rel蛋白对DNA结合的pp40IκB-β差异性抑制作用
Differential pp40I kappa B-beta inhibition of DNA binding by rel proteins.
作者信息
Diehl J A, McKinsey T A, Hannink M
机构信息
Department of Biochemistry, University of Missouri-Columbia 65211.
出版信息
Mol Cell Biol. 1993 Mar;13(3):1769-78. doi: 10.1128/mcb.13.3.1769-1778.1993.
Regulation of gene expression by members of the NF-kappa B/rel transcription factor family is a central component of signal transduction pathways utilized by many cellular processes, including lymphocyte activation, embryonic development, and oncogenesis. The members of the NF-kappa B/rel transcription factor family are regulated by association with a family of inhibitor (I kappa B) proteins (I kappa B) proteins. To address the importance of the association between rel and I kappa B proteins for oncogenesis by rel proteins, we characterized rel-I kappa B interactions in chicken embryo fibroblasts (CEF) infected with retroviral vectors encoding the avian c-rel (p68c-rel), v-rel (p59v-rel), and I kappa B-beta (pp40I kappa B-beta) proteins. In these experiments, the p59v-rel:pp40I kappa B-beta ratio in coinfected CEF was nearly identical to the p59v-rel:pp40I kappa B-beta ratio in v-rel-transformed cells. The avian I kappa B-beta protein, pp40I kappa B-beta, was able to associate with both the nononcogenic p68c-rel and the oncogenic p59v-rel. Association of p68c-rel with pp40I kappa B-beta in coinfected CEF resulted in inhibition of the DNA-binding activity of p68c-rel. Anti-pp40I kappa B-beta serum was able to restore DNA binding to p68c-rel in the presence of high levels of pp40I kappa B-beta, indicating that pp40I kappa B-beta functions in a trans-acting manner to inhibit DNA binding by p68c-rel. In contrast, sequence-specific DNA binding by the oncogenic v-rel protein, p59v-rel, was not abolished by pp40I kappa B-beta in coinfected CEF. Anti-pp40I kappa B-beta serum did not immunoprecipitate the p59v-rel-DNA adduct or alter the electrophoretic mobility of the p59v-rel-DNA adduct, consistent with the idea that pp40I kappa B-beta and DNA are competitive inhibitors for the same or overlapping domains on rel proteins. Internal v-rel-derived sequences were identified that are responsible for loss of pp40I kappa B-beta-mediated inhibition of DNA binding by p59v-rel. Loss of pp40I kappa B-beta-mediated inhibition of DNA binding by recombinant v/c-rel proteins was not sufficient for oncogenic activation of c-rel. Instead, removal of C-terminal c-rel-derived sequences in addition to loss of pp40I kappa B-beta-mediated inhibition of DNA binding was required for oncogenic activation of c-rel. These results demonstrate the presence of an interaction between internal and C-terminal regions of the c-rel protein that is important for the ability of c-rel to regulate the proliferation of lymphoid cells.
NF-κB/rel转录因子家族成员对基因表达的调控是许多细胞过程(包括淋巴细胞激活、胚胎发育和肿瘤发生)所利用的信号转导途径的核心组成部分。NF-κB/rel转录因子家族成员通过与一类抑制剂(IκB)蛋白相关联而受到调控。为了探讨rel蛋白与IκB蛋白之间的关联对于rel蛋白诱导肿瘤发生的重要性,我们对感染了编码禽c-rel(p68c-rel)、v-rel(p59v-rel)和IκB-β(pp40IκB-β)蛋白的逆转录病毒载体的鸡胚成纤维细胞(CEF)中的rel-IκB相互作用进行了表征。在这些实验中,共感染的CEF中p59v-rel:pp40IκB-β的比例与v-rel转化细胞中p59v-rel:pp40IκB-β的比例几乎相同。禽IκB-β蛋白pp40IκB-β能够与非致癌性的p68c-rel和致癌性的p59v-rel都发生关联。在共感染的CEF中,p68c-rel与pp40IκB-β的关联导致p68c-rel的DNA结合活性受到抑制。在存在高水平pp40IκB-β的情况下,抗pp40IκB-β血清能够恢复p68c-rel的DNA结合能力,这表明pp40IκB-β以反式作用方式发挥功能来抑制p68c-rel的DNA结合。相比之下,在共感染的CEF中,致癌性的v-rel蛋白p59v-rel的序列特异性DNA结合并未被pp40IκB-β消除。抗pp40IκB-β血清未免疫沉淀p59v-rel-DNA加合物,也未改变p59v-rel-DNA加合物的电泳迁移率,这与pp40IκB-β和DNA是rel蛋白上相同或重叠结构域的竞争性抑制剂这一观点一致。已鉴定出v-rel内部的序列,这些序列导致pp40IκB-β介导的对p59v-rel DNA结合的抑制作用丧失。pp40IκB-β介导的对重组v/c-rel蛋白DNA结合的抑制作用丧失并不足以使c-rel发生致癌激活。相反,除了pp40IκB-β介导的对DNA结合的抑制作用丧失外,还需要去除c-rel C末端的序列,c-rel才能发生致癌激活。这些结果表明,c-rel蛋白的内部区域和C末端区域之间存在相互作用,这对于c-rel调节淋巴细胞增殖的能力很重要。
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