Abstract
A novel tri--butyl(IV) derivative of 2-thiobarbituric acid (HTBA) of formula (1) has been synthesized and characterized by elemental analysis and -NMR and FT-IR spectroscopic techniques. The crystal structure of complex has been determined by single crystal X-ray diffraction analysis at 120(2)βK. The geometry around Sn(IV) is trigonal bipyramidal. Three -butyl groups and one oxygen atom from a deprotonated 2-thiobarbituric ligand are bonded to the metal center. The geometry is completed with one oxygen from a water molecule. Compound exhibits potent, in vitro, cytotoxicity against sarcoma cancer cells (mesenchymal tissue) from the Wistar rat, polycyclic aromatic hydrocarbons (PAH, benzo[a]pyrene) carcinogenesis. In addition, the inhibition caused by , in the rate of lipoxygenase (LOX) catalyzed oxidation reaction of linoleic acid to hyperoxolinoleic acid, has been also kinetically and theoretically studied. The results are compared to that of cisplatin.
The increasing interest in the bioinorganic chemistry of organotin(IV) compounds has led to extended studies on their interactions with different types of biomolecules such as carbohydrates, nucleic acid derivatives, amino acids and peptides [1, 2]. The organotin(IV) compounds are exhibiting significant antitumor activity [1β8]. More particularly, organotin(IV) complexes with ligands containing phenolic βOH groups and a heterocyclic nitrogen donor atom comprise an interesting class of such complexes because they contain an amide group [9, 10]. Surprisingly, only few organotin(IV) complexes of this type have been structurally characterized up to now [10]. Recently, the inhibition caused by organotin(IV) complexes of thioamide ligands towards lipoxygenase (LOX) catalyzed oxidation reaction of linoleic acid to hyperoxolinoleic acid in relation with the antitumor activity caused by these complexes was studied [3β8] and a mechanism of free radicals was proposed. 2-Thiobarbituric acid, on the other hand, is a reagent in use for the detection of lipid hydroperoxides and lipid oxidation [11, 12].
In order to investigate further the mechanism of cytotoxic activity of organotin(IV)-thioamide complexes, we report here the synthesis of a new complex with formula [(n-Bu)3Sn(TBA)β H2O] (1) (HTBA is the 2-thiobarbituric acid) (Scheme 1). The complex has been characterized by elemental analysis and 119Sn-NMR and FT-IR spectroscopic techniques. The structure of the complex was also determined by X-ray crystallography at 120(2)βK. The tri-n-butlyltin derivative was chosen, since it is known to possess antiparasitic properties [1, 2]. 2-Thiobarbituric acid, a well-known reagent in use for the determination of the lipid peroxidation in biological systems, is chosen in order to possibly increase the LOX inhibition activity of organotin moiety [3β8, 11, 12]. The anticancer cell screening results of the compound tested are also reported. The inhibition caused by 1, in the rate of lipoxygenase (LOX) catalyzed oxidation reaction of linoleic acid to hyperoxolinoleic acid has also been kinetically and theoretically studied.
Complex 1 was synthesized by reacting a methanolic solution of tri-n-butlyltin(IV) chloride (n-Bu)3SnCl with an aqueous solution of 2-thiobarbituric acid (HTBA) which contains an equimolar amount of potassium hydroxide. The structure was solved by direct methods SHELXS97 [13] and successive difference Fourier syntheses. Refinement applied full-matrix least-squares methods SHELXL97 [14]. Atomic scattering factors for neutral atoms and real and imaginary dispersion terms were taken from International Tables for X-ray Crystallography [15]. Intensity data for the colorless crystals were collected on a Nonius Kappa CCD diffractometer with graphite-monochromated MoK radiation at 120(2)βK. C16H32N2O3SSn, MWβ= 451.19, monoclinic in P21/n, aβ= 11.0956(2), bβ= 17.3425(4), c = 11.1879(2)βΓ , β= 95.3080(10)Β°, V = 2143.60(7)βΓ 3, Zβ= 4, Dβ= 1.398βMg/m3, β= 1.303βmm-1, final R = 0.0247 for 4906 unique observed [F2 > 2 Ο (F2)] diffractometer data. Measurements of in vitro cells toxicity have been carried out in preliminary repetitions according to the method described in literature [3β8].
