Leibniz Institut für Molekulare Pharmakologie im Forschungsverbund Berlin e.V. (FMP), Campus Berlin-Buch, Robert-Roessle-Str. 10, D-13125 Berlin, Germany.; Freie Universität Berlin, Fachbereich BCP, Takustr. 3, 14195 Berlin, Germany.
Leibniz Institut für Molekulare Pharmakologie im Forschungsverbund Berlin e.V. (FMP), Campus Berlin-Buch, Robert-Roessle-Str. 10, D-13125 Berlin, Germany.
Sci Adv. 2016 Aug 19;2(8):e1600379. doi: 10.1126/sciadv.1600379. eCollection 2016 Aug.
Proteins are synthesized in cells by ribosomes and, in parallel, prepared for folding or targeting. While ribosomal protein synthesis is progressing, the nascent chain exposes amino-terminal signal sequences or transmembrane domains that mediate interactions with specific interaction partners, such as the signal recognition particle (SRP), the SecA-adenosine triphosphatase, or the trigger factor. These binding events can set the course for folding in the cytoplasm and translocation across or insertion into membranes. A distinction of the respective pathways depends largely on the hydrophobicity of the recognition sequence. Hydrophobic transmembrane domains stabilize SRP binding, whereas less hydrophobic signal sequences, typical for periplasmic and outer membrane proteins, stimulate SecA binding and disfavor SRP interactions. In this context, the formation of helical structures of signal peptides within the ribosome was considered to be an important factor. We applied dynamic nuclear polarization magic-angle spinning nuclear magnetic resonance to investigate the conformational states of the disulfide oxidoreductase A (DsbA) signal peptide stalled within the exit tunnel of the ribosome. Our results suggest that the nascent chain comprising the DsbA signal sequence adopts an extended structure in the ribosome with only minor populations of helical structure.
蛋白质在细胞中由核糖体合成,并同时为折叠或靶向而准备。在核糖体蛋白合成进行的同时,新生链暴露氨基末端信号序列或跨膜结构域,介导与特定相互作用伙伴的相互作用,例如信号识别颗粒(SRP)、SecA-三磷酸腺苷酶或触发因子。这些结合事件可以为细胞质中的折叠和跨膜或插入膜的转移设定方向。各自途径的区别在很大程度上取决于识别序列的疏水性。疏水性跨膜结构域稳定 SRP 结合,而疏水性较小的信号序列,典型的周质和外膜蛋白,刺激 SecA 结合并不利于 SRP 相互作用。在这方面,核糖体内信号肽形成螺旋结构被认为是一个重要因素。我们应用动态核极化魔角旋转核磁共振来研究折叠酶 A(DsbA)信号肽在核糖体出口隧道内停滞的构象状态。我们的结果表明,包含 DsbA 信号序列的新生链在核糖体中采用延伸结构,只有少量的螺旋结构。