Xylem fluid without the bacteria and the bacteria inoculated in PD3 broth or sterile water was used as a control. All tubes were covered with a black cardboard box. The bacterial cell concentration in the U0126 solubility dmso tubes was determined by measuring the OD600 nm at 10 and 20 days after culture. The cells in the tubes were dispersed by repeated pipetting and vortexing. For cell aggregation analysis, the cell concentration in the tubes was measured by determining

the OD540 nm (ODt). The tubes were then kept without shaking for 1 h to allow bacterial cells to clump and settle. The OD540 nm of supernatants of the tubes (ODs) was measured again. The relative percentage of cell aggregation was measured using the following formula: % aggregated cells=(ODt−ODs)/(ODt) × 100 (Burdman et al., 2000). Clumped cells in the bottom of the tubes were photographed at 20 days. Cells from the tubes were cultured on PD3 medium plates and incubated at 28 °C for 10–20 days to determine the growth of the cells. At 20 days, the cells were collected from the plates and confirmed to be X. fastidiosa using primer-specific PCR (Minsavage et al., 1994). This procedure was repeated three times after the initial incubation. For measurements of biofilm formation, X. fastidiosa cells were first cultured in PD3 broth and incubated at 28 °C without shaking for 4–6 days. The bacterial cells were learn more then collected, rinsed,

and adjusted in the

xylem fluid of grapefruit, lemon, orange, and grapevine, respectively, to an OD600 nm of 0.05. One hundred fifty microliter aliquots of each cell suspension were added to 96-well microtiter plates, respectively. The negative control consisted of xylem fluid or PD3 without bacteria. Plates were incubated at 28 °C without shaking. At 10 and 20 days after incubation, biofilm formation on the wall of the wells was determined using a crystal violet staining method (Leite et al., 2004). Each treatment had three replications, and the resulting data were averaged. DNA macroarray membranes were prepared with 111 selected genes with putative roles in X. fastidiosa virulence, as well as others involved in the metabolism of nucleic acids and proteins, and cellular transport and stress tolerance, based on the genome sequences of X. fastidiosa Abiraterone solubility dmso 9a5c (a CVC strain) (Simpson et al., 2000) and X. fastidiosa Temecula1 (a PD strain) (Van Sluys et al., 2003). Several unknown function genes that up- and down-induced in xylem fluid from grapevine were also included (Bi et al., 2007; Shi et al., 2008). DNA fragments (average 600 bp) of the ORF of the 111 genes were individually amplified by specific PCR from the genomic DNA of X. fastidiosa Temecula1, purified, and spotted onto nylon membranes (Hybond, Amersham Pharmacia Biotech Inc., NJ) using a manual 384-pin replicator (V&P Scientific Inc., CA). Spotted DNA was denatured with 0.