Hiserodt J C, Britvan L J, Targan S R
J Immunol. 1983 Dec;131(6):2710-3.
These studies analyze the effects of various enzymes on the terminal, killer cell-independent (KCIL) stages of the human natural killer (NK) cytolytic mechanism. The addition of trypsin (T), chymotrypsin (CT), or papain (P) to standard NK reaction mixtures (PBL or LGL and K562 cells) completely ablated cytolytic activity, whereas collagenase was ineffective. Inhibition by T was reversed by preincubation with soybean trypsin inhibitor (SBTI) or fetal calf serum, indicating that the inhibition was indeed due to T. Kinetic analysis with the Ca++ pulse experiment indicated that T, CT, and P inhibited lysis well beyond the Ca++-dependent (EDTA-sensitive) stages and essentially stopped further 51Cr release at the time of addition. This observation was confirmed by the ability of T, CT, and P to block lysis during KCIL of programmed K562 targets that were detached from NK cells by EDTA and were suspended in dextran-containing media. The lysis of K562 cells by natural killer cell-derived cytotoxic factors (NKCF) was also blocked by T and CT but not by P. Inhibition of NKCF activity by T could be reversed by SBTI or fetal calf serum. The ability of T, CT, or P to inhibit the lysis of "programmed" K562 targets during KCIL indicates that the NK lethal hit is an active process mediated by protease-sensitive structures, possibly NKCF, delivered to the target cell by the NK cell during the Ca++-dependent programming steps.
这些研究分析了各种酶对人类自然杀伤(NK)细胞溶解机制中终末、非杀伤细胞依赖性(KCIL)阶段的影响。向标准NK反应混合物(外周血淋巴细胞或大颗粒淋巴细胞以及K562细胞)中添加胰蛋白酶(T)、胰凝乳蛋白酶(CT)或木瓜蛋白酶(P)可完全消除细胞溶解活性,而胶原酶则无效。用大豆胰蛋白酶抑制剂(SBTI)或胎牛血清预孵育可逆转T的抑制作用,表明这种抑制确实是由T引起的。Ca++脉冲实验的动力学分析表明,T、CT和P对裂解的抑制作用远远超出了Ca++依赖性(对EDTA敏感)阶段,并且在添加时基本上停止了进一步的51Cr释放。通过T、CT和P在KCIL期间阻断程序性K562靶细胞的裂解能力证实了这一观察结果,这些靶细胞通过EDTA与NK细胞分离并悬浮在含葡聚糖的培养基中。自然杀伤细胞衍生的细胞毒性因子(NKCF)对K562细胞的裂解也被T和CT阻断,但未被P阻断。T对NKCF活性的抑制作用可被SBTI或胎牛血清逆转。T、CT或P在KCIL期间抑制“程序性”K562靶细胞裂解的能力表明,NK致命打击是一个由蛋白酶敏感结构介导的活跃过程,可能是NKCF,在Ca++依赖性编程步骤中由NK细胞传递给靶细胞。
