HYBRIDS AND INDUCED AMPHIPLOIDS OF ELYMUS CANADENSIS X AGROPYRON LIBANOTICUM

North American Elymus canadensis L., 2n = 28, and Asian Agropyron libanoticum Hack., 2n = 14, crossed with ease and yielded vigorous but sterile F₁ hybrids, 2n = 21. Chromosome pairing in the hybrids averaged 9.47^I, 5.38^II, and 0.26^III in 150 metaphase-I cells. One genome of E. canadensis is more or less homologous with the A. libanoticum genome. Treatment of the F₁ hybrids with colchicine produced 42-chromosome amphiploids, C₀, which were advanced through two seed generations, C₁ and C₂. More than half of the metaphase-I cells in the C₀ amphiploids contained 21^II; and average associations were 1.09^I, 20.16^II, 0.07^III, and 0.09^IV in 116 cells. Meiosis became increasingly irregular beyond metaphase-I; nevertheless, the C₀ amphiploids produced 68% stainable pollen and averaged 0.75 seed per spikelet. Multivalent frequencies increased in advanced generations, and the C₂ amphiploids averaged 1.11^I, 19.00^II, 0.23^III, and 0.55^IV in 100 metaphase-I cells. Meiosis was essentially regular in the C₁ and C₂ amphiploids beyond metaphase I, and the C₂ amphiploids averaged 73% stainable pollen and 2.28 seeds per spikelet. The amphiploids have an excellent chance of developing into a meiotically stable, fertile, new species. Forage characteristics of the amphiploids indicate that they have considerable economic potential as a forage grass.     

The ‘A’ genome donor of Eleusine coracana (L.) Gaertn. (Gramineae)

Summary In an attempt to discover A and B genome donor(s) to finger millet, Eleusine coracana, or its progenitor species, E. africana (both allotetraploid 2n=4x=36), five diploid species, E. Indica, E. Floccifolia, E. multiflora, E. tristachya and E. intermedia, were crossed to finger millet and its progenitor taxon. Crosses were successful only with E. coracana. Three combinations of triploid hybrids E. coracana x E. indica, E. coracana x E. floccifolia, and E. coracana x E. multiflora were obtained and analysed. Meiotic behaviour was perfectly normal in parental species. The regular number of 18 bivalents in E. coracana, 9 bivalents in E. indica, E. intermedia, E. tristachya and E. floccifolia and 8 bivalents in E. multiflora were invariably noticed. In E. coracana x E. indica hybrids a mean chromosome pairing of 8.84_I+8.80_II+0.03_III+0.10_IV per cell was found. About 86.5% of the cells showed the typical 9_I+9_II configuration, suggesting that E. indica (AA) is one of the diploid genome donors to cultivated species E. coracana. A mean chromosome pairing of 11.08_I+7.63_II+0.16_III+0.04_IV per cell was found in E. coracana x E. floccifolia hybrids. Two to ten bivalents and varying numbers of univalents were seen in 55% of the cells. About 45% of the cells showed the 9_I+9_II configuration. Various evidence suggests that perennial E. floccifolia is a primitive member of the A genome group of Eleusine species, and it may not be a genome donor to E. coracana. In E. coracana x E. multiflora hybrids (2n=26) mean chromosome pairing of 21.45_I+1.97_II+0.13_III+0.04_IV per cell was found. About 91% of the cells were observed to have 20–26 univalents. Only a small percentage of the cells contained bivalents or multivalents. This pairing behaviour indicates that E. multiflora lacks genomic homology with the A or B genome of E. coracana. Genomically E. multiflora is a distinct species and a genomic symbol of C is assigned to it. Identification of the B genome donor species to cultivated millet. E. coracana remains elusive.     

Cytogenetic studies on natural intergeneric hybridization inAster alliances

Natural intergeneric hybrids betweenAster ageratoides subsp.ovatus (2n=36) andKalimeris incisa (2n=72) were found. All of the hybrids studied were found to have 2n=72, 18 more chromosomes than a regular F₁ hybrid. The hybrids were found to be of two types: one having 18 large chromosomes ofovatus, and the other having 9 large chromosomes of the same subspecies. In meiosis of the PMCs of the hybrid with 18 large chromosomes, a regular chromosome configuration, 36_II, was observed. In PMCs of the hybrid with 9 large chromosomes an irregularity of chromosome pairings was observed, showing varied chromosome configurations: 35_II+2_I, 34_II+4_I, 33_II+6_I, I_III+33_II+3_I, 1_IV+32_II+4_I, 32_II+8_I, 31_II+10_I, 29_II+14_I, 3_III+29_II+5_I. Most univalents were large, but a few were small. The hybrids with 18 large chromosomes were found to be partial amphidiploid and possessing double chromosome complements ofovatus. The hybrids with 9 large chromosomes were found to be the first backcrossed generation between the hybrid with 18 large chromosomes andK. incisa.     

