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  1. Artikel ; Online: Myosin-1a: A motor for microvillar membrane movement and mechanics.

    Tyska, Matthew J / Nambiar, Rajalakshmi

    Communicative & integrative biology

    2010  Band 3, Heft 1, Seite(n) 64–66

    Abstract: Myosin-1a is one of eight monomeric, membrane binding class I myosins expressed in vertebrates.1 As the most abundant actin-based motor protein found in the enterocyte microvillus, myosin-1a has long been known to interact with the apical membrane via a ... ...

    Abstract Myosin-1a is one of eight monomeric, membrane binding class I myosins expressed in vertebrates.1 As the most abundant actin-based motor protein found in the enterocyte microvillus, myosin-1a has long been known to interact with the apical membrane via a highly basic C-terminal tail domain.2 Several recent studies shed light on possible functional consequences of this protein/lipid interaction. In vitro and in vivo studies of microvillar function have revealed that myosin-1a can move apical membrane along core actin bundles, leading to the release of small vesicles from microvillar tips.3,4 Additional studies indicate that myosin-1a and other class I myosins contribute to membrane-cytoskeleton adhesion, which enables the apical membrane to resist deformation.5 These findings clearly position myosin-1a as an important player in apical membrane movement and structural stability. How this motor is able to fulfill these two seemingly distinct functions is currently unclear, but will serve as the focus of our discussion below.
    Sprache Englisch
    Erscheinungsdatum 2010-06-07
    Erscheinungsland United States
    Dokumenttyp Journal Article
    ZDB-ID 2451097-X
    ISSN 1942-0889 ; 1942-0889
    ISSN (online) 1942-0889
    ISSN 1942-0889
    DOI 10.4161/cib.3.1.10141
    Datenquelle MEDical Literature Analysis and Retrieval System OnLINE

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  2. Artikel: Fast position measurements with scanning line optical tweezers.

    Nambiar, Rajalakshmi / Meiners, Jens-Christian

    Optics letters

    2007  Band 27, Heft 10, Seite(n) 836–838

    Abstract: Scanning line optical tweezers are a powerful tool for the study of colloidal or biomolecular systems in the low-force regime. We present a fast, high-resolution particle position measurement scheme that extends the capabilities of these instruments into ...

    Abstract Scanning line optical tweezers are a powerful tool for the study of colloidal or biomolecular systems in the low-force regime. We present a fast, high-resolution particle position measurement scheme that extends the capabilities of these instruments into the realm of dynamic measurements. The technique is based on synchronous detection of forward-scattered laser light during a line scan. We demonstrate a position resolution of better than 50 nm for bandwidths of as much as 40 kHz for pairs of microspheres trapped in a flat line potential at center-to-center separations of 1.7-6 microm.
    Sprache Englisch
    Erscheinungsdatum 2007-03-16
    Erscheinungsland United States
    Dokumenttyp Journal Article
    ISSN 0146-9592
    ISSN 0146-9592
    DOI 10.1364/ol.27.000836
    Datenquelle MEDical Literature Analysis and Retrieval System OnLINE

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  3. Artikel ; Online: Myosin motor function: the ins and outs of actin-based membrane protrusions.

    Nambiar, Rajalakshmi / McConnell, Russell E / Tyska, Matthew J

    Cellular and molecular life sciences : CMLS

    2010  Band 67, Heft 8, Seite(n) 1239–1254

    Abstract: Cells build plasma membrane protrusions supported by parallel bundles of F-actin to enable a wide variety of biological functions, ranging from motility to host defense. Filopodia, microvilli and stereocilia are three such protrusions that have been the ... ...

