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Synthesis and evaluation of iridium(III) complexes on antineoplastic activity against human gastric carcinoma SGC-7901 cells.
JBIC Journal of Biological Inorganic Chemistry (2022) 27:201–213
https://doi.org/10.1007/s00775-021-01922-3
ORIGINAL PAPER
Copper(II) and silver(I)‑1,10‑phenanthroline‑5,6‑dione complexes
interact with double‑stranded DNA: further evidence of their apparent
multi‑modal activity towards Pseudomonas aeruginosa
Anna Clara Milesi Galdino1,2 · Lívia Viganor1,3 · Matheus Mendonça Pereira4 · Michael Devereux3 ·
Malachy McCann5 · Marta Helena Branquinha1 · Zara Molphy6,7 · Sinéad O’Carroll6 · Conor Bain6 ·
Georgia Menounou6,7 · Andrew Kellett6,7 · André Luis Souza dos Santos1,2
Received: 29 March 2021 / Accepted: 13 December 2021 / Published online: 10 January 2022
© The Author(s) 2022
Abstract
Tackling microbial resistance requires continuous efforts for the development of new molecules with novel mechanisms of
action and potent antimicrobial activity. Our group has previously identified metal-based compounds, [Ag(1,10-phenanthroline-5,6-dione)2]ClO4 (Ag-phendione) and [Cu(1,10-phenanthroline-5,6-dione)3](ClO4)2.4H2O (Cu-phendione), with
efficient antimicrobial action against multidrug-resistant species. Herein, we investigated the ability of Ag-phendione and
Cu-phendione to bind with double-stranded DNA using a combination of in silico and in vitro approaches. Molecular docking revealed that both phendione derivatives can interact with the DNA by hydrogen bonding, hydrophobic and electrostatic
interactions. Cu-phendione exhibited the highest binding affinity to either major (− 7.9 kcal/mol) or minor (− 7.2 kcal/
mol) DNA grooves. In vitro competitive quenching assays involving duplex DNA with Hoechst 33258 or ethidium bromide
demonstrated that Ag-phendione and Cu-phendione preferentially bind DNA in the minor grooves. The competitive ethidium bromide displacement technique revealed Cu-phendione has a higher binding affinity to DNA (Kapp = 2.55 × 106 M−1)
than Ag-phendione (Kapp = 2.79 × 105 M−1) and phendione (Kapp = 1.33 × 105 M−1). Cu-phendione induced topoisomerase
I-mediated DNA relaxation of supercoiled plasmid DNA. Moreover, Cu-phendione was able to induce oxidative DNA injuries with the addition of free radical scavengers inhibiting DNA damage. Ag-phendione and Cu-phendione avidly displaced
propidium iodide bound to DNA in permeabilized Pseudomonas aeruginosa cells in a dose-dependent manner as judged by
flow cytometry. The treatment of P. aeruginosa with bactericidal concentrations of Cu-phendione (15 µM) induced DNA
fragmentation as visualized by either agarose gel or TUNEL assays. Altogether, these results highlight a possible novel
Anna Clara M. Galdino and Lívia Viganor have contributed
equally to this work.
Andrew Kellett and André L. S. Santos share the senior
authorship.
* Andrew Kellett
andrew.kellett@dcu.ie
4
CICECO—Aveiro Institute of Materials, Department
of Chemistry, University of Aveiro, Aveiro, Portugal
* André Luis Souza dos Santos
andre@micro.ufrj.br
5
Chemistry Department, Maynooth University, Kildare,
Ireland
6
School of Chemical Sciences and The National Institute
for Cellular Biotechnology, Dublin City University, Dublin,
Ireland
7
SSPC, The SFI Research Centre for Pharmaceuticals, School
of Chemical Sciences, Dublin City University, Glasnevin,
Dublin 9, Ireland
1
Department of General Microbiology, Institute
of Microbiology Paulo de Góes, Universidade Federal
do Rio de Janeiro, Rio de Janeiro, Brazil
2
Institute of Chemistry, Postgraduate Program
in Biochemistry, Universidade Federal do Rio de Janeiro,
Rio de Janeiro, Brazil
3
The Centre for Biomimetic and Therapeutic Research, Focas
Research Institute, Technological University Dublin, Dublin,
Ireland
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Vol.:(0123456789)
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JBIC Journal of Biological Inorganic Chemistry (2022) 27:201–213
DNA-targeted mechanism by which phendione-containing complexes, in part, elicit toxicity toward the multidrug-resistant
pathogen P. aeruginosa.
Graphical abstract
Keywords Pseudomonas aeruginosa · Coordination compounds · Antimicrobial action · DNA binding · DNA oxidative
damage · Mechanism of action
Introduction
The therapeutic application of metal-based complexes has
emerged against a multitude of human pathological disorders
[1, 3]. These treatments range from cisplatin in antineoplastic chemotherapy, gold-coordinated compounds for slowing
the progression of rheumatoid arthritis, bismuth-based drugs
for the treatment of ulcers, antimony-based metallodrugs in
antiparasitic therapy, and silver-containing compounds with
antimicrobial action [1–4].
1,10-Phenanthroline (1,10-phen) is a promising ligand in
the development of new metal-based compounds [5, 6]. The
rigid structure of the aromatic rings of 1,10-phen facilitates
the formation of stable complexes with metal ions, thereby
enabling the synthesis of a wide variety of coordination
compounds [7, 8]. Moreover, the extension of the 1,10-phen
backbone at the -5,6-position allows for efficient modulation of its antimicrobial action [6, 9]. With the addition of
an o-quinoid group at the -5,6-position on the 1,10-phen
backbone, 1,10-phenanthroline-5,6-dione (phendione) has
exhibited increased antimicrobial activity when compared to
1,10-phen [10, 11]. Phendione-based complexes have demonstrated excellent antiproliferative activity against the: metronidazole-resistant Trichomonas vaginalis [12], dematiaceous fungus Phialophora verrucosa [13], clinically relevant
yeast Candida albicans [14, 15], multidrug-resistant strains
of Candida haemulonii species complex [16], filamentous
fungus Scedosporium apiospermum [17], Escherichia coli
[18], methicillin-resistant Staphylococcus aureus [18], carbapenemase-producing Acinetobacter baumannii [19], and
multidrug-resistant bacterium Pseudomonas aeruginosa [9].
