Slides were incubated in a wet chamber in the dark at room temperature for 1 h, washed three times with PBS-FCS and once with PBS. They were then fixed a second time with 4% formaldehyde-PBS for 15 min at 4 °C, mounted in VectaShield media containing 4′-6-diamidino-2-phenylindole (DAPI) (Vector Laboratories, Burlingame, PF-562271 cell line CA), covered with
a 1-mm coverslip and sealed with nail polish. A similar protocol was used for B. burgdorferi cells that had been fixed with 50 μL of 60% methanol for 10 min, before being washed and reacted with the primary and secondary antibodies as described above. Stained cells were visualized using a Zeiss Inverted Axiovert 200 motorized microscope with a × 100 PlanApo 1.4 oil PH3 objective and Zeiss filter sets 31, 34 and 38 for AlexaFluor 594, 488 and DAPI, respectively. The pictures were taken using a Zeiss Axiocam MRM cool CCD camera and were analyzed using axiovision 4.3 software. Unabsorbed anti-rBmpA Ig had a dot immunobinding titer of 1 : 10 000 with 10 ng
of rBmpA or rBmpB and reacted minimally with rBmpC or rBmpD. After absorption with rBmpB, anti-rBmpA Ig had a titer of 1 : 100 with 1 and 10 ng selleckchem of rBmpA and did not react with similar quantities of rBmpB, rBmpC or rBmpD (Fig. 1a). Absorbed anti-rBmpA at a 1 : 100 dilution detected a single immunoreactive spot consistent with BmpA at 39 kDa, pI 5.0, in 2D-NEPHGE gels of B.
burgdorferi lysates (Fig. 1b). This dilution of this reagent was used for all subsequent immunoblotting. Fractionation of intact B. burgdorferi cells with Triton X-114 showed that both immunoreactive BmpA and FlaB were present in the detergent-insoluble fraction containing periplasmic core proteins (Fig. 2a, lanes 2), while only BmpA was present in the detergent phase of the Triton X-114-soluble fraction containing the outer-membrane proteins (Fig. 2a, lanes 4). A small amount of BmpA was also detected in the aqueous phase of the Triton X-114-soluble fraction (Fig. 2a, lanes 3). Detection of BmpA in the detergent phase of Triton X-114 fractionation is consistent with its being located in Regorafenib solubility dmso the outer membranes of B. burgdorferi (Brusca & Radolf, 1994; Skare et al., 1995). While the detection of immunoreactive BmpA in the Triton X-114-insoluble fraction might imply that some BmpA is associated with periplasmic cellular proteins and the cytoplasmic membrane, this fraction also includes intact cells with the outer membranes still attached (Crother et al., 2003). These data suggest that BmpA, unlike FlaB, is a lipoprotein, and most probably located in the outer membrane of B. burgdorferi. To provide additional data on BmpA localization, intact B. burgdorferi cells were incubated with increasing concentrations of proteinase K in the absence or presence of Triton X-100.