Ordering selected Zn(II), Cu(II), Pd(II) and Co(III) complex compounds: their separately and combinedly antibacterial therapy and DNA-binding studies

Abstract

In this study, four Co(III)-, Cu(II)-, Zn(II)- and Pd(II)-based potent antibacterial complexes of formula K₃[Co(ox)₃]·3H₂O (I), [Cu(phen)₂Cl]Cl·6.5H₂O (II), [Zn(phen)₃]Cl₂ (III) and [Pd(phen)₂](NO₃)₂ (IV) (where ox is oxalato and phen is 1,10-phenanthroline) were synthesized. They were characterized by elemental analysis, molar conductivity measurements, UV–vis, Fourier transform infrared (FT-IR) and proton nuclear magnetic resonance (¹H-NMR) techniques. These metal complexes were ordered in three combination series of I+II, I+II+III and I+II+III+IV. Antibacterial screening for each metal complex and their combinations against Gram-positive and Gram-negative bacteria revealed that all compounds were more potent antibacterial agents against the Gram-negative than those of the Gram-positive bacteria. The four metal complexes showed antibacterial activity in the order I > II > III > IV, and the activity of their combinations followed the order of I+II+III+IV > I+II+III > I+II. The DNA-binding properties of complex (I) and its three combinations were studied using electronic absorption and fluorescence (ethidium bromide displacement assay) spectroscopy. The results obtained indicated that all series interact effectively with calf thymus DNA (CT-DNA). The binding constant (K_b), the number of binding sites (n) and the Stern–Volmer constant (K_sv) were obtained based on the results of fluorescence measurements. The calculated thermodynamic parameters supported that hydrogen bonding and van der Waals forces play a major role in the association of each series of metal complexes with CT-DNA and follow the above-binding affinity order for the series.

Communicated by Ramaswamy H. Sarma     

THE ORIGIN OF AGROPYRON SMITHII

The hypothesis that North American octoploid Agropyron smithii Rydb., 2n = 56, originated by hybridization between tetraploid Agropyron and Elymus species, followed by chromosome doubling, was tested by observing chromosome pairing in hybrids of A. smithii with an induced amphiploid, 2n = 56, derived from E. canadensis L., 2n = 28, X E. dasystachys Trin., 2n = 28, F₁'s. Chromosome pairing in A. smithii averaged 0.52^I, 27.70^II, 0.01^III, and 0.01^IV in 184 metaphase-I cells; and the amphiploid averaged 1.13^I and 27.44^II in 195 cells. Chromosome pairing in A. smithii X amphiploid hybrids averaged 8.20^I, 23.38^II, 0.34^III, and 0.05^IV in 101 metaphase-I cells. It was concluded that A. smithii was genomically similar to the E. canadensis-E. dasystachys amphiploid. The basic genome formula of the amphiploid is SSHHJJXX, with the SSHH genomes coming from E. canadensis and the JJXX genomes coming from E. dasystachys. Consideration of the morphological, ecological, and reproductive characteristics of all North American species that contain the basic SSHH and JJXX genomes led to the conclusion that A. dasystachyum (Hook.) Scribn., SSHH, and E. triticoides Buckl., JJXX, are the probable progenitors of A. smithii.     

Interspecific hybridization between Vigna pubescens and V. unquiculata (L.) Walp through embryo rescue

Interspecific hybridization was achieved between cowpea (Vigna unquiculata [L.] Walp) and a hairy wild relative (V. pubescens). Hybrid embryos which otherwise would have shrivelled and failed to germinate were excised prematurely and cultured on a solidified MS medium. The F₁ plants were vigorous in growth, partially sterile, slightly hairy and showed some intermediate features between the two parental types. Cytological investigations on F₁ pollen mother cells showed average chromosome associations per cell of 0.66_I+10.00_II+0.34_IV.     

