Synthesis, structure, spectroscopic properties and cytotoxic effect of some thiosemicarbazone complexes of palladium

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Synthesis, structure, spectroscopic properties and cytotoxic eﬀect of some

thiosemicarbazone complexes of palladiumw

Sarmistha Halder,

a

Shie-Ming Peng,

b

Gene-Hsiang Lee,

b

Tanmay Chatterjee,

c

Asama Mukherjee,

d

Sushanta Dutta,

d

Utpal Sanyal

d

and Samaresh Bhattacharya*

a

Received (in Montpellier, France) 17th May 2007, Accepted 21st August 2007 First published as an Advance Article on the web 6th September 2007

DOI: 10.1039/b707448d

Reaction of salicylaldehyde thiosemicarbazone (H2L1), 2-hydroxyacetophenone thiosemicarbazone

(H2L2) and 2-hydroxynaphthaldehyde thiosemicarbazone (H2L3) (general abbreviation H2L,

where H2stands for the two dissociable protons, one phenolic proton and one hydrazinic proton)

with Na2[PdCl4] aﬀords a family of polymeric complexes of type [{Pd(L)}n]. Reaction of the

polymeric species with two monodentate ligands (D), viz. triphenylphosphine (PPh3) and

4-picoline (pic), has yielded complexes of type [Pd(L)(D)]. These mixed-ligand complexes have also been obtained from reaction of the thiosemicarbazones with [Pd(PPh3)2Cl2] and [Pd(pic)2Cl2].

Crystal structures of [Pd(L1)(PPh3)] and [Pd(L2)(pic)] have been determined. The [Pd(L)(D)]

complexes show characteristic1H NMR spectra and intense absorptions in the visible and ultraviolet region. They also ﬂuoresce in the visible region at ambient temperature. In vitro cytotoxicity screenings of the complexes along with four human clinical drugs viz. cisplatin, BCNU, 5-ﬂuorouracil (5-FU) and hydroxyurea have been carried out in two human tumor cell lines, namely promyelocytic leukemia HL-60 and histiocytic lymphoma U-937. [Pd(L2)(PPh3)]

shows the lowest IC50value and is found to be much more cytotoxic than the reference anticancer

drugs in both the cell lines. An apoptosis study in HL-60 with [Pd(L2)(PPh3)] conﬁrms that at

10 mM concentration it induces apoptosis to a greater extent than cisplatin and camptothecin.

1. Introduction

The chemistry of transition metal complexes of thiosemicar-bazones has received considerable attention, largely because of their bioinorganic relevance.1Such complexes are of particular importance due to their potentially beneﬁcial biological (viz. antibacterial, antimalarial, antiviral and antitumor) activities.2 Thiosemicarbazones usually bind to a metal ion, via dissocia-tion of the hydrazinic proton, as bidentate N,S-donors, form-ing a ﬁve-membered chelate rform-ing (1).3If a third donor site (D) is incorporated in such ligands, linked to the carbonylic carbon via one or two intervening atoms, then D,N,S-tricoor-dination (2) normally takes place.4In addition to displaying D,N,S-tricoordination, such ligands are also known to bridge a second metal ion through the sulfur.5 _{It has also been}

observed that salicylaldehyde thiosemicarbazone, in spite of

having the phenolic oxygen as a potential third donor site, coordinates as a bidentate N,S-donor, forming a rather un-usual four-membered chelate ring (3).6_{This mode of binding}

(3) has also been displayed by some other thiosemicarba-zones.7Formation of such a chelate ring (3) by salicylaldehyde thiosemicarbazone, leaving some potential donor sites unused, has been utilized successfully in the synthesis of an interesting polynuclear complex.8 _{This variable binding mode of}

thio-semicarbazones has encouraged us to explore their coordina-tion chemistry further,6,8,9and the present work has originated from this exploration. Herein we have chosen three potentially tridentate thiosemicarbazones, viz. the thiosemicarbazones of salicylaldehyde, 2-hydroxyacetophenone and 2-hydroxy-naphthaldehyde. These thiosemicarbazones are abbreviated in general as H2L, where H2 stands for the two dissociable

protons, the phenolic proton and the hydrazinic proton. Individual ligand abbreviations are shown in 4. To interact with the chosen thiosemicarbazones, palladium has been selected as the metal. It may be mentioned here that, though the chemistry of palladium complexes of some thiosemicarba-zones has been studied,10 that of the chosen thiosemicarba-zones (4) appears to have remained unexplored. Reaction of the three selected thiosemicarbazones (4) has been carried out with three palladium starting materials, viz. Na2[PdCl4],

[Pd(PPh3)2Cl2] and [Pd(pic)2Cl2] (pic = 4-picoline), which

has aﬀorded a family of interesting complexes containing the thiosemicarbazones coordinated in the tridentate fashion (5). The chemistry of these complexes is reported in this paper with special reference to their synthesis, structure and spectral

a

Department of Chemistry, Inorganic Chemistry Section, Jadavpur University, Kolkata 700 032, India. E-mail: [email protected]

b

Department of Chemistry, National Taiwan University, Taipei, Taiwan, ROC

c

School of Chemistry, University of Hyderabad, Hyderabad 500 046, India

d

Department of Anticancer Drug Development, Chittaranjan National Cancer Institute, Kolkata 700 026, India

w Electronic supplementary information (ESI) available: A diagram showing metal–p interaction in the [Pd(L)(PPh3)] complex (Fig. S1), a

diagram showing p–p interaction in the [Pd(L)(pic)] complex (Fig. S2), a table showing metal–p and p–p interactions in the [Pd(L)(PPh3)] and

[Pd(L)(pic)] complexes, respectively (Table S1) and a partial MO diagram of the [Pd(L)(pic)] complex (Fig. S3). See DOI: 10.1039/ b707448d

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properties, and cytotoxic activity in two human tumor cell lines.

