- Email: [email protected]
Regulation of MYB and bHLH Transcription Factors: A Glance at the Protein Level
Accepted Manuscript Regulation of MYB and bHLH transcription factors – a glance at the protein level Marie Pireyre, Meike Burow PII:
S1674-2052(14)00048-3
DOI:
10.1016/j.molp.2014.11.022
Reference:
MOLP 47
To appear in:
MOLECULAR PLANT
Received Date: 1 September 2014 Revised Date:
10 November 2014
Accepted Date: 24 November 2014
Please cite this article as: Pireyre M., and Burow M. (2014). Regulation of MYB and bHLH transcription factors – a glance at the protein level. Mol. Plant. doi: 10.1016/j.molp.2014.11.022. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
ACCEPTED MANUSCRIPT
Title:
2
Regulation of MYB and bHLH transcription factors – a glance at the protein level
3 4
Running title:
6
Protein level regulation of transcription factors
7
Short summary:
This review summarizes the recent progress on molecular regulatory mechanisms of plant transcription factor families MYBs and bHLHs with focus on post-transcriptional modifications such as ubiquitination, phosphorylation, acetylation, and nitrosylation. We conclude by pointing to potential applications of state of the art techniques required to better understand the molecular basis of plant responses to environmental changes.
13
M AN U
8 9 10 11 12
SC
5
RI PT
1
Marie Pireyre and Meike Burow
15
DynaMo DNRF Center of Excellence , Department of Plant and Environmental Sciences,
16
Faculty of Science, University of Copenhagen, Thorvaldsensvej 40, 1871 Frederiksberg C,
17
Denmark
TE D
14
18 Corresponding author:
20
Meike Burow
21
Department of Plant and Environmental Sciences
22
Faculty of Science
23
University of Copenhagen
24
Thorvaldsensvej 40
25
1871 Frederiksberg C, Denmark
26
E-Mail: [email protected]
27
Phone: +45-35 33 37 73
28
Fax: +45-35 28 33 33
AC C
EP
19
ACCEPTED MANUSCRIPT
29
Abstract In complex, constantly changing environments, plants have developed astonishing
31
survival strategies. These elaborated strategies rely on rapid and precise gene regulation
32
mediated by transcription factors (TFs). TFs represent a large fraction of plant genomes and
33
among them, MYBs and bHLHs have unique inherent properties specific to plants. Proteins of
34
these two TF families can act as homo- or heterodimers, associate with proteins from other
35
protein families or form MYB/bHLH complexes to regulate distinct cellular processes. The
36
ability of MYBs and bHLHs to interact with multiple protein partners has evolved to keep up
37
with the increased metabolic complexity of multi-cellular organisms. Association and
38
disassociation of dynamic TF complexes in response to developmental and environmental cues
39
are controlled through a plethora of regulatory mechanisms specifically modulating TF activity.
40
Regulation of TFs at the protein level is critical for efficient and precise control of their activity
41
and thus provides the mechanistic basis for a rapid on-and-off switch of TF activity. In this
42
review, examples of post-translational modifications, protein-protein interaction and subcellular
43
mobilization of TFs will be discussed with regard to the relevance of these regulatory
44
mechanisms for the specific activation of MYBs and bHLHs in response to a given
45
environmental stimulus.
SC
M AN U
TE D
46
RI PT
30
Keywords: transcription factor, MYB, bHLH, post-translational modification, protein-protein
48
interaction, transcriptional regulation
AC C
49
EP
47
50
List of abbreviations: ABA, abscisic acid; bHLH, basic Helix-Loop-Helix; COI-1, coronatine-
51
insensitive protein 1; DBD, DNA-binding domain; GA, Gibberellic acid; HtH, Helix-turn-Helix;
52
HR, Hypersensitive Response; JA, jasmonic acid; JAZ; jasmonate ZIM-domain protein; MBW,
53
MYB/bHLH/WD40 complex; MTTF, membrane-tethered transcription factor; NLS, nuclear
54
localization signal; PPI, protein-protein interaction; PTM, post-transcriptional modification; SA,
55
salicylic acid; SUMO, Small Ubiquitin Modifier; TAD, transcriptional activation domain; TF,
56
transcription factor; UPS, Ubiquitin-Proteasome System.
ACCEPTED MANUSCRIPT
57
Introduction
58 In multicellular organisms, precise gene expression in time and space is regulated by
60
transcription factors (TFs). Mutants affected in spatio-temporal transcriptional regulation often
61
show dramatic developmental phenotypes underlining the importance of the functions of TFs and
62
the importance of efficient on-and-off switches for their activity. In Arabidopsis thaliana,
63
between 6-10% of all genes encode TFs in contrast to only 3% in Drosophila melanogaster and
64
5% in humans. This relatively large number of TFs might allow plants to rapidly adapt to the
65
changing environments they encounter, e.g. by synthesizing, transporting, and relocating
66
metabolites, RNAs, and proteins. A large proportion of the TFs in Arabidopsis are MYB (339)
67
and basic Helix-Loop-Helix (bHLH; 162) TFs. The members of these two transcription factor
68
families can act as homodimers, as heterodimers consisting of proteins from the same family, or
69
in complexes with TFs from other protein families. Interestingly, many cases of MYB/bHLH
70
complexes have been described and the parallel evolution of these two TF families has been
71
associated with the developmental and metabolic plasticity found in plants (Feller et al., 2011).
72
The structural, evolutionary and functional diversity of MYBs and bHLHs has been extensively
73
studied with regard to the distinct pathways controlled by these TFs as well as the mechanisms
74
regulating their activity (reviewed by Feller et al., 2011).
TE D
M AN U
SC
RI PT
59
Different MYB/bHLH complexes regulate distinct cellular processes such as cell wall
76
synthesis, cell death, circadian clock, responses to abiotic and biotic stress, hormone signaling
77
and the biosynthesis of specialized metabolites (Lindemose et al., 2013; Seo and Mas, 2014;
78
Stracke et al., 2007; Stracke et al., 2001; Vailleau et al., 2002). In many cases, bHLH are able to
79
physically interact with different MYBs to achieve their function. In addition, the activity of TFs
80
appears to be regulated by cytosolic WD40 repeat proteins through formation of highly dynamic
81
MYB/bHLH/WD40 (MBW) complexes (Feller et al., 2011). WD40s and bHLHs respond to a
82
variety of environmental triggers and thereby offer a flexible, inducible system to activate
83
transcription of multiple sets of genes, while MYB TFs confer specificity to transcriptional
84
activation (Ramsay and Glover, 2005). In line with the proposition that TF complexes
85
comprising MYBs and bHLHs have evolved to increase fitness in changing environments, MBW
86
complexes have only been described in plants so far.
AC C
EP
75
ACCEPTED MANUSCRIPT
TFs typically bind 6-12 bp long DNA sequences present in the promoters of multiple
88
target genes. A sequence of six specific nucleotides has a high probability to occur in the
89
genome. Moreover, the specificity of the DNA binding domain (DBD) is attributed rather to a
90
family or a clade of TFs than to individual TFs. Those observations speak against precise
91
transcriptional activation solely based on specificity in DNA binding and suggest instead that
92
additional regulatory mechanisms occur to insure high specificity of the transcriptional process.
93
DNA binding can be regulated by chromatin accessibility and nucleosome positioning (reviewed
94
by Spitz and Furlong, 2012), by enhancers, cofactors and protein-protein interactions (PPIs). In
95
this review, we will discuss the mechanisms underlying the spatio-temporal regulation of PPIs
96
and post-transcriptional modifications (PTMs) and their importance for a fast responding
97
regulatory system that includes TFs in an inactive form that can rapidly be activated upon need.
M AN U
SC
RI PT
87
The MYB TF family is divided into sub-clades according to the structure of the DBD that
99
contains one to three repeats (R1-R3) (Figure 1-I). Each repeat consists of approximately 53
100
amino acid residues that form a Helix-turn-Helix (HtH). The N-terminal R2R3 domain binds to
101
DNA and is highly conserved within the whole family. In contrast, the C-terminus of MYB TFs,
102
i.e. the transcriptional activation domain (TAD), is more variable (Dubos et al., 2010) and has
103
been predicted to fail formation of a stable secondary structure (Lindemose et al., 2013). The
104
highly conserved DBD suggests a common mechanism for the regulation of DNA binding,
105
whereas the variable TAD domain might modulate TF activation and DBD accessibility and
106
thereby confer specificity to DNA binding by MYB TFs. bHLH TFs are characterized by 60
107
conserved amino acids at the C-terminus forming a basic DBD and a dimerization domain
108
(Figure 1-II). Similar to C-terminal part of MYB proteins, the N-terminal part of bHLH proteins
109
is more variable and can be grouped by differences in the TADs (Dombrecht, 2007; Cheng,
110
2011; Chen, 2012). BHLH proteins bind to specific sequences called E-box (5'-CANNTG-3')
111
including the well-studied G-box (5'-CACGTG) (Toledo-Ortiz, 2003). In Arabidopsis, fourteen
112
R2R3 MYB and six R1 MYB proteins share a conserved bHLH binding motif
113
([DE]Lx2[RK]x3Lx6Lx3R), which is critical for promoter activation because it stabilizes
114
complexes of these MYBs with R/B-like bHLH proteins (Zhao et al., 2013; Zimmermann et al.,
115
2004). This bHLH binding motif was used to predict MYB/bHLH interactions indicating that the
116
presence of this motif in the MYB protein sequence contributes to MYB/bHLH association
AC C
EP
TE D
98
ACCEPTED MANUSCRIPT
117
(Zimmermann et al., 2004). Nevertheless, this motif does not explain the recruitment of a
118
specific bHLH protein. This review focuses on individual MYB and bHLH TFs as case studies for the regulation
120
TFs and their complexes on the protein level rather than on the specificity of TFs towards their
121
target promoters. As plants are well-known for their ability to control gene expression in a highly
122
coordinated manner, plant MYB/bHLH complexes constitute a suitable model to study dynamic
123
regulation of gene expression. In this review, the regulatory mechanisms of MYBs and bHLHs
124
controlling plant metabolic pathways will serve as examples. We have chosen jasmonate
125
signaling, flavonoid biosynthesis and cell death pathways to investigate functional pairs of
126
MYBs and bHLH proteins. First, background on the regulation of TF activation and activity
127
through MYB/bHLH complex formation will be given; second, TF regulation at the post-
128
transcriptional level will be introduced; and finally, the importance of these mechanisms for
129
stimuli-specific responses will be discussed.
M AN U
SC
RI PT
119
130
132 133
TE D
131
MYB/bHLH as regulators of plant defense pathways
As a part of jasmonate (JA)-mediated responses, the TFs MYC2-4 from the bHLH family
135
activate transcription of different sets of genes involved in plant responses to environmental cues
136
including hormone signaling and development (Chen et al., 2011; Cheng et al., 2011; Fernández-
137
Calvo et al., 2011; Lorenzo et al., 2004). The regulation of MYC2-4 is tightly controlled at the
138
protein level by a PPI/F-BOX/proteasome-based mechanism. Under uninduced conditions, MYC
139
proteins are bound to the repressors NINJA, TOPLESS (TPL) and Jasmonate ZIM-domain (JAZ)
140
proteins (Pauwels et al., 2010; Dombrecht et al., 2007; Lorenzo et al., 2004). Upon stimulation
141
e.g. by exogenous jasmonates or herbivory, the JAZ proteins are bound by the signal receptor F-
142
Box protein CORONATINE-INSENTIVE protein 1 (COI1) and thereby targeted for degradation
143
by the 26S proteasome (Chini et al., 2007; Yan et al., 2013). The MYCs are thereby liberated
144
from the complex to fulfill their function (Dombrecht et al., 2007; Lorenzo et al., 2004). As an
AC C
EP
134
ACCEPTED MANUSCRIPT
145
individual protein, MYC2 has been shown to integrate different signals and to contribute to the
146
regulation of multiple pathways leading to different phenotypic outputs. This makes MYC2 a
147
model TF to discuss the molecular basis of multi-functionality of a single TF (Figure 2). Flavonoids are a class of secondary metabolites involved in plant-environment
149
interactions (e.g. defense, pollinator attraction, UV filtration). They can be divided into three
150
groups: anthocyanins, flavonols and proanthocyanidins. All steps of anthocyanin biosynthesis are
151
regulated by dynamically associating and disassociating MBW complexes (Appelhagen et al.,
152
2011). While the early steps of the pathway are all controlled by MYB11, MYB12 and MYB111,
153
the last and anthocyanin-specific biosynthetic step is regulated by PAP1, PAP2, MYB111, or
154
MYB114. These MYBs interact with different bHLHs, namely TRANSPARENT TESTA8
155
(TT8), GLABROUS3 (GL3), or ENHANCER OF GL3 (EGL30) (Xu et al., 2013). The
156
regulation of the anthocyanin pathway has been extensively studied because of defensive and
157
anti-oxidant properties of the compounds and their role in fruit coloring. Thus, the key regulators
158
as well as some PTMs modulating their interactions are known. The current knowledge on the
159
pathway makes it a useful model to illustrate PPI- and PTM-mediated regulation of TF activity.
160
Hypersensitive response (HR) triggered by pathogens leads to rapid cell death around the
161
infected tissue and thus prevents microbes from spreading. MYB30 is a R2R3 MYB TF that has
162
been shown to be involved in pathogen-induced HR and cell death (Vailleau et al., 2002).
163
Depending on the process it is involved in, MYB30 interacts with different modifying enzymes
164
and undergoes different PTMs leading to its activation or repression (Raffaele and Rivas, 2013).
165
The regulatory network surrounding MYB30 represents a unique multi-step and multi-enzyme
166
regulatory system and will be discussed to illustrate PTM-specific effects on PPIs and the
167
importance of rapid TF deactivation (Figure 3).
169 170 171
SC
M AN U
TE D
EP
AC C
168
RI PT
148
Post-transcriptional activation and inactivation of TFs by ubiquitination
ACCEPTED MANUSCRIPT
PTMs include all modifications on the transcript or protein level after the gene has been read
173
by an RNA polymerase, e.g. alternative splicing, alternative translation start, and protein
174
structure modifications. The latter are mediated by enzymes that catalyze reactions such as
175
phosphorylation, acetylation, or ubiquitination. Depending on where and when a functional
176
group is added, the protein will mature, be activated or inactivated, sequestered or degraded.
177
Ubiquitination is a PTM process conducted by E1, E2, and E3 ligases that will lead to secondary
178
structural changes or protein poly-ubiquitination and subsequent degradation of the protein by
179
the 26S proteasome (Ubiquitin-Proteasome System, UPS). However, mono-ubiquitination of TFs
180
can also lead to proteolysis-independent effects on TF activity and DNA binding properties
181
(reviewed by Geng et al., 2012). Ubiquitination can be reversed by de-ubiquitinases, providing
182
flexibility to the ubiquitin-mediated protein degradation system.
M AN U
SC
RI PT
172
While the first ubiquitination step catalyzed by E1 and E2 ligases shows little specificity for
184
the protein targets, E3 ligases are substrate- or condition-specific. E3 ligases have been
185
extensively studied in mammalian systems as they can be targeted by different drugs (Micel et
186
al., 2013). In Arabidopsis, more than a thousand proteins have been predicted to possess E3
187
ligase activity. Extensive review articles on the action of E3 ligases in response to environmental
188
and developmental cues are available (Duplan and Rivas, 2014; Guo et al., 2013; Stone, 2014).
189
The high diversity of stress-responsive E3 ligases in plants appears to be critical for balancing
190
the TFs present in the cell and thus for mounting appropriate responses to environmental changes
191
with sufficient specificity.
EP
TE D
183
Recently, Marino et al. (2014) showed that the Arabidopsis E3 ligase MIEL1 was able to
193
leave ubiquitin marks on MYB30 leading to the degradation of MYB30 by the proteasome.
194
Under normal conditions, MIEL1 is sufficiently expressed to target MYB30 to degradation and
195
thus to attenuate its action to initiate cell death. Upon pathogen infection, MIEL1 expression is
196
inhibited which allows for higher accumulation of the MYB30 protein and subsequently leads to
197
pathogen-induced cell death (Figure 3, III) (Marino et al., 2013).
AC C
192
198
Similarly, the E3 ubiquitin ligase CONSTITUTIVE PHOTOMORPHO-GENESIS 1 (COP1)
199
controls the stability of the MYB proteins PAP1 and PAP2 to repress transcription of
200
anthocyanin biosynthesis genes only in dark grown plants (Maier et al., 2013). COP1 is generally
201
involved in light-controlled development and gene expression by targeting TFs for proteasome-
ACCEPTED MANUSCRIPT
mediated degradation in the dark (Deng et al., 1991; Wei et al., 1994). For instance, COP1
203
controls the expression of light-responsive genes by ubiquitination of unphosphorylated
204
phytochrome A in response to far red light (Saijo et al., 2008). Moreover, COP1 has been
205
demonstrated to affect the stability of MYC2 in a light-dependent manner (Chico et al., 2014).
206
Accordingly, shading has a repressive effect on JA signaling through degradation of the MYC2
207
protein by the 26S proteasome dependent on COP1 (Figure 2, I) (Chico et al., 2014). These
208
observations exemplify an elegant mechanism that controls the activity of a TF in a trigger-
209
specific manner, here light, while it still allows for fast activation of the downstream responses.
SC
RI PT
202
Ubiquitination possesses a dual role: It can lead to decreased protein accumulation through
211
proteasome-dependent degradation or it can alter TF activity. It has thus been proposed that
212
ubiquitination could act as a timer for the activity of TFs. Indeed, while the first ubiquitin added
213
to the TF is in some cases required for initiation of transcription by favoring DNA binding or by
214
recruiting the transcriptional machinery, subsequent poly-ubiquitination of the same TF on the
215
DNA can target the protein to the proteasome. Mono- followed by poly-ubiquitination thus
216
represents a potential on-and-off switch of TF activity and a high turnover at the promoters
217
(Kodadek et al., 2006). In this model, first described as the timer model, the TF has the time
218
required to bind to a target promoter and activate gene transcription while being poly-
219
ubiquitinated prior to degradation (Wu et al., 2007). Although this mechanism has not been
220
described in plants, yet, it may constitute a regulatory process that facilitates rapid TF activation
221
and high TF turnover to provide an efficient on-and-off switch in plant stress responses.
