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Chemistry and Materials Research www.iiste.org
ISSN 2224- 3224 (Print) ISSN 2225- 0956 (Online)
Vol.7 No.10, 2015
11
Anticancer Activity of New Di-Nuclear Copper (I) Complex
Abeer A. Ibrahim1
Taghreed H. Al- Noor2
1.Department of Pathological Analysis, Technical College of Health, Sulaimani Polytechnic University,
Kurdistan Region-IRAQ
2.Department of Chemistry, Ibn -AI-Haithem College of Education, University of Baghdad, IRAQ
Abstract
In-vitro biological activities of the free new H4L ( indole-7-thiocarbohydrazone) ligand and its Ni(II), Pd(II) , Pt(II),
Cu(II), Ag(I), Zn(II) and Cd(II) complexes are screened against two cancerous cell lines, that revealed significant
activity only for [Cu2Cl2(H4L)2(PPh3)2] after 72 h treatment by the highest tested concentrations. The Copper(I)
complex was characterized by X-ray Crystallography and the NMR spectra, whereas it has been confirmed to have
momentous cytotoxicity against ovarian, breast cancerous cell lines (Caov-3, MCF-7). The apoptosis-inducing
properties of the Cu(I) complex have been investigated through fluorescence microscopy visualization, DNA
fragmentation analysis and propidium iodide flow cytometry.
Keywords: Cu(I) complex, biological investigation, anticancer activity & DNA fragmentation analysis.
Introduction:
Cancer is an imperative area of interest in the life sciences as it has been a prime assassin disease throughout
human history. It is not one disease, but a bulky group of diseases characterized by uncontrolled growth and spread
of abnormal cells. Heterocyclic molecules are distinguished to play a critical role in health care and pharmaceutical
drug design [1,2]. In the relevant annual reviews are to be found examples of metal ions in biological systems and
coordination chemistry for the series. Inorganic chemistry useful in the medical field can be divided into two main
categories: firstly, as metal ions to a target protein is free or whether the drugs as ligands; and secondly, metal-
based drugs and imaging agents of central metal ion is usually significant of the mechanism of action [3-5]. The
choice of the coordinated ligand(s) seems to be as vital as the choice of metal(s) because being the integral part of
biologically active complexes, in addition these organic molecules (ligands) can exert a biological activity of their
own [6-11]. Purine, thiosemicarbazone, imidazole, benzohydroxamic ligands as nitrogen donor ligands include
various types of anti-cancer activities of the range of simple copper complexes have been studied when some
metal-based antitumor drugs in vitro and in vivo studies have demonstrated greater antineoplastic power than
Cisplatin[12] . Copper complexes are behaved as the most promising option anticancer drugs as cisplatin, when
this idea supported by a number of research articles describing the synthesis, thus DNA binding and cytotoxic
activities of many copper complexes [13,14]. There are only few complexes of Copper(I) in the literature, whereas
they also be evidence for a very sturdy cytotoxic activity against tumor cells in vitro [15,16]. Anticancer activity
of Cu(I) complex is related to their ability to produce reactive oxygen species (ROS). Copper(I) ions can reduce
hydrogen peroxide to hydroxyl radical. Copper(II) ions may in turn be reduced to Cu(I) by superoxide anion(O2
•-
).
Consequently, it can be terminated that the production of reactive oxygen species such as OH•
are driven by the
Copper, in spite of the form in which it is initially introduced into the body Cu+
, or Cu2+
[17,18]. The hydroxyl
radical (OH•
) is supposed to be the main factor causing DNA damage in cells under oxidative stress [19-21]. Hence,
we emphasis to report the anticancer activity of new Copper(I) indole-7- thiocarbohydrazone complex .
Cu2+
+ O2
•–
→ Cu+
+ O2
Cu+
+ H2O2 → Cu2+
+ OH•
+ OH–
Experimental
The ligand (H4L) and its Cu(I) complex which were prepared and characterized according to the previously
described procedure [22]. The ligand(H4L) and its Cu(I) complex were evaluated for their in vitro cytotoxicity
towards human ovarian adenocarcinoma and breast cancer cell lines (Caov-3, MCF-7) respectively .