In general, both 1,10-phen- and phendione-based complexes
can interact with DNA by semi-intercalating or electrostatically
13
binding in the minor groove. Several of these complexes can
induce DNA damage by cleaving DNA [20–23]; however, they
may also cause indirect injuries through structural distortion
thereby affecting the machinery that maintains DNA integrity
[24, 25]. Gopu et al. [26] showed that (BOPIP = {2-(4-(benzyloxy)phenyl)-1H-imidazo[4,5-f]1,10-phen}) and its mononuclear Ru(II) polypyridyl complexes exhibited a significant
antiproliferative activity against human tumor cell lines (A549,
Du145, HeLa), as well as inhibiting the growth of E. coli and
S. aureus. The formation of DNA adducts with Ru(II)-complexes and the DNA damage induced by these compounds play
a significant role in their anticancer and antimicrobial activity
[26]. The antimicrobial action of lanthanide phendione-based
complexes, ([Eu(TFN)3(phendione)], [Eu(HFT)3(phendione)]
and [Yb(HFA)3(phendione)]), against E. coli, S. aureus and
Proteus penneri were recently correlated to their binding to
the bacterial DNA [27].
The current study first aimed to investigate whether
[Cu(phendione)3](ClO4)2.4H2O and [Ag(phendione)2]ClO4
were able to interact with double-stranded DNA using in
silico and in vitro approaches. The ability of these test
compounds to cleave DNA and to inhibit topoisomerase
I activity was also evaluated. Finally, we investigated the
possible interaction of both complexes with P. aeruginosa
chromosomal DNA which could explain, at least in part, the
antimicrobial action recently identified against this clinically
relevant human pathogen [11].
�JBIC Journal of Biological Inorganic Chemistry (2022) 27:201–213
Materials and methods
Test compounds
1,10-Phen was obtained from Sigma-Aldrich (USA), and
phendione, [Ag(phendione) 2]ClO 4 (Ag-phendione) and
[Cu(phendione)3](ClO4)2.4H2O (Cu-phendione) (Fig. 1A)
were prepared as previously reported [28, 29].
Molecular docking
Molecular docking analysis of DNA with 1,10-phen, phendione, Ag-phendione and Cu-phendione were calculated
using AutoDock Vina 1.1.2 program [30]. The 3D atomic
coordinates of the test compounds were computed by Discovery Studio, v20 (Accelrys, USA) and their rigid root was
generated using AutoDockTools (ADT) [31], setting all possible rotatable bonds defined as active by torsions. In addition, ADT was used to prepare the receptor (DNA–PDB:
1bna) input file by merging non-polar hydrogen atoms,
adding partial charges and atom types. The grid center at
the center of mass (x-, y-, and z-axes) of DNA major and
minor groove was 21.416 Å × 19.370 Å × 8.812 Å and
203
6.936 Å × 19.732 Å × 11.931 Å, respectively. The grid dimension used for DNA major groove was 18 Å × 38 Å × 24 Å and
minor groove was 16 Å × 34 Å × 32 Å. The binding model was
searched out from 10 different conformers for each ligand.
Electrospray ionization mass spectrometry (ESI–MS)
analyses
ESI–MS spectra were recorded using a Thermo Fisher
Exactive Orbitrap mass spectrometer coupled to an Advion
TriVersa Nanomate injection system with samples prepared
as described below. Accurate mass spectrometry was conducted on a MaXis HD quadrupole electrospray time-offlight (ESI-QTOF) mass spectrometer (Bruker Daltonik
GmbH, Bremen, Germany), using a glass syringe (Hamilton) and syringe pump (KD Scientific, Model 781100) for
infusions at a flow rate of 3 μL/min. Analyses were performed in ESI positive mode with the capillary voltage was
set to 4500 V, nebulizing gas at 0.6 bar, drying gas at 4 L/
min at 180 °C in each case. The TOF scan range was from
75 to 1600 mass-to-charge ratios (m/z). The MS instrument
was calibrated using an infusion of sodium formate calibrate solution. The calibrant solution consisted of 3 parts of
1 M NaOH to 97 parts of 50:50 water:isopropanol with 2%
Fig. 1 Molecular structures of
1,10-phenanthroline (1,10phen), 1,10-phenanthroline5,6-quinone (phendione)
along with copper(II) and
silver(I) phendione (A). Major
and minor grooves of DNA
molecules and the best docking
poses for DNA with the test
compounds (B)
13
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formic acid. Data processing was performed using the Compass Data Analysis software version 4.3 (Bruker Daltonik
GmbH, Bremen, Germany).
To study the stability of Cu(II) complexes, ESI–MS studies were performed in situ in the absence of reductant over
72 h. Accurate mass spectrometry analyses was carried out
using the method described by McStay et al. [32]. Briefly,
in a total volume of 1 mL, stock solutions of 1,10-phen or
phendione (4 mM) in THF:H2O, 50:50 were mixed with
copper(II) nitrate trihydrate (1.3 mM) in ratio 3:1. Samples
were incubated at 37 °C for 30 min and further dilution was
made as required to perform ESI–MS analysis (to reach
a final concentration of 1 mg/mL). ESI–MS spectra were
recorded at time points: 0 h, 24 h, 48 h, and 72 h.