    Abstract Cells build plasma membrane protrusions supported by parallel bundles of F-actin to enable a wide variety of biological functions, ranging from motility to host defense. Filopodia, microvilli and stereocilia are three such protrusions that have been the focus of intense biological and biophysical investigation in recent years. While it is evident that actin dynamics play a significant role in the formation of these organelles, members of the myosin superfamily have also been implicated as key players in the maintenance of protrusion architecture and function. Based on a simple analysis of the physical forces that control protrusion formation and morphology, as well as our review of available data, we propose that myosins play two general roles within these structures: (1) as cargo transporters to move critical regulatory components toward distal tips and (2) as mediators of membrane-cytoskeleton adhesion.
    Mesh-Begriff(e) Actins/metabolism ; Animals ; Cell Movement/physiology ; Cell Surface Extensions/metabolism ; Humans ; Myosins/physiology
    Chemische Substanzen Actins ; Myosins (EC 3.6.4.1)
    Sprache Englisch
    Erscheinungsdatum 2010-01-27
    Erscheinungsland Switzerland
    Dokumenttyp Journal Article ; Research Support, N.I.H., Extramural ; Research Support, Non-U.S. Gov't ; Review
    ZDB-ID 1358415-7
    ISSN 1420-9071 ; 1420-682X
    ISSN (online) 1420-9071
    ISSN 1420-682X
    DOI 10.1007/s00018-009-0254-5
    Datenquelle MEDical Literature Analysis and Retrieval System OnLINE

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  4. Artikel ; Online: Control of cell membrane tension by myosin-I.

    Nambiar, Rajalakshmi / McConnell, Russell E / Tyska, Matthew J

    Proceedings of the National Academy of Sciences of the United States of America

    2009  Band 106, Heft 29, Seite(n) 11972–11977

    Abstract: All cell functions that involve membrane deformation or a change in cell shape (e.g., endocytosis, exocytosis, cell motility, and cytokinesis) are regulated by membrane tension. While molecular contacts between the plasma membrane and the underlying ... ...

    Abstract All cell functions that involve membrane deformation or a change in cell shape (e.g., endocytosis, exocytosis, cell motility, and cytokinesis) are regulated by membrane tension. While molecular contacts between the plasma membrane and the underlying actin cytoskeleton are known to make significant contributions to membrane tension, little is known about the molecules that mediate these interactions. We used an optical trap to directly probe the molecular determinants of membrane tension in isolated organelles and in living cells. Here, we show that class I myosins, a family of membrane-binding, actin-based motor proteins, mediate membrane/cytoskeleton adhesion and thus, make major contributions to membrane tension. These studies show that class I myosins directly control the mechanical properties of the cell membrane; they also position these motor proteins as master regulators of cellular events involving membrane deformation.
    Mesh-Begriff(e) Animals ; Biomechanical Phenomena ; Cell Adhesion ; Cell Membrane/physiology ; Cell Survival ; Cytoskeleton/metabolism ; Epithelial Cells/cytology ; Epithelial Cells/metabolism ; Fibroblasts/cytology ; Fibroblasts/metabolism ; Green Fluorescent Proteins/metabolism ; Mice ; Mice, Knockout ; Microscopy, Confocal ; Microvilli/metabolism ; Myosin Heavy Chains/metabolism ; NIH 3T3 Cells ; Optical Tweezers ; Recombinant Fusion Proteins/metabolism ; Transfection
    Chemische Substanzen Myo1a protein, mouse ; Recombinant Fusion Proteins ; enhanced green fluorescent protein ; Green Fluorescent Proteins (147336-22-9) ; Myosin Heavy Chains (EC 3.6.4.1)
    Sprache Englisch
    Erscheinungsdatum 2009-07-02
    Erscheinungsland United States
    Dokumenttyp Journal Article ; Research Support, N.I.H., Extramural ; Research Support, Non-U.S. Gov't
    ZDB-ID 209104-5
    ISSN 1091-6490 ; 0027-8424
    ISSN (online) 1091-6490
    ISSN 0027-8424
    DOI 10.1073/pnas.0901641106
    Datenquelle MEDical Literature Analysis and Retrieval System OnLINE

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  5. Artikel: Myosin motor function: the ins and outs of actin-based membrane protrusions

    Nambiar, Rajalakshmi / McConnell, Russell E / Tyska, Matthew J

    Cellular and molecular life sciences CMLS. 2010 Apr., v. 67, no. 8

    2010  

    Abstract: Cells build plasma membrane protrusions supported by parallel bundles of F-actin to enable a wide variety of biological functions, ranging from motility to host defense. Filopodia, microvilli and stereocilia are three such protrusions that have been the ... ...

