Mazzarelli J M, Rajur S B, Iadarola P L, McLaughlin L W
Department of Chemistry, Boston College, Chestnut Hill, Massachusetts 01267.
Biochemistry. 1992 Jun 30;31(25):5925-36. doi: 10.1021/bi00140a032.
A series of modified trp operator sequences has been prepared by the incorporation of seven different base analogues. Four of the analogues allow the site-specific deletion of functional groups present on the dA-dT and dT-dA base pairs at positions -4/+4 and -5/+5 in the trp operator. The remaining three analogues permit the incorporation of structural analogues of the native dA-dT or dG-dC base pairs. The duplex operator sequences all exhibit Tm values well above ambient temperature (48-70 degrees C), and these values generally correlate very well with the number of interstrand hydrogen bonds present. The affinity between the trp repressor and 14 modified operator sequences was examined using a recently developed alkaline phosphatase protection assay. The results from the analogue sequences used in this study suggest that the structure of the dA-dT or dT-dA base pairs at positions -4/+4 and -5/+5, respectively, has relatively little effect upon the solution binding by the trp repressor, but the protein is very sensitive to the orientation of the amino and carbonyl functional groups at the -4/+4 positions, which are involved in the formation of an interbase hydrogen bond present in the major groove. (The term structure in this case refers to the hydrogen bonding structure of the base pairs. We recognize that the introduction of conservative functional group deletions or reversals may affect other structural criteria such as hydration.) The deletion of individual functional groups from the operator sequence suggests that the carbonyl at dT+4 is critical for formation of the high-affinity sequence-specific complex. Additionally, the thymine methyl group at dT+4 and the N7 nitrogen of dA+5 appear to be critical contacts necessary for high-affinity binding by the repressor. The thymine carbonyl and the adenine N7 nitrogen are each responsible for approximately -1.5 kcal/mol of apparent free energy of binding. The thymine methyl provides a somewhat smaller contribution of -0.7 kcal/mol. Deletion of either of the adenine amino groups at dA-4 or dA+5 results in a sequence that binds to the repressor with a higher affinity than observed with the native sequence; this can be explained in that the functional groups lost are not critical for binding, and the resulting increased flexibility of the operator, or the creation of a more hydrophobic surface at these sites, enhances van der Waals contacts between the protein and the nucleic acid.
通过掺入七种不同的碱基类似物,制备了一系列修饰的色氨酸操纵子序列。其中四种类似物可实现对色氨酸操纵子中 -4/+4 和 -5/+5 位置的 dA-dT 和 dT-dA 碱基对上存在的官能团进行位点特异性缺失。其余三种类似物允许掺入天然 dA-dT 或 dG-dC 碱基对的结构类似物。双链操纵子序列的解链温度(Tm)值均远高于环境温度(48 - 70℃),并且这些值通常与存在的链间氢键数量密切相关。使用最近开发的碱性磷酸酶保护试验检测了色氨酸阻遏物与 14 种修饰的操纵子序列之间的亲和力。本研究中使用的类似物序列的结果表明,分别位于 -4/+4 和 -5/+5 位置的 dA-dT 或 dT-dA 碱基对的结构对色氨酸阻遏物在溶液中的结合影响相对较小,但该蛋白质对 -4/+4 位置的氨基和羰基官能团的取向非常敏感,这些官能团参与形成存在于大沟中的碱基间氢键。(在这种情况下,结构一词指的是碱基对的氢键结构。我们认识到保守官能团的缺失或反转的引入可能会影响其他结构标准,如水合作用。)从操纵子序列中删除单个官能团表明,dT+4 处的羰基对于形成高亲和力序列特异性复合物至关重要。此外,dT+4 处的胸腺嘧啶甲基和 dA+5 的 N7 氮似乎是阻遏物高亲和力结合所需的关键接触点。胸腺嘧啶羰基和腺嘌呤 N7 氮各自对表观结合自由能贡献约 -1.5 千卡/摩尔。胸腺嘧啶甲基的贡献稍小,为 -0.7 千卡/摩尔。删除 dA-4 或 dA+5 处的腺嘌呤氨基之一会导致一个与阻遏物结合的序列,其亲和力高于天然序列;这可以解释为失去的官能团对结合并不关键,并且操纵子由此增加的灵活性,或者在这些位点形成的更疏水表面,增强了蛋白质与核酸之间的范德华接触。