- Cell Culture
The cell lines (Caov-3, MCF-7) were provided by Department of Pharmacy, Faculty of Medicine, University of
Malaya. The cells were cultured in RPMI 1640 medium supplemented with 10% fetal bovine serum (Sigma
Aldrich) and L-glutamine at 37 °C in a 5% CO2 humidified atmosphere.
- MTT Cytotoxixity Test
MTT (3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide) assay was carried out as described by
Mosmann [23] with some modifications. The cells were seeded into 96-well plates (5000 cells/well) and allowed
to adhere overnight. Copper complex was pre-dissolved in dimethyl sulfoxide (DMSO) and diluted to the desired
concentrations (eight concentrations, 0.39-50 µg/mL), such that the final concentrations of DMSO did not exceed
0.5%. Each cell was treated with the test compound solutions (three wells on a plate for each concentration) for
24, 48 and 72 h. Treated and untreated cells were inspected qualitatively using an inverted light microscope (100
Chemistry and Materials Research www.iiste.org
ISSN 2224- 3224 (Print) ISSN 2225- 0956 (Online)
Vol.7 No.10, 2015
12
X). Then, 10 µl of MTT (5 mg/mL) was added to each well and the plates were incubated at 37 °C for 4 h. The
media was then gently aspirated, and 100 µl DMSO was added to dissolve the formazan crystals. The amount of
formazan product was measured spectrophotometrically at 570 nm using a microplate reader (Power Wave X 340).
The concentration of the test compound required for 50% inhibition of cell growth (IC50)was determined by
interpolation of regression analysis.
- Apoptosis Detection with Fluorescence Microscopy AO/PI Staining Assay
The cancer cell lines were seeded in a 25 mL culture-flask (1 × 106
cells/mL) and treated with the Copper complex
at the corresponding IC50 concentrations for 24, 48 and 72 h. The cells were washed with phosphate buffered saline
(PBS) and suspended in 500 µL of PBS followed by addition of a 1:1 mixture of Acridine orange (AO) 10 µg/ml
and propidium iodide (PI) 10 µg/ml. A drop of the suspension was placed on a glass slide and covered with a cover
slip. Images of the cells were taken by a UV-fluorescence microscope within 30 min.
- DNA-Fragmentation Analysis
The cancer cell lines were seeded in a 25 mL culture-flask (1 × 106
cells/mL) and treated with the respective IC50
concentrations of the test compound for 24, 48 and 72 h (control cells were treated with 0.5% DMSO vehicle).
The cells were then washed with PBS.The treated and control cells were washed with PBS and harvested. Cellular
DNA was extracted using the apoptotic DNA ladder detection kit (Chemicon International Inc., Palo Alto, CA,
USA). The DNA fragments were then separated by a 1.5% agarose gel electrophoresis at 50 V for 3 h.The Gels
were then stained with ethidium bromide and visualized on a UV-illuminator.
- Cell cycle analysis
A flow cytometry analysis was carried out to determine the cell cycle distribution in treated ovarian
adenocarcinoma (Caov-3) cell line with [Cu2(H4L)2(PPh3)2Cl2] [24]. In brief, (Caov-3, MCF-7) cell lines (5×104
cells/ml) were treated with [Cu2(H4L)2(PPh3)2Cl2] at IC50 concentration for 24, 48 and 72 h. After fixation with
cold ethanol, cells were washed with PBS and stained with PI (50 µl, 10 mg/ml) for 1 h at 37 ˚C. In addition,
RNase A (10 mg/ml) was also used to limit the ability of PI to bind only to DNA molecules. The stained cell was
analyzed for DNA content using flow cytometer (BD FACSCanto TM II).
Results and discussion
- Structure of the Copper(I) complex
The reaction of H4L with equimolar amount of CuCl and PPh3 afforded the Cu(I) complex of [Cu2Cl2(H4L)2(PPh3)2]
(Scheme 1). The crystal structure of the complex is shown in (Figure 1). The thiocarbohydrazone is almost planar
(r. m. s. deviation = 0.151 Å) and adopts an anti geometry. Two neutral thiocarbohydrazones, acting as µ2-S-donor
ligands, doubly bridge pairs of the Cu(I) atom into a centrosymmetric dimer. The Cu centers within the Cu2(µ2-S)2
core are separated by 3.0681(6) Å, which is larger than sum of their van der Waals radii (2.80 Å). One Cl atom
and one PPh3 group complete a distorted tetrahedral geometry around each metal center, with coordination angles
being ca. 96-119°.The geometric parameters of the parallelogram and those pertaining to the metal centers are
compatible with the reported values for similar structures [25-27]. The Cl atom is intramolecularly hydrogen
bonded to N3, and intermolecularly H-bonded to a methanol solvate molecule. Theoretical calculations on similar
dinucler Cu(I) structures suggested that the hydrogen bonding between the halogen ligands and the solvent
molecules plays a crucial role in the formation of S-bridged dimers vs. halogen-bridged or monomeric structures
[22,25] .
