A peptide affinity reagent for isolating an intact and catalytically active multi-protein complex from mammalian cells

Hinnerk Saathoff; Mattias Brofelth; Anne Trinh; Benjamin Parker; Daniel Ryan; Jason Low; Sarah Webb; Ana Silva; Joel P. Mackay; Nicholas Shepherd

doi:10.1016/j.bmc.2015.01.023

A peptide affinity reagent for isolating an intact and catalytically active multi-protein complex from mammalian cells

Hinnerk Saathoff, Mattias Brofelth, Anne Trinh, Benjamin Parker, Daniel Ryan, Jason Low, Sarah Webb, Ana Silva, Joel P. Mackay, Nicholas Shepherd

Research output: Contribution to journal › Article › peer-review

Abstract

We have developed an approach for directly isolating an intact multi-protein chromatin remodeling complex from mammalian cell extracts using synthetic peptide affinity reagent 4. FOG1(1-15), a short peptide sequence known to target subunits of the nucleosome remodeling and deacetylase (NuRD) complex, was joined via a 35-atom hydrophilic linker to the StreptagII peptide. Loading this peptide onto Streptactin beads enabled capture of the intact NuRD complex from MEL cell nuclear extract. Gentle biotin elution yielded the desired intact complex free of significant contaminants and in a form that was catalytically competent in a nucleosome remodeling assay. The efficiency of 4 in isolating the NuRD complex was comparable to other reported methods utilising recombinantly produced GST-FOG1(1-45).

Original language	English
Pages (from-to)	960-965
Journal	Bioorganic and Medicinal Chemistry
Volume	23
Issue number	5
DOIs	https://doi.org/10.1016/j.bmc.2015.01.023
Publication status	Published - 2015

Access to Document

10.1016/j.bmc.2015.01.023

Cite this

@article{c0cbad92d62b434b86a75dd5988c8786,

title = "A peptide affinity reagent for isolating an intact and catalytically active multi-protein complex from mammalian cells",

abstract = "We have developed an approach for directly isolating an intact multi-protein chromatin remodeling complex from mammalian cell extracts using synthetic peptide affinity reagent 4. FOG1(1-15), a short peptide sequence known to target subunits of the nucleosome remodeling and deacetylase (NuRD) complex, was joined via a 35-atom hydrophilic linker to the StreptagII peptide. Loading this peptide onto Streptactin beads enabled capture of the intact NuRD complex from MEL cell nuclear extract. Gentle biotin elution yielded the desired intact complex free of significant contaminants and in a form that was catalytically competent in a nucleosome remodeling assay. The efficiency of 4 in isolating the NuRD complex was comparable to other reported methods utilising recombinantly produced GST-FOG1(1-45).",

author = "Hinnerk Saathoff and Mattias Brofelth and Anne Trinh and Benjamin Parker and Daniel Ryan and Jason Low and Sarah Webb and Ana Silva and Mackay, {Joel P.} and Nicholas Shepherd",

year = "2015",

doi = "10.1016/j.bmc.2015.01.023",

language = "English",

volume = "23",

pages = "960--965",

journal = "Bioorganic and Medicinal Chemistry",

publisher = "Pergamon-Elsevier Ltd",

number = "5",

}

TY - JOUR

T1 - A peptide affinity reagent for isolating an intact and catalytically active multi-protein complex from mammalian cells

AU - Saathoff, Hinnerk

AU - Brofelth, Mattias

AU - Trinh, Anne

AU - Parker, Benjamin

AU - Ryan, Daniel

AU - Low, Jason

AU - Webb, Sarah

AU - Silva, Ana

AU - Mackay, Joel P.

AU - Shepherd, Nicholas

PY - 2015

Y1 - 2015

N2 - We have developed an approach for directly isolating an intact multi-protein chromatin remodeling complex from mammalian cell extracts using synthetic peptide affinity reagent 4. FOG1(1-15), a short peptide sequence known to target subunits of the nucleosome remodeling and deacetylase (NuRD) complex, was joined via a 35-atom hydrophilic linker to the StreptagII peptide. Loading this peptide onto Streptactin beads enabled capture of the intact NuRD complex from MEL cell nuclear extract. Gentle biotin elution yielded the desired intact complex free of significant contaminants and in a form that was catalytically competent in a nucleosome remodeling assay. The efficiency of 4 in isolating the NuRD complex was comparable to other reported methods utilising recombinantly produced GST-FOG1(1-45).

AB - We have developed an approach for directly isolating an intact multi-protein chromatin remodeling complex from mammalian cell extracts using synthetic peptide affinity reagent 4. FOG1(1-15), a short peptide sequence known to target subunits of the nucleosome remodeling and deacetylase (NuRD) complex, was joined via a 35-atom hydrophilic linker to the StreptagII peptide. Loading this peptide onto Streptactin beads enabled capture of the intact NuRD complex from MEL cell nuclear extract. Gentle biotin elution yielded the desired intact complex free of significant contaminants and in a form that was catalytically competent in a nucleosome remodeling assay. The efficiency of 4 in isolating the NuRD complex was comparable to other reported methods utilising recombinantly produced GST-FOG1(1-45).

U2 - 10.1016/j.bmc.2015.01.023

DO - 10.1016/j.bmc.2015.01.023

M3 - Article

VL - 23

SP - 960

EP - 965

JO - Bioorganic and Medicinal Chemistry

JF - Bioorganic and Medicinal Chemistry

IS - 5

ER -

A peptide affinity reagent for isolating an intact and catalytically active multi-protein complex from mammalian cells

Abstract

Access to Document

Fingerprint

Cite this