Cytogenetic studies on natural intergeneric hybridization inAster alliances

The karyotype and meiosis of the 12-ploid plants—one of the offspring of the natural F₁ hybrid (Aster ageratoides subsp.ovatus (2n=36) ×Kalimeris incisa (2n=72), 2n=72)—were examined. The 2n=108 chromosomes of the 12-ploids were found to consist of 18 large chromosomes and 90 small chromosomes. In meiosis of the PMCs of the 12-ploid, chromosome configurations of 3_III+46_II+7_I, 2_III+48_II+6_I and 3_III+47_II+5_I were observed. All the univalents and trivalents were small, and among the 46–48 bivalents nine were large and the remaining 37–39 were comparatively small. The large bivalents were found to represent autosyndetic pairings, and the small bivalents and trivalents were probably formed by autosyndetic pairings. The large chromosomes of the 12-ploids were found to coincide with the large chromosomes ofovatus, and the 90 small chromosomes to correspond to small chromosomes ofovatus andK. incisa. The 12-ploids were concluded to have been produced by a fusion of an unreduced gamete of the F₁ plant and a reduced gamete ofK. incisa which was growing in proximity to the F₁s. Thus the 12-ploids were regarded to be an amphidiploid having 36 chromosomes ofovatus and 72 chromosomes ofK. incisa.     

THE ORIGIN OF AGROPYRON LEPTOURUM

Colchicine-induced amphiploids, 2n = 42, of diploid Agropyron libanoticum Hack., 2n = 14, X tetraploid A. caninum (L.) Beauv., 2n = 28, were morphologically and cytologically similar to A. leptourum (Nevski) Grossh., 2n = 42. Both A. leptourum and the induced amphiploids were self-fertilizing. The induced amphiploids crossed readily with A. leptourum and gave rise to partially fertile hexaploid hybrids. Chromosome pairing in the hybrids averaged 0.60^I, 18.29^II, 0.36^III, 0.58^,v, 0.02^v, and 0.22^VI in 90 diakinesis or metaphase-I cells. The genomes of the induced amphiploids are essentially homologous with those of A. leptourum except for two or more reciprocal translocations. The morphological, cytological, fertility, and crossing data provide conclusive evidence that A. libanoticum and A. caninum, or their close relatives, are the parents of A. leptourum. The genome formulas of A. libanoticum, A. caninum, and A. leptourum may be written as SS, S_xS_xH_xH_x, and SSS_xS_xH_xH_x, respectively, where S is the basic A. libanoticum genome and H is a genome derived from Hordeum.     

Cytological relationships in theConvolvulus pluricaulis complex

InConvolvulus pluricaulis Chois. two forms (2n=18, 36) along with one colchicine-autotetraploid have been investigated morphologically and cytologically. The diploid regularly formed 9_II although in the “off-season” plants certain irregularities were observed including formation of unreduced pollen grains. The natural tetraploid and the colchicine-autotetraploid had mean frequencies of configurations of 1.56_IV+14.04_II+1.48_I and 2.95_IV+0.56_III+11,43_II+0.8_I, respectively. The mode of chromosome association in the two types of tetraploids was comparable. A comparison of the morphological characters of the two tetraploid types, further, suggested close similarity. In addition they were indistinguishable from the diploid from except being gigas. From these data it is inferred that the natural tetraploid presumably arose as a result of direct duplication of the diploid form, through the chance fusion of unreduced spores. The lower quadrivalent frequency of the natural polyploid is ascribed to a gradual shift towards bivalent association accompanying natural selection for fertility. The taxonomic status of the two forms (2x, 4x) is discussed and the varietal status accorded to the tetraploid form is supported.     

Intergeneric hybridization between Brassica napus and Sinapis pubescens,and the cytology and crossability of their progenies

The cytological possibility of gene transfer from Sinapis pubescens to Brassica napus was investigated. Intergeneric hybrids between Brassica napus (2n = 38) and Sinapis pubescens (2n = 18) were produced through ovary culture. The F₁ hybrids were dihaploid and the chromosome configurations were (0–1) _III + (2–11) _II + (5–24) _I . One F₂ plant with 38 chromosomes was obtained from open pollination of the F₁ hybrid. Thirty-one seeds were obtained from the backcross of the F₂ plant with B. napus. Five out of seven plants had 38 chromosomes, and the pollen stainability ranged from 0% to 81.4%. In the B₂ plants obtained from the backcross of B₁ plants with B. napus, 66.7% of the plants examined had 38 chromosomes. S. pubescens may become a gene source for the improvement of B. napus.     

