| Muscle assembly and maintenance |
| zfh2 | | np |
none
| no |
ReferenceRNA interference screening in Drosophila primary cells for genes involved in muscle assembly and maintenance. Bai et al.,
2008
To facilitate the genetic analysis of muscle assembly and maintenance, we have developed a method for efficient RNA interference (RNAi) in Drosophila primary cells using double-stranded RNAs (dsRNAs). First, using molecular markers, we confirm and extend the observation that myogenesis in primary cultures derived from Drosophila embryonic cells follows the same developmental course as that seen in vivo. Second, we apply this approach to analyze 28 Drosophila homologs of human muscle disease genes and find that 19 of them, when disrupted, lead to abnormal muscle phenotypes in primary culture. Third, from an RNAi screen of 1140 genes chosen at random, we identify 49 involved in late muscle differentiation. We validate our approach with the in vivo analyses of three genes. We find that Fermitin 1 and Fermitin 2, which are involved in integrin-containing adhesion structures, act in a partially redundant manner to maintain muscle integrity. In addition, we characterize CG2165, which encodes a plasma membrane Ca2+-ATPase, and show that it plays an important role in maintaining muscle integrity. Finally, we discuss how Drosophila primary cells can be manipulated to develop cell-based assays to model human diseases for RNAi and small-molecule screens.
Screen detailsStable Id:
GR00159-A
Screen title:
Muscle assembly and maintenance
Assay:
Muscle cell morphology
Method:
Fluorescence
Scope:
Selected and random genes
Screen type:
Cell-based
Species:
Drosophila melanogaster
Biosource:
Primary cells
Biomodel:
primary embryonic cells
Library:
DRSC, np
Reagent type:
dsRNA
Score type:
Percentage of muscles with a given phenotype
Cutoff:
Severe: > 80 %; medium: ~ 50 %
Notes:
|
| Cell size and cell-cycle regulation (1) | FBgn0037502|FBgn0004607
| CG10113|zfh2 | GH26340 | sp |
none
| no |
ReferenceIdentification of pathways regulating cell size and cell-cycle progression by RNAi. Bjӧrklund et al.,
2006
Many high-throughput loss-of-function analyses of the eukaryotic cell cycle have relied on the unicellular yeast species Saccharomyces cerevisiae and Schizosaccharomyces pombe. In multicellular organisms, however, additional control mechanisms regulate the cell cycle to specify the size of the organism and its constituent organs. To identify such genes, here we analysed the effect of the loss of function of 70% of Drosophila genes (including 90% of genes conserved in human) on cell-cycle progression of S2 cells using flow cytometry. To address redundancy, we also targeted genes involved in protein phosphorylation simultaneously with their homologues. We identify genes that control cell size, cytokinesis, cell death and/or apoptosis, and the G1 and G2/M phases of the cell cycle. Classification of the genes into pathways by unsupervised hierarchical clustering on the basis of these phenotypes shows that, in addition to classical regulatory mechanisms such as Myc/Max, Cyclin/Cdk and E2F, cell-cycle progression in S2 cells is controlled by vesicular and nuclear transport proteins, COP9 signalosome activity and four extracellular-signal-regulated pathways (Wnt, p38betaMAPK, FRAP/TOR and JAK/STAT). In addition, by simultaneously analysing several phenotypes, we identify a translational regulator, eIF-3p66, that specifically affects the Cyclin/Cdk pathway activity.