Results and discussion

Syntheses

Reaction of the selected thiosemicarbazones (H2L, 4) has been

carried out ﬁrst with Na2[PdCl4] in reﬂuxing ethanol in the

presence of triethylamine to aﬀord a family of polymeric complexes of type [{Pd(L)}n] in decent yields. Based on the

compositions of these complexes, as well as the +2 oxidation state of palladium in them, the thiosemicarbazones are be-lieved to coordinate the metal center in the expected dianionic O,N,S-fashion (5). The fourth coordination position on palla-dium in the Pd(L) fragment is assumed to be taken up by the sulfur of a coordinated thiosemicarbazone belonging to an-other Pd(L) fragment (6). This bridging action of the thio-semicarbazone sulfur, which is well documented in the litera-ture,5 appears to be responsible for the formation of the polymeric species.

In order to explore the possibility of forming monomeric complexes by splitting the sulfur bridge in the [{Pd(L)}n]

complexes, their reaction has been carried out with two monodentate ligands (D), viz. triphenylphosphine (PPh3) and

4-picoline (pic). From each of these reactions a monomeric

complex of type [Pd(L)(D)] (D = PPh3 or pic) has been

obtained. The same monomeric complexes have also been synthesized, in better yields, by reaction of the thiosemicarba-zones (4) with [Pd(PPh3)2Cl2] and [Pd(pic)2Cl2] in reﬂuxing

ethanol in the presence of triethylamine. Synthetic methods for all the complexes are illustrated in Scheme 1. The observed elemental (C, H, N) analytical data of the synthesized com-plexes are found to be consistent with their compositions. Crystal structures

In order to authenticate the coordination modes of the thio-semicarbazones in these monomeric [Pd(L)(D)] complexes, structures of a representative member from each family, viz. [Pd(L1)(PPh3)] and [Pd(L2)(pic)], have been determined by

X-ray crystallography. The structure of the [Pd(L1)(PPh3)]

complex is shown in Fig. 1 and some relevant bond parameters are listed in Table 1. The structure shows that the thiosemi-carbazone ligand is coordinated to palladium in the expected tridentate fashion (5), forming six- and ﬁve-membered chelate rings with O–Pd–N and N–Pd–S bite angles of 92.82(7)1 and 84.26(5)1, respectively. A triphenylphosphine is also coordi-nated to the metal center, which is trans to the nitrogen. Palladium is thus nested in an ONSP core, which is slightly distorted from ideal square planar geometry, as reﬂected in the bond parameters around the metal center. The Pd–O, Pd–N, Pd–S and Pd–P distances are all quite normal, as observed in structurally characterized complexes of palladium containing these bonds.10 _{Bond distances within the coordinated}

thiosemicarbazone are also usual.9c

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The absence of any solvent of crystallization in the crystal lattice of [Pd(L1)(PPh3)] indicates the possible existence of

non-covalent interaction(s) between the individual complex molecules. A closer look at the packing pattern of in the crystal reveals that hydrogen bonding interactions of two types, viz. intramolecular C–H O and intermolecular N–H N, are active in the lattice. A selected view of the hydrogen bonding interactions is shown in Fig. 2 and some hydrogen bond parameters are given in Table 2. One ortho C–H of a phenyl ring of the PPh3is intramolecularly hydrogen

bonded to the phenolate oxygen of the thiosemicarbazone ligand. One –NH2 hydrogen of each complex molecule is

hydrogen bonded to the nitrogen next to the azomethine nitrogen of a second molecule and thus a hydrogen bonded dimer is formed. Apart from these hydrogen bonding interac-tions, there also exist Pd–p interactions between the metal center of one complex molecule and the phenyl ring of the thiosemicarbazone ligand of a second complex molecule (Fig. S1, Table S1w). This extended Pd–p interaction seems to be responsible for holding the crystal together. It may be relevant

to note here that such non-covalent interactions are of signiﬁcant importance in molecular recognition processes as well as in crystal engineering.11

The structure of the [Pd(L2)(pic)] complex (Fig. 3) shows that the thiosemicarbazone ligand is coordinated to palladium in the same tridentate fashion (5) as in [Pd(L1)(PPh3)], and a

4-picoline has taken up the fourth coordination site on the metal center. In this complex palladium has an ONSN co-ordination sphere around it. The observed Pd–N(pic) distance is normal,12and the structural features in the Pd(L2) fragment are similar to those observed in the Pd(L1) fragment of the [Pd(L1)(PPh3)] complex. An examination of the packing

pat-tern in this [Pd(L2)(pic)] crystal shows that three intramole-cular hydrogen bonding interactions, viz. C–H O, C–H S and C–H N, and one intermolecular hydrogen bonding interaction, viz. N–H O, are active in the lattice (Fig. 4, Table 2). Two picolyl C–Hs (at the 2 and 6 positions) are intramolecularly hydrogen bonded to the phenolate oxygen and sulfur of the thiosemicarbazone ligand. One methyl C–H of the thiosemicarbazone is also intramolecularly hydrogen bonded to the nitrogen (which is not bound to the metal center) of the same ligand. One –NH2 hydrogen of each

complex molecule is hydrogen bonded to the phenolate oxygen of a second molecule; this intermolecular hydrogen bonding has propagated along the b-axis through the lattice. Besides these hydrogen bonding interactions, there also exist p–p interactions between the picolyl rings and also between the picolyl and phenyl rings of the thiosemicarbazone ligand (Fig. S2, Table S1w). The extended intermolecular interactions have been responsible for holding the crystal together.

