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Target Concepts:
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Query: EC:3.4.25.1 (
proteasome
)
28,817
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
The DELLA proteins GAI, RGA, RGL1 and
RGL2
in Arabidopsis are plant growth repressors, repressing diverse developmental processes. Studies have shown that gibberellin (GA) attenuates the repressive function of DELLA proteins by triggering their degradation via the
proteasome
pathway. However, it is not known if GA-induced protein degradation is the only pathway for regulating the bioactivity of DELLA proteins. We show here that tobacco BY2 cells represent a suitable system for studying GA signaling.
RGL2
exists in a phosphorylated form in BY2 cells.
RGL2
undergoes GA-induced degradation, and this process is blocked by
proteasome
inhibitors and serine/threonine phosphatase inhibitors; however, serine/threonine kinase inhibitors had no detectable effect, suggesting that dephosphorylation of serine/threonine is probably a prerequisite for degradation of
RGL2
via the
proteasome
pathway. Site-directed substitution of all 17 conserved serine and threonine residues showed that six mutants (
RGL2
(S441D,
RGL2
(S542D),
RGL2
(T271E),
RGL2
(T319E),
RGL2
(T411E) and
RGL2
(T535E)) mimicking the status of constitutive phosphorylation are resistant to GA-induced degradation. This suggests that these sites are potential phosphorylation sites. A functional assay based on the expression of GA 20-oxidase revealed that
RGL2
(T271E) is probably a null mutant,
RGL2
(S441D),
RGL2
(S542D),
RGL2
(T319E) and
RGL2
(T411E) only retained about 4-17% of the activity of the wild type
RGL2
, whereas
RGL2
(T535E) retained about 66% of the activity of the wild type
RGL2
. However, expression of GA 20-oxidase in BY2 cells expressing these mutant proteins is still responsive to GA, suggesting that the stabilization of RGL2 protein is not the only pathway for regulating its bioactivity.
...
PMID:Identification of the conserved serine/threonine residues important for gibberellin-sensitivity of Arabidopsis RGL2 protein. 1616 98
Seed germination is antagonistically controlled by the phytohormones gibberellic acid (GA) and abscisic acid (ABA). GA promotes seed germination by enhancing the
proteasome
-mediated destruction of
RGL2
(for RGA-LIKE2), a key DELLA factor repressing germination. By contrast, ABA blocks germination by inducing ABI5 (for ABA-INSENSITIVE5), a basic domain/leucine zipper transcription factor repressing germination. Decreased GA synthesis leads to an increase in endogenous ABA levels through a stabilized
RGL2
, a process that may involve XERICO, a RING-H2 zinc finger factor promoting ABA synthesis. In turn, increased endogenous ABA synthesis is necessary to elevate not only ABI5 RNA and protein levels but also, critically, those of
RGL2
. Increased ABI5 protein is ultimately responsible for preventing seed germination when GA levels are reduced. However, overexpression of ABI5 was not sufficient to repress germination, as ABI5 activity requires phosphorylation. The endogenous ABI5 phosphorylation and inhibition of germination could be recapitulated by the addition of a SnRK2 protein kinase to the ABI5 overexpression line. In sleepy1 mutant seeds,
RGL2
overaccumulates; germination of these seeds can occur under conditions that produce low ABI5 expression. These data support the notion that ABI5 acts as the final common repressor of germination in response to changes in ABA and GA levels.
...
PMID:The gibberellic acid signaling repressor RGL2 inhibits Arabidopsis seed germination by stimulating abscisic acid synthesis and ABI5 activity. 1970 11
Under the canopy, far-red (FR) light represses seed germination by inactivating phytochrome photoreceptors. This elicits a decrease in gibberellins (GA) levels and an increase in abscisic acid (ABA) levels. GA promotes germination by enhancing the
proteasome
-mediated destruction of DELLA repressors. ABA prevents germination by stimulating the expression of ABI repressors. How phytochromes elicit changes in hormone levels or how GA- and ABA-dependent signals are coordinated to repress germination remains poorly understood. We show that repression of germination by FR light involves stabilized DELLA factors GAI, RGA and
RGL2
that stimulate endogenous ABA synthesis. In turn, ABA blocks germination through the transcription factor ABI3. The role of PIL5, a basic helix-loop-helix transcription factor stimulating GAI and RGA expression, is significant, provided GA synthesis is high enough; otherwise, high GAI and RGA protein levels persist to block germination. Under white light, GAI and RGA driven by the
RGL2
promoter can substitute for
RGL2
to promote ABA synthesis and repress germination, consistent with the recent findings with
RGL2
. The three DELLA factors inhibit testa rupture whereas ABI3 blocks endosperm rupture.
