Quorum Sensing

16. Dialyze the ligation mix on a 0.025μm filter paper against
    sterile water for 30 min and transform into electrocompetent
    XL1-Blue cells.


17. Cells recovered from transformation are plated on LB agar
    plates containing 100μg/mL ampicillin. Pick single colonies
    from transformation plates and plasmid DNA prepared by
    routine technique and digest with NcoI–NotI enzymes to
    check the presence of correct sized insert (~750 bp) by gel
    electrophoresis. Check the insert by sequencing using primers
    AH18REV and HuCκFOR.


18. Small scale prokaryotic expression of scAb fragments. Single
    colonies of positive clones selected instep 17are inoculated
    into 5 mL of LB medium containing 1% (wt/vol) glucose,
    50 μg/mL ampicillin, and 12.5μg/mL tetracycline, and incu-
    bated overnight at 37C with shaking.


19. The overnight cultures from step 18 are centrifuged at
    2000
    gfor 10 min and the cell pellets resuspended in 5 mL
    of fresh LB containing 100μg/mL ampicillin and 12.5μg/mL
    tetracycline, and grown at 25C with shaking for 1 h.


20. Protein expression is induced by adding IPTG to a final con-
    centration of 1 mM. After IPTG addition, cells are grown for
    further for 4 h and further processed as described instep 25.


21. Medium scale prokaryotic expression of scAb fragments. Inoc-
    ulate 0.5 mL of overnight cultures of single positive clones
    selected instep 17in 50 mL of TB medium containing potas-
    sium phosphate buffer, 100μg/mL ampicillin, 12.5μg/mL
    tetracycline, and 1% (wt/vol) glucose in 250 mL conical flasks.
    Grow the cultures for 7–8 h at 37C with shaking.


22. Centrifuge the cultures fromstep 21at 2000
    gfor 15 min.
    Resuspend the cell pellets in fresh TB medium as above and
    incubate overnight at 30C with shaking.


23. The following day, collect the pellets by centrifuging at
    2000
    g for 20 min and resuspend in fresh TB medium
    containing potassium phosphate buffer and 100μg/mL ampi-
    cillin by vortexing.


24. Recover cells for 1 h at 25C with shaking and then induce
    with IPTG as described instep 20.


25. Periplasmic release of expressed scAbs. After IPTG induction,
    cultures fromsteps 20and 24 are centrifuged at 4000
    gfor
    20 min, and the cell pellets resuspended in 1/10 of the original
    culture volume of Fractionation buffer. Incubate on ice for
    15 min with gentle shaking. To this suspension, add 1/10 of
    the original culture volume of ice cold 5 mM MgSO 4 and
    incubate 15 min on ice. Centrifuge at 4000
    gfor 20 min,

Monoclonal Antibodies Inactivating AHL Signal Molecules 349