Laccase-dependent lignification of secondary cell walls of protoxylem tracheary elements in Arabidopsis thaliana

Lignin is a phenolic polymer that plays important roles in the structural integrity of plants. Both peroxidases and laccases have been implicated in the polymerization of lignin, and mutant analyses have conclusively demonstrated a role for laccases in lignification of Arabidopsis thaliana stems....

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Main Author: Benske, Anika
Language:English
Published: University of British Columbia 2014
Online Access:http://hdl.handle.net/2429/50247
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spelling ndltd-UBC-oai-circle.library.ubc.ca-2429-502472018-01-05T17:27:37Z Laccase-dependent lignification of secondary cell walls of protoxylem tracheary elements in Arabidopsis thaliana Benske, Anika Lignin is a phenolic polymer that plays important roles in the structural integrity of plants. Both peroxidases and laccases have been implicated in the polymerization of lignin, and mutant analyses have conclusively demonstrated a role for laccases in lignification of Arabidopsis thaliana stems. However, the oxidative enzymes that polymerize lignin in protoxylem tracheary elements (TEs) have not been defined. Induction of the master transcription factor VASCULAR RELATED NAC-DOMAIN 7 (VND7) causes systemic transdifferentiation into protoxylem TEs, providing an inducible-experimental model system to study protoxylem TE differentiation. The transcriptome of these lines has been well characterized, and two laccases, LAC4 and LAC17, are strongly expressed following induction of protoxylem TE development. To test if LAC4 and LAC17 are necessary for the lignification of protoxylem TEs, the inducible VND7 construct was transformed into the lac4-2/lac17 double mutant background and fluorescently labeled monolignols were exogenously applied to differentiating protoxylem TEs. Labeled polymerized lignin was only detected in the wild-type protoxylem TEs, but not in lac4-2/lac17 protoxylem TEs. To test if laccases alone are sufficient to promote lignification, the constitutive 35S promoter was used to drive either LAC4 or LAC17 in wild-type plants, resulting in strong ectopic lignification of primary cell walls upon application of fluorescently labeled monolignols. Fluorescently tagged laccases were transformed into the inducible protoxylem TEs system, where they specifically localize to the secondary, but not primary, cell walls of protoxylem tracheary elements. This research shows that LAC4 and LAC17 are necessary and sufficient for the lignification of secondary cell wall domains of protoxylem TEs and that they are specifically localized to these domains. Science, Faculty of Botany, Department of Graduate 2014-08-28T15:08:33Z 2014-08-28T15:08:33Z 2014 2014-11 Text Thesis/Dissertation http://hdl.handle.net/2429/50247 eng Attribution-NonCommercial-NoDerivs 2.5 Canada http://creativecommons.org/licenses/by-nc-nd/2.5/ca/ University of British Columbia
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language English
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description Lignin is a phenolic polymer that plays important roles in the structural integrity of plants. Both peroxidases and laccases have been implicated in the polymerization of lignin, and mutant analyses have conclusively demonstrated a role for laccases in lignification of Arabidopsis thaliana stems. However, the oxidative enzymes that polymerize lignin in protoxylem tracheary elements (TEs) have not been defined. Induction of the master transcription factor VASCULAR RELATED NAC-DOMAIN 7 (VND7) causes systemic transdifferentiation into protoxylem TEs, providing an inducible-experimental model system to study protoxylem TE differentiation. The transcriptome of these lines has been well characterized, and two laccases, LAC4 and LAC17, are strongly expressed following induction of protoxylem TE development. To test if LAC4 and LAC17 are necessary for the lignification of protoxylem TEs, the inducible VND7 construct was transformed into the lac4-2/lac17 double mutant background and fluorescently labeled monolignols were exogenously applied to differentiating protoxylem TEs. Labeled polymerized lignin was only detected in the wild-type protoxylem TEs, but not in lac4-2/lac17 protoxylem TEs. To test if laccases alone are sufficient to promote lignification, the constitutive 35S promoter was used to drive either LAC4 or LAC17 in wild-type plants, resulting in strong ectopic lignification of primary cell walls upon application of fluorescently labeled monolignols. Fluorescently tagged laccases were transformed into the inducible protoxylem TEs system, where they specifically localize to the secondary, but not primary, cell walls of protoxylem tracheary elements. This research shows that LAC4 and LAC17 are necessary and sufficient for the lignification of secondary cell wall domains of protoxylem TEs and that they are specifically localized to these domains. === Science, Faculty of === Botany, Department of === Graduate
author Benske, Anika
spellingShingle Benske, Anika
Laccase-dependent lignification of secondary cell walls of protoxylem tracheary elements in Arabidopsis thaliana
author_facet Benske, Anika
author_sort Benske, Anika
title Laccase-dependent lignification of secondary cell walls of protoxylem tracheary elements in Arabidopsis thaliana
title_short Laccase-dependent lignification of secondary cell walls of protoxylem tracheary elements in Arabidopsis thaliana
title_full Laccase-dependent lignification of secondary cell walls of protoxylem tracheary elements in Arabidopsis thaliana
title_fullStr Laccase-dependent lignification of secondary cell walls of protoxylem tracheary elements in Arabidopsis thaliana
title_full_unstemmed Laccase-dependent lignification of secondary cell walls of protoxylem tracheary elements in Arabidopsis thaliana
title_sort laccase-dependent lignification of secondary cell walls of protoxylem tracheary elements in arabidopsis thaliana
publisher University of British Columbia
publishDate 2014
url http://hdl.handle.net/2429/50247
work_keys_str_mv AT benskeanika laccasedependentlignificationofsecondarycellwallsofprotoxylemtrachearyelementsinarabidopsisthaliana
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