Screen detailsStable Id:
GR00048-A-1
Screen title:
Cell size and cell-cycle regulation (1)
Assay:
Cell size, DNA content and viability
Method:
Flow cytometry
Scope:
Kinases, phosphatases and selected genes
Screen type:
Cell-based
Species:
Drosophila melanogaster
Biosource:
Cell line
Biomodel:
S2
Library:
Custom-made, DGC1, DGC2 and PHOSPHO
Reagent type:
dsRNA
Score type:
Complex, sp
Cutoff:
Complex criteria
Notes:
Additional information about the primary sccreen (pooled library) and a secondary screen (number of binucleate cells)
|
| Heart development and function (1) | CG1449
| | | 1 |
none
| no |
ReferenceA global in vivo Drosophila RNAi screen identifies NOT3 as a conserved regulator of heart function. Neely et al.,
2010
Heart diseases are the most common causes of morbidity and death in humans. Using cardiac-specific RNAi-silencing in Drosophila, we knocked down 7061 evolutionarily conserved genes under conditions of stress. We present a first global roadmap of pathways potentially playing conserved roles in the cardiovascular system. One critical pathway identified was the CCR4-Not complex implicated in transcriptional and posttranscriptional regulatory mechanisms. Silencing of CCR4-Not components in adult Drosophila resulted in myofibrillar disarray and dilated cardiomyopathy. Heterozygous not3 knockout mice showed spontaneous impairment of cardiac contractility and increased susceptibility to heart failure. These heart defects were reversed via inhibition of HDACs, suggesting a mechanistic link to epigenetic chromatin remodeling. In humans, we show that a common NOT3 SNP correlates with altered cardiac QT intervals, a known cause of potentially lethal ventricular tachyarrhythmias. Thus, our functional genome-wide screen in Drosophila can identify candidates that directly translate into conserved mammalian genes involved in heart function.
Screen detailsStable Id:
GR00138-A-1
Screen title:
Heart development and function (1)
Assay:
Viability
Method:
Fly count
Scope:
Selected genes
Screen type:
in vivo
Species:
Drosophila melanogaster
Biosource:
Tissue
Biomodel:
TinCΔ4 12a-Gal4
Library:
VDRC, np
Reagent type:
UAS-IR construct
Score type:
Developmental lethality
Cutoff:
<= 0.6666
Notes:
|
| Lipid storage | FBgn0004607
| | | -4.41 |
none
| no |
ReferenceCOPI complex is a regulator of lipid homeostasis. Beller et al.,
2008
Lipid droplets are ubiquitous triglyceride and sterol ester storage organelles required for energy storage homeostasis and biosynthesis. Although little is known about lipid droplet formation and regulation, it is clear that members of the PAT (perilipin, adipocyte differentiation related protein, tail interacting protein of 47 kDa) protein family coat the droplet surface and mediate interactions with lipases that remobilize the stored lipids. We identified key Drosophila candidate genes for lipid droplet regulation by RNA interference (RNAi) screening with an image segmentation-based optical read-out system, and show that these regulatory functions are conserved in the mouse. Those include the vesicle-mediated Coat Protein Complex I (COPI) transport complex, which is required for limiting lipid storage. We found that COPI components regulate the PAT protein composition at the lipid droplet surface, and promote the association of adipocyte triglyceride lipase (ATGL) with the lipid droplet surface to mediate lipolysis. Two compounds known to inhibit COPI function, Exo1 and Brefeldin A, phenocopy COPI knockdowns. Furthermore, RNAi inhibition of ATGL and simultaneous drug treatment indicate that COPI and ATGL function in the same pathway. These data indicate that the COPI complex is an evolutionarily conserved regulator of lipid homeostasis, and highlight an interaction between vesicle transport systems and lipid droplets.