Successful crosses between Festuca arundinacea Schreb. and Dactylis glomerata L.

Summary Five F₁ plants have been obtained after extensive crossing between different ecotypes or varieties of Festuca arundinacea Schreb. and Dactylis glomerata L. The success did not appear to depend on specific treatments (spraying with -aminocaproic acid or gibberellic acid or pre-pollination with killed pollen from the seed parent), but the crossability is limited to exceptional plants.F₁ hybrids showed characteristics of both the parents. In four hybrids various developmental disturbances were observed (low viability, aneusomaty, absence of development of inflorescences). Only one hybrid consistently showed 2n=35 chromosomes, good viability and growth, however, it was sterile. After clonal propagation, attempts for polyploidization were started.     

The Effect of 15-Ketosterol Analogues with a 5,6-Dimethylhept-3-en-2-yl Chain at C17 on Cholesterol Metabolism in Hep G2 Hepatoma Cells

The effect on cholesterol metabolism in Hep G2 hepatoma cells was studied for new analogues of 15-ketosterol [3-hydroxy-5-cholest-8(14)-en-15-one] (I): (24S)-3-hydroxy-24-methyl-5-cholesta-8(14),22-diene-15-one (II), (24S)-3-hydroxy-24-methyl-5-cholesta-8(14),22-diene-15-one (III), and (24S)-24-methyl-5-cholesta-8(14),22-diene-3,15-dione (IV). Analogues (I) and (II) were found to be equally effective inhibitors of cholesterol biosynthesis after a 3-h incubation with Hep G2 cells; however, (II) produced a stronger inhibitory effect after a 24-h incubation or after an incubation of cells preliminarily treated with the inhibitor in a medium containing no ketosterol. The ability of ketosterols to inhibit cholesterol biosynthesis decreased in the order (II) > (IV) > (III). Ketosterol (II) inhibited, whereas ketosterol (III) stimulated the biosynthesis of cholesteryl esters. (IV) stimulated the biosynthesis of cholesteryl esters at a concentration of 1–10 M and exerted no marked effect at a concentration of 30 M. These results indicate that 8(14)-15-ketosterols containing a modified side chain are of interest as regulators of cholesterol metabolism in liver cells.     

New derivatization and separation procedures for reducing oligosaccharides

4-Trifluoroacetamidoaniline was reacted with reducing oligosaccharides in the presence of sodium cyanoborohydride to give aminoalditol derivatives, useful for linkage to proteins or solid matrices. A mixture of reducing oligosaccharides, difficult to separate by HPLC, was treated in the same way. The resulting derivatives were easily separated by HPLC.Abbreviations TFAN 4-trifluoroacetamidoaniline - LcOse₄ lacto-N-tetraose - IV²Fuc-LcOse₄ lacto-N-fucopentaose l - III⁴Fuc-LcOse₄ lacto-N-fucopentaose II - III³Fuc-nLcOse₄ lacto-N-fucopentaose III - IV²Fuc, III⁴Fuc-LcOse₄ lacto-N-difucohexaose I - II⁶Galß1-4GlcNAc-LcOse₄ lacto-N-hexaose - II³NeuAc-Lac 3-sialyllactose - GlcNAcß1-4GlcNAcß1-4GlcNAc chitotriose - GalNac1-3|Fuc1-2|Galß1-4Glc A-tetrasaccharide     

