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莱茵衣藻细胞质核糖体和叶绿体核糖体的分离及其解离为活性亚基

Isolation of cytoplasmic and chloroplast ribosomes and their dissociation into active subunits from Chlamydomonas reinhardtii.

作者信息

Chua N H, Blobel G, Siekevitz P

出版信息

J Cell Biol. 1973 Jun;57(3):798-814. doi: 10.1083/jcb.57.3.798.

Abstract

A mixture of cytoplasmic (80S) and chloroplast (70S) ribosomes from Chlamydomonas reinhardtii was freed of contaminating membranes by sedimentation of the postmitochondrial supernatant through a layer of 1.87 M sucrose. The purified ribosomes were separated into 80S and 70S fractions by centrifugation at a relatively low speed on a 10-40% sucrose gradient containing 25 mM KCl and 5 mM MgCl(2). Both the 80S and 70S ribosomes were dissociated into compact subunits by centrifugations in 5-20% high-salt sucrose gradients. The dissociations of both ribosomal species under these conditions were not affected by the addition of puromycin, indicating that the ribosomes as isolated were devoid of nascent chains. Subunits derived from the 80S ribosomes had apparent sedimentation coefficients of 57S and 37S whereas those from the 70S ribosomes had apparent sedimentation coefficients of 50S and 33S. In the presence of polyuridylic acid and cofactors, the 80S and 70S ribosomes incorporated [(14)C]phenylalanine into material insoluble in hot TCA. The requirements for incorporation were found to be similar to those described for eukaryotic and prokaryotic ribosomes. Experiments with antibiotics showed that the activity of the 80S ribosomes was sensitive to cycloheximide, whereas that of the 70S ribosomes was inhibited by streptomycin. The isolated subunits, when mixed together in an incorporation medium, were also active in the polymerization of phenylalanine in vitro.

摘要

莱茵衣藻的胞质(80S)核糖体和叶绿体(70S)核糖体的混合物,通过将线粒体后上清液通过一层1.87M蔗糖进行沉降,去除了污染膜。纯化后的核糖体在含有25mM KCl和5mM MgCl₂的10 - 40%蔗糖梯度上以相对低速离心,分离为80S和70S组分。80S和70S核糖体在5 - 20%高盐蔗糖梯度中离心时均解离为紧密的亚基。在这些条件下,两种核糖体的解离不受嘌呤霉素添加的影响,表明分离得到的核糖体没有新生链。源自80S核糖体的亚基的表观沉降系数为57S和37S,而源自70S核糖体的亚基的表观沉降系数为50S和33S。在多聚尿苷酸和辅因子存在的情况下,80S和70S核糖体将[¹⁴C]苯丙氨酸掺入热三氯乙酸不溶性物质中。发现掺入的要求与真核和原核核糖体所描述的要求相似。抗生素实验表明,80S核糖体的活性对环己酰亚胺敏感,而70S核糖体的活性受链霉素抑制。分离得到的亚基在掺入培养基中混合在一起时,在体外苯丙氨酸聚合中也具有活性。

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