Your search keyword '"Nucleic Acid Denaturation drug effects"' showing total 412 results

151. Evaluation of zearalenone and alpha-zearalenol toxicity on boar sperm DNA integrity.

Author

Tsakmakidis IA, Lymberopoulos AG, Khalifa TA, Boscos CM, Saratsi A, and Alexopoulos C

Subjects

Acridine Orange, Animals, Cell Nucleus drug effects, Cell Nucleus ultrastructure, Chromatin drug effects, Chromatin ultrastructure, Fluorescent Dyes, Male, Nucleic Acid Denaturation drug effects, Sperm Motility drug effects, Swine, Zeranol toxicity, Zona Pellucida physiology, DNA drug effects, Spermatozoa drug effects, Zearalenone toxicity, Zeranol analogs & derivatives

Abstract

This study aimed at investigating the in vitro effects of zearalenone (zen) and alpha-zearalenol (alpha-zen) on motility and nuclear chromatin integrity (NCI) of boar spermatozoa. Mycotoxins were tested, at levels ranging from 10 to 30 microg ml(-1) of diluted semen. Four boars were used for semen collection (eight replicates per boar, four per mycotoxin). After the addition of zen or alpha-zen, semen samples were incubated for 4 h at 38.5 degrees C, 5% CO(2) and 96% humidified air. Motility and NCI were assessed at 0 and 4 h of incubation. No significant differences were noticed in motility among the experimental groups (P > 0.05) for all tested boars. Chromatin instability was significantly higher (P < 0.05) in spermatozoa of only one boar treated with zen and alpha-zen independently of the dose. In conclusion, under our experimental conditions, zen and alpha-zen did not affect the motility of boar sperm, whereas the effects of these toxins on sperm NCI were individual-dependent., (2008 John Wiley & Sons, Ltd)

Published

2008

152. Antibacterial and membrane damaging activity of Livistona chinensis fruit extract.

Author

Kaur G and Singh RP

Subjects

Animals, Anti-Bacterial Agents analysis, Cell Membrane drug effects, Fruit chemistry, Leukocytes drug effects, Nucleic Acid Denaturation drug effects, Phenols analysis, Plant Extracts analysis, Potassium metabolism, Swine, Anti-Bacterial Agents pharmacology, Arecaceae chemistry, Medicine, Chinese Traditional, Phenols pharmacology, Plant Extracts pharmacology, Staphylococcus aureus drug effects

Abstract

Livistona chinensis is used in traditional Chinese medicine as an anticancer agent. Experimental studies have shown the antiproliferative and antiangiogenic properties of extracts of L. chinensis fruits and seeds. In the present study, qualitative phytochemical composition of L. chinensis fruits was investigated. We hypothesized that the presence of high concentration of phenolic compounds with astringent properties may result in bacterial cell death. Hence, antibacterial activity of an aqueous extract of L. chinensis fruits was investigated against Staphylococcus aureus. The antibacterial activity was attributed to DNA, enzyme and protein denaturing properties of the phenolic compounds present in the extract. The extract also resulted in increased membrane permeability. The antibacterial, DNA and enzyme denaturing and membrane damaging activity was limited to an acid-precipitable fraction of the extract and these effects were abrogated in presence of proteins. The membrane damaging activity of phenolic compounds was also observed in leucocytes. In conclusion, this study reported the antibacterial activity of the fruits of L. chinensis due to their high content of phenolic compounds.

Published

2008

153. A method to increase the bioactivity of plasmid DNA by heat treatment.

Author

Hou S, Yang K, Liu Z, and Feng XZ

Subjects

Cell Line, DNA chemistry, DNA ultrastructure, Electrophoresis, Agar Gel, Escherichia coli genetics, Humans, Microscopy, Atomic Force, Nucleic Acid Denaturation drug effects, Plasmids chemistry, Plasmids ultrastructure, Polyethyleneimine pharmacology, Spermidine pharmacology, Transfection, DNA analysis, DNA genetics, Hot Temperature, Plasmids analysis, Plasmids genetics

Abstract

A method to increase the bioactivity of plasmid DNA by heat treatment has been developed. The structure of the heat treated plasmid DNA was investigated by electrophoresis assay and atomic force microscope (AFM) observation. Electrophoresis assay showed that the heat treated DNA consisted of three components: the supercoiled DNA (component I), the open circular DNA (component II) and the heat denatured DNA component. The bioactivity of the heat treated plasmid DNA was investigated by both DNA condensation experiments and gene transfection experiment with mammal cells. DNA condensation experiments showed that the heat denatured DNA component owned higher sensitivity to spermidine and polyethylenimine (PEI) than component I and component II DNA. Gene transfection experiment with PEI indicated that the heat treated DNA had higher gene transfection efficiency than untreated DNA. Our experiment not only shows an effective approach to increase the bioactivity of plasmid DNA but also leads a way to improve the bioactivity of DNA by physically modifying their structure.

Published

2008

154. Probing the mechanical stability of DNA in the presence of monovalent cations.

Author

Vlassakis J, Williams J, Hatch K, Danilowicz C, Coljee VW, and Prentiss M

Subjects

Cations, Monovalent chemistry, Cations, Monovalent pharmacology, Nucleic Acid Denaturation drug effects, DNA chemistry, DNA Probes chemistry, Nucleic Acid Conformation drug effects

Abstract

We examine the interaction between monovalent cations and DNA using several different assays that measure the stability of double-stranded DNA (dsDNA). The thermal melting of dsDNA and the mechanical separation of dsDNA into two single strands both depend on the stability of dsDNA with respect to ssDNA and are sensitive to the interstrand phosphate repulsion. We find that the experimentally measured melting temperatures and unzipping forces are approximately the same for all of the ions considered in this study. Likewise, the force required to transform B-DNA into the overstretched form is also similar for all of the ions. In contrast, for a given ion concentration, the force at which the overstretched state fully relaxes back to the canonical B-DNA form depends on the cation; however, for all cations, the overstretching force decreases with decreasing ion concentration, suggesting that this force is sensitive to screening. We observe a general trend for smaller ions to produce more efficient relaxation. Finally, for a given cation, the relaxation can also depend on the anion.

Published

2008

155. 2D NMR study of the DNA duplex d(CTCTC*A*ACTTCC).d(GGAAGTTGAGAG) cross-linked by the antitumor-active dirhodium(II,II) unit at the cytosine-adenine step.

Author

Kang M, Chifotides HT, and Dunbar KR

Subjects

Adenine chemistry, Base Sequence, Cross-Linking Reagents pharmacology, Cytosine chemistry, DNA Adducts chemical synthesis, Models, Biological, Models, Molecular, Nucleic Acid Denaturation drug effects, Rhodium chemistry, Transition Temperature drug effects, Antineoplastic Agents pharmacology, DNA chemistry, Magnetic Resonance Spectroscopy, Organometallic Compounds pharmacology, Rhodium pharmacology

Abstract

The 2D NMR analysis in solution of the DNA duplex d(CTCTC*A*ACTTCC).d(GGAAGTTGAGAG) binding to the dirhodium unit cis-[Rh2(mu-O2CCH3)2(eta1-O2CCH3)]+ showed that an unprecedented intrastrand adduct, dsII, is formed with the dirhodium unit cross-linking in the major groove residues C5 and A6 (indicated with asterisks), also corroborated by enzyme digestion studies. Formation of the dirhodium complex dsII destabilizes significantly the duplex as indicated by the substantial decrease in its melting temperature (DeltaTm = -22.9 degrees C). The reduced thermal stability of dsII is attributed to the decreased stacking of the bases and the complete disruption and/or weakening of the hydrogen bonds within the base pairs in the immediate vicinity of the metalation site (C5.G20 and A6.T19), but the effects due to the metal binding are more severe for the base pairs in the 5' direction to the lesion site. The NMR spectroscopic data indicate that Watson-Crick hydrogen bonding is completely disrupted for the C5.G20 site and considerably weakened for A6.T19. In dsII, the bases C5 and A6 bind to eq positions of the dirhodium unit cis-[Rh2(mu-O2CCH3)2(eta1-O2CCH3)]+, which retains one monodentate and two bridging acetate groups, presumably due to steric reasons. Binding of A6 takes place via N7, whereas binding of the C5 base takes place via the exocyclic N4 site, resulting in the anti-cytosine rotamer with respect to site N3 in its metal-stabilized rare iminooxo form.

Published

2008

156. Compensation of DNA stabilization and destabilization effects caused by cisplatin is partially disturbed in alkaline medium.

Author

Galyuk EN, Fridman AS, Vorob'ev VI, Haroutiunian SG, Sargsyan SA, Hauruk MM, and Lando DY

Subjects

Animals, Antineoplastic Agents metabolism, Base Pairing drug effects, Base Pairing physiology, Cattle, Cisplatin metabolism, Cross-Linking Reagents metabolism, Hydrogen-Ion Concentration, Nucleic Acid Denaturation drug effects, Antineoplastic Agents pharmacology, Cisplatin pharmacology, Cross-Linking Reagents pharmacology, DNA metabolism

Abstract

Binding of the antitumor compound cisplatin to DNA locally distorts the double helix. These distortions correlate with a decrease in DNA melting temperature (Tm). However, the influence of cisplatin on DNA stability is more complex because it decreases the DNA charge density. In this way, cisplatin increases the melting temperature and partially compensates for the destabilizing influence of structural distortions. The stabilization is stronger at low Na+ ion concentration. Due to this compensation, the total decrease in the DNA melting temperature after cisplatin binding is much lower than the decrease caused by the distortions themselves, especially at low [Na+]. It is shown in this study that, besides Na+ concentration, pH also strongly influences the value of a change in the melting temperature caused by cisplatin. In alkaline medium (pH=10.5-10.8), a fall in the melting temperature caused by platination is enhanced several times with respect to neutral medium. Such a stronger drop in Tm is explained by a decrease in pK values of base pairs caused by lowering the charge density under platination that facilitates proton release. At neutral pH, the proton release is low for both control and platinated DNA and does not influence the melting behavior. Therefore, lowering in the charge density under platination, besides stabilization, gives additional destabilization just in alkaline medium. Destabilization caused by structural distortions due to this pH induced compensation of stabilizing effect is more pronounced. In the presence of carbonate ion, destabilization caused by high pH value is strengthened. As a decrease in DNA charge density, interstrand crosslinking caused by cisplatin also increases the DNA stability due to loss in the entropy of the melted state. However, computer modeling of DNA stability demonstrates that interstrand crosslinks formed by cisplatin do not stabilize long DNA. It is shown that the increase in Tm caused by interstrand crosslinking itself is compensated for by a local destabilization of the double helix at the sites of location of interstrand crosslinks formed by cisplatin.