Three new HLA-G alleles and their linkage disequilibria with HLA-A

Three new allelic forms of the HLA-G DNA sequence (HLA-G*II, HLA-G*III, and HLA-G*IV) have been identified. With the HLA-G*I sequence (previously designated HLA 6.0) as a reference, HLA-G*II shows a silent (G A) mutation at the third base of codon 57, HLA-G*III bears a non-synonymous (A T), but conservative, (Thr Ser) substitution at the first base of codon 31, and HLA-G*IV shows two silent substitutions: (A T) at the third base of codon 107 and (G A) at the third base of codon 57. A rapid method of singling out each allele on genomic DNA has been developed by using polymerase chain reaction amplification followed by restriction endonuclease treatment. Also, more or less strong linkage disequilibria has been found between most HLA-A alleles and either HLA-G*I or *II, both being the most prevalent alleles in the population, with a genotypic frequency of 0.55 and 0.38, respectively; HLA-G*III is very rare and HLA-G*IV has a genotypic frequency of 0.07. An evolutive classification of HLA-A alleles results according to their association with either HLA-G*I or HLA-G*II, which does not correlate with the classical serological cross-reacting groups classification. The finding of a strong and selective A/G linkage disequilibria with most HLA-A alleles, together with the existence of less frequent random A/G associations, may suggest that there exist in different haplotypes true and varied A/G genetic distances (and not a recombinational hotspot). It may be inferred from preliminary data that in primates HLA-A/G haplotypes bearing G*II may have appeared later than those bearing G*I.The nucleotide sequence data reported in this paper have been submitted to the GenBank and EMBL nucleotide sequence databases and have been assigned the following accession numbers: EMBL-X60983 (HLA-G*II), GenBank-M99048 (HLA-G*III), and GenBank-L07784 (HLA-G*IV).The contribution to this paper by P. Morales and A. Corell is equal, and the order of authorship is arbitrary. Correspondence to: A. Arnaiz-Villena.     

The ganglioside GD1α, IV3Neu5Ac,III6Neu5Ac-GgOse4Cer,is a major disialoganglioside in the highly metastatic murine lymphoreticular tumour cell line MDAY-D2

The aim of the present study was to investigate the ganglioside expression of the highly metastatic murine lymphoreticular tumour cell line MDAY-D2. Cells were propagated under controlled pH conditions and oxygen supply in bioreactors of 1 and 7.5l volumes by repeated batch fermentation. Gangliosides were isolated from 2.7×10¹¹ cells, purified by silica gel chromatography and separated into mono- and disialoganglioside fractions by preparative DEAE anion exchange high performance liquid chromatography. Individual gangliosides were obtained by preparative thin layer chromatography. Their structural features were established by immunostaining, fast atom bombardment and gas chromatography mass spectrometry. In addition to gangliosides of the G_M1a-pathway (G_M2, G_M1a and G_D1a) and G_M1b (IV³Neu5Ac-GgOse₄Cer) and GalNAc-G_M1b of the G_M1b-pathway, the dis8aloganglioside G_D1 (IV³Neu5Ac, III⁶Neu5Ac-GgOse₄Cer) was found in equal amounts compared to G_D1a (IV³Neu5Ac, II³Neu5Ac-GgOse₄Cer). All gangliosides were substituted with C_24:0,24:1 and C_16:0 fatty acids, sphingosine andN-acetylneuraminic acid as the sole sialic acid. Abbreviations: FAB-MS, fast atom bombardment-mass spectrometry; GC-MS, gas chromatography-mass spectrometry; GSL(s), glycosphingolipid(s); HPLC, high performance liquid chromatography; HPTLC, high performance thin layer chromatography; Neu5Ac,N-acetylneuraminic acid; Neu5Gc,N-glycoloylneuraminic acid [57]. The designation of the following glycosphingolipids follows the IUPAC-IUB recommendations [58] and the nomenclature of Svennerholm [59]. Gangliotriaosylceramide or GgOse₃Cer, GalNAc1-4Gal1-4Glc1-1Cer; gangliotetraosylceramide or GgOse₄Cer, Gal1-3GalNAc1-4Gal1-4Glc1-1Cer gangliopentaosylceramide or GgOse₅Cer, GalNAc1-4Gal1-3GalNAc1-4Gal1-4Glc1-1Cer; G_M2, II³Neu5Ac-GgOse₃Cer; G_M1a, II³Neu5Ac-GgOse₄Cer; G_M1b, IV³Neu5Ac-GgOse₄Cer; GalNAc-G_M1b, IV³Neu5Ac-GgOse₅Cer; G_D1a, IV³Neu5Ac, II³Neu5Ac-GgOse₄Cer; G_D1b, II³(Neu5Ac)₂-GgOse₄Cer; G_D1 or G_D1e, IV³Neu5Ac, III⁶Neu5AcGgOse₄Cer; G_D1e, IV³(Neu5Ac)₂-GgOse₄Cer; G_T1b, IV³Neu5Ac, II³(Neu5Ac)₂-GgOse₄Cer.     

