Growth cone-specific functions of XMAP215 in restricting microtubule dynamics and promoting axonal outgrowth

Laura A. Lowery; Alina Stout; Anna E. Faris; Liya Ding; Michelle A. Baird; Michael W. Davidson; Gaudenz Danuser; David Van Vactor

doi:10.1186/1749-8104-8-22

Growth cone-specific functions of XMAP215 in restricting microtubule dynamics and promoting axonal outgrowth

Laura A. Lowery, Alina Stout, Anna E. Faris, Liya Ding, Michelle A. Baird, Michael W. Davidson, Gaudenz Danuser, David Van Vactor

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

31 Scopus citations

Abstract

Background: Microtubule (MT) regulators play essential roles in multiple aspects of neural development. In vitro reconstitution assays have established that the XMAP215/Dis1/TOG family of MT regulators function as MT 'plus-end-tracking proteins' (+TIPs) that act as processive polymerases to drive MT growth in all eukaryotes, but few studies have examined their functions in vivo. In this study, we use quantitative analysis of high-resolution live imaging to examine the function of XMAP215 in embryonic Xenopus laevis neurons.Results: Here, we show that XMAP215 is required for persistent axon outgrowth in vivo and ex vivo by preventing actomyosin-mediated axon retraction. Moreover, we discover that the effect of XMAP215 function on MT behavior depends on cell type and context. While partial knockdown leads to slower MT plus-end velocities in most cell types, it results in a surprising increase in MT plus-end velocities selective to growth cones. We investigate this further by using MT speckle microscopy to determine that differences in overall MT translocation are a major contributor of the velocity change within the growth cone. We also find that growth cone MT trajectories in the XMAP215 knockdown (KD) lack the constrained co-linearity that normally results from MT-F-actin interactions.Conclusions: Collectively, our findings reveal unexpected functions for XMAP215 in axon outgrowth and growth cone MT dynamics. Not only does XMAP215 balance actomyosin-mediated axon retraction, but it also affects growth cone MT translocation rates and MT trajectory colinearity, all of which depend on regulated linkages to F-actin. Thus, our analysis suggests that XMAP215 functions as more than a simple MT polymerase, and that in both axon and growth cone, XMAP215 contributes to the coupling between MTs and F-actin. This indicates that the function and regulation of XMAP215 may be significantly more complicated than previously appreciated, and points to the importance of future investigations of XMAP215 function during MT and F-actin interactions.

Original language	English (US)
Article number	22
Journal	Neural Development
Volume	8
Issue number	1
DOIs	https://doi.org/10.1186/1749-8104-8-22
State	Published - Dec 1 2013

Keywords

Actin
Cytoskeleton
Growth cone
Microtubule dynamics
Quantitative imaging
TOG
XMAP215

ASJC Scopus subject areas

Developmental Neuroscience

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10.1186/1749-8104-8-22

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@article{998528e2ffb345f988fda51731eac83a,

title = "Growth cone-specific functions of XMAP215 in restricting microtubule dynamics and promoting axonal outgrowth",

abstract = "Background: Microtubule (MT) regulators play essential roles in multiple aspects of neural development. In vitro reconstitution assays have established that the XMAP215/Dis1/TOG family of MT regulators function as MT 'plus-end-tracking proteins' (+TIPs) that act as processive polymerases to drive MT growth in all eukaryotes, but few studies have examined their functions in vivo. In this study, we use quantitative analysis of high-resolution live imaging to examine the function of XMAP215 in embryonic Xenopus laevis neurons.Results: Here, we show that XMAP215 is required for persistent axon outgrowth in vivo and ex vivo by preventing actomyosin-mediated axon retraction. Moreover, we discover that the effect of XMAP215 function on MT behavior depends on cell type and context. While partial knockdown leads to slower MT plus-end velocities in most cell types, it results in a surprising increase in MT plus-end velocities selective to growth cones. We investigate this further by using MT speckle microscopy to determine that differences in overall MT translocation are a major contributor of the velocity change within the growth cone. We also find that growth cone MT trajectories in the XMAP215 knockdown (KD) lack the constrained co-linearity that normally results from MT-F-actin interactions.Conclusions: Collectively, our findings reveal unexpected functions for XMAP215 in axon outgrowth and growth cone MT dynamics. Not only does XMAP215 balance actomyosin-mediated axon retraction, but it also affects growth cone MT translocation rates and MT trajectory colinearity, all of which depend on regulated linkages to F-actin. Thus, our analysis suggests that XMAP215 functions as more than a simple MT polymerase, and that in both axon and growth cone, XMAP215 contributes to the coupling between MTs and F-actin. This indicates that the function and regulation of XMAP215 may be significantly more complicated than previously appreciated, and points to the importance of future investigations of XMAP215 function during MT and F-actin interactions.",

keywords = "Actin, Cytoskeleton, Growth cone, Microtubule dynamics, Quantitative imaging, TOG, XMAP215",

author = "Lowery, {Laura A.} and Alina Stout and Faris, {Anna E.} and Liya Ding and Baird, {Michelle A.} and Davidson, {Michael W.} and Gaudenz Danuser and {Van Vactor}, David",

note = "Funding Information: We thank Drs. Tim Mitchison and Elizabeth Engle, as well as members of the Van Vactor and Danuser labs, for helpful discussions and constructive criticism. We thank Bob Freeman and Marc Kirschner for their generous assistance in learning Xenopus husbandry. We thank the Nikon Imaging Center at Harvard Medical School for expert advice and assistance in microscopy. This work was funded by: NRSA NIH F32 NS063512 fellowship and NIH K99 MH095768 award to LAL, Basic Science Partnership funding (https://bsp.med.harvard.edu/) to AEF, and NIH R01 NS035909 and NIH SBIR 2R44GM077774 to DVV and NIH U01 GM067230 to GD.",

year = "2013",

month = dec,

day = "1",

doi = "10.1186/1749-8104-8-22",

language = "English (US)",

volume = "8",

journal = "Neural Development",

issn = "1749-8104",

publisher = "BioMed Central",

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TY - JOUR

T1 - Growth cone-specific functions of XMAP215 in restricting microtubule dynamics and promoting axonal outgrowth

AU - Lowery, Laura A.