Screen detailsStable Id:
GR00002-A-0
Screen title:
Lipid storage
Assay:
Lipid droplet staining
Method:
High content (microscopy)
Scope:
Screen type:
Cell-based
Species:
Drosophila melanogaster
Biosource:
Cell line
Biomodel:
Kc167
Library:
, DRSC
Reagent type:
dsRNA
Score type:
B-score
Cutoff:
2.0 / -1.7
Notes:
|
| Adiposity regulation (1) | FBgn0004607
| zfh2 | | -0.76 |
none
| no |
ReferenceDrosophila genome-wide obesity screen reveals hedgehog as a determinant of brown versus white adipose cell fate. Pospisilik et al.,
2010
Over 1 billion people are estimated to be overweight, placing them at risk for diabetes, cardiovascular disease, and cancer. We performed a systems-level genetic dissection of adiposity regulation using genome-wide RNAi screening in adult Drosophila. As a follow-up, the resulting approximately 500 candidate obesity genes were functionally classified using muscle-, oenocyte-, fat-body-, and neuronal-specific knockdown in vivo and revealed hedgehog signaling as the top-scoring fat-body-specific pathway. To extrapolate these findings into mammals, we generated fat-specific hedgehog-activation mutant mice. Intriguingly, these mice displayed near total loss of white, but not brown, fat compartments. Mechanistically, activation of hedgehog signaling irreversibly blocked differentiation of white adipocytes through direct, coordinate modulation of early adipogenic factors. These findings identify a role for hedgehog signaling in white/brown adipocyte determination and link in vivo RNAi-based scanning of the Drosophila genome to regulation of adipocyte cell fate in mammals.
Screen detailsStable Id:
GR00190-A-1
Screen title:
Adiposity regulation (1)
Assay:
Total fly triglyceride expression
Method:
Colorimetric determination
Scope:
Genome-wide
Screen type:
in vivo
Species:
Drosophila melanogaster
Biosource:
Organism
Biomodel:
Hsp70-GAL4;Tub-GAL80ts
Library:
VDRC, np
Reagent type:
UAS-IR construct
Score type:
Triglyceride change
Cutoff:
Z-score > 1.65 after 3 screening rounds
Notes:
Additional information about the primary screen
|
| Cell growth and viability (2) |
| | | 0.3 |
none
| no |
ReferenceGenome-wide RNAi analysis of growth and viability in Drosophila cells. Boutros et al.,
2004
A crucial aim upon completion of whole genome sequences is the functional analysis of all predicted genes. We have applied a high-throughput RNA-interference (RNAi) screen of 19,470 double-stranded (ds) RNAs in cultured cells to characterize the function of nearly all (91%) predicted Drosophila genes in cell growth and viability. We found 438 dsRNAs that identified essential genes, among which 80% lacked mutant alleles. A quantitative assay of cell number was applied to identify genes of known and uncharacterized functions. In particular, we demonstrate a role for the homolog of a mammalian acute myeloid leukemia gene (AML1) in cell survival. Such a systematic screen for cell phenotypes, such as cell viability, can thus be effective in characterizing functionally related genes on a genome-wide scale.
Screen detailsStable Id:
GR00031-A-2
Screen title:
Cell growth and viability (2)
Assay:
Cell number and viability
Method:
Luminescence
Scope:
Genome-wide
Screen type:
Cell-based
Species:
Drosophila melanogaster
Biosource:
Cell line
Biomodel:
S2R+
Library:
Custom-made, HFA
Reagent type:
dsRNA
Score type:
Z-score
Cutoff:
>= 3.0
Notes:
|
| Cell growth and viability (1) |
| | | 0.1 |
none
| yes |
ReferenceGenome-wide RNAi analysis of growth and viability in Drosophila cells. Boutros et al.,
2004
A crucial aim upon completion of whole genome sequences is the functional analysis of all predicted genes. We have applied a high-throughput RNA-interference (RNAi) screen of 19,470 double-stranded (ds) RNAs in cultured cells to characterize the function of nearly all (91%) predicted Drosophila genes in cell growth and viability. We found 438 dsRNAs that identified essential genes, among which 80% lacked mutant alleles. A quantitative assay of cell number was applied to identify genes of known and uncharacterized functions. In particular, we demonstrate a role for the homolog of a mammalian acute myeloid leukemia gene (AML1) in cell survival. Such a systematic screen for cell phenotypes, such as cell viability, can thus be effective in characterizing functionally related genes on a genome-wide scale.
