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来自两种酵母的VDE归巢内切酶中不同DNA识别特异性的进化

Evolution of divergent DNA recognition specificities in VDE homing endonucleases from two yeast species.

作者信息

Posey Karen L, Koufopanou Vassiliki, Burt Austin, Gimble Frederick S

机构信息

Center for Genome Research, Institute of Biosciences and Technology, Texas A&M University System Health Science Center, 2121 W. Holcombe Blvd, Houston, TX 77030, USA.

出版信息

Nucleic Acids Res. 2004 Jul 27;32(13):3947-56. doi: 10.1093/nar/gkh734. Print 2004.

Abstract

Homing endonuclease genes (HEGs) are mobile DNA elements that are thought to confer no benefit to their host. They encode site-specific DNA endonucleases that perpetuate the element within a species population by homing and disseminate it between species by horizontal transfer. Several yeast species contain the VMA1 HEG that encodes the intein-associated VMA1-derived endonuclease (VDE). The evolutionary state of VDEs from 12 species was assessed by assaying their endonuclease activities. Only two enzymes are active, PI-ZbaI from Zygosaccharomyces bailii and PI-ScaI from Saccharomyces cariocanus. PI-ZbaI cleaves the Z.bailii recognition sequence significantly faster than the Saccharomyces cerevisiae site, which differs at six nucleotide positions. A mutational analysis indicates that PI-ZbaI cleaves the S.cerevisiae substrate poorly due to the absence of a contact that is analogous to one made in PI-SceI between Gln-55 and nucleotides +9/+10. PI-ZbaI cleaves the Z.bailii substrate primarily due to a single base-pair substitution (A/T+5 --> T/A+5). Structural modeling of the PI-ZbaI/DNA complex suggests that Arg-331, which is absent in PI-SceI, contacts T/A+5, and the reduced activity observed in a PI-ZbaI R331A mutant provides evidence for this interaction. These data illustrate that homing endonucleases evolve altered specificity as they adapt to recognize alternative target sites.

摘要

归巢内切核酸酶基因(HEGs)是一种可移动的DNA元件,人们认为它对其宿主没有益处。它们编码位点特异性DNA内切核酸酶,通过归巢在物种群体中使该元件永久存在,并通过水平转移在物种间传播。几种酵母物种含有编码内含肽相关的VMA1衍生内切核酸酶(VDE)的VMA1 HEG。通过检测12种物种的VDE的内切核酸酶活性来评估其进化状态。只有两种酶具有活性,即来自拜耳接合酵母的PI-ZbaI和来自卡氏酵母的PI-ScaI。PI-ZbaI切割拜耳接合酵母识别序列的速度明显快于酿酒酵母的位点,后者在六个核苷酸位置上有所不同。突变分析表明,由于缺少类似于PI-SceI中Gln-55与核苷酸+9/+10之间形成的接触,PI-ZbaI对酿酒酵母底物的切割效果很差。PI-ZbaI切割拜耳接合酵母底物主要是由于单个碱基对的替换(A/T+5 --> T/A+5)。PI-ZbaI/DNA复合物的结构模型表明,PI-SceI中不存在的Arg-331与T/A+5接触,并且在PI-ZbaI R331A突变体中观察到的活性降低为这种相互作用提供了证据。这些数据表明,归巢内切核酸酶在适应识别替代靶位点时会进化出改变的特异性。

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