The phytochrome (phy)-interacting basic helix-loop-helix transcription factors (PIFs) constitutively sustain the etiolated state of dark-germinated seedlings by actively repressing deetiolation in darkness. This action is rapidly reversed upon light exposure by phy-induced proteolytic degradation of the PIFs. Here, we combined a microarray-based approach with a functional profiling strategy and identified four PIF3-regulated genes misexpressed in the dark (MIDAs) that are novel regulators of seedling deetiolation. We provide evidence that each one of these four MIDA genes regulates a specific facet of etiolation (hook maintenance, cotyledon appression, or hypocotyl elongation), indicating that there is branching in the signaling that PIF3 relays. Furthermore, combining inferred MIDA gene function from mutant analyses with their expression profiles in response to light-induced degradation of PIF3 provides evidence consistent with a model where the action of the PIF3/MIDA regulatory network enables an initial fast response to the light and subsequently prevents an overresponse to the initial light trigger, thus optimizing the seedling deetiolation process. Collectively, the data suggest that at least part of the phy/PIF system acts through these four MIDAs to initiate and optimize seedling deetiolation, and that this mechanism might allow the implementation of spatial (i.e., organ-specific) and temporal responses during the photomorphogenic program.

Functional profiling identifies genes involved in organ-specific branches of the PIF3 regulatory network in Arabidopsis / M. Sentandreu, G. Martín, N. González-Schain, P. Leivar, J. Soy, J.M. Tepperman, P.H. Quail, E. Monte. - In: PLANT CELL. - ISSN 1040-4651. - 23:11(2011 Nov), pp. 3974-3991. [10.1105/tpc.111.088161]

Functional profiling identifies genes involved in organ-specific branches of the PIF3 regulatory network in Arabidopsis

N. González-Schain;
2011

Abstract

The phytochrome (phy)-interacting basic helix-loop-helix transcription factors (PIFs) constitutively sustain the etiolated state of dark-germinated seedlings by actively repressing deetiolation in darkness. This action is rapidly reversed upon light exposure by phy-induced proteolytic degradation of the PIFs. Here, we combined a microarray-based approach with a functional profiling strategy and identified four PIF3-regulated genes misexpressed in the dark (MIDAs) that are novel regulators of seedling deetiolation. We provide evidence that each one of these four MIDA genes regulates a specific facet of etiolation (hook maintenance, cotyledon appression, or hypocotyl elongation), indicating that there is branching in the signaling that PIF3 relays. Furthermore, combining inferred MIDA gene function from mutant analyses with their expression profiles in response to light-induced degradation of PIF3 provides evidence consistent with a model where the action of the PIF3/MIDA regulatory network enables an initial fast response to the light and subsequently prevents an overresponse to the initial light trigger, thus optimizing the seedling deetiolation process. Collectively, the data suggest that at least part of the phy/PIF system acts through these four MIDAs to initiate and optimize seedling deetiolation, and that this mechanism might allow the implementation of spatial (i.e., organ-specific) and temporal responses during the photomorphogenic program.
English
Gene Expression Regulation, Plant ; Arabidopsis ; Arabidopsis Proteins ; Basic Helix-Loop-Helix Transcription Factors ; Cotyledon ; Darkness ; Gene Expression Profiling ; Hypocotyl ; Light ; Mutation ; Organ Specificity ; Seedling
Settore BIO/11 - Biologia Molecolare
Articolo
Esperti anonimi
Ricerca pura
nov-2011
American Society of Plant Biologists
23
11
3974
3991
18
Pubblicato
Periodico con rilevanza internazionale
info:eu-repo/semantics/article
Functional profiling identifies genes involved in organ-specific branches of the PIF3 regulatory network in Arabidopsis / M. Sentandreu, G. Martín, N. González-Schain, P. Leivar, J. Soy, J.M. Tepperman, P.H. Quail, E. Monte. - In: PLANT CELL. - ISSN 1040-4651. - 23:11(2011 Nov), pp. 3974-3991. [10.1105/tpc.111.088161]
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Article (author)
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M. Sentandreu, G. Martín, N. González-Schain, P. Leivar, J. Soy, J.M. Tepperman, P.H. Quail, E. Monte
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Utilizza questo identificativo per citare o creare un link a questo documento: https://hdl.handle.net/2434/233118
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