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A Novel Motif in Geminivirus Replication Proteins Interacts with the Plant Retinoblastoma-Related Protein

机译:双子病毒复制蛋白中的新型母题与植物视网膜母细胞瘤相关蛋白相互作用。

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摘要

The geminivirus replication factor AL1 interacts with the plant retinoblastoma-related protein (pRBR) to modulate host gene expression. The AL1 protein of tomato golden mosaic virus (TGMV) binds to pRBR through an 80-amino-acid region that contains two highly predicted α-helices designated 3 and 4. Earlier studies suggested that the helix 4 motif, whose amino acid sequence is strongly conserved across geminivirus replication proteins, plays a role in pRBR binding. We generated a series of alanine substitutions across helix 4 of TGMV AL1 and examined their impact on pRBR binding using yeast two-hybrid assays. These experiments showed that several helix 4 residues are essential for efficient pRBR binding, with a critical residue being a leucine at position 148 in the middle of the motif. Various amino acid substitutions at leucine-148 indicated that both structural and side chain components contribute to pRBR binding. The replication proteins of the geminiviruses tomato yellow leaf curl virus and cabbage leaf curl virus (CaLCuV) also bound to pRBR in yeast dihybrid assays. Mutation of the leucine residue in helix 4 of CaLCuV AL1 reduced binding. Together, these results suggest that helix 4 and the conserved leucine residue are part of a pRBR-binding interface in begomovirus replication proteins.
机译:双生病毒复制因子AL1与植物成视网膜细胞瘤相关蛋白(pRBR)相互作用,以调节宿主基因的表达。番茄金色花叶病毒(TGMV)的AL1蛋白通过一个80个氨基酸的区域与pRBR结合,该区域包含两个高度预测的标为3和4的α螺旋。早期的研究表明,螺旋4基序的氨基酸序列很强在双生病毒复制蛋白中保守,在pRBR结合中起作用。我们在TGMV AL1的螺旋4上生成了一系列丙氨酸取代,并使用酵母双杂交测定法检查了它们对pRBR结合的影响。这些实验表明,几个螺旋4残基对于有效的pRBR结合是必不可少的,关键残基是基序中间148位的亮氨酸。亮氨酸-148处的各种氨基酸取代表明结构和侧链成分均有助于pRBR结合。在酵母双杂交试验中,双生病毒番茄黄叶卷曲病毒和白菜叶卷曲病毒(CaLCuV)的复制蛋白也与pRBR结合。 CaLCuV AL1螺旋4中亮氨酸残基的突变降低了结合。在一起,这些结果表明螺旋4和保守的亮氨酸残基是在begomovirus复制蛋白中pRBR结合界面的一部分。

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