    Abstract Cells build plasma membrane protrusions supported by parallel bundles of F-actin to enable a wide variety of biological functions, ranging from motility to host defense. Filopodia, microvilli and stereocilia are three such protrusions that have been the focus of intense biological and biophysical investigation in recent years. While it is evident that actin dynamics play a significant role in the formation of these organelles, members of the myosin superfamily have also been implicated as key players in the maintenance of protrusion architecture and function. Based on a simple analysis of the physical forces that control protrusion formation and morphology, as well as our review of available data, we propose that myosins play two general roles within these structures: (1) as cargo transporters to move critical regulatory components toward distal tips and (2) as mediators of membrane-cytoskeleton adhesion.
    Sprache Englisch
    Erscheinungsverlauf 2010-04
    Umfang p. 1239-1254.
    Verlag SP Birkhäuser Verlag Basel
    Erscheinungsort Basel
    Dokumenttyp Artikel
    ZDB-ID 1358415-7
    ISSN 1420-9071 ; 1420-682X
    ISSN (online) 1420-9071
    ISSN 1420-682X
    DOI 10.1007/s00018-009-0254-5
    Datenquelle NAL Katalog (AGRICOLA)

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  6. Artikel: Control of cell membrane tension by myosin-I

    Nambiar, Rajalakshmi / McConnell, Russell E / Tyska, Matthew J

    Proceedings of the National Academy of Sciences of the United States of America. 2009 July 21, v. 106, no. 29

    2009  

    Abstract: All cell functions that involve membrane deformation or a change in cell shape (e.g., endocytosis, exocytosis, cell motility, and cytokinesis) are regulated by membrane tension. While molecular contacts between the plasma membrane and the underlying ... ...

    Abstract All cell functions that involve membrane deformation or a change in cell shape (e.g., endocytosis, exocytosis, cell motility, and cytokinesis) are regulated by membrane tension. While molecular contacts between the plasma membrane and the underlying actin cytoskeleton are known to make significant contributions to membrane tension, little is known about the molecules that mediate these interactions. We used an optical trap to directly probe the molecular determinants of membrane tension in isolated organelles and in living cells. Here, we show that class I myosins, a family of membrane-binding, actin-based motor proteins, mediate membrane/cytoskeleton adhesion and thus, make major contributions to membrane tension. These studies show that class I myosins directly control the mechanical properties of the cell membrane; they also position these motor proteins as master regulators of cellular events involving membrane deformation.
    Schlagwörter adhesion ; cell movement ; cytokinesis ; deformation ; endocytosis ; exocytosis ; mechanical properties ; microfilaments ; myosin ; optical traps ; organelles ; plasma membrane
    Sprache Englisch
    Erscheinungsverlauf 2009-0721
    Umfang p. 11972-11977.
    Erscheinungsort National Academy of Sciences
    Dokumenttyp Artikel
    ZDB-ID 209104-5
    ISSN 1091-6490 ; 0027-8424
    ISSN (online) 1091-6490
    ISSN 0027-8424
    DOI 10.1073/pnas.0901641106
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  7. Artikel: All-optical constant-force laser tweezers.

    Nambiar, Rajalakshmi / Gajraj, Arivalagan / Meiners, Jens-Christian

    Biophysical journal

    2004  Band 87, Heft 3, Seite(n) 1972–1980

    Abstract: Optical tweezers are a powerful tool for the study of single biomolecules. Many applications require that a molecule be held under constant tension while its extension is measured. We present two schemes based on scanning-line optical tweezers to ... ...