Published

2008

157. DNA intercalation by quinacrine and methylene blue: a comparative binding and thermodynamic characterization study.

Author

Hossain M, Giri P, and Kumar GS

Subjects

Binding, Competitive, Circular Dichroism, DNA drug effects, Hot Temperature, Models, Biological, Nucleic Acid Denaturation drug effects, Thermodynamics, Titrimetry, DNA metabolism, Intercalating Agents pharmacokinetics, Methylene Blue pharmacokinetics, Quinacrine pharmacokinetics

Abstract

There is compelling evidence that cellular DNA is the target of many anticancer agents. Consequently, elucidation of the molecular nature governing the interaction of small molecules to DNA is paramount to the progression of rational drug design strategies. In this study, we have compared the binding and thermodynamic aspects of two known DNA-binding agents, quinacrine (QNA) and methylene blue (MB), with calf thymus (CT) DNA. The study revealed noncooperative binding phenomena for both the drugs to DNA with an affinity one order higher for QNA compared to MB as observed from diverse techniques, but both bindings obeyed neighbor exclusion principle. The data of the salt dependence of QNA and MB from the plot of log K versus log [Na+] revealed a slope of 1.06 and 0.93 consistent with the values predicted by theories for the binding of monovalent cations, and have been analyzed for contributions from polyelectrolytic and nonpolyelectrolytic forces. The binding of both drugs was further characterized by strong stabilization of DNA against thermal strand separation in both optical melting and differential scanning calorimetry studies. The binding data analyzed from the thermal denaturation and from isothermal titration calorimetry (ITC) were in close proximity to those obtained from spectral titration data. ITC results revealed the binding to be exothermic and favored by both negative enthalpy and positive entropy changes. The heat capacity changes obtained from temperature dependence of enthalpy indicated -146 and -78 cal/(mol.K), respectively, for the binding of QNA and MB to CT DNA. Circular dichroism study further characterized the structural changes on DNA upon intercalation of these molecules. Molecular aspects of interaction of these molecules to DNA are discussed.

Published

2008

158. Guanidinoneomycin B recognition of an HIV-1 RNA helix.

Author

Staple DW, Venditti V, Niccolai N, Elson-Schwab L, Tor Y, and Butcher SE

Subjects

Aminoglycosides chemistry, Aminoglycosides genetics, Base Sequence, Binding Sites, Frameshifting, Ribosomal genetics, Humans, Magnetic Resonance Spectroscopy, Models, Molecular, Nucleic Acid Conformation drug effects, Nucleic Acid Denaturation drug effects, RNA, Viral chemistry, RNA, Viral genetics, Substrate Specificity, Thermodynamics, Urea pharmacology, Aminoglycosides metabolism, HIV-1 genetics, RNA, Viral metabolism

Abstract

Aminoglycoside antibiotics are small-molecule drugs that bind RNA. The affinity and specificity of aminoglycoside binding to RNA can be increased through chemical modification, such as guanidinylation. Here, we report the binding of guanidinoneomycin B (GNB) to an RNA helix from the HIV-1 frameshift site. The binding of GNB increases the melting temperature (T(m)) of the frameshift-site RNA by at least 10 degrees C, to a point at which a melting transition is not even observed in 2 M urea. A structure of the complex was obtained by using multidimensional heteronuclear NMR spectroscopic methods. We also used a novel paramagnetic-probe assay to identify the site of GNB binding to the surface of the RNA. GNB makes major-groove contacts to two sets of Watson-Crick bases and is in van der Waals contact with a highly structured ACAA tetraloop. Rings I and II of GNB fit into the major groove and form the binding interface with the RNA, whereas rings III and IV are exposed to the solvent and disordered. The binding of GNB causes a broadening of the major groove across the binding site.

Published

2008

159. Quantifying DNA-protein interactions by single molecule stretching.

Author

Williams MC, Rouzina I, and Karpel RL

Subjects

DNA-Binding Proteins chemistry, Hydrogen-Ion Concentration, Kinetics, Models, Biological, Nucleic Acid Denaturation drug effects, Protein Binding drug effects, Protein Processing, Post-Translational drug effects, Protein Structure, Tertiary, Sodium Chloride pharmacology, Static Electricity, Thermodynamics, Viral Proteins chemistry, DNA metabolism, DNA-Binding Proteins metabolism, Optical Tweezers, Viral Proteins metabolism

Abstract

In this chapter, we discuss a new method for quantifying DNA-protein interactions. A single double-stranded DNA (dsDNA) molecule is stretched beyond its contour length, causing the base pairs to break while increasing the length from that of dsDNA to that of ssDNA. When applied in a solution containing DNA binding ligands, this method of force-induced DNA melting can be used to quantify the free energy of ligand binding, including the free energy of protein binding. The dependence of melting force on protein concentration is used to obtain the equilibrium binding constant of the ligand to DNA. We have applied this method to a well-studied DNA-binding protein, bacteriophage T4 gene 32 protein (gp32), and have obtained binding constants for the protein to single-stranded DNA (ssDNA) under a wide range of solution conditions. Our analysis of measurements conducted at several salt concentrations near physiological conditions indicates that a salt-dependent conformational change regulates DNA binding by gp32.

Published

2008

160. Unique properties of DNA interstrand cross-links of antitumor oxaliplatin and the effect of chirality of the carrier ligand.

Author

Kasparkova J, Vojtiskova M, Natile G, and Brabec V

Subjects

Antineoplastic Agents pharmacology, Base Sequence, Circular Dichroism, Cisplatin metabolism, Cisplatin pharmacology, Cyclohexylamines chemistry, Cyclohexylamines pharmacology, DNA genetics, HMGB1 Protein metabolism, Ligands, Nucleic Acid Conformation drug effects, Nucleic Acid Denaturation drug effects, Organoplatinum Compounds pharmacology, Oxaliplatin, Stereoisomerism, Substrate Specificity, Transition Temperature drug effects, Antineoplastic Agents chemistry, Cross-Linking Reagents chemistry, DNA chemistry, Organoplatinum Compounds chemistry

Abstract

The different antitumor and other biological effects of the third-generation antitumor platinum drug oxaliplatin [(1R,2R-diamminocyclohexane)oxalatoplatinum(II)] in comparison with those of conventional cisplatin [cis-diamminedichloridoplatinum(II)] are often explained by the ability of oxaliplatin to form DNA adducts of different conformation and consequently to exhibit different cytotoxic effects. This work describes, for the first time, the structural and biochemical characteristics of the interstrand cross-links of oxaliplatin. We find that: 1) DNA bending, unwinding, thermal destabilization, and delocalization of the conformational alteration induced by the cross-link of oxaliplatin are greater than those observed with the cross-link of cisplatin; 2) the affinity of high-mobility-group proteins (which are known to mediate the antitumor activity of platinum complexes) for the interstrand cross-links of oxaliplatin is markedly lower than for those of cisplatin; and 3) the chirality at the carrier 1,2-diaminocyclohexane ligand can affect some important structural properties of the interstrand cross-links of cisplatin analogues. Thus, the information contained in the present work is also useful for a better understanding of how the stereochemistry of the carrier amine ligands of cisplatin analogues can modulate their anticancer and mutagenic properties. The significance of this study is also reinforced by the fact that, in general, interstrand cross-links formed by various compounds of biological significance result in greater cytotoxicity than is expected for monofunctional adducts or other intrastrand DNA lesions. Therefore, we suggest that the unique properties of the interstrand cross-links of oxaliplatin are at least partly responsible for this drug's unique antitumor effects.

Published

2008

161. Low-power laser irradiation inhibiting Abeta25-35-induced PC12 cell apoptosis via PKC activation.

Author

Zhang L, Xing D, Zhu D, and Chen Q

Subjects

Animals, Apoptosis radiation effects, Bisbenzimidazole, Cell Proliferation drug effects, Cell Proliferation radiation effects, Cell Survival drug effects, Cell Survival radiation effects, Enzyme Activation drug effects, Enzyme Activation radiation effects, Gene Expression Regulation drug effects, Gene Expression Regulation radiation effects, Models, Biological, Nucleic Acid Denaturation drug effects, Nucleic Acid Denaturation radiation effects, PC12 Cells, Protein Kinase C antagonists & inhibitors, Protein Kinase Inhibitors pharmacology, RNA, Messenger genetics, RNA, Messenger metabolism, Rats, bcl-2-Associated X Protein genetics, bcl-2-Associated X Protein metabolism, bcl-X Protein genetics, bcl-X Protein metabolism, Amyloid beta-Peptides pharmacology, Apoptosis drug effects, Low-Level Light Therapy, Peptide Fragments pharmacology, Protein Kinase C metabolism

Abstract

Apoptosis is a contributing pathophysiological mechanism of Alzheimer's disease (AD). Recently, low-power laser irradiation (LPLI) has been applied to moderate AD, but the underlying mechanism remains unknown. In this study, the techniques of fluorescence resonance energy transfer (FRET) and real-time quantitative RT-PCR were used to investigate the anti-apoptotic mechanism of LPLI. Rat pheochromocytoma (PC12) cells were treated with amyloid beta 25-35 (Abeta(25-35)) for induction of apoptosis before LPLI treatment. The cell viability assays and morphological examinations show that low fluence of LPLI (0.156 J/cm(2)-0.624 J/cm(2)) could inhibit the cells apoptosis. An increase of PKC activation was dynamically monitored in the cells treated with PMA (specific activator of PKC), LPLI only or Abeta(25-35) followed by 5 min LPLI treatment, respectively. However, the effect of LPLI activating PKC could be inhibited by Go 6983 (specific inhibitor of PKC). Similar results were obtained by using Western blot analysis. Furthermore, LPLI involved an increase in mRNA of the cell survival member bcl-xl and a decrease in the up-regulation of cell death member bax mRNA caused by Abeta(25-35). Further data show that low fluence of LPLI could reverse the increased level of bax/bcl-xl mRNA ratio caused by Abeta(25-35) treatment. In addition, Go 6983 could inhibit the decreased level of bax/bcl-xl mRNA ratio. Taken together, these data clearly indicate that LPLI inhibited Abeta(25-35)-induced PC12 cell apoptosis via PKC-mediated regulation of bax/bcl-xl mRNA ratio., (Copyright 2008 S. Karger AG, Basel.)

Published

2008

162. 1,2,4-benzothiadiazine linked pyrrolo[2,1-c][1,4]benzodiazepine conjugates: synthesis, DNA-binding affinity and cytotoxicity.

Author

Kamal A, Khan MN, Reddy KS, Ahmed SK, Kumar MS, Juvekar A, Sen S, and Zingde S

Subjects

Animals, Antineoplastic Agents pharmacology, Benzodiazepines pharmacology, Benzothiadiazines pharmacology, Breast Neoplasms drug therapy, Breast Neoplasms pathology, Cattle, Cell Line, Tumor, DNA Restriction Enzymes chemistry, Drug Screening Assays, Antitumor, Female, Humans, Indicators and Reagents, Male, Nucleic Acid Denaturation drug effects, Prostatic Neoplasms drug therapy, Prostatic Neoplasms pathology, Structure-Activity Relationship, Antineoplastic Agents chemical synthesis, Antineoplastic Agents metabolism, Benzodiazepines chemical synthesis, Benzodiazepines metabolism, Benzothiadiazines chemical synthesis, Benzothiadiazines metabolism, DNA metabolism

Abstract

Benzothiadiazine-pyrrolobenzodiazepine conjugates linked through different alkane spacers have been prepared. These new classes of hybrid molecules exhibit cytotoxicity against many cancer cell lines. Their DNA thermal denaturation studies have been carried out and one of the compounds (4b) elevates the DNA helix melting temperature of the CT-DNA by 6.7 degrees C after incubation for 36 h.