224 225
TE D
EP
223
AC C
222
M AN U
210
Reversible modification of TF proteins by lysine acetylation
226
Lysine acetylation is a reversible type of PTM mediated by lysine acetyl-transferases and
227
de-acetylases. The finding that acetylation regulates the activity of the animal TF p53 marked the
228
beginning of a new search for acetylated proteins. Indeed, numerous proteins involved in general
229
regulation of gene expression were shown to be acetylated in yeast and humans, including TFs
ACCEPTED MANUSCRIPT
and other DNA-binding proteins (Gu and Roeder, 1997). In plants, lysine acetylation has so far
231
been studied in processes such as cell wall modifications during plant infection, secondary
232
metabolism as well as chromatin remodeling through histone acetylation (Xing and Poirier,
233
2012). Recently, a global analysis of lysine acetylation in rice (Oryza sativa) underlined the role
234
of this PTM mechanism in multiple biological processes (Nallamilli et al., 2014). The nuclear-
235
localized, acetylated proteins identified in rice included primarily histones but also a few bHLHs.
236
In JA signaling, the repressor TPL interacts with MYC2 to inhibit MYC2 activity (Pauwels et al.,
237
2010; Dombrecht et al., 2007). TPL has been described as a Groucho (GR)/TP1 family protein,
238
involved in transcriptional repression by recruiting histone de-acetylase to induce local
239
chromatin compaction (Causier et al., 2012). Despite the technical limitations to study this PTM,
240
numerous lines of evidence suggest an effect of acetylation on transcriptional regulation. Further
241
studies are needed to understand the biological functions of acetylation of histones and TFs.
M AN U
SC
RI PT
230
242 243
245
Phosphorylation regulates TF activity and turnover
TE D
244
Phosphorylation has so far been the most-studied PTM due to its implication in MAP
247
kinase cascades. In mammals, the role of phosphorylation in signaling pathways was initially
248
described for the regulation of the cell cycle and for oncogenesis. This PTM was intensely
249
studied in the context of plant signaling during plant response to stress and immune response
250
(Boudsocq and Sheen, 2013; Kaufmann et al, 2011; Ni et al., 2014; Spoel and Loake, 2011).
251
Phosphorylation has moreover received a lot of attention because of the availability of a strong
252
anti-body for detection of phosphorylated proteins by Western blotting and because of its value
253
as a model PTM to detect modified peptides by LC-MS (Kaufman et al, 2011; Zhou et al., 2001).
254
Upon JA signaling, phosphorylation of MYC2 in its TAD domain induces its proteolysis
255
but also stimulates the transcriptional activity of MYC2 (Zhai et al., 2013). Based on these
256
findings, two rounds of DNA binding by two MYC2 proteins have been proposed to be
257
necessary to activate target gene transcription. It has been further suggested that there is a need
AC C
EP
246
ACCEPTED MANUSCRIPT
for a high turnover provided by the UPS. The degradation of the MYC2 bound in the first round
259
might favor binding of the next active MYC2 protein to the promoter, while on the other hand,
260
the presence of the first MYC2 at the promoter might decrease the target search time for the
261
second MYC2 protein. The observations made for MYC2 are not congruent with the “timer
262
model” above, but rather follow the proposed model of “activation by destruction” described in
263
mammals and yeast (Catic et al., 2013; Collins and Tansey, 2006; Geng et al., 2012) where TF
264
degradation is not only essential to regulate TF turnover but also dependent on the TF’s
265
transcriptional activity.
SC
RI PT
258
266
268
REDOX-dependent regulation of TFs
269
M AN U
267
Changes in the REDOX potential of the cell can affect disulfide bridges in TF proteins and
271
thereby affect their activity in response to stress conditions that lead to higher accumulation of
272
hormones in the cell, i.e. JA, Salicylic Acid (SA), ethylene, Gibberellic Acid (GA), Abscisic
273
Acid (ABA) and auxins. As an example, intracellular translocation of SA results in elevated
274
accumulation of glutathione as well as a shift in the ratio of reduced to oxidized glutathione
275
(Spoel and Loake, 2011). On the other hand, JA perception will decrease the pool of reduced
276
glutathione in favor of the oxidized form (Spoel and Loake, 2011). These changes in the
277
REDOX state can be perceived by reactive cysteines of regulatory proteins and thereby lead to
278
changes in their structure. Heine and coworkers identified two conserved cysteine residues as a
279
regulatory module in the R2R3 domain of MYB TFs (Heine et al., 2004). In the absence of
280
reducing agents, MYB TFs were not able to bind DNA in vitro. While cys-53 is highly
281
conserved among MYBs from different organisms, cys-49 is specific to plant R2R3 domains.
282
The emergence of this second cysteine residue in plants has been suggested to change the
283
accessibility of cys-53 as thus its capacity to form a disulfide bond. Cys-49 might therefore
284
regulate the DNA binding capacity of the plant MYB TFs by modulating their dimerization
285
capabilities. This higher complexity observed in plants talks in favor of a mechanistic adaptation
286
to ensure fast and specific responses to different internal or external signals (Figure 3, II).
AC C
EP
TE D
270
ACCEPTED MANUSCRIPT
Another type of REDOX-related PTMs is nitrosylation. Following REDOX changes in the
288
cell, S-nitroglutathione donors change availability. In mammalian systems, nitrosylation of the
289
myc oncogenic proteins has been reported to reduce their DNA binding capacity (Brendeford et
290
al., 1998; Lüscher and Vervoorts, 2012). In plants, the activity of MYB30 has been shown to be
291
influenced by S-nitrosylation through regulation of the secondary structure of its R2R3 domain
292
(Tavares et al., 2014). Moreover and in accordance with the previous paragraph, treatment of
293
nitrosylated MYB30 with reducing agent partially restored its capacity to interact with DNA,
294
thus confirming that the REDOX state of the protein can change its ability to bind DNA (Tavares
295
et al., 2014). In the case of MYB30, SA-induced stress decreases the pool of S-nitroglutathione
296
donors leading to increased activity of MYB30 and thus to pathogen-induced cell death. On the
297
other hand, a JA-induced increase of the available pool of oxidized donors might lead to an
298
increase in MYB30 nitrosylation and a decrease in its activity (Figure 3, II). The REDOX state
299
of the cell might thereby play a role in crosstalk between SA and JA signaling.
M AN U
SC
RI PT
287
300 301
303
Stabilization of MYB by sumoylation
TE D
302
SUMO stands for Small Ubiquitin Modifier and refers to a protein able to covalently attach
305
itself to another protein. SUMO has been shown to be involved in different regulatory processes
306
such as nucleus-to-cytosol protein translocation, protein degradation, plant development (Conti
307
et al., 2014; Elrouby, 2014), and stress responses (Miller et al., 2013). In ABA signaling, gene
308
expression studies combined with phenotypic analyses have demonstrated a functional
309
relationship between MYB30 and the small ubiquitin-like modifier E3 ligase SIZ1 (Zheng et al.,
310
2012). Upon ABA treatment, it has been shown that SIZ1 has the capacity to stabilize MYB30
311
by sumoylation of the K283 residue (Figure 3, II) (Zheng et al., 2012). This observation adds
312
another mechanism to the model of stress-induced control of TFs by PTMs to mount rapid and
313
specific responses in changing environment. It appears advantageous to have key regulators
314
available as inactive proteins that can be activated by different PTMs occurring in response to
315
different signals. Different PTMs regulate the stability/turnover, the DNA binding and the
AC C
EP
304
ACCEPTED MANUSCRIPT
activation of TFs which points at the need for robust coordination of these mechanisms. This
317
complexity in TF regulation by PTMs confers the capacity of plant regulatory systems to
318
integrate multiple signals. It also adumbrates the importance of combinatorial effects of different
319
PTMs for the activation and the deactivation of TFs.
RI PT
316
320 321
Membrane-tethered TFs require activation by proteolytic cleavage
SC
322 323
Membrane-tethered transcription factors (MTTF) are membrane-bound TFs that are activated
325
through cleavage by a protease which releases the DBD and allows its translocation to the
326
nucleus. Plant MTTFs have been shown to be involved in Endoplasmic Reticulum (ER) and
327
mitochondrial retrograde signaling (De Clercq et al., 2013; Ng et al., 2013; Yang et al., 2014b).
328
In mammals, MTTFs have been extensively studied as part of the unfolded protein responses
329
associated with Alzheimer’s disease and due to their role in Notch signaling (Brown et al., 2000).
330
The regulation of their proteolytic activation seems to be linked to protease activity as well as
331
membrane fluidity. In plants, seven MTTFs from the bZIP and NAC TF family as well as one
332
Membrane-anchored MYB (MaMYB) have been described to date (Chen et al., 2008; De Clercq
333
et al., 2013; Ng et al., 2013; Seo, 2014; Yang et al., 2014b). Their rapid release upon changes in
334
the cellular environment has been hypothesized to play a role in rapid stress responses (Chen et
335
al., 2008).
AC C
EP
TE D
M AN U
324
336
The identification of MaMYB was the first and is so far the only case of an ER-anchored
337
MYB TF (Dunkley et al, 2006). Whereas the membrane localization of the full-length MaMYB
338
and the nuclear localization of a truncated form have been demonstrated, no experimental proof
339
of cleavage and re-localization has been furnished to date. This unique case of MTTF behavior in
340
the MYB family could be important for induced responses. The protein might be kept at the ER
341
to be quickly released upon stress. More recently, ANAC013 and ANAC017 have been shown to
342
be membrane-anchored to the chloroplast and their proteolysis upon H2O2 stress liberates their
343
C-terminal DBD which is then be targeted to the nucleus. (De Clercq et al., 2013; Ng et al.,
ACCEPTED MANUSCRIPT
2013). The same has been described for a membrane-bound plant homeodomain transcription
345
factor, released upon proteolysis and associated with histone modifications in response to
346
retrograde signaling (Sun et al, 2011). In both cases, stress responses appear to regulate
347
transcriptional activation by cleaving membrane-bound regulatory proteins and releasing their
348
DBD. Nevertheless, no direct experimental evidence for this mechanisms has been provided for
349
a member of the MYB or bHLH family.
RI PT
344
350
TF localization can be modulated by interacting partners
M AN U
352
SC
351
353
TFs without a membrane anchor can also reside in the cytosol, either as free, soluble proteins
355
or physically associated with soluble cytoplasmic proteins until they tranlocate to the nucleus
356
upon a trigger. One example is the bHLH TF MYC1, a regulator of root hair development and
357
trichome patterning (Pesch et al., 2013). Despite the presence of a Nuclear Localization Signal
358
(NLS) as also described for other bHLH, the soluble MYC1 protein has been shown to mostly
359
reside in the cytosol, which also determines the localization of the bHLH TF GLABRA1 (GL1),
360
another regulator of trichome development. Upon interaction with MYC1, GL1 has been shown
361
to be re-localized from the nucleus to the cytosol, which inhibits its function as transcriptional
362
activator in the nucleus (Pesch et al., 2013). Although MYC1 induces trichome development,
363
MYC1 over-expression lines showed lower trichome density. Overexpression of MYC1 might
364
disturb the stoichiometry of the TF complex and thereby trichome development. GL1, likely in
365
combination with other TFs, has been suggested to bind the MYC1 promoter to form a negative
366
feedback loop and thereby balance MYC1expression levels (Pesch et al., 2013). MYC1 thus
367
constitutes an example of TF regulation comprising multiple regulatory layers on the protein
368
level. First, the GL1/MYC1 complex is formed and activated. Second, GL1 activity is repressed
369
by subcellular re-localization of the protein mediated by MYC1. Finally, active TF complexes
370
can feedback-regulate MYC1 transcription. In this example, a TF both activates and represses the
371
same pathway dependent on its concentration and the presence of its interacting partners.
AC C
EP
TE D
354
ACCEPTED MANUSCRIPT
The identification of mechanisms regulating the subcellular localization of TFs has recently
373
provided new insight into retrograde signaling in response to stress. Future studies on stress-
374
induced changes in membrane composition and their relevance for TF cleavage will deepen our
375
understanding of the fast responses to complex triggers characteristic for plants. The regulatory
376
mechanism of MTTF activation by proteolytic cleavage is likely to be extended to TFs that do
377
not possess a membrane anchor themselves but are anchored through interacting partners. A
378
membrane-anchored protein, potentially acting as a signal receptor, could interact with a TF and
379
dissociation of the complex could release the TF and enable rapid fine-tuning of transcriptional
380
regulation.
SC
RI PT
372
M AN U
381 382 383
The role of TF complexes in the nucleus
384
In 2008, small TFs that repress the transcriptional activity of MYBs have been described in
386
plants (Dubos et al., 2008). Those small MYB-like proteins, which only contain the R3 domain,
387
inhibit transcriptional activation by R2R3 MYBs by competing with them for formation of
388
MBW complexes. Therefore, TFs possessing only a R3 domain are generally predicted to be
389
repressors of transcription (Dubos et al., 2008). In the case of the flavonoid biosynthetic
390
pathway, numerous small proteins negatively regulate the formation of active MBW complexes
391
by interacting with the bHLHs in these complexes (Dubos et al., 2008; Matsui et al., 2008;
392
Nemie-Feyissa et al., 2014). The expression of small R3 proteins is regulated by environmental
393
and developmental factors. When co-expressed with the MYB TFs controlling anthocyanin
394
biosynthesis, the MYB-like proteins compete for binding to the bHLHs involved, which leads to
395
disruption of MBW complexes and thereby counter-balances MYB activity e.g. during nitrate
396
starvation (Nemie-Feyissa et al., 2014). Moreover, miRNA156 has been shown to influence
397
MBW complexes by activating SQUAMOSA PROMOTER BINDING PROTEIN-LIKE (SPL)
398
proteins that compete for bHLH binding and thereby coordinate anthocyanin production during
399
the transition from the vegetative to the reproductive stage (Gou et al., 2011). This example
AC C
EP
TE D
385
ACCEPTED MANUSCRIPT
400
illustrates how different conditions can affect regulation of a biosynthetic pathway by controlling
401
inhibitors of TF activity. Similar to the regulation of the MYB TFs controlling anthocyanin biosynthesis, negative
403
regulators modulates the transcriptional activity of MYB30. The secretory phospholipase PLA2
404
protein localizes to the Golgi where it controls auxin-dependent protein trafficking (Lee et al.,
405
2010) and possibly regulates plant defense chemistry independently of its enzymatic function
406
(Froidure et al., 2010). In the nucleus, PLA2-α inhibits MYB30 through physical interaction.
407
Upon pathogen attack, expression of PLA2-α is induced in periphery of the infection zone
408
suggesting a role for PLA2-α in limiting the HR response mediated by MYB30 (Figure 2, III).
SC
RI PT
402
Examples of TF regulation by PPIs in the nucleus can also be found in the bHLH family.
410
Recently, different labs identified a new clade of transcriptional regulators that are
411
phylogenetically closely related to the MYC2-4. BHLH003, bHLH013 and bHLH017 (also
412
named JAM1, JAM2 and JAM3) bind DNA with a specificity similar to that of MYC2, MYC3,
413
and MYC4 suggesting that they might compete with the MYCs for the binding of cis-regulatory
414
elements (Fonseca et al., 2014; Nakata and Ohme-Takagi, 2013; Sasaki-Sekimoto et al., 2013).
415
Importantly, physical interaction between the JAMs and MYC2 appears to play a role in the
416
nuclear targeting of JAZ1 and JAZ9 (Withers et al., 2012). Since the MYC TFs are almost
417
constitutively expressed in all tissues, their regulation at the PPI level is likely to be of primary
418
importance for their biological functions. Indeed, while MYC2 is present in various tissues at
419
various stages during development, it drives transcription only under certain conditions
420
dependent on its interacting partners.
EP
TE D
M AN U
409
MYC2, MYC3 and MYC4, have been shown to physically associate with MYB28, MYB29,
422
MYB76, MYB51, MYB34 and MYB122 to regulate the accumulation of glucosinolate defense
423
compounds (Figure 1, III) (Schweizer et al., 2013; Frerigmann et al., 2014). The expression
424
patterns of the six MYB TFs show high similarity (Gigolashvili et al., 2007a; Gigolashvili et al.,
425
2007b; Hirai et al., 2007; Sønderby et al., 2007) and strongly overlap with those of the MYCs.
426
Although all three MYCs can interact with all six MYBs (Frerigmann et al., 2014; Schweizer et
427
al., 2013), highly specific changes in the glucosinolate output can be triggered by different
428
hormones or stresses (Beekwilder et al., 2008; Frerigmann and Gigolashvili, 2014; Sonderby et
AC C
421
ACCEPTED MANUSCRIPT
al., 2010). Accordingly, analysis of glucosinolate levels in myc and myb single and double
430
mutants revealed specific mutant profiles (Frerigmann and Gigolashvili, 2014; Schweizer et al.,
431
2013; Sonderby et al., 2010) suggesting specific in planta roles of the individual TFs that cannot
432
be fully compensated by their closest homologues.
RI PT
429
Another example of TF complex-mediated transcriptional regulation is the interaction
434
DELLA and JAZ proteins, which provides the molecular basis of synergism between GA and JA
435
signaling (Hou et al., 2014). Both JA and GA have been shown to induce degradation of DELLA
436
and JAZ proteins to coordinately activate the MBW complex required to induce trichome
437
initiation (Qi et al., 2014). The DELLAs compete with the MYCs to bind the JAZs, thus
438
inducing JA-independent MYC2 activity (Figure 2-III) (Davière et al., 2008; Wild et al., 2012,
439
Hou et al., 2010; Lan et al., 2014). Upon increased GA levels, DELLAs are degraded and
440
MYC2-dependent JA synthesis is inhibited. The interaction of the DELLAs with MYC2
441
mediates induction of sesquiterpene synthase genes in a JA and red light dependent manner
442
(Hong et al., 2012). JA and GA signaling thus exhibit balancing effects on each other’s pathways
443
depending on their abundance in the cell. The molecular basis of the synergy between JAZ and
444
DELLA proteins provides insight into how plants integrate different signals, how they sense
445
environmental changes and how they prioritize different processes. This allows plants to
446
orchestrate their responses precisely in space and time and thus to optimize their fitness in
447
fluctuating environments.
450 451 452
M AN U
TE D
EP
449
AC C
448
SC
433
Integration of regulatory mechanisms
An individual TF can be involved in multiple biological processes during the plant’s life
453
cycle. Combinations of different PTMs and PPIs serve to establish different layers of TF
454
regulation on the protein level specific to environmental changes. To optimize their fitness,
455
plants have built complex regulatory systems ensuring fast and robust responses. A large number
456
of modifications occurring at the protein level modulate TF activity e.g. through altering the TF’s
ACCEPTED MANUSCRIPT
457
ability to bind interaction partners or DNA, through a change in turnover rate, or through
458
ubiquitination-dependent timing of degradation. In combination, all these mechanisms contribute
459
to the specificity of plant responses and at the same time increase their plasticity. The bHLH transcription factor MYC2 has been described as a master regulator of various
461
plant defense pathways in response to different environmental cues (Figure 2) (Kazan and
462
Manners, 2013). The idea that MYC2 has a more general effect on transcriptional activation
463
rather that high specificity to its target promoters is supported by the finding that MYC2 does not
464
act as transcriptional activator without an interaction partner (Kazan and Manners, 2013).