    Abstract Optical tweezers are a powerful tool for the study of single biomolecules. Many applications require that a molecule be held under constant tension while its extension is measured. We present two schemes based on scanning-line optical tweezers to accomplish this, providing all-optical alternatives to force-clamp traps that rely on electronic feedback to maintain constant-force conditions for the molecule. In these schemes, a laser beam is rapidly scanned along a line in the focal plane of the microscope objective, effectively creating an extended one-dimensional optical potential over distances of up to 8 microm. A position-independent lateral force acting on a trapped particle is created by either modulating the laser beam intensity during the scan or by using an asymmetric beam profile in the back focal plane of the microscope objective. With these techniques, forces of up to 2.69 pN have been applied over distances of up to 3.4 microm with residual spring constants of <26.6 fN/microm. We used these techniques in conjunction with a fast position measurement scheme to study the relaxation of lambda-DNA molecules against a constant external force with submillisecond time resolution. We compare the results to predictions from the wormlike chain model.
    Mesh-Begriff(e) Biophysical Phenomena ; Biophysics ; DNA/chemistry ; DNA/ultrastructure ; Lasers ; Light ; Micromanipulation/instrumentation ; Micromanipulation/methods ; Microscopy/methods ; Microspheres ; Models, Statistical ; Scattering, Radiation ; Stress, Mechanical ; Time Factors
    Chemische Substanzen DNA (9007-49-2)
    Sprache Englisch
    Erscheinungsdatum 2004-09
    Erscheinungsland United States
    Dokumenttyp Journal Article ; Research Support, Non-U.S. Gov't ; Research Support, U.S. Gov't, Non-P.H.S. ; Research Support, U.S. Gov't, P.H.S.
    ZDB-ID 218078-9
    ISSN 1542-0086 ; 0006-3495
    ISSN (online) 1542-0086
    ISSN 0006-3495
    DOI 10.1529/biophysj.103.037697
    Datenquelle MEDical Literature Analysis and Retrieval System OnLINE

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  8. Artikel ; Online: Enterocyte microvillus-derived vesicles detoxify bacterial products and regulate epithelial-microbial interactions.

    Shifrin, David A / McConnell, Russell E / Nambiar, Rajalakshmi / Higginbotham, James N / Coffey, Robert J / Tyska, Matthew J

    Current biology : CB

    2012  Band 22, Heft 7, Seite(n) 627–631

    Abstract: The continuous monolayer of intestinal epithelial cells (IECs) lining the gut lumen functions as the site of nutrient absorption and as a physical barrier to prevent the translocation of microbes and associated toxic compounds into the peripheral ... ...

