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Parallel-stranded duplex DNA containing blocks of trans purine-purine and purine-pyrimidine base pairs.

机译:包含反式嘌呤-嘌呤和嘌呤-嘧啶碱基对的嵌段的平行链双链DNA。

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摘要

A 30 base pair parallel-stranded (ps) duplex ps-L1.L2 composed of two adjoined purine-purine and purine-pyrimidine sequence blocks has been characterized thermodynamically and spectroscopically. The 5'-terminal 15 residues in both strands ('left-half') consisted of the alternating d(GA)7G sequence that forms a ps homoduplex secondary structure stabilized by d(G.G) and d(A.A) base pairs. The 3'-terminal 15 positions of the sequence ('right-half') were combinations of A and T with complementary reverse Watson-Crick d(A.T) base pairing between the two strands. The characteristics of the full length duplex were compared to those of the constituent left and right halves in order to determine the compatibility of the two ps helical forms. The thermal denaturation curves and hyperchromicity profiles of all three duplexes determined by UV absorption spectroscopy were characteristic of ps-DNA, in accordance with previous studies. The thermodynamic properties of the 30 bp duplex corresponded within experimental error to the linear combination of the two 15-mers. Thus, the Tm and delta HvH of ps-L1.L2 in 10 mM MgCl2, derived from analyses according to a statistical mechanical formulation for the helix-coil transition, were 43 degrees C and 569 kJ mol-1, compared to 21 degrees C, 315 kJ mol-1 (ps-F5.F6) and 22 degrees C, 236 kJ mol-1 (ps-GA15). The UV absorption and CD spectra of ps-L1.L2 and the individual 15-mer ps motifs were also compared quantitatively. The sums of the two constituent native spectra (left+right halves) accurately matched that of the 30 bp duplex, with only small deviations in the 195-215 nm (CD) and 220-240 nm (absorption) regions. Based on analysis by native gel electrophoresis, the sequences studied formed duplex structures exclusively; there were no indications of higher order species. Chemical modification with diethyl pyrocarbonate showed no hyperreactivity of the junctional bases, indicating a smooth transition between the two parallel-stranded conformations. We conclude that under given salt conditions, oligonucleotides with normal primary chemical structures can readily form a parallel-stranded double helix based on blocks of very disparate non-canonical purine-purine and purine-pyrimidine base pairs and without perceptible destabilization at the junction. There are biological implications of these findings in relation to genetic structure and expression.
机译:由两个相邻的嘌呤-嘌呤和嘌呤-嘧啶序列嵌段组成的30个碱基对的平行链(ps)双链ps-L1.L2具有热力学和光谱学特征。两条链中的5'-末端15个残基(“左半”)由交替的d(GA)7G序列组成,形成了由d(G.G)和d(A.A)碱基对稳定的ps同源双链二级结构。序列的3'端15个位置(“右半”)是A和T的组合,在两条链之间具有互补的反向Watson-Crick d(A.T)碱基对。将全长双链体的特征与组成的左右两半的特征进行比较,以确定两个ps螺旋形式的相容性。根据先前的研究,通过紫外线吸收光谱法测定的所有三个双链体的热变性曲线和增色曲线是ps-DNA的特征。 30 bp双链体的热力学性质在实验误差内与两个15-mer的线性组合相对应。因此,根据针对螺旋-螺旋转变的统计机械公式进行分析得出的10 mM MgCl2中的ps-L1.L2的Tm和HvH值分别为21摄氏度和43摄氏度和569 kJ mol-1。 ,315 kJ mol-1(ps-F5.F6)和22摄氏度,236 kJ mol-1(ps-GA15)。还定量比较了ps-L1.L2和各个15-mer ps图案的UV吸收和CD光谱。两个组成本征光谱的总和(左半部分和右半部分)与30 bp双链体的总谱精确匹配,在195-215 nm(CD)和220-240 nm(吸收)区域只有很小的偏差。基于天然凝胶电泳的分析,所研究的序列仅形成双链结构。没有迹象表明有更高的物种。用焦碳酸二乙酯进行的化学修饰没有显示连接碱基的高反应性,表明两个平行链构象之间的平滑过渡。我们得出的结论是,在给定的盐条件下,具有正常一级化学结构的寡核苷酸可以基于非常不同的非规范性嘌呤-嘌呤和嘌呤-嘧啶碱基对的嵌段,很容易形成平行链双螺旋,并且在连接处没有明显的不稳定。这些发现与遗传结构和表达有关,具有生物学意义。

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