Fig. 1 Structure of the [Pd(L1_)(PPh

3)] complex drawn at the 50%

probability level.

Table 1 Selected bond distances and bond angles for [Pd(L1)(PPh3)]

and [Pd(L2_)(pic)] [Pd(L1_)(PPh 3)] Bond distances/A˚ Pd–N(3) 2.0147(17) C(8)–N(1) 1.354(3) Pd–P 2.2711(5) C(7)–N(3) 1.290(3) Pd–S 2.2411(6) C(1)–O(1) 1.306(3) Pd–O(1) 2.0157(16) N(2)–N(3) 1.397(2) C(8)–S 1.748(2) Bond angles/1 N(3)–Pd–P 173.95(5) N(3)–Pd–O(1) 92.82(7) O(1)–Pd–S(1) 177.07(5) N(3)–Pd–S 84.26(5) [Pd(L2_)(pic)] Bond distances/A˚ Pd(1)–N(3) 1.9861(15) C(8)–N(1) 1.359(3) Pd(1)–N(4) 2.0698(18) C(7)–N(3) 1.309(2) Pd(1)–S(1) 2.2510(7) C(1)–O(1) 1.321(2) Pd(1)–O(1) 1.9981(14) N(2)–N(3) 1.397(2) C(8)–S(1) 1.736(2) Bond angles/1 N(3)–Pd1–N(4) 179.16(6) N(3)–Pd1–O(1) 91.74(7) O(1)–Pd1–S(1) 175.69(5) N(3)–Pd1–S(1) 85.04(5)

Fig. 2 Hydrogen bonding interactions in the lattice of

[Pd(L1)(PPh3)].

Table 2 Hydrogen bond distances and bond angles for

[Pd(L1_)(PPh

3)] and [Pd(L2)(pic)]a

Bond distances/A˚ Bond angles/1

[Pd(L1_)(PPh 3)] N1–H1A N2i 0.86 2.18 3.004(3) 160 C10–H10A O1 0.93 2.35 3.025(4) 130 [Pd(L2_)(pic)] N1–H2N O1ii 0.86 2.24 2.888(2) 132 C9–H9A N2 0.96 2.25 2.621(3) 102 C10–H10 S1 0.93 2.66 3.246(2) 122 C14–H14 O1 0.93 2.26 2.829(3) 119 a_{Symmetry: i = 1} _{x, 2} _{y, 1} _{z; ii =}1 2 x,12+ y, z.

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Spectral properties

1

H NMR spectra of the [Pd(L)(PPh3)] complexes, recorded in

CDCl3solutions, show all the expected signals. Broad signals

for the PPh3ligands are observed within 7.4–7.8 ppm. In the

[Pd(L1)(PPh3)] and [Pd(L 3

)(PPh3)] complexes the azomethine

proton signal of the coordinated thiosemicarbazone is ob-served at 8.24 and 9.52 ppm, respectively. The methyl signal from the coordinated thiosemicarbazone in the [Pd(L2)(PPh3)]

complex is observed at 2.89 ppm. The NH2 signal of the

coordinated thiosemicarbazone is observed around 4.8 ppm. Most of the expected signals from the aryl fragment of the coordinated thiosemicarbazone are clearly observed in the aromatic region, while few could not be detected due to their overlap with other signals. In the 1H NMR spectra of the [Pd(L)(pic)] complexes, the methyl signal of the coordinated 4-picoline is observed at around 2.4 ppm and a distinct doublet is observed near 8.6 ppm, which is attributable to the a-proton of the picoline. The other expected doublet for

the b-proton of the picoline is observed at 7.24 ppm in the [Pd(L1_{)(pic)] complex, but the same signal could not be}

detected in the other two complexes because of overlap problems. The1H NMR spectral features for the coordinated thiosemicarbazones in these [Pd(L)(pic)] complexes are quali-tatively similar to those observed for the corresponding [Pd(L)(PPh3)] complexes. The1H NMR spectral data of the

[Pd(L)(PPh3)] and [Pd(L)(pic)] complexes are therefore

con-sistent with their compositions.

Infrared spectra of all the [Pd(L)(PPh3)] complexes show

many vibrations of diﬀerent intensities in the 1600–400 cm 1 region. Assignment of each individual band to a speciﬁc vibration has not been attempted. However, three strong bands displayed near 533, 694 and 743 cm 1by these com-plexes, are attributed to the coordinated PPh3ligands.

