The cells were disrupted using a Fast Prep Cell Disrupter (Bio 101, Thermo electron corporation, check details Milford, USA) and centrifuged, the total RNA was extracted from the supernatant according to the manufacturer’s protocol of Qiagen RNeasy® mini kit (Qiagen Benelux B.V.). The residual contaminating Q VD Oph genomic DNA was removed by Turbo DNA-free™ kit (Ambion, Austin,
USA). mRNA was then reverse transcribed using the Fermentas first-strand cDNA synthesis kit (Fermentas GmbH, St. Leon-Rot, Germany) according to the manufacturer’s protocol. The synthesized cDNA was further analyzed using Real-Time PCR with gene-specific primers on an ABI Prism 7000 Sequence Detecting System (Applied Biosystems, Nieuwerkerk a/d lJssel, The Netherlands). Gene expression
was normalized to the expression of glucokinase (glk), amplified with primers glk F and glk R [40]. The relative hup-1 expression levels of W83 from three independent experiments were compared in duplicate to those of the epsC mutant. Conjugation of P. gingivalis To complement the epsC mutant, plasmid pT-PG0120 was transferred into the mutant by conjugation following a protocol described earlier [41], with slight modifications. For selection of P. gingivalis after the over-night conjugation we used 50 μg/ml of gentamycin in our blood agar plates instead of 150 μg/ml. Integrity of the trans-conjugants was confirmed by colony PCR and plasmid isolation combined with restriction analysis using a plasmid isolation kit (Qiagen Benelux B.V.). Percoll density gradient centrifugation Percoll density gradients were in principle prepared as described by Patrick selleck compound and Reid [24]. In short, a 9:1 stock solution of Percoll (Pharmacia, Biotech AB, Uppsala, Sweden) was prepared with 1.5 M NaCl. Solutions containing 80, 70, why 60, 50, 40, 30, 20 and 10% Percoll in 0.15 NaCl were prepared from the stock. In an open top 14 ml polycarbonate tube (Kontron instruments, Milan, Italy) 1.5 ml of each of the solutions was carefully layered on top of the previous starting with 80%. 1 ml of an anaerobically grown over night culture of wild type and the epsC mutant concentrated to an OD690 of
4 in PBS was added to the top of the 10% layer and centrifuged for one hour at 8000 × g at 20°C in a Centrikon TST 41.14 rotor (Kontron instruments, Milan, Italy) using a Centrikon T-1170 (Kontron instruments, Milan, Italy) centrifuge. Hydrophobicty of P. gingivalis W83, the epsC mutant and the complemented mutant were grown 18 hours in BHI+H/M. The bacteria were washed twice in PBS after which the OD600 was set to 0.5. After addition of 150 μl n-hexadecane to 3 ml of this suspension the mix was vortexed 30 seconds, rested for 5 seconds and vortexed for 25 seconds. After exactly 10 minutes incubation at room temperature a sample was taken to measure the OD600 of the aqueous phase. The percentage of bacteria adhered to hexadecane was calculated by the formula: (OD600 before-OD600 after)/OD600 before × 100%.