Figure 1 Molecular structure of [Cu2Cl2(H4L)2(PPh3)2] with thermal ellipsoids drawn at the 30% probability level.
C-bound H atoms and methanol solvent molecules are omitted for clarity. Symmetry code: i = -x+1, -y+1, -z+1.
Chemistry and Materials Research www.iiste.org
ISSN 2224- 3224 (Print) ISSN 2225- 0956 (Online)
Vol.7 No.10, 2015
13
Scheme 1. Synthesis of the Cu(I) complex
The Cu complex also characterized by 1
H , 13
C NMR and HSQC spectra in DMSO-d6 that in agreement
with the crystal structure, indicating the stability of the structure in the solution . The 13
C NMR spectrum shows
an upfield shift of the CS signal (∼3 ppm) from that in the spectrum of H4L. Yield 0.38 g, 53%. Anal. Calc. for
C74H62Cl2Cu2N12P2S2: C, 61.57; H, 4.33; N, 11.64. Found: C, 61.44; H, 4.08; N, 11.98%. 1
H NMR (DMSO-d6): δ
6.59 (2H, br.s, Ar-H); 6.65 (2H, br.s, Ar-H); 6.99 (2H, br.s, Ar-H); 7.16 (2H, t, J = 6.8 Hz, Ar-H); 7.24-7.48 (34H,
Ar-H); 7.58 (2H, br.s, Ar-H); 7.69(4H, m, Ar-H); 7.77 (2H, d, J = 7.7 Hz, Ar-H); 8.55 (2H, br.s, HCNN); 8.94
(2H, br.s, HCNN); 11.30 (2H, s, indole-NH); 11.33 (2H, s, indole-NH); 12.32 (2H, s, NNH); 12.55 (2H, s, NNH )
ppm. 13
C NMR (DMSO-d6): δ 102.86, 116.82, 117.92, 119.75, 119.84, 123.96, 124.14, 124.70, 126.44, 126.96,
127.14, 128.75-129.37, 130.48, 131.57, 133.71-133.96 (Ar); 149.89, 150.29 (HCNN); 172.43 (CS) ppm.
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Vol.7 No.10, 2015
14
- Cytotoxicity assay for Cu(I) complex
(Table1) lists the IC50 values of the Copper(I) complex after treating the (Caov-3, MCF-7) cancer cell lines for
24, 48 and 72 h. Based on outcomes that, the IC50 values were (13, 25.75) µM for 24 h treatment; however, the
value declined, in case of prolonged treatment, where, IC50 values were (10, 4.25) µM for 48 h treatment, and
further dropped to (4, 2.5) µM for 72 h treatment; which obviously signifies that, the prolonged treatment
considerably decreased the IC50 values, and elevated the toxic activity. For the purpose of comparability, ovarian
adenocarcinoma and breast cancer cell lines were also treated with cisplatin a clinical anticancer drug (Figure 5,
Figure 6 ), and the results presented in (Table1) that [Cu2(H4L)2(PPh3)2Cl2] revealed higher cytotoxicity than
cisplatin against the (Caov-3, MCF-7) cancer cell lines .
Table 1 IC50 (µM) values of [Cu2(H4L)2(PPh3)2Cl2] and cisplatin at different time (24, 48 and 72) h
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Vol.7 No.10, 2015
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- Apoptosis assay
Apoptosis initiation is an anti-proliferative mechanism by which the cancer cells go through programmed death.
Cells undergoing apoptosis are characterized by morphological and biochemical changes including cell shrinkage,
chromatin condensation and DNA fragmentation. Based on the results of the in vitro cytotoxicity assay
for [Cu2(H4L)2(PPh3)2Cl2], it was considered valuable to explore the apoptotic properties of the compound.