Com-parison with the spectrum of [Pd(PPh3)2Cl2] shows the

presence of several new bands (e.g. near 811, 1130, 1229, 1285, 1346, 1562 and 1599 cm 1_{) in the spectra of the}

[Pd(L)(PPh3)] complexes, which must be due to the presence

of the coordinated thiosemicarbazone ligand. Besides the absence of the three diagnostic bands for the PPh3 ligands

near 533, 694 and 743 cm 1, infrared spectral properties of the [Pd(L)(pic)] complexes are qualitatively similar to those of the [Pd(L)(PPh3)] complexes.

The [Pd(L)(PPh3)] and [Pd(L)(pic)] complexes are soluble in

common organic solvents such as methanol, ethanol, acetone, acetonitrile, dichloromethane, chloroform, etc., producing intense yellow solutions. Electronic spectra of these complexes have been recorded in dichloromethane solution. Spectral data are presented in Table 3 and a selected spectrum is shown in Fig. 5. All the mixed-ligand complexes show several intense absorptions in the visible and ultraviolet regions. The absorp-tions in the ultraviolet region are assignable to transiabsorp-tions within the ligand orbitals and those in the visible region are probably due to charge-transfer transitions involving both metal and ligand orbitals. To have an understanding of the nature of the transitions in the visible region, qualitative extended Hu¨ckel molecular orbital (EHMO) calculations have been performed13 _{on computer generated models of the}

[Pd(L)(PPh3)] and [Pd(L)(pic)] complexes. The results

ob-tained are found to be similar for the three members of each group. A partial MO diagram for a representative [Pd(L)(PPh3)] complex is shown in Fig. 6 and that of a selected Fig. 3 Structure of the [Pd(L2_{)(pic)] complex drawn at the 50%}

probability level.

Fig. 4 Hydrogen bonding interactions in the lattice of [Pd(L2_)(pic)].

Table 3 Electronic spectral data in dichloromethane solution

Compound lmax/nm (e/dm

3 mol 1cm 1)a [Pd(L1)(PPh3)] 398(9000), 342(11 300)s, 315(15 500), 298(16 100) [Pd(L2_)(PPh 3)] 389(9800), 340(12 600)s, 313(19 000), 298(16 800) [Pd(L3_)(PPh 3)] 430(9800), 408(9500), 389(5800)s, 348(12 000), 317(19 400), 261(41 300) [Pd(L1_)(pic)] _{402(6000), 386(5400), 339(6600)}s_, 314(7800)s, 299(8700)s [Pd(L2_)(pic)] _{406(9000), 386(10 100), 341(11 800)}s_, 312(16 000)s, 297(17 500) [Pd(L3_)(pic)] _{432(3300), 409(3100), 389(2100)}s_, 348(3800)s, 326(4700), 258(14 200) a_{s = shoulder.}

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[Pd(L)(pic)] is deposited as Fig. S3.w The compositions of selected molecular orbitals are given in Table 4. In all the cases, the highest occupied molecular orbital (HOMO) has major contributions from the palladium d (dz2 and d_xy) orbitals. The lowest unoccupied molecular orbital (LUMO) is delocalized almost entirely on the thiosemicarbazone ligand and is concentrated heavily on the imine (CQN) fragment. The lower energy absorption in these complexes may therefore be assigned to a charge-transfer transition taking place from the ﬁlled palladium d orbital (HOMO) to the vacant

p*(imine) orbital of the coordinated thiosemicarbazone ligand (LUMO). Such charge-transfer transition in palladium complexes is, to our knowledge, rare.14The electronic spectral properties, as well as features of the molecular orbitals, of the [Pd(L)(pic)] complexes are similar to those of the [Pd(L)(PPh3)] analogues.

The intensities of the charge-transfer transitions in the visible region have tempted us to explore the luminescence properties of these complexes and this has been carried out in dichloromethane solution at ambient temperature (298 K). All six [Pd(L)(D)] complexes have been found to display emission in the visible region using an excitation wavelength of

B350 nm and a selected spectrum is shown in Fig. 5. Quantum

yields (f) of these emissions have been evaluated (Table 5) with reference to [Ru(bpy)3]Cl2(f = 0.028 at 298 K).

15

The

Fig. 5 (a) Electronic spectrum and (b) emission spectrum of [Pd(L3_)(PPh

3)] in dichloromethane solution.

Fig. 6 Partial molecular orbital diagram of the [Pd(L1_)(PPh 3)]

complex.

Table 4 Composition of selected molecular orbitals of the complexes

Compound Contributing fragments % contribution of fragments to HOMO LUMO [Pd(L1)(PPh3)] Pd 89 — L1 ₇ ₉₆ (CQN, 49) [Pd(L2)(PPh3)] Pd 87 — L2 ₈ ₉₃ (CQN, 44) [Pd(L3_)(PPh 3)]a Pd 73 — L3 21 97 (CQN, 30) [Pd(L1)(pic)] Pd 92 — L1 ₂ ₉₃ (CQN, 47) pic — 12 [Pd(L2_)(pic)] _Pd ₉₀ _— L2 6 91 (CQN, 26) pic — 44 [Pd(L3_)(pic)]b _Pd ₅₀ _— L3 41 95 (CQN, 23) pic — —

a_{The HOMO-1 has 88% contribution from the metal.}b_The

HOMO-1 has 93% contribution from the metal.

