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RNA噬菌体Qβ RNA体外复制所需的宿主因子。细胞内定位、定量及通过聚腺苷酸纤维素层析法进行纯化。

The host factor required for RNA phage Qbeta RNA replication in vitro. Intracellular location, quantitation, and purification by polyadenylate-cellulose chromatography.

作者信息

Carmichael G G, Weber K, Niveleau A, Wahba A J

出版信息

J Biol Chem. 1975 May 25;250(10):3607-612.

PMID:805130
Abstract

The Qbeta host factor, a heat-stable protein necessary in concert with Qbeta replicase for phage Qbeta RNA replication in vitro, has been localized in Escherichia coli and found to be associated primarily with ribosomes. This location has been established both by complement fixation assays with highly specific antiserum directed against the host factor, and by in vitro stimulation of Qbeta RNA replication by the Qbeta replicase. The complement fixation assay has provided the estimate that there are approximately 2500 copies of the host factor polypeptide per cell. The host factor is released from the ribosomes by a 1 M NH4Cl wash and concentrated by ammonium sulfate precipitation. It can be purified to apparent homogeneity in one further step by chromatography on poly(A)-cellulose. Ribosomal protein S1 subunit I of Qbeta replicase) also binds to the poly(A)-cellulose column and elutes before the host factor. In agreement with previous reports, we find that the host factor has a monomer molecular weight of 12,000 as judged by sodium dodecyl sulfate-polyacrylamide gels, and a native molecular weight of 72,000 as judged by the stoichiometric interaction of the host factor with Qbeta RNA, by sedimentation in sucrose velocity gradients, and by sodium dodecyl sulfate gel mobility when incompletely disaggregated. The Qbeta host factor is a potent inhibitor of an in vitro poly(A)-directed polylysine protein-synthesizing system, but has less effect on the in vitro translation of poly(U), R17 RNA, late T7 mRNA, or endogenous E. coli mRNA. The amino acid composition and NH2- terminal sequence rule out the host factor as one of the known 30 S or 50 S E. coli ribosomal proteins. The finding that the Qbeta host factor is associated with ribosomes in vivo completes the demonstration that all of the host-supplied proteins required for phage Qbeta RNA replication in vitro are either associated with ribosomes or are involved in the protein-synthetic machinery of the cell.

摘要

Qβ宿主因子是一种热稳定蛋白,在体外与Qβ复制酶协同作用对噬菌体Qβ RNA复制是必需的。它已在大肠杆菌中定位,并发现主要与核糖体相关。通过用针对宿主因子的高度特异性抗血清进行补体结合试验,以及通过Qβ复制酶对Qβ RNA复制的体外刺激,确定了该位置。补体结合试验估计每个细胞中宿主因子多肽约有2500个拷贝。宿主因子通过1M NH4Cl洗涤从核糖体上释放出来,并通过硫酸铵沉淀进行浓缩。通过在聚(A)-纤维素上进行色谱分离,可在进一步的步骤中将其纯化至表观均一。Qβ复制酶的核糖体蛋白S1亚基I也与聚(A)-纤维素柱结合,并在宿主因子之前洗脱。与先前的报道一致,我们发现通过十二烷基硫酸钠-聚丙烯酰胺凝胶判断,宿主因子的单体分子量为12000,通过宿主因子与Qβ RNA的化学计量相互作用、在蔗糖速度梯度中的沉降以及在不完全解离时的十二烷基硫酸钠凝胶迁移率判断,其天然分子量为72000。Qβ宿主因子是体外聚(A)指导的聚赖氨酸蛋白质合成系统的有效抑制剂,但对聚(U)、R17 RNA、晚期T7 mRNA或内源性大肠杆菌mRNA的体外翻译影响较小。氨基酸组成和NH2末端序列排除了宿主因子是已知的30S或50S大肠杆菌核糖体蛋白之一。Qβ宿主因子在体内与核糖体相关这一发现完成了证明体外噬菌体Qβ RNA复制所需的所有宿主提供的蛋白质要么与核糖体相关,要么参与细胞的蛋白质合成机制。

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