Apoptosis in the ovarian adenocarcinoma (Caov-3) and breast (MCF-7) cancer cell lines were screened through
fluorescence microscopy visualization and DNA fragmentation analysis and propidium iodide flow cytometry.
- Fluorescence microscopy visualization
Apoptotic cells display increased plasma membrane permeability to certain fluorescent dyes. Acridine orange
(AO)/propidium iodide (PI) is a fluorochrome mixture for nuclear staining which permits uniqueness between
viable, apoptotic and necrotic cells. In this work, the ovarian adenocarcinoma (Caov-3) plus breast cancer (MCF-
7) were subjected to AO/PI staining after treatment with respective IC50 concentrations of [Cu2(H4L)2(PPh3)2Cl2]
for 24, 48 and 72 h. Fluorescence microscopy exposes that in the (Caov-3, MCF-7) cancer cell lines the Copper
complex encouraged cell death fundamentally via apoptosis especially at 72h when the apoptotic cell
clearly observed (Figure 7, Figure 8).
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- DNA Fragmentation analysis
The degeneration of nuclear DNA into nucleosomal units is a biochemical feature of apoptosis. To evaluate the
apoptotic DNA fragmentation in the cancer cells, the ovarian and breast cancer cell lines were incubated with the
correspond IC50 value of [Cu2(H4L)2(PPh3)2Cl2] for 48 and 72 h. The cells were then lysed, the nuclear DNA was
extracted, and subjected to gel electrophoresis. Inspection of the electrophoretic profiles discovered a ladder
formation detected only at 72h at both of ovarian and breast cancer cells (fragments range from 400 to 1000 bp),
which signify the incidence of apoptosis (Figure 9, Figure 10).
- Cell cycle analysis
The DNA content of cells duplicates during the S phase, therefore cells in the G0 and G1 phases (before the S phase)
have unreplicated DNA, while those in the G2 and M phases (after the S phase) have replicated DNA. Analysis of
cell cycles by flow cytometry enables to distinguish and quantify the cells in different phases of the cell cycle. On
the flow cytometry DNA histograms cells with degraded and thus hypodiploid DNA are represented in so-called
“sub-G0/G1” peaks therefore, sub-G0/G1 is a specific marker of cell death by apoptosis [28,29]. Flow cytometry
analysis of the Caov-3, MCF-7 cancer cell lines after treatments with respective IC50 concentrations of the
[Cu2(H4L)2(PPh3)2Cl2] for 24, 48 and 72 h was carried out (Figure11, Figure12). Moreover, the histogram of Caov-
3 illustrates gradual increases in the populations of sub-G0/G1 phase during the incubation periods whereas the
histogram of MCF-7 illustrates gradual increases in the populations of G2/M phase In general, flow cytometry
suggests the induction of apoptosis by the Copper(I) complex in the Caov-3 cancer cell through G0/G1 phase while
through Sub-G0/G1 phase for MCF-7 cell cycle arrest.
Conclusion
As it was presented in this article, Copper(I) coordination complex has notable and cancer-selective cytotoxicity
against the Caov-3, MCF-7 cancer cell lines as inferred from the MTT-based IC50 values and different apoptotic
assay methods in consequence, Intensive research possibly will enable to apply it as anticancer drug.
ACKNOWLEDGMENTS
We would like to thank Mashitoh Abd Rahman and Hamed Karimian from Faculty of Medicine, University of
Malaya for their assistance with the biological data collection and analysis. Financial Support from the University
of Malaya ( PPP Grant Number PV048/2012A) is highly appreciated.