Table 5 Emission spectral data for the complexes

Compound Emission data lmax/nm Quantum yield (f) Excitation Emissiona [Pd(L1_)(PPh 3)] 340 367 1.17 10 3 428 [Pd(L2_)(PPh 3)] 340 380s 1.38 10 3 423 [Pd(L3_)(PPh 3)] 350 382 0.36 10 3 450 [Pd(L1)(pic)] 339 380 2.21 10 3 445s [Pd(L2)(pic)] 341 380 0.83 10 3 440 478s [Pd(L3_)(pic)] ₃₇₉ ₃₈₅ _7.64 10 3 450 525 a s = shoulder.

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observed quantum yields indicate that these [Pd(L)(PPh3)] and

[Pd(L)(pic)] complexes are relatively poor emitters at room temperature.

Cytotoxicity assay

The in vitro growth inhibitory eﬀects of the [Pd(L)(D)] com-plexes were evaluated in two human cell lines viz. promyelo-cytic HL-60 and histiopromyelo-cytic lymphoma U-937. Four human clinical drugs, cisplatin, BCNU, 5-FU and hydroxyurea, were used as reference compounds for comparison. The activities are expressed in terms of IC50value, the concentration of the

respective compound required to reduce the cell survival fraction to 50% after 72 h of exposure. The lower the IC50

value is, the greater is the cytotoxicity. From the results presented in Table 6, it is found that the [Pd(L1)(PPh3)] and

[Pd(L2)(PPh3)] complexes are much more active than all the

clinical drugs, including cisplatin, in HL-60. In U-937, [Pd(L2_)(PPh

3)] is more active than cisplatin and other

refer-ence compounds, while the activity of [Pd(L1)(PPh3)] is higher

than BCNU and hydroxyurea, comparable to 5-FU, and less than cisplatin. The [Pd(L3)(PPh3)] complex did not show any

appreciable activity in the cell lines. In HL-60, the [Pd(L)(pic)] complexes are more active than BCNU, 5-FU and hydroxy-urea. The activity of [Pd(L1)(pic)] is less than cisplatin, while that of the other two complexes is comparable to cisplatin. In U-937 the [Pd(L)(pic)] complexes are more active than BCNU and hydroxyurea, and less active than cisplatin and 5-FU. In vitro apoptosis assay

Cell death may occur by one of two distinct mechanisms: necrosis or apoptosis. The most common and well-deﬁned form of programmed cell death is apoptosis. During the past decade, cell biology as well as oncology research has focused on apoptosis. Hence, based on the results of our in vitro cytotoxicity assay in HL-60, it was thought worthwhile to further explore the apoptotic properties of [Pd(L2)(PPh3)] and

[Pd(L3)(pic)], the most active members from each group. The apoptosis assay was conducted in HL-60 by the annexin V-FITC/PI method in a ﬂow cytometer after an incubation period of 24 h. The results obtained for the complexes have been compared with those for cisplatin and the well-known apoptosis inducer camptothecin, and are shown in Fig. 7. Each drug treatment was done at 5 and 10 mM concentration. Exposure of cells to cisplatin resulted to 1.39% and 1.20% of gated cells in LR and 3.23% and 6.31% in UR, respectively

(Fig. 7C and D).16_{Camptothecin induced 7.79% and 10.52%}

in LR and 5.46% and 5.30% in UR (Fig. 7E and F). The [Pd(L2)(PPh3)] complex exhibited 1.84% and 3.31% in LR

and 2.48% and 27.35% in UR (Fig. 7G and H). Thus, it

Table 6 Cytotoxicity assay IC50values (mM)a

Compound HL-60 U-937 [Pd(L1_)(PPh 3)] 2.5 4.8 [Pd(L2)(PPh3)] 0.6 1.3 [Pd(L3_)(PPh 3)] 203.0 231.6 [Pd(L1)(pic)] 16.2 7.3 [Pd(L2_)(pic)] _7.1 _6.6 [Pd(L3_)(pic)] _6.5 _7.7 Cisplatin 7.0 3.2 BCNU 30.5 12.3 5-FU 266.0 4.7 Hydroxyurea 204.0 115.0 a

For details, see experimental.

Fig. 7 Flow cytometric analysis of apoptosis and necrosis in HL-60 cells after treatment with four drugs or complexes at two diﬀerent concentrations. Quadrant analysis of ﬂuorescence intensity of gated cells in FL-1 and FL-2 channels was from 10 000 events. Figures in the cytogram indicate the percent of gated cells in each quadrant. (FL1-H = annexin V, FL2-H = propidium iodide).

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induces apoptosis to a greater extent than cisplatin as well as camptothecin at 10 mM concentration. On the other hand, the [Pd(L3)(pic)] complex induces 2.09% and 2.16% in LR and 2.01% and 2.02% in UR (Fig. 7I and J).

Conclusions

The present study shows that salicylaldehyde thiosemicarba-zones and similar ligands can smoothly bind to metal ions as tridentate O,N,S-donors, provided an adequate number of coordination sites are readily available on the target metal ion. This study also demonstrates that [Pd(L2)(PPh3)] has

remarkable cytotoxic properties among all the compounds tested, including recognized anticancer drugs, which is mani-fested through the IC50 values and has been further

corro-borated by the apoptosis study in HL-60, where it induces apoptosis to a greater extent than cisplatin and camptothecin.