Gas Chromatographic Determination of Optical Isomers of α-Phenylethylamine and α-Phenyl-β-(p-tolyl)-ethylamine on Optically Active Stationary Phases

The nondialyzable melanoidins prepared from glucose-butylamine (I) and xylose–butylamine (II) reaction systems, freeze-dried powder obtained from the dialyzable fraction of the glucose–butylamine reaction system (III) and N-butyl-glucosylamine (IV) were pyrolyzed at 350°C for 0.5-2 hr and the volatile pyrolysate was investigated. To trap the volatile compounds, Tenax GC trapping and cold trapping methods were used. Identification of these volatiles was made by gas chromatography-mass spectrometry, using a glass capillary column. The volatile components in the pyrolysates of I, II, III and IV were qualitatively similar to each other. The major volatile components in the pyrolysates of I, II, III and IV were identified as two furans, 1-butanol, two 1-butylpyrroles, 1-butylpyrrolidine, 1-butylaziridine and two N-butylamides. The results are discussed in relation to those obtained from previously investigated sugar-amino acid melanoidins.     

Cytogenetics of ditelotetrasomics for short arms of four chromosomes of barley (Hordeum vulgare L.)

Summary Plants with a pair of extra homologous telocentric chromosomes in addition to the normal chromosome complement are called ditelotetrasomics. Six types of ditelotetrasomics of barley have been obtained. Four types obtained in the selfed progenies of telotrisomics (Triplo 2S, Triplo 5S, Triplo 6S, and Triplo 7S) are reported in this paper. The ditelotetra 2S showed a stronger expression of the diagnostic characteristics of Triplo 2S. It was weak and small, with narrow, short, dark-green leaves, and was almost completely pollen and seed sterile. However, three other ditelotetrasomics (ditelotetra 5S, 6S, and 7S) did not show specific diagnostic characteristics and were similar to normal diploid plants, with the exception of ditelotetrasomic 5S, which showed some effects. At meiotic diakinesis and metaphase I, these ditelotetrasomic plants showed chromosome configurations of 6_II+1_IV, 7_II+1 telo_II, 6_II+1_III+1telo_I, or 7_II+2 telo_I. Most of the sporocytes at anaphase and telophase in the first and second meiotic divisions showed almost normal chromosome behavior. Quartets were mostly normal with no micronuclei. Approximately 30% of the selfed progenies of these three ditelotetrasomics were ditelotetrasomics and almost 50% were telotrisomics, indicating a high percentage of male and female transmission of the extra telocentric chromosomes.     

Antibacterial combination therapy using Co3+, Cu2+, Zn2+ and Pd2+ complexes: Their calf thymus DNA binding studies

Four Co(III)-, Cu(II)-, Zn(II)-, and Pd(II)-based potent antibacterial complexes of formula K₃[Co(ox)₃].3H₂O (I), [Cu(bpy)₂Cl]Cl.5H₂O (II), [Zn(bpy)₃]Cl₂ (III), and [Pd(bpy)₂](NO₃)₂ (IV) (where ox is oxalate and bpy is 2,2′-bipyridine) were synthesized. They were characterized by elemental analyses, molar conductance measurements, UV–Vis, FTIR, ¹H NMR, and ¹³C NMR spectra. These metal complexes were ordered in three combination series of I + II, I + II + III, and I + II + III + IV. Antibacterial activity was tested for each of these four metal complexes and their combinations against Gram-positive and Gram-negative bacteria. All compounds were more potent antibacterial agents against the Gram-negative than those of the Gram-positive bacteria. The four metal complexes showed antibacterial activity in the order I > II > III > IV and the activity of their combinations followed the order of I + II + III + IV > I + II + III > I + II. CT-DNA binding studies of complex I and its three combinations were carried out using UV–vis spectral titration, displacement of ethidium bromide (EB), and electrophoretic mobility assay. The results obtained from UV–vis studies indicated that all series interact effectively with CT-DNA. Fluorescence titration revealed that the complexes quench DNA-EB strongly through the static quenching procedures. The binding constant (K_b), the Stern–Volmer constant (K_sv), and the number of binding sites (n) were determined at different temperatures of 293, 300, and 310 K, respectively. The calculated thermodynamic parameters supported that hydrogen binding and Van der Waals forces play a major role in association of each series of metal complexes with CT-DNA and follow the above-binding affinity order for the series.