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Characterization and developmental expression of single-stranded telomeric DNA-binding proteins from mung bean (Vigna radiata)

机译:绿豆(Vigna radiata)单链端粒DNA结合蛋白的表征和发育表达

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We have identified and characterized protein factors from mung bean (Vigna radiata) nuclear extracts that specifically bind the single-stranded G-rich telomeric DNA repeats. Nuclear extracts were prepared from three different types of plant tissue, radicle, hypocotyl, and root, in order to examine changes in the expression patterns of telomere-binding proteins during the development of mung bean. At least three types of specific complexes (A, B, and C) were detected by gel retardation assays with synthetic telomere and nuclear extract from radicle tissue, whereas the two major faster-migrating complexes (A and B) were formed with nuclear extracts from hypocotyl and root tissues. Gel retardation assays also revealed differences in relative amount of each complex forming activity in radicle, hypocotyl, and root nuclear extracts. These data suggest that the expression of telomere-binding proteins is developmentally regulated in plants, and that the factor involved in the formation of complex C may be required during the early stages of development. The binding factors have properties of proteins and are hence designated as mung bean G-rich telomere-binding proteins (MGBP). MGBPs bind DNA substrates with three or more single-stranded TTTAGGG repeats, while none of them show binding affinity to either double-stranded or single-stranded C-rich telomeric DNA. These proteins have a lower affinity to human telomeric sequences than to plant telomeric sequences and do not exhibit a significant binding activity to Tetrahymena telomeric sequence or mutated plant telomeric sequences, indicating that their binding activities are specific to plant telomere. Furthermore, RNase treatment of the nuclear extracts did not affect the complex formation activities. This result indicates that the single-stranded telomere-binding activities may be attributed to a simple protein but not a ribonucleoprotein. The ability of MGBPs to bind specifically the single-stranded TTTAGGG repeats may suggest their in vivo functions in the chromosome ends of plants. [References: 47]
机译:我们已经从绿豆(Vigna radiata)核提取物中鉴定并表征了蛋白质因子,这些蛋白因子特异性结合了单链富含G的端粒DNA重复序列。为了检查绿豆发育过程中端粒结合蛋白表达模式的变化,从三种不同类型的植物组织(胚根,下胚轴和根)制备了核提取物。通过凝胶阻滞分析,用合成的端粒和来自胚根组织的核提取物检测到至少三种类型的特异性复合物(A,B和C),而两个主要的较快迁移的复合物(A和B)则由来自核组织的核提取物形成。下胚轴和根组织。凝胶阻滞分析还揭示了在胚根,下胚轴和根核提取物中每种复合物形成活性的相对量的差异。这些数据表明端粒结合蛋白的表达在植物中受到发育调节,并且在发育的早期阶段可能需要参与复合物C形成的因子。结合因子具有蛋白质的特性,因此被称为富含绿豆G的端粒结合蛋白(MGBP)。 MGBP用三个或更多的单链TTTAGGG重复序列结合DNA底物,而它们都没有显示出与双链或单链富含C的端粒DNA的结合亲和力。这些蛋白质对人端粒序列的亲和力比植物端粒序列的亲和力低,并且对四膜虫端粒序列或突变的植物端粒序列没有显着的结合活性,表明它们的结合活性对植物端粒具有特异性。此外,核提取物的RNase处理不影响复合物的形成活性。该结果表明,单链端粒结合活性可能归因于简单的蛋白质,而不是核糖核蛋白。 MGBPs特异性结合单链TTTAGGG重复序列的能力可能表明它们在植物染色体末端的体内功能。 [参考:47]

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