Screen detailsStable Id:
GR00031-A-1
Screen title:
Cell growth and viability (1)
Assay:
Cell number and viability
Method:
Luminescence
Scope:
Genome-wide
Screen type:
Cell-based
Species:
Drosophila melanogaster
Biosource:
Cell line
Biomodel:
Kc167
Library:
Custom-made, HFA
Reagent type:
dsRNA
Score type:
Z-score
Cutoff:
>= 3.0
Notes:
|
| Lipid storage | FBgn0004607
| | | 0.67 |
none
| no |
ReferenceCOPI complex is a regulator of lipid homeostasis. Beller et al.,
2008
Lipid droplets are ubiquitous triglyceride and sterol ester storage organelles required for energy storage homeostasis and biosynthesis. Although little is known about lipid droplet formation and regulation, it is clear that members of the PAT (perilipin, adipocyte differentiation related protein, tail interacting protein of 47 kDa) protein family coat the droplet surface and mediate interactions with lipases that remobilize the stored lipids. We identified key Drosophila candidate genes for lipid droplet regulation by RNA interference (RNAi) screening with an image segmentation-based optical read-out system, and show that these regulatory functions are conserved in the mouse. Those include the vesicle-mediated Coat Protein Complex I (COPI) transport complex, which is required for limiting lipid storage. We found that COPI components regulate the PAT protein composition at the lipid droplet surface, and promote the association of adipocyte triglyceride lipase (ATGL) with the lipid droplet surface to mediate lipolysis. Two compounds known to inhibit COPI function, Exo1 and Brefeldin A, phenocopy COPI knockdowns. Furthermore, RNAi inhibition of ATGL and simultaneous drug treatment indicate that COPI and ATGL function in the same pathway. These data indicate that the COPI complex is an evolutionarily conserved regulator of lipid homeostasis, and highlight an interaction between vesicle transport systems and lipid droplets.
Screen detailsStable Id:
GR00002-A-0
Screen title:
Lipid storage
Assay:
Lipid droplet staining
Method:
High content (microscopy)
Scope:
Screen type:
Cell-based
Species:
Drosophila melanogaster
Biosource:
Cell line
Biomodel:
Kc167
Library:
, DRSC
Reagent type:
dsRNA
Score type:
B-score
Cutoff:
2.0 / -1.7
Notes:
|
| Cell size and cell-cycle regulation (1) | FBgn0004607
| zfh2 | GH11902 | sp |
none
| no |
ReferenceIdentification of pathways regulating cell size and cell-cycle progression by RNAi. Bjӧrklund et al.,
2006
Many high-throughput loss-of-function analyses of the eukaryotic cell cycle have relied on the unicellular yeast species Saccharomyces cerevisiae and Schizosaccharomyces pombe. In multicellular organisms, however, additional control mechanisms regulate the cell cycle to specify the size of the organism and its constituent organs. To identify such genes, here we analysed the effect of the loss of function of 70% of Drosophila genes (including 90% of genes conserved in human) on cell-cycle progression of S2 cells using flow cytometry. To address redundancy, we also targeted genes involved in protein phosphorylation simultaneously with their homologues. We identify genes that control cell size, cytokinesis, cell death and/or apoptosis, and the G1 and G2/M phases of the cell cycle. Classification of the genes into pathways by unsupervised hierarchical clustering on the basis of these phenotypes shows that, in addition to classical regulatory mechanisms such as Myc/Max, Cyclin/Cdk and E2F, cell-cycle progression in S2 cells is controlled by vesicular and nuclear transport proteins, COP9 signalosome activity and four extracellular-signal-regulated pathways (Wnt, p38betaMAPK, FRAP/TOR and JAK/STAT). In addition, by simultaneously analysing several phenotypes, we identify a translational regulator, eIF-3p66, that specifically affects the Cyclin/Cdk pathway activity.
