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用丝裂霉素C处理的大肠杆菌中核糖体颗粒的分解

Decomposition of ribosomal particles in Escherichia coli treated with mitomycin C.

作者信息

Suzuki H, Kilgore W W

出版信息

J Bacteriol. 1967 Sep;94(3):666-76. doi: 10.1128/jb.94.3.666-676.1967.

Abstract

Exposure of cells of Escherichia coli to mitomycin C (5 mug/ml) resulted in a marked change in the sedimentation profiles of the cell-free extracts, indicating a specific decomposition of ribosomal particles. When the extracts were prepared in the presence of 0.01 m Mg(++) and analyzed by sucrose density gradient centrifugations, the 100S fraction disappeared rapidly from the treated cells. The 70S ribosomes were also degraded, but more slowly, with a concomitant accumulation of a fraction having a sedimentation coefficient of about 50S. However, decomposition of the 70S ribosomes was preceded by an almost complete loss of the 50S ribosomal subunits, as revealed by sedimentation analyses in the presence of 10(-4)m Mg(++). Synthesis of the ribosomes in the treated cells was also suppressed, being demonstrated by a lower incorporation of uracil-2-(14)C into the ribosomal fractions. However, the change in the ribosomal profile in the treated cells apparently resulted from the decomposition of pre-existing ribosomes, rather than from the inhibition of the net synthesis of ribosomes. Sedimentation analyses and chromatography of the nucleic acids extracted from the treated cells indicated extensive but delayed degradation of the ribosomal ribonucleic acid (RNA), but not of the soluble RNA or deoxyribonucleic acid fractions. Altered structure of the ribosomes in the treated cells was also indicated by their lower melting temperature, broadened thermal profile, higher electrophoretic mobility, and extreme sensitivity to ribonuclease treatment, compared with normal ribosomes. The synthesis of messenger RNA was inhibited progressively with time in the treated cells.

摘要

将大肠杆菌细胞暴露于丝裂霉素C(5微克/毫升)会导致无细胞提取物的沉降图谱发生显著变化,表明核糖体颗粒发生了特异性分解。当在0.01摩尔/升Mg(++)存在的情况下制备提取物并通过蔗糖密度梯度离心进行分析时,100S组分在处理过的细胞中迅速消失。70S核糖体也会降解,但速度较慢,同时会积累一个沉降系数约为50S的组分。然而,如在10(-4)摩尔/升Mg(++)存在下进行的沉降分析所示,70S核糖体的分解之前50S核糖体亚基几乎完全丧失。处理过的细胞中核糖体的合成也受到抑制,这通过尿嘧啶-2-(14)C掺入核糖体组分的量较低得到证明。然而,处理过的细胞中核糖体图谱的变化显然是由于预先存在的核糖体的分解,而不是由于核糖体净合成的抑制。对从处理过的细胞中提取的核酸进行沉降分析和色谱分析表明,核糖体核糖核酸(RNA)发生了广泛但延迟的降解,而可溶性RNA或脱氧核糖核酸组分则没有。与正常核糖体相比,处理过的细胞中核糖体结构的改变还表现为其较低的解链温度、变宽的热谱、较高的电泳迁移率以及对核糖核酸酶处理的极端敏感性。处理过的细胞中信使RNA的合成随时间逐渐受到抑制。

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