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Artikel ; Online: Recent advances in proximity-based labeling methods for interactome mapping.

Trinkle-Mulcahy, Laura

2019 Band 8

Abstract: Proximity-based labeling has emerged as a powerful complementary approach to classic affinity purification of multiprotein complexes in the mapping of protein-protein interactions. Ongoing optimization of enzyme tags and delivery methods has improved ... ...

Abstract	Proximity-based labeling has emerged as a powerful complementary approach to classic affinity purification of multiprotein complexes in the mapping of protein-protein interactions. Ongoing optimization of enzyme tags and delivery methods has improved both temporal and spatial resolution, and the technique has been successfully employed in numerous small-scale (single complex mapping) and large-scale (network mapping) initiatives. When paired with quantitative proteomic approaches, the ability of these assays to provide snapshots of stable and transient interactions over time greatly facilitates the mapping of dynamic interactomes. Furthermore, recent innovations have extended biotin-based proximity labeling techniques such as BioID and APEX beyond classic protein-centric assays (tag a protein to label neighboring proteins) to include RNA-centric (tag an RNA species to label RNA-binding proteins) and DNA-centric (tag a gene locus to label associated protein complexes) assays.
Mesh-Begriff(e)	Multiprotein Complexes/chemistry ; Protein Interaction Mapping ; Proteomics
Chemische Substanzen	Multiprotein Complexes
Sprache	Englisch
Erscheinungsdatum	2019-01-31
Erscheinungsland	England
Dokumenttyp	Journal Article ; Research Support, Non-U.S. Gov't ; Review
ZDB-ID	2699932-8
ISSN	2046-1402 ; 2046-1402
ISSN (online)	2046-1402
ISSN	2046-1402
DOI	10.12688/f1000research.16903.1
Datenquelle	MEDical Literature Analysis and Retrieval System OnLINE

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Artikel: BioID organelle mapping: you are the company you keep.

Gaudreau-Lapierre, Antoine / Trinkle-Mulcahy, Laura

Trends in biochemical sciences

2021 Band 46, Heft 12, Seite(n) 950–952

Abstract: In a recent study, Go, Knight et al. combined a panel of protein markers with BioID proximity-dependent labeling to profile the composition of 20 distinct subcellular compartments. Comparison with similar global datasets acquired using imaging or ... ...

Abstract	In a recent study, Go, Knight et al. combined a panel of protein markers with BioID proximity-dependent labeling to profile the composition of 20 distinct subcellular compartments. Comparison with similar global datasets acquired using imaging or fractionation-based approaches confirmed the consistency of the results while highlighting unique advantages.
Mesh-Begriff(e)	Biotinylation ; Organelles/metabolism ; Protein Interaction Mapping/methods ; Proteins/metabolism
Chemische Substanzen	Proteins
Sprache	Englisch
Erscheinungsdatum	2021-09-28
Erscheinungsland	England
Dokumenttyp	Journal Article ; Research Support, Non-U.S. Gov't
ZDB-ID	194216-5
ISSN	1362-4326 ; 0968-0004 ; 0376-5067
ISSN (online)	1362-4326
ISSN	0968-0004 ; 0376-5067
DOI	10.1016/j.tibs.2021.09.003
Datenquelle	MEDical Literature Analysis and Retrieval System OnLINE

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Artikel ; Online: Mapping New Residents of the Mitochondrial Nucleoid.

Trinkle-Mulcahy, Laura

Cell chemical biology

2017 Band 24, Heft 3, Seite(n) 250–251

Abstract: In this issue of Cell Chemical Biology, Han et al. (2017) used a powerful combination of quantitative ratiometric mass spectrometry with APEX peroxidase-catalyzed proximity biotinylation to selectively highlight proteins associated with mitochondrial DNA ...

Abstract	In this issue of Cell Chemical Biology, Han et al. (2017) used a powerful combination of quantitative ratiometric mass spectrometry with APEX peroxidase-catalyzed proximity biotinylation to selectively highlight proteins associated with mitochondrial DNA above the background of contaminants and matrix proteins. In addition to identifying novel nucleoid factors, this study extends the APEX strategy to the proteomic mapping of non-membrane-bound multiprotein complexes.
Mesh-Begriff(e)	Biotinylation ; DNA, Mitochondrial ; Mitochondria/genetics ; Proteins ; Proteomics
Chemische Substanzen	DNA, Mitochondrial ; Proteins
Sprache	Englisch
Erscheinungsdatum	2017-03-15
Erscheinungsland	United States
Dokumenttyp	Journal Article ; Comment
ISSN	2451-9448
ISSN (online)	2451-9448
DOI	10.1016/j.chembiol.2017.03.006
Datenquelle	MEDical Literature Analysis and Retrieval System OnLINE

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Artikel ; Online: Cooperative assembly of filopodia by the formin FMNL2 and I-BAR domain protein IRTKS.