Published

2007

163. Enzymatic synthesis of DNA on glycerol nucleic acid templates without stable duplex formation between product and template.

Author

Tsai CH, Chen J, and Szostak JW

Subjects

Base Pairing, Base Sequence, Buffers, Catalysis, Cations, Divalent chemistry, Circular Dichroism, Hot Temperature, Hydrogen-Ion Concentration, Kinetics, Manganese chemistry, Mass Spectrometry, Molecular Sequence Data, Molecular Structure, Nucleic Acid Denaturation drug effects, Nucleic Acids chemical synthesis, Oligonucleotides chemical synthesis, Oligonucleotides pharmacology, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Templates, Genetic, DNA biosynthesis, DNA-Directed DNA Polymerase metabolism, Glycerol chemistry, Nucleic Acids chemistry

Abstract

Glycerol nucleic acid (GNA) is an interesting alternative base-pairing system based on an acyclic, glycerol-phosphate backbone repeat unit. The question of whether DNA polymerases can catalyze efficient template-dependent synthesis using GNA as the template is of particular interest because GNA is unable to form a stable duplex with DNA. In the present study, we screened a variety of DNA polymerases for GNA-dependent DNA synthesis. We find that Bst DNA polymerase can catalyze full-length DNA synthesis on a dodecamer GNA template. The efficiency of DNA synthesis is increased by replacing adenine with diaminopurine in both the GNA template and the DNA monomers and by the presence of manganese ions. We suggest that the BstDNA polymerase maintains a short, transient region of base-pairing between the DNA product strand and the GNA template, but that stable duplex formation between product and template strands is not required for template-dependent polymerization.

Published

2007

164. On the origin of the decrease in stability of the DNA hairpin d(GCGAAGC) on complexation with aromatic drugs.

Author

Kostjukov VV, Lantushenko AO, Davies DB, and Evstigneev MP

Subjects

Base Sequence, Binding Sites, Daunorubicin pharmacology, Ethidium pharmacology, Hot Temperature, Hydrocarbons, Aromatic chemistry, Hydrocarbons, Aromatic pharmacology, Mitoxantrone pharmacology, Nucleic Acid Conformation drug effects, Proflavine pharmacology, Thermodynamics, Water chemistry, DNA chemistry, Nucleic Acid Denaturation drug effects, Pharmaceutical Preparations chemistry

Abstract

Molecular dynamics simulations of drug-DNA complexes have been carried out in order to explain the experimentally observed decrease in thermal stability of the DNA hairpin d(GCGAAGC) on binding the aromatic drug molecules, daunomycin, ethidium bromide, novantrone and proflavine. This complexation behavior is in contrast to the stabilizing effect of the same aromatic drug molecules on DNA duplexes. Analysis of the energy parameters and the hydration properties of the complexes shows that the main factor correlating with the decrease in melting temperatures of the drug-hairpin complexes is the number of water bridges, with a reduction of at least 40% on ligand binding.

Published

2007

165. Effects of the chemotherapeutic agents for non-Hodgkin lymphoma, cyclophosphamide, doxorubicin, vincristine, and prednisone (CHOP), on the male rat reproductive system and progeny outcome.

Author

Vaisheva F, Delbes G, Hales BF, and Robaire B

Subjects

Animals, Antineoplastic Combined Chemotherapy Protocols administration & dosage, Apoptosis drug effects, Cyclophosphamide administration & dosage, Doxorubicin administration & dosage, Female, Humans, In Situ Nick-End Labeling, Lymphoma, Non-Hodgkin drug therapy, Male, Nucleic Acid Denaturation drug effects, Prednisone administration & dosage, Pregnancy, Pregnancy Outcome, Rats, Rats, Sprague-Dawley, Testis drug effects, Testosterone blood, Vincristine administration & dosage, Antineoplastic Combined Chemotherapy Protocols pharmacology, Cyclophosphamide pharmacology, Doxorubicin pharmacology, Testis pathology, Vincristine pharmacology

Abstract

Chemotherapy of non-Hodgkin lymphoma (NHL) with cyclophosphamide, doxorubicin, vincristine, and prednisone (CHOP) is associated with significant gonadal damage. Our goal was to determine the impact of CHOP chemotherapy on the male reproductive system, fertility, and progeny outcome in the rat model. Adult male Sprague-Dawley rats received saline or CHOP, 4 cycles of 3 weeks each, at doses analogous to 1/3x, 2/3x, or 1x the human dose; males were mated to evaluate effects on progeny outcome. Reproductive organ weights were significantly decreased in the 1x CHOP-exposed group. The spermatozoal contents of the testes and epididymides were decreased in 1x CHOP-treated males; the 1/3x and 2/3x doses also affected testicular sperm contents. Seminiferous tubule diameters were decreased by 20% in 1x CHOP-treated males. Damage ranged from the presence of small vacuoles in the epithelium to tubules deprived of spermatocytes and spermatids and was accompanied by an increased incidence of germ cell apoptosis. The acridine orange assay revealed a significant increase in sperm with abnormal DNA integrity profiles in the 1x CHOP group. Despite effects on germ cell number and quality, CHOP-exposed rats remained fertile. However, a 50% decrease in live fetuses was observed in litters sired by 1x CHOP-treated males due to a significant increase in both pre-implantation and postimplantation losses; postimplantation loss was also elevated among litters sired by 2/3x CHOP-treated males. Thus, CHOP treatment affected both the quantity and quality of male germ cells; conceptal loss is a sensitive measure of the integrity of the male genome.

Published

2007

166. Effect of lactose and glycerol on the motility, normal apical ridge, chromatin condensation and chromatin stability of frozen boar spermatozoa.

Author

Corcuera BD, Marigorta P, Sagüés A, Saiz-Cidoncha F, and Pérez-Gutiérrez JF

Subjects

Animals, Male, Nucleic Acid Denaturation drug effects, Osmolar Concentration, Spermatozoa cytology, Chromatin Assembly and Disassembly drug effects, Cryopreservation methods, Glycerol pharmacology, Lactose pharmacology, Sperm Motility drug effects, Spermatozoa drug effects, Sus scrofa

Abstract

The effect of lactose and glycerol concentration, as well as the equilibration time with glycerol was studied on motility, normal apical ridge (NAR), and chromatin state of boar spermatozoa after the freezing and thawing process. In the first experiment, samples were frozen in first and second extenders containing different concentrations of lactose (11, 12 and 14%). In the second experiment samples were frozen using second extenders with different concentrations of glycerol (4, 6, 8 and 10%) and were incubated at 5 degrees C for 0 and 30 min. Motility, motility after caffeine treatment, NAR, chromatin condensation and stability (susceptibility to de-condense after heparin treatment) were evaluated. The results indicated that freezing spermatozoa in extenders with increasing concentrations of lactose adversely affected motility but provided a protective effect on acrosomes. Increased lactose concentration induced higher chromatin condensation but maintained the same stability. Increasing the glycerol concentration in the second extender from 4-6 to 8% led to higher motility and NAR as well as lower chromatin condensation and stability. When 30 min equilibration time was allowed after dilution with the same extenders, spermatozoa showed higher NAR and lower chromatin condensation and stability. The longer equilibration time was detrimental for motility when freezing in the 8% glycerol extender but favourable when using the 4% glycerol extender. Compared to the 8% glycerol, spermatozoa frozen in the 10% glycerol extender showed similar motility and increased chromatin condensation and stability, as well as low values of NAR that did not improve by longer incubation time.

Published

2007

167. Effects of the chemotherapy cocktail used to treat testicular cancer on sperm chromatin integrity.

Author

Delbes G, Hales BF, and Robaire B

Subjects

Animals, Antineoplastic Combined Chemotherapy Protocols administration & dosage, Bleomycin administration & dosage, Bleomycin pharmacology, Cisplatin administration & dosage, Cisplatin pharmacology, Comet Assay, DNA Damage drug effects, DNA Fragmentation drug effects, Etoposide administration & dosage, Etoposide pharmacology, Hydrogen-Ion Concentration, In Situ Nick-End Labeling, Male, Nucleic Acid Denaturation drug effects, Rats, Rats, Sprague-Dawley, Sperm Motility drug effects, Spermatozoa ultrastructure, Antineoplastic Combined Chemotherapy Protocols pharmacology, Chromatin drug effects, Spermatozoa drug effects, Testicular Neoplasms drug therapy

Abstract

The incidence of testicular cancer has increased dramatically over the past 50 years. Advances in treatment, which include the coadministration of bleomycin, etoposide, and cis-platinum (BEP), have brought the cure rate to over 90%. After treatment, most patients go through a temporary period of azoo/oligozoospermia. Although the sperm concentration in approximately 80% of the patients returns to at least 10 million/mL, little is known about the integrity of the chromatin of their germ cells. Using an animal model, we assessed DNA integrity in the spermatozoa of male rats treated for 3, 6 or 9 weeks with BEP at doses, adjusted for surface area, equivalent to 0X, 1/3X, 2/3X, or 1X of the human dose. We did not observe any difference in protamination content, as assessed by the chromomycin A3 (CMA3) assay. After 9 weeks of 1X treatment, the susceptibility of DNA to denaturation evaluated by the sperm chromatin structure assay (SCSA/acridine orange assay (AO) was increased, as well as the number of single and double DNA strand breaks measured by the TUNEL and COMET assays. Parameters obtained from the AO and TUNEL assays were highly correlated with the motility of the spermatozoa, suggesting that conventional sperm analysis parameters can serve as a good indicator of chromatin integrity and vice versa. Correlation studies also suggested that the parameters obtained with the different assays do not overlap, but complement each other. Thus, BEP treatment altered spermatozoal chromatin quality, and these alterations may impact adversely on progeny outcome.