465
Instead, MYC2’s intrinsic property to bind different partners in different transcriptional networks
466
allows the plant to coordinate multiple signals and mount appropriate responses. The regulation
467
of DNA availability at the target loci has not been discussed in this review, but there is
468
experimental evidence suggesting that TFs also interact with histone-modifying enzymes as well
469
as mediator complexes (Badeaux and Shi, 2013; Lai et al., 2014; Yang et al., 2014a).
M AN U
SC
RI PT
460
As discussed above, flavonoids constitute a well-studied class of secondary plant
471
metabolites. Contrary to the example of MYC2, which represents the case of a TF as a hub, the
472
anthocyanin pathway is an example of a complex TF network regulating one specific output.
473
Although multiple PPIs and specific expression patterns have been identified, the fine-tuning of
474
flavonoid accumulation keeps providing novel insight into how a multitude of regulatory
475
mechanisms insure specificity of MYB/bHLH complexes. In the future, the regulatory network
476
controlling anthocyanin biosynthesis could serve as a model pathway to build in silico tools for
477
the integration of both mechanistic models and larger gene network effects on the composition of
478
TF complexes in a pathway-specific context. As different TFs have been shown to control the
479
different parts of the pathway in a tightly controlled way, anthocyanin biosynthesis could prove
480
its value as a model for other metabolic pathways, e.g. to predict the flux through a pathway for
481
engineering purposes.
EP
AC C
482
TE D
470
In this review, MYB30 served as example of a TF involved in different stress responses
483
and modulated by different PTMs (Figure 3). The different interactors and modifying enzymes
484
allow for tight control of MYB30 activity in terms of a specific spatial and temporal regulation
485
of its targets genes. The mechanisms controlling MYB30 activity support a model in which
486
different trigger-specific signaling pathways have the same biological output, i.e. cell death. This
ACCEPTED MANUSCRIPT
type of regulation facilitates the adaptation of the regulation of a specific TF to different cellular
488
environments, e.g. maybe changing its ability to bind interaction partners depending. In different
489
cell types, the activity of MYB30 can be regulated through interaction with different partners and
490
through different PTMs. As opposed to MYC2 as an example of a TF with multiple targets and a
491
broad effect on transcriptional activation, future studies on MYB30 have the potential to
492
elucidate what confers specificity in DNA binding downstream of different internal and external
493
cues.
RI PT
487
SC
494 495 Future outlook
M AN U
496 497
Comprehension of the complexity of transcriptional regulation will strongly benefit from
499
a deeper understanding of the underlying mechanistic events. Thus, studies that investigate how
500
TFs function at the single molecule level will help to improve current models of transcriptional
501
regulation. Chen et al. (2014) have recently proposed a technique to visualize the binding of
502
single proteins to DNA which can help to resolve trial-and-error calculations of TF binding. This
503
approach allows classification of TFs in complexes based on their promoter search method and
504
binding order. Future studies using this and similar approaches to study know TF complexes will
505
provide valuable mechanistic insight into how TFs associate and disassociate to control the
506
expression of their target genes. In the case of MYC2, this level of mechanistic understanding
507
may explain how MYC2 can activate different target genes dependent on its interacting partners.
EP
AC C
508
TE D
498
The challenges to improve our understanding of the DNA binding specificity of TFs that
509
serve as regulatory hubs, like MYC2, are linked to their involvement in fast and cell-specific
510
responses. Thus, using tools for in planta visualization of bHLHs and their interactors as well as
511
investigating the chromatin landscape in the neighborhood of TF target promoters will provide
512
novel insight into the specificity of TF-DNA interaction (Sahu et al., 2013). Next generation
513
Chromatin-Immuno-Precipitation (ChIP) assays such as exo-ChIP with higher sensitivity and
514
higher spatial and temporal resolution will enable us to obtain a more comprehensive image of
ACCEPTED MANUSCRIPT
what happens in the cell (Zentner and Henikoff, 2012). This kind of in planta studies are
516
necessary because of the complexity of plants as multicellular organisms and will help to
517
integrate cell-to-cell communication with different signaling mechanisms controlling TF
518
activation (Chen and Zhu, 2004). Studies combining proteasome inhibitors and ChIP have
519
already been used in mammalian cells will also be needed in plants to detect DNA-associated
520
protein degradation, thereby e.g. linking MYC2 activity with turnover of the protein at the
521
promoter (Catic et al., 2013).
RI PT
515
Finally, recent advances in immuno-precipitation techniques and mass spectrometry will
523
enable the identification of novel components of regulatory protein complexes, As an example, a
524
cross-linking strategy combined with mass spectrometry was recently successful in identifying
525
protein complexes in planta (Luo et al., 2012). This methodology can in the future be extended
526
to the enrichment of cells or organelles isolated from plants grown under specific conditions at
527
different time points to study the dynamics of protein complex formation and to determine which
528
interaction partners are available in a given cell. Integrative bioinformatics will be key to
529
incorporate these proteomics data with transcriptional network models.
M AN U
SC
522
531
TE D
530
Acknowledgments
533
The authors thank Frederik Rook and Sophie Lambertz for critical reading of the manuscript.
EP
532
AC C
534 535
Funding
536
Financial support was provided by the Danish National Research Foundation DNRF grant 99.
537 538 539
References
ACCEPTED MANUSCRIPT
540 Appelhagen, I., Jahns, O., Bartelniewoehner, L., Sagasser, M., Weisshaar, B., and Stracke, R.
542
(2011). Leucoanthocyanidin Dioxygenase in Arabidopsis thaliana: Characterization of
543
mutant alleles and regulation by MYB–BHLH–TTG1 transcription factor complexes.
544
Gene 484:61-68.
545 546
RI PT
541
Badeaux, A.I., and Shi, Y. (2013). Emerging roles for chromatin as a signal integration and storage platform. Nature reviews. Molecular Cell Biology 14:211-224.
Beekwilder, J., van Leeuwen, W., van Dam, N.M., Bertossi, M., Grandi, V., Mizzi, L., Soloviev,
548
M., Szabados, L., Molthoff, J.W., and Schipper, B. (2008). The impact of the absence of
549
aliphatic glucosinolates on insect herbivory in Arabidopsis. PLoS ONE 3:e2068.
551
M AN U
550
SC
547
Boudsocq, M., and Sheen, J. (2013). CDPKs in immune and stress signaling. Trends in Plant Science 18:30-40.
Brendeford, E.M., Andersson, K.B., and Gabrielsen, O.S. (1998). Nitric oxide (NO) disrupts
553
specific DNA binding of the transcription factor c-Myb in vitro. FEBS Letters 425:52-56.
554
Brown, M.S., Ye, J., Rawson, R.B., and Goldstein, J.L. (2000). Regulated intramembrane
555
TE D
552
proteolysis: a control mechanism conserved from bacteria to humans. Cell 100:391-398. Catic, A., Suh, Carol Y., Hill, Cedric T., Daheron, L., Henkel, T., Orford, Keith W.,
557
Dombkowski, David M., Liu, T., Liu, X.S., and Scadden, David T. (2013). Genome-wide
558
Map of Nuclear Protein Degradation Shows NCoR1 Turnover as a Key to Mitochondrial
559
Gene Regulation. Cell 155:1380-1395.
561 562 563
Causier, B., Ashworth, M., Guo, W., and Davies, B. (2012). The TOPLESS interactome: a
AC C
560
EP
556
framework for gene repression in Arabidopsis. Plant Physiology 158:423-438.
Chen, W.J., and Zhu, T. (2004). Networks of transcription factors with roles in environmental stress response. Trends in Plant Science 9:591-596.
564
Chen, Y.-N., Slabaugh, E., and Brandizzi, F. (2008). Membrane-tethered transcription factors in
565
Arabidopsis thaliana: novel regulators in stress response and development. Current
566
Opinion in Plant Biology 11:695-701.
ACCEPTED MANUSCRIPT
567
Chen, Y., Pang, Q., Dai, S., Wang, Y., Chen, S., and Yan, X. (2011). Proteomic identification of
568
differentially expressed proteins in Arabidopsis in response to methyl jasmonate. Journal
569
of Plant Physiology 168:995-1008. Chen, J., Zhang, Z., Li, L., Chen, B.C., Revyakin, A., Hajj, B., Legant, W., Dahan, M., Lionnet,
571
T., Betzig, E., et al. (2014). Single-molecule dynamics of enhanceosome assembly in
572
embryonic stem cells. Cell 156:1274-1285.
RI PT
570
Cheng, Z., Sun, L., Qi, T., Zhang, B., Peng, W., Liu, Y., and Xie, D. (2011). The bHLH
574
transcription factor MYC3 interacts with the jasmonate ZIM-domain proteins to mediate
575
jasmonate response in Arabidopsis. Molecular Plant 4:279-288.
SC
573
Chico, J.-M., Fernández-Barbero, G., Chini, A., Fernández-Calvo, P., Díez-Díaz, M., and
577
Solano, R. (2014). Repression of Jasmonate-Dependent Defenses by Shade Involves
578
Differential Regulation of Protein Stability of MYC Transcription Factors and Their JAZ
579
Repressors in Arabidopsis. The Plant Cell Online 26:1967-1980.
M AN U
576
Chini, A., Fonseca, S., Fernandez, G., Adie, B., Chico, J., Lorenzo, O., Garcia-Casado, G.,
581
Lopez-Vidriero, I., Lozano, F., and Ponce, M. (2007). The JAZ family of repressors is the
582
missing link in jasmonate signalling. Nature 448:666-671.
583 584
TE D
580
Collins, G.A., and Tansey, W.P. (2006). The proteasome: a utility tool for transcription? Current Opinion in Genetics & Development 16:197-202. Conti, L., Nelis, S., Zhang, C., Woodcock, A., Swarup, R., Galbiati, M., Tonelli, C., Napier, R.,
586
Hedden, P., and Bennett, M. (2014). Small Ubiquitin-like Modifier Protein SUMO
587
Enables Plants to Control Growth Independently of the Phytohormone Gibberellin.
588
Developmental Cell 28:102-110.
AC C
EP
585
589
Davière, J.-M., de Lucas, M., and Prat, S. (2008). Transcriptional factor interaction: a central
590
step in DELLA function. Current Opinion in Genetics & Development 18:295-303.
591
De Clercq, I., Vermeirssen, V., Van Aken, O., Vandepoele, K., Murcha, M.W., Law, S.R., Inze,
592
A., Ng, S., Ivanova, A., Rombaut, D., et al. (2013). The membrane-bound NAC
593
transcription factor ANAC013 functions in mitochondrial retrograde regulation of the
594
oxidative stress response in Arabidopsis. The Plant Cell 25:3472-3490.
ACCEPTED MANUSCRIPT
595
Deng, X.W., Caspar, T., and Quail, PH. (1991). Cop1: a regulatory locus involved in light-
596
controlled development and gene expression in Arabidopsis. Genes and Development
597
5:1172-1182. Dombrecht, B., Xue, G.P., Sprague, S.J., Kirkegaard, J.A., Ross, J.J., Reid, J.B., Fitt, G.P.,
599
Sewelam, N., Schenk, P.M., and Manners, J.M. (2007). MYC2 differentially modulates
600
diverse jasmonate-dependent functions in Arabidopsis. The Plant Cell Online 19:2225-
601
2245.
RI PT
598
Dubos, C., Le Gourrierec, J., Baudry, A., Huep, G., Lanet, E., Debeaujon, I., Routaboul, J.M.,
603
Alboresi, A., Weisshaar, B., and Lepiniec, L. (2008). MYBL2 is a new regulator of
604
flavonoid biosynthesis in Arabidopsis thaliana. The Plant Journal 55:940-953.
609 610 611 612 613 614 615 616 617 618 619
M AN U
608
Dunkley, T.P.J., Hester, S., Shadforth, I.P. et al. (2006). Mapping the Arabidopsis organelle proteome. Proc. Natl Acad. Sci. USA 103:6518–6523.
Duplan, V., and Rivas, S. (2014). E3 ubiquitin-ligases and their target proteins during the regulation of plant innate immunity. Frontiers in Plant Science 5:42.
TE D
607
transcription factors in Arabidopsis. Trends in Plant Science 15:573-581.
Elrouby, N. (2014). Extent and significance of non-covalent SUMO interactions in plant development. Plant Signaling & Behavior 9:e27948. Feller, A., Machemer, K., Braun, E.L., and Grotewold, E. (2011). Evolutionary and comparative
EP
606
Dubos, C., Stracke, R., Grotewold, E., Weisshaar, B., Martin, C., and Lepiniec, L. (2010). MYB
analysis of MYB and bHLH plant transcription factors. The Plant Journal 66:94-116. Fernández-Calvo, P., Chini, A., Fernández-Barbero, G., Chico, J.-M., Gimenez-Ibanez, S.,
AC C
605
SC
602
Geerinck, J., Eeckhout, D., Schweizer, F., Godoy, M., and Franco-Zorrilla, J.M. (2011). The Arabidopsis bHLH transcription factors MYC3 and MYC4 are targets of JAZ repressors and act additively with MYC2 in the activation of jasmonate responses. The Plant Cell Online 23:701-715.
620
Fonseca, S., Fernández-Calvo, P., Fernández, G.M., Díez-Díaz, M., Gimenez-Ibanez, S., López-
621
Vidriero, I., Godoy, M., Fernández-Barbero, G., Van Leene, J., and De Jaeger, G. (2014).
622
bHLH003, bHLH013 and bHLH017 Are New Targets of JAZ Repressors Negatively
623
Regulating JA Responses. PloS ONE 9:e86182.
ACCEPTED MANUSCRIPT
624 625
Frerigmann, H., and Gigolashvili, T. (2014). MYB34, MYB51 and MYB122 Distinctly Regulate Indolic Glucosinolate Biosynthesis in Arabidopsis thaliana. Molecular Plant. Froidure, S., Canonne, J., Daniel, X., Jauneau, A., Briere, C., Roby, D., and Rivas, S. (2010).
627
AtsPLA2-alpha nuclear relocalization by the Arabidopsis transcription factor AtMYB30
628
leads to repression of the plant defense response. Proc. Natl Acad. Sci. USA 107:15281-
629
15286.
631
Geng, F., Wenzel, S., and Tansey, W.P. (2012). Ubiquitin and Proteasomes in Transcription. Annual Review of Biochemistry 81:177-201.
SC
630
RI PT
626
Gigolashvili, T., Berger, B., Mock, H.P., Muller, C., Weisshaar, B., and Fluegge, U.I. (2007a).
633
The transcription factor HIG1/MYB51 regulates indolic glucosinolate biosynthesis in
634
Arabidopsis thaliana. The Plant Journal 50:886-901.
M AN U
632
Gigolashvili, T., Yatusevich, R., Berger, B., Muller, C., and Flugge, U.I. (2007b). The R2R3-
636
MYB transcription factor HAG1/MYB28 is a regulator of methionine-derived
637
glucosinolate biosynthesis in Arabidopsis thaliana. The Plant Journal 51:247-261.
638
Gou, J.Y., Felippes, F.F., Liu, C.J., Weigel, D., and Wang, J.W. (2011). Negative regulation of
639
anthocyanin biosynthesis in Arabidopsis by a miR156-targeted SPL transcription factor.
640
The Plant Cell 23:1512-1522.
642
Gu, W., and Roeder, R.G. (1997). Activation of p53 Sequence-Specific DNA Binding by Acetylation of the p53 C-Terminal Domain. Cell 90:595-606.
EP
641
TE D
635
Guo, L., Nezames, C.D., Sheng, L., Deng, X., and Wei, N. (2013). Cullin‐RING Ubiquitin
644
Ligase Family in Plant Abiotic Stress Pathways. Journal of Integrative Plant Biology
645 646 647
AC C
643
55:21-30.
Han, J., Zhang, H., Zhang, H., Wang, Z., Zhou, H., and Zhang, Z. (2013). A Cul4 E3 Ubiquitin Ligase Regulates Histone Hand-Off during Nucleosome Assembly. Cell 155:817-829.
648
Heine, G.F., Hernandez, J.M., and Grotewold, E. (2004). Two cysteines in plant R2R3 MYB
649
domains participate in REDOX-dependent DNA binding. Journal of Biological
650
Chemistry 279:37878-37885.
ACCEPTED MANUSCRIPT
Hirai, M.Y., Sugiyama, K., Sawada, Y., Tohge, T., Obayashi, T., Suzuki, A., Araki, R., Sakurai,
652
N., Suzuki, H., and Aoki, K. (2007). Omics-based identification of Arabidopsis Myb
653
transcription factors regulating aliphatic glucosinolate biosynthesis. Proc. Natl Acad. Sci.
654
USA 104:6478-6483.
RI PT
651
655
Hong, G.-J., Xue, X.-Y., Mao, Y.-B., Wang, L.-J., and Chen, X.-Y. (2012). Arabidopsis MYC2
656
Interacts with DELLA Proteins in Regulating Sesquiterpene Synthase Gene Expression.
657
The Plant Cell Online 24:2635-2648.
660 661
SC
659
Hou, X., Lee, L.Y.C., Xia, K., Yan, Y., and Yu, H. (2010). DELLAs Modulate Jasmonate Signaling via Competitive Binding to JAZs. Developmental Cell 19:884-894. Kaufmann, K., Smaczniak, C., de Vries, S., Angenent, G.C., and Karlova, R. (2011). Proteomics insights into plant signaling and development. Proteomics 11:744-755.
M AN U
658
662
Kazan, K., and Manners, J.M. (2013). MYC2: the master in action. Molecular Plant 6:686-703.
663
Kodadek, T., Sikder, D., and Nalley, K. (2006). Keeping Transcriptional Activators under
664
Control. Cell 127:261-264.
Lai, Z., Schluttenhofer, C.M., Bhide, K., Shreve, J., Thimmapuram, J., Lee, S.Y., Yun, D.-J., and
666
Mengiste, T. (2014). MED18 interaction with distinct transcription factors regulates
667
multiple plant functions. Nature Communications 5.
