Arima N, Molitor J A, Smith M R, Kim J H, Daitoku Y, Greene W C
Department of Medicine, Howard Hughes Medical Institute, Duke University Medical Center, Durham, North Carolina 27710.
J Virol. 1991 Dec;65(12):6892-9. doi: 10.1128/JVI.65.12.6892-6899.1991.
The Tax protein of the human T-cell leukemia virus type I (HTLV-I) serves as a potent transcriptional activator of its own long terminal repeat as well as select cellular genes, including interleukin-2 and the alpha subunit of the interleukin-2 receptor. Tax activation of these two growth-related genes appears to involve the induced nuclear expression of DNA-binding proteins that specifically engage related kappa B enhancer elements present in the 5' regulatory regions of these genes. In human T cells, kappa B enhancer-binding activity has been discerned as an unexpectedly large family of UV cross-linked nucleoprotein adducts, termed p50, p55, p75, and p85. The protein components of each of these DNA-protein adducts have been shown to share structural similarity with the v-rel oncogene product. The p55 adduct is composed of the 50-kDa subunit of NF-kappa B derived from a 105-kDa precursor polypeptide, while the p50 adduct contains a smaller protein that is closely related to NF-kappa B p50. The p75 adduct contains the 65-kDa subunit of NF-kappa B, while the p85 adduct is composed of the human c-rel proto-oncogene product. We now demonstrate that HTLV-I Tax, in the absence of other viral pX gene products, is capable of inducing the nuclear expression of all four of these kappa B-binding proteins in human T cells, with most marked effects involving c-Rel and NF-kappa B p65. Tax induction of the nuclear expression of c-Rel and NF-kappa B p50 is regulated, at least in part, at a pretranslational level involving increases in c-rel and NF-kappa B p105 mRNA expression. To study the pattern of expression of these kappa B-specific proteins in cells infected with the whole HTLV-I, seven cloned HTLV-I-infected T-cell lines were established from the peripheral blood of patients with adult T-cell leukemia. Of note, only three of these seven cell lines produced Tax, and c-rel mRNA and nuclear protein expression was confined to these three cell lines. In contrast, NF-kappa B p50 and NF-kappa B p65 were constitutively expressed in the nuclei of all seven of the HTLV-I-infected cell lines, even in the absence of detectable Tax or other viral gene expression. These findings raise the possibility of an alternate, Tax-independent pathway for the induced nuclear expression of NF-kappa B p50 and NF-kappa B p65 following HTLV-I infection.
人类嗜T细胞病毒I型(HTLV-I)的Tax蛋白可作为其自身长末端重复序列以及特定细胞基因(包括白细胞介素-2和白细胞介素-2受体的α亚基)的强效转录激活剂。Tax对这两个与生长相关基因的激活似乎涉及诱导DNA结合蛋白的核表达,这些蛋白特异性结合这些基因5'调控区中存在的相关κB增强子元件。在人类T细胞中,κB增强子结合活性已被识别为一个意外庞大的紫外线交联核蛋白加合物家族,称为p50、p55、p75和p85。已证明这些DNA-蛋白质加合物中每一个的蛋白质成分与v-rel癌基因产物具有结构相似性。p55加合物由源自105 kDa前体多肽的NF-κB 50 kDa亚基组成,而p50加合物包含一种与NF-κB p50密切相关的较小蛋白质。p75加合物包含NF-κB 65 kDa亚基,而p85加合物由人类c-rel原癌基因产物组成。我们现在证明,在没有其他病毒pX基因产物的情况下,HTLV-I Tax能够诱导人类T细胞中所有这四种κB结合蛋白的核表达,其中对c-Rel和NF-κB p65的影响最为显著。Tax对c-Rel和NF-κB p50核表达的诱导至少部分在翻译前水平受到调控,涉及c-rel和NF-κB p105 mRNA表达的增加。为了研究在感染完整HTLV-I的细胞中这些κB特异性蛋白的表达模式,从成人T细胞白血病患者的外周血中建立了七个克隆的HTLV-I感染T细胞系。值得注意的是,这七个细胞系中只有三个产生Tax,并且c-rel mRNA和核蛋白表达仅限于这三个细胞系。相反