    Abstract The continuous monolayer of intestinal epithelial cells (IECs) lining the gut lumen functions as the site of nutrient absorption and as a physical barrier to prevent the translocation of microbes and associated toxic compounds into the peripheral vasculature. IECs also express host defense proteins such as intestinal alkaline phosphatase (IAP), which detoxify bacterial products and prevent intestinal inflammation. Our laboratory recently showed that IAP is enriched on vesicles that are released from the tips of IEC microvilli and accumulate in the intestinal lumen. Here, we show that these native "lumenal vesicles" (LVs) (1) contain catalytically active IAP that can dephosphorylate lipopolysaccharide (LPS), (2) cluster on the surface of native lumenal bacteria, (3) prevent the adherence of enteropathogenic E. coli (EPEC) to epithelial monolayers, and (4) limit bacterial population growth. We also find that IECs upregulate LV production in response to EPEC and other Gram-negative pathogens. Together, these results suggest that microvillar vesicle shedding represents a novel mechanism for distributing host defense machinery into the intestinal lumen and that microvillus-derived LVs modulate epithelial-microbial interactions.
    Mesh-Begriff(e) Alkaline Phosphatase/metabolism ; Animals ; Caco-2 Cells ; Cytoplasmic Vesicles/metabolism ; Cytoplasmic Vesicles/microbiology ; Cytoplasmic Vesicles/ultrastructure ; Enterocytes/cytology ; Enterocytes/metabolism ; Enteropathogenic Escherichia coli/growth & development ; Enteropathogenic Escherichia coli/immunology ; Enteropathogenic Escherichia coli/metabolism ; Epithelial Cells/immunology ; Humans ; Intestine, Small/cytology ; Intestine, Small/metabolism ; Intestine, Small/microbiology ; Lipopolysaccharides/metabolism ; Microscopy, Electron, Transmission ; Microvilli/metabolism ; Microvilli/microbiology ; Microvilli/ultrastructure ; Myosin Heavy Chains/metabolism ; Myosin Type I/metabolism ; Rats
    Chemische Substanzen Lipopolysaccharides ; MYO1A protein, human ; Alkaline Phosphatase (EC 3.1.3.1) ; Myosin Type I (EC 3.6.1.-) ; Myosin Heavy Chains (EC 3.6.4.1)
    Sprache Englisch
    Erscheinungsdatum 2012-03-01
    Erscheinungsland England
    Dokumenttyp Journal Article ; Research Support, N.I.H., Extramural ; Research Support, Non-U.S. Gov't
    ZDB-ID 1071731-6
    ISSN 1879-0445 ; 0960-9822
    ISSN (online) 1879-0445
    ISSN 0960-9822
    DOI 10.1016/j.cub.2012.02.022
    Datenquelle MEDical Literature Analysis and Retrieval System OnLINE

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  9. Artikel ; Online: Detection of rare antigen-presenting cells through T cell-intrinsic meandering motility, mediated by Myo1g.

    Gérard, Audrey / Patino-Lopez, Genaro / Beemiller, Peter / Nambiar, Rajalakshmi / Ben-Aissa, Khadija / Liu, Yin / Totah, Fadi J / Tyska, Matthew J / Shaw, Stephen / Krummel, Matthew F

    Cell

    2014  Band 158, Heft 3, Seite(n) 492–505

    Abstract: To mount an immune response, T lymphocytes must successfully search for foreign material bound to the surface of antigen-presenting cells. How T cells optimize their chances of encountering and responding to these antigens is unknown. T cell motility in ... ...

    Abstract To mount an immune response, T lymphocytes must successfully search for foreign material bound to the surface of antigen-presenting cells. How T cells optimize their chances of encountering and responding to these antigens is unknown. T cell motility in tissues resembles a random or Levy walk and is regulated in part by external factors including chemokines and lymph-node topology, but motility parameters such as speed and propensity to turn may also be cell intrinsic. Here we found that the unconventional myosin 1g (Myo1g) motor generates membrane tension, enforces cell-intrinsic meandering search, and enhances T-DC interactions during lymph-node surveillance. Increased turning and meandering motility, as opposed to ballistic motility, is enhanced by Myo1g. Myo1g acts as a "turning motor" and generates a form of cellular "flânerie." Modeling and antigen challenges show that these intrinsically programmed elements of motility search are critical for the detection of rare cognate antigen-presenting cells.
    Mesh-Begriff(e) Animals ; Antigen-Presenting Cells/immunology ; Antigen-Presenting Cells/metabolism ; Cell Membrane/metabolism ; Cell Movement ; Immunologic Surveillance ; Lymph Nodes/immunology ; Mice ; Minor Histocompatibility Antigens ; Myosins/genetics ; Myosins/metabolism ; Receptors, Antigen, T-Cell/metabolism ; T-Lymphocytes/cytology ; T-Lymphocytes/immunology ; T-Lymphocytes/metabolism
    Chemische Substanzen Minor Histocompatibility Antigens ; Myo1g protein, mouse ; Receptors, Antigen, T-Cell ; Myosins (EC 3.6.4.1)
    Sprache Englisch
    Erscheinungsdatum 2014-08-01
    Erscheinungsland United States
    Dokumenttyp Journal Article ; Research Support, N.I.H., Extramural ; Research Support, N.I.H., Intramural ; Research Support, Non-U.S. Gov't
    ZDB-ID 187009-9
    ISSN 1097-4172 ; 0092-8674
    ISSN (online) 1097-4172
    ISSN 0092-8674
    DOI 10.1016/j.cell.2014.05.044
    Datenquelle MEDical Literature Analysis and Retrieval System OnLINE