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Anticancer Activity of New Di-Nuclear Copper (I) Complex

  • 1. Chemistry and Materials Research www.iiste.org ISSN 2224- 3224 (Print) ISSN 2225- 0956 (Online) Vol.7 No.10, 2015 11 Anticancer Activity of New Di-Nuclear Copper (I) Complex Abeer A. Ibrahim1 Taghreed H. Al- Noor2 1.Department of Pathological Analysis, Technical College of Health, Sulaimani Polytechnic University, Kurdistan Region-IRAQ 2.Department of Chemistry, Ibn -AI-Haithem College of Education, University of Baghdad, IRAQ Abstract In-vitro biological activities of the free new H4L ( indole-7-thiocarbohydrazone) ligand and its Ni(II), Pd(II) , Pt(II), Cu(II), Ag(I), Zn(II) and Cd(II) complexes are screened against two cancerous cell lines, that revealed significant activity only for [Cu2Cl2(H4L)2(PPh3)2] after 72 h treatment by the highest tested concentrations. The Copper(I) complex was characterized by X-ray Crystallography and the NMR spectra, whereas it has been confirmed to have momentous cytotoxicity against ovarian, breast cancerous cell lines (Caov-3, MCF-7). The apoptosis-inducing properties of the Cu(I) complex have been investigated through fluorescence microscopy visualization, DNA fragmentation analysis and propidium iodide flow cytometry. Keywords: Cu(I) complex, biological investigation, anticancer activity & DNA fragmentation analysis. Introduction: Cancer is an imperative area of interest in the life sciences as it has been a prime assassin disease throughout human history. It is not one disease, but a bulky group of diseases characterized by uncontrolled growth and spread of abnormal cells. Heterocyclic molecules are distinguished to play a critical role in health care and pharmaceutical drug design [1,2]. In the relevant annual reviews are to be found examples of metal ions in biological systems and coordination chemistry for the series. Inorganic chemistry useful in the medical field can be divided into two main categories: firstly, as metal ions to a target protein is free or whether the drugs as ligands; and secondly, metal- based drugs and imaging agents of central metal ion is usually significant of the mechanism of action [3-5]. The choice of the coordinated ligand(s) seems to be as vital as the choice of metal(s) because being the integral part of biologically active complexes, in addition these organic molecules (ligands) can exert a biological activity of their own [6-11]. Purine, thiosemicarbazone, imidazole, benzohydroxamic ligands as nitrogen donor ligands include various types of anti-cancer activities of the range of simple copper complexes have been studied when some metal-based antitumor drugs in vitro and in vivo studies have demonstrated greater antineoplastic power than Cisplatin[12] . Copper complexes are behaved as the most promising option anticancer drugs as cisplatin, when this idea supported by a number of research articles describing the synthesis, thus DNA binding and cytotoxic activities of many copper complexes [13,14]. There are only few complexes of Copper(I) in the literature, whereas they also be evidence for a very sturdy cytotoxic activity against tumor cells in vitro [15,16]. Anticancer activity of Cu(I) complex is related to their ability to produce reactive oxygen species (ROS). Copper(I) ions can reduce hydrogen peroxide to hydroxyl radical. Copper(II) ions may in turn be reduced to Cu(I) by superoxide anion(O2 •- ). Consequently, it can be terminated that the production of reactive oxygen species such as OH• are driven by the Copper, in spite of the form in which it is initially introduced into the body Cu+ , or Cu2+ [17,18]. The hydroxyl radical (OH• ) is supposed to be the main factor causing DNA damage in cells under oxidative stress [19-21]. Hence, we emphasis to report the anticancer activity of new Copper(I) indole-7- thiocarbohydrazone complex . Cu2+ + O2 •– → Cu+ + O2 Cu+ + H2O2 → Cu2+ + OH• + OH– Experimental The ligand (H4L) and its Cu(I) complex which were prepared and characterized according to the previously described procedure [22]. The ligand(H4L) and its Cu(I) complex were evaluated for their in vitro cytotoxicity towards human ovarian adenocarcinoma and breast cancer cell lines (Caov-3, MCF-7) respectively . - Cell Culture The cell lines (Caov-3, MCF-7) were provided by Department of Pharmacy, Faculty of Medicine, University of Malaya. The cells were cultured in RPMI 1640 medium supplemented with 10% fetal bovine serum (Sigma Aldrich) and L-glutamine at 37 °C in a 5% CO2 humidified atmosphere. - MTT Cytotoxixity Test MTT (3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide) assay was carried out as described by Mosmann [23] with some modifications. The cells were seeded into 96-well plates (5000 cells/well) and allowed to adhere overnight. Copper complex was pre-dissolved in dimethyl sulfoxide (DMSO) and diluted to the desired concentrations (eight concentrations, 0.39-50 µg/mL), such that the final concentrations of DMSO did not exceed 0.5%. Each cell was treated with the test compound solutions (three wells on a plate for each concentration) for 24, 48 and 72 h. Treated and untreated cells were inspected qualitatively using an inverted light microscope (100
