Department of Chemistry, University of Toronto, Mississauga, ON L5L1C6, Canada.
Protein Eng Des Sel. 2010 May;23(5):337-46. doi: 10.1093/protein/gzp082. Epub 2010 Jan 19.
To explore the role of the HLH subdomain in bHLHZ proteins, we designed sets of minimalist proteins based on bHLHZ protein Max, bHLH/PAS protein Arnt and bZIP protein C/EBP. In the first, the Max bHLH and C/EBP leucine zipper were fused such that the leucine heptad repeats were not in register; therefore, the protein dimerization interface was disrupted. Max1bHLH-C/EBP showed little ability to activate transcription from the E-box (5'-CACGTG) in the yeast one-hybrid assay, and no E-box binding by quantitative fluorescence anisotropy. Max1bHLH-C/EBP's activity was significantly improved after library selection (three amino acids randomized between HLH and leucine zipper), despite the Max bHLH and C/EBP zipper still being out of register: a representative mutant gave a high nanomolar K(d) value for E-box binding. Thus, selection proved to be a powerful tool for salvaging the flawed Max1bHLH-C/EBP, although the out-of-register mutants still did not achieve the strong DNA-binding affinities displayed by their in-register counterparts. ArntbHLH-C/EBP hybrids further demonstrated the importance of maintaining register, as out-of-register mutants showed no E-box-responsive activity, whereas the in-register hybrid showed moderate activity. In another design, we eliminated the HLH altogether and fused the Max basic region to the C/EBP zipper to generate bZIP-like hybrids. Despite numerous designs and selections, these hybrids possessed no E-box-responsive activity. Finally, we tested the importance of the loop sequence in MaxbHLHZ by fluorescence and circular dichroism. In one mutant, the loop was shortened by two residues; in the other, the Lys57:DNA-backbone interaction was abolished by mutation to Gly57. Both showed markedly decreased E-box-binding relative to MaxbHLHZ. Our results suggest that, in contrast to the more rigid bZIP, the HLH is capable of significant conformational adaptation to enable gene-regulatory function and is required for protein dimerization and positioning the basic region for DNA recognition.
为了探索 HLH 结构域在 bHLHZ 蛋白中的作用,我们基于 bHLHZ 蛋白 Max、bHLH/PAS 蛋白 Arnt 和 bZIP 蛋白 C/EBP 设计了一系列最小化蛋白。在第一个设计中,Max bHLH 和 C/EBP 亮氨酸拉链融合,使得亮氨酸七肽重复序列不能匹配;因此,蛋白二聚化界面被破坏。Max1bHLH-C/EBP 在酵母单杂交测定中几乎不能激活 E-box(5'-CACGTG)的转录,并且通过定量荧光各向异性没有检测到 E-box 结合。经过文库选择(HLH 和亮氨酸拉链之间的三个氨基酸随机化)后,Max1bHLH-C/EBP 的活性显著提高:一个代表性的突变体对 E-box 结合的高纳摩尔 K(d) 值。因此,选择证明是挽救有缺陷的 Max1bHLH-C/EBP 的有力工具,尽管 Max bHLH 和 C/EBP 拉链仍然没有匹配:一个代表突变体对 E-box 结合的高纳摩尔 K(d) 值。因此,选择证明是挽救有缺陷的 Max1bHLH-C/EBP 的有力工具,尽管 Max bHLH 和 C/EBP 拉链仍然没有匹配:一个代表突变体对 E-box 结合的高纳摩尔 K(d) 值。因此,选择证明是挽救有缺陷的 Max1bHLH-C/EBP 的有力工具,尽管 Max bHLH 和 C/EBP 拉链仍然没有匹配:一个代表突变体对 E-box 结合的高纳摩尔 K(d) 值。因此,选择证明是挽救有缺陷的 Max1bHLH-C/EBP 的有力工具,尽管 Max bHLH 和 C/EBP 拉链仍然没有匹配:一个代表突变体对 E-box 结合的高纳摩尔 K(d) 值。尽管如此,突变体仍然没有达到其匹配的同类蛋白的强 DNA 结合亲和力。ArntbHLH-C/EBP 杂种进一步证明了保持匹配的重要性,因为不匹配的突变体没有表现出对 E-box 的反应活性,而匹配的杂种则表现出适度的活性。在另一个设计中,我们完全消除了 HLH,并将 Max 碱性区域融合到 C/EBP 拉链上,生成了 bZIP 样杂种。尽管进行了多次设计和选择,这些杂种仍然没有表现出对 E-box 的反应活性。最后,我们通过荧光和圆二色性测试了 MaxbHLHZ 中环序列的重要性。在一个突变体中,环缩短了两个残基;在另一个突变体中,Lys57:DNA-骨架相互作用被突变到 Gly57 而被破坏。与 MaxbHLHZ 相比,这两种突变体的 E-box 结合都明显减少。我们的结果表明,与更刚性的 bZIP 相比,HLH 能够进行显著的构象适应,从而实现基因调控功能,并且需要蛋白二聚化和定位碱性区域以进行 DNA 识别。
