Pre-steady-state kinetics of nucleotide insertion following 8-oxo-7,8-dihydroguanine base pair mismatches by bacteriophage T7 DNA polymerase exo

Furge LL.; Guengerich FP.

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Pre-steady-state kinetics of nucleotide insertion following 8-oxo-7,8-dihydroguanine base pair mismatches by bacteriophage T7 DNA polymerase exo

机译：噬菌体T7 DNA聚合酶外切后8-氧代7,8-二氢鸟嘌呤碱基对错配后核苷酸插入的稳态前动力学

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8-Oxx-7,8-dihydroguanine (8-oxoGua) can base pair with either cytosine (C) or adenine (A) when replicated by DNA polymerases. The 8-oxoGua.A mismatch is extended in preference to the 8-oxoGua.C pair. Using a model 25-mer/36-mer DNA duplex containing either guanine (Gua).C, 8-oxoGua.C, or 8-oxoGua.A base pairs at the primer terminus and A at the standing start position, we found that the pre-steady-state addition of dTTP opposite A following all three base pairs by bacteriophage T7 DNA polymerase exo(-) showed burst kinetics, suggesting that extension of all three base pairs is controlled by the rate of a step at or before phosphodiester bond formation, Substitution of dTTP alpha S for dTTP yielded modest thio effects of 1-6, suggesting that extension of all three pairs is limited by the rate of the conformational change prior to phosphodiester bond formation. Pre-steady-state values for k(pol) (maximum polymerization rate) were 120, 12, and 28 s(-1), and K-d values were 2, 75, and 22 mu M for insertion of dTTP following Gua.C, 8-oxoGua.C, and 8-oxoGua.A base pairs, respectively. Additional analysis of extension was provided by substitution of A in the standing start position by 2-aminopurine (2-AP), a fluorescent base analogue. Comparison of rapid-quench gel-based assays with stopped-flow fluorescence quenching assays suggested that during addition of dTTP opposite 2-AP phosphodiester bond formation was rate-limiting when 8-oxoGua.C or 8-oxoGua.A were the preceding base pairs, while conformational change was rate-limiting when Gua.C was the preceding base pair, Furthermore, the difference in apparent conformational change rates for addition of dTTP opposite 2-AP following the 8-oxoGua base pairs was greater than the differences in their phosphodiester bond formation rates, suggesting that discrimination in extension may be influenced more by conformational change rates than the rates of phosphodiester bond formation in this mispaired system. [References: 26]

机译：当DNA聚合酶复制时，8-Oxx-7,8-二氢鸟嘌呤（8-oxoGua）可以与胞嘧啶（C）或腺嘌呤（A）碱基配对。 8-oxoGua.A不匹配优先于8-oxoGua.C对扩展。使用包含鸟嘌呤（Gua）.C，8-oxoGua.C或8-oxoGua.A碱基对的20-mer / 36-mer DNA双链体模型，该碱基对位于引物末端，而A处于站立起始位置，我们发现噬菌体T7 DNA聚合酶exo（-）在所有三个碱基对之后的相对于A的dTTP的稳态前添加显示爆发动力学，这表明所有三个碱基对的延伸受磷酸二酯键或磷酸二酯键之前的步伐速率控制形成，用dTTPαS替代dTTP产生1-6的适度硫代效应，这表明所有三对的延伸都受到磷酸二酯键形成之前构象变化率的限制。在Gua.C之后插入dTTP的k（pol）（最大聚合速率）的稳态前值为120、12和28 s（-1），Kd值为2、75和22μM。 8-oxoGua.C和8-oxoGua.A碱基对。通过用荧光基团类似物2-氨基嘌呤（2-AP）代替站立起始位置的A，提供了延伸的其他分析。将基于快速猝灭凝胶的测定与停止流荧光猝灭测定的比较表明，在添加dTTP的过程中，当8-oxoGua.C或8-oxoGua.A是前面的碱基对时，相反的2-AP磷酸二酯键形成是限速的。，而当Gua.C是前面的碱基对时，构象变化是限速的;此外，在8-oxoGua碱基对之后，添加与2-AP相反的dTTP的表观构象变化率的差异大于其磷酸二酯的差异键形成速率，这表明在构象变化速率方面，延伸的区分可能比在这种错配系统中磷酸二酯键形成速率的影响更大。 [参考：26]