Experimental

Materials

Palladium chloride was obtained from Arora Matthey, Kolk-ata, India, and was converted to Na2[PdCl4].17

Salicylalde-hyde, 2-hydroxyacetophenone and 2-hydroxynaphthaldehyde were obtained from S. D. ﬁne-chem, Mumbai, India. Thio-semicarbazide was procured from Loba Chemie, Mumbai, India. All other chemicals and solvents were reagent grade commercial materials and were used as received. The [Pd(PPh3)2Cl2] and [Pd(pic)2Cl2] complexes were prepared

starting from Na2[PdCl4] by following reported

proce-dures.18,19 The thiosemicarbazone ligands (H2L1, H2L2 and

H2L 3

) were prepared by condensing the respective aldehyde or ketone with thiosemicarbazide in hot ethanol.

Synthesis

[{Pd(L1)}n]. To a solution of H2L1(64 mg, 0.33 mmol) in hot

ethanol (30 ml), was added triethylamine (66 mg, 0.66 mmol) followed by Na2[PdCl4] (100 mg, 0.33 mmol). The mixture was

heated at reflux for 6 h. A brown precipitate settled down on cooling, which was collected by filtration, washed with ethanol and dried in air to afford [{Pd(L1)}n] as a brown powder.

Yield: 84 mg (85%). Anal. calc. for (C8H7N3SOPd)n: C 31.96;

H 2.33; N 13.98. Found: C 31.77; H 2.43; N 14.11%. The [{Pd(L2_)}

n] and [{Pd(L3)}n] complexes were prepared by

following the same above procedure using, respectively, H2L2

and H2L3instead of H2L1.

[{Pd(L2)}n]. Anal. calc. for (C9H9N3SOPd)n: C 34.46;

H 2.87; N 13.40. Found: C 34.58; H 2.99; N 13.23%. [{Pd(L3)}n]. Anal. calc. for (C12H9N3SOPd)n: C 48.82;

H 3.62; N 12.66. Found: C 48.67; H 3.77; N 12.87%. [Pd(L1_)(PPh

3)]. Method A. The polymeric [{Pd(L 1

)}n]

spe-cies (100 mg) and triphenylphosphine (88 mg) were taken together in ethanol (30 ml) and the solution was reﬂuxed for 24 h to yield a yellow solution. Evaporation of this solution gave a yellow solid, which was subjected to puriﬁcation by thin layer chromatography on a silica plate. With 1 : 40 aceto-nitrile–benzene as the eluant, a major yellow band separated,

which was extracted with acetonitrile. Upon evaporation of the acetonitrile extract [Pd(L1_)(PPh

3)] was obtained as a

crystalline yellow solid. Yield: 113 mg (60%). Method B. To a solution of H2L

1

(28 mg, 0.14 mmol) in hot ethanol (30 ml) was added triethylamine (29 mg, 0.29 mmol) followed by [Pd(PPh3)2Cl2] (100 mg, 0.14 mmol). The mixture

was heated at reﬂux for 5 h to yield a yellow solution. Evaporation of this solution gave a yellow solid, which was subjected to puriﬁcation by thin layer chromatography on a silica plate. With benzene as the eluant, a yellow band separated, which was extracted with acetonitrile. Upon eva-poration of the acetonitrile extract [Pd(L1)(PPh3)] was

ob-tained as a crystalline yellow solid. Yield: 52 mg (65%) Anal. calc. for C26H22N3SOPd: C 55.57; H 3.92; N 7.48. Found: C

55.62; H 3.86; N 7.50%. 1H NMR in CDCl3 d/ppm: 4.76

(s, 2H), 6.62 (t, J = 7.3 Hz, 1H), 6.68 (d, J = 8.5 Hz, 1H), 7.22 (t, J = 7.7 Hz, 1H), 7.31 (d, J = 8.0 Hz, 1H), 7.41–7.7520 (PPh3), 8.24 (d, J = 12.99 Hz, 1H).

The [Pd(L2)(PPh3)] and [Pd(L3)(PPh3)] complexes were

pre-pared by following the same above procedure using, respec-tively, H2L2and H2L3instead of H2L1.

[Pd(L2)(PPh3)]. Anal. calc. for C27H24N3SOPd: C 56.31; H

4.17; N 7.30. Found: C 56.40; H 4.23; N 7.33%.1H NMR in CDCl3d/ppm: 2.89 (s, 3H), 4.78 (s, 2H), 6.62 (d, J = 8.34 Hz,

1H), 6.68 (t, J = 7.6 Hz, 1H), 7.17 (t, J = 7.7 Hz, 1H), 7.43–7.7220(PPh3), 7.62 (d, J = 1.4 Hz, 1H).

[Pd(L3_)(PPh

3)]. Anal. calc. for C30H24N3SOPd: C 58.88; H

3.93; N 6.87. Found: C 58.86; H 3.88; N 6.94%.1H NMR in CDCl3 d/ppm: 4.83 (s, 2H), 6.76 (d, J = 9.2 Hz, 1H), 7.32

(t, J = 5.6 Hz, 1H), 7.50–7.8320(m, 15H (PPh3) and t, 1H),

8.11 (d, J = 8.5 Hz, 1H), 9.52 (d, J = 13.2 Hz, 1H). [Pd(L1)(pic)]. Method A. The polymeric [{Pd(L1)}n] species

(100 mg) and 4-picoline (31 mg) were taken in ethanol (30 ml) and the solution was reﬂuxed for 24 h to yield a yellow solution. Evaporation of this solution gave a yellow solid, which was subjected to puriﬁcation by thin layer chromato-graphy on a silica plate. With 1 : 20 acetonitrile–benzene as the eluant, a prominent yellow band separated, which was ex-tracted with acetonitrile. Upon evaporation of the acetonitrile extract [Pd(L1)(pic)] was obtained as a crystalline yellow solid. Yield: 66 mg (50%).

