Fig 5. Western blotting and SDD-AGE analysis of Hrp1 and related chimera.

Western blots were used to examine expression of Hrp1. Whole cell lysates from strains DY388, DY387, DY387F, DY389, DY3242, and DY3243 were boiled in loading buffer, resolved by SDS-PAGE, transferred to nitrocellulose, and probed with anti-Hrp1 antibody, as described in Methods. Pre-stained marker proteins were run in an adjacent lane and their sizes are indicated at left. To the right are SDD-AGE assays analyzing lysates from strains bearing the indicated Hrp1-derivatives (lane 7 = DY308, lane 8 = DY3243, lane 9 = DY4500, lanes 10–12 = DY387F, lanes 13 and 14 = DY388, lane 15 and 16 = DY387F), and developed with anti-Hrp1 antibody, as described in Methods. Lanes 7–12 (all lanes are derived from the same gel and filter) show that the oligomeric forms of Hrp1CT25 (“*”) are specific for that Hrp1 derivative, and that the proteins are relatively resistant to reducing agent. Lanes 13–16 show that the oligomers (“*”) and high molecular weight (MW) forms of Hrp1 and Hrp1CT25 are relatively resistant to boiling in SDS for 5 min before electrophoresis.