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《Biochemistry》 |1998年第10期|共8页
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Furge LL.; Guengerich FP.;
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1. Pre-steady-state kinetics of nucleotide insertion following 8-oxo-7,8-dihydroguanine base pair mismatches by bacteriophage T7 DNA polymerase exo [J] . Furge LL., Guengerich FP. Biochemistry . 1998,第10期

机译：噬菌体T7 DNA聚合酶外切后8-氧代7,8-二氢鸟嘌呤碱基对错配后核苷酸插入的稳态前动力学
2. Analysis of nucleotide insertion and extension at 8-oxo-7,8-dihydroguanine by replicative T7 polymerase exo- and human immunodeficiency virus-1 reverse transcriptase using steady-state and pre-steady-state kinetics. [J] . Furge LL, Guengerich FP Biochemistry . 1997,第21期

机译：使用稳态和稳态前动力学，通过复制性T7聚合酶外切和人免疫缺陷病毒1逆转录酶分析8-oxo-7,8-dihydroguanine在8-oxo-7,8-氢鸟嘌呤的核苷酸插入和延伸。
3. STEADY-STATE AND PRE-STEADY-STATE KINETIC ANALYSIS OF DNTP INSERTION OPPOSITE 8-OXO-7,8-DIHYDROGUANINE BY ESCHERICHIA COLI POLYMERASES I EXO(-) AND II EXO(-) [J] . Lowe LG, Guengerich FP Biochemistry . 1996,第30期

机译：大肠埃希氏菌大肠杆菌I EXO（-）和II EXO（-）对DNTP插入对位8-OXO-7,8-二氢鸟嘌呤的稳态和稳态前动力学分析
4. VOLTAMMETRIC ANALYSIS OF DNA FILMS IMMOBILIZED ON GOLD FILM ELECTRODES CARRYING SINGLE BASE PAIR MISMATCHES [C] . Oliver Panke, Fred Lisdat, The Institute of Electrical and Electronics EngineersInc. International Solid-State Sensors, Actuators and Microsystems Conference . 2007

机译：固定在金膜电极上固定的DNA膜的伏安分析，其单个碱基对失配
5. I. Comparison of translesion bypass of guanine-N2 monoadducts of mitomycin C and guanine -N7 monoadducts of 2,7-diaminomitosene by T7 exo-, Klenow exo-, eta and Klenow exo+ DNA polymerases. II. Structure-based design, synthesis, structure-conformation and structure -activity relationships studies of D-Phe-Pro-D-Arg-P1'-CONH2 tetrapeptides with inhibitory activity for thrombin. [D] . Clement, Cristina C. 2006

机译：I.通过T7 exo-，Klenow exo-，eta和Klenow exo + DNA聚合酶比较丝裂霉素C的鸟嘌呤-N2单加合物和2,7-二氨基光油的鸟嘌呤-N7单加合物的跨病变旁路。二。具有凝血酶抑制活性的D-Phe-Pro-D-Arg-P1'-CONH2四肽的基于结构的设计，合成，结构构象和结构-活性关系研究。
6. Location analysis of 8-oxo-7,8-dihydroguanine in DNA by polymerase-mediated differential coding [O] . Feng Tang, Shan Liu, Qiao-Ying Li, 2011

机译：聚合酶介导的差异编码法分析DNA中8-氧代7,8-二氢鸟嘌呤的位置
7. Kinetics of Nucleotide Incorporation Opposite Polycyclic Aromatic Hydrocarbon-DNA Adducts by Processive Bacteriophage T7 DNA Polymerase [O] . -1

机译：通过加工噬菌体T7 DNA聚合酶对核苷酸掺入相反的多环芳烃-DNA加合物的动力学

Pre-steady-state kinetics of nucleotide insertion following 8-oxo-7,8-dihydroguanine base pair mismatches by bacteriophage T7 DNA polymerase exo

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