Ecdysone receptor
The ecdysone response
hierarchy mediates egg chamber maturation during
mid-oogenesis. E75, E74 and BR-C are expressed in a stage-specific
manner while EcR expression is ubiquitous
throughout oogenesis. Decreasing or increasing the ovarian
ecdysone titer using a temperature-sensitive mutation or
exogenous ecdysone results in corresponding changes in
early gene expression. The stage 10 follicle cell expression
of E75 in wild-type, K10 and EGF receptor (Egfr) mutant
egg chambers reveals regulation of E75 by both the Egfr
and ecdysone signaling pathways. Genetic analysis
indicates a germline requirement for ecdysone-responsive
gene expression. Germline clones of E75 mutations arrest
and degenerate during mid-oogenesis and EcR germline
clones exhibit a similar phenotype, demonstrating a
functional requirement for ecdysone responsiveness during
the vitellogenic phase of oogenesis. Finally, the expression
of Drosophila Adrenodoxin Reductase increases during
mid-oogenesis and clonal analysis confirms that this
steroidogenic enzyme is required in the germline for egg
chamber development. Together these data suggest that the
temporal expression profile of E75, E74 and BR-C may be
a functional reflection of ecdysone levels and that ecdysone
provides temporal signals regulating the progression of
oogenesis and proper specification of dorsal follicle cell
fates (Buszczak, 1999).
In order to investigate the role of ecdysone-responsive
gene expression in the ovary,
expression of three classical early ecdysone-responsive
genes, E75, E74 and BR-C were examined. In situ hybridization
revealed that the E75 and E74 genes are transcribed
in remarkably similar patterns during oogenesis. Both
E75 and E74 transcripts are first detected in region 2b
of the germarium. Expression decreases
during stages 2-4 and low levels of E75 and E74 mRNA
are again detected in stage 5-7 egg chambers.
Transcription of E75 and E74 appears to be
upregulated during stage 8 in both the germline and
soma. This expression continues to increase until stage
10B when transcription of both genes peaks in the
follicle cells and the nurse cells.
Immunofluorescent staining reveals the
presence of BR-C protein in the follicle cell nuclei
beginning between stages 5 and 6 of oogenesis. In most of the egg chambers examined, BR-C
appears to be completely absent from the germline.
However, in rare cases, low levels of expression could
be detected in the nurse cell nuclei. These observations
are consistent with a recent report that describes follicle
cell expression of BR-C mRNA (Buszczak, 1999).
The expression of E75, E74 and BR-C in egg
chambers suggests that these genes are co-regulated by a
common signal. If these early response genes are
being regulated by ecdysone, one would expect a
dependence on the ecdysone receptor. To determine whether
the ecdysone receptor is present in the ovary, egg chambers
from Canton-S females were stained using anti-EcR
antibodies. Antibody staining reveals that germline and
somatic cells express EcR protein in their nuclei.
This expression is first detected in the germarium, appears
to be slightly upregulated during stage 4 and persists until the
late stages of oogenesis. Additionally, border cells strongly
express EcR during their migration through the nurse cell
cluster. Uso has also been detected in all cells
within the ovary. Thus, both
components of the functional ecdysone receptor are present in
the germline and soma during all stages of oogenesis (Buszczak, 1999).
To test the dependence of early response gene expression on
ecdysone, a study was made of the effects in ovaries of the ecdysoneless1 (l(3)ecd1)
mutation, in which low levels of ecdysone are generated. Females homozygous for the temperature-sensitive
mutation l(3)ecd1 lose the ability
to lay eggs after just 2 days at the restrictive temperature and to
have 13% of the wild-type ovarian ecdysone titer when shifted
to the restrictive temperature for 4 days. E75
transcript levels were compared in wild-type and l(3)ecd1
females shifted to the restrictive temperature for different lengths
of time. Using in situ hybridization, no difference in E75 mRNA
levels could be detected between ovaries taken from wild-type
and l(3)ecd1 females maintained at 25ƒC.
However, there is a reproducible reduction of E75 mRNA in
l(3)ecd1 ovaries relative to wild-type controls shifted to the
restrictive temperature for 2 days. An RNAse
protection assay was used to quantitate the difference in E75
transcription in l(3)ecd1 and wild-type ovaries. This analysis
reveals that l(3)ecd1 ovaries contain approximately half the
E75 mRNA of wild-type ovaries when subjected to restrictive
conditions. BR-C expression in wild-type and l(3)ecd1
ovaries was also assayed. Immunofluorescent staining showed
that BR-C protein levels appear to be reduced in l(3)ecd1
ovaries relative to wild-type controls. A reduction of
BR-C expression in ovaries from mutants shifted to 29ƒC was
also detected on Western blots (Buszczak, 1999).
The presence of EcR protein and the
presence of USP in ovarian cells of all stages suggests that
these cells are competent to respond to ecdysone. A test was performed to see whether an increase in the
ecdysone titer could induce E75 expression in the ovary.
Ovaries were cultured in the presence or absence of 20-hydroxyecdysone. In situ hybridization shows that E75
transcription increases in early egg chambers in response to
ecdysone and that the increase of expression occurs in both
the follicle cells and germline. An RNAse
protection assay was used to quantitate the induction of E75
transcription by exogenous ecdysone. This analysis has
demonstrated that increasing amounts of ecdysone in the
culture media leads to increased expression of E75 (Buszczak, 1999).