The ir spectrum of complex 1 shows distinct absorption at 2959βcm-1 due to the CβH bond vibrations of n-butyl groups, at 1546 and 1398βcm-1, which are assigned to (CN) vibrations (thioamide I and II bands) and at 1194 and 906βcm-1, which are attributed to the (CS) vibrations (thioamide III and IV bands). The corresponding thioamide I and II bands in crystalline HTBA appear at 1527 and 1350βcm-1 while thioamide bands III and IV are observed at 1154 and 801βcm-1 [16].
119Sn-NMR spectrum of complex 1, in DMSO-d6 solution, shows a resonance signal at 5.7βppm indicating a four coordinated Sn atom [17]. Since the corresponding value for the (n-Bu)3SnCl in DMSO-d6 is found to be at 2.7βppm [18], this is indicative of a partial positive charged Sn atom in 1 (see crystal structure). Chemical shifts are given in ppm referenced to119Sn-Me4Sn. The stability of 1 in DMSO-d6 solution was verified by recording its 1H-NMR spectrum, as a function of time. Free HTBA ligand shows a resonance signal at 12.1βppm (s, H(N)), 4.9βppm (s, H(C)), and 3.5 ppm (s, H(C)) (Scheme 1) [16] which are shifted at 10.9βppm (s, H(N)) and at 4.2βppm (s, H(C)) in case of 1 . The signal at 3.5βppm (s, H(C)) could not be observed in the 1H-NMR of the complex since enol-keton tautomerims can not be established in case of coordinated HTBA. Resonance signals at 1.55βppm (t), 1.28βppm (m), 1.09βppm (m), and at 0.87βppm (t) were assigned to the H(C) of the n-butyl group.
A diagram of 1 as well as selected bond lengths and angles are shown in Figure 1(a).
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(b)
The structure of compound 1 consists of one (-Bu)3Sn(IV) moiety bonded with a de-protonated 2-thiobarbituric acid (HTBA) molecule and a water molecule. The Sn1 atom exhibits a distorted trigonal bipyramidal configuration with C (5), C (9), and C (13) occupying the equatorial and O2 from HTBA ligand and O3 from the water molecule, occupying the axial positions. According to Reedijkβs geometric parameter ( = (β)/60 where is the greatest and the second greatest bond angle around the metal center) [19] the calculated value is 0.94, being equal to zero for perfectly tetragonal pyramidal geometry and unity for perfectly trigonal pyramidal [19].
The Sn1βO2 bond distance of 2.2287(14)βΓ is in accordance with that found in [Ph2(pyO)SnCH2Sn(OH)Ph2]2 (where pyO = anion of 2-hydroxypyridine), [10] (SnβOβ= 2.227(2)βΓ ). The two CβO bond distances (C1βO2β= 1.274(2), and C3βO1 = 1.261(2)βΓ , resp.) are almost equal. The C1βC2 and C2βC3 bond lengths of 1.386(3) and 1.394(3)βΓ , respectively, are also equal. This bond distribution in 1 (shown in Scheme 2) leads to a zwitterionic form of the compound (Scheme 2) and is in agreement with 119Sn-NMR, in DMSO-d6 solutions. The molar conductance (Ξm) value of the complex in DMSO solution (5 10-3M) is 5.3β(cm-1mole-1Ξ©-1) showing that the complex is not conducting in solution confirming the stability of the zwiterion, also in solution [20].
Contrary to this coordination mode, HTBA coordinates to the gold(I) ion through its deprotonated form with the negative charge to be located at the sulphur atom forming neutral complexes [21].
Extended intermolecular hydrogen bonding interactions [H96]S = 3.2692(17), N1[H97]Oβ= 2.790(2), O3[H98]O = 2.630(2), and O3[H99]S = 3.2302(17)βΓ , respectively, where the symmetry transformations used to generate equivalent atoms are (i) βx+1, βy, βz+2, (ii) βx+2, βy, βz+2, (iii) x+1/2, βy+1/2, zβ1/2, (iv) βx+3/2, y+1/2, βz+3/2 lead to the supramolecular assembly of the complex (Figure 1(b)).
