Improved Native Isolation of Endogenous Protein A-Tagged Protein Complexes

John LaCava; Nagarajan Chandramouli; Hua Jiang; Michael P. Rout

doi:10.2144/000114012

Improved Native Isolation of Endogenous Protein A-Tagged Protein Complexes

John LaCava, Nagarajan Chandramouli, Hua Jiang, Michael P. Rout^*

^*Corresponding author for this work

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

10 Citations (Scopus)

22 Downloads (Pure)

Abstract

Here we report a modified peptide reagent useful for the rapid, native elution of protein complexes containing a Protein-A-tagged component. We tested this reagent for the elution of tagged endogenous protein complexes from yeast (Nup53p/Nup170p dimer; Nup1p/Kap95p/Kap60p trimer; pentameric GINS complex) and bacteria (RNAPII holoenzyme). The majority of the affinity-isolated material is released within 15 minutes under mild conditions, and the elution reagent itself is readily depleted from the elution mixture by simple spin column gel filtration. This reagent is ideal for eluting protein complexes after Protein A / IgG affinity isolation when protease cleavage is not possible or not desirable and facile depletion of the elution reagent is needed.

Original language	English
Pages (from-to)	213-216
Number of pages	4
Journal	Biotechniques
Volume	54
Issue number	4
DOIs	https://doi.org/10.2144/000114012
Publication status	Published - 2013
Externally published	Yes

Keywords

AFFINITY PURIFICATION
BINDING
IGG
DOMAINS
POLYMERASE
RESOLUTION
ELUTION

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title = "Improved Native Isolation of Endogenous Protein A-Tagged Protein Complexes",

abstract = "Here we report a modified peptide reagent useful for the rapid, native elution of protein complexes containing a Protein-A-tagged component. We tested this reagent for the elution of tagged endogenous protein complexes from yeast (Nup53p/Nup170p dimer; Nup1p/Kap95p/Kap60p trimer; pentameric GINS complex) and bacteria (RNAPII holoenzyme). The majority of the affinity-isolated material is released within 15 minutes under mild conditions, and the elution reagent itself is readily depleted from the elution mixture by simple spin column gel filtration. This reagent is ideal for eluting protein complexes after Protein A / IgG affinity isolation when protease cleavage is not possible or not desirable and facile depletion of the elution reagent is needed.",

keywords = "AFFINITY PURIFICATION, BINDING, IGG, DOMAINS, POLYMERASE, RESOLUTION, ELUTION",

author = "John LaCava and Nagarajan Chandramouli and Hua Jiang and Rout, {Michael P.}",

year = "2013",

doi = "10.2144/000114012",

language = "English",

volume = "54",

pages = "213--216",

journal = "Biotechniques",

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TY - JOUR

T1 - Improved Native Isolation of Endogenous Protein A-Tagged Protein Complexes

AU - LaCava, John

AU - Chandramouli, Nagarajan

AU - Jiang, Hua

AU - Rout, Michael P.

PY - 2013

Y1 - 2013

N2 - Here we report a modified peptide reagent useful for the rapid, native elution of protein complexes containing a Protein-A-tagged component. We tested this reagent for the elution of tagged endogenous protein complexes from yeast (Nup53p/Nup170p dimer; Nup1p/Kap95p/Kap60p trimer; pentameric GINS complex) and bacteria (RNAPII holoenzyme). The majority of the affinity-isolated material is released within 15 minutes under mild conditions, and the elution reagent itself is readily depleted from the elution mixture by simple spin column gel filtration. This reagent is ideal for eluting protein complexes after Protein A / IgG affinity isolation when protease cleavage is not possible or not desirable and facile depletion of the elution reagent is needed.

AB - Here we report a modified peptide reagent useful for the rapid, native elution of protein complexes containing a Protein-A-tagged component. We tested this reagent for the elution of tagged endogenous protein complexes from yeast (Nup53p/Nup170p dimer; Nup1p/Kap95p/Kap60p trimer; pentameric GINS complex) and bacteria (RNAPII holoenzyme). The majority of the affinity-isolated material is released within 15 minutes under mild conditions, and the elution reagent itself is readily depleted from the elution mixture by simple spin column gel filtration. This reagent is ideal for eluting protein complexes after Protein A / IgG affinity isolation when protease cleavage is not possible or not desirable and facile depletion of the elution reagent is needed.

KW - AFFINITY PURIFICATION

KW - BINDING

KW - IGG

KW - DOMAINS

KW - POLYMERASE

KW - RESOLUTION

KW - ELUTION

U2 - 10.2144/000114012

DO - 10.2144/000114012

M3 - Article

SN - 0736-6205

VL - 54

SP - 213

EP - 216

JO - Biotechniques

JF - Biotechniques

IS - 4

ER -

Improved Native Isolation of Endogenous Protein A-Tagged Protein Complexes

Abstract

Keywords

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