Fig. 6
PilG and DprA immunoblots. MC58 wt and ΔdprA mutant overnight cultures were harvested in 1× PBS and heat inactivated at 600C for 30 min. The cells were disrupted using MagNa Lyser (6× 90s at a speed of 6000 rpm). The cell lysates were prepared in Laemmli sample buffer and SDS-PAGE was run. The proteins transferred onto PVDF membrane. The membranes were incubated with ati-PilG (a) and ati-DprA (b) rabbit polyclonal primary antibodies, and anti-rabbit-IgG-horseradish peroxidase conjugate secondary antibody. The immunoblots were developed with Immun-Star WesternC Chemiluminescent kit (Bio-Rad) and visualized using a ChemiDoc Touch imager (Bio-Rad). Results were analysed using the Image Lab software (Bio-Rad)