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RNA and Protein Complexes of trp RNA-Binding Attenuation Protein Characterized by Mass Spectrometry

机译:质谱表征的trp RNA结合减弱蛋白的RNA和蛋白复合物

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We have characterized both wild-type and mutant TRAP (trp RNA-binding attenuation protein) from Bacillus stearo-thermophilus, and their complexes with RNA or its regulator anti-TRAP protein (AT), by electrospray ionization mass spectrometry (ESI-MS). Wild-type TRAP mainly forms homo-11mer rings. The mutant used carries three copies of the TRAP monomer on a single polypeptide chain so that it associates to form a 12mer ring with four polypeptide molecules. Mass spectra showed that both the wild-type TRAP 11mer and the mutant TRAP 12mer can bind a cognate single-stranded RNA molecule with a molar ratio of 1:1. The crystal structure of wild-type TRAP complexed with AT shows a TRAP 12mer ring surrounded by six AT trimers. However, nanoESI-MS of wild-type TRAP mixed with AT shows four species with different binding stoichiometries, and the complex observed by crystallography represents only a minor species in solution; most of the TRAP remains in an 11mer ring form. Mass spectra of mutant TRAP showed only a single species, TRAP 12mer + six copies of AT trimer, which is observed by crystallography. These results suggest that crystallization selects only the most symmetrical TRAP-AT complex from the solution, whereas ESI-MS can take a "snapshot" of all the species in solution.
机译:我们已经通过电喷雾电离质谱(ESI-MS)鉴定了来自嗜热脂肪芽孢杆菌的野生型和突变型TRAP(trp RNA结合减弱蛋白)及其与RNA或其调节剂抗TRAP蛋白(AT)的复合物。 。野生型TRAP主要形成同11聚体环。所使用的突变体在一条多肽链上带有三份TRAP单体,因此它与四个多肽分子结合形成一个12mer环。质谱表明,野生型TRAP 11mer和突变型TRAP 12mer均可以摩尔比为1:1结合同源单链RNA分子。与AT复合的野生型TRAP的晶体结构显示,TRAP 12mer环被六个AT三聚体包围。然而,野生型TRAP与AT混合的nanoESI-MS显示出四种具有不同结合化学计量的物种,并且通过晶体学观察到的复合物仅代表溶液中的一小部分。大多数TRAP仍为11mer环形式。突变TRAP的质谱显示仅单个物种,TRAP 12mer + AT三聚体的六个拷贝,其通过晶体学观察到。这些结果表明,结晶仅从溶液中选择最对称的TRAP-AT络合物,而ESI-MS可以对溶液中所有物质进行“快照”。

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