To study the solution stability of both copper complexes
during redox processes, a second experiment was designed
to monitor both complexes in situ in the presence of reductant Na-L-ascorbate (Na-L-asc). Both complexes were prepared as described above and spectra were recorded before
and after reduction with 3 mM Na-L-asc (t = 0 h). After 24 h,
a second titration of 3 mM Na-L-asc was performed and the
spectra for each solution recorded. At 48 h, ESI–MS spectra
were recorded before and after a third addition of 3 mM of
Na-L-asc. A final measurement was then taken at 72 h.
DNA‑binding studies
JBIC Journal of Biological Inorganic Chemistry (2022) 27:201–213
aliquots were added until the fluorescence was 30–40% of
the initial control. Each drug concentration was measured
in triplicate, on at least two independent experiments. From
a plot of fluorescence versus added drug concentration, the
Q value is given by the concentration required to effect 50%
removal of the initial fluorescence of the bound dye [28].
Topoisomerase I inhibition assay
pUC19 plasmid DNA (400 ng; NEB, N3041) was
exposed to increasing concentrations of each complex
(2.5–400 µM) for 30 min at 20 °C in a final volume of
20 µL containing 80 mM HEPES buffer, 10 × CutSmart®
buffer, and 100 × BSA (NEB). One unit of topoisomerase
I (E. coli) (NEB) was added to the mixture and incubated
for 20 min at 37 °C. The reaction was stopped through the
addition of 0.25% SDS and 250 µg/mL protein kinase and
further incubated for 30 min at 50 °C. The 6 × loading dye
was added and topoisomers of DNA were separated by
electrophoresis in 1 × TBE buffer for 180 min/40 V and
150 min/50 V. The agarose gel (1.2%) was post-stained
using an EtBr bath and photographed using a SynGene
G:BOX mini6 [34].
DNA damage studies
DNA cleavage in the absence of reductant
Competitive ethidium bromide (EtBr) displacement
To analyze the binding affinity between DNA and test compounds, the competitive EtBr (Sigma-Aldrich) displacement
was employed as previously reported [33]. Briefly, a solution
of 20 µM calf thymus DNA (ctDNA, Invitrogen 15633-019,
Ɛ260 = 12.824 M (bp)−1/cm) and 25.2 µM EtBr was prepared
in 80 mM HEPES buffer and 40 mM NaCl, pH 7.2. The
test compounds were prepared in DMSO at 4 mM. Assays
were carried out in 96-well microplates (Corning, USA)
and the fluorescence readings were recorded (Ex: 530 nm,
Em: 590 nm; Bio-Tek Synergy HT Multi-mode). Triplicate
titrations were performed, and the apparent binding constants were calculated using Kapp = Ke × 12.6/C50, where,
Ke = 9.5 × 106 M−1 and C50 is the concentration of test compounds required to reduce the EtBr fluorescence by half [33].
pUC19 (400 ng) was exposed to 10–75 µM of each complex in a final volume of 20 µL containing 80 mM HEPES
buffer and 25 mM NaCl. Reactions were incubated at 37 °C
in darkness for either 3 h (Cu-phendione) or 24 h (Agphendione). The 6 × loading dye was added to each sample
prior to loading on a 1% agarose gel containing 4 µL SYBR
Safe. Electrophoresis was carried out at 70 V for 60 min in
1 × TAE buffer and photographed.
DNA cleavage in the presence of reductant
pUC19 (400 ng) was exposed to varying concentrations
(5–50 µM) of Cu-phendione in the presence of 25 mM NaCl
and 1 mM Na-L-asc and incubated at 37 °C for either 30 or
60 min. Electrophoresis was carried out at 70 V for 60 min
in 1 × TAE buffer and photographed.
Fluorescence quenching of EtBr‑DNA and Hoechst
33258‑DNA
Kinetic DNA cleavage study
Experiments were conducted in accordance to the method
reported by Molphy et al. [28]. Fluorescence readings were
recorded using a Bio-Tek Synergy HT Multi-mode microplate reader at an excitation wavelength of 530 or 360 nm
and an emission wavelength of 590 or 460 nm for EtBr and
Hoechst fluorescence detection, respectively. Repeated
pUC19 (400 ng) was exposed to either 30 or 40 µM of
Cu-phendione in the presence of 25 mM NaCl and 1 mM
Na-L-asc. Incubation times varied from 10 to 60 min and
were performed at 37 °C in darkness. Electrophoresis was
conducted at 70 V for 60 min in 1 × TAE buffer and photographed. To quantify DNA damage using band densitometry,
13
�JBIC Journal of Biological Inorganic Chemistry (2022) 27:201–213
40 µM of Cu-phendione was exposed to DNA in the presence of Na-L-asc (10–60 min). This experiment was conducted in triplicate and band densitometry was analyzed
on the SynGene G:BOX mini6 using SynGene Gene Tools
software.
DNA cleavage in the presence of reactive oxygen species
(ROS) scavengers
pUC19 (400 ng) was treated with increasing complex
concentrations in the presence of 25 mM NaCl, 1 mM
Na-L-asc and a range of ROS scavengers: 4,5-dihydroxy1,3-benzenedisulfonic acid (Tiron, O
2•−, 10 mM), KI
•
(H2O2, 10 mM), DMSO ( OH, 10%) and D2O (1O2, 10%)
in 80 mM HEPES. Reactions were incubated at 37 °C for
60 min in darkness.