TE D
665
Lan, Z., Krosse, S., Achard, P., van Dam, N.M., and Bede, J.C. (2014). DELLA proteins
669
modulate Arabidopsis defences induced in response to caterpillar herbivory. Journal of
670
Experimental Botany 65:571-583.
672 673
Lee, C.M. (2014). Transport of c-MYC by Kinesin-1 for proteasomal degradation in the
AC C
671
EP
668
cytoplasm. Biochimica et Biophysica Acta (BBA) - Molecular Cell Research 1843:20272036.
674
Lee, O.R., Kim, S.J., Kim, H.J., Hong, J.K., Ryu, S.B., Lee, S.H., Ganguly, A., and Cho, H.-T.
675
(2010). Phospholipase A2 is required for PIN-FORMED protein trafficking to the plasma
676
membrane in the Arabidopsis root. The Plant Cell Online 22:1812-1825.
ACCEPTED MANUSCRIPT
677
Lindemose, S., O'Shea, C., Jensen, M.K., and Skriver, K. (2013). Structure, function and
678
networks of transcription factors involved in abiotic stress responses. International
679
Journal of Molecular Sciences 14:5842-5878. Lorenzo, O., Chico, J.M., Sánchez-Serrano, J.J., and Solano, R. (2004). JASMONATE-
681
INSENSITIVE1 encodes a MYC transcription factor essential to discriminate between
682
different jasmonate-regulated defense responses in Arabidopsis. The Plant Cell Online
683
16:1938-1950.
RI PT
680
Luo, J., Fishburn, J., Hahn, S., and Ranish, J. (2012). An integrated chemical cross-linking and
685
mass spectrometry approach to study protein complex architecture and function.
686
Molecular & Cellular Proteomics 11:M111. 008318.
688
Lüscher, B., and Vervoorts, J. (2012). Regulation of gene transcription by the oncoprotein MYC.
M AN U
687
SC
684
Gene 494:145-160.
Maier, A., Schrader, A., Kokkelink, L., Falke, C., Welter, B., Iniesto, E., Rubio, V., Uhrig, J.F.,
690
Hülskamp, M., and Hoecker, U. (2013). Light and the E3 ubiquitin ligase COP1/SPA
691
control the protein stability of the MYB transcription factors PAP1 and PAP2 involved in
692
anthocyanin accumulation in Arabidopsis. The Plant Journal 74:638-651.
TE D
689
Marino, D., Froidure, S., Canonne, J., Khaled, S.B., Khafif, M., Pouzet, C., Jauneau, A., Roby,
694
D., and Rivas, S. (2013). Arabidopsis ubiquitin ligase MIEL1 mediates degradation of the
695
transcription factor MYB30 weakening plant defence. Nature Communications 4:1476.
EP
693
Matsui, K., Umemura, Y., and Ohme‐Takagi, M. (2008). AtMYBL2, a protein with a single
697
MYB domain, acts as a negative regulator of anthocyanin biosynthesis in Arabidopsis.
698
The Plant Journal 55:954-967.
AC C
696
699
Micel, L.N., Tentler, J.J., Smith, P.G., and Eckhardt, G.S. (2013). Role of Ubiquitin Ligases and
700
the Proteasome in Oncogenesis: Novel Targets for Anticancer Therapies. Journal of
701
Clinical Oncology 31:1231-1238.
702
Miller, M.J., Scalf, M., Rytz, T.C., Hubler, S.L., Smith, L.M., and Vierstra, R.D. (2013).
703
Quantitative Proteomics Reveals Factors Regulating RNA Biology as Dynamic Targets
704
of Stress-induced SUMOylation in Arabidopsis. Molecular & Cellular Proteomics
705
12:449-463.
ACCEPTED MANUSCRIPT
706
Nakata, M. and Ohme-Takagi, M. (2013). Two bHLH-type transcription factors, JA-
707
ASSOCIATED MYC2-LIKE2 and JAM3, are transcriptional repressors and affect male
708
fertility. Plant Signaling and Behaviour 8:e26473. Nallamilli, B.R.R., Edelmann, M.J., Zhong, X., Tan, F., Mujahid, H., Zhang, J., Nanduri, B., and
710
Peng, Z. (2014). Global Analysis of Lysine Acetylation Suggests the Involvement of
711
Protein Acetylation in Diverse Biological Processes in Rice (Oryza sativa). PLoS ONE
712
9:e89283.
RI PT
709
Nemie-Feyissa, D., Olafsdottir, S.M., Heidari, B., and Lillo, C. (2014). Nitrogen depletion and
714
small R3-MYB transcription factors affecting anthocyanin accumulation in Arabidopsis
715
leaves. Phytochemistry 98:34-40.
SC
713
Ng, S., Ivanova, A., Duncan, O., Law, S.R., Van Aken, O., De Clercq, I., Wang, Y., Carrie, C.,
717
Xu, L., and Kmiec, B. (2013). A membrane-bound NAC transcription factor, ANAC017,
718
mediates mitochondrial retrograde signaling in Arabidopsis. The Plant Cell Online
719
25:3450-3471.
M AN U
716
Ni, W., Xu, S.-L., Tepperman, J.M., Stanley, D.J., Maltby, D.A., Gross, J.D., Burlingame, A.L.,
721
Wang, Z.-Y., and Quail, P.H. (2014). A mutually assured destruction mechanism
722
attenuates light signaling in Arabidopsis. Science 6:1160-1164.
TE D
720
Pauwels, L., Barbero, G.F., Geerinck, J., Tilleman, S., Grunewald, W., Perez, A.C., Chico, J.M.,
724
Bossche, R.V., Sewell, J., Gil, E., et al. (2010). NINJA connects the co-repressor
725
TOPLESS to jasmonate signalling. Nature 464:788-793.
EP
723
Pesch, M., Schultheiß, I., Digiuni, S., Uhrig, J.F., and Hülskamp, M. (2013). Mutual control of
727
intracellular localisation of the patterning proteins AtMYC1, GL1 and TRY/CPC in
728
AC C
726
Arabidopsis. Development 140:3456-3467.
729
Qi, T., Huang, H., Wu, D., Yan, J., Qi, Y., Song, S., and Xie, D. (2014). Arabidopsis DELLA
730
and JAZ Proteins Bind the WD-Repeat/bHLH/MYB Complex to Modulate Gibberellin
731 732 733
and Jasmonate Signaling Synergy. The Plant Cell 26:1118-1133. Raffaele, S., and Rivas, S. (2013). Regulate and be regulated: integration of defense and other signals by the AtMYB30 transcription factor. Frontiers in Plant Science 4:98.
ACCEPTED MANUSCRIPT
734 735
Ramsay, N.A., and Glover, B.J. (2005). MYB–bHLH–WD40 protein complex and the evolution of cellular diversity. Trends in Plant Science 10:63-70. Sahu, P., Pandey, G., Sharma, N., Puranik, S., Muthamilarasan, M., and Prasad, M. (2013).
737
Epigenetic mechanisms of plant stress responses and adaptation. Plant Cell Reports
738
32:1151-1159.
RI PT
736
Saijo, Y., Zhu, D., Li, J., Rubio, V., Zhou, Z., Shen, Y., Hoecker, U., Wang, H., and Deng, X.W.
740
(2008).Arabidopsis COP1/SPA1 complex and phytochrome A signaling intermediates
741
associate with distinct phosphorylated forms of phytochrome A in balancing signal
742
propagation and attenuation. Molecular Cell 31:607–613.
SC
739
Sasaki-Sekimoto, Y., Jikumaru, Y., Obayashi, T., Saito, H., Masuda, S., Kamiya, Y., Ohta, H.,
744
and Shirasu, K. (2013). Basic Helix-Loop-Helix transcription factors JASMONATE-
745
ASSOCIATED MYC2-LIKE1 (JAM1), JAM2, and JAM3 are negative regulators of
746
jasmonate responses in Arabidopsis. Plant Physiology 163:291-304.
M AN U
743
Schweizer, F., Bodenhausen, N., Lassueur, S., Masclaux, F.G., and Reymond, P. (2013).
748
Differential Contribution of Transcription Factors to Arabidopsis thaliana Defense
749
Against Spodoptera littoralis. Frontiers in Plant Science 4:13.
752 753 754 755 756 757 758 759 760
emphasis on intracellular movement. Journal of Integrative Plant Biology 56:334-342. Seo, P.J., and Mas, P. (2014). Multiple Layers of Posttranslational Regulation Refine Circadian
EP
751
Seo, P.J. (2014). Recent advances in plant membrane-bound transcription factor research:
Clock Activity in Arabidopsis. The Plant Cell Online 26: 79-87. Sonderby, I.E., Burow, M., Rowe, H.C., Kliebenstein, D.J., and Halkier, B.A. (2010). A complex
AC C
750
TE D
747
interplay of three R2R3 MYB transcription factors determines the profile of aliphatic glucosinolates in Arabidopsis. Plant Physiology 153:348-363.
Spitz, F., and Furlong, E.E. (2012). Transcription factors: from enhancer binding to developmental control. Nature Reviews. Genetics 13:613-626.
Spoel, S.H., and Loake, G.J. (2011). Redox-based protein modifications: the missing link in plant immune signalling. Current Opinion in Plant Biology 14:358-364.
ACCEPTED MANUSCRIPT
761 762
Stone, S.L. (2014). The role of ubiquitin and the 26S proteasome in plant abiotic stress signaling. Frontiers in Plant Science 5:135. Stracke, R., Ishihara, H., Huep, G., Barsch, A., Mehrtens, F., Niehaus, K., and Weisshaar, B.
764
(2007). Differential regulation of closely related R2R3-MYB transcription factors
765
controls flavonol accumulation in different parts of the Arabidopsis thaliana seedling.
766
The Plant Journal 50:660-677.
768
Stracke, R., Werber, M., and Weisshaar, B. (2001). The R2R3-MYB gene family in Arabidopsis thaliana. Current Opinion in Plant Biology 4:447-456.
SC
767
RI PT
763
Sun, X., Feng, P., Xu, X., Guo, H., Ma, J., Chi, W., Lin, R., Lu, C., and Zhang, L. (2011). A
770
chloroplast envelope-bound PHD transcription factor mediates chloroplast signals to the
771
nucleus. Nature Communications 2:477.
M AN U
769
772
Sønderby, I.E., Hansen, B.G., Bjarnholt, N., Ticconi, C., Halkier, B.A., and Kliebenstein, D.J.
773
(2007). A systems biology approach identifies a R2R3 MYB gene subfamily with distinct
774
and overlapping functions in regulation of aliphatic glucosinolates. PLoS ONE 2:e1322. Tavares, C.P., Vernal, J., Delena, R.A., Lamattina, L., Cassia, R., and Terenzi, H. (2014). S-
776
nitrosylation influences the structure and DNA binding activity of AtMYB30
777
transcription factor from Arabidopsis thaliana. Biochimica et Biophysica Acta (BBA)-
778
Proteins and Proteomics 1844:810-817.
781 782 783 784
EP
780
Toledo-Ortiz, G. (2003). The Arabidopsis Basic/Helix-Loop-Helix Transcription Factor Family. The Plant Cell Online 15:1749-1770. Vailleau, F., Daniel, X., Tronchet, M., Montillet, J.-L., Triantaphylidès, C., and Roby, D. (2002).
AC C
779
TE D
775
A R2R3-MYB gene, AtMYB30, acts as a positive regulator of the hypersensitive cell death program in plants in response to pathogen attack. Proc. Natl Acad. Sci. USA 99:10179-10184.
785
Wei, N., Kwok, S.F., von Arnim, A.G., Lee, A., McNellis, T.W., Piekos, B. and Deng, X.W.
786
(1994). Arabidopsis COP8, COP10, and COP11 genes are involved in repression of
787
photomorphogenic development in darkness. The Plant Cell 6: 629-643.
788
Wild, M., Daviere, J.M., Cheminant, S., Regnault, T., Baumberger, N., Heintz, D., Baltz, R.,
789
Genschik, P., and Achard, P. (2012). The Arabidopsis DELLA RGA-LIKE3 is a direct
ACCEPTED MANUSCRIPT
790
target of MYC2 and modulates jasmonate signaling responses. The Plant Cell 24:3307-
791
3319. Withers, J., Yao, J., Mecey, C., Howe, G.A., Melotto, M., and He, S.Y. (2012). Transcription
793
factor-dependent nuclear localization of a transcriptional repressor in jasmonate hormone
794
signaling. Proc. Natl Acad. Sci. 109:20148-20153.
RI PT
792
Wu, R.-C., Feng, Q., Lonard, D.M., and O'Malley, B.W. (2007). SRC-3 Coactivator Functional
796
Lifetime Is Regulated by a Phospho-Dependent Ubiquitin Time Clock. Cell 129:1125-
797
1140.
799
Xing, S., and Poirier, Y. (2012). The protein acetylome and the regulation of metabolism. Trends in Plant Science 17:423-430.
M AN U
798
SC
795
800
Xu, W., Grain, D., Le Gourrierec, J., Harscoët, E., Berger, A., Jauvion, V., Scagnelli, A., Berger,
801
N., Bidzinski, P., Kelemen, Z., et al. (2013). Regulation of flavonoid biosynthesis
802
involves an unexpected complex transcriptional regulation of TT8 expression in
803
Arabidopsis. New Phytologist 198:59-70.
Yan, J., Li, H., Li, S., Yao, R., Deng, H., Xie, Q., and Xie, D. (2013). The Arabidopsis F-box
805
protein CORONATINE INSENSITIVE1 is stabilized by SCFCOI1 and degraded via the
806
26S proteasome pathway. The Plant Cell 25:486-498.
TE D
804
Yang, Y., Ou, B., Zhang, J., Si, W., Gu, H., Qin, G., and Qu, L.J. (2014a). Arabidopsis Mediator
808
subunit MED16 regulates iron homeostasis by associating with EIN3/EIL1 through
809
subunit MED25. The Plant Journal 77:838-851.
811 812 813 814
Yang, Z.T., Wang, M.J., Sun, L., Lu, S.J., Bi, D.L., Sun, L., Song, Z.T., Zhang, S.S., Zhou, S.F.,
AC C
810
EP
807
and Liu, J.X. (2014b). The membrane-associated transcription factor NAC089 controls ER-stress-induced programmed cell death in plants. PLoS Genetics 10:e1004243.
Zentner, G.E., and Henikoff, S. (2012). Surveying the epigenomic landscape, one base at a time. Genome Biology 13:1186.
815
Zhai, Q., Yan, L., Tan, D., Chen, R., Sun, J., Gao, L., Dong, M.Q., Wang, Y., and Li, C. (2013).
816
Phosphorylation-coupled proteolysis of the transcription factor MYC2 is important for
817
jasmonate-signaled plant immunity. PLoS Genetics 9:e1003422.
ACCEPTED MANUSCRIPT
818
Zhao, L., Gao, L., Wang, H., Chen, X., Wang, Y., Yang, H., Wei, C., Wan, X., and Xia, T.
819
(2013). The R2R3-MYB, bHLH, WD40, and related transcription factors in flavonoid
820
biosynthesis. Functional & Integrative Genomics 13:75-98. Zheng, Y., Schumaker, K.S., and Guo, Y. (2012). Sumoylation of transcription factor MYB30 by
822
the small ubiquitin-like modifier E3 ligase SIZ1 mediates abscisic acid response in
823
Arabidopsis thaliana. Proc. Natl Acad. Sci. 109:12822-12827.
825
Zhou, H., Watts, J.D., and Aebersold, R. (2001). A systematic approach to the analysis of protein phosphorylation. Nature Biotechnology 19:375-378.
SC
824
RI PT
821
Zimmermann, I.M., Heim, M.A., Weisshaar, B., and Uhrig, J.F. (2004). Comprehensive
827
identification of Arabidopsis thaliana MYB transcription factors interacting with R/B‐
828
like BHLH proteins. The Plant Journal 40:22-34.
M AN U
826
AC C
EP
TE D
829
ACCEPTED MANUSCRIPT
830
Figure legends
831 Figure 1: Schematic representation of MYB and BHLH TFs. A) R2R3 MYB TFs have a
833
conserved DNA-Binding Domain (DBD) at the N-terminal of the protein and a more variable,
834
C-terminal Trans-Activation Domain (TAD). B) bHLH TFs of the MYC clade are characterized
835
by a bHLH domain containing the DNA binding motif (G-Box), a dimerization domain (DD)
836
and a Nuclear Localisation Signal (NLS) at the C-terminus. The JAZ Interaction Domain (JID) is
837
found in the N-terminal TAD.
SC
RI PT
832
M AN U
838
Figure 2: Signal integration by the hub TF MYC2. MYC2 has the ability to integrate multiple
840
environmental and developmental signals and to control the expression levels of various
841
pathways precisely in space and time. I: Constitutive expression levels and activation of MYC2
842
are balanced by different PTMs. II: Upon herbivore or JA treatment, MYC2 inhibition by JAZs
843
is released leading to an accumulation of active MYC2. III: Depending on the developmental
844
stage, DELLAs interact with MYC2 to inhibit its JA-dependent transcriptional activity. GA will
845
lead to MYC2 activation to trigger GA-mediated developmental processes. IV: Active MYC2
846
can bind different promoters and initiate specific responses. Squares represent MYC2 in an
847
inactive form, while circles depict active proteins. Roman numbers refer to different regulatory
848
layers described in the text. JA, jasmonic acid; GA, giberillic acid; PTM, post-transcriptional
849
modification.
EP
AC C
850
TE D
839
851
Figure 3: Combinatorial effects of PTMs and PPIs on MYB30 activity. MYB30 represents
852
an example of a TF that is regulated by multiple mechanisms on the protein level. Different
853
signals are integrated on this level to ensure tight regulation of a single output, i.e. cell death. I:
854
Basal levels of transcript lead to accumulation of MYB30 protein balanced between an active
855
and inactive state by different PTMs. Upon stimulation by hormones, transcript levels incease
856
and the balance shifts towards more active protein. II: when activated, the MYB30 binds specific
857
promoters and thereby induces cell death-specific genes. III: Cell death is tightly balanced by
ACCEPTED MANUSCRIPT
modifying enzymes which will inactivate the protein to ensure locally restrict cell death. Inactive
859
MYB30 is shown as square, the active form as circle. Roman numbers refer to different
860
regulatory layers that are described in the text. BRs, Brassinosteroids; SA, salicylic acid; ABA,
861
abscisic acid; PTM, post-transcriptional modification.
