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Separation of ribosomal subunits of Escherichia coli by Sepharose chromatography using reverse salt gradient.

机译:使用反向盐梯度通过琼脂糖层析分离大肠埃希氏菌核糖体亚基。

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摘要

A mixture of 30 S and 50 S subunits quantitatively absorbs on a column of Sepharose--4B from the buffer: 0.02 M Tris--HCl, pH 7.5, containing 1.5 M (NH4)2SO4. During elution by reverse gradient of ammonium sulphate (1.5--0.05 M) the subunits are eluted at different salt concentrations. Complete separation of subunits is attained in the absence of Mg2+ ions. The 30 S subunits prepared from 70 S ribosomes according to this procedure are fully active in the codon--dependent binding of a specific aminoacyl--tRNA. After their reassociation with 50 S subunits isolated by zonal centrifugation, the resulting 70 S ribosomes are active in polypeptide synthesis at the same degree as control 70 S ribosomes in which both types of subunits were prepared by zonal centrifugation. The initial 70 S ribosomes for the chromatographic separation into subunits can be obtained by their pelleting from a crude extract with subsequent washing with concentrated solutions of NH4Cl in the ultracentrifuge, or by salt fractionation of the crude extract according to a slightly modified procedure of Kurland.
机译:30 S和50 S亚基的混合物在Sepharose--4B色谱柱上从以下缓冲液中定量吸收:0.02 M Tris-HCl,pH 7.5,含有1.5 M(NH4)2SO4。在通过硫酸铵(1.5--0.05 M)的反向梯度洗脱期间,亚基以不同的盐浓度洗脱。在不存在Mg2 +离子的情况下,可以实现亚基的完全分离。根据此程序由70 S核糖体制备的30 S亚基在特定氨酰基tRNA的密码子依赖性结合中具有完全活性。将它们与通过区带离心分离的50 S亚单位重新结合后,所得的70 S核糖体在多肽合成中的活性与对照70 S核糖体的程度相同,在对照中,通过区带离心制备两种类型的亚单位。用于色谱分离成亚基的最初的70 S核糖体可通过以下方法获得:从粗提物中沉淀出颗粒,然后在超速离心机中用NH4Cl浓溶液洗涤,或根据Kurland稍加修改的程序对粗提物进行盐分馏。

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