PURIFICATION OF STAPHYLOCOCCUS-AUREUS BETA-TOXIN - COMPARISON OF 3 ISOELECTRIC-FOCUSING METHODS

beta-Toxin (beta-hemolysin) is one of several extracellular proteins p roduced by Staphylococcus aureus. It is a sphingomyelinase which disru pts the membranes of erythrocytes and other mammalian cells. Despite i ts characterized mechanism of action, the role of beta-toxin in human and animal disease remains unclear. In this report, we compare three g entle, rapid methods to purify enzymatically active beta-toxin. Extrac ellular proteins in S. aureus strain RN4220 cell supernatants, contain ing a high concentration of the toxin, were precipitated by ethanol, d ialyzed, and separated by preparative isoelectric focusing (IEF). We c ompared the efficiency of three preparative IEF methods: a Sephadex fl at-bed IEF using pH 3.5-10.0 Ampholine, a liquid IEF using pH 7.8-8.9 Rotolyte buffers, and a liquid IEF with two consecutive steps using pH 3.0-10.0 Bio-Lytes in the first separation followed by a second step using pH 6.0-8.0 Bio-Lytes. All three IEF methods purified milligram a mounts of enzymatically and biologically active beta-toxin. Typically, 2-5 mg of purified beta-toxin was obtained from 1.2 liters of culture medium. The total enzymatic activity recovered and overall yield were similar for all three methods. However, the single-step liquid IEF se paration using Rotolyte buffers was the most preferred method because it purified beta-toxin to >95% purity, did not require dialysis to rem ove ampholytes, and was the most rapid of the three methods. (C) 1997 Academic Press.