Published

2007

168. Bending and unwinding of nucleic acid by prion protein.

Author

Bera A, Roche AC, and Nandi PK

Subjects

DNA-Binding Proteins, Fluorescence Resonance Energy Transfer, Hot Temperature, Humans, Nucleic Acid Conformation drug effects, Nucleic Acid Denaturation drug effects, Oligonucleotides metabolism, Peptide Fragments metabolism, Prions metabolism, Prions pharmacology, Oligonucleotides chemistry, Prions chemistry

Abstract

Nucleic acid induces conformational changes in the prion protein (23-231 amino acids) to a structure resembling its pathological isoform. The prion protein, in turn, facilitates DNA strand transfer and acts as a DNA chaperone which is modulated by the N-terminal unstructured basic segment of the protein. Here we have studied the prion protein induced conformational changes in DNA using oligonucleotides covalently labeled with the energy donor fluorescein and the acceptor rhodamine moieties by fluorescence resonance energy transfer (FRET) and by thermal stability of the unlabeled oligonucleotides. The protein induces a strong FRET effect in the oligonucleotides evidenced from the simultaneous quenching of fluorescence intensity of the donor and increase in the fluorescence intensity of the acceptor, which indicate bending of the oligonucleotides by the prion protein. The energy transfer efficiency induced by the protein is greater for the larger oligonucleotide. The prion protein also induces significant structural destabilization of the oligonucleotides observed from the lowering of their melting temperatures in the presence of the protein. The truncated globular prion protein 121-231 fragment neither induces FRET effect on the oligonucleotides nor destabilizes their structures, indicating that the N-terminal segment of the prion protein is essential for the DNA bending process. Equilibrium binding and kinetics of FRET show that the protein binding to the oligonucleotides and their bending occur simultaneously. The DNA structural changes observed in the presence of the prion protein are similar to those caused by proteins involved in initiation and regulation for protein synthesis.

Published

2007

169. Structural transitions and thermodynamics of a glycine-dependent riboswitch from Vibrio cholerae.

Author

Lipfert J, Das R, Chu VB, Kudaravalli M, Boyd N, Herschlag D, and Doniach S

Subjects

Aptamers, Nucleotide genetics, Base Sequence, Hydroxyl Radical metabolism, Magnesium pharmacology, Models, Molecular, Molecular Sequence Data, Nucleic Acid Conformation drug effects, Nucleic Acid Denaturation drug effects, RNA, Bacterial genetics, Scattering, Small Angle, Solvents, Thermodynamics, X-Ray Diffraction, Aptamers, Nucleotide chemistry, Glycine metabolism, RNA, Bacterial chemistry, Vibrio cholerae chemistry

Abstract

Riboswitches are complex folded RNA domains found in noncoding regions of mRNA that regulate gene expression upon small molecule binding. Recently, Breaker and coworkers reported a tandem aptamer riboswitch (VCI-II) that binds glycine cooperatively. Here, we use hydroxyl radical footprinting and small-angle X-ray scattering (SAXS) to study the conformations of this tandem aptamer as a function of Mg(2+) and glycine concentration. We fit a simple three-state thermodynamic model that describes the energetic coupling between magnesium-induced folding and glycine binding. Furthermore, we characterize the structural conformations of each of the three states: In low salt with no magnesium present, the VCI-II construct has an extended overall conformation, presumably representing unfolded structures. Addition of millimolar concentrations of Mg(2+) in the absence of glycine leads to a significant compaction and partial folding as judged by hydroxyl radical protections. In the presence of millimolar Mg(2+) concentrations, the tandem aptamer binds glycine cooperatively. The glycine binding transition involves a further compaction, additional tertiary packing interactions and further uptake of magnesium ions relative to the state in high Mg(2+) but no glycine. Employing density reconstruction algorithms, we obtain low resolution 3-D structures for all three states from the SAXS measurements. These data provide a first glimpse into the structural conformations of the VCI-II aptamer, establish rigorous constraints for further modeling, and provide a framework for future mechanistic studies.

Published

2007

170. Involvement of DEAD-box proteins in group I and group II intron splicing. Biochemical characterization of Mss116p, ATP hydrolysis-dependent and -independent mechanisms, and general RNA chaperone activity.

Author

Halls C, Mohr S, Del Campo M, Yang Q, Jankowsky E, and Lambowitz AM

Subjects

Animals, DEAD-box RNA Helicases isolation & purification, Hydrolysis drug effects, Introns drug effects, Magnesium pharmacology, Mitochondria drug effects, Mitochondria metabolism, Neurospora crassa, Nucleic Acid Denaturation drug effects, Open Reading Frames drug effects, Open Reading Frames genetics, Protein Binding drug effects, RNA Splicing drug effects, RNA, Catalytic metabolism, RNA-Binding Proteins metabolism, Saccharomyces cerevisiae, Saccharomyces cerevisiae Proteins isolation & purification, Substrate Specificity drug effects, Tetrahymena thermophila, Adenosine Triphosphate metabolism, DEAD-box RNA Helicases metabolism, Introns genetics, Molecular Chaperones metabolism, RNA Splicing genetics, RNA, Fungal metabolism, Saccharomyces cerevisiae Proteins metabolism

Abstract

The RNA-catalyzed splicing of group I and group II introns is facilitated by proteins that stabilize the active RNA structure or act as RNA chaperones to disrupt stable inactive structures that are kinetic traps in RNA folding. In Neurospora crassa and Saccharomyces cerevisiae, the latter function is fulfilled by specific DEAD-box proteins, denoted CYT-19 and Mss116p, respectively. Previous studies showed that purified CYT-19 stimulates the in vitro splicing of structurally diverse group I and group II introns, and uses the energy of ATP binding or hydrolysis to resolve kinetic traps. Here, we purified Mss116p and show that it has RNA-dependent ATPase activity, unwinds RNA duplexes in a non-polar fashion, and promotes ATP-independent strand-annealing. Further, we show that Mss116p binds RNA non-specifically and promotes in vitro splicing of both group I and group II intron RNAs, as well as RNA cleavage by the aI5gamma-derived D135 ribozyme. However, Mss116p also has ATP hydrolysis-independent effects on some of these reactions, which are not shared by CYT-19 and may reflect differences in its RNA-binding properties. We also show that a non-mitochondrial DEAD-box protein, yeast Ded1p, can function almost as efficiently as CYT-19 and Mss116p in splicing the yeast aI5gamma group II intron and less efficiently in splicing the bI1 group II intron. Together, our results show that Mss116p, like CYT-19, can act broadly as an RNA chaperone to stimulate the splicing of diverse group I and group II introns, and that Ded1p also has an RNA chaperone activity that can be assayed by its effect on splicing mitochondrial introns. Nevertheless, these DEAD-box protein RNA chaperones are not completely interchangeable and appear to function in somewhat different ways, using biochemical activities that have likely been tuned by coevolution to function optimally on specific RNA substrates.

Published

2007

171. More pronounced salt dependence and higher reactivity for platination of the hairpin r(CGCGUUGUUCGCG) compared with d(CGCGTTGTTCGCG).

Author

Hägerlöf M, Papsai P, Chow CS, and Elmroth SK

Subjects

Base Sequence, Binding Sites, Circular Dichroism, Kinetics, Nucleic Acid Conformation drug effects, Nucleic Acid Denaturation drug effects, Platinum Compounds pharmacology, Salts pharmacology, Temperature, Oligodeoxyribonucleotides chemistry, Oligoribonucleotides chemistry, Platinum Compounds chemistry

Abstract

The DNA interference pathways exhibited by cisplatin and related anticancer active metal complexes have been extensively studied. Much less is known to what extent RNA interaction pathways may operate in parallel, and perhaps contribute to both antineoplastic activity and toxicity. The present study was designed with the aim of comparing the reactivity of two model systems comprising RNA and DNA hairpins, r(CGCGUUGUUCGCG) and d(CGCGTTGTTCGCG), towards a series of platinum(II) complexes. Three platinum complexes were used as metallation reagents; cis-[PtCl(NH3)2(OH2)]+ (1), cis-[PtCl(NH3)(c-C6H11NH2)(OH2)]+ (2), and trans-[PtCl(NH3)(quinoline)(OH2)]+ (3). The reaction kinetics were studied at pH 6.0, 25 degrees C, and 1.0 mM < or = I < or = 500 mM. For both types of nucleic acid targets, compound 3 was found to react about 1 order of magnitude more rapidly than compounds 1 and 2. Further, all platinum compounds exhibited a more pronounced salt dependence for the interaction with r(CGCGUUGUUCGCG). Chemical and enzymatic cleavage studies revealed similar interaction patterns with r(CGCGUUGUUCGCG) after long exposure times to 1 and 2. A substantial decrease of cleavage intensity was found at residues G4 and G7, indicative of bifunctional adduct formation. Circular dichroism studies showed that platinum adduct formation leads to a structural change of the ribonucleic acid. Thermal denaturation studies revealed platination to cause a decrease of the RNA melting temperatures by 5-10 degrees C. Our observations therefore suggest that RNA is a kinetically competitive target to DNA. Furthermore, platination causes destabilization of RNA structural elements, which may lead to deleterious intracellular effects on biologically relevant RNA targets.

Published

2006

172. Dramatic selectivity differences in the association of DNA and RNA models with new ethylene- and propylene diamine derivatives and their copper complexes.

Author

Lomadze N, Schneider HJ, Albelda MT, García-España E, and Verdejo B

Subjects

Binding Sites, DNA metabolism, Diamines pharmacology, Intercalating Agents, Models, Molecular, Nucleic Acid Denaturation drug effects, Poly A-U chemistry, Poly A-U metabolism, Poly dA-dT chemistry, Poly dA-dT metabolism, RNA metabolism, Copper pharmacology, DNA chemistry, Diamines chemistry, RNA chemistry

Abstract

The affinities of polyamines consisting of ethylenediamine units equipped with either one or two terminal naphthyl-, anthryl-, or acridyl units towards PolyA.PolyU as an RNA model, and Poly(dA).Poly(dT) as a DNA model are screened by measuring the melting point changes (DeltaT(m)) of the double strands, and also partially by a fluorimetric binding assay using ethidium bromide. The larger aromatic moieties with long spacers between them allow bisintercalation; this leads to an increased preference for DNA in comparison to RNA, where ion pairing of the ammonium centers with the major RNA groove phosphates dominates. Allosteric affinity control by metalation is achieved e.g. with Cu(2+) ions, which induce conformational distortions within the chains. With anthryl- in contrast to naphthyl derivatives intercalation can be so strong that distortion of the ethylenediamine chain by metalation is not powerful enough. A particularly high concentration of positive charges is accessible with tripodal derivatives built up from ethylenediamine and propylenediamine units; in the absence of aryl parts, which interfere with the RNA groove preference, one observes the highest affinity difference known until today, reflected in a melting point ratio of DeltaT(m(RNA))/DeltaT(m(DNA)) = 40, whereas other synthetic ligands reach only a DeltaT(m(RNA))/DeltaT(m(DNA)) ratio of about 3.

Published

2006

173. [Effect of alkaloids from celandine on calcium accumulation and oxidative phosphorylation in mitochondria depending on their DNA intercalating properties].

