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大肠杆菌DnaJ和DnaK热休克蛋白在oriC质粒复制中的体外作用。

In vitro roles of Escherichia coli DnaJ and DnaK heat shock proteins in the replication of oriC plasmids.

作者信息

Malki A, Hughes P, Kohiyama M

机构信息

Institute Jacques Monod, Centre National de la Recherche Scientifique, Université Paris, France.

出版信息

Mol Gen Genet. 1991 Mar;225(3):420-6. doi: 10.1007/BF00261682.

Abstract

Heat shock proteins have been shown to be involved in many cellular processes in procaryotic and eucaryotic cells. Using an in vitro DNA replication assay, we show that DNA synthesis initiated at the chromosomal origin of replication of Escherichia coli (oriC) is considerably reduced in enzyme extracts isolated from cells bearing mutations in the dnaK and dnaJ genes, which code for heat shock proteins. Furthermore, unlike DNA synthesis in wild-type extracts, residual DNA synthesis in dnaK and dnaJ extracts is thermosensitive. Although thermosensitivity can be complemented by the addition of DnaK and DnaJ proteins, restoration of near wild-type replication levels requires supplementary quantities of purified DnaA protein. This key DNA synthesis initiator protein is shown to be adsorbed to DnaK affinity columns. These results suggest that at least one of the heat shock proteins. DnaK, exerts an effect on the initiation of DNA synthesis at the level of DnaA protein activity. However, our observation of normal oriC plasmid transformation ratios and concentrations in heat shock mutants at permissive temperatures would suggest that heat shock proteins play a role in DNA replication mainly at high temperatures or under other stressful growth conditions.

摘要

热休克蛋白已被证明参与原核细胞和真核细胞中的许多细胞过程。利用体外DNA复制试验,我们发现,在从携带编码热休克蛋白的dnaK和dnaJ基因突变的细胞中分离出的酶提取物中,从大肠杆菌染色体复制起点(oriC)起始的DNA合成显著减少。此外,与野生型提取物中的DNA合成不同,dnaK和dnaJ提取物中的残余DNA合成对温度敏感。虽然通过添加DnaK和DnaJ蛋白可以弥补温度敏感性,但要恢复到接近野生型的复制水平需要补充大量纯化的DnaA蛋白。这种关键的DNA合成起始蛋白被证明可吸附到DnaK亲和柱上。这些结果表明,至少有一种热休克蛋白,即DnaK,在DnaA蛋白活性水平上对DNA合成的起始产生影响。然而,我们观察到在允许温度下热休克突变体中oriC质粒的转化率和浓度正常,这表明热休克蛋白主要在高温或其他应激生长条件下在DNA复制中发挥作用。

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