![Fig. 2. Purified human perforin efficiently binds to PAF. / Perforin was immunopurified from the perforin-positive YT2C2 NK-cell line using an appropriate binding gel (antiperforin 6.4-IgM, antiperforin mAb, coupled with Affi-Gel 10 gel). (A) Successful purification of perforin was controlled by a Western blot using the specific antiperforin antibody 2d4-perf. In lane C, for YT cell line extracts as positive control, the procedure revealed 2 bands at the molecular weight of 66 and 30-kd as recently reported by Uellner et al.24 Perforin was further purified by ultracentrifugation to obtain the active form of 66-kd (Uellner et al24), expressed in lane 1. No other band was detected in lanes 2, 3, 4, and 5 using, respectively, the perforin-negative Jurkat cell line lysate, the gel cross-linked to the mAb, the gel alone, or the gel with an irrelevant protein BSA instead of perforin. Active perforin was then exposed to [3H]PAF C18:0 during 30 minutes at 20°C and washed 5 times with the cold buffer as shown in “Materials and methods.” The resulting radioactivity was then measured for perforin. (B) In this assay, lane 1 shows the formation of perforin-[3H]PAF complexes expressed in disintegrations per minute. In contrast, no significant radioactivity was detected in lanes 2, 3, 4, and 5 using, respectively, the perforin-negative Jurkat cell line lysate, the gel cross-linked to the mAb, the gel alone, or the gel with an irrelevant protein BSA instead of perforin as already mentioned for Western blot analysis.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/95/7/10.1182_blood.v95.7.2329/5/bloo00734002bx.jpeg?Expires=1735832610&Signature=axY-hJkPOKnO6LX6YMiD~lyYitBHgwoCULINExMoejbAj4Ub5qSLKcbD8P7W6i3tMwUYD2HzIb9xqGIM0Ne11KN9Es0cNRSInPpaAuXYQZ8juTUXj0e57BvzwK8FbI~8VEC30rZ3ON2aTeGsNqWbIj-WTJ0RmaCrw7N23Ep04iIEprMOUHTxNlBWzqKIV5gywvU9TXr01K1Rz6dht5DZe1Un4sglefCmWxrKx-nuR6B3bxF0GAVOxk2nC4irE-1QhhOoBoBO8UTvwObtDn4nkiYh1apcFAVWpC6TRTWRn66YSxG-IInAEa-1B4vZLKzvD2T5e2P2Z7iX2W7WoJuaJw__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Purified human perforin efficiently binds to PAF.
Perforin was immunopurified from the perforin-positive YT2C2 NK-cell line using an appropriate binding gel (antiperforin 6.4-IgM, antiperforin mAb, coupled with Affi-Gel 10 gel). (A) Successful purification of perforin was controlled by a Western blot using the specific antiperforin antibody 2d4-perf. In lane C, for YT cell line extracts as positive control, the procedure revealed 2 bands at the molecular weight of 66 and 30-kd as recently reported by Uellner et al.24 Perforin was further purified by ultracentrifugation to obtain the active form of 66-kd (Uellner et al24), expressed in lane 1. No other band was detected in lanes 2, 3, 4, and 5 using, respectively, the perforin-negative Jurkat cell line lysate, the gel cross-linked to the mAb, the gel alone, or the gel with an irrelevant protein BSA instead of perforin. Active perforin was then exposed to [3H]PAF C18:0 during 30 minutes at 20°C and washed 5 times with the cold buffer as shown in “Materials and methods.” The resulting radioactivity was then measured for perforin. (B) In this assay, lane 1 shows the formation of perforin-[3H]PAF complexes expressed in disintegrations per minute. In contrast, no significant radioactivity was detected in lanes 2, 3, 4, and 5 using, respectively, the perforin-negative Jurkat cell line lysate, the gel cross-linked to the mAb, the gel alone, or the gel with an irrelevant protein BSA instead of perforin as already mentioned for Western blot analysis.
