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The Integrase of the Conjugative Transposon Tn916 Directs Strand- and Sequence-Specific Cleavage of the Origin of Conjugal Transfer, oriT, by the Endonuclease Orf20

机译:结合转座子Tn916的整合指导核酸内切酶Orf20进行结合转移特异性oriT的链和序列特异性切割。

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摘要

Orf20 of the conjugative transposon Tn916 was purified as a chimeric protein fused to maltose binding protein (MBP-Orf20). The chimeric protein possessed endonucleolytic activity, cleaving both strands of the Tn916 origin of conjugal transfer (oriT) at several distinct sites and favoring GT dinucleotides. Incubation of the oriT DNA with purified Tn916 integrase (Int) and MBP-Orf20 resulted in strand- and sequence-specific cleavage of oriT at a TGGT motif in the transferred strand. This motif lies immediately adjacent to a sequence in oriT previously shown to be protected from DNase I cleavage by Int. The endonucleolytic cleavages produced by Orf20 generated a 3′ OH group that could be radiolabeled by dideoxy ATP and terminal transferase. The production of a 3′ OH group distinguished these Orf20-dependent cleavage events from those catalyzed by Int at the ends of Tn916. Thus, Orf20 functions as the relaxase of Tn916, nicking oriT as the first step in conjugal DNA transfer. Remarkably for a tyrosine recombinase, Tn916 Int acts as a specificity factor in the reaction, conferring both strand and sequence specificities on the endonucleolytic cleavage activity of Orf20.
机译:将结合转座子Tn916的Orf20纯化为与麦芽糖结合蛋白(MBP-Orf20)融合的嵌合蛋白。嵌合蛋白具有内切核酸酶活性,在几个不同的位点切割了Tn916接合转移的起源(oriT)的两条链,并有利于GT二核苷酸。将oriT DNA与纯化的Tn916整合酶(Int)和MBP-Orf20一起孵育,会导致oriT在转移链中的TGGT基序处发生链特异性和序列特异性切割。该基序紧邻oriT中的序列,该序列先前显示已被Int保护免于DNase I切割。 Orf20产生的内切核酸裂解产生了一个3'OH基团,该基团可以通过双脱氧ATP和末端转移酶进行放射性标记。 3'OH基团的产生将这些Orf20依赖的裂解事件与Int在Tn916末端催化的裂解事件区分开。因此,Orf20充当Tn916的松弛酶,而oriT则是接合DNA转移的第一步。对于酪氨酸重组酶,Tn916 Int在反应中起特异性因子的作用,赋予Orf20内切核酸裂解活性以链和序列特异性。

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