M Kundu, S A Ansari, L G Chepenik, R J Pomerantz, K Khalili, J Rappaport, S Amini
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STUDY DESIGN-METHODS: Using the previously established astrocytic cell line of human origin stably transfected with Tat cDNA, we analyzed the formation of a nucleoprotein complex consisting of three cellular proteins associated with TAR RNA using ultraviolet (UV) crosslinking and glutathione-S-transferase (GST) pull-down assays.</p><p><strong>Results: </strong>UV crosslinking experiments reveal that the molecular masses of the proteins range from 50 to 62 kd. Transient transfection studies demonstrate that the presence of these proteins correlates with the ability of Tat to transactivate the HIV-1 LTR in the absence of the trinucleotide bulge, a region within TAR that has been shown to be important for Tat-TAR interaction. A combination of GST pull-down assays and RNA binding studies demonstrates that the 50-kd protein interacts with both Tat and TAR and is likely to be NF-kappa B p50.</p><p><strong>Conclusions: </strong>Taken together, these data suggest that in the absence of a functional Tat binding site such as TAR (which tethers the viral protein to the RNA), cellular protein NF-kappa B p50 may be able to bring Tat into the RNA binding complex Tat has been shown to activate expression of a variety of cellular genes that may not contain a binding site for Tat but do contain binding sites for NF-kappa B family members. The results presented in this study may be relevant for Tat-mediated transactivation of cellular as well as viral genes, both of which might contribute to the central nervous system damage associated with HIV-1 infection.</p>","PeriodicalId":80032,"journal":{"name":"Journal of human virology","volume":"2 2","pages":"72-80"},"PeriodicalIF":0.0000,"publicationDate":"1999-03-01","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"","citationCount":"0","resultStr":"{\"title\":\"HIV-1 regulatory protein tat induces RNA binding proteins in central nervous system cells that associate with the viral trans-acting-response regulatory motif.\",\"authors\":\"M Kundu, S A Ansari, L G Chepenik, R J Pomerantz, K Khalili, J Rappaport, S Amini\",\"doi\":\"\",\"DOIUrl\":null,\"url\":null,\"abstract\":\"<p><strong>Objectives: </strong>To investigate some of the cellular consequences of HIV-1 Tat expression in human astrocytic cells. 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A combination of GST pull-down assays and RNA binding studies demonstrates that the 50-kd protein interacts with both Tat and TAR and is likely to be NF-kappa B p50.</p><p><strong>Conclusions: </strong>Taken together, these data suggest that in the absence of a functional Tat binding site such as TAR (which tethers the viral protein to the RNA), cellular protein NF-kappa B p50 may be able to bring Tat into the RNA binding complex Tat has been shown to activate expression of a variety of cellular genes that may not contain a binding site for Tat but do contain binding sites for NF-kappa B family members. 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引用次数: 0
摘要
目的:探讨人类星形细胞中HIV-1 Tat表达的一些细胞后果。这项研究是基于细胞因子通过其与反式作用-反应(TAR) RNA元件和上游HIV-1长末端重复(LTR)启动子结合位点的相互作用,在促进Tat转录激活中发挥关键作用的证据。研究设计-方法:利用先前建立的稳定转染Tat cDNA的人源星形细胞细胞系,我们使用紫外线(UV)交联和谷胱甘肽- s -转移酶(GST)下拉试验分析了由三种与TAR RNA相关的细胞蛋白组成的核蛋白复合物的形成。结果:紫外交联实验表明,该蛋白的分子量在50 ~ 62 kd之间。瞬时转染研究表明,这些蛋白质的存在与Tat在没有三核苷酸突起(TAR内的一个区域,已被证明对TAR -TAR相互作用很重要)的情况下反激活HIV-1 LTR的能力相关。GST下拉试验和RNA结合研究表明,50-kd蛋白与Tat和TAR相互作用,可能是NF-kappa bp50。综上所述,这些数据表明,在缺乏功能性Tat结合位点如TAR(将病毒蛋白连接到RNA上)的情况下,细胞蛋白NF-kappa B p50可能能够将Tat带入RNA结合复合体。Tat已被证明可以激活多种细胞基因的表达,这些基因可能不包含Tat的结合位点,但确实包含NF-kappa B家族成员的结合位点。这项研究的结果可能与tat介导的细胞和病毒基因的反激活有关,这两种基因都可能导致与HIV-1感染相关的中枢神经系统损伤。
HIV-1 regulatory protein tat induces RNA binding proteins in central nervous system cells that associate with the viral trans-acting-response regulatory motif.
Objectives: To investigate some of the cellular consequences of HIV-1 Tat expression in human astrocytic cells. This study is based on evidence that cellular factors play a critical role in facilitating transcriptional activation by Tat through its interaction with the trans-acting-response (TAR) RNA element and upstream HIV-1 long terminal repeat (LTR) promoter binding site. STUDY DESIGN-METHODS: Using the previously established astrocytic cell line of human origin stably transfected with Tat cDNA, we analyzed the formation of a nucleoprotein complex consisting of three cellular proteins associated with TAR RNA using ultraviolet (UV) crosslinking and glutathione-S-transferase (GST) pull-down assays.
Results: UV crosslinking experiments reveal that the molecular masses of the proteins range from 50 to 62 kd. Transient transfection studies demonstrate that the presence of these proteins correlates with the ability of Tat to transactivate the HIV-1 LTR in the absence of the trinucleotide bulge, a region within TAR that has been shown to be important for Tat-TAR interaction. A combination of GST pull-down assays and RNA binding studies demonstrates that the 50-kd protein interacts with both Tat and TAR and is likely to be NF-kappa B p50.
Conclusions: Taken together, these data suggest that in the absence of a functional Tat binding site such as TAR (which tethers the viral protein to the RNA), cellular protein NF-kappa B p50 may be able to bring Tat into the RNA binding complex Tat has been shown to activate expression of a variety of cellular genes that may not contain a binding site for Tat but do contain binding sites for NF-kappa B family members. The results presented in this study may be relevant for Tat-mediated transactivation of cellular as well as viral genes, both of which might contribute to the central nervous system damage associated with HIV-1 infection.
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