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首页> 外文期刊>Journal of Molecular Biology >phi29 DNA polymerase active site: role of residue Val250 as metal-dNTP complex ligand and in protein-primed initiation.
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phi29 DNA polymerase active site: role of residue Val250 as metal-dNTP complex ligand and in protein-primed initiation.

机译:phi29 DNA聚合酶活性位点:残基Val250作为金属-dNTP复合物配体并在蛋白质引发的启动作用。

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摘要

DNA polymerases require two acidic residues to coordinate metal ions A and B at their polymerisation active site during catalysis of nucleotide incorporation. Crystallographic resolution of varphi29 DNA polymerase ternary complex showed that metal B coordination also depends on the carbonyl group of Val250 that belongs to the highly conserved Dx(2)SLYP motif of eukaryotic-type (family B) DNA polymerases. In addition, multiple sequence alignments have shown the specific conservation of this residue among the DNA polymerases that use a protein as primer. Thus, to ascertain its role in polymerisation, we have analysed the behaviour of single mutations introduced at the corresponding Val250 of varphi29 DNA polymerase. The differences in nucleotide binding affinity shown by mutants V250A and V250F with respect to the wild-type DNA polymerase agree to a role for Val250 as a metal B-dNTP complex ligand. In addition, mutant V250F was severely affected in varphi29 DNA replication because of a large reduction in the catalytic efficiency of the protein-primed reactions. In the light of the varphi29 DNA polymerase structures, a role for Val250 residue in the maintenance of the proper architecture of the enzyme to perform the protein-primed reactions is also proposed.
机译:DNA聚合酶在核苷酸掺入的催化过程中需要两个酸性残基在其聚合活性位点配位金属离子A和B。 varphi29 DNA聚合酶三元复合物的晶体学解析表明,金属B的配位也取决于Val250的羰基,Val250属于真核型(家族B)DNA聚合酶的高度保守的Dx(2)SLYP主题。另外,多个序列比对已经显示了在使用蛋白质作为引物的DNA聚合酶中该残基的特异性保守性。因此,为了确定其在聚合反应中的作用,我们分析了在varphi29 DNA聚合酶的相应Val250处引入的单个突变的行为。突变体V250A和V250F相对于野生型DNA聚合酶显示的核苷酸结合亲和力差异同意Val250作为金属B-dNTP复合物配体的作用。另外,由于蛋白质引发的反应的催化效率大大降低,突变体V250F在varphi29 DNA复制中受到严重影响。根据varphi29 DNA聚合酶的结构,还提出了Val250残基在维持酶的适当结构以进行蛋白引发的反应中的作用。

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