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团藻中一个多聚泛素基因的重复结构与转录调控

Repetitious structure and transcription control of a polyubiquitin gene in Volvox carteri.

作者信息

Schiedlmeier B, Schmitt R

机构信息

Lehrstuhl für Genetik, Universität Regensburg, Germany.

出版信息

Curr Genet. 1994 Feb;25(2):169-77. doi: 10.1007/BF00309544.

Abstract

Southern analysis indicated the presence of at least four ubiquitin gene loci in the Volvox carteri genome. Three of these, a polyubiquitin gene described here and a non-segregating ubiquitin gene pair, were assigned to two different linkage groups by RFLP mapping; the non-polymorphic fourth gene locus remained unassigned. The polyubiquitin gene was cloned and its 2,116-bp sequence determined. It contains six exons each interrupted by an intron at Gly35, and it encodes a pentameric polyubiquitin polypeptide consisting of five runs of 76 identical amino-acid residues and a C-terminal extension of one leucine. The five tandem repeats of coding units plus introns exhibit an unusually high degree of overall sequence identity indicating an efficient process of gene homogenization in this region of the V. carteri genome. S1 mapping revealed two closely-spaced transcription starts, 24 and 28 nucleotides downstream from a putative TATA sequence. Preceding the TATA box are two 14-bp conserved heat-shock elements (HSEs) and two octameric sequences closely resembling an yesat HSE. Consistent with a 1.6-kb transcript seen on Northern blots are two polyadenylation signals (TGTAA) located 99 bp and 169 bp downstream from the TGA translational stop. The polyubiquitin gene was transcribed throughout the Volvox life cycle with peaks in the 1.6-kb mRNA levels during pre-cleavage, cleavage, and post-inversion. In contrast, an 0.6-kb monoubiquitin transcript was abundant only at the pre-cleavage stage suggesting a different type of gene control. Heat shock increased the level of polyubiquitin mRNA, whereas the level of monoubiquitin mRNA was down-regulated.

摘要

Southern印迹分析表明,在团藻(Volvox carteri)基因组中存在至少四个泛素基因位点。其中三个,即本文所述的一个多聚泛素基因和一对不分离的泛素基因,通过RFLP图谱分析被定位到两个不同的连锁群;第四个非多态性基因位点尚未定位。克隆了多聚泛素基因并测定了其2116bp的序列。它包含六个外显子,每个外显子在甘氨酸35处被一个内含子打断,编码一个五聚体多聚泛素多肽,由五个76个相同氨基酸残基的重复序列和一个C末端的亮氨酸延伸组成。编码单元加上内含子的五个串联重复序列显示出异常高的整体序列同一性,表明在团藻基因组的这个区域存在一个有效的基因同质化过程。S1图谱分析揭示了两个紧密间隔的转录起始位点,位于假定的TATA序列下游24和28个核苷酸处。在TATA框之前有两个14bp的保守热休克元件(HSEs)和两个与yesat HSE非常相似的八聚体序列。与Northern印迹上看到的1.6kb转录本一致的是,在TGA翻译终止下游99bp和169bp处有两个聚腺苷酸化信号(TGTAA)。多聚泛素基因在团藻的整个生命周期中都有转录,在卵裂前、卵裂和反转后1.6kb mRNA水平出现峰值。相比之下,一个0.6kb的单泛素转录本仅在卵裂前阶段丰富,表明存在不同类型的基因调控。热休克增加了多聚泛素mRNA的水平,而单泛素mRNA的水平则被下调。

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