Native β-barrel substrates pass through two shared intermediates during folding on the BAM complex

巴马 折叠(DSP实现) 木桶(钟表) 生物物理学 蛋白质折叠 化学 结晶学 细菌外膜 生物化学 生物 大肠杆菌 材料科学 基因 电气工程 工程类 复合材料
作者
Thiago M. A. Santos,Benjamin D. Thomson,Melissa D. Marquez,Lydia C. Pan,Tabasom H. Monfared,Daniel Kahne
出处
期刊:Proceedings of the National Academy of Sciences of the United States of America [National Academy of Sciences]
卷期号:121 (42)
标识
DOI:10.1073/pnas.2409672121
摘要

The assembly of β-barrel proteins into membranes is mediated by the evolutionarily conserved β-barrel assembly machine (BAM) complex. In Escherichia coli , BAM folds numerous substrates which vary considerably in size and shape. How BAM is able to efficiently fold such a diverse array of β-barrel substrates is not clear. Here, we develop a disulfide crosslinking method to trap native substrates in vivo as they fold on BAM. By placing a cysteine within the luminal wall of the BamA barrel as well as in the substrate β-strands, we can compare the residence time of each substrate strand within the BamA lumen. We validated this method using two defective, slow-folding substrates. We used this method to characterize stable intermediates which occur during folding of two structurally different native substrates. Strikingly, these intermediates occur during identical stages of folding for both substrates: soon after folding has begun and just before folding is completed. We suggest that these intermediates arise due to barriers to folding that are common between β-barrel substrates, and that the BAM catalyst is able to fold so many different substrates because it addresses these common challenges.

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