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A developmentally regulated deletion element with long terminal repeats has cis-acting sequences in the flanking DNA

机译:具有长末端重复序列的发育调控缺失元件在侧翼DNA中具有顺式作用序列

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Approximately 6000 specific DNA deletion events occur during development of the somatic macro-nucleus of the ciliate Tetrahymena. The eliminated Tlr1 element is 13 kb or more in length and has an 825 bp inverted repeat near the rearrangement junctions. A functional analysis of the cis-acting sequences required for Tlr1 rearrangement was performed. A construct consisting of the entire inverted repeat and several hundred base pairs of flanking DNA on each side was rearranged accurately in vivo and displayed junctional variability similar to the chromosomal Tlr1 rearrangement. Thus, 11 kb or more of internal element DNA is not required in cis for DNA rearrangement. A second construct with only 51 bp of Tetra-hymena DNA flanking the right junction underwent aberrant rearrangement. Thus, a signal for determination of the Tlr1 junction is located in the flanking DNA, 51 bp or more from the right junction. Within the Tlr1 inverted repeat are 19 bp tandem repeats. A construct with the 19mer repeat region deleted from the right half of the inverted repeat utilized normal rearrangement junctions. Thus, despite its transposon-like structure, Tlr1 is similar to other DNA rearrangements in Tetrahymena in possessing cis-acting sequences outside the deleted DNA.
机译:纤毛四膜虫的体细胞大核发育过程中发生大约6000个特定的DNA缺失事件。消除的Tlr1元件的长度为13 kb或更长,并且在重排连接附近具有825 bp的反向重复序列。对Tlr1重排所需的顺式作用序列进行了功能分析。由完整的反向重复序列和两侧各侧DNA的数百个碱基对组成的构建体在体内进行了精确重排,并显示出与染色体Tlr1重排类似的连接变异性。因此,顺式进行DNA重排不需要11kb或更多的内部元件DNA。右连接旁侧仅有四十一处子膜的第二个构建体进行了异常重排。因此,用于确定Tlr1连接的信号位于侧翼DNA中,距右连接51bp或更多。 Tlr1反向重复序列内有19 bp串联重复序列。从反向重复的右半部分缺失19mer重复区的构建体利用正常的重排连接。因此,尽管Tlr1具有类似转座子的结构,但它与四膜虫中的其他DNA重排相似,在缺失的DNA之外具有顺式作用序列。

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