THERMODYNAMICS OF OLIGODEOXYRIBONUCLEOTIDE-DIRECTED TRIPLE HELIX FORMATION - AN ANALYSIS USING QUANTITATIVE AFFINITY CLEAVAGE TITRATION

被引：80

作者：

SINGLETON, SF ^{[1
]}

DERVAN, PB ^{[1
]}

机构：

[1] CALTECH, ARNOLD & MABEL BECKMAN LABS CHEM SYNTH, PASADENA, CA 91125 USA

来源：

JOURNAL OF THE AMERICAN CHEMICAL SOCIETY | 1992年 / 114卷 / 18期

关键词：

D O I：

10.1021/ja00044a002

中图分类号：

O6 [化学];

学科分类号：

0703 ;

摘要：

The free energy for oligodeoxyribonucleotide-directed triple helix formation at a single site on a DNA plasmid fragment has been analyzed using quantitative affinity cleavage titration. Measurement of the amount of site-specific cleavage of a 339-bp radiolabeled DNA duplex produced at 24-degrees-C (100 mM Na+, 1 mM spermine-4HCl, 50 mM Tris-acetate, pH 7.0) over a concentration change of four orders of magnitude for oligodeoxyribonucleotide-EDTA.Fe 1.Fe, (5'-T*TTTTCTCTCTCTCT-3') yields an equilibrium binding constant, K(T) = 3.7 +/- 1.1 x 10(6) M-1 (DELTA-G(T) = -9.0 +/- 0.2 kcal.mol-1). Quantitative affinity cleavage titration affords association constants that are identical within experimental uncertainty with those obtained from quantitative DNase I footprint titration of the same oligonucleotide with and without EDTA.In (1.In and 6, respectively). Removal of one thymidine and one cytidine residue from the 3' end of 1.Fe reduces the free energy of binding by 0.5 kcal.mol-1, and removal of two thymidine and two cytidine residues from its 3' terminus decreases the binding free energy by 1.1 kcal.mol-1 at pH 7.0. Single internal base triplet mismatches result in a destabilization of the local triple-helical structure by 2.5-3.0 kcal.mol-1. Quantitative affinity cleavage titration is a general method which should allow for the measurement of equilibrium constants for the association of many DNA-binding molecules to single sites on relatively large DNA under a broad range of solution conditions.

引用

页码：6957 / 6965

页数：9

共 82 条

[61] NMR STRUCTURAL STUDIES OF INTRAMOLECULAR (Y+)N.(R+)N(Y-)N DNA TRIPLEXES IN SOLUTION - IMINO AND AMINO PROTON AND NITROGEN MARKERS OF G.TA BASE TRIPLE FORMATION [J].

RADHAKRISHNAN, I ;

GAO, XL ;

DELOSSANTOS, C ;

LIVE, D ;

PATEL, DJ .

BIOCHEMISTRY, 1991, 30 (37) :9022-9030

[62] NUCLEAR-MAGNETIC-RESONANCE STRUCTURAL STUDIES OF INTRAMOLECULAR PURINE.PURINE.PYRIMIDINE DNA TRIPLEXES IN SOLUTION - BASE TRIPLE PAIRING ALIGNMENTS AND STRAND DIRECTION [J].

RADHAKRISHNAN, I ;

DELOSSANTOS, C ;

PATEL, DJ .

JOURNAL OF MOLECULAR BIOLOGY, 1991, 221 (04) :1403-1418

[63] 3-DIMENSIONAL HOMONUCLEAR NOESY-TOCSY OF AN INTRAMOLECULAR PYRIMIDINE.PURINE.PYRIMIDINE DNA TRIPLEX CONTAINING A CENTRAL G.TA TRIPLE - NONEXCHANGEABLE PROTON ASSIGNMENTS AND STRUCTURAL IMPLICATIONS [J].

RADHAKRISHNAN, I ;

PATEL, DJ ;

GAO, XL .

BIOCHEMISTRY, 1992, 31 (09) :2514-2523

[64] NMR-STUDIES OF TRIPLE-STRAND FORMATION FROM THE HOMOPURINE HOMOPYRIMIDINE DEOXYRIBONUCLEOTIDE-D(GA)4 AND DEOXYRIBONUCLEOTIDE-D(TC)4 [J].

RAJAGOPAL, P ;

FEIGON, J .

BIOCHEMISTRY, 1989, 28 (19) :7859-7870

[65] TRIPLE-STRAND FORMATION IN THE HOMOPURINE HOMOPYRIMIDINE DNA OLIGONUCLEOTIDE-D(G-A)4 AND OLIGONUCLEOTIDE-D(T-C)4 [J].

RAJAGOPAL, P ;

FEIGON, J .

NATURE, 1989, 339 (6226) :637-640

[66] QUANTITATIVE FOOTPRINTING ANALYSIS - BINDING TO A SINGLE SITE [J].

REHFUSS, R ;

GOODISMAN, J ;

DABROWIAK, JC .

BIOCHEMISTRY, 1990, 29 (03) :777-781

[67] SPECIFICITY AND STRINGENCY IN DNA TRIPLEX FORMATION [J].

ROBERTS, RW ;

CROTHERS, DM .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1991, 88 (21) :9397-9401

[68] HEAT OF REACTION FORMING 3-STRANDED POLY (A PLUS 2U) COMPLEX [J].

ROSS, PD ;

SCRUGGS, RL .

BIOPOLYMERS, 1965, 3 (04) :491-&

[69]

RUNNEBAUM IB, 1991, BIOTECHNIQUES, V11, P446

[70] ENERGETICS OF COOPERATIVE PROTEIN DNA INTERACTIONS - COMPARISON BETWEEN QUANTITATIVE DEOXYRIBONUCLEASE FOOTPRINT TITRATION AND FILTER BINDING [J].

SENEAR, DF ;

BRENOWITZ, M ;

SHEA, MA ;

ACKERS, GK .

BIOCHEMISTRY, 1986, 25 (23) :7344-7354

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