The association of BAG6 with SGTA and tail-anchored proteins

Pawel Leznicki; Quentin P Roebuck; Lydia Wunderley; Anne Clancy; Ewelina M Krysztofinska; Rivka L Isaacson; Jim Warwicker; Blanche Schwappach; Stephen High

doi:10.1371/journal.pone.0059590

The association of BAG6 with SGTA and tail-anchored proteins

Standard

The association of BAG6 with SGTA and tail-anchored proteins. / Leznicki, Pawel; Roebuck, Quentin P; Wunderley, Lydia; Clancy, Anne; Krysztofinska, Ewelina M; Isaacson, Rivka L; Warwicker, Jim; Schwappach, Blanche; High, Stephen.

in: PLOS ONE, Jahrgang 8, Nr. 3, 2013, S. e59590.

Publikationen: SCORING: Beitrag in Fachzeitschrift/Zeitung › SCORING: Zeitschriftenaufsatz › Forschung › Begutachtung

Harvard

Leznicki, P, Roebuck, QP, Wunderley, L, Clancy, A, Krysztofinska, EM, Isaacson, RL, Warwicker, J, Schwappach, B & High, S 2013, 'The association of BAG6 with SGTA and tail-anchored proteins', PLOS ONE, Jg. 8, Nr. 3, S. e59590. https://doi.org/10.1371/journal.pone.0059590

APA

Leznicki, P., Roebuck, Q. P., Wunderley, L., Clancy, A., Krysztofinska, E. M., Isaacson, R. L., Warwicker, J., Schwappach, B., & High, S. (2013). The association of BAG6 with SGTA and tail-anchored proteins. PLOS ONE, 8(3), e59590. https://doi.org/10.1371/journal.pone.0059590

Vancouver

Leznicki P, Roebuck QP, Wunderley L, Clancy A, Krysztofinska EM, Isaacson RL et al. The association of BAG6 with SGTA and tail-anchored proteins. PLOS ONE. 2013;8(3):e59590. https://doi.org/10.1371/journal.pone.0059590

Bibtex

@article{6782d3faa2ba4fabae87413592cade7e,

title = "The association of BAG6 with SGTA and tail-anchored proteins",

abstract = "BACKGROUND: The BAG6 protein is a subunit of a heterotrimeric complex that binds a range of membrane and secretory protein precursors localized to the cytosol, enforcing quality control and influencing their subsequent fate.METHODOLOGY AND PRINCIPAL FINDINGS: BAG6 has an N-terminal ubiquitin-like domain, and a C-terminal Bcl-2-associated athanogene domain, separated by a large central proline-rich region. We have used in vitro binding approaches to identify regions of BAG6 important for its interactions with: i) the small-glutamine rich tetratricopeptide repeat-containing protein alpha (SGTA) and ii) two model tail-anchored membrane proteins as a paradigm for its hydrophobic substrates. We show that the BAG6-UBL is essential for binding to SGTA, and find that the UBL of a second subunit of the BAG6-complex, ubiquitin-like protein 4A (UBL4A), competes for SGTA binding. Our data show that this binding is selective, and suggest that SGTA can bind either BAG6, or UBL4A, but not both at the same time. We adapted our in vitro binding assay to study the association of BAG6 with an immobilized tail-anchored protein, Sec61β, and find both the UBL and BAG domains are dispensable for binding this substrate. This conclusion was further supported using a heterologous subcellular localization assay in yeast, where the BAG6-dependent nuclear relocalization of a second tail-anchored protein, GFP-Sed5, also required neither the UBL, nor the BAG domain of BAG6.SIGNIFICANCE: On the basis of these findings, we propose a working model where the large central region of the BAG6 protein provides a binding site for a diverse group of substrates, many of which expose a hydrophobic stretch of polypeptide. This arrangement would enable the BAG6 complex to bring together its substrates with potential effectors including those recruited via its N-terminal UBL. Such effectors may include SGTA, and the resulting assemblies influence the subsequent fate of the hydrophobic BAG6 substrates.",

keywords = "Carrier Proteins/chemistry, Membrane Proteins/genetics, Protein Binding, Protein Structure, Tertiary, Saccharomyces cerevisiae Proteins/chemistry",

author = "Pawel Leznicki and Roebuck, {Quentin P} and Lydia Wunderley and Anne Clancy and Krysztofinska, {Ewelina M} and Isaacson, {Rivka L} and Jim Warwicker and Blanche Schwappach and Stephen High",