Fox, Sarah / Tran, Amanda / Trinkle-Mulcahy, Laura / Copeland, John W

The Journal of biological chemistry

2022 Band 298, Heft 11, Seite(n) 102512

Abstract: Filopodia are long finger-like actin-based structures that project out from the plasma membrane as cells navigate and explore their extracellular environment. The initiation of filopodia formation requires release of tension at the plasma membrane ... ...

Abstract	Filopodia are long finger-like actin-based structures that project out from the plasma membrane as cells navigate and explore their extracellular environment. The initiation of filopodia formation requires release of tension at the plasma membrane followed by the coordinated assembly of long unbranched actin filaments. Filopodia growth is maintained by a tip complex that promotes actin polymerization and protects the growing barbed ends of the actin fibers from capping proteins. Filopodia growth also depends on additional F-actin bundling proteins to stiffen the actin filaments as well as extension of the membrane sheath projecting from the cell periphery. These activities can be provided by a number of actin-binding and membrane-binding proteins including formins such as formin-like 2 (FMNL2) and FMNL3, and Inverse-Bin-Amphiphysin-Rvs (I-BAR) proteins such as IRTKS and IRSp53, but the specific requirement for these proteins in filopodia assembly is not clear. We report here that IRTKS and IRSp53 are FMNL2-binding proteins. Coexpression of FMNL2 with either I-BAR protein promotes cooperative filopodia assembly. We find IRTKS, but not IRSp53, is required for FMNL2-induced filopodia assembly, and FMNL2 and IRTKS are mutually dependent cofactors in this process. Our results suggest that the primary function for FMNL2 during filopodia assembly is binding to the plasma membrane and that regulation of actin dynamics by its formin homology 2 domain is secondary. From these results, we conclude that FMNL2 initiates filopodia assembly via an unexpected novel mechanism, by bending the plasma membrane to recruit IRTKS and thereby nucleate filopodia assembly.
Mesh-Begriff(e)	Pseudopodia/metabolism ; Formins ; Actins/metabolism ; Actin Cytoskeleton/metabolism ; Carrier Proteins/metabolism
Chemische Substanzen	Formins ; amphiphysin (147954-52-7) ; Actins ; Carrier Proteins
Sprache	Englisch
Erscheinungsdatum	2022-09-19
Erscheinungsland	United States
Dokumenttyp	Journal Article ; Research Support, Non-U.S. Gov't
ZDB-ID	2997-x
ISSN	1083-351X ; 0021-9258
ISSN (online)	1083-351X
ISSN	0021-9258
DOI	10.1016/j.jbc.2022.102512
Datenquelle	MEDical Literature Analysis and Retrieval System OnLINE

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Artikel ; Online: Recent advances in proximity-based labeling methods for interactome mapping [version 1; referees

Laura Trinkle-Mulcahy

F1000Research, Vol

2 approved]

2019 Band 8

Abstract: Proximity-based labeling has emerged as a powerful complementary approach to classic affinity purification of multiprotein complexes in the mapping of protein–protein interactions. Ongoing optimization of enzyme tags and delivery methods has improved ... ...

Abstract	Proximity-based labeling has emerged as a powerful complementary approach to classic affinity purification of multiprotein complexes in the mapping of protein–protein interactions. Ongoing optimization of enzyme tags and delivery methods has improved both temporal and spatial resolution, and the technique has been successfully employed in numerous small-scale (single complex mapping) and large-scale (network mapping) initiatives. When paired with quantitative proteomic approaches, the ability of these assays to provide snapshots of stable and transient interactions over time greatly facilitates the mapping of dynamic interactomes. Furthermore, recent innovations have extended biotin-based proximity labeling techniques such as BioID and APEX beyond classic protein-centric assays (tag a protein to label neighboring proteins) to include RNA-centric (tag an RNA species to label RNA-binding proteins) and DNA-centric (tag a gene locus to label associated protein complexes) assays.
Schlagwörter	Medicine ; R ; Science ; Q
Thema/Rubrik (Code)	612
Sprache	Englisch
Erscheinungsdatum	2019-01-01T00:00:00Z
Verlag	F1000 Research Ltd
Dokumenttyp	Artikel ; Online
Datenquelle	BASE - Bielefeld Academic Search Engine (Lebenswissenschaftliche Auswahl)

