4.6 Article

Tuning Functional Amyloid Formation Through Disulfide Engineering

Journal

FRONTIERS IN MICROBIOLOGY
Volume 11, Issue -, Pages -

Publisher

FRONTIERS MEDIA SA
DOI: 10.3389/fmicb.2020.00944

Keywords

disulfide engineering; functional amyloid; CsgA; curli; protein engineering

Categories

Funding

  1. National Institutes of Health [R01 GM118651, R21 AI137535]

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Many organisms produce functional amyloid fibers, which are stable protein polymers that serve many roles in cellular biology. Certain Enterobacteriaceae assemble functional amyloid fibers called curli that are the main protein component of the biofilm extracellular matrix. CsgA is the major protein subunit of curli and will rapidly adopt the polymeric amyloid conformation in vitro. The rapid and irreversible nature of CsgA amyloid formation makes it challenging to study in vitro. Here, we engineered CsgA so that amyloid formation could be tuned to the redox state of the protein. A double cysteine variant of CsgA called CsgA(CC) was created and characterized for its ability to form amyloid. When kept under oxidizing conditions, CsgA(CC) did not adopt a beta-sheet rich structure or form detectable amyloid-like aggregates. Oxidized CsgA(CC) remained in a soluble, non-amyloid state for at least 90 days. The addition of reducing agents to CsgA(CC) resulted in amyloid formation within hours. The amyloid fibers formed by CsgA(CC) were indistinguishable from the fibers made by CsgA WT. When measured by thioflavin T fluorescence the amyloid formation by CsgA(CC) in the reduced form displayed the same lag, fast, and plateau phases as CsgA WT. Amyloid formation by CsgA(CC) could be halted by the addition of oxidizing agents. Therefore, CsgA(CC) serves as a proof-of-concept for capitalizing on the convertible nature of disulfide bonds to control the aggregation of amyloidogenic proteins.

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