Screen detailsStable Id:
GR00048-A-1
Screen title:
Cell size and cell-cycle regulation (1)
Assay:
Cell size, DNA content and viability
Method:
Flow cytometry
Scope:
Kinases, phosphatases and selected genes
Screen type:
Cell-based
Species:
Drosophila melanogaster
Biosource:
Cell line
Biomodel:
S2
Library:
Custom-made, DGC1, DGC2 and PHOSPHO
Reagent type:
dsRNA
Score type:
Complex, sp
Cutoff:
Complex criteria
Notes:
Additional information about the primary sccreen (pooled library) and a secondary screen (number of binucleate cells)
|
| Serratia marcescens infection (1) | CG1449
| zfh2 | | -0.15 |
none
| no |
ReferenceGenome-wide RNAi screen identifies genes involved in intestinal pathogenic bacterial infection. Cronin et al.,
2009
Innate immunity represents the first line of defense in animals. We report a genome-wide in vivo Drosophila RNA interference screen to uncover genes involved in susceptibility or resistance to intestinal infection with the bacterium Serratia marcescens. We first employed whole-organism gene suppression, followed by tissue-specific silencing in gut epithelium or hemocytes to identify several hundred genes involved in intestinal antibacterial immunity. Among the pathways identified, we showed that the JAK-STAT signaling pathway controls host defense in the gut by regulating stem cell proliferation and thus epithelial cell homeostasis. Therefore, we revealed multiple genes involved in antibacterial defense and the regulation of innate immunity.
Screen detailsStable Id:
GR00142-A-1
Screen title:
Serratia marcescens infection (1)
Assay:
Heat shock and viability
Method:
Fly count
Scope:
Random genes
Screen type:
in vivo
Species:
Drosophila melanogaster
Biosource:
Organism
Biomodel:
HSP70-GAL4; TubGAL80ts
Library:
VDRC, np
Reagent type:
UAS-IR construct
Score type:
Days life time (LT50)
Cutoff:
< -1.5 SD OR > 2 SD
Notes:
|
| PGN-induced dJNK phosphorylation | FBgn0004607
| zfh2 | np | 2.02 |
Increased P-JNK protein expression with PGN
| no |
ReferenceA quantitative RNAi screen for JNK modifiers identifies Pvr as a novel regulator of Drosophila immune signaling. Bond and Foley,
2009
Drosophila melanogaster responds to gram-negative bacterial challenges through the IMD pathway, a signal transduction cassette that is driven by the coordinated activities of JNK, NF-kappaB and caspase modules. While many modifiers of NF-kappaB activity were identified in cell culture and in vivo assays, the regulatory apparatus that determines JNK inputs into the IMD pathway is relatively unexplored. In this manuscript, we present the first quantitative screen of the entire genome of Drosophila for novel regulators of JNK activity in the IMD pathway. We identified a large number of gene products that negatively or positively impact on JNK activation in the IMD pathway. In particular, we identified the Pvr receptor tyrosine kinase as a potent inhibitor of JNK activation. In a series of in vivo and cell culture assays, we demonstrated that activation of the IMD pathway drives JNK-dependent expression of the Pvr ligands, Pvf2 and Pvf3, which in turn act through the Pvr/ERK MAP kinase pathway to attenuate the JNK and NF-kappaB arms of the IMD pathway. Our data illuminate a poorly understood arm of a critical and evolutionarily conserved innate immune response. Furthermore, given the pleiotropic involvement of JNK in eukaryotic cell biology, we believe that many of the novel regulators identified in this screen are of interest beyond immune signaling.