Author

Kamins'kyĭ VO, Kryv'iak NV, Lutsyk MD, and Stoĭka RS

Subjects

Alkaloids isolation & purification, Animals, In Vitro Techniques, Intercalating Agents isolation & purification, Mitochondria, Liver metabolism, Nucleic Acid Denaturation drug effects, Oxidative Phosphorylation drug effects, Rats, Alkaloids pharmacology, Calcium metabolism, Chelidonium chemistry, DNA, Mitochondrial metabolism, Intercalating Agents pharmacology, Mitochondria, Liver drug effects

Abstract

The effect of principal alkaloids (sanguinarine, chelerythrine, coptisine, chelidonine) of greater celandine Chelidonium majus L., as well as the alkaloids from Colchicum autumnale L. (colchicine and colchamine) on calcium accumulation and oxidative phosphorylation in rat liver mitochondria has been studied. The obtained data were compared with DNA intercalating properties of alkaloids detected by the method of thermodenaturation (DNA melting curve plots). It was found that chelerythrine and sanguinarine blocked absorption and accumulation of calcium cations and inhibited oxidative phosphorylation, while the coptisine significantly diminished those indices. Chelidonine, colchicines and colchamine had no influence on the studied characteristics. The effect of alkaloids upon mitochondria functional state correlated tightly with their DNA intercalating properties: chelerythrine and sanguinarine were strong intercalators, while coptisine was a weak one, and chelidonine, colchicine and colchamine did not interact with DNA and caused no changes in its melting point. Correlation coefficient between the intercalating properties of alkaloids and their inhibition of calcium accumulation was 0.89, and with their oxidative phosphorylation inhibition - 0.93. It is suggested that the effect of studied alkaloids upon functional properties of mitochondria can be mediated by mtDNA.

Published

2006

174. A new approach to DNA bending by polyamines and its implication in DNA condensation.

Author

Pastré D, Piétrement O, Landousy F, Hamon L, Sorel I, David MO, Delain E, Zozime A, and Le Cam E

Subjects

Binding Sites, Bleomycin chemistry, DNA drug effects, DNA, Viral, Electrochemistry, Entropy, Microscopy, Atomic Force methods, Solutions, Spermidine chemistry, DNA chemistry, Models, Chemical, Models, Molecular, Nucleic Acid Conformation drug effects, Nucleic Acid Denaturation drug effects, Polyamines chemistry

Abstract

Polyamines are known to induce dynamical bending of DNA molecules. This mechanism is very important since many DNA binding proteins (DNAse, transcription factor, etc.) exert their action by their ability to bend DNA. We propose an analytical model which describes the dynamical bending of DNA by polyamine ions in highly diluted DNA solutions. The bending probability depends on the entropy loss of polyamines due to their localization. This localization is facilitated by the electrostatic repulsion between multivalent counterions condensed on DNA, which reduces the entropy loss in counterion localization. Therefore DNA bending by polyamines depends on the competition between monovalent counterions and polyamines. We find that the bending probability is weak for a low binding ratio of polyamines (i.e. number of bound polyamines per base pair), whereas a high bending probability can be reached at large polyamine binding ratio. In addition, we describe a new mechanism of DNA bending. It occurs with the help of thermal agitation, which initiates the bending and favours the polyamine localization. This model provides further insights into DNA bending by polyamines and its implication in DNA condensation. A qualitative estimation of the DNA bending probability is obtained by measuring the cleavage efficiency of DNA by bleomycin versus spermidine concentration. Indeed, a local helix distortion by polyamines results in an amplification of the double-strand cleavage by bleomycin. The measurement of the bleomycin amplification is performed by analysing images of DNA molecules with atomic force microscope. Some features of the dynamical bending indicate that condensation and bending are interrelated.

Published

2006

175. DNA and non-DNA targets in the mechanism of action of the antitumor drug trabectedin.

Author

David-Cordonnier MH, Gajate C, Olmea O, Laine W, de la Iglesia-Vicente J, Perez C, Cuevas C, Otero G, Manzanares I, Bailly C, and Mollinedo F

Subjects

Antineoplastic Agents chemistry, Base Sequence, Caspase 3, Caspases metabolism, Cell Cycle drug effects, Cell Line, Tumor, DNA chemistry, DNA genetics, Dioxoles chemistry, Enzyme Activation drug effects, Gene Expression Regulation, Neoplastic, Humans, Isoquinolines chemistry, JNK Mitogen-Activated Protein Kinases metabolism, Molecular Structure, Nucleic Acid Denaturation drug effects, Substrate Specificity, Temperature, Tetrahydroisoquinolines, Trabectedin, Antineoplastic Agents metabolism, Antineoplastic Agents pharmacology, DNA metabolism, Dioxoles metabolism, Dioxoles pharmacology, Isoquinolines metabolism, Isoquinolines pharmacology

Abstract

We have analyzed the DNA binding properties of the antitumor agent trabectedin (ET-743, Yondelis) and different analogs, namely, ET-745, lacking the C21-hydroxyl group, and ET-637, ET-594, ET-637-OBu, with modifications at the trabectedin C domain, versus their effects on cell cycle, apoptosis, and gene expression. ET-745 failed to bind DNA, highlighting the importance of the C21-hydroxyl group for DNA binding. Analogs ranked trabectedin >> ET-637 approximately ET-594 > ET-637-OBu >> ET-745 for their DNA binding capacity; ET-637 and ET-594 display very different biological activities. Drugs were clustered in three major groups showing high (trabectedin, ET-637), intermediate (ET-637-OBu), and low (ET-594, ET-745) cytotoxic activity and similar transcriptional profiling responses. C21-hydroxyl-deficient analogs of the above-mentioned compounds showed a dramatic decrease in biological activity. Our data suggest that trabectedin interacts with an additional non-DNA target to raise an effective antitumor response, and that this interaction is favored through trabectedin-DNA complexes.

Published

2005

176. [Effect of toluene on stability of chromatin of white rat hippocampus and olfactory bulb in vivo. Microcalorimetric study].

Author

Monaselidze D, Kiladze M, Barbakadze Sh, Kvavadze R, Chkhaidze M, Gelazonia L, and Svanidze I

Subjects

Animals, Calorimetry, Differential Scanning, Hypothalamus drug effects, Nucleic Acid Denaturation drug effects, Olfactory Bulb drug effects, Rats, Solvents administration & dosage, Toluene administration & dosage, Chromatin chemistry, DNA chemistry, Hypothalamus chemistry, Olfactory Bulb chemistry, Solvents toxicity, Toluene toxicity

Abstract

The denaturation heat parameters of hippocampus and olfactory bulb nodulus tissues were determined. The total denaturation heat calculated from the areas of endotherms I-IX onto which the dependence deltaH = f(T) is factorized equals to 13.03 +/- 1.3 J/g for bulb nodules and 9.91 J/g for the hippocampus. It was shown that chromatin in the composition of tissues had two stages of denaturation with the following parameters: for bulb nodules: Td(VIII) = 99.4 degrees C, Qd(VIII) = 62.3 +/- 0.8 J/g DNA, Td = (IX) = 106 degrees C, Qd = 28.8 ; 0.4 J/g DNA; and for hippocampus: Td(VIII) = 95 degrees C; Qd(VIII) = 62.0 +/- 9 J/g. Td(IX) - 107 degrees C; Qd(IX) = 29.0 +/- 4.5 J/g DNA. It was established that, along with denaturation of cytoplasmatic structures, nonhistone, nuclear proteins and damage to the nuclear matrix, toluene caused the redistribution of heat between endotherms IX, VIII, VIII(I) connected with the infolding of chromatin loops and 30-nm fibers. It is supposed that toluene causes the damage to the genetic material due to not only its oxidative influence on chromatin DNA but also the disturbance of nuclear matrix structural organization and partial denaturation of nuclear proteins of non-histone origin.

Published

2005

177. The global regulator H-NS acts directly on the transpososome to promote Tn10 transposition.

Author

Wardle SJ, O'Carroll M, Derbyshire KM, and Haniford DB

Subjects

Bacterial Proteins genetics, Base Pairing, Base Sequence, Binding Sites, Calcium Chloride pharmacology, DNA Footprinting, DNA, Bacterial chemistry, DNA, Bacterial genetics, DNA, Bacterial metabolism, DNA-Binding Proteins genetics, Electrophoretic Mobility Shift Assay, Escherichia coli Proteins genetics, Escherichia coli Proteins metabolism, Heparin pharmacology, Integration Host Factors genetics, Integration Host Factors metabolism, Kinetics, Models, Genetic, Mutation, Nucleic Acid Conformation, Nucleic Acid Denaturation drug effects, Protein Binding, Transposases genetics, Bacterial Proteins metabolism, DNA Transposable Elements, DNA-Binding Proteins metabolism, Transposases metabolism

Abstract

The histone-like nucleoid structuring (H-NS) protein is a global transcriptional regulator that is known to regulate stress response pathways and virulence genes in bacteria. It has also been implicated in the regulation of bacterial transposition systems, including Tn10. We demonstrate here that H-NS promotes Tn10 transposition by binding directly to the transposition complex (or transpososome). We present evidence that, upon binding, H-NS induces the unfolding of the Tn10 transpososome and helps to maintain the transpososome in an unfolded state. This ensures that intermolecular (as opposed to self-destructive intramolecular) transposition events are favored. We present evidence that H-NS binding to the flanking donor DNA of the transpososome is the initiating event in the unfolding process. We propose that by recruiting H-NS as a modulator of transposition, Tn10 has evolved a means of sensing changes in host physiology, as the amount of H-NS in the cell, as well its activity, are responsive to changes in environmental conditions. Sensing of environmental changes through H-NS would allow transposition to occur when it is most opportune for both the transposon and the host.

Published

2005

178. Comparison of SYTO9 and SYBR Green I for real-time polymerase chain reaction and investigation of the effect of dye concentration on amplification and DNA melting curve analysis.

Author

Monis PT, Giglio S, and Saint CP

Subjects

Benzothiazoles, DNA genetics, Diamines, Fluorescent Dyes analysis, Fluorescent Dyes pharmacology, Legionella genetics, Nucleic Acid Denaturation drug effects, Organic Chemicals analysis, Quinolines, Reproducibility of Results, Vibrio genetics, Base Pairing, DNA biosynthesis, DNA chemistry, Organic Chemicals pharmacology, Polymerase Chain Reaction instrumentation, Polymerase Chain Reaction methods

Abstract

Following the initial report of the use of SYBR Green I for real-time polymerase chain reaction (PCR) in 1997, little attention has been given to the development of alternative intercalating dyes for this application. This is surprising considering the reported limitations of SYBR Green I, which include limited dye stability, dye-dependent PCR inhibition, and selective detection of amplicons during DNA melting curve analysis of multiplex PCRs. We have tested an alternative to SYBR Green I and report the first detailed evaluation of the intercalating dye SYTO9. Our findings demonstrate that SYTO9 produces highly reproducible DNA melting curves over a broader range of dye concentrations than does SYBR Green I, is far less inhibitory to PCR than SYBR Green I, and does not appear to selectively detect particular amplicons. The low inhibition and high melting curve reproducibility of SYTO9 means that it can be readily incorporated into a conventional PCR at a broad range of concentrations, allowing closed tube analysis by DNA melting curve analysis. These features simplify the use of intercalating dyes in real-time PCR and the improved reproducibility of DNA melting curve analysis will make SYTO9 useful in a diagnostic context.

