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首页> 外文期刊>Applied and Environmental Microbiology >Characterization of an Extremely Thermostable Restriction Enzyme, PspGI, from a PyrococcusStrain and Cloning of the PspGI Restriction-Modification System in Escherichia coli
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Characterization of an Extremely Thermostable Restriction Enzyme, PspGI, from a PyrococcusStrain and Cloning of the PspGI Restriction-Modification System in Escherichia coli

机译:从热球菌菌株的极端热限制酶PspGI的表征和大肠杆菌中PspGI限制-修饰系统的克隆。

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An extremely thermostable restriction endonuclease,PspGI, was purified from Pyrococcus sp. strain GI-H. PspGI is an isoschizomer of EcoRII and cleaves DNA before the first C in the sequence 5′ ^CCWGG 3′ (W is A or T). PspGI digestion can be carried out at 65 to 85°C. To express PspGI at high levels, the PspGI restriction-modification genes (pspGIR andpspGIM) were cloned in Escherichia coli. M.PspGI contains the conserved sequence motifs of α-aminomethyltransferases; therefore, it must be an N4-cytosine methylase. M.PspGI shows 53% similarity to (44% identity with) its isoschizomer, M.MvaI fromMicrococcus variabilis. In a segment of 87 amino acid residues, PspGI shows significant sequence similarity toEcoRII and to regions of SsoII andStyD4I which have a closely related recognition sequence (5′ ^CCNGG 3′). PspGI was expressed in E. coli via a T7 expression system. Recombinant PspGI was purified to near homogeneity and had a half-life of 2 h at 95°C. PspGI remained active following 30 cycles of thermocycling; thus, it can be used in DNA-based diagnostic applications.
机译:极热稳定的限制性核酸内切酶PspGI是从火球菌中纯化得到的。菌株GI-H。 PspGI是EcoRII的同分异构体,并且在序列5'^ CCWGG 3'(W是A或T)中的第一个C之前切割DNA。 PspGI消化可以在65至85℃下进行。为了高水平表达PspGI,将PspGI限制性修饰基因(pspGIR和pspGIM)克隆到大肠杆菌中。 M.PspGI含有α-氨基甲基转移酶的保守序列基序;因此,它必须是N4-胞嘧啶甲基化酶。 M.PspGI与来自异球菌微球菌的M.MvaI表现出53%的相似性(与其相同性为44%)。在87个氨基酸残基的片段中,PspGI显示出与EcoRII以及与具有紧密相关的识别序列(5'^ CCNGG 3')的SsoII和StyD4I的区域显着的序列相似性。 PspGI通过T7表达系统在大肠杆菌中表达。重组PspGI纯化至接近均一,在95°C下的半衰期为2小时。在30个热循环后,PspGI仍然保持活性。因此,它可以用于基于DNA的诊断应用中。

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