Displacement of propidium iodide (PI)
from the bacterial genomic DNA
Pseudomonas aeruginosa (ATCC 27853) cells were cultured
in LB broth at 37 °C for 24 h. Then, 106 colony-forming
units (CFUs)/mL in saline solution (0.85% NaCl) were
heated at 72 °C for 30 min to inactivate the bacteria and
allow for passive internalization of PI. The permeabilized
bacteria were incubated with 20 mM PI for 1 h in the dark
followed by three washes with saline. Subsequently, the
cells were incubated with each compound (50, 250, 500 and
1000 mM) for 1 h. Finally, the fluorescence reading from
each sample was analyzed in a flow cytometer (FACS Calibur, BD Bioscience, USA) equipped with a 15-mW argon
laser emitting at 488 nm. The reduction of fluorescence
of the treated systems compared to the untreated control
reflects the displacement of the PI bound to the bacterial
DNA by the compounds [35].
Bacterial genomic DNA fragmentation
First, bacteria ( 106 CFUs/ml) were grown in LB broth in the
absence and in the presence of 2 × MIC value (15 μM) [11]
of Cu-phendione [9] or H2O2 (17.5 mM) for 5 h at 37 °C
under shaking (150 rpm). Bacteria were then harvested by
centrifugation (4000 × g/10 min/4 °C) and washed with
saline (3 ×). To evaluate bacterial genomic DNA integrity
by electrophoretic mobility, the genomic DNA was extracted
using the Gentra Puregene Yeast and Bacteria Kit (Qiagen,
USA) according to the manufacture instructions. DNA samples were subjected to electrophoresis (1% agarose gel in
TBE buffer) for 90 min at 100 V and then stained using an
EtBr bath and photographed.
205
TUNEL assay
Bacteria grown in LB broth as reported above were fixed
with 4% paraformaldehyde for 30 min. DNA fragmentation was evaluated using the DeadEndTM Fluorometric
TUNEL System Kit (Promega, USA) following the manufacturer's recommendations and then analyzed by flow
cytometry. The data obtained were analyzed using Flowing
software 2.5.1.
Statistics
The results were evaluated by analysis of variance (ANOVA)
and Dunnett’s multiple comparison tests using GraphPad
Prism 8 computer software (GraphPad Software Inc., USA).
In all analyses, p values ≤ 0.05 were considered statistically
significant.
Results and discussion
Copper‑ and silver‑phendione complexes interact
with double‑stranded DNA: in silico experiments
Molecular docking analysis was performed to identify interactions and binding affinities of 1,10-phen, phendione, Agphendione and Cu-phendione with both major and minor
grooves of double-stranded DNA. The best docking poses
for DNA with each compound were visualized (Fig. 1B).
Details of the best binding simulations and docking affinities, nucleic acid interactions, type of interaction and geometry distance of each ligand and double-stranded DNA were
displayed in the Supporting Material (Tables S1 and S2).
The results showed that test compounds were able to bind
to the DNA by means of hydrogen bonds and hydrophobic
interactions. In addition, Cu-phendione displayed the ability
to promote electrostatic interactions with DNA molecules.
Conversely, the interactions of DNA minor grooves with
1,10-phen and phendione were based on hydrogen bonds.
Ag-phendione and Cu-phendione showed particular behaviors, exhibiting additional ability to establish hydrogen
bonds and electrostatic interactions with the minor groove.
Hydrophobic interactions were only observed between Cuphendione and DNA molecules. Kamran et al. [36] have
applied computational methods to investigate the interaction
of DNA and binuclear Cu(II) complexes represented by the
general formula {(DMSO)Cu(µ-L)4Cu(DMSO)} and {(1,10phen)(L)Cu(µ-L)2Cu(L)(1,10-phen)}, where L = 2-bromophenyl acetate. It was observed that both binuclear Cu(II)
complexes formed H–π interaction with adenine and guanine
residues of the DNA [36].
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JBIC Journal of Biological Inorganic Chemistry (2022) 27:201–213
Copper‑ and silver‑phendione complexes interact
with double‑stranded DNA: in vitro analysis
DNA-binding constants of the Ag-phendione and Cu-phendione were determined indirectly by high throughput saturation binding analysis (Fig. 2, Table 1) that employs the heterocyclic EtBr as a reporter molecule. The method involved
treating calf thymus DNA (ctDNA; 20 µM) in 80 mM
HEPES buffer (pH 7.2) containing 40 mM NaCl with a saturated concentration of EtBr (25.2 µM) prior to the titration
of tested complex. Both Ag-phendione and Cu-phendione
were found to bind ctDNA with Kapp values of ca. 2.8 × 105
%
% Fluorescence
Fluorescense
A
1,10-phen
Phendione
Ag-phendione
Cu-phendione
100
50
0
200
400
600
800
1000
Compounds (µM)
B
% Fluorescense
Fluorescence
Compounds
Actinomycin D
[28]
Netropsin [28]
1,10-phen
Phendione
Ag-phendione
Cu-phendione
Q EtBr
100
1,10-phen
Phendione
Ag-phendione
Cu-phendione
50
0
0
200
400
600
800
1000
Compounds (µM)
C
Q Hoechst
100
1,10-phen
Phendione
Ag-phendione
Cu-phendione
50
0
0
200
400
600
800
1000
Compounds (µM)
Fig. 2 Interaction between 1,10-phen and phendione-based compounds and calf thymus DNA (ctDNA). Competitive EtBr displacement assays (A), fluorescence quenching of EtBr (B), and Hoechst
33258 (C) with ctDNA. Fluorescence readings were recorded in a
microplate reader and expressed as the percentage of fluorescence
in comparison to each control, which was read in the absence of the
test compounds. The dashed lines represent 50% fluorescence of control. Data points are presented as an average of triplicate measurements ± SD
13
C50 (μM)a Kappb
Q EtBrc Q Hoechst (µM)c
4.1
2.92 × 107
4.8
26.3
46.27
941.0
899.1
429.0
46.9
2.50 × 106
1.27 × 105
1.33 × 105
2.79 × 105
2.55 × 106
20.0
659.9
648.8
482.2
100.7
2.4
768.6
664.0
274.4
66.0
Apparent ctDNA binding constants (Kapp) determined using competitive ethidium bromide (EtBr) quenching and fluorescence quenching (Q) of DNA bound with either EtBr or Hoechst 33258. Classical DNA-binding drugs of actinomycin D and netropsin tested under
identical conditions [28] are provided for reference
a
0
Fluorescence
% Fluorescense
Table 1 DNA-binding properties
b
c
C50 = concentration required to reduce fluorescence by 50%,
Kapp = Ke × 12.6/C50 where Ke = 9.5 × 106 M (bp)−1,
Q = displacement of 50% initial fluorescence from DNA-bound dye
and 2.6 × 106 M−1, respectively (note: Kapp = Ke × 12.6/C50,
where Ke = 9.5 × 106 M−1 and C50 is the concentration of
test compounds required to reduce the EtBr fluorescence
by half). The binding constants are in line with a number of
Cu(II)-phenanthroline systems previously reported [36] and
it should also be noted that the influence of charge may play
a role in the higher binding affinity associated with the Cuphendione complex, which carries a 2+ cationic charge. Furthermore, the binding constant of Cu-phendione is similar to
that identified for the minor groove binding agent netropsin
tested under similar conditions but is an order of magnitude
lower that actinomycin D (Table 1) [33]. Competitive fluorescence quenching experiments in the presence of limited
bound Hoechst 33258 (minor groove binder) or EtBr were
carried out to identify a preference for DNA-binding sites.
