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二氢链霉素与大肠杆菌核糖体的结合:反应动力学

Binding of dihydrostreptomycin to Escherichia coli ribosomes: kinetics of the reaction.

作者信息

Chang F N, Flaks J G

出版信息

Antimicrob Agents Chemother. 1972 Oct;2(4):308-19. doi: 10.1128/AAC.2.4.308.

Abstract

Investigations were carried out on the binding of dihydrostreptomycin to purified (and reassociated) 70S ribosomes and 30S subunits from streptomycin-susceptible strains, and the results were compared with those of similar studies with native (run-off) 70S ribosomes. At 0 C, only a small fraction of purified 70S ribosomes and 30S sub-units bound 1 molecule of the antibiotic tightly, and at a rate comparable to the binding occurring with native 70S ribosomes. At temperatures of 10 C and above, there was a temperature-dependent increase in the extent of antibiotic binding to purified 70S and 30S particles up to a maximum of 1 molecule/ribosomal particle, but the kinetics of binding was slow in comparison to that taking place at 0 C. These and other results suggest that a major fraction of 30S subunits and purified (or reassociated) 70S ribosomes are inactive in binding the antibiotic. This has been localized to an instability of the free 30S subunit, which in solution at 0 C has a half-life of 5 hr or less. Inactive 30S or 70S particles could be thermally activated, with the latter being identical in their streptomycin-binding properties to native 70S ribosomes. The activation kinetics were slow in comparison to the binding kinetics for the antibiotic and were indicative of a conformational change in ribosomal structure. There thus appears to be a reversible transition between active and inactive forms of the ribosomal particles for streptomycin binding, but additional binding sites for the antibiotic are not created by the transitions. The active form of the 30S subunit can be stabilized in the presence of polyuridylic acid, but much more effectively by association with the 50S subunit to form a 70S ribosome. The kinetics of dihydrostreptomycin binding were studied in both directions of the reaction, and the reaction in the direction of binding was found to be several orders of magnitude faster than that of the reverse, or debinding, direction. The kinetics of the exchange of bound dihydrostreptomycin with the free antibiotic were also determined and shown to have rate constants that are very similar to those of the debinding reaction, which is the rate-limiting step. It appears likely that the exchange reaction is proceeding via the same reaction pathway. The temperature dependence of the kinetics of dissociation of the bound complex was much greater than that in the direction of binding and accounted for most of the temperature dependence of the binding equilibrium. From the determined thermodynamic and activation parameters, it appears likely that binding of the antibiotic induces a conformational change in ribosomal structure to one that is less ordered than the native particle. Heterogeneity has been found in the kinetics of binding and of exchange, with a fraction of the 70S population showing slower kinetics for both directions of the reaction.

摘要

对二氢链霉素与来自链霉素敏感菌株的纯化(及重新缔合)的70S核糖体和30S亚基的结合进行了研究,并将结果与对天然(连续延伸)70S核糖体的类似研究结果进行了比较。在0℃时,只有一小部分纯化的70S核糖体和30S亚基紧密结合1分子抗生素,其结合速率与天然70S核糖体的结合速率相当。在10℃及以上温度时,抗生素与纯化的70S和30S颗粒的结合程度随温度升高而增加,最高可达1分子/核糖体颗粒,但与0℃时相比,结合动力学较慢。这些及其他结果表明,大部分30S亚基和纯化(或重新缔合)的70S核糖体在结合抗生素方面是无活性的。这已被定位到游离30S亚基的不稳定性,其在0℃溶液中的半衰期为5小时或更短。无活性的30S或70S颗粒可被热激活,后者在链霉素结合特性上与天然70S核糖体相同。与抗生素的结合动力学相比,激活动力学较慢,表明核糖体结构发生了构象变化。因此,对于链霉素结合,核糖体颗粒的活性形式和无活性形式之间似乎存在可逆转变,但转变不会产生额外的抗生素结合位点。30S亚基的活性形式在聚尿苷酸存在下可被稳定,但与50S亚基缔合形成70S核糖体时更有效。研究了二氢链霉素结合反应两个方向的动力学,发现结合方向的反应比反向(即解离)方向快几个数量级。还测定了结合的二氢链霉素与游离抗生素交换的动力学,结果表明其速率常数与解离反应的速率常数非常相似,解离反应是限速步骤。交换反应似乎是通过相同的反应途径进行的。结合复合物解离动力学的温度依赖性远大于结合方向的温度依赖性,这是结合平衡温度依赖性的主要原因。根据测定的热力学和活化参数,抗生素的结合似乎诱导核糖体结构发生构象变化,变为比天然颗粒无序程度更低的结构。在结合和交换动力学中发现了异质性,一部分70S群体在反应的两个方向上都表现出较慢的动力学。

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