Wang Y, de los Santos C, Gao X O, Greene K, Live D, Patel D J
Department of Biochemistry and Molecular Biophysics, College of Physicians and Surgeons, Columbia University, New York, NY 10032.
J Mol Biol. 1991 Dec 5;222(3):819-32. doi: 10.1016/0022-2836(91)90513-6.
There has been much recent interest in the self-association of short deoxyguanosine-rich motifs within single-stranded DNAs to generate monovalent cation modulated four-stranded helical segments called G-quadruplexes stabilized by hydrogen-bonded G-tetrad alignments. We have addressed structural aspects of this novel alignment and report on multinuclear 1H, 31P and 13C nuclear magnetic resonance studies on the d(G2T4CG2) deoxynonanucleotide with Na cation as counterion in aqueous solution at low temperature. This sequence forms stable structures even though it cannot align by Watson-Crick hydrogen bond formation (see the paper on d(G2T5G2) describing optical and calorimetric measurements by Jin, R., Breslauer, K. J., Jones, R. A. & Gaffney, B. L. (1990), Science, 250, 543-546). The four narrow exchangeable protons detected between 11.5 and 12.0 parts per million (p.p.m.), which are common to the d(G2T4CG2) deoxynonanucleotide and the d(G2TCG2) deoxyhexanucleotide sequences, are assigned to deoxyguanosine imino protons hydrogen-bonded to carbonyl acceptor groups. These narrow imino protons are not detected for d(IGN5IG) and d(I2N5G2), where two deoxyguanosine residues are replaced by two deoxyinosine residues in the deoxynonanucleotide sequences. This implies that the 2-amino protons of deoxyguanosine must also participate in hydrogen bond formation and stabilize the structured conformation of d(G2T4CG2) in Na cation-containing solution. We have completely assigned the base and sugar H1', H2',2'', H3', and H4' protons of the d(G2T4CG2) oligomer following analysis of two-dimensional nuclear Overhauser enhancement spectroscopy and two-dimensional correlated spectroscopy data sets in 0.1 M-NaCl, 10 mM-sodium phosphate, 2H2O solution at 0 degree C. The relative magnitude of the nuclear Overhauser enhancements (NOEs) between the base H8 and its own sugar H1' protons of individual deoxyguanosine residues establishes that G1 and G8 adopt syn orientations while G2 and G9 adopt anti orientations about the glycosidic bond in the d(G1-G2-T3-T4-T5-T6-C7-G8-G9) sequence in both Na and K cation-containing aqueous solution. Consequently, any structure proposed for the tetramolecular complex of d(G2T4CG2) must exhibit alternating G(syn) and G(anti) glycosidic torsion angles within each strand. The directionality and magnitude of the observed NOEs are consistent with the G(syn)-G(anti) steps adopting right-handed helical conformations in solution. We also note that the H8 protons of G1 and G8 (7.35 to 7.45 p.p.m.) in a syn alignment are shifted significantly upfield from the H8 protons of G2 and G9 (8.0 to 8.3 p.p.m.) in an anti alignment.(ABSTRACT TRUNCATED AT 400 WORDS)
最近,单链DNA中富含脱氧鸟苷的短基序的自缔合引起了广泛关注,这种自缔合能够生成由氢键连接的G-四联体排列稳定的单价阳离子调节的四链螺旋片段,即G-四链体。我们研究了这种新型排列的结构方面,并报告了在低温下以Na + 为抗衡离子的水溶液中对d(G2T4CG2)脱氧九核苷酸进行的多核1H、31P和13C核磁共振研究。即使该序列不能通过沃森-克里克氢键形成进行排列(见关于d(G2T5G2)的论文,Jin, R., Breslauer, K. J., Jones, R. A. & Gaffney, B. L. (1990), Science, 250, 543 - 546描述了光学和量热测量),它也能形成稳定结构。在百万分之11.5至12.0(ppm)之间检测到的四个窄可交换质子,是d(G2T4CG2)脱氧九核苷酸和d(G2TCG2)脱氧六核苷酸序列共有的,它们被指定为与羰基受体基团形成氢键的脱氧鸟苷亚氨基质子。对于d(IGN5IG)和d(I2N5G2),未检测到这些窄亚氨基质子,在脱氧九核苷酸序列中,两个脱氧鸟苷残基被两个脱氧肌苷残基取代。这意味着脱氧鸟苷的2-氨基质子也必须参与氢键形成,并在含Na + 的溶液中稳定d(G2T4CG2)的结构构象。在0.1 M - NaCl、10 mM - 磷酸钠、2H2O溶液中,于0℃分析二维核Overhauser增强光谱和二维相关光谱数据集后,我们已完全确定了d(G2T4CG2)寡聚物的碱基和糖的H1'、H2'、2''、H3'和H4'质子。单个脱氧鸟苷残基的碱基H8与其自身糖的H1'质子之间的核Overhauser增强(NOE)的相对大小表明,在含Na + 和K + 的水溶液中,d(G1 - G2 - T3 - T4 - T5 - T6 - C7 - G8 - G9)序列中,G1和G8围绕糖苷键采取顺式取向,而G2和G9采取反式取向。因此,为d(G2T4CG2)的四分子复合物提出的任何结构在每条链内都必须呈现交替的G(顺式)和G(反式)糖苷扭转角。观察到的NOE的方向性和大小与溶液中采取右手螺旋构象的G(顺式)-G(反式)步长一致。我们还注意到,顺式排列的G1和G8的H8质子(7.35至7.45 ppm)比反式排列的G2和G9的H8质子(8.0至8.3 ppm)明显向高场移动。(摘要截短于400字)