This experiment revealed a preference for both complexes
to bind ctDNA at the minor groove as quenching (Q) values
obtained in the presence of Hoechst 33258 were over half
that of concentrations required to quench fluorescence in the
presence of EtBr. A similar effect was reported in a series of
bis-chelate Cu2+-phenanthroline–phenazine cationic complexes, where the systematic extension of the ligated phenazine ligand was found to influence DNA recognition [28]. In
accordance, it was demonstrated that the copper 1,10-phenderivative has a higher binding affinity to DNA than the
1,10-phen itself [38]. That study reported 1,10-phen (up to
200 μM) had little effect on ctDNA pre-exposed to EtBr
fluorogenic dye [38]. However, the addition of ([Cu(1,10phen)x]2+) to DNA system reduced the QEtBr to 2.7 μM, suggesting that the interaction between 1,10-phen and DNA is
dependent on the presence of a metal ion. Furthermore, Cuphendione exhibited the lowest concentration that inhibits
50% fluorescence (QEtBr = 100.7 μM and QHoechst = 66.0 μM),
�JBIC Journal of Biological Inorganic Chemistry (2022) 27:201–213
which suggests that this compound has a dual-mode of interaction with DNA, being able to intercalate into the compact array of stacked bases as well as partially groove bind
to the DNA. Previously, it was reported that [Ag(PDT)2]
ClO4.2MeOH and [Cu(PDT)2](ClO4)2 displayed high DNAbinding affinities (Kapp = 7.60 × 106 M−1 and 7.62 × 106 M−1,
respectively), and similarly to Cu-phendione, [Ag(PDT)2]
ClO4.2MeOH and [Cu(PDT)2](ClO4)2 were able to act as
intercalators and as a minor groove binders (respectively,
Q EtBr = 18.2 μM and 18.6 μM, Q Hoechst = 24.7 μM and
18.0 μM) [33]. Likewise, Kellett et al. [39] reported that both
[Cu(ph)(1,10-phen)]0.2H2O and [Cu(ph)(2,2’-bipy)]0.2H2O
(where ph = o-phthalate) bind to duplex DNA as either a
semi-intercalating agent or by binding to the minor groove
(Kapp = 1.2 × 105 M−1 and 1.1 × 105 M−1, respectively).
Cu‑phendione induces topoisomerase I‑mediated
DNA relaxation
To characterize the intercalative activity of the Ag-phendione and Cu-phendione, the topoisomerase I-mediated DNA
relaxation assay was performed on supercoiled (SC) plasmid DNA (Fig. 3A). Plasmid unwinding by both complexes
was examined between 0.5 and 400 µM. Cu-phendione was
found to first unwind negatively SC DNA prior to introducing DNA damage at concentrations greater than 50 µM.
This effect has also been observed in mono-nuclear systems
including Cu-TPMA-N,N’ (where N,N’ = 1,10-phen, DPQ
and DPPZ) and in di-nuclear Cu(II) systems such as CuOda and Cu-Terph [40, 41]. In the presence of increasing
concentrations of Ag-phendione, pUC19 became wound in
207
the opposite direction with positive supercoils observed at
10 µM. This electrophoretic mobility shift assay revealed
Ag-phendione treated DNA remained intact up to the maximum exposure concentration (400 µM).