  • 2. Chemistry and Materials Research www.iiste.org ISSN 2224- 3224 (Print) ISSN 2225- 0956 (Online) Vol.7 No.10, 2015 12 X). Then, 10 µl of MTT (5 mg/mL) was added to each well and the plates were incubated at 37 °C for 4 h. The media was then gently aspirated, and 100 µl DMSO was added to dissolve the formazan crystals. The amount of formazan product was measured spectrophotometrically at 570 nm using a microplate reader (Power Wave X 340). The concentration of the test compound required for 50% inhibition of cell growth (IC50)was determined by interpolation of regression analysis. - Apoptosis Detection with Fluorescence Microscopy AO/PI Staining Assay The cancer cell lines were seeded in a 25 mL culture-flask (1 × 106 cells/mL) and treated with the Copper complex at the corresponding IC50 concentrations for 24, 48 and 72 h. The cells were washed with phosphate buffered saline (PBS) and suspended in 500 µL of PBS followed by addition of a 1:1 mixture of Acridine orange (AO) 10 µg/ml and propidium iodide (PI) 10 µg/ml. A drop of the suspension was placed on a glass slide and covered with a cover slip. Images of the cells were taken by a UV-fluorescence microscope within 30 min. - DNA-Fragmentation Analysis The cancer cell lines were seeded in a 25 mL culture-flask (1 × 106 cells/mL) and treated with the respective IC50 concentrations of the test compound for 24, 48 and 72 h (control cells were treated with 0.5% DMSO vehicle). The cells were then washed with PBS.The treated and control cells were washed with PBS and harvested. Cellular DNA was extracted using the apoptotic DNA ladder detection kit (Chemicon International Inc., Palo Alto, CA, USA). The DNA fragments were then separated by a 1.5% agarose gel electrophoresis at 50 V for 3 h.The Gels were then stained with ethidium bromide and visualized on a UV-illuminator. - Cell cycle analysis A flow cytometry analysis was carried out to determine the cell cycle distribution in treated ovarian adenocarcinoma (Caov-3) cell line with [Cu2(H4L)2(PPh3)2Cl2] [24]. In brief, (Caov-3, MCF-7) cell lines (5×104 cells/ml) were treated with [Cu2(H4L)2(PPh3)2Cl2] at IC50 concentration for 24, 48 and 72 h. After fixation with cold ethanol, cells were washed with PBS and stained with PI (50 µl, 10 mg/ml) for 1 h at 37 ˚C. In addition, RNase A (10 mg/ml) was also used to limit the ability of PI to bind only to DNA molecules. The stained cell was analyzed for DNA content using flow cytometer (BD FACSCanto TM II). Results and discussion - Structure of the Copper(I) complex The reaction of H4L with equimolar amount of CuCl and PPh3 afforded the Cu(I) complex of [Cu2Cl2(H4L)2(PPh3)2] (Scheme 1). The crystal structure of the complex is shown in (Figure 1). The thiocarbohydrazone is almost planar (r. m. s. deviation = 0.151 Å) and adopts an anti geometry. Two neutral thiocarbohydrazones, acting as µ2-S-donor ligands, doubly bridge pairs of the Cu(I) atom into a centrosymmetric dimer. The Cu centers within the Cu2(µ2-S)2 core are separated by 3.0681(6) Å, which is larger than sum of their van der Waals radii (2.80 Å). One Cl atom and one PPh3 group complete a distorted tetrahedral geometry around each metal center, with coordination angles being ca. 96-119°.The geometric parameters of the parallelogram and those pertaining to the metal centers are compatible with the reported values for similar structures [25-27]. The Cl atom is intramolecularly hydrogen bonded to N3, and intermolecularly H-bonded to a methanol solvate molecule. Theoretical calculations on similar dinucler Cu(I) structures suggested that the hydrogen bonding between the halogen ligands and the solvent molecules plays a crucial role in the formation of S-bridged dimers vs. halogen-bridged or monomeric structures [22,25] . Figure 1 Molecular structure of [Cu2Cl2(H4L)2(PPh3)2] with thermal ellipsoids drawn at the 30% probability level. C-bound H atoms and methanol solvent molecules are omitted for clarity. Symmetry code: i = -x+1, -y+1, -z+1.
