一种与1型人类免疫缺陷病毒TAR DNA序列基序结合的新型细胞蛋白TDP-43的克隆与鉴定。
Cloning and characterization of a novel cellular protein, TDP-43, that binds to human immunodeficiency virus type 1 TAR DNA sequence motifs.
作者信息
Ou S H, Wu F, Harrich D, García-Martínez L F, Gaynor R B
机构信息
Department of Medicine, University of Texas Southwestern Medical Center at Dallas 75235, USA.
出版信息
J Virol. 1995 Jun;69(6):3584-96. doi: 10.1128/JVI.69.6.3584-3596.1995.
Human immunodeficiency virus type 1 (HIV-1) gene expression is modulated by both viral and cellular factors. A regulatory element in the HIV-1 long terminal repeat known as TAR, which extends from nucleotides -18 to +80, is critical for the activation of gene expression by the transactivator protein, Tat. RNA transcribed from TAR forms a stable stem-loop structure which serves as the binding site for both Tat and cellular factors. Although TAR RNA is critical for Tat activation, the role that TAR DNA plays in regulating HIV-1 gene expression is not clear. Several studies have demonstrated that TAR DNA can bind cellular proteins, such as UBP-1/LBP-1, which repress HIV-1 gene expression and other factors which are involved in the generation of short, nonprocessive transcripts. In an attempt to characterize additional cellular factors that bind to TAR DNA, a lambda gt11 expression cloning strategy involving the use of a portion of TAR DNA extending from -18 to +28 to probe a HeLa cDNA library was used. We identified a cDNA, designated TAR DNA-binding protein (TDP-43), which encodes a cellular factor of 43 kDa that binds specifically to pyrimidine-rich motifs in TAR. Antibody to TDP-43 was used in gel retardation assays to demonstrate that endogenous TDP-43, present in HeLa nuclear extract, also bound to TAR DNA. Although TDP-43 bound strongly to double-stranded TAR DNA via its ribonucleoprotein protein-binding motifs, it did not bind to TAR RNA extending from +1 to +80. To determine the function of TDP-43 in regulating HIV-1 gene expression, in vitro transcription analysis was performed. TDP-43 repressed in vitro transcription from the HIV-1 long terminal repeat in both the presence and absence of Tat, but it did not repress transcription from other promoters such as the adenovirus major late promoter. In addition, transfection of a vector which expressed TDP-43 resulted in the repression of gene expression from an HIV-1 provirus. These results indicate that TDP-43 is capable of modulating both in vitro and in vivo HIV-1 gene expression by either altering or blocking the assembly of transcription complexes that are capable of responding to Tat.
1型人类免疫缺陷病毒(HIV-1)的基因表达受病毒和细胞因子的共同调节。HIV-1长末端重复序列中一个名为TAR的调控元件(从核苷酸-18延伸至+80),对于反式激活蛋白Tat激活基因表达至关重要。从TAR转录而来的RNA形成一个稳定的茎环结构,它是Tat和细胞因子的结合位点。尽管TAR RNA对Tat激活至关重要,但TAR DNA在调节HIV-1基因表达中所起的作用尚不清楚。多项研究表明,TAR DNA可结合细胞蛋白,如UBP-1/LBP-1,它们可抑制HIV-1基因表达,以及其他参与短的、非持续性转录本生成的因子。为了鉴定与TAR DNA结合的其他细胞因子,采用了一种λgt11表达克隆策略,该策略使用从-18至+28的一段TAR DNA来探测HeLa细胞cDNA文库。我们鉴定出一个cDNA,命名为TAR DNA结合蛋白(TDP-43),它编码一种43 kDa的细胞因子,该因子能特异性结合TAR中富含嘧啶的基序。使用针对TDP-43的抗体进行凝胶阻滞试验,以证明HeLa细胞核提取物中存在的内源性TDP-43也能与TAR DNA结合。尽管TDP-43通过其核糖核蛋白结合基序与双链TAR DNA紧密结合,但它不与从+1至+80的TAR RNA结合。为了确定TDP-43在调节HIV-1基因表达中的功能,进行了体外转录分析。无论有无Tat,TDP-43均抑制从HIV-1长末端重复序列的体外转录,但它不抑制来自其他启动子(如腺病毒主要晚期启动子)的转录。此外,转染表达TDP-43的载体导致HIV-1前病毒的基因表达受到抑制。这些结果表明,TDP-43能够通过改变或阻断能够响应Tat的转录复合物的组装,在体外和体内调节HIV-1基因表达。
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