During stage 10, the follicle cell expression of E75 becomes
enriched in the dorsal anterior cells. This suggested
that inputs in addition to ecdysone are needed to refine E75
expression. Previous work has shown that follicle cell polarity
is established during mid- to late-oogenesis and depends on the
interaction between Gurken and the Drosophila
homolog of the mammalian EGF receptor (Egfr). To determine whether E75 expression is
under control of the dorsoventral signaling pathway, ovarian E75 mRNA distribution was examined in dorsalized and
ventralized mutant backgrounds. In fs(1)K10 mutants,
mislocalization of Grk protein results in activation of Egfr
in all anterior follicle cells surrounding the oocyte. In
fs(1)K10 mutant egg chambers, E75 expression expands to a
ring of anterior follicle cells surrounding the oocyte.
Mutations in Egfr prevent signal transduction by the receptor
and lead to the ventralization of the eggshell and embryo. In situ analysis indicates that stage 10
follicle cells overlying the oocyte in Egfr mutants no longer
express E75. However, E75 expression in the nurse
cells is unaffected. These experiments show that
the Egfr signaling pathway regulates E75 expression in the
dorsal follicle cells but not in the germline (Buszczak, 1999).
To investigate the functional role of E75 in the germline, germline clones of a strong E75 allele were generated using the
FLP/FRT system of mitotic recombination and the ovoD1
dominant female sterile transgene. While heterozygotes carrying a control
chromosome over ovoD1 laid eggs following clone induction,
females carrying the E75 e213 mutation in trans to the ovo D1
chromosome did not lay eggs after clone induction. Upon
dissection, E75 e213 germline clones appear to arrest and
degenerate at stages 8-9. Some yolk can be seen
in the oocyte but the follicle cells rarely complete their migration to the oocyte. While the germline in these clonal egg chambers
degenerates, the follicle cell layer remains remarkably intact. Oocytes in E75 e213 germline clones are small and
sometimes displaced to one side of the posterior end of the egg
chamber. The frequency of the observed phenotypes
strongly suggests that E75 function is required in the
germline to progress beyond early vitellogenesis.
If E75 expression depends upon ecdysone response, similar
phenotypes should result from ecdysone receptor mutations. To
test whether EcR is required for the completion of oogenesis,
germline clones of the EcR null mutation, EcR M554fs, were analyzed. A small number of females
laid eggs 2-4 days after eclosion. Although few in number (2-
3/female/day), these eggs appear to be normal in shape and
size. However, egg laying ceases after 4-5 days. Upon
dissection, ovaries from several females (15/202) appear to
have clonal egg chambers many of which are arrested at stage
6 or 7. These egg chambers are easily distinguished from
non-clonal ovo D1 egg chambers by the lack of EcR antibody
staining in nurse cell nuclei. Therefore, it appears as though EcR is required for egg
chamber progression beyond mid-oogenesis (Buszczak, 1999).
In order to address more directly the timing and autonomy of
steroid hormone signaling in the Drosophila ovary, the expression pattern and germline requirements for
the recently described dare gene were analyzed (Freeman, 1999). dare
encodes the Drosophila homolog of adrenodoxin reductase,
an enzyme required for the synthesis of steroid hormones in
vertebrates. Biochemical studies from insects,
and genetic analysis of the dare locus in Drosophila, strongly
suggest that insect steroid hormone production is also critically
dependent upon adrenodoxin reductase, and null alleles of dare
appear to effectively block the synthesis of ecdysteroids
(Freeman, 1999).
In situ hybridization reveals that low levels of Dare mRNA
can be detected in the germline beginning at stage 6 of
oogenesis. Expression of dare remains relatively low
until stage 10 when egg chambers exhibit a dramatic increase
of dare transcription.
To further assess the requirements for dare during oogenesis,
germline clones using the dare 34 allele (Freeman, 1999)
were induced. While all of the control females
laid eggs, very few females with presumptive
dare 34 clones lay eggs, and these females lose the ability to lay
eggs after 1-2 days. These findings indicate that dare
has a critical germline function, and are consistent with the
possibility that dare clones arrest at a point similar to that seen
for other components of the ecdysone response pathway.
Interestingly, significant dare expression is not seen in the
germarium; while lower levels of dare could potentially be
sufficient to allow some ecdysone synthesis, this raises the
possibility that signals other than ecdysone could contribute to
germarial expression of early response genes (Buszczak, 1999).
In other insects, including the mosquito Aedes aegypti, the
transition from the previtellogenic to the vitellogenic state is
governed by ecdysone-regulated hierarchies. Aedes
egg chambers develop synchronously and remain arrested in a
previtellogenic state until the female takes a blood meal. This
triggers production of the ecdysiotropic neuoropeptide
(EDNH) that stimulates ovarian synthesis of ecdysone. The
resulting increase in the ecdysone titer leads to the expression
of E75 and controls induction and progression of vitellogenesis
and further egg development (Pierceall, 1999). In a similar fashion,
ecdysone could be regulating egg chamber progression
past stage 8 in Drosophila. Thus, the stage-specific
expression of ecdysone response hierarchies and their
control over egg chamber development may represent an
evolutionarily conserved mechanism for coordinating the
developmental processes that occur during insect oogenesis.
