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盐类和多胺对T4多核苷酸连接酶的动力学及作用

Kinetics and effect of salts and polyamines on T4 polynucleotide ligase.

作者信息

Raae A J, Kleppe R K, Kleppe K

出版信息

Eur J Biochem. 1975 Dec 15;60(2):437-43. doi: 10.1111/j.1432-1033.1975.tb21021.x.

Abstract

The kinetics of T4 polynucleotide ligase has been investigated at pH 8,20 degrees C and using the double-stranded DNA substrate (dA)n - [(dT)10]n/10. Double-reciprocal plots of initial rates vs substrate concentrations as well as product inhibition studies have indicated that the enzyme reacts according to a ping-pong mechanism. The overall mechanism was found to be non-processive. The true Km for the DNA substrate was 0.6 muM and that of ATP 100 muM. Several attempts were made to reverse the T4 polynucleotide ligase joining reaction using 32-p-labelled (dA)n - [(DT)40]n/40 as substrate. No breakdown of this DNA could be detected. The joining reaction was inhibited by high concentrations, i.e. above approximately 70mM, of salts such as KCl, NaCl, NH4Cl and CsCl. At a concentration of 200 mM almost 100% inhibition was observed. Polyamines also caused inhibition of the enzyme, the most efficient inhibitor being spermine followed by spermidine. At a concentration of 1 mM spermine, virtually no joining took place. Addition of salts or polyamines resulted in a large increase in the apparent Km for the DNA substrate whereas the apparent Km for ATP remained unchanged. It is suggested that the affinity of the enzyme for the DNA substrate is decreased in the presence of inhibiting agents.

摘要

在pH 8、20℃条件下,使用双链DNA底物(dA)n - [(dT)10]n/10对T4多核苷酸连接酶的动力学进行了研究。初始速率与底物浓度的双倒数图以及产物抑制研究表明,该酶按照乒乓机制反应。发现总体机制是非持续的。DNA底物的真实Km为0.6μM,ATP的真实Km为100μM。使用32P标记的(dA)n - [(DT)40]n/40作为底物,多次尝试逆转T4多核苷酸连接酶的连接反应。未检测到该DNA的分解。高浓度(即高于约70mM)的盐(如KCl、NaCl、NH4Cl和CsCl)会抑制连接反应。在200mM浓度下,观察到几乎100%的抑制。多胺也会抑制该酶,最有效的抑制剂是精胺,其次是亚精胺。在1mM精胺浓度下,几乎不发生连接。添加盐或多胺会导致DNA底物的表观Km大幅增加,而ATP的表观Km保持不变。有人认为,在存在抑制剂的情况下,酶对DNA底物的亲和力会降低。

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