  • 3. Chemistry and Materials Research www.iiste.org ISSN 2224- 3224 (Print) ISSN 2225- 0956 (Online) Vol.7 No.10, 2015 13 Scheme 1. Synthesis of the Cu(I) complex The Cu complex also characterized by 1 H , 13 C NMR and HSQC spectra in DMSO-d6 that in agreement with the crystal structure, indicating the stability of the structure in the solution . The 13 C NMR spectrum shows an upfield shift of the CS signal (∼3 ppm) from that in the spectrum of H4L. Yield 0.38 g, 53%. Anal. Calc. for C74H62Cl2Cu2N12P2S2: C, 61.57; H, 4.33; N, 11.64. Found: C, 61.44; H, 4.08; N, 11.98%. 1 H NMR (DMSO-d6): δ 6.59 (2H, br.s, Ar-H); 6.65 (2H, br.s, Ar-H); 6.99 (2H, br.s, Ar-H); 7.16 (2H, t, J = 6.8 Hz, Ar-H); 7.24-7.48 (34H, Ar-H); 7.58 (2H, br.s, Ar-H); 7.69(4H, m, Ar-H); 7.77 (2H, d, J = 7.7 Hz, Ar-H); 8.55 (2H, br.s, HCNN); 8.94 (2H, br.s, HCNN); 11.30 (2H, s, indole-NH); 11.33 (2H, s, indole-NH); 12.32 (2H, s, NNH); 12.55 (2H, s, NNH ) ppm. 13 C NMR (DMSO-d6): δ 102.86, 116.82, 117.92, 119.75, 119.84, 123.96, 124.14, 124.70, 126.44, 126.96, 127.14, 128.75-129.37, 130.48, 131.57, 133.71-133.96 (Ar); 149.89, 150.29 (HCNN); 172.43 (CS) ppm.
  • 4. Chemistry and Materials Research www.iiste.org ISSN 2224- 3224 (Print) ISSN 2225- 0956 (Online) Vol.7 No.10, 2015 14 - Cytotoxicity assay for Cu(I) complex (Table1) lists the IC50 values of the Copper(I) complex after treating the (Caov-3, MCF-7) cancer cell lines for 24, 48 and 72 h. Based on outcomes that, the IC50 values were (13, 25.75) µM for 24 h treatment; however, the value declined, in case of prolonged treatment, where, IC50 values were (10, 4.25) µM for 48 h treatment, and further dropped to (4, 2.5) µM for 72 h treatment; which obviously signifies that, the prolonged treatment considerably decreased the IC50 values, and elevated the toxic activity. For the purpose of comparability, ovarian adenocarcinoma and breast cancer cell lines were also treated with cisplatin a clinical anticancer drug (Figure 5, Figure 6 ), and the results presented in (Table1) that [Cu2(H4L)2(PPh3)2Cl2] revealed higher cytotoxicity than cisplatin against the (Caov-3, MCF-7) cancer cell lines . Table 1 IC50 (µM) values of [Cu2(H4L)2(PPh3)2Cl2] and cisplatin at different time (24, 48 and 72) h
  • 5. Chemistry and Materials Research www.iiste.org ISSN 2224- 3224 (Print) ISSN 2225- 0956 (Online) Vol.7 No.10, 2015 15 - Apoptosis assay Apoptosis initiation is an anti-proliferative mechanism by which the cancer cells go through programmed death. Cells undergoing apoptosis are characterized by morphological and biochemical changes including cell shrinkage, chromatin condensation and DNA fragmentation. Based on the results of the in vitro cytotoxicity assay for [Cu2(H4L)2(PPh3)2Cl2], it was considered valuable to explore the apoptotic properties of the compound. Apoptosis in the ovarian adenocarcinoma (Caov-3) and breast (MCF-7) cancer cell lines were screened through fluorescence microscopy visualization and DNA fragmentation analysis and propidium iodide flow cytometry. - Fluorescence microscopy visualization Apoptotic cells display increased plasma membrane permeability to certain fluorescent dyes. Acridine orange (AO)/propidium iodide (PI) is a fluorochrome mixture for nuclear staining which permits uniqueness between viable, apoptotic and necrotic cells. In this work, the ovarian adenocarcinoma (Caov-3) plus breast cancer (MCF- 7) were subjected to AO/PI staining after treatment with respective IC50 concentrations of [Cu2(H4L)2(PPh3)2Cl2] for 24, 48 and 72 h. Fluorescence microscopy exposes that in the (Caov-3, MCF-7) cancer cell lines the Copper complex encouraged cell death fundamentally via apoptosis especially at 72h when the apoptotic cell clearly observed (Figure 7, Figure 8).