While the synchronous development of a cohort of eggs
under endocrine control, as seen in the mosquito, would not be
unexpected, the asynchronous progression of Drosophila
oogenesis under similar hormonal control raises an interesting
and important question. How can a presumed endocrine factor,
such as ecdysone, regulate the sequential, asynchronous
induction of these genetic regulatory programs during
Drosophila oogenesis? Stage specificity of ecdysone-responsive
gene expression could, in principle, be controlled
either at the level of competence to respond to ecdysone or at
the level of the production or availability of the hormone itself.
The results presented here suggest the latter possibility. While analysis of EcR
germline clones indicates that the receptor is required during
mid-oogenesis, the ecdysone receptor is present throughout
oogenesis. The expression of the ecdysone response genes BR-C,
E74 and E75, in contrast, is stage-specific, and varies in
conjunction with experimental manipulation of hormone titer.
These findings suggest that individual egg chambers are
exposed to different amounts of hormone as they progress
through oogenesis (Buszczak, 1999).
Drosophila metamorphosis is characterized by diverse
developmental phenomena, including cellular proliferation, tissue
remodeling, cell migration, and programmed cell death. Cells undergo
one or more of these processes in response to the hormone
20-hydroxyecdysone (ecdysone), which initiates metamorphosis at the end
of the third larval instar and before puparium formation (PF) via a
transcriptional hierarchy.
Additional pulses of ecdysone further coordinate these processes during
the prepupal and pupal phases of metamorphosis. Larval tissues such as
the gut, salivary glands, and larval-specific muscles undergo
programmed cell death and subsequent histolysis. The imaginal discs
undergo physical restructuring and differentiation to form rudimentary
adult appendages such as wings, legs, eyes, and antennae. Ecdysone also
triggers neuronal remodeling in the central nervous system (White, 1999).
Wild-type patterns of gene expression in
D. melanogaster during early metamorphosis were examined by assaying whole
animals at stages that span two pulses of ecdysone. Microarrays were constructed containing
6240 elements that included more than 4500 unique cDNA expressed
sequence tag (EST) clones along with a number of
ecdysone-regulated control genes having predictable expression
patterns. These ESTs represent
approximately 30% to 40% of the total estimated number of genes in the
Drosophila genome. In order to gauge
expression levels, microarrays were hybridized with fluorescent probes
derived from polyA+ RNA isolated from developmentally
staged animals. The time points examined are relative to PF, which
last approximately 15 to 30 min, during which time the larvae cease to move
and evert their anterior spiracles. Nineteen arrays were examined representing
six time points relative to PF: one time point before the late larval
ecdysone pulse; one time
point just after the initiation of this pulse (4 hours BPF), and time
points at 3, 6, 9, and 12 hours after PF (APF). The prepupal pulse of
ecdysone occurs 9 to 12 hours APF (White, 1999).
In order to manage, analyze, and disseminate the large amount of data,
a searchable database was constructed that includes
the average expression differential at each time point. The analysis
set consists of all elements that reproducibly fluctuate in
expression threefold or more at any time point relative to PF, leaving
534 elements containing sequences represented by 465 ESTs and control
genes. More than 10% of the genes represented by the
ESTs display threefold or more differential expression during early
metamorphosis. This may be a conservative estimate of the percentage of
Drosophila genes that change in expression level during
early metamorphosis, because of the stringent criteria used for their
selection (White, 1999).
To interpret these data, genes were grouped according to similarity of
expression patterns by two methods. The first relied on pairwise
correlation statistics, and the second relied on the use
of self-organizing maps (SOMs). Differentially expressed genes fall into two main categories. The first
category contains genes that are expressed at >18 hours BFP (before
the late larval ecdysone pulse) but then fall to low or undetectable
levels during this pulse. These genes are potentially repressed by ecdysone and
make up 44% of the 465 ESTs identified in this set. The second
category consists of genes expressed at low or undetectable levels
before the late larval ecdysone pulse but then are induced during this pulse. These genes are
potentially induced by ecdysone and make up 31% of the 465 ESTs.
Consequently, 75% of genes that changed in expression by threefold or
more do so during the late larval ecdysone pulse that marks the
initial transition from larva to prepupa. This result is consistent
with the extreme morphological changes that are about to occur in these
animals. There are clearly discrete subdivisions of gene expression within these
categories (White, 1999).
Relatively little is known about basic metabolic processes during
metamorphosis. Most work has focused on the alcohol dehydrogenase gene,
which is known to be repressed by ecdysone, but a few studies have included the ecdysone-inducible glucose dehydrogenase gene and the ecdysone-repressible urate oxidase locus. All three of these genes behave as expected. Nine genes
encoding enzymes in the glycolytic pathway are present on the array and
are down-regulated during the late larval ecdysone pulse. Also, there are reduced expression levels of genes
encoding enzymatic constituents of the citric acid cycle, oxidative
phosphorylation, amino acid metabolism, fatty acid
oxidation and synthesis, glycogen synthesis and breakdown, and the
pentose phosphate pathway. Thus, some tissues must be responding to the initiation of
metamorphosis by tempering their metabolic activity. This reduction may
represent an early response in certain tissues that are destined to
undergo programmed cell death, or it may reflect a global response to the transition from an active larva to a sessile prepupa (White, 1999).