...
PMID:Far-red light inhibits germination through DELLA-dependent stimulation of ABA synthesis and ABI3 activity. 1955 68
Dormancy prevents seeds from germinating under favorable conditions until they have experienced dormancy-breaking conditions, such as after-ripening through a period of dry storage or cold imbibition. Abscisic acid (ABA) hormone signaling establishes and maintains seed dormancy, whereas gibberellin (GA) signaling stimulates germination. ABA levels decrease and GA levels increase with after-ripening and cold stratification. However, increasing GA sensitivity may also be critical to dormancy loss since increasing seed GA levels are detectable only with long periods of after-ripening and imbibition. After-ripening and cold stratification act additively to enhance GA hormone sensitivity in ga1-3 seeds that cannot synthesize GA. Since the overexpression of the GA receptor GID1 (GIBBERELLIN-INSENSITIVE DWARF1) enhanced this dormancy loss, and because gid1a gid1b gid1c triple mutants show decreased germination, the effects of dormancy-breaking treatments on GID1 mRNA and protein accumulation were examined. Partial after-ripening resulted in increased GID1b, but not GID1a or GID1c mRNA levels. Cold imbibition stimulated the accumulation of all three GID1 transcripts, but resulted in no increase in GA sensitivity during ga1-3 seed germination unless seeds were also partially after-ripened. This is probably because after-ripening was needed to enhance GID1 protein accumulation, independently of transcript abundance. The rise in GID1b transcript with after-ripening was not associated with decreased ABA levels, suggesting there is ABA-independent GID1b regulation by after-ripening and the 26S
proteasome
. GA and the DELLA
RGL2
repressor of GA responses differentially regulated the three GID1 transcripts. Moreover, DELLA
RGL2
appeared to switch between positive and negative regulation of GID1 expression in response to dormancy-breaking treatments.
...
PMID:Loss of Arabidopsis thaliana Seed Dormancy is Associated with Increased Accumulation of the GID1 GA Hormone Receptors. 2613 98
Bud dormancy release is regulated by gibberellins (GAs). DELLA proteins are highly conserved and act as negative regulators in GA signaling pathway. The present study established a relationship between
PmRGL2
in Japanese apricot and GA
4
levels during dormancy release of floral buds. Overexpression of
PmRGL2
in poplar delayed the onset of bud dormancy and resulted in dwarf plants, relative to wild-type trees.
PmRGL2
exhibited higher expression during ecodormancy and relatively lower expression during endodormancy. The relative level of GA
4
exhibited an increasing trend at the transition from endodormancy to ecodormancy and displayed a similar expression pattern of genes related to GA metabolism,
PmGA20ox2
,
PmGA3ox1, PmGID1b
, in both Japanese apricot and transgenic poplar. These results suggests that
PmRGL2
acts as an integrator and negative regulator of dormancy via a GA-signaling pathway. Moreover, an interaction between
RGL2
and SLY1 in a yeast two hybrid (Y2H) system further suggests that SCF E3 ubiquitin ligases, such as
SLY1
, may be a critical factor in the regulation of
RGL2
through an SCF
SLY1
-
proteasome
pathway. Our study demonstrated that
PmRGL2
plays a negative role in bud dormancy release by regulating the GA biosynthetic enzymes,
GA20ox
and
GA3ox1
and the GA receptor,
GID1b
.
...
PMID:Isolation and Role of
PmRGL2
in GA-mediated Floral Bud Dormancy Release in Japanese Apricot (
Prunus mume
Siebold et Zucc.). 2943 10