Cu‑phendione promotes oxidative DNA damage
A number of experimental conditions were explored during DNA damage investigations of both metal-phendione
complexes including the (i) presence/absence of exogenous
reductants, (ii) complex exposure concentration/duration and
(iii) influence of scavenging species. First, the DNA damage
profiles of both complexes were assessed in the absence of
reductant. Over a 24-h exposure period, Ag-phendione failed
to induce damage up to 75 µM and it was, therefore, not
further investigated (Fig. 3B). As anticipated, Cu-phendione
was more active and found to cleave SC plasmid to OC at
30 µM in a shorter time frame (3 h) in the absence of reductant (Fig. 3C). In the presence of exogenous reductant (1 mM
Na-L-asc), the active Cu(I) species catalyzes the production
of ROS at the DNA interface resulting in enhanced oxidative chemical nuclease activity. A 30-min incubation carried
out in the range of 5–50 µM Cu-phendione resulted in the
stepwise conversion of SC DNA to both OC and L forms,
with three isoforms becoming visible at 40 µM treatment
(Fig. 4A, lane 6). A follow-up experiment was conducted
where the time frame was extended out to 60 min and it
was again possible to detect SC, OC and L forms, but at a
lower complex concentration of 30 µM (Fig. 4B, lane 5). In
an effort to improve separation of DNA isoforms, a kinetic
experiment was preformed, where 400 ng of plasmid was
Fig. 3 Release of topological tension from supercoiled
pUC19 using the topoisomerase
I-mediated relaxation assay
in the presence Ag-phendione
(A) or Cu-phendione (B).
pUC19 treated with increasing
concentrations of Ag-phendione
in the absence of reductant over
24 h (C). pUC19 treated with
increasing concentrations of
Cu-phendione in the absence of
reductant over 3 h (D)
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JBIC Journal of Biological Inorganic Chemistry (2022) 27:201–213
Fig. 4 pUC19 DNA treated with
increasing concentrations of Cuphendione for 30 min (A) and
60 min (B) in the presence of
1 mM Na-L-ascorbate. Kinetic
DNA damage study over 60 min
in the presence of reductant
at 30 µM (C) and 40 µM (D)
Cu-phendione exposure. DNA
densitometry analysis of pUC19
treated with 40 µM Cu-phendione over 60 min (E)
treated with 30 µM Cu-phendione with measurements taken
every 10 min for a total of 60 min; however, no significant
enhancement in separation was observed (Fig. 4C). The concentration in the kinetic experiment was increased to 40 µM
with three isoforms of pUC19 plasmid DNA qualitatively
observed by electrophoresis (Fig. 4D). The experiment was
repeated in triplicate (Fig. S1) and isoforms were quantitatively determined by band densitometry analysis (Fig. 4E).
Traces of all three DNA isoforms were detected between 20
and 40 min complex exposures. At 50 min of Cu-phendione
exposure, SC DNA was fully depleted and plasmid DNA
was fully converted to OC and L forms.
To shed further light on the ROS species involved in
DNA damage by Cu-phendione, oxidative DNA cleavage
was triggered in the presence of a variety of ROS specific scavengers and stabilizers including tiron ( O 2•−),
D-mannitol (•OH), KI ( H2O2) and D
2O (1O2 stabilizer).
13
A preliminary study indicated that •OH, H 2O 2 and 1O 2
play only a minor role in oxidative mechanism of Cuphendione and they were not further investigated (data
not shown). However, when the O
2•− radical was scavenged by tiron, DNA damage was significantly impeded.
Sequestering the superoxide radical with tiron resulted in
significant protection of plasmid DNA. A delayed onset
of OC-DNA formation and protection of SC DNA were
particularly evident. It was also possible to visualize all
three isoforms (SC, OC and L) up to 75 µM of complex
exposure (Fig. 5, lanes 6–9). Sequestering the O2•− radical has been recently found to have a significant impact
on DNA damage induced by mono-nuclear Cu-TPMAphenanthrene and Cu-DPA-phenanthrene systems
[39]. Similarly, the nuclease activity of Cu-phen-CipA
(CipA = ciprofloxacin) was inhibited by KI ( H2O2 scavenger), NaN 3 ( 1O 2 scavenger), DMSO ( •OH scavenger)
and Tiron ( O2•− scavenger) [42]. Oxidative mechanisms
were crucial for the artificial metallo-nuclease activity
�JBIC Journal of Biological Inorganic Chemistry (2022) 27:201–213
209
Fig. 5 pUC19 DNA treated
with increasing concentrations
of Cu-phendione in the presence
of 1 mM Na-L-ascorbate (lanes
2–5) and 10 mM of scavenging
species Tiron (lanes 6–9) (A).
Representative band densitometry analysis of DNA isoforms in
the absence and in the presence
of Tiron (B)
of [Cu(DPQ)2(NO3)](NO3) (DPQ = dipyrido[3,2-f:2′,3′-h]
quinoxaline) [43].
Solution stability of Cu‑phen and Cu‑phendione
complexes
To identify reasons for the chemical nuclease activity of
Cu-phendione, detailed ESI–MS and UV–Vis absorbance measurements were undertaken and compared with
Cu-phen. Here, 1,10-phen or phendione (4 mM) were dissolved in THF:H2O (50:50) and incubated with copper(II)
nitrate trihydrate (1.3 mM) in a 3:1 molar ratio at 37 °C
for 30 min. Samples of each spectra were then recorded
every 24 h over a 72 h period where predominant species
of [Cu(phendione)2]2+ and [Cu(phen)3]2+ were characterized and remained stable over the time-course measurements
(Figs. S2 and S3). This experiment was then performed
using UV–Vis spectroscopy and no significant change to
the d–d absorbance properties of either complex solution
was observed over time (Fig. 6C). A second in situ ESI–MS
experiment was then undertaken where spectra of both 3:1
solutions were recorded after reduction with 3, 6, and 9 mM
of Na-L-asc introduced over 72 h (Fig. 6A, B). After addition
of 3 mM of ascorbate (t = 0 h) the [Cu(phendione)2]2+ cation
([M + 2H]+ = 243.07 m/z) diminishes (but is still detectable) while the [Cu(phen)3]2+ cation ( [M]+ = 301.56 m/z)
is consumed with concomitant generation of [Cu(phen)2]+
([M]+ = 423.06 m/z). The addition of a second aliquot of
3 mM of ascorbate at 24 h ablates the [Cu(phendione)2]2+
cation with no further changes to the Cu-phen solution
observed. Interestingly, after 48 h, the [Cu(phendione)2]2+
cation begins to re-emerge (Fig. 6A), while by comparison,
only a small fraction of the [Cu(phen)3]2+ and none of the
[Cu(phen)2]+ cation was detectable (Fig. 6B). The addition of a further aliquot of ascorbate (3 mM) at 48 h then
ablated [Cu(phendione)2]2+ and, in the phen solution, leads
to the formation of [Cu(phen)2]+. The final measurement at
72 h revealed partial re-emergence of [Cu(phendione)2]2+
(Fig. 6A) where, in parallel, a smaller fraction of
[Cu(phen)3]2+ and no detectable [Cu(phen)2]+ was found
(Fig. 6B). Results here suggest that although both complexes
form stable in situ species—namely Cu(II) bis-phendione
and Cu(II) tris-phen complexes—differences emerge in the
presence of a reductant. First, [Cu(phendione)2]2+ appears
to have greater solution stability and is less easily reduced
compared to [Cu(phen)3]2+. This phendione complex also
begins to re-emerge as the solution becomes oxidised over
48 h and 72 h periods. In contrast, very little of the initial
[Cu(phen)3]2+ complex regenerates and, after prolonged
incubation of 48 and 72 h, neither Cu(II) or Cu(I) phen
complexes are detectable. Although these conditions reveal
the [Cu(phendione)2]2+ complex is potentially more stable
than [Cu(phen)3]2+, care must be taken in interpreting these
in situ data in the absence of DNA.
