the hydrophobic core of twin-arginine signal sequences orchestrates specific binding to tat-pathway related chaperonestwin-arginine信号序列的疏水核心协调相关的特定绑定tat-pathway陪伴.pdfVIP

the hydrophobic core of twin-arginine signal sequences orchestrates specific binding to tat-pathway related chaperonestwin-arginine信号序列的疏水核心协调相关的特定绑定tat-pathway陪伴.pdf

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the hydrophobic core of twin-arginine signal sequences orchestrates specific binding to tat-pathway related chaperonestwin-arginine信号序列的疏水核心协调相关的特定绑定tat-pathway陪伴

The Hydrophobic Core of Twin-Arginine Signal Sequences Orchestrates Specific Binding to Tat-Pathway Related Chaperones ¤a ¤b ¨ ¤c Anitha Shanmugham , Adil Bakayan , Petra Voller , Joost Grosveld, Holger Lill, Yves J. M. Bollen* Department of Molecular Cell Biology, VU University Amsterdam, Amsterdam, The Netherlands Abstract Redox enzyme maturation proteins (REMPs) bind pre-proteins destined for translocation across the bacterial cytoplasmic membrane via the twin-arginine translocation system and enable the enzymatic incorporation of complex cofactors. Most REMPs recognize one specific pre-protein. The recognition site usually resides in the N-terminal signal sequence. REMP binding protects signal peptides against degradation by proteases. REMPs are also believed to prevent binding of immature pre-proteins to the translocon. The main aim of this work was to better understand the interaction between REMPs and substrate signal sequences. Two REMPs were investigated: DmsD (specific for dimethylsulfoxide reductase, DmsA) and TorD (specific for trimethylamine N-oxide reductase, TorA). Green fluorescent protein (GFP) was genetically fused behind the signal sequences of TorA and DmsA. This ensures native behavior of the respective signal sequence and excludes any effects mediated by the mature domain of the pre-protein. Surface plasmon resonance analysis revealed that these chimeric pre- proteins specifically bind to the cognate REMP. Furthermore, the region of the signal sequence that is responsible for specific binding to the corresponding REMP was identified by creating region-swapped chimeric signal se

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