1 inverted fluorescence
microscope.
Cell cycle analysis
NCI-H460 cells were seeded in 6-well plates and treated with
8 μM 6 at various time intervals. Then, the cells were collected
and subsequently fixed with ice-cold 70% ethanol and kept at
4 °C for 24 h. Finally, the cells were washed with PBS, suspended in a PI solution (500 μL staining buffer, 12 μL RNase
(50×) and 25 μL propidium iodide (20×), and stained for
30 minutes at 37 °C in the dark. All samples were then analyzed using a flow cytometer.
Cell apoptosis assay
NCI-H460 cells were seeded into 6-well plates. Complex 6 (0.5,
1, 4, 8, and 10 μM) was added to the cells for 24 h treatment,
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or the cells were treated with 8 μM 6 for 6, 12, 24, 36, and 48 h.
Then, the cells were collected, centrifuged at 1000 rpm for
5 min, washed with PBS twice, resuspended in 500 μL binding
buffer (1×), and stained with 5 μL Annexin V and 5 μL propidium iodide for 10 min at room temperature. The flow cytometer was used for the analysis.
with a digital caliper by measuring the length (l) and width (w)
and calculating with the formula of V = lw2/2. Meanwhile, the
body weight of mice was measured and taken as a parameter
of systemic toxicity. On day 29, the animals were sacrificed and
the tumors were weighed and recorded.
ROS detection
Conflicts of interest
NCI-H460 cells were plated in 6-well plates and treated with
compound 6 at the required concentrations for 6 h. Rosup
(10 µM) was incubated for 20 min as a positive control. The
treated cells were collected and washed with a serum-free
medium three times. Then, the cells were stained with
10 µmol L−1 DCFH-DA for 20 min at 37 °C in the dark. At last,
the fluorescence intensity was detected using a flow cytometer
and ZEISS Observer A1 inverted fluorescence microscope.
MMP detection
NCI-H460 cells were cultured with complex 6 for 24 h at indicated concentrations. The treated cells were digested and collected. Then, the cells were incubated with JC-1 staining buffer
for 20 min at 37 °C in the dark. The cells were washed with
JC-1 washing buffer (1×) twice and analyzed by flow cytometry
to detect the red/green fluorescence intensity.
Western blot analysis
NCI-H460 cells were seeded in 6-well plates. After treatment
with 6 at different concentrations and times, the cells were
lysed in cell lysis buffer, which contains a protease inhibitor.
The protein was extracted and quantified using the BCA
Protein Assay Kit. The protein samples were separated on
8–15% SDS-PAGE and transferred onto a nitrocellulose membrane (BOSTER). After blocking with 5% nonfat milk for 1 h at
room temperature, the membranes were probed with the
primary antibody overnight at 4 °C and incubated with a secondary antibody (anti-rabbit or anti-mouse, 1 : 10 000) for 1 h
at room temperature. The target proteins were examined using
a High ChemiDoc XRS (Bio-Rad ChemiDoc XRS+, USA).
In vivo xenograft model
The mice were approved by the Animal Laboratory Center at
Shantou University Medical College; the license number is
SYXK2022-0079 (Guangdong, China). 3 × 106 NCI-H460 cells
were suspended with 0.1 mL of serum-free culture medium
and injected subcutaneously into the right flank region of
BALB/c-nu mice to establish the xenograft models. When the
xenograft tumor volume reached about 50–100 mm3, the mice
were randomly divided into solvent control and treatment
groups (n = 3 per group). Complex 6 was given via intravenous
tail injection every 4 days at 12.5 mg kg−1 (10% v/v PET/PBS).
PET solution = ( polyethylene glycol 400, 60%; ethanol 30%;
Tween 80, 10%). Cisplatin was given to mice at a dosage of
3 mg kg−1 and used as a positive reference for comparison.
Control mice received the solvent (10% v/v PET/PBS) via intravenous tail injection. The tumor size and body weight were
monitored every 2 d. The tumor volumes were determined
This journal is © The Royal Society of Chemistry 2023
There are no conflicts to declare.
Acknowledgements
This work was supported by the Guangdong Basic and Applied
Basic Research Foundation (No. 2019B030302009, No.
2023A1515011759) and the Li Ka Shing Foundation CrossDisciplinary Research Grant (2020LKSFG01F) to Dr Wenxiu
Ni. W. L. M. thanks the Research Grants Council of Hong
Kong (HKBU 12300121) and Hong Kong Baptist University
Tier-2 fund (RC-OFSGT2/20-21/SCI/008) for financial support.
We thank Shantou University Medical College.
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