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HTLV-I Tax self-association in optimal trans-activation function.

机译:HTLV-I在最佳反式激活功能中赋税自缔合。

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摘要

HTLV-I Tax protein is a potent transcriptional activator of viral and cellular genes. Tax does not bind DNA directly but interacts through protein-protein contact with host cell factors that recognize the viral long terminal repeat (LTR). Domains within Tax needed for protein-protein interaction have not been fully characterized. In studying transcriptional function in yeast cells, we unexpectedly found that Tax functions optimally not as a monomer, but as a homodimer. Here we have used the one hybrid and two hybrid genetic approaches in yeast to investigate the region(s) within Tax necessary for self-association. Dimer formation was also confirmed biochemically by using electrophoretic mobility shift (EMSA) and supershift assays. Twenty two Tax point mutants were utilized to map relevant residues. Genetic results from this series of mutants revealed that a necessary region for dimerization is contained within a previously characterized zinc finger domain. Two loss-of-function Tax mutants, each poorly active when assayed individually, were found to have complementing activity when co-expressed together. This genetic complementation suggests a mechanism fortrans-activation resulting from simultaneous but non-identical contact with a responsive target by each of two Tax monomers in a dimer.
机译:HTLV-I Tax蛋白是病毒和细胞基因的有效转录激活因子。税收不直接结合DNA,而是通过蛋白质与识别病毒长末端重复序列(LTR)的宿主细胞因子相互作用而相互作用。蛋白质-蛋白质相互作用所需的Tax内的域尚未完全表征。在研究酵母细胞中的转录功能时,我们意外地发现,Tax的最佳功能不是作为单体,而是作为同型二聚体。在这里,我们已经在酵母中使用了一种杂交和两种杂交遗传方法来研究自我结合所必需的Tax区域。二聚体的形成还通过使用电泳迁移率迁移(EMSA)和超迁移测定法在生物化学上得到证实。利用二十二个Taxpoint突变体绘制相关残基。该系列突变体的遗传结果表明,二聚化的必要区域包含在先前表征的锌指结构域中。发现两个功能丧失的Tax突变体,当分别进行测定时,每个活性较差,当共同表达时,它们具有互补活性。这种遗传互补暗示了反式激活的机制,这是由于二聚体中的两个Tax单体中的每一个与反应性靶标同时但不完全接触而导致的。

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