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2
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Mode of insertion of the signal sequence of a bacterial precursor protein into phospholipid bilayers as revealed by cysteine-based site-directed spectroscopy.基于半胱氨酸的定点光谱法揭示细菌前体蛋白信号序列插入磷脂双层膜的模式
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8
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Rate constants of sugar transport through two LamB mutants of Escherichia coli: comparison with wild-type maltoporin and LamB of Salmonella typhimurium.糖通过大肠杆菌两个LamB突变体的转运速率常数:与野生型麦芽糖孔蛋白及鼠伤寒沙门氏菌LamB的比较。
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Use of synthetic signal sequences to explore the protein export machinery.利用合成信号序列探索蛋白质输出机制。
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Effect of protein aggregation in the aqueous phase on the binding of membrane proteins to membranes.水相中蛋白质聚集对膜蛋白与膜结合的影响。
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Regulation of the ribosome-membrane junction at early stages of presecretory protein translocation in the mammalian endoplasmic reticulum.哺乳动物内质网中分泌前蛋白转运早期核糖体 - 膜连接的调控。
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本文引用的文献

1
Incorporation of melittin into phosphatidylcholine bilayers. Study of binding and conformational changes.蜂毒肽融入磷脂酰胆碱双层膜的研究:结合与构象变化研究
FEBS Lett. 1981 Nov 2;134(1):37-42. doi: 10.1016/0014-5793(81)80545-5.
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Conformational behavior of Escherichia coli OmpA signal peptides in membrane mimetic environments.大肠杆菌外膜蛋白A信号肽在膜模拟环境中的构象行为
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Membrane-bound conformation of a signal peptide: a transferred nuclear Overhauser effect analysis.信号肽的膜结合构象:转移核Overhauser效应分析
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Mechanism of exchange of cytochrome b5 between phosphatidylcholine vesicles.细胞色素b5在磷脂酰胆碱囊泡间的交换机制。
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A simple method for displaying the hydropathic character of a protein.一种展示蛋白质亲水性特征的简单方法。
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Use of resonance energy transfer to study the kinetics of amphiphile transfer between vesicles.利用共振能量转移研究两亲分子在囊泡间转移的动力学。
Biochemistry. 1982 Apr 13;21(8):1720-6. doi: 10.1021/bi00537a003.
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Suppressor mutations that restore export of a protein with a defective signal sequence.抑制突变可恢复具有缺陷信号序列的蛋白质的输出。
Cell. 1981 Jan;23(1):79-88. doi: 10.1016/0092-8674(81)90272-5.
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Assembly of proteins into membranes.蛋白质组装进入细胞膜。
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9
Partition of fatty acids and fluorescent fatty acids into membranes.
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10
Thermodynamics and kinetics of protein incorporation into membranes.蛋白质整合到膜中的热力学与动力学
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带电残基取代对大肠杆菌LamB信号序列信号肽-脂质相互作用热力学的影响。

Effect of charged residue substitutions on the thermodynamics of signal peptide-lipid interactions for the Escherichia coli LamB signal sequence.

作者信息

Jones J D, Gierasch L M

机构信息

Department of Pharmacology, University of Texas Southwestern Medical Center at Dallas 75235-9041.

出版信息

Biophys J. 1994 Oct;67(4):1546-61. doi: 10.1016/S0006-3495(94)80628-9.

DOI:10.1016/S0006-3495(94)80628-9
PMID:7819487
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1225517/
Abstract

We have used tryptophan fluorescence spectroscopy to characterize the binding affinities of an Escherichia coli LamB signal peptide family for lipid vesicles. These peptides harbor charged residue substitutions in the hydrophobic core region. Titrations of peptides with vesicles composed of 1-palmitoyl-2-oleoyl-sn-glycero-3-phosphoethanolamine and 1-palmitoyl-2-oleoyl-sn-3-phosphoglycerol (65:35 mol%), in conjunction with evaluation of peptide dissociation rates from these vesicles, were used to determine binding parameters quantitatively. We find that under low ionic strength conditions, point mutations introducing negatively charged aspartate residues substantially reduce peptide affinity relative to the wild-type peptide. However, the difference between wild-type and mutant peptide affinities was much lower under approximately physiological ionic strength. In addition, the lipid affinities of model surface-binding and transmembrane peptides were determined. These comparative studies with signal and model peptides permitted semi-quantitative deconvolution of signal peptide binding into electrostatic and hydrophobic components. We find that both interactions contribute significantly to binding, although the theoretically available hydrophobic free energy is largely offset by unfavorable polar-group effects. The implications of these results for understanding the potential roles of the signal sequence in protein translocation are discussed.

摘要

我们利用色氨酸荧光光谱法来表征大肠杆菌LamB信号肽家族与脂质囊泡的结合亲和力。这些肽在疏水核心区域存在带电残基取代。用由1-棕榈酰-2-油酰-sn-甘油-3-磷酸乙醇胺和1-棕榈酰-2-油酰-sn-3-磷酸甘油(65:35摩尔%)组成的囊泡对肽进行滴定,并结合评估肽从这些囊泡上的解离速率,用于定量确定结合参数。我们发现,在低离子强度条件下,引入带负电荷天冬氨酸残基的点突变相对于野生型肽显著降低了肽的亲和力。然而,在大约生理离子强度下,野生型和突变型肽亲和力之间的差异要低得多。此外,还测定了模型表面结合肽和跨膜肽的脂质亲和力。这些对信号肽和模型肽的比较研究允许将信号肽结合半定量地解卷积为静电和疏水成分。我们发现,尽管理论上可用的疏水自由能在很大程度上被不利的极性基团效应抵消,但这两种相互作用对结合都有显著贡献。讨论了这些结果对于理解信号序列在蛋白质转运中潜在作用的意义。