Baier-Bitterlich G, Uberall F, Bauer B, Fresser F, Wachter H, Grunicke H, Utermann G, Altman A, Baier G
Institute for Medical Chemistry and Biochemistry, University of Innsbruck, Austria.
Mol Cell Biol. 1996 Apr;16(4):1842-50. doi: 10.1128/MCB.16.4.1842.
T-lymphocyte stimulation requires activation of several protein kinases, including the major phorbol ester receptor protein kinase C (PKC), ultimately leading to induction of lymphokines, such as interleukin-2 (IL-2). The revelant PKC isoforms which are involved in the activation cascades of nuclear transcription factors involved in IL-2 production have not yet been clearly defined. We have examined the potential role of two representative PKC isoforms in the induction of the IL-2 gene, i.e., PKC-alpha and PKC-theta, the latter being expressed predominantly in hematopoietic cell lines, particularly T cells. Similar to that of PKC-alpha, PKC-theta overexpression in murine EL4 thymoma cells caused a significant increase in phorbol 12-myristate 13-acetate (PMA)-induced transcriptional activation of full-length IL-2-chloramphenicol acetyltransferase (CAT) and NF-AT-CAT but not of NF-IL2A-CAT or NF-kappaB promoter-CAT reporter gene constructs. Importantly, the critical AP-1 enhancer element was differentially modulated by these two distinct PKC isoenzymes, since only PKC-theta but not PKC-alpha overexpression resulted in an approximately 2.8-fold increase in AP-1-collagenase promoter CAT expression in comparison with the vector control. Deletion of the AP-1 enhancer site in the collagenase promoter rendered it unresponsive to PKC-theta. Expression of a constitutively active mutant PKC-theta A148E (but not PKC-alpha A25E) was sufficient to induce activation of AP-1 transcription factor complex in the absence of PMA stimulation. Conversely, a catalytically inactive PKC-theta K409R (but not PKC-alpha K368R) mutant abrogated endogenous PMA-mediated activation of AP-1 transcriptional complex. Dominant negative mutant Ha-RasS17N completely inhibited the PKC-O A148E-induced signal, PKC-O. Expression of a constitutively active mutant PKC-O A148E (but not PKC-alpha A25E) was sufficient to induce activation of AP-1 transcription factor complex in the absence of PMA stimulation. Conversely, a catalytically inactive PKC-O K409R (but not PKC-alpha K368R) mutant abrogated endogenous PMA-mediated activation of AP-1 transcriptional complex. Dominant negative mutant Ha-enRasS17N completely inhibited in the PKC-O A148E-induced signal, identifying PKC-theta as a specific constituent upstream of or parallel to Ras in the signaling cascade leading to AP transcriptional activation.
T淋巴细胞的刺激需要多种蛋白激酶的激活,包括主要的佛波酯受体蛋白激酶C(PKC),最终导致淋巴因子如白细胞介素-2(IL-2)的诱导。尚未明确参与IL-2产生的核转录因子激活级联反应的相关PKC亚型。我们研究了两种代表性的PKC亚型,即PKC-α和PKC-θ在IL-2基因诱导中的潜在作用,后者主要在造血细胞系特别是T细胞中表达。与PKC-α类似,在小鼠EL4胸腺瘤细胞中过表达PKC-θ导致佛波醇12-肉豆蔻酸酯13-乙酸酯(PMA)诱导的全长IL-2-氯霉素乙酰转移酶(CAT)和NF-AT-CAT的转录激活显著增加,但对NF-IL2A-CAT或NF-κB启动子-CAT报告基因构建体没有影响。重要的是,关键的AP-1增强子元件受到这两种不同的PKC同工酶的差异调节,因为只有PKC-θ过表达而非PKC-α过表达导致与载体对照相比,AP-1-胶原酶启动子CAT表达增加约2.8倍。胶原酶启动子中AP-1增强子位点的缺失使其对PKC-θ无反应。组成型活性突变体PKC-θ A148E(而非PKC-α A25E)的表达足以在无PMA刺激的情况下诱导AP-1转录因子复合物的激活。相反,催化无活性的PKC-θ K409R(而非PKC-α K368R)突变体消除了内源性PMA介导的AP-1转录复合物的激活。显性负性突变体Ha-RasS17N完全抑制了PKC-θ A148E诱导的信号,PKC-θ。组成型活性突变体PKC-θ A148E(而非PKC-α A25E)的表达足以在无PMA刺激的情况下诱导AP-1转录因子复合物的激活。相反,催化无活性的PKC-θ K409R(而非PKC-α K368R)突变体消除了内源性PMA介导的AP-1转录复合物的激活。显性负性突变体Ha-enRasS17N完全抑制了PKC-θ A148E诱导的信号,确定PKC-θ是在导致AP转录激活的信号级联中Ras上游或与其平行的特定成分。