Gene expression changes during metamorphosis also foreshadow both
larval muscle breakdown and adult myogenesis. At approximately 2 hours
APF, the anterior larval musculature begins to break down. This breakdown lasts until approximately 6 hours APF. Genes encoding both structural and regulatory components of muscle formation are down-regulated as early as 4 hours BPF (see Muscle-specific genes regulated during metamorphosis). In
addition to the repression of genes encoding components of thin and
thick filaments, genes encoding other muscle-specific molecules are
also repressed, including factors that compose the mesh in which these
filaments lie and regulatory factors involved in the specification of
muscle tissue. The mRNAs of all these repressed genes
decrease substantially many hours before histolysis of the anterior
larval muscles and therefore predict the occurrence of this
morphological event well before it begins. Twenty-four hours APF, adult myogenesis is well underway. The genes DMef-2, bagpipe, and tinman are all up-regulated at 12 hours APF from the baseline at PF, coincident with the prepupal pulse
of ecdysone. It is suggested that induction of these regulatory factors
initiates the development of the adult musculature, which will establish
itself several hours later (White, 1999).
In contrast to the histolyzing larval muscles, the CNS undergoes
dramatic differentiation and restructuring during early metamorphosis. The majority of the CNS is composed of adult-specific neurons that
reorganize at this time by extending processes and establishing new
connections. Several genes known to be involved in
neuronal-specific processes are differentially regulated during the
late larval ecdysone pulse (see Developmental control genes induced during metamorphosis.) For example, the Drosophila
neurotactin and plexin A genes are induced.
These genes are involved in axonal pathfinding and in establishing
synaptic connections. The neurotactin (nrt) gene
product is involved in growth cone guidance and is localized to the
cell surface at points of interneuronal cell contact in the presumptive
imaginal neurons within the larval CNS. Nerve
cord condensation does not occur normally in the late third instar CNS
of nrt mutant animals. In prepupae, nrt is
expressed in a tissue- and cell type-specific manner: it is restricted
to a small set of ocellar pioneer neurons in the brain, photoreceptors
of the eye, and some sensory neurons in the developing wing. It is suggested that nrt, like the
control genes induced from >18 hours BPF to PF, is regulated by the
late larval ecdysone pulse. The plexin A gene belongs to a
family of genes that encode Ca2+-dependent homophilic cell
adhesion molecules first identified in the vertebrate CNS and PNS. Drosophila Plexin A also acts as a
receptor for class I semaphorins, and both loss of function and
overexpression experiments demonstrate that Plexin A is involved in
axon guidance and repulsion of adjacent neurons (defasciculation). Many neurons defasciculate in response
to ecdysone during nervous system remodeling, and it is
suggested that an increase in plexin A expression may be partly responsible for this response. Several more differentially expressed neuronal-specific molecules are shown at The Drosophila Microarray Project. These genes provide several new candidates for
factors that are involved in the neuronal outgrowth and morphological
remodeling responses to ecdysone (White, 1999).
Larval-specific tissues such as the aforementioned larval muscles, the
midgut, and the salivary glands undergo programmed cell death during
metamorphosis. Genes involved in programmed cell death were identified
in these experiments. The apoptosis-activating reaper gene
has previously been shown to be ecdysone-inducible, and
this is reflected in the data. Expression of the
Drosophila caspase-1 gene is also observed during the prepupal ecdysone pulse
but not during the late larval pulse. This gene is also an
activator of apoptosis, and mutants display melanotic tumors and larval
lethality. Induction of a cell death inhibitor
gene, thread (also known as Diap1), is
observed during the late larval pulse but not the prepupal phase. The DIAP1 protein includes inhibitor-of-apoptosis (IAP) domains
and has been identified as a factor that can block reaper activity. Because different tissues begin apoptosis at
different stages of development, changes in the expression of
inhibitors and activators of apoptosis are expected to be tissue-specific. For
example, the expression profiles observed for the
caspase-1 activator and the Diap1 inhibitor are
those expected in tissues such as the larval salivary glands.
Tissue-specific information on the induction of these genes will be
important to an understanding of the coordination of apoptosis during
metamorphosis (White, 1999).
The expression levels of genes involved in cellular
differentiation also dynamically change during metamorphosis. The
gene headcase is expressed in all proliferating imaginal
cell lineages. This gene is
induced during the prepupal ecdysone pulse but does not substantially change expression levels during the late larval ecdysone pulse. Imaginal tissues in headcase null mutants appear normal in
size and shape but fail to differentiate normally. These mutants are invariably pupal lethal and show pleiotropic effects
in adult tissues. The predominant headcase loss of function phenotype is defective head development. Mutants can display deletion of the head capsule, leaving only a protruding proboscis. Another gene
expressed in this manner with a known role in ecdysone-mediated differentiation of imaginal discs is IMP-L2, an essential secreted immunoglobulin family member implicated in neural and ectodermal development in Drosophila.
These data demonstrate that factors required for cellular
differentiation during metamorphosis are present in the data set. There
are 29 other EST sequences encoding novel genes that display a greater than threefold induction from PF to 12 hours APF but do not display a
threefold or greater change in expression level during the late larval
ecdysone pulse. Perhaps some of these genes, such as
headcase and IMP-L2, are involved in
differentiation of adult-specific tissues (White, 1999).
