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从小鼠肝脏中制备活性流失的80S核糖体及其亚基。

Preparation of active run-off 80S ribosomes and their subunits from mouse liver.

作者信息

Faber A J, Tamaoki T

出版信息

Can J Biochem. 1976 Dec;54(12):1034-9. doi: 10.1139/o76-151.

Abstract

A method is described for the preparation of active "run-off" 80S ribosomes and 40S and 60S subunits of mouse liver. A polysome preparation was incubated at 37 degrees C for 10 min under the condition for protein synthesis (4 mM Mg2+, 100 mM KCL). Puromycin (10 mM)and 2 M KCL were added to a final concentration of 0.1 mM and 500 mM, respectively, and the reaction mixture was further incubated at 37 degrees C for 10 min. This latter treatment destabilized small polysomes and "stuck" 80S particles, which were remaining after the first incubation, leading to complete release of 40S and 60S particles. Thus, the present method minimized variations in yield of subunits due to polysome preparations and preincubation conditions. The subunits were separated by sucrose density-gradient centrifugation or recovered by precipitation following reassociation into 80S particles (run-off 80S). The reformation of 80S particles from the subunits occurred spontaneously at 5 mM Mg2+ and 100mM KCL. The isolated 40S and 60S subunits, separately, showed low phenylalanine-incorporating activity in the presence of poly(U), but when recombined, polymerized up to 10 phenylalanine residues per couple.

摘要

本文描述了一种制备小鼠肝脏活性“溢流”80S核糖体以及40S和60S亚基的方法。将多核糖体制剂在蛋白质合成条件(4 mM Mg2+,100 mM KCl)下于37℃孵育10分钟。加入嘌呤霉素(10 mM)和2 M KCl,使其终浓度分别为0.1 mM和500 mM,反应混合物在37℃进一步孵育10分钟。后一种处理使小多核糖体不稳定,并使第一次孵育后剩余的80S颗粒“固定”下来,导致40S和60S颗粒完全释放。因此,本方法将由于多核糖体制剂和预孵育条件导致的亚基产量变化降至最低。通过蔗糖密度梯度离心分离亚基,或将重新缔合为80S颗粒(溢流80S)后沉淀回收亚基。亚基在5 mM Mg2+和100 mM KCl条件下自发重新形成80S颗粒。分离得到的40S和60S亚基单独存在时,在聚(U)存在下显示出较低的苯丙氨酸掺入活性,但重新组合后,每对可聚合多达10个苯丙氨酸残基。

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Isolation of active ribosomal subunits from yeast.从酵母中分离活性核糖体亚基。
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