Published

2005

179. Anions or cations: who is in charge of inhibiting the nickel(II) promoted B- to Z-DNA transition?

Author

Spingler B

Subjects

Anions, Borohydrides pharmacology, Cations, Lithium Chloride pharmacology, Magnesium Chloride pharmacology, Methylamines chemistry, Nucleic Acid Conformation drug effects, Nucleic Acid Denaturation drug effects, Sodium Chloride pharmacology, Sodium Fluoride pharmacology, DNA chemistry, DNA, Z-Form chemistry, Nickel chemistry, Polydeoxyribonucleotides chemistry

Abstract

Various weakly binding cations and anions were studied at a concentration of 10 mM to ascertain their interaction with the nickel(II) promoted B- to Z-DNA transition of poly d(GC). These salts were ranked according to the decreasing amounts of nickel needed for the B- to Z-DNA transition and provided the following order: NaCl approximately Me4NCl > LiCl >> MgCl2 > no salt > NaBF4 approximately NaNO3 approximately NaClO4. Remarkably, it was found that going from sodium nitrate to sodium chloride increased the necessary amount of nickel to induce the transition to the left-handed helix of poly d(GC) by a factor of 10. This dramatic effect cannot be explained by the binding constant of nickel(II) to chloride to form the monocationic complex. We believe that this is the first reported example of the role of chloride anions, which appear to modulate the interaction of nickel(II) ions with the polyanionic DNA.

Published

2005

180. New triple-helix DNA stabilizing agents.

Author

Strekowski L, Hojjat M, Wolinska E, Parker AN, Paliakov E, Gorecki T, Tanious FA, and Wilson WD

Subjects

Drug Design, Ligands, Nucleic Acid Conformation drug effects, Nucleic Acid Denaturation drug effects, Polydeoxyribonucleotides chemistry, Quinolines pharmacology, Structure-Activity Relationship, Temperature, DNA chemistry, Quinolines chemical synthesis

Abstract

Several substituted quinolin-4-amines and heteroaromatic analogs were synthesized and evaluated for interaction with triplex polydA.2polydT and duplex polydA.polydT by using UV-thermal melting experiments. Excellent triple-helix DNA ligands with high affinity toward T.A.T triplets and triple/duplex selectivity were designed through a rational approach.

Published

2005

181. Effects of fluorescent dyes, quenchers, and dangling ends on DNA duplex stability.

Author

Moreira BG, You Y, Behlke MA, and Owczarzy R

Subjects

Base Sequence, DNA genetics, DNA metabolism, Fluorescent Dyes chemistry, Nucleic Acid Denaturation drug effects, Spectrum Analysis, Temperature, Thermodynamics, DNA chemistry, DNA drug effects, Fluorescent Dyes pharmacology

Abstract

Single and dual-labeled fluorescent oligodeoxynucleotides are used in many molecular biology applications. We investigated the effects of commonly used fluorescent dyes and quenchers on the thermodynamic stability of a model probe-target DNA duplex. We demonstrate that those effects can be significant. Fluorescent dyes and quenchers were attached to the probe ends. In certain combinations, these groups stabilized the duplex up to 1.8kcal/mol and increased T(m) up to 4.3 degrees C. None of the groups tested significantly destabilized the duplex. Rank order of potency was, starting with the most stabilizing group: Iowa Black RQ approximately Black Hole 2>Cy5 approximately Cy3>Black Hole 1>QSY7 approximately Iowa Black FQ>Texas Red approximately TAMRA>FAM approximately HEX approximately Dabcyl>TET. Longer linkers decreased stabilizing effects. Hybridizations to targets with various dangling ends were also studied and were found to have only minor effects on thermodynamic stability. Depending on the dye/quencher combination employed, it can be important to include thermodynamic contributions from fluorophore and quencher when designing oligonucleotide probe assays.

Published

2005

182. Specific recognition of napthyridine-based ligands toward guanine-containing bulges in RNA duplexes and RNA-DNA heteroduplexes.

Author

Tok JB, Bi L, and Saenz M

Subjects

Anti-HIV Agents chemical synthesis, Binding Sites, Genes, env, Humans, Ligands, Nucleic Acid Conformation drug effects, Nucleic Acid Denaturation drug effects, RNA, Viral chemistry, Structure-Activity Relationship, Temperature, Base Pair Mismatch, Guanine, Naphthyridines chemistry, Nucleic Acid Heteroduplexes chemistry

Abstract

Mismatched bulges in nucleic acid constructs are important in the recognition event between biological molecules. Herein, it is observed that napthyridine dimer 2 is able to specifically bind G-G mismatches in all nucleic acid constructs comprising of RNA-RNA, RNA-DNA and DNA-DNA duplexes. However, the binding affinity of 2 is strongest toward DNA duplex, followed by RNA-DNA heteroduplex and RNA duplex being the weakest binding partner. Nonetheless, this binding behavior suggests that the binding process primarily occurs between the guanine base pairs and the napthyridine moiety, and is independent of the tertiary structure of the nucleic acid duplexes.

Published

2005

183. Truncated azinomycin analogues intercalate into DNA.

Author

Casely-Hayford MA, Pors K, Patterson LH, Gerner C, Neidle S, and Searcey M

Subjects

Antibiotics, Antineoplastic pharmacology, Azabicyclo Compounds, Cell Line, Tumor, Cell Survival drug effects, DNA chemistry, DNA metabolism, Dipeptides, Glycopeptides chemistry, Humans, Nucleic Acid Denaturation drug effects, Piperidines chemistry, Structure-Activity Relationship, Antibiotics, Antineoplastic chemical synthesis, DNA drug effects, Glycopeptides chemical synthesis, Intercalating Agents chemical synthesis

Abstract

The design and synthesis of a potentially more therapeutically-viable azinomycin analogue 4 based upon 3 has been completed. It involved coupling of a piperidine mustard to the acid chloride of the azinomycin chromophore. Both the designed azinomycin analogue 4 and the natural product 3 bind to DNA and cause unwinding, supporting an intercalative mode of binding.

Published

2005

184. Hitting multiple targets with multimeric ligands.

Author

Handl HL, Vagner J, Han H, Mash E, Hruby VJ, and Gillies RJ

Subjects

Antineoplastic Agents chemistry, Antineoplastic Agents pharmacology, Antineoplastic Agents therapeutic use, DNA drug effects, Drug Carriers, Kinetics, Models, Chemical, Molecular Structure, Nucleic Acid Denaturation drug effects, Nucleic Acid Hybridization drug effects, Polymers chemistry, Polymers pharmacokinetics, Protein Binding, Structure-Activity Relationship, Substrate Specificity, Thermodynamics, Drug Design, Ligands, Polymers pharmacology, Receptors, Drug drug effects

Abstract

Multimeric ligands consist of multiple monomeric ligands attached to a single backbone molecule, creating a multimer that can bind to multiple receptors or targets simultaneously. Numerous examples of multimeric binding exist within nature. Due to the multiple and simultaneous binding events, multimeric ligands bind with an increased affinity compared to their corresponding monomers. Multimeric ligands may provide opportunities in the field of drug discovery by providing enhanced selectivity and affinity of binding interactions, thus providing molecular-based targeted therapies. However, gaps in our knowledge currently exist regarding the quantitative measures for important design characteristics, such as flexibility, length and orientation of the inter-ligand linkers, receptor density and ligand sequence. In this review, multimeric ligand binding in two separate phases is examined. The prerecruitment phase describes the binding of one ligand of a multimer to its corresponding receptor, an event similar to monomeric ligand binding. This results in transient increases in the local concentration of the other ligands, leading to apparent cooperativity. The postrecruitment phase only occurs once all receptors have been aligned and bound by their corresponding ligand. This phase is analogous to DNA-DNA interactions in that the stability of the complex is derived from physical orientation. Multiple factors influence the kinetics and thermodynamics of multimeric binding, and these are discussed.

Published

2004

185. [The influence of the peptide bioregulator prostamax on heterochromatin of human lymphocytes in situ].

Author

Meskhi T, Khachidze D, Barbakadze Sh, Madzhagaladze G, Gorgoshidze M, Monaselidze D, Lezhava T, and Tadumadze N

Subjects

Aged, Calorimetry, Differential Scanning, Cells, Cultured, Humans, Lymphocytes ultrastructure, Middle Aged, Nucleic Acid Denaturation drug effects, Nucleosomes chemistry, Thermodynamics, Heterochromatin chemistry, Lymphocytes drug effects, Nucleosomes drug effects, Oligopeptides pharmacology

Abstract

It was shown that chromatin contained in human lymphocytes has two stages of denaturation: with T(d)VII = 94.4 degrees C, Q(d)VII = 50.8 J/g DNA, and T(d)VIII = 105.1 degrees C Q(d)VIII = 44.9 J/g DNA. The peptide bioregulator prostamax causes a redistribution of heat among endotherms T(d)III and T(d)IV and a shift of both endotherms to low temperatures by 2.9 and 1.0 degrees C, respectively. It was supposed that the redistribution of heat among endotherms is connected with a partial relaxation of the 30-nm-thick fiber in the 10-nm filament. A weak decrease in T(d)VIII and T(d)VII of lymphocytes treated with prostamax compared to untreated ones is connected with small structural changes of nucleosomal organization in the 10-nm filament and 30-nm-thick fiber.

Published

2004

186. Characterization of the synthetic compatible solute homoectoine as a potent PCR enhancer.

Author

Schnoor M, Voss P, Cullen P, Böking T, Galla HJ, Galinski EA, and Lorkowski S

Subjects

Base Sequence, DNA chemistry, DNA drug effects, DNA Primers, Dose-Response Relationship, Drug, Kinetics, Nucleic Acid Denaturation drug effects, Templates, Genetic, Amino Acids, Diamino pharmacology, Polymerase Chain Reaction

Abstract

Different substances such as dimethyl sulfoxide, tetramethylene sulfoxide, 2-pyrollidone, and the naturally occurring compatible solute betaine enhance PCR amplification of GC-rich DNA templates with high melting temperatures. In particular, cyclic compatible solutes outperform traditional PCR enhancers. We therefore investigated the effects that cyclic naturally occurring ectoine-type compatible solutes and their synthetic derivatives have on melting temperature of double-stranded DNA (dsDNA) and on PCR amplification of different templates. L-ectoine, betaine, and derivatives of L-ectoine decreased, whereas beta-hydroxyectoine increased, the melting temperature of dsDNA. The ability to decrease the melting temperature was greatest for homoectoine, a new synthetic derivative of l-ectoine. Furthermore, compatible solutes, especially homoectoine, enhanced PCR amplification of GC-rich DNA (72.6% GC content; effective range: 0.1-0.5M).

Published

2004

187. Binding of cationic porphyrin to isolated and encapsidated viral DNA analyzed by comprehensive spectroscopic methods.

