Shea T B, Beermann M L, Griffin W R, Leli U
Laboratories for Molecular Neuroscience, Mailman Research Center, McLean Hospital, Belmont, MA 02178.
FEBS Lett. 1994 Aug 22;350(2-3):223-9. doi: 10.1016/0014-5793(94)00769-1.
Proteolytic cleavage of protein kinase C (PKC) under cell-free conditions generates a co-factor independent, free catalytic subunit (PKM). However, the difficulty in visualizing PKM in intact cells has generated controversy regarding its physiological relevance. In the present study, treatment of SH-SY-5Y cells with 2-O-tetradecanoylphorbol 13-acetate resulted in complete down-regulation of PKC within 24 h without detection of PKM. By contrast, low levels of PKM were transiently detected following ionophore-mediated calcium influx under conditions which induced no detectable PKC loss. PKM was not detected during rapid cell-free degradation of partially purified SH-SY-5Y PKC alpha by purified human brain mM calpain. However, when the kinetics of PKC degradation were slowed by lowering levels of calpain, PKM was transiently detected. PKM was also only transiently observed following calpain-mediated degradation of purified rat brain PKC alpha. Densitometric analyses indicated that, once formed, PKM was degraded approximately 10 times faster than PKC. These data provide an explanation as to why PKM is difficult to observe in situ, and indicate that PKM should not be considered as an 'unregulated' kinase, since its persistence is apparently strictly regulated by proteolysis.
在无细胞条件下,蛋白激酶C(PKC)经蛋白水解切割可产生一种不依赖辅因子的游离催化亚基(PKM)。然而,在完整细胞中可视化PKM存在困难,这引发了关于其生理相关性的争议。在本研究中,用2-O-十四烷酰佛波醇13-乙酸酯处理SH-SY-5Y细胞,24小时内PKC完全下调,未检测到PKM。相比之下,在离子载体介导的钙内流后,在未检测到PKC损失的条件下短暂检测到低水平的PKM。在用纯化的人脑μ-钙蛋白酶对部分纯化的SH-SY-5Y PKCα进行快速无细胞降解过程中未检测到PKM。然而,当通过降低钙蛋白酶水平减缓PKC降解动力学时,短暂检测到了PKM。在钙蛋白酶介导的纯化大鼠脑PKCα降解后也仅短暂观察到PKM。密度分析表明,一旦形成,PKM的降解速度比PKC快约10倍。这些数据解释了为什么PKM在原位难以观察到,并表明PKM不应被视为“不受调控”的激酶,因为其持久性显然受到蛋白水解的严格调控。
