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Identification of Proteins Required for Precise Positioning of Apc2 in Dendrites

In Drosophila neurons, uniform minus-end-out polarity in dendrites is maintained in part by kinesin-2-mediated steering of growing microtubules at branch points. Apc links the kinesin motor to growing microtubule plus ends and Apc2 recruits Apc to branch points where it functions. Because Apc2 acts...

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Autores principales: Weiner, Alexis T., Seebold, Dylan Y., Michael, Nick L., Guignet, Michelle, Feng, Chengye, Follick, Brandon, Yusko, Brandon A., Wasilko, Nathan P., Torres-Gutierrez, Pedro, Rolls, Melissa M.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Genetics Society of America 2018
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5940173/
https://www.ncbi.nlm.nih.gov/pubmed/29602811
http://dx.doi.org/10.1534/g3.118.200205
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author Weiner, Alexis T.
Seebold, Dylan Y.
Michael, Nick L.
Guignet, Michelle
Feng, Chengye
Follick, Brandon
Yusko, Brandon A.
Wasilko, Nathan P.
Torres-Gutierrez, Pedro
Rolls, Melissa M.
author_facet Weiner, Alexis T.
Seebold, Dylan Y.
Michael, Nick L.
Guignet, Michelle
Feng, Chengye
Follick, Brandon
Yusko, Brandon A.
Wasilko, Nathan P.
Torres-Gutierrez, Pedro
Rolls, Melissa M.
author_sort Weiner, Alexis T.
collection PubMed
description In Drosophila neurons, uniform minus-end-out polarity in dendrites is maintained in part by kinesin-2-mediated steering of growing microtubules at branch points. Apc links the kinesin motor to growing microtubule plus ends and Apc2 recruits Apc to branch points where it functions. Because Apc2 acts to concentrate other steering proteins to branch points, we wished to understand how Apc2 is targeted. From an initial broad candidate RNAi screen, we found Miro (a mitochondrial transport protein), Ank2, Axin, spastin and Rac1 were required to position Apc2-GFP at dendrite branch points. YFP-Ank2-L8, Axin-GFP and mitochondria also localized to branch points suggesting the screen identified relevant proteins. By performing secondary screens, we found that energy production by mitochondria was key for Apc2-GFP positioning and spastin acted upstream of mitochondria. Ank2 seems to act independently from other players, except its membrane partner, Neuroglian (Nrg). Rac1 likely acts through Arp2/3 to generate branched actin to help recruit Apc2-GFP. Axin can function in a variety of wnt signaling pathways, one of which includes heterotrimeric G proteins and Frizzleds. Knockdown of Gαs, Gαo, Fz and Fz2, reduced targeting of Apc2 and Axin to branch points. Overall our data suggest that mitochondrial energy production, Nrg/Ank2, branched actin generated by Arp2/3 and Fz/G proteins/Axin function as four modules that control localization of the microtubule regulator Apc2 to its site of action in dendrite branch points.
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spelling pubmed-59401732018-05-10 Identification of Proteins Required for Precise Positioning of Apc2 in Dendrites Weiner, Alexis T. Seebold, Dylan Y. Michael, Nick L. Guignet, Michelle Feng, Chengye Follick, Brandon Yusko, Brandon A. Wasilko, Nathan P. Torres-Gutierrez, Pedro Rolls, Melissa M. G3 (Bethesda) Investigations In Drosophila neurons, uniform minus-end-out polarity in dendrites is maintained in part by kinesin-2-mediated steering of growing microtubules at branch points. Apc links the kinesin motor to growing microtubule plus ends and Apc2 recruits Apc to branch points where it functions. Because Apc2 acts to concentrate other steering proteins to branch points, we wished to understand how Apc2 is targeted. From an initial broad candidate RNAi screen, we found Miro (a mitochondrial transport protein), Ank2, Axin, spastin and Rac1 were required to position Apc2-GFP at dendrite branch points. YFP-Ank2-L8, Axin-GFP and mitochondria also localized to branch points suggesting the screen identified relevant proteins. By performing secondary screens, we found that energy production by mitochondria was key for Apc2-GFP positioning and spastin acted upstream of mitochondria. Ank2 seems to act independently from other players, except its membrane partner, Neuroglian (Nrg). Rac1 likely acts through Arp2/3 to generate branched actin to help recruit Apc2-GFP. Axin can function in a variety of wnt signaling pathways, one of which includes heterotrimeric G proteins and Frizzleds. Knockdown of Gαs, Gαo, Fz and Fz2, reduced targeting of Apc2 and Axin to branch points. Overall our data suggest that mitochondrial energy production, Nrg/Ank2, branched actin generated by Arp2/3 and Fz/G proteins/Axin function as four modules that control localization of the microtubule regulator Apc2 to its site of action in dendrite branch points. Genetics Society of America 2018-03-30 /pmc/articles/PMC5940173/ /pubmed/29602811 http://dx.doi.org/10.1534/g3.118.200205 Text en Copyright © 2018 Weiner et al. http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution 4.0 International License (http://creativecommons.org/licenses/by/4.0/), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Investigations
Weiner, Alexis T.
Seebold, Dylan Y.
Michael, Nick L.
Guignet, Michelle
Feng, Chengye
Follick, Brandon
Yusko, Brandon A.
Wasilko, Nathan P.
Torres-Gutierrez, Pedro
Rolls, Melissa M.
Identification of Proteins Required for Precise Positioning of Apc2 in Dendrites
title Identification of Proteins Required for Precise Positioning of Apc2 in Dendrites
title_full Identification of Proteins Required for Precise Positioning of Apc2 in Dendrites
title_fullStr Identification of Proteins Required for Precise Positioning of Apc2 in Dendrites
title_full_unstemmed Identification of Proteins Required for Precise Positioning of Apc2 in Dendrites
title_short Identification of Proteins Required for Precise Positioning of Apc2 in Dendrites
title_sort identification of proteins required for precise positioning of apc2 in dendrites
topic Investigations
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5940173/
https://www.ncbi.nlm.nih.gov/pubmed/29602811
http://dx.doi.org/10.1534/g3.118.200205
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