Cu‑phendione interacts with pseudomonal DNA
and promotes oxidative damage
Having observed the in silico/in vitro interactions between
Cu-phendione and DNA molecules, the direct harmful
13
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JBIC Journal of Biological Inorganic Chemistry (2022) 27:201–213
Fig. 6 In situ ESI–MS analyses of 3:1 Cu(II):phendione after reduction with 3, 6, and 9 mM of Na-L-ascorbate over 72 h (A). In situ
ESI–MS analyses of 3:1 Cu(II):phen after reduction with 3, 6,
and 9 mM Na-L-ascorbate over 72 h (B). In situ UV–Vis stability study of 5 mM solutions of 3:1 Cu(II) nitrate:phen and Cu(II)
nitrate:phendione recorded in CH3CN:H2O (50:50) over 72 h (C)
action of this complex on pseudomonal DNA was investigated, since Cu-phendione had a powerful anti-P. aeruginosa action as previously reported by our group [9]. Initially,
P. aeruginosa cells were heat-inactivated to permeabilize
them without disrupting bacterial architecture, followed by
sequential incubation with the DNA intercalator PI and different concentrations of test compounds; finally, the fluorescent cells were analyzed by flow cytometry. Our results
revealed that 1,10-phen and phendione were not able to
significantly displace the PI dye from DNA, indicating the
weak or lack of interaction between these compounds and
bacterial DNA (Table 2). Contrarily, Ag-phendione and
Cu-phendione avidly displaced PI bound to pseudomonal
DNA in a typically dose-dependent manner; both complexes
at 1000 μM, for example, significantly reduced the cellassociated fluorescence around 51% and 62%, respectively
(Table 2).
Subsequently, the DNA fragmentation profile was verified by agarose gel using genomic DNA extracted from P.
aeruginosa cultures treated with bactericidal concentrations
of Cu-phendione [9]. After 5 h of treatment, the bactericidal
concentration of Cu-phendione (15 μM) and H2O2 (17 mM)
induced the fragmentation of P. aeruginosa genomic DNA,
as visualized in the agarose gel as a smear corresponding
to degradation of intact DNA molecules in small molecular
weight fragments (Fig. 7A). In parallel, Cu-phendione-mediated DNA fragmentation was confirmed by TUNEL assay.
This method relies on the attachment of modified nucleotides (FITC-labeled) into the 3'-hydroxyl terminal of DNA
double-strand breaks [44]. Similarly, both Cu-phendione and
H2O2 showed, respectively, an increase of 62.8% and 78.5%
in the incorporation of fluorescent nucleotides, revealing
the induction of oxidative DNA fragmentation (Fig. 7B).
The overproduction/accumulation of ROS can promote
the damage of pentose and nucleotides [45, 46]. Due to
the abstraction of a hydrogen atom from deoxyribose or
inadequate repair of oxidized nitrogenous bases, especially
8-oxoguanine, ROS production enhances double-stranded
DNA damage [45–47]. Herein, an increased level of fragmented DNA was observed in P. aeruginosa cells treated
with Cu-phendione. Similarly, the treatment of E. coli with
bactericidal antibiotics (β-lactams, fluoroquinolones and
aminoglycosides) showed higher levels of DNA oxidation
and fragmentation [48]. The treatment of C. albicans with
Ag-phendione induced extensive smearing of DNA, indicating non-specific cleavage of the DNA [25]. In addition,
several studies have reported that copper nanoparticles dramatically affect the bacterial redox systems that culminate
with DNA fragmentation [49–51].
13
Conclusions
The emergence of antimicrobial resistance is a severe publichealth threat worldwide. It was reported that at least 700,000
people die annually from multidrug-resistant infections, and
it was also estimated that the number of antimicrobial resistant-associated deaths could reach 10 million by 2050 [52].
