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磷酸葡萄糖酸脱水酶和DnaK的N端对大肠杆菌中固定相伴侣毒性的多拷贝质粒抑制作用。

Multicopy plasmid suppression of stationary phase chaperone toxicity in Escherichia coli by phosphogluconate dehydratase and the N-terminus of DnaK.

作者信息

Rockabrand D, Blum P

机构信息

School of Biological Sciences, University of Nebraska, Lincoln 68588-0118, USA.

出版信息

Mol Gen Genet. 1995 Dec 15;249(5):498-506. doi: 10.1007/BF00290575.

Abstract

Overproduction of DnaK in Escherichia coli results in a bacteriocidal effect. This effect is most acute in stationary phase cells. A selection scheme was developed to isolate multicopy suppressors from an E. coli plasmid expression library, which overcome the stationary phase toxicity of excess DnaK. Two suppressor plasmids were recovered which contained inserts of 1.85 kb and 2.69 kb, respectively. Rearranged and deleted plasmid derivatives were constructed and used to further localize the suppressors. DNA sequence analysis demonstrated that one suppressor encoded phosphogluconate dehydratase (Edd) while the other suppressor encoded the N-terminal 237 amino acids of DnaK itself (DnaK'). Strains bearing the suppressor plasmids constitutively overproduced proteins with apparent masses of 66 kDa (Edd) and 37 kDa (DnaK') as determined by gel electrophoresis. Western blot analysis using polyclonal antisera specific for either Edd or DnaK confirmed the identity of these overproduced proteins. Suppression of DnaK toxicity was eliminated by the introduction of a + 1 frameshift mutation early in the respective coding regions of either of the two suppressors. These results suggest that suppressor gene translation plays a role in the mechanism of DnaK suppression.

摘要

大肠杆菌中DnaK的过量产生会导致杀菌作用。这种作用在稳定期细胞中最为明显。我们开发了一种筛选方案,从大肠杆菌质粒表达文库中分离多拷贝抑制子,这些抑制子可克服过量DnaK的稳定期毒性。回收了两个抑制质粒,其插入片段分别为1.85 kb和2.69 kb。构建了重排和缺失的质粒衍生物,并用于进一步定位抑制子。DNA序列分析表明,一个抑制子编码磷酸葡萄糖酸脱水酶(Edd),而另一个抑制子编码DnaK自身的N端237个氨基酸(DnaK')。通过凝胶电泳测定,携带抑制质粒的菌株组成型过量表达表观分子量分别为66 kDa(Edd)和37 kDa(DnaK')的蛋白质。使用针对Edd或DnaK的多克隆抗血清进行的蛋白质印迹分析证实了这些过量表达蛋白质的身份。通过在两个抑制子中任何一个的相应编码区域早期引入+1移码突变,消除了DnaK毒性的抑制作用。这些结果表明,抑制基因的翻译在DnaK抑制机制中起作用。

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