Overexpression of CsgG restores curli fiber formation to the csgE mutant.
(A) The following strains were grown on YESCA-Congo red agar for 48 hrs at 26°C: wild type (WT, MC4100); csgE (MHR480); csgE/v (MHR480/pLR1); csgE/pE (MHR480/pLR70); csgE/pF (MHR480/pLR73); csgE/pG (MHR480/pLR93); csgE/v⁺ (MHR480/pTrc99a); csgE/pE⁺ (MHR480/pLR71); csgE/pF⁺ (MHR480/pLR74); csgE/pG⁺ (MHR480/pMC1). ⁺ indicates an overexpression vector.
(B) Negative stain electron micrographs of strains csgE/v (MHR480/pLR1), csgE/pE (MHR480/pLR70), csgE/pE⁺ (MHR480/pLR71) and csgE/pG⁺ (MHR480/pMC1) after 48 hrs of growth on YESCA agar at 26°C. Scale bars = 0.5 μm.
(C) Western blot analysis of the same strains as in panel A. Whole cells were collected from YESCA agar after 48 hrs of growth at 26°C, treated with formic acid and analyzed for the presence of CsgA, CsgB, CsgF and CsgG.

Effect of CsgE on erythromycin sensitivity conferred by the overexpression of CsgG. LSR11 (MC4100Δcsg) overexpressing CsgG from pMC1 along with an empty vector (pBAD33, open circles), CsgE (pLR42, filled squares), or CsgF (pLR58, filled triangles) were grown in LB shaking cultures at 37°C with 30 μg/ml erthromycin added 30 min after plasmid induction, and then measured by OD₆₀₀ at ~40 min intervals.

Effects of CsgE on the CsgG-dependent secretion of PapD2 and A22-PapD2.
(A) A schematic diagram of the PapD2 and A22-PapD2 constructs used in the secretion assays. PapD2 consists of the 21 amino acid sec-dependent signal sequence of PapD (ss^D) fused to domain 2 of PapD with a C-terminal 6-his tag; domain 2 is the C-terminal 93 amino acids of PapD encompassing the second domain of this 2-domain chaperone. A22-PapD2 consists of the PapD signal sequence (ss^D), the N-terminal 22 amino acids of mature CsgA (A22), domain 2 of PapD and a C-terminal 6-his tag. The carat indicates the sec cleavage site.
(B-C) CsgG-dependent protein secretion assay: cells were grown in LB shaking cultures at 37°C to OD₆₀₀~0.8, protein expression induced for 1 hr, then whole cell and supernatant (or concentrated supernatant) fractions were subjected to Western blot analysis using PapD-specific antisera. < corresponds to the predicted size of ss^D-A22-PapD2 (i.e., prior to sec signal cleavage); * indicates a non-specific background band.
(B) The bacterial strain LSR11 (MC4100Δcsg) expressing PapD2 (lanes 1-2; pAN87) or A22-PapD2 (lanes 3-4; pAN88) and an empty vector (lanes 1 and 3; pTrc99A) or CsgG (lanes 2 and 4; pMC1).
(C) The bacterial strain LSR35 (MC4100ΔcsgEF::kan^R) expressing CsgG from the chromosome contained the following plasmids: PapD2 (lanes 5-7; pAN93) or A22-PapD2 (lanes 8-10; pAN94); and, empty vector (lanes 5 and 8; pBAD33), CsgE (lanes 6 and 9; pLR42) or CsgF (lanes 7 and 10; pLR75).
(D) Whole cell samples of the strains in panel B and C were subjected to Western blot analysis using CsgG-specific antiseria. Lane numbers correlate to those of panels B and C.

CsgE prevents self-assembly of CsgA into amyloid fibers.
(A) Freshly purified CsgA was incubated alone (top) or in the presence of CsgE in a near 1:1 molar ratio (bottom) for 24 hours before visualization with transmission electron microscopy (TEM). Scale bars equal 1 μm.
(B) Real-time monitoring of CsgA self-assembly into amyloid fibers by ThT fluorescence. 25 μM CsgA was incubated in reaction buffer containing ThT alone (open circles) or with 22.5 μM CsgE (filled diamonds). 22.5 μM CsgE was also incubated alone in ThT reaction buffer (open triangles).