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Artikel ; Online: SPECC1L binds the myosin phosphatase complex MYPT1/PP1β and can regulate its distribution between microtubules and filamentous actin.

Mehta, Virja / Decan, Nathalie / Ooi, Sarah / Gaudreau-Lapierre, Antoine / Copeland, John W / Trinkle-Mulcahy, Laura

The Journal of biological chemistry

2023 Band 299, Heft 2, Seite(n) 102893

Abstract: The subcellular localization, activity , and substrate specificity of the serine/threonine protein phosphatase 1 catalytic subunit ( ... ...

Abstract	The subcellular localization, activity , and substrate specificity of the serine/threonine protein phosphatase 1 catalytic subunit (PP1
Mesh-Begriff(e)	Humans ; Actins/metabolism ; Microtubules/metabolism ; Myosin-Light-Chain Phosphatase/metabolism ; Phosphorylation ; Protein Phosphatase 1/metabolism ; Protein Binding
Chemische Substanzen	Actins ; Myosin-Light-Chain Phosphatase (EC 3.1.3.53) ; Protein Phosphatase 1 (EC 3.1.3.16) ; SPECC1 protein, human ; PPP1R12A protein, human (EC 3.1.3.53) ; PPP1CB protein, human (EC 3.1.3.16)
Sprache	Englisch
Erscheinungsdatum	2023-01-10
Erscheinungsland	United States
Dokumenttyp	Journal Article ; Research Support, Non-U.S. Gov't
ZDB-ID	2997-x
ISSN	1083-351X ; 0021-9258
ISSN (online)	1083-351X
ISSN	0021-9258
DOI	10.1016/j.jbc.2023.102893
Datenquelle	MEDical Literature Analysis and Retrieval System OnLINE

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Artikel ; Online: Nuclear High Mobility Group A2 (HMGA2) Interactome Revealed by Biotin Proximity Labeling.

Gaudreau-Lapierre, Antoine / Klonisch, Thomas / Nicolas, Hannah / Thanasupawat, Thatchawan / Trinkle-Mulcahy, Laura / Hombach-Klonisch, Sabine

International journal of molecular sciences

2023 Band 24, Heft 4

Abstract: The non-histone chromatin binding protein High Mobility Group AT-hook protein 2 (HMGA2) has important functions in chromatin remodeling, and genome maintenance and protection. Expression of HMGA2 is highest in embryonic stem cells, declines during cell ... ...

Abstract	The non-histone chromatin binding protein High Mobility Group AT-hook protein 2 (HMGA2) has important functions in chromatin remodeling, and genome maintenance and protection. Expression of HMGA2 is highest in embryonic stem cells, declines during cell differentiation and cell aging, but it is re-expressed in some cancers, where high HMGA2 expression frequently coincides with a poor prognosis. The nuclear functions of HMGA2 cannot be explained by binding to chromatin alone but involve complex interactions with other proteins that are incompletely understood. The present study used biotin proximity labeling, followed by proteomic analysis, to identify the nuclear interaction partners of HMGA2. We tested two different biotin ligase HMGA2 constructs (BioID2 and miniTurbo) with similar results, and identified known and new HMGA2 interaction partners, with functionalities mainly in chromatin biology. These HMGA2 biotin ligase fusion constructs offer exciting new possibilities for interactome discovery research, enabling the monitoring of nuclear HMGA2 interactomes during drug treatments.
Mesh-Begriff(e)	Biotin ; Cell Differentiation ; Chromatin ; Ligases ; Proteomics ; HMGA2 Protein
Chemische Substanzen	Biotin (6SO6U10H04) ; Chromatin ; Ligases (EC 6.-) ; HMGA2 Protein
Sprache	Englisch
Erscheinungsdatum	2023-02-20
Erscheinungsland	Switzerland
Dokumenttyp	Journal Article
ZDB-ID	2019364-6
ISSN	1422-0067 ; 1422-0067 ; 1661-6596
ISSN (online)	1422-0067
ISSN	1422-0067 ; 1661-6596
DOI	10.3390/ijms24044246
Datenquelle	MEDical Literature Analysis and Retrieval System OnLINE

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Artikel: Recent advances in large-scale protein interactome mapping.

