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Substrate Transport Activation Is Mediated through Second Periplasmic Loop of Transmembrane Protein MalF in Maltose Transport Complex of Escherichia coli

机译:底物运输激活是通过第二个周质环的跨膜蛋白MalF在大肠杆菌的麦芽糖运输复合物中介导的。

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摘要

In a recent study we described the second periplasmic loop P2 of the transmembrane protein MalF (MalF-P2) of the maltose ATP-binding cassette transporter (MalFGK2-E) as an important element in the recognition of substrate by the maltose-binding protein MalE. In this study, we focus on MalE and find that MalE undergoes a structural rearrangement after addition of MalF-P2. Analysis of residual dipolar couplings (RDCs) shows that binding of MalF-P2 induces a semiopen state of MalE in the presence and absence of maltose, whereas maltose is retained in the binding pocket. These data are in agreement with paramagnetic relaxation enhancement experiments. After addition of MalF-P2, an increased solvent accessibility for residues in the vicinity of the maltose-binding site of MalE is observed. MalF-P2 is thus not only responsible for substrate recognition, but also directly involved in activation of substrate transport. The observation that substrate-bound and substrate-free MalE in the presence of MalF-P2 adopts a similar semiopen state hints at the origin of the futile ATP hydrolysis of MalFGK2-E.
机译:在最近的研究中,我们描述了麦芽糖ATP结合盒转运蛋白(MalFGK2-E)的跨膜蛋白MalF(MalF-P2)的第二周质环P2是麦芽糖结合蛋白MalE识别底物的重要元素。在这项研究中,我们专注于MalE,发现添加MalF-P2后MalE发生结构重排。残留偶极偶合(RDC)的分析表明,在存在和不存在麦芽糖的情况下,MalF-P2的结合会诱导MalE的半开放状态,而麦芽糖则保留在结合口袋中。这些数据与顺磁弛豫增强实验一致。添加MalF-P2后,观察到MalE的麦芽糖结合位点附近残基的溶剂可及性增加。因此,MalF-P2不仅负责底物识别,还直接参与底物运输的激活。在存在MalF-P2的情况下,与底物结合和不含底物的MalE采取类似的半开放状态的观察结果暗示了MalFGK2-E的无用ATP水解的起源。

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