Quorum Sensing

7. The plates containing young worms are washed with M9
   buffer, transferred onto NGM agar plates containing fresh
   lawns ofE. coliOP50, and incubated at 25C for the next
   3 days.


8. GrowP. aeruginosaPA14 andE. coliOP50 cultures in 5 mL of
   LB at 37C overnight, with shaking. Dilute theP. aeruginosa
   PA14 overnight culture 1:100 in 5 mL of LB containing
   600 nM anti-QS polyclonal sera or pre-immune and nonspe-
   cific antigen immunized polyclonal sera (negative control) in
   duplicate. Dilute theE. coliOP50 overnight culture 1:100 in
   5 mL LB without any antibody. An additional negative control
   consisting ofP. aeruginosaPA14 culture supplemented with
   PBS can also be included.


9. Grow bacterial cultures by shaking at 37C until A 600 0.4 is
   reached. 100μL of anti-QS polyclonal sera or control sera
   made up to 600 nM in PBS are added to the center of 3.5 cm
   NGM-EP plates in duplicates and allowed to dry.


10. Ten microliters ofP. aeruginosaPA14 orE. coliOP50 cultures
    grown up to log phase are spotted onto NGM-EP plates and
    incubated at 37C overnight.


11. The following day, another 100μL of 600 nM anti-QS poly-
    clonal sera or control sera are added on top of PA14/OP50
    cultures on NGM-EP plates and incubated at 37C for 8 h.


12. The process is repeated and the plates are incubated at 25C
    overnight.


13. The plates were treated with antibodies as before and synchro-
    nized adult worms suspended in a drop of M9 were added onto
    the center of each of the PA14 plates containing anti-QS
    polyclonal sera or control sera. As a positive control, worms
    were added onto NGM-EP plates containingE. coliOP50.


14. The number of worms in each plate is counted and plates are
    incubated at 25C for ~24 h.


15. Worm count is repeated every 12 h and dead worms are
    removed with a wire pick.


16. The plates are treated with 600 nM polyclonal sera / control
    antibodies at 12 h time intervals as before. Overall, the worms
    are monitored for 80 h.

3.3 Preparation of
Monoclonal Antibodies

1. To separate peripheral blood lymphocytes (PBLs) from sheep
   blood, PBLs are prepared from sheep blood collected 4 days
   after antigen-boost and processed within 18 h using Accuspin
   system Histopaque 1077 columns (Sigma). About 250 mL of
   production bleed in 3.2% (wt/vol) sodium citrate solution are
   used for the procedure.

Monoclonal Antibodies Inactivating AHL Signal Molecules 337