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巴氏芽孢梭菌核糖体和多核糖体在体外对合成信使核糖核酸和内源性信使核糖核酸的翻译

Translation of synthetic and endogenous messenger ribonucleic acid in vitro by ribosomes and polyribosomes from Clostridium pasteurianum.

作者信息

Himes R H, Stallcup M R, Rabinowitz J C

出版信息

J Bacteriol. 1972 Dec;112(3):1057-69. doi: 10.1128/jb.112.3.1057-1069.1972.

Abstract

Ribosomes and polyribosomes from Clostridium pasteurianum were isolated and their activities were compared with those of ribosomes from Escherichia coli in protein synthesis in vitro. C. pasteurianum ribosomes exhibited a high level of activity due to endogenous messenger ribonucleic acid (RNA). For translation of polyuridylic acid [poly(U)], C. pasteurianum ribosomes required a higher concentration of Mg(2+) and a much higher level of poly(U) than did E. coli ribosomes. Phage f2 RNA added to the system with C. pasteurianum ribosomes gave no significant stimulation of protein synthesis in a homologous system or with E. coli initiation factors. The 30S and 50S subunits prepared from C. pasteurianum ribosomes reassociated less readily than subunits from E. coli. The ability of the C. pasteurianum subunits to reassociated was found to be dependent upon the presence of a reducing agent during preparation and during analysis of the reassociation products. In heterologous combinations, E. coli 30S subunits associated readily with C. pasteurianum 50S subunits to form 70S particles, but C. pasteurianum 30S subunits and E. coli 50S subunits did not associate. In poly(U) translation, E. coli 30S subunits were active in combination with 50S subunits from either E. coli or C. pasteurianum, but C. pasteurianum 30S subunits were not active in combination with either type of 50S subunits. Polyribosomes prepared from C. pasteurianum were very active in protein synthesis, and well-defined ribosomal aggregates as large as heptamers could be seen on sucrose gradients. An attempt was made to demonstrate synthesis in vitro of ferredoxin.

摘要

分离了巴斯德梭菌的核糖体和多核糖体,并在体外蛋白质合成中将它们的活性与大肠杆菌核糖体的活性进行了比较。由于内源性信使核糖核酸(RNA),巴斯德梭菌核糖体表现出高水平的活性。对于聚尿苷酸[poly(U)]的翻译,巴斯德梭菌核糖体比大肠杆菌核糖体需要更高浓度的Mg(2+)和更高水平的poly(U)。添加到含有巴斯德梭菌核糖体的系统中的噬菌体f2 RNA,在同源系统或与大肠杆菌起始因子一起时,对蛋白质合成没有明显的刺激作用。从巴斯德梭菌核糖体制备的30S和50S亚基重新结合的能力不如大肠杆菌亚基。发现巴斯德梭菌亚基重新结合的能力取决于制备过程中和重新结合产物分析过程中还原剂的存在。在异源组合中,大肠杆菌30S亚基很容易与巴斯德梭菌50S亚基结合形成70S颗粒,但巴斯德梭菌30S亚基和大肠杆菌50S亚基不结合。在poly(U)翻译中,大肠杆菌30S亚基与来自大肠杆菌或巴斯德梭菌的50S亚基结合时具有活性,但巴斯德梭菌30S亚基与任何一种50S亚基结合时都没有活性。从巴斯德梭菌制备的多核糖体在蛋白质合成中非常活跃,并且在蔗糖梯度上可以看到明确的核糖体聚集体,大到七聚体。尝试证明铁氧化还原蛋白的体外合成。

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