Structure-function analysis of rgs1 in magnaporthe oryzae : role of DEP domains in subcellular targeting

Structure-function analysis of rgs1 in magnaporthe oryzae : role of DEP domains in subcellular targeting

Rgs1, a prototypical Regulator of G protein Signaling, negatively modulates the cyclic AMP pathway thereby influencing various aspects of asexual development and pathogenesis in the rice-blast fungus Magnaporthe oryzae. Rgs1 possesses tandem DEP motifs (termed DEP-A and DEP-B; for Dishevelled, Egl-1...

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Main Authors: Ramanujam, Ravikrishna., Yishi, Xu., Liu, Hao., Naqvi, Naweed Issak.
Other Authors: School of Biological Sciences
Format: Article
Language:English
Published: 2013
Online Access:https://hdl.handle.net/10356/95053
http://hdl.handle.net/10220/9214
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Language: English
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spelling sg-ntu-dr.10356-950532023-02-28T16:56:19Z Structure-function analysis of rgs1 in magnaporthe oryzae : role of DEP domains in subcellular targeting Ramanujam, Ravikrishna. Yishi, Xu. Liu, Hao. Naqvi, Naweed Issak. School of Biological Sciences Rgs1, a prototypical Regulator of G protein Signaling, negatively modulates the cyclic AMP pathway thereby influencing various aspects of asexual development and pathogenesis in the rice-blast fungus Magnaporthe oryzae. Rgs1 possesses tandem DEP motifs (termed DEP-A and DEP-B; for Dishevelled, Egl-10, Pleckstrin) at the N-terminus, and a Gα-GTP interacting RGS catalytic core domain at the C-terminus. In this study, we focused on gaining further insights into the mechanisms of Rgs1 regulation and subcellular localization by characterizing the role(s) of the individual domains and the full-length protein during asexual development and pathogenesis in Magnaporthe. Methodology/Principal Findings: Utilizing western blot analysis and specific antisera against the N- and C-terminal halves of Rgs1, we identify and report the in vivo endoproteolytic processing/cleavage of full-length Rgs1 that yields an N-terminal DEP and a RGS core domain. Independent expression of the resultant DEP-DEP half (N-Rgs1) or RGS core (C-Rgs1) fragments, failed to complement the rgs1Δ defects in colony morphology, aerial hyphal growth, surface hydrophobicity, conidiation, appressorium formation and infection. Interestingly, the full-length Rgs1-mCherry, as well as the tagged N-terminal DEP domains (individually or in conjunction) localized to distinct punctate vesicular structures in the cytosol, while the catalytic RGS core motif was predominantly vacuolar. Published version 2013-02-21T07:03:21Z 2019-12-06T19:07:22Z 2013-02-21T07:03:21Z 2019-12-06T19:07:22Z 2012 2012 Journal Article Ramanujam, R., Yishi, X., Liu, H., & Naqvi, N. I. (2012). Structure-function analysis of rgs1 in magnaporthe oryzae : role of DEP domains in subcellular targeting. PLoS ONE, 7(7). 1932-6203 https://hdl.handle.net/10356/95053 http://hdl.handle.net/10220/9214 10.1371/journal.pone.0041084 22927898 en PLoS ONE © 2012 The Authors. application/pdf
institution Nanyang Technological University
building NTU Library
continent Asia
country Singapore
Singapore
content_provider NTU Library
collection DR-NTU
language English
description Rgs1, a prototypical Regulator of G protein Signaling, negatively modulates the cyclic AMP pathway thereby influencing various aspects of asexual development and pathogenesis in the rice-blast fungus Magnaporthe oryzae. Rgs1 possesses tandem DEP motifs (termed DEP-A and DEP-B; for Dishevelled, Egl-10, Pleckstrin) at the N-terminus, and a Gα-GTP interacting RGS catalytic core domain at the C-terminus. In this study, we focused on gaining further insights into the mechanisms of Rgs1 regulation and subcellular localization by characterizing the role(s) of the individual domains and the full-length protein during asexual development and pathogenesis in Magnaporthe. Methodology/Principal Findings: Utilizing western blot analysis and specific antisera against the N- and C-terminal halves of Rgs1, we identify and report the in vivo endoproteolytic processing/cleavage of full-length Rgs1 that yields an N-terminal DEP and a RGS core domain. Independent expression of the resultant DEP-DEP half (N-Rgs1) or RGS core (C-Rgs1) fragments, failed to complement the rgs1Δ defects in colony morphology, aerial hyphal growth, surface hydrophobicity, conidiation, appressorium formation and infection. Interestingly, the full-length Rgs1-mCherry, as well as the tagged N-terminal DEP domains (individually or in conjunction) localized to distinct punctate vesicular structures in the cytosol, while the catalytic RGS core motif was predominantly vacuolar.
author2 School of Biological Sciences
author_facet School of Biological Sciences
Ramanujam, Ravikrishna.
Yishi, Xu.
Liu, Hao.
Naqvi, Naweed Issak.
format Article
author Ramanujam, Ravikrishna.
Yishi, Xu.
Liu, Hao.
Naqvi, Naweed Issak.
spellingShingle Ramanujam, Ravikrishna.
Yishi, Xu.
Liu, Hao.
Naqvi, Naweed Issak.
Structure-function analysis of rgs1 in magnaporthe oryzae : role of DEP domains in subcellular targeting
author_sort Ramanujam, Ravikrishna.
title Structure-function analysis of rgs1 in magnaporthe oryzae : role of DEP domains in subcellular targeting
title_short Structure-function analysis of rgs1 in magnaporthe oryzae : role of DEP domains in subcellular targeting
title_full Structure-function analysis of rgs1 in magnaporthe oryzae : role of DEP domains in subcellular targeting
title_fullStr Structure-function analysis of rgs1 in magnaporthe oryzae : role of DEP domains in subcellular targeting
title_full_unstemmed Structure-function analysis of rgs1 in magnaporthe oryzae : role of DEP domains in subcellular targeting
title_sort structure-function analysis of rgs1 in magnaporthe oryzae : role of dep domains in subcellular targeting
publishDate 2013
url https://hdl.handle.net/10356/95053
http://hdl.handle.net/10220/9214
_version_ 1759853429158576128

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