Other genes known to be involved in cellular differentiation exhibit
changes in level of expression during metamorphosis. For example,
corkscrew is induced during the late larval ecdysone pulse. This gene encodes a protein tyrosine phosphatase that is
involved in receptor tyrosine kinase signaling during
photoreceptor differentiation.
shortsighted encodes a bZIP transcription factor
homologous to a mouse TGF-beta-responsive gene and acts in the decapentaplegic pathway. This gene is induced during the late larval ecdysone pulse and then further induced during the prepupal pulse. tolkin encodes a TGF-beta homolog and is induced
during the late larval ecdysone pulse but not during the prepupal pulse. tolkin is expressed in imaginal discs during
metamorphosis and causes pupal lethality when mutated. These results establish potential
connections between known signal transduction pathways and
ecdysone-initiated metamorphosis (White, 1999).
Description of wild-type development is a first step in understanding
metamorphosis from a global perspective. However, it is of interest to
understand the composition of the genetic hierarchy that leads to
metamorphosis. To test whether new targets of
transcription factors could be identified in the ecdysone genetic hierarchy, the ecdysone-induced nuclear receptor DHR3 was
prematurely expressed at >18 hours BPF. DHR3 is responsible for the coordination of part of the
transcriptional program controlling metamorphosis and can act as either
a repressor or an activator of transcription, depending on the target
gene. DHR3 can induce betaFTZ-F1, a nuclear receptor
that is active during midprepupal development and is responsible for
the difference in the genetic response to ecdysone between the late
larval and prepupal ecdysone pulses.
betaFTZ-F1 induction is confirmed by
the microarray results. Several
other genes are induced by DHR3 when it is expressed at >18 hours
BPF. One of these is represented by a novel EST (LD24139) that is
induced from 3 to 9 hours APF during wild-type development. ESTs representing 12 other DHR3-induced genes that have less than
threefold induction at 3 to 9 hours APF are listed at DHR3-regulated genes.
Some of these additional genes may not normally be DHR3 targets or may
be induced by DHR3 at other stages during development (White, 1999).
DHR3 has been shown to inhibit the induction of
ecdysone-inducible genes, and with E75B it can act as a repressor of
the betaFTZ-F1 gene. DHR3 is expressed
before the ecdysone-inducible genes are up-regulated but is still
capable of repressing genes. Four out of seven such genes
belong to the cytochrome P450 (CYP) class of genes. Three of these CYP genes are normally
repressed during the late larval pulse, and this repression begins
before DHR3 induction occurs (approximately 4 hours BPF). Thus, DHR3
cannot be solely responsible for their repression, although it may
contribute to it. One function of cytochrome P450 molecules is
hydroxylation of steroids; the depletion of
transcripts of the CYP genes may provide a mechanism by
which production of the biologically active form of ecdysone
(20-hydroxyecdysone) is stifled at PF. Regulation of these
CYP genes within the ecdysone hierarchy further suggests
that they may have a role in controlling the ecdysone genetic cascade (White, 1999).
Taken together, these results demonstrate the utility of DNA
microarrays in determining the genetic foundations of metamorphosis. The identities of the differentially expressed genes discovered in this
study suggest several points of coordination between the ecdysone-regulated pathways that control the temporal aspects of
metamorphosis and the developmental pathways that control the specification and differentiation of particular cell types and tissues.
Despite the experimental restrictions imposed by the use of whole
animals, changes have been observed in the abundance of transcripts that
correlate with the late larval or prepupal ecdysone pulses (or both)
for genes whose activities have not been known to be influenced by
this hormone. Further studies are now needed to delineate
the relationship between the ecdysone-regulated genetic hierarchies and
the functions of both the known and the novel genes that are
differentially expressed during metamorphosis. For example, a next step
would be to distinguish genes that are directly regulated by ecdysone from
those that are secondary targets of ecdysone-regulated factors (White, 1999).
Data produced on a genomic scale can be used to similarly assist in
deciphering the complex genetic networks that control other stages of
Drosophila development. Great strides have of course been
made in defining these networks by use of mutations and expression
constructs. The resulting stick diagrams describing these networks
must, however, be incomplete, in part because inactivation of the
majority of genes does not result in obvious mutant phenotypes. Genomic approaches have the potential to expand these stick diagrams to include all functional genes. Integrating and
visualizing data derived from genomic studies present a substantial challenge. Nonetheless, combining the powerful molecular and genetic approaches that Drosophila offers with genomic information
will inevitably produce a reasonably complete picture of gene
regulation and its implications for metazoan development (White, 1999).
During insect metamorphosis, each tissue displays a unique physiological and morphological response to the steroid hormone 20-hydroxyecdysone (ecdysone). Gene expression was assayed in five tissues during metamorphosis onset. Larval-specific tissues display major changes in genome-wide expression profiles, whereas tissues that survive into adulthood display few changes. In one larval tissue, the salivary gland, a computational approach was used to identify a regulatory motif and a cognate transcription factor involved in regulating a set of coexpressed genes. During the metamorphosis of another tissue, the midgut, genes encoding factors from the hedgehog, Notch, EGF, dpp, and wingless pathways are activated by the ecdysone regulatory network. Mutation of the ecdysone receptor abolishes their induction. Cell cycle genes are also activated during the initiation of midgut metamorphosis, and they are also dependent on ecdysone signaling. These results establish multiple new connections between the ecdysone regulatory network and other well-studied regulatory networks (Li, 2003).