year = "2013",

doi = "10.1371/journal.pone.0059590",

language = "English",

volume = "8",

pages = "e59590",

journal = "PLOS ONE",

issn = "1932-6203",

publisher = "Public Library of Science",

number = "3",

}

RIS

TY - JOUR

T1 - The association of BAG6 with SGTA and tail-anchored proteins

AU - Leznicki, Pawel

AU - Roebuck, Quentin P

AU - Wunderley, Lydia

AU - Clancy, Anne

AU - Krysztofinska, Ewelina M

AU - Isaacson, Rivka L

AU - Warwicker, Jim

AU - Schwappach, Blanche

AU - High, Stephen

PY - 2013

Y1 - 2013

N2 - BACKGROUND: The BAG6 protein is a subunit of a heterotrimeric complex that binds a range of membrane and secretory protein precursors localized to the cytosol, enforcing quality control and influencing their subsequent fate.METHODOLOGY AND PRINCIPAL FINDINGS: BAG6 has an N-terminal ubiquitin-like domain, and a C-terminal Bcl-2-associated athanogene domain, separated by a large central proline-rich region. We have used in vitro binding approaches to identify regions of BAG6 important for its interactions with: i) the small-glutamine rich tetratricopeptide repeat-containing protein alpha (SGTA) and ii) two model tail-anchored membrane proteins as a paradigm for its hydrophobic substrates. We show that the BAG6-UBL is essential for binding to SGTA, and find that the UBL of a second subunit of the BAG6-complex, ubiquitin-like protein 4A (UBL4A), competes for SGTA binding. Our data show that this binding is selective, and suggest that SGTA can bind either BAG6, or UBL4A, but not both at the same time. We adapted our in vitro binding assay to study the association of BAG6 with an immobilized tail-anchored protein, Sec61β, and find both the UBL and BAG domains are dispensable for binding this substrate. This conclusion was further supported using a heterologous subcellular localization assay in yeast, where the BAG6-dependent nuclear relocalization of a second tail-anchored protein, GFP-Sed5, also required neither the UBL, nor the BAG domain of BAG6.SIGNIFICANCE: On the basis of these findings, we propose a working model where the large central region of the BAG6 protein provides a binding site for a diverse group of substrates, many of which expose a hydrophobic stretch of polypeptide. This arrangement would enable the BAG6 complex to bring together its substrates with potential effectors including those recruited via its N-terminal UBL. Such effectors may include SGTA, and the resulting assemblies influence the subsequent fate of the hydrophobic BAG6 substrates.

AB - BACKGROUND: The BAG6 protein is a subunit of a heterotrimeric complex that binds a range of membrane and secretory protein precursors localized to the cytosol, enforcing quality control and influencing their subsequent fate.METHODOLOGY AND PRINCIPAL FINDINGS: BAG6 has an N-terminal ubiquitin-like domain, and a C-terminal Bcl-2-associated athanogene domain, separated by a large central proline-rich region. We have used in vitro binding approaches to identify regions of BAG6 important for its interactions with: i) the small-glutamine rich tetratricopeptide repeat-containing protein alpha (SGTA) and ii) two model tail-anchored membrane proteins as a paradigm for its hydrophobic substrates. We show that the BAG6-UBL is essential for binding to SGTA, and find that the UBL of a second subunit of the BAG6-complex, ubiquitin-like protein 4A (UBL4A), competes for SGTA binding. Our data show that this binding is selective, and suggest that SGTA can bind either BAG6, or UBL4A, but not both at the same time. We adapted our in vitro binding assay to study the association of BAG6 with an immobilized tail-anchored protein, Sec61β, and find both the UBL and BAG domains are dispensable for binding this substrate. This conclusion was further supported using a heterologous subcellular localization assay in yeast, where the BAG6-dependent nuclear relocalization of a second tail-anchored protein, GFP-Sed5, also required neither the UBL, nor the BAG domain of BAG6.SIGNIFICANCE: On the basis of these findings, we propose a working model where the large central region of the BAG6 protein provides a binding site for a diverse group of substrates, many of which expose a hydrophobic stretch of polypeptide. This arrangement would enable the BAG6 complex to bring together its substrates with potential effectors including those recruited via its N-terminal UBL. Such effectors may include SGTA, and the resulting assemblies influence the subsequent fate of the hydrophobic BAG6 substrates.

KW - Carrier Proteins/chemistry

KW - Membrane Proteins/genetics

KW - Protein Binding

KW - Protein Structure, Tertiary

KW - Saccharomyces cerevisiae Proteins/chemistry

U2 - 10.1371/journal.pone.0059590

DO - 10.1371/journal.pone.0059590

M3 - SCORING: Journal article

C2 - 23533635

VL - 8

SP - e59590

JO - PLOS ONE

JF - PLOS ONE

SN - 1932-6203

IS - 3

ER -