双功能 TaqII 限制性内切酶:重新定义原型 DNA 识别位点,并建立部分切割的保真度指数。
Bifunctional TaqII restriction endonuclease: redefining the prototype DNA recognition site and establishing the Fidelity Index for partial cleaving.
机构信息
Institute for Environmental and Human Health Protection, Department of Chemistry University of Gdańsk, Gdańsk, Poland.
出版信息
BMC Biochem. 2011 Dec 5;12:62. doi: 10.1186/1471-2091-12-62.
BACKGROUND
The TaqII enzyme is a member of the Thermus sp. enzyme family that we propounded previously within Type IIS restriction endonucleases, containing related thermophilic bifunctional endonucleases-methyltransferases from various Thermus sp.: TaqII, Tth111II, TthHB27I, TspGWI, TspDTI and TsoI. These enzymes show significant nucleotide and amino acid sequence similarities, a rare phenomenon among restriction endonucleases, along with similarities in biochemical properties, molecular size, DNA recognition sequences and cleavage sites. They also feature some characteristics of Types I and III.
RESULTS
Barker et al. reported the Type IIS/IIC restriction endonuclease TaqII as recognizing two distinct cognate site variants (5'-GACCGA-3' and 5'-CACCCA-3') while cleaving 11/9 nucleotides downstream. We used four independent methods, namely, shotgun cloning and sequencing, restriction pattern analysis, digestion of particular custom substrates and GeneScan analysis, to demonstrate that the recombinant enzyme recognizes only 5'-GACCGA-3' sites and cleaves 11/9 nucleotides downstream. We did not observe any 5'-CACCCA-3' cleavage under a variety of conditions and site arrangements tested. We also characterized the enzyme biochemically and established new digestion conditions optimal for practical enzyme applications. Finally, we developed and propose a new version of the Fidelity Index - the Fidelity Index for Partial Cleavage (FI-PC).
CONCLUSIONS
The DNA recognition sequence of the bifunctional prototype TaqII endonuclease-methyltransferase from Thermus aquaticus has been redefined as recognizing only 5'-GACCGA-3' cognate sites. The reaction conditions (pH and salt concentrations) were designed either to minimize (pH = 8.0 and 10 mM ammonium sulphate) or to enhance star activity (pH = 6.0 and no salt). Redefinition of the recognition site and reaction conditions makes this prototype endonuclease a useful tool for DNA manipulation; as yet, this enzyme has no practical applications. The extension of the Fidelity Index will be helpful for DNA manipulation with enzymes only partially cleaving DNA.
背景
TaqII 酶是我们之前在 II 型限制内切酶中提出的 Thermus sp. 酶家族的成员,它包含来自不同 Thermus sp. 的相关嗜热双功能内切酶-甲基转移酶:TaqII、Tth111II、TthHB27I、TspGWI、TspDTI 和 TsoI。这些酶在核苷酸和氨基酸序列上具有显著的相似性,这在限制内切酶中是罕见的现象,同时在生化特性、分子大小、DNA 识别序列和切割位点上也具有相似性。它们还具有 I 型和 III 型的一些特征。
结果
Barker 等人报道 II 型/IIC 限制内切酶 TaqII 识别两种不同的同源识别位点变体(5'-GACCGA-3'和 5'-CACCCA-3'),同时在下游切割 11/9 个核苷酸。我们使用了四种独立的方法,即鸟枪法克隆和测序、限制图谱分析、特定定制底物的消化和 GeneScan 分析,证明重组酶仅识别 5'-GACCGA-3'位点,并在下游切割 11/9 个核苷酸。在测试的各种条件和位点排列下,我们都没有观察到任何 5'-CACCCA-3'的切割。我们还对该酶进行了生化特性分析,并建立了新的酶切条件,以优化其实用性。最后,我们开发并提出了一个新的保真度指数版本-部分切割保真度指数(FI-PC)。
结论
来自水生栖热菌的双功能原型 TaqII 内切酶-甲基转移酶的 DNA 识别序列已被重新定义为仅识别 5'-GACCGA-3'同源位点。反应条件(pH 和盐浓度)被设计为最小化(pH=8.0 和 10 mM 硫酸铵)或增强星活性(pH=6.0 和无盐)。识别位点和反应条件的重新定义使这种原型内切酶成为 DNA 操作的有用工具;到目前为止,这种酶还没有实际应用。保真度指数的扩展将有助于仅部分切割 DNA 的酶进行 DNA 操作。
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