Developmental patterns of gene expression were studied from five different tissues and organs: central nervous system (CNS), wing imaginal disc (WD), larval epidermis and attached connective tissue (ED), midgut (MG), and salivary gland (SG), during late larval and early prepupal development when ecdysone triggers metamorphosis. At these stages of development, the five tissues display very different morphological and physiological responses to ecdysone. The wing imaginal disc responds to the hormone by initiating evagination, or unfolding, as it changes from a compact epithelial bilayer to an extended appendage. The salivary glands secrete glue proteins that are used to immobilize the puparium during metamorphosis. The cuticle attached to the larval epidermis undergoes a process of hardening and tanning to form the pupal case. The central nervous system (CNS) displays little morphological change during the late third instar ecdysone pulse, but the animal displays changes in behavior and in neurosecretory status. The two major types of cells in the larval midgut, larval epidermal cells and adult epidermal progenitor cells (midgut imaginal islands), respond in opposite ways to ecdysone. The larval epidermal cells initiate the process of programmed cell death, while the imaginal cells proliferate and form the adult midgut (Li, 2003).
One tissue, the midgut, was selected to assay during its complete metamorphosis, which occurs from 18 hr before puparium formation (BPF) to 12 hr APF. During this 30 hr period, eleven time points were examined as the larval midgut is destroyed and replaced with the adult midgut. The two major cell types present in this organ are distinguishable by size. The larval epithelial cells are large, with decondensed polyploid nuclei, and undergo programmed cell death in response to ecdysone. Embedded among the larval cells are small diploid imaginal midgut cells, which proliferate in response to the hormone to form the adult epithelial cells. Additionally, the midgut contains relatively small numbers of muscle, tracheal, and endocrine cells (Li, 2003).
In total, transcripts from a surprisingly large fraction of the genome, >30%, changed significantly during the metamorphosis of the midgut (18 hr BPF to 12 hr APF). Broad classes of temporally separable gene expression patterns are evident. These classes include sets of transcripts that rapidly decrease coincident with onset of programmed cell death in the larval cells, sets that are induced during early or late metamorphosis, and sets of transcripts expressed at highest levels during the middle period of the time course when the larval cells are in the final stages of cell death and the adult cells are rearranging to form new tissue (Li, 2003).
Within these broad classes, specific sets of genes that have related functions and show parallel expression were identified, indicating that they make up gene batteries. Six such examples, included coregulated transcripts that encode proteins found in specific macromolecular complexes, biochemical pathways, organellar functions, and structural components of the cells that compose this tissue. Transcripts encoding proteasome components increase during the ecdysone pulse that triggers the onset of cell death in larval cells. Transcripts encoding glycolytic enzymes rapidly decrease during the initiation of metamorphosis, but gradually resume expression as the imaginal cells proliferate. Vacuolar ATPases shows a pattern similar to the glycolytic enzymes, whereas tubulin- and actin-encoding transcripts peak during the intense period of imaginal cell proliferation and migration as the adult midgut is formed. Transcripts encoding structural components of the peritrophic membrane of the mature larval gut gradually decrease during its replacement with adult tissue (Li, 2003).
The expression patterns were examined of regulatory genes known to be involved in the ecdysone transcriptional hierarchy predicted to control the gene batteries that were identified. Also examined was the expression of genes with known roles in programmed cell death or cell cycle control. The expression of known ecdysone-responsive regulatory genes was consistent with previous observations in midgut. Although the larval midgut is composed of cell types that undergo divergent responses to ecdysone -- apoptosis and cell proliferation -- it was nonetheless possible to detect significant changes in transcript levels from genes encoding proteins involved in both processes. The apoptosis activator gene ark was expressed at 4 hr BPF. E93 and reaper, which encode proteins that serve as critical control points in the commitment to programmed cell death, were expressed at PF, as was the initiator caspase dronc. These midgut expression profiles were compared to those reported for salivary glands at and after 10 hr APF, when a prepupal pulse of ecdysone triggers apoptosis in that tissue; almost the entire genetic cascade was found to be similarly activated in salivary glands and midgut albeit at two distinct periods of development. However, one notable difference was observed at the top level of the cascade. In the salivary gland, E93 is activated by βFTZ-F1, whereas in the midgut the βFTZ-F1 gene is not induced until 6-8 hr after E93 is induced. The regulation of E93 therefore does not depend on βFTZ-F1 in the midgut, but must rely on another as yet unidentified factor(s). During midgut metamorphosis, developmental modulation of transcript levels were also observed for genes encoding DNA polymerases, cyclins, CDCs, and other cell cycle regulators, as well as genes encoding DNA repair proteins such as Hus1, Rad23, and PCNA/Mus209 (Li, 2003).
Which of the genes that are differentially expressed at the onset of midgut metamorphosis require ecdysone signaling? Ecdysone-dependent transcriptional activity was removed using mutant Ecdysone Receptor (EcR) alleles, rescuing null EcR mutants to the third larval instar by using a heat shock-inducible EcR transgene. Gene expression was examined in mutant midguts that were isolated from mutant animals arrested at the end of the third larval stage (stage 2a mutants). 376 (76%) of the 495 genes that are significantly induced during the onset of midgut metamorphosis (18 hr BPF to 2 hr APF) required EcR function, whereas 296 (64%) of 460 transcripts that decline significantly in level during this time period require ecdysone signaling through EcR. Thus, a very large proportion of the genes that are developmentally regulated at the initiation of metamorphosis in this organ are under the control of the transcription factors that mediate the ecdysone signal. However, it does not appear that EcR function is a general requirement for transcription, because a significant fraction of differentially expressed genes are unaffected in EcR mutant tissue (Li, 2003).