Method B. To a solution of H2L1(54 mg, 0.28 mmol) in hot

ethanol (30 ml) was added triethylamine (56 mg, 0.55 mmol) followed by [Pd(pic)2Cl2] (100 mg, 0.28 mmol). The mixture

was heated at reﬂux for 6 h to yield a yellow solution. Evaporation of this solution gave a yellow solid, which was subjected to puriﬁcation by thin layer chromatography on a silica plate. With 1 : 20 acetonitrile–benzene as the eluant, a major yellow band separated, which was extracted with acet-onitrile. Upon evaporation of the acetonitrile extract [Pd(L1)(pic)] was obtained as a crystalline yellow solid. Yield: 59 mg (55%). Anal. calc. for C14H14N4SOPd: C 42.56; H 3.42;

N 14.29. Found: C 42.38; H 3.45; N 14.23%. 1_{H NMR in}

CDCl3d/ppm: 2.44 (s, 3H), 4.87 (s, 2H), 6.67 (t, J = 7.3 Hz,

1H), 7.03 (d, J = 8.8 Hz, 1H), 7.24 (d, J = 5.7 Hz, 2H), 7.29–7.3420(2H), 7.92 (s, 1H), 8.62 (d, J = 5.9 Hz, 2H).

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The [Pd(L2_{)(pic)] and [Pd(L}3_{)(pic)] complexes were prepared}

by following the same above procedure using, respectively, H2L2and H2L3instead of H2L1.

[Pd(L2)(pic)]. Anal. calc. for C15H16N4SOPd: C 44.29; H

3.94; N 13.78. Found: C 44.44; H 3.86; N 13.76%.1H NMR in CDCl3 d/ppm: 2.43 (s, 3H), 2.75 (s, 3H), 4.84 (s, 2H), 6.68

(t, J = 7.3 Hz, 1H), 7.04 (d, J = 8.2 Hz, 1H), 7.21–7.2620

(3H), 7.68 (d, J = 8.2 Hz, 1H), 8.61 (d, J = 6.2 Hz, 1H). [Pd(L3)(pic)]. Anal. calc. for C18H16N4SOPd: C 48.82; H

3.62; N 12.66. Found: C 48.99; H 3.78; N 12.45%.1H NMR in CDCl3d/ppm: 2.45 (s, 3H), 4.87 (s, 2H), 7.13–7.26 20 (4H), 7.48 (d, J = 7.44 Hz, 1H), 7.69–7.5020_{(2H), 8.06 (d, J = 8.5 Hz,} 1H), 8.65 (d, J = 2.5 Hz, 2H), 8.93 (s, 1H). Cytotoxicity assay

Cell lines and culture. HL-60 and U-937 (purchased from National Center for Cell Sciences, Pune, India) were main-tained in complete sterile growth medium RPMI-1640 with

L-glutamine (GIBCO, Invitrogen Corporation, USA), con-taining 10% heat inactivated fetal bovine serum (GIBCO, Invitrogen Corporation, USA) and 1% antibiotics [10 000 U penicillin ml 1 and 10 000 mg streptomycin ml 1, BioWhit-taker, Cambrex Bio Science, USA]. Cell cultures were main-tained in log phase using a subculture ratio of 1 : 5 twice a week.

Preparation of test material. Working stock solutions of all the compounds were prepared by dissolving 20 mg of each compound in 1 ml of DMSO [Hybri-Max grade, Sigma-Aldrich Co., USA] and ﬁltered under sterile conditions. These were serially diluted with complete RPMI-1640 medium prior to use to obtain diﬀerent drug concentrations.

MTT-based cytotoxicity test. 100 ml of cell suspension from the stock 2 105HL-60 or 1 105 U-937 cells ml 1 were added to 96-well cell culture plates. Next, 10 ml of drug solutions of diﬀerent concentrations were added to respective wells followed by the addition of the medium (90 ml) in triplicate (total volume 200 ml/well). All vehicle controls con-tained the same concentration of DMSO. Plates were incu-bated for 72 h at 37 1C, 5% CO2–95% air with humidity.

After removal of 100 ml of media from each well, 10 ml of a ;5 mg ml 1solution of 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide [MTT, Sigma, USA] in Dulbec-co’s PBS (GIBCO, BRL) were added to each well and the plate was incubated for 4 h at 37 1C. Subsequently 100 ml of acidic isopropanol solution (0.04 N HCl in isopropanol) was added to the wells to dissolve formed formazan crystals. The plate was read in a microplate reader (Bio-Rad, USA, Model 550) at 540 nm. The percentage cell viability was calculated by dividing the average absorbance of the cells treated with compounds by that of the control; IC50(drug concentration

needed for 50% inhibition of cells relative to control) was determined through Curveﬁt software by plotting % inhibition vs. drug concentration and expressed in mM concentration.

