Literature DB >> 23758098

Purification of a membrane protein with conjugated engineered micelles.

Guy Patchornik1, Dganit Danino, Ellina Kesselman, Ellen Wachtel, Noga Friedman, Mordechai Sheves.   

Abstract

A novel method for purifying membrane proteins is presented. The approach makes use of engineered micelles composed of a nonionic detergent, β-octylglucoside, and a hydrophobic metal chelator, bathophenanthroline. Via the chelators, the micelles are specifically conjugated, i.e., tethered, in the presence of Fe(2+) ions, thereby forming micellar aggregates which provide the environment for separation of lipid-soluble membrane proteins from water-soluble proteins. The micellar aggregates (here imaged by cryo-transmission electron microscopy) successfully purify the light driven proton pump, bacteriorhodopsin (bR), from E. coli lysate. Purification takes place within 15 min and can be performed both at room temperature and at 4 °C. More than 94% of the water-soluble macromolecules in the lysate are excluded, with recovery yields of the membrane protein ranging between 74% and 85%. Since this approach does not require precipitants, high concentrations of detergent to induce micellar aggregates, high temperature, or changes in pH, it is suggested that it may be applied to the purification of a wide variety of membrane proteins.

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Year:  2013        PMID: 23758098     DOI: 10.1021/bc400069w

Source DB:  PubMed          Journal:  Bioconjug Chem        ISSN: 1043-1802            Impact factor:   4.774


  1 in total

1.  Data on peptidyl platform-based anticancer drug synthesis and triton-x-based micellar clusters (MCs) self-assembly peculiarities for enhanced solubilization, encapsulation of hydrophobic compounds and their interaction with HeLa cells.

Authors:  Alexey V Solomonov; Yuriy S Marfin; Evgeniy V Rumyantsev; Elena Ragozin; Talia Shekhter Zahavi; Gary Gellerman; Alexander B Tesler; Falk Muench; Akiko Kumagai; Atsushi Miyawaki
Journal:  Data Brief       Date:  2019-05-24
  1 in total

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