Of the several different classes of genes expressed during midgut metamorphosis, the regulation of all genes in the proteasome, tubulin/actin, and lysozyme clusters requires EcR to exhibit their normal changes in developmental expression. However, many genes in the v-ATPase cluster and nearly half the genes in the peritrophin cluster did not require EcR. The downregulation of hexokinase A, 6-phosphofructokinase, and pyruvate kinase genes in the glycolysis pathway were affected in the EcR mutants, while many others in this pathway were not. Hexokinase A, 6-phosphofructokinase, and pyruvate kinase are rate-controlling enzymes in the glycolytic pathway, indicating that their ecdysone dependence is functionally significant. The expression of the numerous known ecdysone receptor target genes such as E75, E74, broad, E23, and DHR3 required EcR as expected. The induction dynamics for the E74 and DHR3 transcription factor genes was as expected, as was their dependence on EcR. In contrast to E74 and DHR3, DHR78 has previously been described to reside upstream of EcR at the top of the ecdysone regulatory hierarchy -- the expression of EcR is dependent on the wild-type function of DHR78. However, DHR78 can also be induced by ecdysone in organ culture. The results demonstrate that DHR78 wild-type induction is indeed dependent on EcR function. Taken together, these data indicate a positive feedback loop between EcR and DHR78 during the onset of metamorphosis in the midgut (Li, 2003).
Genes encoding factors involved in cell cycle and growth control, and in DNA repair, are also under the control of EcR. In spite of the role of ecdysone in stimulating cell proliferation during metamorphosis, no cell cycle genes have previously been linked to the ecdysone regulatory hierarchy. The induction of the cell cycle regulatory genes CyclinB, cdc2, and CyclinD were all observed to be dependent on EcR function. The rapid induction of cdc2 during the late third instar ecdysone pulse is similar to that observed for direct targets of EcR. The CyclinD gene is also induced at this time, but its maximal induction occurs several hours after that observed for cdc2. Cyclin D promotes cellular growth, whereas Cyclin B/Cdc2 controls G2/M transitions in proliferative cells. The dependence of these three genes on EcR function indicates that ecdysone may control cell proliferation, at least in part, through their regulation. Coordinate with the induction of CyclinB, cdc2, and CyclinD, the induction was observed of DNA polymerase-delta and DNA repair genes such as Rad23, and PCNA/mus209. The induction of these DNA repair and synthesis genes is also EcR dependent. The expression changes of these genes may be the result of the direct action of EcR, or due to the action of factors directly controlled by the ecdysone receptor complex. It is unlikely that the increase in expression of these genes is simply due to increased numbers of proliferative cells because the total number of divisions between 18 hr BPF and PF are few, and not all cell cycle or DNA repair genes showed an increase in expression at the initiation of metamorphosis. For example, the level of CyclinJ, which is known to be required during early embryonic division cycles, is actually reduced in expression from 18 hr BPF to PF. When the expression of cell death genes was examined in EcR mutant tissue, E93 induction was observed as well as induction of the Ark caspase activator and the dronc caspase gene required wild-type function of EcR (Li, 2003).
Factors in several well-studied signaling pathways are induced during midgut metamorphosis. These include Wnt (dishevelled, armadillo, and zeste white 3), TGFβ/BMP (sara, daughters against dpp, and glass bottom boat), EGFR (torpedo/egfr, rhomboid/veinlet, vein, and keren/spitz2), and Notch pathway genes (delta, kuzbanian, suppressor of hairless, E(spl)malpha, and E(spl)mβ). All of these pathways are used during embryonic midgut development, and these data indicate they are reused during midgut metamorphosis. Genes in the Hedgehog signaling pathway (hedgehog, smoothened, and cubitus interruptus) changed significantly as well (Li, 2003).
To determine whether any of the genes in these pathways are expressed as a consequence of ecdysone signaling, the EcR mutant expression data was examined for those genes that were induced during the late third instar ecdysone pulse. The induction of zeste white-3/shaggy, keren/spitz2, kuzbanian, and hedgehog are all dependent on the presence of functional EcR. The induction dynamics of the EGFR ligand gene keren/spitz2, the Notch proteolytic activation factor gene kuzbanian, and the shaggy/zeste white-3 kinase gene are similar to genes that are known direct targets of ecdysone signaling. The induction of hedgehog follows a secondary response pattern, as do genes from the E(spl) complex that are induced in response to Notch activation, although these induction kinetics are also consistent with these genes being partially activated directly by the ecdysone receptor and partially with other factors (i.e., they may be 'early-late' genes). These data show that the regulatory network controlled by ecdysone in midguts includes the activation of known components of the Wnt, EGFR, Hedgehog, and Notch pathways. Notably, ligand production for the EGF, Hedgehog, TGFβ/BMP, and Notch pathways is under control of ecdysone. The specific roles that each of these pathways plays during metamorphosis are currently unknown. These results nonetheless indicate new connections between ecdysone signaling and the activity of several other signaling pathways during the metamorphosis of this organ, either through direct targeting of the ecdysone receptor or through the actions of downstream factors (Li, 2003).