AC C
EP
TE D
M AN U
SC
RI PT
858
AC C
EP
TE D
M AN U
SC
RI PT
ACCEPTED MANUSCRIPT
AC C
EP
TE D
M AN U
SC
RI PT
ACCEPTED MANUSCRIPT
AC C
EP
TE D
M AN U
SC
RI PT
ACCEPTED MANUSCRIPT
S1674-2052(14)00048-3
DOI:
10.1016/j.molp.2014.11.022
Reference:
MOLP 47
To appear in:
MOLECULAR PLANT
Received Date: 1 September 2014 Revised Date:
10 November 2014
Accepted Date: 24 November 2014
Please cite this article as: Pireyre M., and Burow M. (2014). Regulation of MYB and bHLH transcription factors – a glance at the protein level. Mol. Plant. doi: 10.1016/j.molp.2014.11.022. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
ACCEPTED MANUSCRIPT
Title:
2
Regulation of MYB and bHLH transcription factors – a glance at the protein level
3 4
Running title:
6
Protein level regulation of transcription factors
7
Short summary:
This review summarizes the recent progress on molecular regulatory mechanisms of plant transcription factor families MYBs and bHLHs with focus on post-transcriptional modifications such as ubiquitination, phosphorylation, acetylation, and nitrosylation. We conclude by pointing to potential applications of state of the art techniques required to better understand the molecular basis of plant responses to environmental changes.
13
M AN U
8 9 10 11 12
SC
5
RI PT
1
Marie Pireyre and Meike Burow
15
DynaMo DNRF Center of Excellence , Department of Plant and Environmental Sciences,
16
Faculty of Science, University of Copenhagen, Thorvaldsensvej 40, 1871 Frederiksberg C,
17
Denmark
TE D
14
18 Corresponding author:
20
Meike Burow
21
Department of Plant and Environmental Sciences
22
Faculty of Science
23
University of Copenhagen
24
Thorvaldsensvej 40
25
1871 Frederiksberg C, Denmark
26
E-Mail: [email protected]
27
Phone: +45-35 33 37 73
28
Fax: +45-35 28 33 33
AC C
EP
19
ACCEPTED MANUSCRIPT
29
Abstract In complex, constantly changing environments, plants have developed astonishing
31
survival strategies. These elaborated strategies rely on rapid and precise gene regulation
32
mediated by transcription factors (TFs). TFs represent a large fraction of plant genomes and
33
among them, MYBs and bHLHs have unique inherent properties specific to plants. Proteins of
34
these two TF families can act as homo- or heterodimers, associate with proteins from other
35
protein families or form MYB/bHLH complexes to regulate distinct cellular processes. The
36
ability of MYBs and bHLHs to interact with multiple protein partners has evolved to keep up
37
with the increased metabolic complexity of multi-cellular organisms. Association and
38
disassociation of dynamic TF complexes in response to developmental and environmental cues
39
are controlled through a plethora of regulatory mechanisms specifically modulating TF activity.
40
Regulation of TFs at the protein level is critical for efficient and precise control of their activity
41
and thus provides the mechanistic basis for a rapid on-and-off switch of TF activity. In this
42
review, examples of post-translational modifications, protein-protein interaction and subcellular
43
mobilization of TFs will be discussed with regard to the relevance of these regulatory
44
mechanisms for the specific activation of MYBs and bHLHs in response to a given
45
environmental stimulus.
SC
M AN U
TE D
46
RI PT
30
Keywords: transcription factor, MYB, bHLH, post-translational modification, protein-protein
48
interaction, transcriptional regulation
AC C
49
EP
47
50
List of abbreviations: ABA, abscisic acid; bHLH, basic Helix-Loop-Helix; COI-1, coronatine-
51
insensitive protein 1; DBD, DNA-binding domain; GA, Gibberellic acid; HtH, Helix-turn-Helix;
52
HR, Hypersensitive Response; JA, jasmonic acid; JAZ; jasmonate ZIM-domain protein; MBW,
53
MYB/bHLH/WD40 complex; MTTF, membrane-tethered transcription factor; NLS, nuclear
54
localization signal; PPI, protein-protein interaction; PTM, post-transcriptional modification; SA,
55
salicylic acid; SUMO, Small Ubiquitin Modifier; TAD, transcriptional activation domain; TF,
56
transcription factor; UPS, Ubiquitin-Proteasome System.
ACCEPTED MANUSCRIPT
57
Introduction
58 In multicellular organisms, precise gene expression in time and space is regulated by
60
transcription factors (TFs). Mutants affected in spatio-temporal transcriptional regulation often
61
show dramatic developmental phenotypes underlining the importance of the functions of TFs and
62
the importance of efficient on-and-off switches for their activity. In Arabidopsis thaliana,
63
between 6-10% of all genes encode TFs in contrast to only 3% in Drosophila melanogaster and
64
5% in humans. This relatively large number of TFs might allow plants to rapidly adapt to the
65
changing environments they encounter, e.g. by synthesizing, transporting, and relocating
66
metabolites, RNAs, and proteins. A large proportion of the TFs in Arabidopsis are MYB (339)
67
and basic Helix-Loop-Helix (bHLH; 162) TFs. The members of these two transcription factor
68
families can act as homodimers, as heterodimers consisting of proteins from the same family, or
69
in complexes with TFs from other protein families. Interestingly, many cases of MYB/bHLH
70
complexes have been described and the parallel evolution of these two TF families has been
71
associated with the developmental and metabolic plasticity found in plants (Feller et al., 2011).
72
The structural, evolutionary and functional diversity of MYBs and bHLHs has been extensively
73
studied with regard to the distinct pathways controlled by these TFs as well as the mechanisms
74
regulating their activity (reviewed by Feller et al., 2011).
TE D
M AN U
SC
RI PT
59
Different MYB/bHLH complexes regulate distinct cellular processes such as cell wall
76
synthesis, cell death, circadian clock, responses to abiotic and biotic stress, hormone signaling
77
and the biosynthesis of specialized metabolites (Lindemose et al., 2013; Seo and Mas, 2014;
78
Stracke et al., 2007; Stracke et al., 2001; Vailleau et al., 2002). In many cases, bHLH are able to
79
physically interact with different MYBs to achieve their function. In addition, the activity of TFs
80
appears to be regulated by cytosolic WD40 repeat proteins through formation of highly dynamic
81
MYB/bHLH/WD40 (MBW) complexes (Feller et al., 2011). WD40s and bHLHs respond to a
82
variety of environmental triggers and thereby offer a flexible, inducible system to activate
83
transcription of multiple sets of genes, while MYB TFs confer specificity to transcriptional
84
activation (Ramsay and Glover, 2005). In line with the proposition that TF complexes
85
comprising MYBs and bHLHs have evolved to increase fitness in changing environments, MBW
86
complexes have only been described in plants so far.
AC C
EP
75
ACCEPTED MANUSCRIPT
TFs typically bind 6-12 bp long DNA sequences present in the promoters of multiple
88
target genes. A sequence of six specific nucleotides has a high probability to occur in the
89
genome. Moreover, the specificity of the DNA binding domain (DBD) is attributed rather to a
90
family or a clade of TFs than to individual TFs. Those observations speak against precise
91
transcriptional activation solely based on specificity in DNA binding and suggest instead that
92
additional regulatory mechanisms occur to insure high specificity of the transcriptional process.
93
DNA binding can be regulated by chromatin accessibility and nucleosome positioning (reviewed
94
by Spitz and Furlong, 2012), by enhancers, cofactors and protein-protein interactions (PPIs). In
95
this review, we will discuss the mechanisms underlying the spatio-temporal regulation of PPIs
96
and post-transcriptional modifications (PTMs) and their importance for a fast responding
97
regulatory system that includes TFs in an inactive form that can rapidly be activated upon need.
M AN U
SC
RI PT
87
The MYB TF family is divided into sub-clades according to the structure of the DBD that
99
contains one to three repeats (R1-R3) (Figure 1-I). Each repeat consists of approximately 53
100
amino acid residues that form a Helix-turn-Helix (HtH). The N-terminal R2R3 domain binds to
101
DNA and is highly conserved within the whole family. In contrast, the C-terminus of MYB TFs,
102
i.e. the transcriptional activation domain (TAD), is more variable (Dubos et al., 2010) and has
103
been predicted to fail formation of a stable secondary structure (Lindemose et al., 2013). The
104
highly conserved DBD suggests a common mechanism for the regulation of DNA binding,
105
whereas the variable TAD domain might modulate TF activation and DBD accessibility and
106
thereby confer specificity to DNA binding by MYB TFs. bHLH TFs are characterized by 60
107
conserved amino acids at the C-terminus forming a basic DBD and a dimerization domain
108
(Figure 1-II). Similar to C-terminal part of MYB proteins, the N-terminal part of bHLH proteins
109
is more variable and can be grouped by differences in the TADs (Dombrecht, 2007; Cheng,
110
2011; Chen, 2012). BHLH proteins bind to specific sequences called E-box (5'-CANNTG-3')
111
including the well-studied G-box (5'-CACGTG) (Toledo-Ortiz, 2003). In Arabidopsis, fourteen
112
R2R3 MYB and six R1 MYB proteins share a conserved bHLH binding motif
113
([DE]Lx2[RK]x3Lx6Lx3R), which is critical for promoter activation because it stabilizes
114
complexes of these MYBs with R/B-like bHLH proteins (Zhao et al., 2013; Zimmermann et al.,
115
2004). This bHLH binding motif was used to predict MYB/bHLH interactions indicating that the
116
presence of this motif in the MYB protein sequence contributes to MYB/bHLH association
AC C
EP
TE D
98
ACCEPTED MANUSCRIPT
117
(Zimmermann et al., 2004). Nevertheless, this motif does not explain the recruitment of a
118
specific bHLH protein. This review focuses on individual MYB and bHLH TFs as case studies for the regulation
120
TFs and their complexes on the protein level rather than on the specificity of TFs towards their
121
target promoters. As plants are well-known for their ability to control gene expression in a highly
122
coordinated manner, plant MYB/bHLH complexes constitute a suitable model to study dynamic
123
regulation of gene expression. In this review, the regulatory mechanisms of MYBs and bHLHs
124
controlling plant metabolic pathways will serve as examples. We have chosen jasmonate
125
signaling, flavonoid biosynthesis and cell death pathways to investigate functional pairs of
126
MYBs and bHLH proteins. First, background on the regulation of TF activation and activity
127
through MYB/bHLH complex formation will be given; second, TF regulation at the post-
128
transcriptional level will be introduced; and finally, the importance of these mechanisms for
129
stimuli-specific responses will be discussed.
M AN U
SC
RI PT
119
130
132 133
TE D
131
MYB/bHLH as regulators of plant defense pathways
As a part of jasmonate (JA)-mediated responses, the TFs MYC2-4 from the bHLH family
135
activate transcription of different sets of genes involved in plant responses to environmental cues
136
including hormone signaling and development (Chen et al., 2011; Cheng et al., 2011; Fernández-
137
Calvo et al., 2011; Lorenzo et al., 2004). The regulation of MYC2-4 is tightly controlled at the
138
protein level by a PPI/F-BOX/proteasome-based mechanism. Under uninduced conditions, MYC
139
proteins are bound to the repressors NINJA, TOPLESS (TPL) and Jasmonate ZIM-domain (JAZ)
140
proteins (Pauwels et al., 2010; Dombrecht et al., 2007; Lorenzo et al., 2004). Upon stimulation
141
e.g. by exogenous jasmonates or herbivory, the JAZ proteins are bound by the signal receptor F-
142
Box protein CORONATINE-INSENTIVE protein 1 (COI1) and thereby targeted for degradation
143
by the 26S proteasome (Chini et al., 2007; Yan et al., 2013). The MYCs are thereby liberated
144
from the complex to fulfill their function (Dombrecht et al., 2007; Lorenzo et al., 2004). As an
AC C
EP
134
ACCEPTED MANUSCRIPT
145
individual protein, MYC2 has been shown to integrate different signals and to contribute to the
146
regulation of multiple pathways leading to different phenotypic outputs. This makes MYC2 a
147
model TF to discuss the molecular basis of multi-functionality of a single TF (Figure 2). Flavonoids are a class of secondary metabolites involved in plant-environment
149
interactions (e.g. defense, pollinator attraction, UV filtration). They can be divided into three
150
groups: anthocyanins, flavonols and proanthocyanidins. All steps of anthocyanin biosynthesis are
151
regulated by dynamically associating and disassociating MBW complexes (Appelhagen et al.,
152
2011). While the early steps of the pathway are all controlled by MYB11, MYB12 and MYB111,
153
the last and anthocyanin-specific biosynthetic step is regulated by PAP1, PAP2, MYB111, or
154
MYB114. These MYBs interact with different bHLHs, namely TRANSPARENT TESTA8
155
(TT8), GLABROUS3 (GL3), or ENHANCER OF GL3 (EGL30) (Xu et al., 2013). The
156
regulation of the anthocyanin pathway has been extensively studied because of defensive and
157
anti-oxidant properties of the compounds and their role in fruit coloring. Thus, the key regulators
158
as well as some PTMs modulating their interactions are known. The current knowledge on the
159
pathway makes it a useful model to illustrate PPI- and PTM-mediated regulation of TF activity.
160
Hypersensitive response (HR) triggered by pathogens leads to rapid cell death around the
161
infected tissue and thus prevents microbes from spreading. MYB30 is a R2R3 MYB TF that has
162
been shown to be involved in pathogen-induced HR and cell death (Vailleau et al., 2002).
163
Depending on the process it is involved in, MYB30 interacts with different modifying enzymes
164
and undergoes different PTMs leading to its activation or repression (Raffaele and Rivas, 2013).
165
The regulatory network surrounding MYB30 represents a unique multi-step and multi-enzyme
166
regulatory system and will be discussed to illustrate PTM-specific effects on PPIs and the
167
importance of rapid TF deactivation (Figure 3).
169 170 171
SC
M AN U
TE D
EP
AC C
168
RI PT
148
Post-transcriptional activation and inactivation of TFs by ubiquitination
ACCEPTED MANUSCRIPT
PTMs include all modifications on the transcript or protein level after the gene has been read
173
by an RNA polymerase, e.g. alternative splicing, alternative translation start, and protein
174
structure modifications. The latter are mediated by enzymes that catalyze reactions such as
175
phosphorylation, acetylation, or ubiquitination. Depending on where and when a functional
176
group is added, the protein will mature, be activated or inactivated, sequestered or degraded.
177
Ubiquitination is a PTM process conducted by E1, E2, and E3 ligases that will lead to secondary
178
structural changes or protein poly-ubiquitination and subsequent degradation of the protein by
179
the 26S proteasome (Ubiquitin-Proteasome System, UPS). However, mono-ubiquitination of TFs
180
can also lead to proteolysis-independent effects on TF activity and DNA binding properties
181
(reviewed by Geng et al., 2012). Ubiquitination can be reversed by de-ubiquitinases, providing
182
flexibility to the ubiquitin-mediated protein degradation system.
M AN U
SC
RI PT
172
While the first ubiquitination step catalyzed by E1 and E2 ligases shows little specificity for
184
the protein targets, E3 ligases are substrate- or condition-specific. E3 ligases have been
185
extensively studied in mammalian systems as they can be targeted by different drugs (Micel et
186
al., 2013). In Arabidopsis, more than a thousand proteins have been predicted to possess E3
187
ligase activity. Extensive review articles on the action of E3 ligases in response to environmental
188
and developmental cues are available (Duplan and Rivas, 2014; Guo et al., 2013; Stone, 2014).
189
The high diversity of stress-responsive E3 ligases in plants appears to be critical for balancing
190
the TFs present in the cell and thus for mounting appropriate responses to environmental changes
191
with sufficient specificity.
EP
TE D
183
Recently, Marino et al. (2014) showed that the Arabidopsis E3 ligase MIEL1 was able to
193
leave ubiquitin marks on MYB30 leading to the degradation of MYB30 by the proteasome.
194
Under normal conditions, MIEL1 is sufficiently expressed to target MYB30 to degradation and
195
thus to attenuate its action to initiate cell death. Upon pathogen infection, MIEL1 expression is
196
inhibited which allows for higher accumulation of the MYB30 protein and subsequently leads to
197
pathogen-induced cell death (Figure 3, III) (Marino et al., 2013).
AC C
192
198
Similarly, the E3 ubiquitin ligase CONSTITUTIVE PHOTOMORPHO-GENESIS 1 (COP1)
199
controls the stability of the MYB proteins PAP1 and PAP2 to repress transcription of
200
anthocyanin biosynthesis genes only in dark grown plants (Maier et al., 2013). COP1 is generally
201
involved in light-controlled development and gene expression by targeting TFs for proteasome-
ACCEPTED MANUSCRIPT
mediated degradation in the dark (Deng et al., 1991; Wei et al., 1994). For instance, COP1
203
controls the expression of light-responsive genes by ubiquitination of unphosphorylated
204
phytochrome A in response to far red light (Saijo et al., 2008). Moreover, COP1 has been
205
demonstrated to affect the stability of MYC2 in a light-dependent manner (Chico et al., 2014).
206
Accordingly, shading has a repressive effect on JA signaling through degradation of the MYC2
207
protein by the 26S proteasome dependent on COP1 (Figure 2, I) (Chico et al., 2014). These
208
observations exemplify an elegant mechanism that controls the activity of a TF in a trigger-
209
specific manner, here light, while it still allows for fast activation of the downstream responses.
SC
RI PT
202
Ubiquitination possesses a dual role: It can lead to decreased protein accumulation through
211
proteasome-dependent degradation or it can alter TF activity. It has thus been proposed that
212
ubiquitination could act as a timer for the activity of TFs. Indeed, while the first ubiquitin added
213
to the TF is in some cases required for initiation of transcription by favoring DNA binding or by
214
recruiting the transcriptional machinery, subsequent poly-ubiquitination of the same TF on the
215
DNA can target the protein to the proteasome. Mono- followed by poly-ubiquitination thus
216
represents a potential on-and-off switch of TF activity and a high turnover at the promoters
217
(Kodadek et al., 2006). In this model, first described as the timer model, the TF has the time
218
required to bind to a target promoter and activate gene transcription while being poly-
219
ubiquitinated prior to degradation (Wu et al., 2007). Although this mechanism has not been
220
described in plants, yet, it may constitute a regulatory process that facilitates rapid TF activation
221
and high TF turnover to provide an efficient on-and-off switch in plant stress responses.