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  10. Artikel ; Online: Differential localization and dynamics of class I myosins in the enterocyte microvillus.

    Benesh, Andrew E / Nambiar, Rajalakshmi / McConnell, Russell E / Mao, Suli / Tabb, David L / Tyska, Matthew J

    Molecular biology of the cell

    2010  Band 21, Heft 6, Seite(n) 970–978

    Abstract: Epithelial cells lining the intestinal tract build an apical array of microvilli known as the brush border. Each microvillus is a cylindrical membrane protrusion that is linked to a supporting actin bundle by myosin-1a (Myo1a). Mice lacking Myo1a ... ...

    Abstract Epithelial cells lining the intestinal tract build an apical array of microvilli known as the brush border. Each microvillus is a cylindrical membrane protrusion that is linked to a supporting actin bundle by myosin-1a (Myo1a). Mice lacking Myo1a demonstrate no overt physiological symptoms, suggesting that other myosins may compensate for the loss of Myo1a in these animals. To investigate changes in the microvillar myosin population that may limit the Myo1a KO phenotype, we performed proteomic analysis on WT and Myo1a KO brush borders. These studies revealed that WT brush borders also contain the short-tailed class I myosin, myosin-1d (Myo1d). Myo1d localizes to the terminal web and striking puncta at the tips of microvilli. In the absence of Myo1a, Myo1d peptide counts increase twofold; this motor also redistributes along the length of microvilli, into compartments normally occupied by Myo1a. FRAP studies demonstrate that Myo1a is less dynamic than Myo1d, providing a mechanistic explanation for the observed differential localization. These data suggest that Myo1d may be the primary compensating class I myosin in the Myo1a KO model; they also suggest that dynamics govern the localization and function of different yet closely related myosins that target common actin structures.
    Mesh-Begriff(e) Animals ; Cell Line ; Enterocytes/cytology ; Fluorescence Recovery After Photobleaching ; Mice ; Mice, Knockout ; Microvilli/metabolism ; Microvilli/ultrastructure ; Myosin Heavy Chains/genetics ; Myosin Heavy Chains/metabolism ; Myosins/genetics ; Myosins/metabolism ; Protein Isoforms/genetics ; Protein Isoforms/metabolism ; Proteomics/methods ; Rats ; Recombinant Fusion Proteins/genetics ; Recombinant Fusion Proteins/metabolism
    Chemische Substanzen Myo1a protein, mouse ; Protein Isoforms ; Recombinant Fusion Proteins ; Myo1d protein, mouse (EC 3.6.4.1) ; Myosin Heavy Chains (EC 3.6.4.1) ; Myosins (EC 3.6.4.1)
    Sprache Englisch
    Erscheinungsdatum 2010-01-20
    Erscheinungsland United States
    Dokumenttyp Journal Article ; Research Support, N.I.H., Extramural ; Research Support, Non-U.S. Gov't
    ZDB-ID 1098979-1
    ISSN 1939-4586 ; 1059-1524
    ISSN (online) 1939-4586
    ISSN 1059-1524
    DOI 10.1091/mbc.E09-07-0638
    Datenquelle MEDical Literature Analysis and Retrieval System OnLINE

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