Eukaryotic cells catabolize their own cytoplasm by autophagy in response to amino acid starvation and inductive signals during programmed tissue remodeling and cell death. The Tor and PI3K signaling pathways have been shown to negatively control autophagy in eukaryotes, but the mechanisms that link these effectors to overall animal development and nutritional status in multicellular organisms remain poorly understood. This study reveals a complex regulation of programmed and starvation-induced autophagy in the Drosophila fat body. Gain-of-function genetic analysis indicates that Ecdysone receptor signaling induces programmed autophagy whereas PI3K signaling represses programmed autophagy. Genetic interaction studies show that ecdysone signaling downregulates PI3K signaling and that this represents the effector mechanism for induction of programmed autophagy. Hence, these studies link hormonal induction of autophagy to the regulatory function of the PI3K signaling pathway in vivo (Rusten, 2004).
The fat body is a primary nutrient-responsive tissue that emulates the functions of the liver and adipose tissue of vertebrates. Fat body cells undergo programmed autophagy during the last larval stage (L3) preceding pupariation. Findings in Mamestra brassicae have demonstrated that autophagy can be induced by ecdysone. In Drosophila, autophagy is developmentally upregulated from mid-L3 stage in fat body cells. Although previously the levels of ecdysone during the L3 stage of development in Drosophila have been detected only at low levels at the wandering-L3 stage and increase markedly before puparium formation in most studies, a small hormonal peak before the initiation of wandering has been reported. Expression of dominant-negative Ecdysone receptor from the mid-L3 stage under Lsp-Gal4 control results in a dramatic reduction of autophagy. The autophagic area is severely reduced, and fewer acidic structures are observed. Since complete inhibiton of autophagy was not observed, the timing of Lsp-Gal4 expression was closely followed and it was found that expression initiated reporter gene expression 20-30 min after programmed autophagy had been started. Most likely, this latency of Lsp-Gal4 expression accounts for the incomplete penetrance of the phenotypes. In fact, driving expression of the dominant-negative EcR using a constitutive fat body Gal4 driver (cg-Gal4), or placing a temperature-sensitive mutant of ecdysoneless (ecd1) to restrictive temperature at the start of the L3 stage, led to a complete inhibition of autophagy. This suggests that ecdysone has a regulatory role on programmed autophagy already at the early L3 stage and that the ecdysone titer at this stage of development is at the threshold of detection. The issue of ecdysone levels during larval development has recently been revisited: radioimmunoassay measurements detected low but continuously increasing levels of ecdysone during mid-L3 stage. Taken together, these results suggest that programmed autophagy is due to this low but rising level of ecdysone during the L3 stage of development (Rusten, 2004).
A simple explanation of ecdysone-induced programmed autophagy could be the initiation of wandering and therefore starvation-induced autophagy. This is not likely, however, for the following reasons. Developmental autophagy is initiated in fat bodies of late feeding animals at least 6 hr before the animals stop feeding and leave the food, and 12 hr before ingested food starts to disappear from the anterior part of the midgut. In addition, the autophagic response in fat body cells is uncoupled from the change in feeding behavior since expression of a dominant-negative ecdysone receptor cell autonomously inhibited programmed autophagy in late wandering L3 animals that ceased feeding 8 hr earlier (Rusten, 2004).
PI3K signaling is able to regulate autophagy and is unlikely to be a part of the amino acid sensing mechanism during an acute starvation response; amino acids and insulin have been shown to control autophagic proteolysis through different signaling pathways in rat hepatocytes. This is supported by the fact that the presence of the PIP3 binding probe, GFP-PH, at the cell membrane is not affected by amino acid deprivation in the fat body. The loss of PI3K signaling was only observed after 24 hr of starvation, long after the acute starvation response of autophagy. This concurs with observations in cultured mammalian cells in which insulin signaling and PI3K activity do not respond to variations in nutrient levels (Rusten, 2004).
What is then the physiological significance of PI3K signaling regulating autophagy? PI3K signaling was modulated in the fat body to see if it could influence the autophagic response to ecdysone. Elevation of PI3K signaling during the period of programmed autophagy prevented the biogenesis of autolysosomes. This epistatic regulation of PI3K signaling over ecdysone-induced programmed autophagy suggests that PI3K signaling is a part of the same pathway or a dominant repressor. A strong reduction and ultimately loss of PI3K signaling was observed in the fat body during the induction of programmed autophagy, suggesting that ecdysone downregulates PI3K signaling. In addition, a reduction in PI3K signaling failed to increase the autophagic activity during programmed autophagy, in line with the idea that it is in the same pathway and is already inhibited completely. In contrast, reducing Tor signaling in the fat body could further increase autophagic activity during developmental autophagy, suggesting that Tor is not inhibited completely, or not involved in programmed autophagy. Elucidating the role of Tor signaling during this process requires further studies (Rusten, 2004).
Several lines of evidence support a role for PI3K signaling in ecdysone-induced programmed autophagy in the fat body. (1) Inhibition of Ecdysone receptor activity or an increase in PI3K signaling produced very similar phenotypes, indicating that these pathways perform opposite regulatory roles on programmed autophagy. (2) Administration of the ecdysone analog RH5849 to feeding larvae promoted attenuation of PI3K signaling. (3) Clonal inactivation of ecdysone receptor signaling led to a failure of this attenuation. (4) Simultaneous downregulation of PI3K signaling and inhibiton of ecdysone receptor activity restored programmed autophagy to wild-type levels. Thus, ecdysone signaling is both necessary and sufficient for downregulation of the PI3K pathway during programmed autophagy. Taken together, these results suggest a model in which ecdysone receptor signaling has the ability to promote autophagy through the downregulation of PI3K signaling (Rusten, 2004).
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