224 225
TE D
EP
223
AC C
222
M AN U
210
Reversible modification of TF proteins by lysine acetylation
226
Lysine acetylation is a reversible type of PTM mediated by lysine acetyl-transferases and
227
de-acetylases. The finding that acetylation regulates the activity of the animal TF p53 marked the
228
beginning of a new search for acetylated proteins. Indeed, numerous proteins involved in general
229
regulation of gene expression were shown to be acetylated in yeast and humans, including TFs
ACCEPTED MANUSCRIPT
and other DNA-binding proteins (Gu and Roeder, 1997). In plants, lysine acetylation has so far
231
been studied in processes such as cell wall modifications during plant infection, secondary
232
metabolism as well as chromatin remodeling through histone acetylation (Xing and Poirier,
233
2012). Recently, a global analysis of lysine acetylation in rice (Oryza sativa) underlined the role
234
of this PTM mechanism in multiple biological processes (Nallamilli et al., 2014). The nuclear-
235
localized, acetylated proteins identified in rice included primarily histones but also a few bHLHs.
236
In JA signaling, the repressor TPL interacts with MYC2 to inhibit MYC2 activity (Pauwels et al.,
237
2010; Dombrecht et al., 2007). TPL has been described as a Groucho (GR)/TP1 family protein,
238
involved in transcriptional repression by recruiting histone de-acetylase to induce local
239
chromatin compaction (Causier et al., 2012). Despite the technical limitations to study this PTM,
240
numerous lines of evidence suggest an effect of acetylation on transcriptional regulation. Further
241
studies are needed to understand the biological functions of acetylation of histones and TFs.
M AN U
SC
RI PT
230
242 243
245
Phosphorylation regulates TF activity and turnover
TE D
244
Phosphorylation has so far been the most-studied PTM due to its implication in MAP
247
kinase cascades. In mammals, the role of phosphorylation in signaling pathways was initially
248
described for the regulation of the cell cycle and for oncogenesis. This PTM was intensely
249
studied in the context of plant signaling during plant response to stress and immune response
250
(Boudsocq and Sheen, 2013; Kaufmann et al, 2011; Ni et al., 2014; Spoel and Loake, 2011).
251
Phosphorylation has moreover received a lot of attention because of the availability of a strong
252
anti-body for detection of phosphorylated proteins by Western blotting and because of its value
253
as a model PTM to detect modified peptides by LC-MS (Kaufman et al, 2011; Zhou et al., 2001).
254
Upon JA signaling, phosphorylation of MYC2 in its TAD domain induces its proteolysis
255
but also stimulates the transcriptional activity of MYC2 (Zhai et al., 2013). Based on these
256
findings, two rounds of DNA binding by two MYC2 proteins have been proposed to be
257
necessary to activate target gene transcription. It has been further suggested that there is a need
AC C
EP
246
ACCEPTED MANUSCRIPT
for a high turnover provided by the UPS. The degradation of the MYC2 bound in the first round
259
might favor binding of the next active MYC2 protein to the promoter, while on the other hand,
260
the presence of the first MYC2 at the promoter might decrease the target search time for the
261
second MYC2 protein. The observations made for MYC2 are not congruent with the “timer
262
model” above, but rather follow the proposed model of “activation by destruction” described in
263
mammals and yeast (Catic et al., 2013; Collins and Tansey, 2006; Geng et al., 2012) where TF
264
degradation is not only essential to regulate TF turnover but also dependent on the TF’s
265
transcriptional activity.
SC
RI PT
258
266
268
REDOX-dependent regulation of TFs
269
M AN U
267
Changes in the REDOX potential of the cell can affect disulfide bridges in TF proteins and
271
thereby affect their activity in response to stress conditions that lead to higher accumulation of
272
hormones in the cell, i.e. JA, Salicylic Acid (SA), ethylene, Gibberellic Acid (GA), Abscisic
273
Acid (ABA) and auxins. As an example, intracellular translocation of SA results in elevated
274
accumulation of glutathione as well as a shift in the ratio of reduced to oxidized glutathione
275
(Spoel and Loake, 2011). On the other hand, JA perception will decrease the pool of reduced
276
glutathione in favor of the oxidized form (Spoel and Loake, 2011). These changes in the
277
REDOX state can be perceived by reactive cysteines of regulatory proteins and thereby lead to
278
changes in their structure. Heine and coworkers identified two conserved cysteine residues as a
279
regulatory module in the R2R3 domain of MYB TFs (Heine et al., 2004). In the absence of
280
reducing agents, MYB TFs were not able to bind DNA in vitro. While cys-53 is highly
281
conserved among MYBs from different organisms, cys-49 is specific to plant R2R3 domains.
282
The emergence of this second cysteine residue in plants has been suggested to change the
283
accessibility of cys-53 as thus its capacity to form a disulfide bond. Cys-49 might therefore
284
regulate the DNA binding capacity of the plant MYB TFs by modulating their dimerization
285
capabilities. This higher complexity observed in plants talks in favor of a mechanistic adaptation
286
to ensure fast and specific responses to different internal or external signals (Figure 3, II).
AC C
EP
TE D
270
ACCEPTED MANUSCRIPT
Another type of REDOX-related PTMs is nitrosylation. Following REDOX changes in the
288
cell, S-nitroglutathione donors change availability. In mammalian systems, nitrosylation of the
289
myc oncogenic proteins has been reported to reduce their DNA binding capacity (Brendeford et
290
al., 1998; Lüscher and Vervoorts, 2012). In plants, the activity of MYB30 has been shown to be
291
influenced by S-nitrosylation through regulation of the secondary structure of its R2R3 domain
292
(Tavares et al., 2014). Moreover and in accordance with the previous paragraph, treatment of
293
nitrosylated MYB30 with reducing agent partially restored its capacity to interact with DNA,
294
thus confirming that the REDOX state of the protein can change its ability to bind DNA (Tavares
295
et al., 2014). In the case of MYB30, SA-induced stress decreases the pool of S-nitroglutathione
296
donors leading to increased activity of MYB30 and thus to pathogen-induced cell death. On the
297
other hand, a JA-induced increase of the available pool of oxidized donors might lead to an
298
increase in MYB30 nitrosylation and a decrease in its activity (Figure 3, II). The REDOX state
299
of the cell might thereby play a role in crosstalk between SA and JA signaling.
M AN U
SC
RI PT
287
300 301
303
Stabilization of MYB by sumoylation
TE D
302
SUMO stands for Small Ubiquitin Modifier and refers to a protein able to covalently attach
305
itself to another protein. SUMO has been shown to be involved in different regulatory processes
306
such as nucleus-to-cytosol protein translocation, protein degradation, plant development (Conti
307
et al., 2014; Elrouby, 2014), and stress responses (Miller et al., 2013). In ABA signaling, gene
308
expression studies combined with phenotypic analyses have demonstrated a functional
309
relationship between MYB30 and the small ubiquitin-like modifier E3 ligase SIZ1 (Zheng et al.,
310
2012). Upon ABA treatment, it has been shown that SIZ1 has the capacity to stabilize MYB30
311
by sumoylation of the K283 residue (Figure 3, II) (Zheng et al., 2012). This observation adds
312
another mechanism to the model of stress-induced control of TFs by PTMs to mount rapid and
313
specific responses in changing environment. It appears advantageous to have key regulators
314
available as inactive proteins that can be activated by different PTMs occurring in response to
315
different signals. Different PTMs regulate the stability/turnover, the DNA binding and the
AC C
EP
304
ACCEPTED MANUSCRIPT
activation of TFs which points at the need for robust coordination of these mechanisms. This
317
complexity in TF regulation by PTMs confers the capacity of plant regulatory systems to
318
integrate multiple signals. It also adumbrates the importance of combinatorial effects of different
319
PTMs for the activation and the deactivation of TFs.
RI PT
316
320 321
Membrane-tethered TFs require activation by proteolytic cleavage
SC
322 323
Membrane-tethered transcription factors (MTTF) are membrane-bound TFs that are activated
325
through cleavage by a protease which releases the DBD and allows its translocation to the
326
nucleus. Plant MTTFs have been shown to be involved in Endoplasmic Reticulum (ER) and
327
mitochondrial retrograde signaling (De Clercq et al., 2013; Ng et al., 2013; Yang et al., 2014b).
328
In mammals, MTTFs have been extensively studied as part of the unfolded protein responses
329
associated with Alzheimer’s disease and due to their role in Notch signaling (Brown et al., 2000).
330
The regulation of their proteolytic activation seems to be linked to protease activity as well as
331
membrane fluidity. In plants, seven MTTFs from the bZIP and NAC TF family as well as one
332
Membrane-anchored MYB (MaMYB) have been described to date (Chen et al., 2008; De Clercq
333
et al., 2013; Ng et al., 2013; Seo, 2014; Yang et al., 2014b). Their rapid release upon changes in
334
the cellular environment has been hypothesized to play a role in rapid stress responses (Chen et
335
al., 2008).
AC C
EP
TE D
M AN U
324
336
The identification of MaMYB was the first and is so far the only case of an ER-anchored
337
MYB TF (Dunkley et al, 2006). Whereas the membrane localization of the full-length MaMYB
338
and the nuclear localization of a truncated form have been demonstrated, no experimental proof
339
of cleavage and re-localization has been furnished to date. This unique case of MTTF behavior in
340
the MYB family could be important for induced responses. The protein might be kept at the ER
341
to be quickly released upon stress. More recently, ANAC013 and ANAC017 have been shown to
342
be membrane-anchored to the chloroplast and their proteolysis upon H2O2 stress liberates their
343
C-terminal DBD which is then be targeted to the nucleus. (De Clercq et al., 2013; Ng et al.,
ACCEPTED MANUSCRIPT
2013). The same has been described for a membrane-bound plant homeodomain transcription
345
factor, released upon proteolysis and associated with histone modifications in response to
346
retrograde signaling (Sun et al, 2011). In both cases, stress responses appear to regulate
347
transcriptional activation by cleaving membrane-bound regulatory proteins and releasing their
348
DBD. Nevertheless, no direct experimental evidence for this mechanisms has been provided for
349
a member of the MYB or bHLH family.
RI PT
344
350
TF localization can be modulated by interacting partners
M AN U
352
SC
351
353
TFs without a membrane anchor can also reside in the cytosol, either as free, soluble proteins
355
or physically associated with soluble cytoplasmic proteins until they tranlocate to the nucleus
356
upon a trigger. One example is the bHLH TF MYC1, a regulator of root hair development and
357
trichome patterning (Pesch et al., 2013). Despite the presence of a Nuclear Localization Signal
358
(NLS) as also described for other bHLH, the soluble MYC1 protein has been shown to mostly
359
reside in the cytosol, which also determines the localization of the bHLH TF GLABRA1 (GL1),
360
another regulator of trichome development. Upon interaction with MYC1, GL1 has been shown
361
to be re-localized from the nucleus to the cytosol, which inhibits its function as transcriptional
362
activator in the nucleus (Pesch et al., 2013). Although MYC1 induces trichome development,
363
MYC1 over-expression lines showed lower trichome density. Overexpression of MYC1 might
364
disturb the stoichiometry of the TF complex and thereby trichome development. GL1, likely in
365
combination with other TFs, has been suggested to bind the MYC1 promoter to form a negative
366
feedback loop and thereby balance MYC1expression levels (Pesch et al., 2013). MYC1 thus
367
constitutes an example of TF regulation comprising multiple regulatory layers on the protein
368
level. First, the GL1/MYC1 complex is formed and activated. Second, GL1 activity is repressed
369
by subcellular re-localization of the protein mediated by MYC1. Finally, active TF complexes
370
can feedback-regulate MYC1 transcription. In this example, a TF both activates and represses the
371
same pathway dependent on its concentration and the presence of its interacting partners.
AC C
EP
TE D
354
ACCEPTED MANUSCRIPT
The identification of mechanisms regulating the subcellular localization of TFs has recently
373
provided new insight into retrograde signaling in response to stress. Future studies on stress-
374
induced changes in membrane composition and their relevance for TF cleavage will deepen our
375
understanding of the fast responses to complex triggers characteristic for plants. The regulatory
376
mechanism of MTTF activation by proteolytic cleavage is likely to be extended to TFs that do
377
not possess a membrane anchor themselves but are anchored through interacting partners. A
378
membrane-anchored protein, potentially acting as a signal receptor, could interact with a TF and
379
dissociation of the complex could release the TF and enable rapid fine-tuning of transcriptional
380
regulation.
SC
RI PT
372
M AN U
381 382 383
The role of TF complexes in the nucleus
384
In 2008, small TFs that repress the transcriptional activity of MYBs have been described in
386
plants (Dubos et al., 2008). Those small MYB-like proteins, which only contain the R3 domain,
387
inhibit transcriptional activation by R2R3 MYBs by competing with them for formation of
388
MBW complexes. Therefore, TFs possessing only a R3 domain are generally predicted to be
389
repressors of transcription (Dubos et al., 2008). In the case of the flavonoid biosynthetic
390
pathway, numerous small proteins negatively regulate the formation of active MBW complexes
391
by interacting with the bHLHs in these complexes (Dubos et al., 2008; Matsui et al., 2008;
392
Nemie-Feyissa et al., 2014). The expression of small R3 proteins is regulated by environmental
393
and developmental factors. When co-expressed with the MYB TFs controlling anthocyanin
394
biosynthesis, the MYB-like proteins compete for binding to the bHLHs involved, which leads to
395
disruption of MBW complexes and thereby counter-balances MYB activity e.g. during nitrate
396
starvation (Nemie-Feyissa et al., 2014). Moreover, miRNA156 has been shown to influence
397
MBW complexes by activating SQUAMOSA PROMOTER BINDING PROTEIN-LIKE (SPL)
398
proteins that compete for bHLH binding and thereby coordinate anthocyanin production during
399
the transition from the vegetative to the reproductive stage (Gou et al., 2011). This example
AC C
EP
TE D
385
ACCEPTED MANUSCRIPT
400
illustrates how different conditions can affect regulation of a biosynthetic pathway by controlling
401
inhibitors of TF activity. Similar to the regulation of the MYB TFs controlling anthocyanin biosynthesis, negative
403
regulators modulates the transcriptional activity of MYB30. The secretory phospholipase PLA2
404
protein localizes to the Golgi where it controls auxin-dependent protein trafficking (Lee et al.,
405
2010) and possibly regulates plant defense chemistry independently of its enzymatic function
406
(Froidure et al., 2010). In the nucleus, PLA2-α inhibits MYB30 through physical interaction.
407
Upon pathogen attack, expression of PLA2-α is induced in periphery of the infection zone
408
suggesting a role for PLA2-α in limiting the HR response mediated by MYB30 (Figure 2, III).
SC
RI PT
402
Examples of TF regulation by PPIs in the nucleus can also be found in the bHLH family.
410
Recently, different labs identified a new clade of transcriptional regulators that are
411
phylogenetically closely related to the MYC2-4. BHLH003, bHLH013 and bHLH017 (also
412
named JAM1, JAM2 and JAM3) bind DNA with a specificity similar to that of MYC2, MYC3,
413
and MYC4 suggesting that they might compete with the MYCs for the binding of cis-regulatory
414
elements (Fonseca et al., 2014; Nakata and Ohme-Takagi, 2013; Sasaki-Sekimoto et al., 2013).
415
Importantly, physical interaction between the JAMs and MYC2 appears to play a role in the
416
nuclear targeting of JAZ1 and JAZ9 (Withers et al., 2012). Since the MYC TFs are almost
417
constitutively expressed in all tissues, their regulation at the PPI level is likely to be of primary
418
importance for their biological functions. Indeed, while MYC2 is present in various tissues at
419
various stages during development, it drives transcription only under certain conditions
420
dependent on its interacting partners.
EP
TE D
M AN U
409
MYC2, MYC3 and MYC4, have been shown to physically associate with MYB28, MYB29,
422
MYB76, MYB51, MYB34 and MYB122 to regulate the accumulation of glucosinolate defense
423
compounds (Figure 1, III) (Schweizer et al., 2013; Frerigmann et al., 2014). The expression
424
patterns of the six MYB TFs show high similarity (Gigolashvili et al., 2007a; Gigolashvili et al.,
425
2007b; Hirai et al., 2007; Sønderby et al., 2007) and strongly overlap with those of the MYCs.
426
Although all three MYCs can interact with all six MYBs (Frerigmann et al., 2014; Schweizer et
427
al., 2013), highly specific changes in the glucosinolate output can be triggered by different
428
hormones or stresses (Beekwilder et al., 2008; Frerigmann and Gigolashvili, 2014; Sonderby et
AC C
421
ACCEPTED MANUSCRIPT
al., 2010). Accordingly, analysis of glucosinolate levels in myc and myb single and double
430
mutants revealed specific mutant profiles (Frerigmann and Gigolashvili, 2014; Schweizer et al.,
431
2013; Sonderby et al., 2010) suggesting specific in planta roles of the individual TFs that cannot
432
be fully compensated by their closest homologues.
RI PT
429
Another example of TF complex-mediated transcriptional regulation is the interaction
434
DELLA and JAZ proteins, which provides the molecular basis of synergism between GA and JA
435
signaling (Hou et al., 2014). Both JA and GA have been shown to induce degradation of DELLA
436
and JAZ proteins to coordinately activate the MBW complex required to induce trichome
437
initiation (Qi et al., 2014). The DELLAs compete with the MYCs to bind the JAZs, thus
438
inducing JA-independent MYC2 activity (Figure 2-III) (Davière et al., 2008; Wild et al., 2012,
439
Hou et al., 2010; Lan et al., 2014). Upon increased GA levels, DELLAs are degraded and
440
MYC2-dependent JA synthesis is inhibited. The interaction of the DELLAs with MYC2
441
mediates induction of sesquiterpene synthase genes in a JA and red light dependent manner
442
(Hong et al., 2012). JA and GA signaling thus exhibit balancing effects on each other’s pathways
443
depending on their abundance in the cell. The molecular basis of the synergy between JAZ and
444
DELLA proteins provides insight into how plants integrate different signals, how they sense
445
environmental changes and how they prioritize different processes. This allows plants to
446
orchestrate their responses precisely in space and time and thus to optimize their fitness in
447
fluctuating environments.
450 451 452
M AN U
TE D
EP
449
AC C
448
SC
433
Integration of regulatory mechanisms
An individual TF can be involved in multiple biological processes during the plant’s life
453
cycle. Combinations of different PTMs and PPIs serve to establish different layers of TF
454
regulation on the protein level specific to environmental changes. To optimize their fitness,
455
plants have built complex regulatory systems ensuring fast and robust responses. A large number
456
of modifications occurring at the protein level modulate TF activity e.g. through altering the TF’s
ACCEPTED MANUSCRIPT
457
ability to bind interaction partners or DNA, through a change in turnover rate, or through
458
ubiquitination-dependent timing of degradation. In combination, all these mechanisms contribute
459
to the specificity of plant responses and at the same time increase their plasticity. The bHLH transcription factor MYC2 has been described as a master regulator of various
461
plant defense pathways in response to different environmental cues (Figure 2) (Kazan and
462
Manners, 2013). The idea that MYC2 has a more general effect on transcriptional activation
463
rather that high specificity to its target promoters is supported by the finding that MYC2 does not
464
act as transcriptional activator without an interaction partner (Kazan and Manners, 2013).