The influence of complex 1 on the oxidation of linoleic acid by the enzyme LOX was studied in a wide concentration range. The degree of LOX activity (A, %) in the presence of the complex was calculated according to the method described previously [3β8]. Figure 2 gives the inhibitory effect of complex 1 at various concentrations. It is shown that the catalytic activity of LOX was decreased in the presence of low concentrations (about 5β75βM) of the complex 1 (IC50β= 25βM) while no such activity was shown for cisplatin [3β8]. These values are comparable to the ones found for other similar Sn(IV) complexes. For example, the IC50 values found for the organotin compounds tested towards LOX, were 26 and 14βM for [(C6H5)2SnCl(HMNA)] and [(C6H5)3Sn(MNA)Sn(C6H5)3 (acetone)] (H2MNAβ= 2-thiobarbituric acid), respectively [6], 19, 16, and 21βM for ([(C6H5)3Sn(MBZT)]), ([(C6H5)3Sn(MBZO)]), and ([(C6H5)3Sn(CMBZT)]) (MBZTβ= 2-mercapto-benzothiazole, MBZO = 2-mercapto-benzoxazole and CMBZTβ= 5-chloro-2-mercapto-benzothiazole), respectively [3], 10, 13, and 14βM for ([(C6H5)2Sn(CMBZT)2]), ([(n-C4H9)2Sn(CMBZT)2]), and ([(CH3)2Sn(CMBZT)2]), respectively [3] and 61.3, 26.2, 20.5, and 16.9βM for ([(CH3)2Sn(PMT)2]), ([(n-C4H9)2Sn(PMT)2]), ([(C6H5)2Sn(PMT)2]), and ([(C6H5)3Sn(PMT)]) (PMT = 2mercapto-pyrimidine), respectively [4].
In order to investigate further the complex-protein interactions, we performed computational molecular docking studies for the complexes. The binding energy (E) of the substrate (S = linoleic acid) to its binding site in the enzyme LOX (E) when ES is the complex formed was βkcal/mole [6]. The corresponding binding energies of the inhibitor (I) are calculated to and kcal/mol for ESI and EI, respectively. Figure 3 shows the binding site of compound 1 towards LOX. Compound 1 binds to both ESI and EI complexes at the same pocket where the strong inhibitors of LOX bind [3], supporting its strong inhibition activity, found experimentally. Since high inhibition activity of LOX has been detected for all cytotoxic organotin(IV)-thione compounds tested previously, [3β8] such a strong activity is also expected for this compound.
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Complex 1 was also tested for antitumor potential against sarcoma cancer cells (mesenchymal tissue) from the Wistar rat, polycyclic aromatic hydrocarbons (PAH, benzo[a]pyrene) carcinogenesis. Cytotoxic activity for complex 1 was evaluated as % percentage of the cell survived in variable concentrations 50 to 1000βnM (or 0.05 to 1βM) of the complex after 24 hours. The IC50 value found for 1 was 125βnM or 0.125βM indicating very strong cytotoxic activity against leiomyosarcoma cells as compared to cisplatin (IC50β= 4-5βM [8]). The corresponding IC50 values of other organotin(IV) complexes found against leiomyosarcoma cells were 0.005βM for [(C6H5)3Sn(MNA)Sn(C6H5)3 (acetone)] [7], 1.5β3, 1.3β3, and 0.5β0.8βM for ([(C6H5)3Sn(MBZT)]), ([(C6H5)3Sn(MBZO)]), and ([(C6H5)3Sn(CMBZT)]) (MBZTβ= 2-mercapto-benzothiazole, MBZO = 2-mercapto-benzoxazole and CMBZTβ= 5-chloro-2-mercapto-benzothiazole), respectively [3], 0.3β0.5, 0.6β0.8, and 5β7.5βM for ([(C6H5)2Sn(CMBZT)2]), ([(n-C4H9)2Sn(CMBZT)2]), and ([(CH3)2Sn(CMBZT)2]), respectively [3] and 20β60, 0.7, 1-2, and 0.1βM for ([(CH3)2Sn(PMT)2]), ([(n-C4H9)2Sn(PMT)2]), ([(C6H5)2Sn(PMT)2]), and ([(C6H5)3Sn(PMT)]) (PMT = 2mercapto-pyrimidine), respectively [4].
Acknowledgments
This work was carried out in partial fulfillment of the requirements for an M.S. thesis of Mr. V.I. Balas within the graduate program in Bioinorganic Chemistry financed by the Ministry of Education of Greece and coordinated by Professor N. Hadjiliadis.