Membrane docking of an aggregation-prone protein improves its solubilization
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- 作者:Jihen Tagourti ; Abderrahim Malki ; René ; e Kern ; Emmanuelle d'Alenç ; on ; Gilbert Richarme
- 关键词:Protein aggregation ; Heat stress ; Inclusion bodies ; N ; N′ ; -diacetylchitobiose phosphotransferase transporter ; Membrane
- 刊名:Gene
- 出版年:2008
- 出版时间:15 December 2008
- 年:2008
- 卷:426
- 期:1-2
- 页码:32-38
- 全文大小:359 K
文摘
We used preS2-S′-β-galactosidase, a three domain fusion protein that aggregates extensively at 43 °C in the cytoplasm of Escherichia coli to search for multicopy suppressors of protein aggregation and inclusion bodies formation, and took advantage of the known differential solubility of preS2-S′-β-galactosidase at 37 and 43 °C to develop a selection procedure for the gene products that would prevent its aggregation in vivo at 43 °C. First, we demonstrate that the differential solubility of preS2-S′-β-galactosidase results in a lactose-positive phenotype at 37 °C as opposed to a lactose-negative phenotype at 43 °C. We searched for multicopy suppressors of preS2-S′-β-galactosidase aggregation at 43 °C by selecting pink lactose-positive colonies on a background of white lactose-negative colonies after transformation of bacteria with an E. coli gene bank. We found only two multicopy suppressors of preS2-S′-β-galactosidase aggregation at 43 °C, protein isoaspartate methyltransferase (PIMT) and the membrane components ChbBC of the N,N′-diacetylchitobiose phosphotransferase transporter.
We have previously shown that PIMT overexpression reduces the level of isoaspartate in preS2-S′-β-galactosidase, increases its thermal stability and consequently helps in its solubilization at 43 °C (Kern et al., J. Bacteriol. 187, 1377–1383). In the present work, we show that ChbBC overexpression targets a fraction of preS2-S′-β-galactosidase to the membrane, and decreases its amount in inclusion bodies, which results in its decreased thermodenaturation and in a lactose-positive phenotype at 43 °C. Cross-linking experiments show that the inner membrane protein ChbC interacts with preS2-S′-β-galactosidase. Our results suggest that membrane docking of aggregation-prone proteins might be a useful method for their solubilization.