Author

Zupán K, Herényi L, Tóth K, Majer Z, and Csík G

Subjects

Bacteriophage T7 genetics, Binding Sites, Cations, DNA, Viral drug effects, Nucleic Acid Denaturation drug effects, Phase Transition, Spectrum Analysis, Temperature, DNA, Viral chemistry, Porphyrins chemistry

Abstract

The complexation of tetrakis(4-N-methylpyridyl)porphyrin (TMPyP) with free and encapsidated DNA of T7 bacteriophage was investigated. To identify binding modes and relative concentrations of bound TMPyP forms, the porphyrin absorption spectra at various base pair/porphyrin ratios were analyzed. Spectral decomposition, fluorescent lifetime, and circular dichroism measurements proved the presence of two main binding types of TMPyP, e.g., external binding and intercalation both in free and in encapsidated DNA. Optical melting studies revealed that TMPyP increases the strand separation temperature of both free and native phage DNA and does not change the phase transition temperature of phage capsid proteins. From these findings we concluded that TMPyP binding does not influence the protein structure and/or the protein-DNA interaction. A combined analysis of absorption spectra and fluorescence decay curves made possible the determination of concentrations of free, externally bound, and intercalated porphyrin. As a perspective, our results facilitate a qualitative analysis of the TMPyP binding process at various experimental conditions.

Published

2004

188. The influence of intercalator binding on DNA triplex stability: correlation with effects on A-tract duplex structure.

Author

Sandström K, Wärmländer S, Bergman J, Engqvist R, Leijon M, and Gräslund A

Subjects

Animals, DNA genetics, Humans, Nucleic Acid Denaturation drug effects, Poly A genetics, Transition Temperature drug effects, DNA chemistry, DNA metabolism, Intercalating Agents metabolism, Intercalating Agents pharmacology, Nucleic Acid Conformation drug effects, Poly A metabolism

Abstract

The triplex form of DNA is of interest because of a possible biological role as well as the potential therapeutic use of this structure. In this paper the stabilizing effects of two intercalating drugs, ethidium and the quinoxaline derivative 9-OH-B220, on DNA triplexes have been studied by thermal denaturation measurements. The corresponding duplex structures of the DNA triplex systems investigated are either A-tract or normal B-DNA. The largest increases in the triplex melting temperatures caused by the intercalators were found for sequences having A-tract duplex structures. Inserting a single base pair with an N2-amino group in the minor groove, e.g. a G-C pair, breaks up the A-tract duplex structure and also reduces the stabilizing effect of the drugs on the triplex melting temperatures. The large drug-induced increase in triplex melting temperature for complexes having an original duplex A-tract structure is correlated with a low initial melting point of the triplex, not with the triplex being unusually stable in the presence of the drug. Hence, we conclude that the large thermal stabilizing effect exhibited by ethidium and 9-OH-B220 on dTn.dAn-dTn triplexes is partly caused by the intercalators breaking up the intrinsic A-tract structure of the underlying duplex., (Copyright 2004 John Wiley & Sons, Ltd.)

Published

2004

189. Peripheral substituents of di(pyridiumyl)porphyrins affected on their interactions with DNA.

Author

Wu S, Wang P, Tian T, Wu L, He H, Zhou X, Zhang X, and Cao X

Subjects

Animals, Cell Line, Tumor, Cell Survival drug effects, DNA chemistry, DNA drug effects, DNA Damage drug effects, Humans, Inhibitory Concentration 50, Nucleic Acid Denaturation drug effects, Photolysis, Plasmids chemistry, Plasmids metabolism, Pyridinium Compounds chemical synthesis, Pyridinium Compounds pharmacology, Structure-Activity Relationship, DNA metabolism, Porphyrins chemical synthesis, Porphyrins pharmacology

Abstract

meso- and beta-Substituted di(pyridiumyl)porphyrins 3, 4, and 7 have been synthesized and their interactions with DNA have been investigated. meso-Substituted porphyrins showed the stronger effect on DNA than that of beta-substituted porphyrin. Cytotoxicity of compound 3 (IC(50)) to THP-1 tumor cell was up to 0.11 nM.

Published

2004

190. The effect of C2-fluoro group on the biological activity of DC-81 and its dimers.

Author

Kamal A, Reddy PS, and Reddy DR

Subjects

Antineoplastic Agents pharmacology, Benzodiazepines chemical synthesis, Cell Line, Tumor, Cell Proliferation drug effects, DNA chemistry, Dimerization, Humans, Nucleic Acid Denaturation drug effects, Organophosphorus Compounds chemical synthesis, Structure-Activity Relationship, Temperature, Antineoplastic Agents chemical synthesis, Benzodiazepines pharmacology, Organophosphorus Compounds pharmacology

Abstract

C2-Fluoro substituted pyrrolobenzodiazepines (PBDs) have been synthesized that exhibit potential anticancer activity in a number of human tumour cell lines. These C2-fluoro substituted PBDs also exhibit significant DNA-binding ability.

Published

2004

191. Electrophoresis time impacts the denaturing gradient gel electrophoresis-based assessment of bacterial community structure.

Author

Sigler WV, Miniaci C, and Zeyer J

Subjects

Nucleic Acid Denaturation drug effects, Time Factors, Electrophoresis, Polyacrylamide Gel methods, Soil Microbiology

Abstract

We investigated the impact of denaturing gradient gel electrophoresis (DGGE) run time on the assessment of bacterial community structure. Results indicated that increased electrophoresis run time (while maintaining 1000 volt-hours) resulted in dissimilar profiles, likely due to instability of the denaturing gradient. We recommend that DGGE run times be minimized to provide optimal band resolution, as extended electrophoresis times can greatly impact subsequent band-based analyses.

Published

2004

192. YB-1 promotes strand separation in vitro of duplex DNA containing either mispaired bases or cisplatin modifications, exhibits endonucleolytic activities and binds several DNA repair proteins.

Author

Gaudreault I, Guay D, and Lebel M

Subjects

Adenosine Triphosphate metabolism, Antigens, Nuclear metabolism, Base Sequence, Catalysis, Cell Line, Cell Nucleus metabolism, Chromatography, Affinity, Cisplatin pharmacology, DNA chemistry, DNA genetics, DNA-Binding Proteins chemistry, DNA-Binding Proteins genetics, DNA-Binding Proteins isolation & purification, Endonucleases chemistry, Endonucleases genetics, Endonucleases isolation & purification, Humans, Ku Autoantigen, MutS Homolog 2 Protein, Nuclear Proteins, Nucleic Acid Denaturation drug effects, Protein Binding, Protein Structure, Quaternary, Protein Transport, Proto-Oncogene Proteins metabolism, Sequence Deletion, Substrate Specificity, Transcription Factors chemistry, Transcription Factors genetics, Transcription Factors isolation & purification, Y-Box-Binding Protein 1, Base Pair Mismatch, Base Pairing drug effects, Cisplatin metabolism, DNA metabolism, DNA Helicases, DNA Repair, DNA-Binding Proteins metabolism, Endonucleases metabolism, Transcription Factors metabolism

Abstract

YB-1 is a multifunctional protein involved in the regulation of transcription, translation, mRNA splicing and probably DNA repair. It contains a conserved cold shock domain and it binds strongly to inverted CCAAT box of different promoters. In this study, we have found that purified YB-1 oligomerizes readily in solutions to form trimers, hexamers and oligomers of 12 molecules. The presence of ATP changed the conformation of YB-1 in such a way that only dimers were detected by gel filtration analyses. Purified YB-1 can separate different DNA duplexes containing blunt ends, 5' or 3' recessed ends, or forked structures. This strand separation activity is increased on cisplatin-modified DNA or with duplex molecules containing mismatches. In addition to its exonuclease activity, YB-1 exhibits endonucleolytic activities in vitro. Finally, YB-1 affinity chromatography experiments have indicated that in addition to prespliceosome factors like nucleolin and ALY, YB-1 binds the DNA repair proteins MSH2, DNA polymerase delta, Ku80 and WRN proteins in vitro. Furthermore, immunofluorescence studies have shown that YB-1 re-localizes from the cytoplasm to nuclear areas containing either Ku80 or MSH2 proteins in human 293 embryonic kidney cells. These results suggest that YB-1 is involved in base excision and mismatch repair pathways.

Published

2004

193. Synthesis and alternate-stranded triplex forming ability of novel alpha-beta chimeric oligonucleotides bearing an intercalator-conjugated nucleobase.

Author

Azam AT, Hasegawa M, Moriguchi T, and Shinozuka K

Subjects

Base Sequence, DNA radiation effects, Deoxycytidine chemistry, Molecular Sequence Data, Nucleic Acid Conformation radiation effects, Nucleic Acid Denaturation drug effects, Nucleic Acid Denaturation radiation effects, Ultraviolet Rays, DNA chemical synthesis, Deoxycytidine analogs & derivatives, Intercalating Agents pharmacology, Nucleic Acid Conformation drug effects, Oligonucleotides chemical synthesis, Oligonucleotides chemistry

Abstract

A series of novel alpha-beta chimeric oligonucleotides bearing anthraquinone-attached nucleobase at linker position, were synthesized as a triplex-forming oligonucleotide (TFO). Their ability to stabilize the alternate-stranded triple helix was investigated through the UV-melting experiments.

Published

2004

194. Silver (I) cation specifically stabilizes heteroduplex with C:C mismatch base pair: toward the efficient detection of single nucleotide polymorphism (2).

Author

Torigoe H, Ono A, and Takamori A

Subjects

Base Pair Mismatch radiation effects, Base Sequence, Hydrogen-Ion Concentration, Molecular Sequence Data, Nucleic Acid Denaturation drug effects, Nucleic Acid Denaturation radiation effects, Nucleic Acid Heteroduplexes genetics, Nucleic Acid Heteroduplexes radiation effects, Transition Temperature, Ultraviolet Rays, Base Pair Mismatch drug effects, Nucleic Acid Heteroduplexes drug effects, Polymorphism, Single Nucleotide genetics, Silver pharmacology

Abstract

We examined the effect of silver (I) cation on the thermal stability of heteroduplex and homoduplex. Addition of silver (I) cation increased the melting temperature of heteroduplex containing C:C mismatch base pair by about 3-4 degrees C. The thermal stability of homoduplex and heteroduplexes containing other kinds of mismatch base pairs was not significantly changed by the addition of silver (I) cation. We conclude that silver (I) cation specifically stabilizes heteroduplex containing C:C mismatch base pair. Our results certainly support the idea that the addition of silver (I) cation to C:C mismatch base pair in heteroduplex could be a convenient strategy for heteroduplex analysis and may eventually lead to progress in single nucleotide polymorphism genotyping.

Published

2004

195. Interaction of DAPI with individual strands of trinucleotide repeats. Effects of replication in vitro of the AAT x ATT triplet.