AU - Stout, Alina

AU - Faris, Anna E.

AU - Ding, Liya

AU - Baird, Michelle A.

AU - Davidson, Michael W.

AU - Danuser, Gaudenz

AU - Van Vactor, David

N1 - Funding Information: We thank Drs. Tim Mitchison and Elizabeth Engle, as well as members of the Van Vactor and Danuser labs, for helpful discussions and constructive criticism. We thank Bob Freeman and Marc Kirschner for their generous assistance in learning Xenopus husbandry. We thank the Nikon Imaging Center at Harvard Medical School for expert advice and assistance in microscopy. This work was funded by: NRSA NIH F32 NS063512 fellowship and NIH K99 MH095768 award to LAL, Basic Science Partnership funding (https://bsp.med.harvard.edu/) to AEF, and NIH R01 NS035909 and NIH SBIR 2R44GM077774 to DVV and NIH U01 GM067230 to GD.

PY - 2013/12/1

Y1 - 2013/12/1

N2 - Background: Microtubule (MT) regulators play essential roles in multiple aspects of neural development. In vitro reconstitution assays have established that the XMAP215/Dis1/TOG family of MT regulators function as MT 'plus-end-tracking proteins' (+TIPs) that act as processive polymerases to drive MT growth in all eukaryotes, but few studies have examined their functions in vivo. In this study, we use quantitative analysis of high-resolution live imaging to examine the function of XMAP215 in embryonic Xenopus laevis neurons.Results: Here, we show that XMAP215 is required for persistent axon outgrowth in vivo and ex vivo by preventing actomyosin-mediated axon retraction. Moreover, we discover that the effect of XMAP215 function on MT behavior depends on cell type and context. While partial knockdown leads to slower MT plus-end velocities in most cell types, it results in a surprising increase in MT plus-end velocities selective to growth cones. We investigate this further by using MT speckle microscopy to determine that differences in overall MT translocation are a major contributor of the velocity change within the growth cone. We also find that growth cone MT trajectories in the XMAP215 knockdown (KD) lack the constrained co-linearity that normally results from MT-F-actin interactions.Conclusions: Collectively, our findings reveal unexpected functions for XMAP215 in axon outgrowth and growth cone MT dynamics. Not only does XMAP215 balance actomyosin-mediated axon retraction, but it also affects growth cone MT translocation rates and MT trajectory colinearity, all of which depend on regulated linkages to F-actin. Thus, our analysis suggests that XMAP215 functions as more than a simple MT polymerase, and that in both axon and growth cone, XMAP215 contributes to the coupling between MTs and F-actin. This indicates that the function and regulation of XMAP215 may be significantly more complicated than previously appreciated, and points to the importance of future investigations of XMAP215 function during MT and F-actin interactions.

AB - Background: Microtubule (MT) regulators play essential roles in multiple aspects of neural development. In vitro reconstitution assays have established that the XMAP215/Dis1/TOG family of MT regulators function as MT 'plus-end-tracking proteins' (+TIPs) that act as processive polymerases to drive MT growth in all eukaryotes, but few studies have examined their functions in vivo. In this study, we use quantitative analysis of high-resolution live imaging to examine the function of XMAP215 in embryonic Xenopus laevis neurons.Results: Here, we show that XMAP215 is required for persistent axon outgrowth in vivo and ex vivo by preventing actomyosin-mediated axon retraction. Moreover, we discover that the effect of XMAP215 function on MT behavior depends on cell type and context. While partial knockdown leads to slower MT plus-end velocities in most cell types, it results in a surprising increase in MT plus-end velocities selective to growth cones. We investigate this further by using MT speckle microscopy to determine that differences in overall MT translocation are a major contributor of the velocity change within the growth cone. We also find that growth cone MT trajectories in the XMAP215 knockdown (KD) lack the constrained co-linearity that normally results from MT-F-actin interactions.Conclusions: Collectively, our findings reveal unexpected functions for XMAP215 in axon outgrowth and growth cone MT dynamics. Not only does XMAP215 balance actomyosin-mediated axon retraction, but it also affects growth cone MT translocation rates and MT trajectory colinearity, all of which depend on regulated linkages to F-actin. Thus, our analysis suggests that XMAP215 functions as more than a simple MT polymerase, and that in both axon and growth cone, XMAP215 contributes to the coupling between MTs and F-actin. This indicates that the function and regulation of XMAP215 may be significantly more complicated than previously appreciated, and points to the importance of future investigations of XMAP215 function during MT and F-actin interactions.

KW - Actin

KW - Cytoskeleton

KW - Growth cone

KW - Microtubule dynamics

KW - Quantitative imaging

KW - TOG

KW - XMAP215

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DO - 10.1186/1749-8104-8-22

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AN - SCOPUS:84888343833

SN - 1749-8104

VL - 8

JO - Neural Development

JF - Neural Development

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ER -

Growth cone-specific functions of XMAP215 in restricting microtubule dynamics and promoting axonal outgrowth

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