Mehta, Virja / Trinkle-Mulcahy, Laura

F1000Research

2016 Band 5

Abstract: Protein-protein interactions (PPIs) underlie most, if not all, cellular functions. The comprehensive mapping of these complex networks of stable and transient associations thus remains a key goal, both for systems biology-based initiatives (where it can ... ...

Abstract	Protein-protein interactions (PPIs) underlie most, if not all, cellular functions. The comprehensive mapping of these complex networks of stable and transient associations thus remains a key goal, both for systems biology-based initiatives (where it can be combined with other 'omics' data to gain a better understanding of functional pathways and networks) and for focused biological studies. Despite the significant challenges of such an undertaking, major strides have been made over the past few years. They include improvements in the computation prediction of PPIs and the literature curation of low-throughput studies of specific protein complexes, but also an increase in the deposition of high-quality data from non-biased high-throughput experimental PPI mapping strategies into publicly available databases.
Sprache	Englisch
Erscheinungsdatum	2016
Erscheinungsland	England
Dokumenttyp	Journal Article ; Review
ZDB-ID	2699932-8
ISSN	2046-1402
ISSN	2046-1402
DOI	10.12688/f1000research.7629.1
Datenquelle	MEDical Literature Analysis and Retrieval System OnLINE

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Artikel ; Online: Expansion microscopy-based imaging of nuclear structures in cultured cells.

Gaudreau-Lapierre, Antoine / Mulatz, Kirk / Béïque, Jean-Claude / Trinkle-Mulcahy, Laura

STAR protocols

2021 Band 2, Heft 3, Seite(n) 100630

Abstract: Expansion microscopy is a sample preparation technique in which fixed and immunostained cells or tissues are embedded in a cross-linked network of swellable polyelectrolyte hydrogel that expands isotropically upon addition of deionized water. We utilize ... ...

Abstract	Expansion microscopy is a sample preparation technique in which fixed and immunostained cells or tissues are embedded in a cross-linked network of swellable polyelectrolyte hydrogel that expands isotropically upon addition of deionized water. We utilize the X10 method for tenfold expansion of U2OS cells with concurrent DNA staining. A custom 3D-printed gel cutter and chambered slides minimize gel drift, facilitating analysis of the components of nuclear structures at nanoscale resolution by conventional microscopy or Airyscan confocal imaging. For complete information on the generation and use of this protocol, please refer to Do et al. (2020).
Mesh-Begriff(e)	Cell Line ; Cell Nucleus/ultrastructure ; Microscopy/methods ; Reproducibility of Results ; Software
Sprache	Englisch
Erscheinungsdatum	2021-06-26
Erscheinungsland	United States
Dokumenttyp	Journal Article ; Research Support, Non-U.S. Gov't
ISSN	2666-1667
ISSN (online)	2666-1667
DOI	10.1016/j.xpro.2021.100630
Datenquelle	MEDical Literature Analysis and Retrieval System OnLINE

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Artikel: BioID organelle mapping: you are the company you keep

Gaudreau-Lapierre, Antoine / Trinkle-Mulcahy, Laura

Trends in biochemical sciences. 2021 Dec., v. 46, no. 12

2021

Abstract	In a recent study, Go, Knight et al. combined a panel of protein markers with BioID proximity-dependent labeling to profile the composition of 20 distinct subcellular compartments. Comparison with similar global datasets acquired using imaging or fractionation-based approaches confirmed the consistency of the results while highlighting unique advantages.
Schlagwörter	business enterprises ; data collection ; image analysis ; proteins
Sprache	Englisch
Erscheinungsverlauf	2021-12
Umfang	p. 950-952.
Erscheinungsort	Elsevier Ltd
Dokumenttyp	Artikel
ZDB-ID	194220-7
ISSN	0968-0004 ; 0376-5067
ISSN	0968-0004 ; 0376-5067
DOI	10.1016/j.tibs.2021.09.003
Datenquelle	NAL Katalog (AGRICOLA)

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