465
Instead, MYC2’s intrinsic property to bind different partners in different transcriptional networks
466
allows the plant to coordinate multiple signals and mount appropriate responses. The regulation
467
of DNA availability at the target loci has not been discussed in this review, but there is
468
experimental evidence suggesting that TFs also interact with histone-modifying enzymes as well
469
as mediator complexes (Badeaux and Shi, 2013; Lai et al., 2014; Yang et al., 2014a).
M AN U
SC
RI PT
460
As discussed above, flavonoids constitute a well-studied class of secondary plant
471
metabolites. Contrary to the example of MYC2, which represents the case of a TF as a hub, the
472
anthocyanin pathway is an example of a complex TF network regulating one specific output.
473
Although multiple PPIs and specific expression patterns have been identified, the fine-tuning of
474
flavonoid accumulation keeps providing novel insight into how a multitude of regulatory
475
mechanisms insure specificity of MYB/bHLH complexes. In the future, the regulatory network
476
controlling anthocyanin biosynthesis could serve as a model pathway to build in silico tools for
477
the integration of both mechanistic models and larger gene network effects on the composition of
478
TF complexes in a pathway-specific context. As different TFs have been shown to control the
479
different parts of the pathway in a tightly controlled way, anthocyanin biosynthesis could prove
480
its value as a model for other metabolic pathways, e.g. to predict the flux through a pathway for
481
engineering purposes.
EP
AC C
482
TE D
470
In this review, MYB30 served as example of a TF involved in different stress responses
483
and modulated by different PTMs (Figure 3). The different interactors and modifying enzymes
484
allow for tight control of MYB30 activity in terms of a specific spatial and temporal regulation
485
of its targets genes. The mechanisms controlling MYB30 activity support a model in which
486
different trigger-specific signaling pathways have the same biological output, i.e. cell death. This
ACCEPTED MANUSCRIPT
type of regulation facilitates the adaptation of the regulation of a specific TF to different cellular
488
environments, e.g. maybe changing its ability to bind interaction partners depending. In different
489
cell types, the activity of MYB30 can be regulated through interaction with different partners and
490
through different PTMs. As opposed to MYC2 as an example of a TF with multiple targets and a
491
broad effect on transcriptional activation, future studies on MYB30 have the potential to
492
elucidate what confers specificity in DNA binding downstream of different internal and external
493
cues.
RI PT
487
SC
494 495 Future outlook
M AN U
496 497
Comprehension of the complexity of transcriptional regulation will strongly benefit from
499
a deeper understanding of the underlying mechanistic events. Thus, studies that investigate how
500
TFs function at the single molecule level will help to improve current models of transcriptional
501
regulation. Chen et al. (2014) have recently proposed a technique to visualize the binding of
502
single proteins to DNA which can help to resolve trial-and-error calculations of TF binding. This
503
approach allows classification of TFs in complexes based on their promoter search method and
504
binding order. Future studies using this and similar approaches to study know TF complexes will
505
provide valuable mechanistic insight into how TFs associate and disassociate to control the
506
expression of their target genes. In the case of MYC2, this level of mechanistic understanding
507
may explain how MYC2 can activate different target genes dependent on its interacting partners.
EP
AC C
508
TE D
498
The challenges to improve our understanding of the DNA binding specificity of TFs that
509
serve as regulatory hubs, like MYC2, are linked to their involvement in fast and cell-specific
510
responses. Thus, using tools for in planta visualization of bHLHs and their interactors as well as
511
investigating the chromatin landscape in the neighborhood of TF target promoters will provide
512
novel insight into the specificity of TF-DNA interaction (Sahu et al., 2013). Next generation
513
Chromatin-Immuno-Precipitation (ChIP) assays such as exo-ChIP with higher sensitivity and
514
higher spatial and temporal resolution will enable us to obtain a more comprehensive image of
ACCEPTED MANUSCRIPT
what happens in the cell (Zentner and Henikoff, 2012). This kind of in planta studies are
516
necessary because of the complexity of plants as multicellular organisms and will help to
517
integrate cell-to-cell communication with different signaling mechanisms controlling TF
518
activation (Chen and Zhu, 2004). Studies combining proteasome inhibitors and ChIP have
519
already been used in mammalian cells will also be needed in plants to detect DNA-associated
520
protein degradation, thereby e.g. linking MYC2 activity with turnover of the protein at the
521
promoter (Catic et al., 2013).
RI PT
515
Finally, recent advances in immuno-precipitation techniques and mass spectrometry will
523
enable the identification of novel components of regulatory protein complexes, As an example, a
524
cross-linking strategy combined with mass spectrometry was recently successful in identifying
525
protein complexes in planta (Luo et al., 2012). This methodology can in the future be extended
526
to the enrichment of cells or organelles isolated from plants grown under specific conditions at
527
different time points to study the dynamics of protein complex formation and to determine which
528
interaction partners are available in a given cell. Integrative bioinformatics will be key to
529
incorporate these proteomics data with transcriptional network models.
M AN U
SC
522
531
TE D
530
Acknowledgments
533
The authors thank Frederik Rook and Sophie Lambertz for critical reading of the manuscript.
EP
532
AC C
534 535
Funding
536
Financial support was provided by the Danish National Research Foundation DNRF grant 99.
537 538 539
References
ACCEPTED MANUSCRIPT
540 Appelhagen, I., Jahns, O., Bartelniewoehner, L., Sagasser, M., Weisshaar, B., and Stracke, R.
542
(2011). Leucoanthocyanidin Dioxygenase in Arabidopsis thaliana: Characterization of
543
mutant alleles and regulation by MYB–BHLH–TTG1 transcription factor complexes.
544
Gene 484:61-68.
545 546
RI PT
541
Badeaux, A.I., and Shi, Y. (2013). Emerging roles for chromatin as a signal integration and storage platform. Nature reviews. Molecular Cell Biology 14:211-224.
Beekwilder, J., van Leeuwen, W., van Dam, N.M., Bertossi, M., Grandi, V., Mizzi, L., Soloviev,
548
M., Szabados, L., Molthoff, J.W., and Schipper, B. (2008). The impact of the absence of
549
aliphatic glucosinolates on insect herbivory in Arabidopsis. PLoS ONE 3:e2068.
551
M AN U
550
SC
547
Boudsocq, M., and Sheen, J. (2013). CDPKs in immune and stress signaling. Trends in Plant Science 18:30-40.
Brendeford, E.M., Andersson, K.B., and Gabrielsen, O.S. (1998). Nitric oxide (NO) disrupts
553
specific DNA binding of the transcription factor c-Myb in vitro. FEBS Letters 425:52-56.
554
Brown, M.S., Ye, J., Rawson, R.B., and Goldstein, J.L. (2000). Regulated intramembrane
555
TE D
552
proteolysis: a control mechanism conserved from bacteria to humans. Cell 100:391-398. Catic, A., Suh, Carol Y., Hill, Cedric T., Daheron, L., Henkel, T., Orford, Keith W.,
557
Dombkowski, David M., Liu, T., Liu, X.S., and Scadden, David T. (2013). Genome-wide
558
Map of Nuclear Protein Degradation Shows NCoR1 Turnover as a Key to Mitochondrial
559
Gene Regulation. Cell 155:1380-1395.
561 562 563
Causier, B., Ashworth, M., Guo, W., and Davies, B. (2012). The TOPLESS interactome: a
AC C
560
EP
556
framework for gene repression in Arabidopsis. Plant Physiology 158:423-438.
Chen, W.J., and Zhu, T. (2004). Networks of transcription factors with roles in environmental stress response. Trends in Plant Science 9:591-596.
564
Chen, Y.-N., Slabaugh, E., and Brandizzi, F. (2008). Membrane-tethered transcription factors in
565
Arabidopsis thaliana: novel regulators in stress response and development. Current
566
Opinion in Plant Biology 11:695-701.
ACCEPTED MANUSCRIPT
567
Chen, Y., Pang, Q., Dai, S., Wang, Y., Chen, S., and Yan, X. (2011). Proteomic identification of
568
differentially expressed proteins in Arabidopsis in response to methyl jasmonate. Journal
569
of Plant Physiology 168:995-1008. Chen, J., Zhang, Z., Li, L., Chen, B.C., Revyakin, A., Hajj, B., Legant, W., Dahan, M., Lionnet,
571
T., Betzig, E., et al. (2014). Single-molecule dynamics of enhanceosome assembly in
572
embryonic stem cells. Cell 156:1274-1285.
RI PT
570
Cheng, Z., Sun, L., Qi, T., Zhang, B., Peng, W., Liu, Y., and Xie, D. (2011). The bHLH
574
transcription factor MYC3 interacts with the jasmonate ZIM-domain proteins to mediate
575
jasmonate response in Arabidopsis. Molecular Plant 4:279-288.
SC
573
Chico, J.-M., Fernández-Barbero, G., Chini, A., Fernández-Calvo, P., Díez-Díaz, M., and
577
Solano, R. (2014). Repression of Jasmonate-Dependent Defenses by Shade Involves
578
Differential Regulation of Protein Stability of MYC Transcription Factors and Their JAZ
579
Repressors in Arabidopsis. The Plant Cell Online 26:1967-1980.
M AN U
576
Chini, A., Fonseca, S., Fernandez, G., Adie, B., Chico, J., Lorenzo, O., Garcia-Casado, G.,
581
Lopez-Vidriero, I., Lozano, F., and Ponce, M. (2007). The JAZ family of repressors is the
582
missing link in jasmonate signalling. Nature 448:666-671.
583 584
TE D
580
Collins, G.A., and Tansey, W.P. (2006). The proteasome: a utility tool for transcription? Current Opinion in Genetics & Development 16:197-202. Conti, L., Nelis, S., Zhang, C., Woodcock, A., Swarup, R., Galbiati, M., Tonelli, C., Napier, R.,
586
Hedden, P., and Bennett, M. (2014). Small Ubiquitin-like Modifier Protein SUMO
587
Enables Plants to Control Growth Independently of the Phytohormone Gibberellin.
588
Developmental Cell 28:102-110.
AC C
EP
585
589
Davière, J.-M., de Lucas, M., and Prat, S. (2008). Transcriptional factor interaction: a central
590
step in DELLA function. Current Opinion in Genetics & Development 18:295-303.
591
De Clercq, I., Vermeirssen, V., Van Aken, O., Vandepoele, K., Murcha, M.W., Law, S.R., Inze,
592
A., Ng, S., Ivanova, A., Rombaut, D., et al. (2013). The membrane-bound NAC
593
transcription factor ANAC013 functions in mitochondrial retrograde regulation of the
594
oxidative stress response in Arabidopsis. The Plant Cell 25:3472-3490.
ACCEPTED MANUSCRIPT
595
Deng, X.W., Caspar, T., and Quail, PH. (1991). Cop1: a regulatory locus involved in light-
596
controlled development and gene expression in Arabidopsis. Genes and Development
597
5:1172-1182. Dombrecht, B., Xue, G.P., Sprague, S.J., Kirkegaard, J.A., Ross, J.J., Reid, J.B., Fitt, G.P.,
599
Sewelam, N., Schenk, P.M., and Manners, J.M. (2007). MYC2 differentially modulates
600
diverse jasmonate-dependent functions in Arabidopsis. The Plant Cell Online 19:2225-
601
2245.
RI PT
598
Dubos, C., Le Gourrierec, J., Baudry, A., Huep, G., Lanet, E., Debeaujon, I., Routaboul, J.M.,
603
Alboresi, A., Weisshaar, B., and Lepiniec, L. (2008). MYBL2 is a new regulator of
604
flavonoid biosynthesis in Arabidopsis thaliana. The Plant Journal 55:940-953.
609 610 611 612 613 614 615 616 617 618 619
M AN U
608
Dunkley, T.P.J., Hester, S., Shadforth, I.P. et al. (2006). Mapping the Arabidopsis organelle proteome. Proc. Natl Acad. Sci. USA 103:6518–6523.
Duplan, V., and Rivas, S. (2014). E3 ubiquitin-ligases and their target proteins during the regulation of plant innate immunity. Frontiers in Plant Science 5:42.
TE D
607
transcription factors in Arabidopsis. Trends in Plant Science 15:573-581.
Elrouby, N. (2014). Extent and significance of non-covalent SUMO interactions in plant development. Plant Signaling & Behavior 9:e27948. Feller, A., Machemer, K., Braun, E.L., and Grotewold, E. (2011). Evolutionary and comparative
EP
606
Dubos, C., Stracke, R., Grotewold, E., Weisshaar, B., Martin, C., and Lepiniec, L. (2010). MYB
analysis of MYB and bHLH plant transcription factors. The Plant Journal 66:94-116. Fernández-Calvo, P., Chini, A., Fernández-Barbero, G., Chico, J.-M., Gimenez-Ibanez, S.,
AC C
605
SC
602
Geerinck, J., Eeckhout, D., Schweizer, F., Godoy, M., and Franco-Zorrilla, J.M. (2011). The Arabidopsis bHLH transcription factors MYC3 and MYC4 are targets of JAZ repressors and act additively with MYC2 in the activation of jasmonate responses. The Plant Cell Online 23:701-715.
620
Fonseca, S., Fernández-Calvo, P., Fernández, G.M., Díez-Díaz, M., Gimenez-Ibanez, S., López-
621
Vidriero, I., Godoy, M., Fernández-Barbero, G., Van Leene, J., and De Jaeger, G. (2014).
622
bHLH003, bHLH013 and bHLH017 Are New Targets of JAZ Repressors Negatively
623
Regulating JA Responses. PloS ONE 9:e86182.
ACCEPTED MANUSCRIPT
624 625
Frerigmann, H., and Gigolashvili, T. (2014). MYB34, MYB51 and MYB122 Distinctly Regulate Indolic Glucosinolate Biosynthesis in Arabidopsis thaliana. Molecular Plant. Froidure, S., Canonne, J., Daniel, X., Jauneau, A., Briere, C., Roby, D., and Rivas, S. (2010).
627
AtsPLA2-alpha nuclear relocalization by the Arabidopsis transcription factor AtMYB30
628
leads to repression of the plant defense response. Proc. Natl Acad. Sci. USA 107:15281-
629
15286.
631
Geng, F., Wenzel, S., and Tansey, W.P. (2012). Ubiquitin and Proteasomes in Transcription. Annual Review of Biochemistry 81:177-201.
SC
630
RI PT
626
Gigolashvili, T., Berger, B., Mock, H.P., Muller, C., Weisshaar, B., and Fluegge, U.I. (2007a).
633
The transcription factor HIG1/MYB51 regulates indolic glucosinolate biosynthesis in
634
Arabidopsis thaliana. The Plant Journal 50:886-901.
M AN U
632
Gigolashvili, T., Yatusevich, R., Berger, B., Muller, C., and Flugge, U.I. (2007b). The R2R3-
636
MYB transcription factor HAG1/MYB28 is a regulator of methionine-derived
637
glucosinolate biosynthesis in Arabidopsis thaliana. The Plant Journal 51:247-261.
638
Gou, J.Y., Felippes, F.F., Liu, C.J., Weigel, D., and Wang, J.W. (2011). Negative regulation of
639
anthocyanin biosynthesis in Arabidopsis by a miR156-targeted SPL transcription factor.
640
The Plant Cell 23:1512-1522.
642
Gu, W., and Roeder, R.G. (1997). Activation of p53 Sequence-Specific DNA Binding by Acetylation of the p53 C-Terminal Domain. Cell 90:595-606.
EP
641
TE D
635
Guo, L., Nezames, C.D., Sheng, L., Deng, X., and Wei, N. (2013). Cullin‐RING Ubiquitin
644
Ligase Family in Plant Abiotic Stress Pathways. Journal of Integrative Plant Biology
645 646 647
AC C
643
55:21-30.
Han, J., Zhang, H., Zhang, H., Wang, Z., Zhou, H., and Zhang, Z. (2013). A Cul4 E3 Ubiquitin Ligase Regulates Histone Hand-Off during Nucleosome Assembly. Cell 155:817-829.
648
Heine, G.F., Hernandez, J.M., and Grotewold, E. (2004). Two cysteines in plant R2R3 MYB
649
domains participate in REDOX-dependent DNA binding. Journal of Biological
650
Chemistry 279:37878-37885.
ACCEPTED MANUSCRIPT
Hirai, M.Y., Sugiyama, K., Sawada, Y., Tohge, T., Obayashi, T., Suzuki, A., Araki, R., Sakurai,
652
N., Suzuki, H., and Aoki, K. (2007). Omics-based identification of Arabidopsis Myb
653
transcription factors regulating aliphatic glucosinolate biosynthesis. Proc. Natl Acad. Sci.
654
USA 104:6478-6483.
RI PT
651
655
Hong, G.-J., Xue, X.-Y., Mao, Y.-B., Wang, L.-J., and Chen, X.-Y. (2012). Arabidopsis MYC2
656
Interacts with DELLA Proteins in Regulating Sesquiterpene Synthase Gene Expression.
657
The Plant Cell Online 24:2635-2648.
660 661
SC
659
Hou, X., Lee, L.Y.C., Xia, K., Yan, Y., and Yu, H. (2010). DELLAs Modulate Jasmonate Signaling via Competitive Binding to JAZs. Developmental Cell 19:884-894. Kaufmann, K., Smaczniak, C., de Vries, S., Angenent, G.C., and Karlova, R. (2011). Proteomics insights into plant signaling and development. Proteomics 11:744-755.
M AN U
658
662
Kazan, K., and Manners, J.M. (2013). MYC2: the master in action. Molecular Plant 6:686-703.
663
Kodadek, T., Sikder, D., and Nalley, K. (2006). Keeping Transcriptional Activators under
664
Control. Cell 127:261-264.
Lai, Z., Schluttenhofer, C.M., Bhide, K., Shreve, J., Thimmapuram, J., Lee, S.Y., Yun, D.-J., and
666
Mengiste, T. (2014). MED18 interaction with distinct transcription factors regulates
667
multiple plant functions. Nature Communications 5.
TE D
665
Lan, Z., Krosse, S., Achard, P., van Dam, N.M., and Bede, J.C. (2014). DELLA proteins
669
modulate Arabidopsis defences induced in response to caterpillar herbivory. Journal of
670
Experimental Botany 65:571-583.