  • 6. Chemistry and Materials Research www.iiste.org ISSN 2224- 3224 (Print) ISSN 2225- 0956 (Online) Vol.7 No.10, 2015 16
  • 7. Chemistry and Materials Research www.iiste.org ISSN 2224- 3224 (Print) ISSN 2225- 0956 (Online) Vol.7 No.10, 2015 17
  • 8. Chemistry and Materials Research www.iiste.org ISSN 2224- 3224 (Print) ISSN 2225- 0956 (Online) Vol.7 No.10, 2015 18 - DNA Fragmentation analysis The degeneration of nuclear DNA into nucleosomal units is a biochemical feature of apoptosis. To evaluate the apoptotic DNA fragmentation in the cancer cells, the ovarian and breast cancer cell lines were incubated with the correspond IC50 value of [Cu2(H4L)2(PPh3)2Cl2] for 48 and 72 h. The cells were then lysed, the nuclear DNA was extracted, and subjected to gel electrophoresis. Inspection of the electrophoretic profiles discovered a ladder formation detected only at 72h at both of ovarian and breast cancer cells (fragments range from 400 to 1000 bp), which signify the incidence of apoptosis (Figure 9, Figure 10). - Cell cycle analysis The DNA content of cells duplicates during the S phase, therefore cells in the G0 and G1 phases (before the S phase) have unreplicated DNA, while those in the G2 and M phases (after the S phase) have replicated DNA. Analysis of cell cycles by flow cytometry enables to distinguish and quantify the cells in different phases of the cell cycle. On the flow cytometry DNA histograms cells with degraded and thus hypodiploid DNA are represented in so-called “sub-G0/G1” peaks therefore, sub-G0/G1 is a specific marker of cell death by apoptosis [28,29]. Flow cytometry analysis of the Caov-3, MCF-7 cancer cell lines after treatments with respective IC50 concentrations of the [Cu2(H4L)2(PPh3)2Cl2] for 24, 48 and 72 h was carried out (Figure11, Figure12). Moreover, the histogram of Caov- 3 illustrates gradual increases in the populations of sub-G0/G1 phase during the incubation periods whereas the histogram of MCF-7 illustrates gradual increases in the populations of G2/M phase In general, flow cytometry suggests the induction of apoptosis by the Copper(I) complex in the Caov-3 cancer cell through G0/G1 phase while through Sub-G0/G1 phase for MCF-7 cell cycle arrest. Conclusion As it was presented in this article, Copper(I) coordination complex has notable and cancer-selective cytotoxicity against the Caov-3, MCF-7 cancer cell lines as inferred from the MTT-based IC50 values and different apoptotic assay methods in consequence, Intensive research possibly will enable to apply it as anticancer drug. ACKNOWLEDGMENTS We would like to thank Mashitoh Abd Rahman and Hamed Karimian from Faculty of Medicine, University of Malaya for their assistance with the biological data collection and analysis. Financial Support from the University of Malaya ( PPP Grant Number PV048/2012A) is highly appreciated. References [1] Violeta Jevtovic, Research In Cancer and Tumor 3 (2014) 1-5. [2] American Cancer Society, Global Cancer – Facts & Figures (2007), 1 [3]Sigel, H.; Sigel, A., Eds., Metal Ions in Biological Systems; Marcel Dekker: New York 1995; Vol. 31. [4] Reynolds, J. E. F. Ed., Martindale The Extra Pharmacopoeia, 31sted.; The Royal Pharmaceutical Society; London, 1996. Martindales Pharmacopeia [5] Ismail Warad 1*, Ala’a F. Eftaiha 2, Mohammed A. Al-Nuri 1, Ahmad I. Husein 1, Mohamed Assal 2, Ahmad
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