首页> 美国卫生研究院文献>Nucleic Acids Research >The binding of ribosomal protein S1 to S1-depleted 30S and 70S ribosomes. A fluorescence anisotropy study of the effects of Mg2+.
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The binding of ribosomal protein S1 to S1-depleted 30S and 70S ribosomes. A fluorescence anisotropy study of the effects of Mg2+.

机译:核糖体蛋白S1与贫S1的30S和70S核糖体的结合。荧光各向异性研究Mg2 +的影响。

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摘要

We have determined the equilibrium constants for the binding of AEDANS-labelled S1 to S1-depleted 30S and 70S ribosomes. For "tight" ribosomes, the association of S1 increases with the sixth power of Mg2+ concentration, but for 30S subunits and "loose" ribosomes, there is virtually no dependence of the association on Mg2+ over the same concentration range, 2-10 mM in Mg2+. The binding of S1 to 70S ribosomes at 10 mM Mg2+ is stabilized by 2 kcal/mol compared to the binding to 30S subunits. When intact S1 binds to tight ribosomes, the fluorescence anisotrophy is that for virtually complete rotational immobilization. The anisotropies vary considerably with the preparation and treatment of both S1 and ribosomes and these variations are detailed here. The results suggest the linkage of Mg2+-dependent conformational changes in the intact ribosomes, perhaps including rRNA, and the binding of S1.
机译:我们已经确定了AEDANS标记的S1与S1耗尽的30S和70S核糖体结合的平衡常数。对于“致密”核糖体,S1的缔合随Mg2 +浓度的六次幂而增加,但对于30S亚基和“松散”核糖体,在相同浓度范围内(2-10 mM),对Mg2 +的缔合几乎没有依赖性。镁2+。 S1与70S核糖体在10 mM Mg2 +的结合比与30S亚基的结合稳定2 kcal / mol。当完整的S1与紧密的核糖体结合时,荧光的各向异性是实际上完成了旋转固定的过程。各向异性随S1和核糖体的制备和治疗而有很大不同,这些变化在此详述。结果表明完整核糖体中可能包含rRNA的Mg2 +依赖性构象变化与S1的结合有关。

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