Author

Trotta E, Del Grosso N, Erba M, Melino S, Cicero D, and Paci M

Subjects

Base Sequence, DNA biosynthesis, DNA genetics, Fluorescence, Indoles chemistry, Indoles pharmacology, Models, Molecular, Molecular Structure, Nucleic Acid Denaturation drug effects, Templates, Genetic, DNA chemistry, DNA metabolism, DNA Replication drug effects, Indoles metabolism, Nucleic Acid Conformation drug effects, Trinucleotide Repeats

Abstract

The structural changes produced by the minor-groove binding ligand DAPI (4',6-diamidine-2-phenylindole) on individual strands of trinucleotide repeat sequences were detected by electrophoretic band-shift analysis and related to their effects on DNA replication in vitro. Among the 20 possible single-stranded trinucleotide repeats, only the T-rich strand of the AAT.ATT triplet exhibits an observable fluorescence band and a change in electrophoretic mobility due to the drug binding. This is attributable to the property of DAPI that favours folding of the random coil ATT strand into a fast-migrating hairpin structure by a minor-groove binding mechanism. Electrophoretic characteristics of AAT, ACT, AGT, ATG and ATC are unchanged by DAPI, suggesting the crucial role of T.T with respect to A.A, C.C and G.G mismatch, in favouring the binding properties and the structural features of the ATT-DAPI complexes. Primer extension experiments, using the Klenow fragment of DNA polymerase I, demonstrate that such a selective structural change at ATT targets presents a marked property to stall DNA replication in vitro in comparison with the complementary AAT and a random GC-rich sequence. The results suggest a novel molecular mechanism of action of the DNA minor-groove binding ligand DAPI.

Published

2003

196. Mg2+-induced triplex formation of an equimolar mixture of poly(rA) and poly(rU).

Author

Kankia BI

Subjects

Binding, Competitive, Calorimetry methods, Magnesium pharmacology, Nucleic Acid Denaturation drug effects, Spectrophotometry, Ultraviolet, Temperature, Ultrasonics, Water chemistry, Magnesium chemistry, Nucleic Acid Conformation drug effects, Poly A chemistry, Poly U chemistry

Abstract

Magnesium ions strongly influence the structure and biochemical activity of RNA. The interaction of Mg2+ with an equimolar mixture of poly(rA) and poly(rU) has been investigated by UV spectroscopy, isothermal titration calorimetry, ultrasound velocimetry and densimetry. Measurements in dilute aqueous solutions at 20 degrees C revealed two differ ent processes: (i) Mg2+ binding to unfolded poly(rA)*poly(rU) up to [Mg2+]/[phosphate] = 0.25; and (ii) poly(rA)*2poly(rU) triplex formation at [Mg2+]/[phosphate] between 0.25 and 0.5. The enthalpies of these two different processes are favorable and similar to each other, approximately -1.6 kcal x mol(-1) of base pairs. Volume and compressibility effects of the first process are positive, 8 cm3 x mol(-1) and 24 x 10(-4) cm3 x mol(-1) x bar(-1), respectively, and correspond to the release of water molecules from the hydration shells of Mg2+ and the polynucleotides. The triplex formation is also accompanied by a positive change in compressibility, 14 x 10(-4) cm3 x mol(-1) x bar(-1), but only a small change in volume, 1 cm3 x mol(-1). A phase diagram has been constructed from the melting experiments of poly(rA)*poly(rU) at a constant K+ concentration, 140 mM, and various amounts of Mg2+. Three discrete regions were observed, corresponding to single-, double- and triple-stranded complexes. The phase boundary corresponding to the transition between double and triple helical conformations lies near physiological salt concentrations and temperature.

Published

2003

197. Influence of copper(II) and magnesium(II) ions on the ciprofloxacin binding to DNA.

Author

Drevensek P, Turel I, and Poklar Ulrih N

Subjects

Anti-Infective Agents metabolism, Ciprofloxacin metabolism, DNA metabolism, Fluorescence, Nucleic Acid Denaturation drug effects, Spectrum Analysis, Anti-Infective Agents chemistry, Ciprofloxacin chemistry, Copper chemistry, DNA chemistry, Magnesium chemistry

Abstract

The influence of magnesium(II) and copper(II) ions on the binding of ciprofloxacin to double stranded calf thymus DNA was studied by fluorescence emission spectroscopy, ultraviolet- and circular dichroism (CD) spectroscopy. The interaction of ciprofloxacin and copper(II) ions was followed by strong fluorescence quenching which was almost unaffected by the presence of DNA. On the other hand, only a slight decrease in fluorescence emission intensity, which was enhanced in the presence of DNA, was observed for ciprofloxacin interaction with magnesium(II) ions. Furthermore, magnesium(II) ions increase the thermal stability of the DNA, while, in the presence of ciprofloxacin, the degree of stabilisation is smaller. In contrast, copper(II) ions destabilise double helical DNA to heat, while ciprofloxacin slightly affects only the second transition of the biphasic melting curve of calf thymus DNA. Magnesium(II) ions at 25 degrees C induce conformational transitions of DNA at concentrations of 1.5 mM and 2.5 M, as monitored by CD. On the other hand copper(II) ions induce only one conformational transition, at a concentration of 12.7 microM. At higher concentrations of copper(II) ions (c>700 microM) DNA starts to precipitate. Significant changes in the CD spectra of DNA were observed after addition of ciprofloxacin to a solution containing DNA and copper(II) ions, but not to DNA and magnesium(II) ions. Based on our spectroscopic results, we propose that copper(II) ions are not directly involved into ciprofloxacin binding to DNA via phosphate groups as it has been suggested for magnesium(II) ions.

Published

2003

198. DNA binding mode of the cis and trans geometries of new antitumor nonclassical platinum complexes containing piperidine, piperazine, or 4-picoline ligand in cell-free media. Relations to their activity in cancer cell lines.

Author

Kasparkova J, Marini V, Najajreh Y, Gibson D, and Brabec V

Subjects

Animals, Antineoplastic Agents pharmacology, Base Sequence, Binding Sites, Cattle, Cell-Free System, Cisplatin analogs & derivatives, Cisplatin chemistry, Cisplatin metabolism, Cisplatin pharmacology, Cross-Linking Reagents, DNA chemistry, DNA genetics, DNA Adducts, Humans, In Vitro Techniques, Kinetics, Nucleic Acid Denaturation drug effects, Organoplatinum Compounds pharmacology, Stereoisomerism, Tumor Cells, Cultured, Antineoplastic Agents chemistry, Antineoplastic Agents metabolism, DNA metabolism, Organoplatinum Compounds chemistry, Organoplatinum Compounds metabolism

Abstract

The global modification of mammalian and plasmid DNAs by novel platinum compounds, cis- or trans-[PtCl(2)(NH(3))(Am)], where Am = NH(3), nonplanar heterocycle piperidine, piperazine, or aromatic planar heterocycle 4-picoline, was investigated in cell-free media using various biochemical and biophysical methods. These modifications have been compared with the activity of these new compounds in several tumor cell lines including those resistant to antitumor cis-diamminedichloroplatinum(II) (cisplatin). The results show that the replacement of the NH(3) group in cisplatin by the heterocyclic ligands does not considerably affect the DNA binding mode of this drug. Cytotoxicity studies have revealed that the replacement lowers the activity of the platinum compound in both sensitive and resistant cell lines. It has been suggested that the reduced activity of these analogues of cisplatin is associated with some features of the damaged DNA and/or its cellular processing. Alternatively, the reduced activity of the analogues of cisplatin might also be due to the factors that do not operate directly at the level of the target DNA, such as intracellular platinum uptake. In contrast to the analogues of cisplatin, the replacement of one ammine group by the heterocyclic ligand in its clinically ineffective trans isomer (transplatin) results in a radical enhancement of its activity in tumor cell lines. Importantly, this replacement also markedly alters the DNA binding mode of transplatin. The results support the view that one strategy of how to activate the trans geometry in bifunctional platinum(II) compounds including circumvention of resistance to cisplatin may consist of a chemical modification of the ineffective transplatin that results in an increased stability of its intrastrand cross-links in double-helical DNA and/or in an increased efficiency to form interstrand cross-links.

Published

2003

199. Effect of urea on the polymer buffer solutions used for the electrophoretic separations of nucleic acids.

Author

Todorov TI, Yamaguchi Y, and Morris MD

Subjects

Buffers, Nucleic Acid Denaturation drug effects, Nucleic Acids analysis, Polymers, Viscosity, Cellulose analogs & derivatives, Electrophoresis, Capillary methods, Nucleic Acids isolation & purification, Urea pharmacology

Abstract

The present study describes the effect of urea on the properties of hydroxyethyl cellulose (HEC) polymer solutions used for the separation of nucleic acids. Solution properties were investigated by viscosity measurements and supplemented by Raman spectroscopy of the solution components. By using viscosimetry, it was possible to identify that borate, urea, and HEC participate in an interaction causing an increase in the viscosity of dilute solutions. In addition, short polymer chains exhibited a 4-fold decrease in the entanglement threshold in the presence of 4 M urea and 0.356 M total borate concentration. These interactions were found to be specific to HEC. Raman spectroscopy monitored serial addition of 8 M urea to HEC sieving solutions combined with factor analysis indicated formation of minor urea species. Lack of change in the Raman spectrum and relative amount of borate suggested that there is no direct interaction between borate and urea. These effects on HEC sieving solution properties lead to the use of low HEC concentrations that are beneficial for the separation of nucleic acids under denaturing conditions.

Published

2003

200. Thermodynamics of DNA containing very stable chemically modified base pairs.

Author

Lando DY, Fridman AS, and Wartell R

Subjects

Algorithms, Cross-Linking Reagents pharmacology, DNA drug effects, Hot Temperature, Models, Chemical, Models, Molecular, Nucleic Acid Denaturation drug effects, Thermodynamics, Base Pairing, DNA chemistry, DNA Adducts chemistry

Abstract

DNA chemical modifications caused by the binding of some antitumor drugs give rise to a very strong local stabilization of the double helix. These sites melt at a temperature that is well above the melting temperatures of ordinary AT and GC base pairs. In this work we have examined the melting behavior of DNA containing very stable sites. Analytical expressions were derived and used to evaluate the thermodynamic properties of homopolymer DNA with several different distributions of stable sites. The results were extended to DNA with a heterogeneous sequence of AT and GC base pairs. The results were compared to the melting properties of DNA with ordinary covalent interstrand cross-links. It was found that, as with an ordinary interstrand cross-link, a single strongly stabilized site makes a DNA's melting temperature (T(m)) independent of strand concentration. However in contrast to a DNA with an interstrand cross-link, a strongly stabilized site makes the DNA's T(m) independent of DNA length and equal to T(infinity), the melting temperature of an infinite length DNA with the same GC-content and without a stabilized site. Moreover, at a temperature where more than 80% of base pairs are melted, the number of ordinary (non-modified) helical base pairs (n) is independent of both the DNA length and the location of the stabilized sites. For this condition, n(T) = (2 omega-a)S/(1-S) and S = exp[DeltaS(T(infinity)-T)/(RT)] where omega is the number of strongly stabilized sites in the DNA chain, a is the number of DNA ends that contain a stabilized site, and DeltaS, T, and R are the base pair entropy change, the temperature, and the universal gas constant per mole. The above expression is valid for a temperature interval that corresponds to n<0.2N for omega=1, and n<0.1N for omega>1, where N is the number of ordinary base pairs in the DNA chain.

Published

2003