�JBIC Journal of Biological Inorganic Chemistry (2022) 27:201–213
Table 2 Interaction between
phendione-based compounds
and pseudomonal DNA
211
Systems
Compounds
(µM)
Mean fluorescence
intensity
% Fluorescent cells
Bacterial cells
Bacterial cells + PI
Bacterial cells + 1,10-Phen
Bacterial cells + phendione
Bacterial cells + Ag-phendione
Bacterial cells + Cu-phendione
Bacterial cells + PI + 1,10-Phen
–
–
1000
1000
1000
1000
1000
500
250
50
1000
500
250
50
1000
500
250
50
1000
500
250
50
8.55 ± 0.07
32.85 ± 0.07
8.2 ± 0.07
8.1 ± 0.06
8.7 ± 0.07
9.0 ± 0.08
35.35 ± 4.31
35.95 ± 0.78
33.70 ± 3.11
24.55 ± 7.14
28.55 ± 1.48
30.30 ± 2.89
27.80 ± 1.41
32.90 ± 3.68
15.25 ± 0.07*
16.25 ± 0.50*
20.55 ± 1.06*
21.65 ± 2.90*
12.65 ± 0.07*
13.05 ± 0.07*
16.80 ± 2.40*
21.85 ± 0.07*
0.05 ± 0.07
63.05 ± 0.07
0.1 ± 0.07
0.1 ± 0.07
0.1 ± 0.07
0.1 ± 0.07
64.65 ± 2.47
65.10 ± 1.41
63.95 ± 2.47
54.10 ± 9.19
60.45 ± 0.35
61.40 ± 2.69
59.60 ± 1.56
63.51 ± 2.69
34.40 ± 0.28*
39.05 ± 0.64*
43.50 ± 3.54*
47.85 ± 6.01*
24.35 ± 0.35*
29.90 ± 0.14*
40.85 ± 4.45*
51.30 ± 0.85*
Bacterial cells + PI + phendione
Bacterial cells + PI + Ag-phendione
Bacterial cells + PI + Cu-phendione
B
H2O2
Cu-phendione
A
Control
*Significant difference of the treated systems compared to the control (P < 0.05—analysis of variance oneway (ANOVA) (Dunnett’s multiple comparison test)
TUNEL (MIF)
80
60
* P=0.018
* P=0.045
40
20
0
Control
Cu-phendione
H 2O2
Fig. 7 Cu-phendione induces oxidative DNA damage in P. aeruginosa. The fragmentation of pseudomonal DNA was evaluated by
the electrophoretic profile of genomic DNA (control) obtained from
ATCC 27853 cells cultured with either 2 × MIC of Cu-phendione or
17 mM H2O2 (A). Bacterial cells exposed to Cu-phendione (2 × MIC;
15 µM) or 17 mM H2O2 were labeled with the TUNEL probe for
DNA detection with the 3'-OH end; DNA fragmentation was evaluated by flow cytometry and expressed as mean fluorescence intensity (MFI) (B). Data points are displayed as an average of triplicate
measurement. The asterisks (∗ P < 0.05, one-way ANOVA, Dunnett’s
multiple comparison test) denote the statistically significant difference among Cu-phendione-treated and H
2O2-treated systems and the
untreated one
The current work aims to provide an understanding of the
interaction between phendione-derivative compounds and
DNA, which can at least in part highlight the antimicrobial
potential of Ag-phendione and Cu-phendione. Our group has
been investigating the biological activity of Ag-phendione
and Cu-phendione against both planktonic- and biofilmgrowing of P. aeruginosa cells [9]. Herein, we showed that
phendione-based compound, particularly Cu-phendione,
were able to interact with double-stranded DNA and promote oxidative damage. In addition, Cu-phendione promoted
damage in pseudomonal DNA. Reasons for this enhanced
activity may stem from the superior DNA-binding affinity
of Cu-phendione (Kapp = 2.55 × 106 M−1) compared to the
parent [Cu(1,10-phen)2]2+ complex (Kapp = 6.67 × 105 M−1)
[28]. Thus, it appears a combination of DNA binding and
redox activity is required to achieve appropriate intracellular
DNA cleavage. In vitro studies with pUC19 DNA can demonstrate cleavage activity by Cu(II) complexes—including
those with moderate/low binding affinity—however, in more
complex biological environments, the DNA-binding affinity of metal complexes becomes important and those with
higher affinity (in particular polynuclear complexes) often
produce significantly higher levels of intracellular DNA
damage [37]. Altogether, we conclude that the antimicrobial
13
�212
activity of Cu-phendione could, in part, be correlated with
the artificial metallo-nuclease activity of Cu-phendione.
Still, Ag-phendione was not able to induce oxidative damage to DNA, indicating that this molecule might rely on
other bactericidal mechanisms to kill P. aeruginosa cells.
The potential application of phendione-derivative compounds as antimicrobial agents was supported by in vivo
studies that showed that these compounds have non-mutagenic profile, and low toxicity in Swiss mice model (100%
survival ≤ 150 mg/kg) [10, 17], which opens a new avenue
in the search for biologically activity compounds especially
against widespread and multidrug-resistant bacterial pathogens like P. aeruginosa.
Supplementary Information The online version contains supplementary material available at https://d oi.o rg/1 0.1 007/s 00775-0 21-0 1922-3.
JBIC Journal of Biological Inorganic Chemistry (2022) 27:201–213
4.
5.
6.
7.
8.
9.
Funding Open Access funding provided by the IReL Consortium.
This study was supported by grants and fellowships from the Brazilian
Agencies: Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq), Fundação de Amparo à Pesquisa no Estado do Rio
de Janeiro (FAPERJ) and Coordenação de Aperfeiçoamento de Pessoal
de Nível Superior (CAPES—Financial code 001). Andrew Kellett and
Zara Molphy acknowledge funding from Science Foundation Ireland
Career Development Award (SFI-CDA) [15/CDA/3648]. This publication has emanated from research supported in part by a research
grant from Science Foundation Ireland (SFI) and is co-funded under
the European Regional Development Fund under Grant Number 12/
RC/2275_P2.
11.
Declarations
13.
10.
12.
Conflict of interest The authors declare no conflict of interest.
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