672 673
Lee, C.M. (2014). Transport of c-MYC by Kinesin-1 for proteasomal degradation in the
AC C
671
EP
668
cytoplasm. Biochimica et Biophysica Acta (BBA) - Molecular Cell Research 1843:20272036.
674
Lee, O.R., Kim, S.J., Kim, H.J., Hong, J.K., Ryu, S.B., Lee, S.H., Ganguly, A., and Cho, H.-T.
675
(2010). Phospholipase A2 is required for PIN-FORMED protein trafficking to the plasma
676
membrane in the Arabidopsis root. The Plant Cell Online 22:1812-1825.
ACCEPTED MANUSCRIPT
677
Lindemose, S., O'Shea, C., Jensen, M.K., and Skriver, K. (2013). Structure, function and
678
networks of transcription factors involved in abiotic stress responses. International
679
Journal of Molecular Sciences 14:5842-5878. Lorenzo, O., Chico, J.M., Sánchez-Serrano, J.J., and Solano, R. (2004). JASMONATE-
681
INSENSITIVE1 encodes a MYC transcription factor essential to discriminate between
682
different jasmonate-regulated defense responses in Arabidopsis. The Plant Cell Online
683
16:1938-1950.
RI PT
680
Luo, J., Fishburn, J., Hahn, S., and Ranish, J. (2012). An integrated chemical cross-linking and
685
mass spectrometry approach to study protein complex architecture and function.
686
Molecular & Cellular Proteomics 11:M111. 008318.
688
Lüscher, B., and Vervoorts, J. (2012). Regulation of gene transcription by the oncoprotein MYC.
M AN U
687
SC
684
Gene 494:145-160.
Maier, A., Schrader, A., Kokkelink, L., Falke, C., Welter, B., Iniesto, E., Rubio, V., Uhrig, J.F.,
690
Hülskamp, M., and Hoecker, U. (2013). Light and the E3 ubiquitin ligase COP1/SPA
691
control the protein stability of the MYB transcription factors PAP1 and PAP2 involved in
692
anthocyanin accumulation in Arabidopsis. The Plant Journal 74:638-651.
TE D
689
Marino, D., Froidure, S., Canonne, J., Khaled, S.B., Khafif, M., Pouzet, C., Jauneau, A., Roby,
694
D., and Rivas, S. (2013). Arabidopsis ubiquitin ligase MIEL1 mediates degradation of the
695
transcription factor MYB30 weakening plant defence. Nature Communications 4:1476.
EP
693
Matsui, K., Umemura, Y., and Ohme‐Takagi, M. (2008). AtMYBL2, a protein with a single
697
MYB domain, acts as a negative regulator of anthocyanin biosynthesis in Arabidopsis.
698
The Plant Journal 55:954-967.
AC C
696
699
Micel, L.N., Tentler, J.J., Smith, P.G., and Eckhardt, G.S. (2013). Role of Ubiquitin Ligases and
700
the Proteasome in Oncogenesis: Novel Targets for Anticancer Therapies. Journal of
701
Clinical Oncology 31:1231-1238.
702
Miller, M.J., Scalf, M., Rytz, T.C., Hubler, S.L., Smith, L.M., and Vierstra, R.D. (2013).
703
Quantitative Proteomics Reveals Factors Regulating RNA Biology as Dynamic Targets
704
of Stress-induced SUMOylation in Arabidopsis. Molecular & Cellular Proteomics
705
12:449-463.
ACCEPTED MANUSCRIPT
706
Nakata, M. and Ohme-Takagi, M. (2013). Two bHLH-type transcription factors, JA-
707
ASSOCIATED MYC2-LIKE2 and JAM3, are transcriptional repressors and affect male
708
fertility. Plant Signaling and Behaviour 8:e26473. Nallamilli, B.R.R., Edelmann, M.J., Zhong, X., Tan, F., Mujahid, H., Zhang, J., Nanduri, B., and
710
Peng, Z. (2014). Global Analysis of Lysine Acetylation Suggests the Involvement of
711
Protein Acetylation in Diverse Biological Processes in Rice (Oryza sativa). PLoS ONE
712
9:e89283.
RI PT
709
Nemie-Feyissa, D., Olafsdottir, S.M., Heidari, B., and Lillo, C. (2014). Nitrogen depletion and
714
small R3-MYB transcription factors affecting anthocyanin accumulation in Arabidopsis
715
leaves. Phytochemistry 98:34-40.
SC
713
Ng, S., Ivanova, A., Duncan, O., Law, S.R., Van Aken, O., De Clercq, I., Wang, Y., Carrie, C.,
717
Xu, L., and Kmiec, B. (2013). A membrane-bound NAC transcription factor, ANAC017,
718
mediates mitochondrial retrograde signaling in Arabidopsis. The Plant Cell Online
719
25:3450-3471.
M AN U
716
Ni, W., Xu, S.-L., Tepperman, J.M., Stanley, D.J., Maltby, D.A., Gross, J.D., Burlingame, A.L.,
721
Wang, Z.-Y., and Quail, P.H. (2014). A mutually assured destruction mechanism
722
attenuates light signaling in Arabidopsis. Science 6:1160-1164.
TE D
720
Pauwels, L., Barbero, G.F., Geerinck, J., Tilleman, S., Grunewald, W., Perez, A.C., Chico, J.M.,
724
Bossche, R.V., Sewell, J., Gil, E., et al. (2010). NINJA connects the co-repressor
725
TOPLESS to jasmonate signalling. Nature 464:788-793.
EP
723
Pesch, M., Schultheiß, I., Digiuni, S., Uhrig, J.F., and Hülskamp, M. (2013). Mutual control of
727
intracellular localisation of the patterning proteins AtMYC1, GL1 and TRY/CPC in
728
AC C
726
Arabidopsis. Development 140:3456-3467.
729
Qi, T., Huang, H., Wu, D., Yan, J., Qi, Y., Song, S., and Xie, D. (2014). Arabidopsis DELLA
730
and JAZ Proteins Bind the WD-Repeat/bHLH/MYB Complex to Modulate Gibberellin
731 732 733
and Jasmonate Signaling Synergy. The Plant Cell 26:1118-1133. Raffaele, S., and Rivas, S. (2013). Regulate and be regulated: integration of defense and other signals by the AtMYB30 transcription factor. Frontiers in Plant Science 4:98.
ACCEPTED MANUSCRIPT
734 735
Ramsay, N.A., and Glover, B.J. (2005). MYB–bHLH–WD40 protein complex and the evolution of cellular diversity. Trends in Plant Science 10:63-70. Sahu, P., Pandey, G., Sharma, N., Puranik, S., Muthamilarasan, M., and Prasad, M. (2013).
737
Epigenetic mechanisms of plant stress responses and adaptation. Plant Cell Reports
738
32:1151-1159.
RI PT
736
Saijo, Y., Zhu, D., Li, J., Rubio, V., Zhou, Z., Shen, Y., Hoecker, U., Wang, H., and Deng, X.W.
740
(2008).Arabidopsis COP1/SPA1 complex and phytochrome A signaling intermediates
741
associate with distinct phosphorylated forms of phytochrome A in balancing signal
742
propagation and attenuation. Molecular Cell 31:607–613.
SC
739
Sasaki-Sekimoto, Y., Jikumaru, Y., Obayashi, T., Saito, H., Masuda, S., Kamiya, Y., Ohta, H.,
744
and Shirasu, K. (2013). Basic Helix-Loop-Helix transcription factors JASMONATE-
745
ASSOCIATED MYC2-LIKE1 (JAM1), JAM2, and JAM3 are negative regulators of
746
jasmonate responses in Arabidopsis. Plant Physiology 163:291-304.
M AN U
743
Schweizer, F., Bodenhausen, N., Lassueur, S., Masclaux, F.G., and Reymond, P. (2013).
748
Differential Contribution of Transcription Factors to Arabidopsis thaliana Defense
749
Against Spodoptera littoralis. Frontiers in Plant Science 4:13.
752 753 754 755 756 757 758 759 760
emphasis on intracellular movement. Journal of Integrative Plant Biology 56:334-342. Seo, P.J., and Mas, P. (2014). Multiple Layers of Posttranslational Regulation Refine Circadian
EP
751
Seo, P.J. (2014). Recent advances in plant membrane-bound transcription factor research:
Clock Activity in Arabidopsis. The Plant Cell Online 26: 79-87. Sonderby, I.E., Burow, M., Rowe, H.C., Kliebenstein, D.J., and Halkier, B.A. (2010). A complex
AC C
750
TE D
747
interplay of three R2R3 MYB transcription factors determines the profile of aliphatic glucosinolates in Arabidopsis. Plant Physiology 153:348-363.
Spitz, F., and Furlong, E.E. (2012). Transcription factors: from enhancer binding to developmental control. Nature Reviews. Genetics 13:613-626.
Spoel, S.H., and Loake, G.J. (2011). Redox-based protein modifications: the missing link in plant immune signalling. Current Opinion in Plant Biology 14:358-364.
ACCEPTED MANUSCRIPT
761 762
Stone, S.L. (2014). The role of ubiquitin and the 26S proteasome in plant abiotic stress signaling. Frontiers in Plant Science 5:135. Stracke, R., Ishihara, H., Huep, G., Barsch, A., Mehrtens, F., Niehaus, K., and Weisshaar, B.
764
(2007). Differential regulation of closely related R2R3-MYB transcription factors
765
controls flavonol accumulation in different parts of the Arabidopsis thaliana seedling.
766
The Plant Journal 50:660-677.
768
Stracke, R., Werber, M., and Weisshaar, B. (2001). The R2R3-MYB gene family in Arabidopsis thaliana. Current Opinion in Plant Biology 4:447-456.
SC
767
RI PT
763
Sun, X., Feng, P., Xu, X., Guo, H., Ma, J., Chi, W., Lin, R., Lu, C., and Zhang, L. (2011). A
770
chloroplast envelope-bound PHD transcription factor mediates chloroplast signals to the
771
nucleus. Nature Communications 2:477.
M AN U
769
772
Sønderby, I.E., Hansen, B.G., Bjarnholt, N., Ticconi, C., Halkier, B.A., and Kliebenstein, D.J.
773
(2007). A systems biology approach identifies a R2R3 MYB gene subfamily with distinct
774
and overlapping functions in regulation of aliphatic glucosinolates. PLoS ONE 2:e1322. Tavares, C.P., Vernal, J., Delena, R.A., Lamattina, L., Cassia, R., and Terenzi, H. (2014). S-
776
nitrosylation influences the structure and DNA binding activity of AtMYB30
777
transcription factor from Arabidopsis thaliana. Biochimica et Biophysica Acta (BBA)-
778
Proteins and Proteomics 1844:810-817.
781 782 783 784
EP
780
Toledo-Ortiz, G. (2003). The Arabidopsis Basic/Helix-Loop-Helix Transcription Factor Family. The Plant Cell Online 15:1749-1770. Vailleau, F., Daniel, X., Tronchet, M., Montillet, J.-L., Triantaphylidès, C., and Roby, D. (2002).
AC C
779
TE D
775
A R2R3-MYB gene, AtMYB30, acts as a positive regulator of the hypersensitive cell death program in plants in response to pathogen attack. Proc. Natl Acad. Sci. USA 99:10179-10184.
785
Wei, N., Kwok, S.F., von Arnim, A.G., Lee, A., McNellis, T.W., Piekos, B. and Deng, X.W.
786
(1994). Arabidopsis COP8, COP10, and COP11 genes are involved in repression of
787
photomorphogenic development in darkness. The Plant Cell 6: 629-643.
788
Wild, M., Daviere, J.M., Cheminant, S., Regnault, T., Baumberger, N., Heintz, D., Baltz, R.,
789
Genschik, P., and Achard, P. (2012). The Arabidopsis DELLA RGA-LIKE3 is a direct
ACCEPTED MANUSCRIPT
790
target of MYC2 and modulates jasmonate signaling responses. The Plant Cell 24:3307-
791
3319. Withers, J., Yao, J., Mecey, C., Howe, G.A., Melotto, M., and He, S.Y. (2012). Transcription
793
factor-dependent nuclear localization of a transcriptional repressor in jasmonate hormone
794
signaling. Proc. Natl Acad. Sci. 109:20148-20153.
RI PT
792
Wu, R.-C., Feng, Q., Lonard, D.M., and O'Malley, B.W. (2007). SRC-3 Coactivator Functional
796
Lifetime Is Regulated by a Phospho-Dependent Ubiquitin Time Clock. Cell 129:1125-
797
1140.
799
Xing, S., and Poirier, Y. (2012). The protein acetylome and the regulation of metabolism. Trends in Plant Science 17:423-430.
M AN U
798
SC
795
800
Xu, W., Grain, D., Le Gourrierec, J., Harscoët, E., Berger, A., Jauvion, V., Scagnelli, A., Berger,
801
N., Bidzinski, P., Kelemen, Z., et al. (2013). Regulation of flavonoid biosynthesis
802
involves an unexpected complex transcriptional regulation of TT8 expression in
803
Arabidopsis. New Phytologist 198:59-70.
Yan, J., Li, H., Li, S., Yao, R., Deng, H., Xie, Q., and Xie, D. (2013). The Arabidopsis F-box
805
protein CORONATINE INSENSITIVE1 is stabilized by SCFCOI1 and degraded via the
806
26S proteasome pathway. The Plant Cell 25:486-498.
TE D
804
Yang, Y., Ou, B., Zhang, J., Si, W., Gu, H., Qin, G., and Qu, L.J. (2014a). Arabidopsis Mediator
808
subunit MED16 regulates iron homeostasis by associating with EIN3/EIL1 through
809
subunit MED25. The Plant Journal 77:838-851.
811 812 813 814
Yang, Z.T., Wang, M.J., Sun, L., Lu, S.J., Bi, D.L., Sun, L., Song, Z.T., Zhang, S.S., Zhou, S.F.,
AC C
810
EP
807
and Liu, J.X. (2014b). The membrane-associated transcription factor NAC089 controls ER-stress-induced programmed cell death in plants. PLoS Genetics 10:e1004243.
Zentner, G.E., and Henikoff, S. (2012). Surveying the epigenomic landscape, one base at a time. Genome Biology 13:1186.
815
Zhai, Q., Yan, L., Tan, D., Chen, R., Sun, J., Gao, L., Dong, M.Q., Wang, Y., and Li, C. (2013).
816
Phosphorylation-coupled proteolysis of the transcription factor MYC2 is important for
817
jasmonate-signaled plant immunity. PLoS Genetics 9:e1003422.
ACCEPTED MANUSCRIPT
818
Zhao, L., Gao, L., Wang, H., Chen, X., Wang, Y., Yang, H., Wei, C., Wan, X., and Xia, T.
819
(2013). The R2R3-MYB, bHLH, WD40, and related transcription factors in flavonoid
820
biosynthesis. Functional & Integrative Genomics 13:75-98. Zheng, Y., Schumaker, K.S., and Guo, Y. (2012). Sumoylation of transcription factor MYB30 by
822
the small ubiquitin-like modifier E3 ligase SIZ1 mediates abscisic acid response in
823
Arabidopsis thaliana. Proc. Natl Acad. Sci. 109:12822-12827.
825
Zhou, H., Watts, J.D., and Aebersold, R. (2001). A systematic approach to the analysis of protein phosphorylation. Nature Biotechnology 19:375-378.
SC
824
RI PT
821
Zimmermann, I.M., Heim, M.A., Weisshaar, B., and Uhrig, J.F. (2004). Comprehensive
827
identification of Arabidopsis thaliana MYB transcription factors interacting with R/B‐
828
like BHLH proteins. The Plant Journal 40:22-34.
M AN U
826
AC C
EP
TE D
829
ACCEPTED MANUSCRIPT
830
Figure legends
831 Figure 1: Schematic representation of MYB and BHLH TFs. A) R2R3 MYB TFs have a
833
conserved DNA-Binding Domain (DBD) at the N-terminal of the protein and a more variable,
834
C-terminal Trans-Activation Domain (TAD). B) bHLH TFs of the MYC clade are characterized
835
by a bHLH domain containing the DNA binding motif (G-Box), a dimerization domain (DD)
836
and a Nuclear Localisation Signal (NLS) at the C-terminus. The JAZ Interaction Domain (JID) is
837
found in the N-terminal TAD.
SC
RI PT
832
M AN U
838
Figure 2: Signal integration by the hub TF MYC2. MYC2 has the ability to integrate multiple
840
environmental and developmental signals and to control the expression levels of various
841
pathways precisely in space and time. I: Constitutive expression levels and activation of MYC2
842
are balanced by different PTMs. II: Upon herbivore or JA treatment, MYC2 inhibition by JAZs
843
is released leading to an accumulation of active MYC2. III: Depending on the developmental
844
stage, DELLAs interact with MYC2 to inhibit its JA-dependent transcriptional activity. GA will
845
lead to MYC2 activation to trigger GA-mediated developmental processes. IV: Active MYC2
846
can bind different promoters and initiate specific responses. Squares represent MYC2 in an
847
inactive form, while circles depict active proteins. Roman numbers refer to different regulatory
848
layers described in the text. JA, jasmonic acid; GA, giberillic acid; PTM, post-transcriptional
849
modification.
EP
AC C
850
TE D
839
851
Figure 3: Combinatorial effects of PTMs and PPIs on MYB30 activity. MYB30 represents
852
an example of a TF that is regulated by multiple mechanisms on the protein level. Different
853
signals are integrated on this level to ensure tight regulation of a single output, i.e. cell death. I:
854
Basal levels of transcript lead to accumulation of MYB30 protein balanced between an active
855
and inactive state by different PTMs. Upon stimulation by hormones, transcript levels incease
856
and the balance shifts towards more active protein. II: when activated, the MYB30 binds specific
857
promoters and thereby induces cell death-specific genes. III: Cell death is tightly balanced by
ACCEPTED MANUSCRIPT
modifying enzymes which will inactivate the protein to ensure locally restrict cell death. Inactive
859
MYB30 is shown as square, the active form as circle. Roman numbers refer to different
860
regulatory layers that are described in the text. BRs, Brassinosteroids; SA, salicylic acid; ABA,
861
abscisic acid; PTM, post-transcriptional modification.
AC C
EP
TE D
M AN U
SC
RI PT
858
AC C
EP
TE D
M AN U
SC
RI PT
ACCEPTED MANUSCRIPT
AC C
EP
TE D
M AN U
SC
RI PT
ACCEPTED MANUSCRIPT
AC C
EP
TE D
M AN U
SC
RI PT
ACCEPTED MANUSCRIPT