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Structure of the metal-independent restriction enzyme Bfil reveals fusion of a specific DNA-binding domain with a nonspecific nuclease

机译:不依赖金属的限制酶Bfil的结构揭示了特定DNA结合域与非特异性核酸酶的融合

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摘要

Among all restriction endonucleases known to date, Bfil is unique in cleaving DNA in the absence of metal ions. Bfil represents a different evolutionary lineage of restriction enzymes, as shown by its crystal structure at 1.9-A resolution. The protein consists of two structural domains. The N-terminal catalytic domain is similar to Nuc, an EDTA-resistant nuclease from the phospholipase D super-family. The C-terminal DNA-binding domain of Bfil exhibits a β-barrel-like structure very similar to the effector DNA-binding domain of the Mg~(2+)-dependent restriction enzyme EcoRII and to the B3-like DNA-binding domain of plant transcription factors. Bfil presumably evolved through domain fusion of a DNA-recognition element to a nonspecific nuclease akin to Nuc and elaborated a mechanism to limit DNA cleavage to a single double-strand break near the specific recognition sequence. The crystal structure suggests that the interdomain linker may act as an autoinhibitor controlling Bfil catalytic activity in the absence of a specific DNA sequence. A PSI-BLAST search identified a Bfil homologue in a Mesorhizobium sp. BNC1 bacteria strain, a plant symbiont isolated from an EDTA-rich environment.
机译:在迄今已知的所有限制性核酸内切酶中,Bfil在不存在金属离子的情况下切割DNA方面是独特的。 Bfil代表限制酶的不同进化谱系,如其在1.9-A分辨率下的晶体结构所示。该蛋白质由两个结构域组成。 N末端催化结构域类似于Nuc,Nuc是来自磷脂酶D超家族的EDTA抗性核酸酶。 Bfil的C端DNA结合结构域表现出类似于Mg〜(2+)限制性酶EcoRII的效应子DNA结合结构域以及B3样DNA结合结构域的β桶状结构。植物转录因子。据推测,Bfil通过DNA识别元件与类似于Nuc的非特异性核酸酶的结构域融合而进化,并阐述了将DNA切割限制为在特定识别序列附近的单双链断裂的机制。晶体结构表明,在不存在特定DNA序列的情况下,域间连接子可作为控制Bfil催化活性的自抑制剂。 PSI-BLAST搜索在中生根瘤菌中鉴定出Bfil同源物。 BNC1细菌菌株,一种从富含EDTA的环境中分离出来的植物共生体。

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