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大肠杆菌膜结合多核糖体对输出蛋白的合成。

Synthesis of exported proteins by membrane-bound polysomes from Escherichia coli.

作者信息

Randall L L, Hardy S J

出版信息

Eur J Biochem. 1977 May 2;75(1):43-53. doi: 10.1111/j.1432-1033.1977.tb11502.x.

Abstract

A membrane-bound fraction of polysomes of Escherichia coli has been isolated after lysis of cells without the use of lysozyme. Protein-synthesis studies in vitro show that membrane-bound and free polysomes are different in the following respects. 1. Membrane-bound polysomes synthesize proteins which are exported from the cell. The products include proteins of the outer membrane and a secreted periplasmic protein, the maltose-binding protein. 2. The major product synthesized by free polysomes is elongation factor Tu, a soluble cytoplasmic protein. 3. The activity of membrane-bound polysomes in vitro is more resistant to puromycin than is the activity of free polysomes. In addition, the mRNA associated with membrane-bound polysomes is more stable than the bulk of cellular mRNA as revealed by studies with rifampicin.

摘要

在不使用溶菌酶裂解细胞后,已分离出大肠杆菌多核糖体的膜结合部分。体外蛋白质合成研究表明,膜结合多核糖体和游离多核糖体在以下方面存在差异。1. 膜结合多核糖体合成从细胞输出的蛋白质。产物包括外膜蛋白和一种分泌的周质蛋白,即麦芽糖结合蛋白。2. 游离多核糖体合成的主要产物是延伸因子Tu,一种可溶性细胞质蛋白。3. 体外膜结合多核糖体的活性比游离多核糖体的活性对嘌呤霉素更具抗性。此外,如用利福平研究所揭示的,与膜结合多核糖体相关的mRNA比大部分细胞mRNA更稳定。

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