In vitro apoptosis assay

Induction of apoptosis in vitro by two representative com-plexes of each type [Pd(L)(D)] (when D = PPh3 and pic),

cisplatin and camptothecin were determined by a ﬂow cyto-metric assay using an annexin V-FITC21apoptosis detection kit (BD Biosciences Pharmingen, San Diego, USA). Exponen-tially growing HL-60 cells in complete RPMI-1640 media (100 ml of 5 106

) were plated in six well plates. 10 ml of each compound in DMSO (5 and 10 mM concentrations) was added to the wells followed by the addition of required media (total volume 1 ml). Plates were incubated at 37 1C for 24 h. The cells were centrifuged at room temperature at 1500 rpm for 5 min. The pellet was washed twice with cold PBS and re-suspended in the binding buffer (1X, 100 ml) provided in the kit. The cells were stained with annexin V-FITC (5 ml) and propidium iodide [PI] (5 ml) and incubated for 15 min in the dark at 25 1C. Next, 400 ml of binding buffer was added to each tube and analyzed on a FACScan flow cytometer (Becton Dick-inson, Mountainview, CA) using Cell Quest software. Two controls, viz. unstained cells and cells stained with both annexin V-FITC and PI, containing DMSO as vehicle were used. Cells that were annexin+_/PI _{and annexin}+_/PI+_were

considered positive for apoptosis. Physical measurements

Microanalyses (C, H, N) were performed using a Heraeus Carlo Erba 1108 elemental analyzer. IR spectra were obtained on a Shimadzu FTIR-8300 spectrometer with samples pre-pared as KBr pellets. Electronic spectra were recorded on a JASCO V-570 spectrophotometer. Emission spectra were recorded on a Perkin Elmer LS55 luminescence spectrometer.

1_{H NMR spectra were recorded in CDCl}

3 solutions on a

Table 7 Crystallographic data for [Pd(L1)(PPh3)] and [Pd(L 2

)(pic)] [Pd(L1_)(PPh

3)] [Pd(L2)(pic)]

Empirical formula C26H22N3OPSPd C15H16N4OSPd

Formula mass 561.9 406.78

Crystal system Triclinic Orthorhombic

Space group P1 Pbca

a/A˚ 7.5385(4) 8.3942(12) b/A˚ 10.2179(5) 15.149(2) c/A˚ 16.9756(9) 25.099(4) a/1 77.025(1) 90 b/1 80.819(1) 90 g/1 71.567(1) 90 V/A˚3 1203.27(11) 3191.7(8) Z 2 8 Dcalc/mg m 3 1.551 1.693 F(000) 568 1632 l/A˚ 0.71073 0.71073 Crystal size/mm3 0.38 0.30 0.15 0.12 0.28 0.48 T/K 295(2) 298 m/mm 1 0.948 1.3 Independent reﬂections 5525 3135 Rint 0.0261 0.022 Collected reﬂections 15972 30751 R1a 0.026 0.0219 wR2b 0.0702 0.0595 GOFc _1.159 _1.076 a_R 1 = S||Fo7 7Fc||/S7Fo7.bwR2 = [S[w(Fo 2 Fc 2 )2]/ S[w(Fo 2 )2]]12_.c_{GOF = [S[w(F} o 2 Fc 2 )2]/(M N)]12_{, where M is the}

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Bruker Avance DPX 300 NMR spectrometer using TMS as the internal standard.

X-Ray crystallography

Single crystals of [Pd(L1)(PPh3)] and [Pd(L2)(pic)] were grown

by slow evaporation of 1 : 1 dichloromethane–acetonitrile solutions of the respective compounds. Selected crystal data and data collection parameters are given in Table 7. Data on the crystals were collected on a BRUKER SMART ApexCCD area detector. A total 15 972 and 30 571 reﬂections giving 5525 and 3135 unique reﬂections were collected (Rint= 0.0261 and

0.022) for [Pd(L1_)(PPh

3)] and [Pd(L2)(pic)], respectively.

X-Ray data reduction, structure solution and reﬁnement were done using the SHELXS-97 and SHELXL-97 packages.22The structures were solved by direct methods.

CCDC reference numbers 646551 and 646552. For crystal-lographic data for the [Pd(L)(PPh3)] and [Pd(L)(pic)]

com-plexes in CIF or other electronic format see DOI: 10.1039/ b707448d

Acknowledgements

Financial assistance received from the Council of Scientiﬁc and Industrial Research, New Delhi, India, [grant no. 01(1952)/04/EMR-II] is gratefully acknowledged. The authors thank the anonymous referees for their constructive criticisms and suggestions, which have been of great help in preparing the revised manuscript. Sincere thanks are due to Prof. Chittaranjan Sinha and Dr Asok Nath Mandal of the Depart-ment of Chemistry, Jadavpur University, for their help with the ﬂorescence and NMR spectral measurements, respectively. Sincere thanks are also due to Dr Golam Mostafa of the Department of Physics, Jadavpur University, for his help in resolving some crystallographic queries. The authors are grate-ful to Dr Jaydip Biswas, Director, Chittaranjan National Cancer Institute, for his encouragement and Dr R. N. Baral, In-Charge, Department of Immunoregulation & Immuno-diagnostics, for helpful discussions. Sarmistha Halder thanks the University Grants Commission, New Delhi, India, for her fellowship [grant no. 10-2(5)2004(1)-E.U.II].

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