Screen detailsStable Id:
GR00148-A
Screen title:
PGN-induced dJNK phosphorylation
Assay:
P-JNK protein expression
Method:
Fluorescence
Scope:
Genome-wide
Screen type:
Cell-based
Species:
Drosophila melanogaster
Biosource:
Cell line
Biomodel:
S2
Library:
Open Biosystems and custom-made, np and custom-made
Reagent type:
dsRNA
Score type:
Z-score
Cutoff:
Complex criteria
Notes:
Only hits stored in GenomeRNAi
|
| Muscle morphogenesis and function (1) | CG1449
| zfh2 | | np |
none
| no |
ReferenceSystematic genetic analysis of muscle morphogenesis and function in Drosophila. Schnorrer et al.,
2010
Systematic genetic approaches have provided deep insight into the molecular and cellular mechanisms that operate in simple unicellular organisms. For multicellular organisms, however, the pleiotropy of gene function has largely restricted such approaches to the study of early embryogenesis. With the availability of genome-wide transgenic RNA interference (RNAi) libraries in Drosophila, it is now possible to perform a systematic genetic dissection of any cell or tissue type at any stage of the lifespan. Here we apply these methods to define the genetic basis for formation and function of the Drosophila muscle. We identify a role in muscle for 2,785 genes, many of which we assign to specific functions in the organization of muscles, myofibrils or sarcomeres. Many of these genes are phylogenetically conserved, including genes implicated in mammalian sarcomere organization and human muscle diseases.
Screen detailsStable Id:
GR00134-A-1
Screen title:
Muscle morphogenesis and function (1)
Assay:
Posture, locomotion, flight and viability
Method:
Visual inspection
Scope:
Genome-wide
Screen type:
in vivo
Species:
Drosophila melanogaster
Biosource:
Tissue
Biomodel:
Mef2-GAL4
Library:
VDRC, np
Reagent type:
UAS-IR construct
Score type:
rp
Cutoff:
S19 > 0.5
Notes:
|
| Dendrite pattern formation | CG1449
| zfh2 | zfh2 | np |
none
| no |
ReferenceGenome-wide analyses identify transcription factors required for proper morphogenesis of Drosophila sensory neuron dendrites. Parrish et al.,
2006
Dendrite arborization patterns are critical determinants of neuronal function. To explore the basis of transcriptional regulation in dendrite pattern formation, we used RNA interference (RNAi) to screen 730 transcriptional regulators and identified 78 genes involved in patterning the stereotyped dendritic arbors of class I da neurons in Drosophila. Most of these transcriptional regulators affect dendrite morphology without altering the number of class I dendrite arborization (da) neurons and fall primarily into three groups. Group A genes control both primary dendrite extension and lateral branching, hence the overall dendritic field. Nineteen genes within group A act to increase arborization, whereas 20 other genes restrict dendritic coverage. Group B genes appear to balance dendritic outgrowth and branching. Nineteen group B genes function to promote branching rather than outgrowth, and two others have the opposite effects. Finally, 10 group C genes are critical for the routing of the dendritic arbors of individual class I da neurons. Thus, multiple genetic programs operate to calibrate dendritic coverage, to coordinate the elaboration of primary versus secondary branches, and to lay out these dendritic branches in the proper orientation.
Screen detailsStable Id:
GR00065-A
Screen title:
Dendrite pattern formation
Assay:
mCD8 protein expression
Method:
Fluorescence
Scope:
Transcription factors
Screen type:
in vivo
Species:
Drosophila melanogaster
Biosource:
Tissue
Biomodel:
GAL4221
Library:
Custom-made, Custom-made
Reagent type:
UAS-IR construct
Score type:
np
Cutoff:
Phenotypes in multiple blind tests
Notes:
Additional information about secondary screens
|
| Heat nociception (1) | CG1449
| zfh2 | | 0 |
Lethal
| no |
ReferenceA genome-wide Drosophila screen for heat nociception identifies α2δ3 as an evolutionarily conserved pain gene. Neely et al.,
2010
Worldwide, acute, and chronic pain affects 20% of the adult population and represents an enormous financial and emotional burden. Using genome-wide neuronal-specific RNAi knockdown in Drosophila, we report a global screen for an innate behavior and identify hundreds of genes implicated in heat nociception, including the α2δ family calcium channel subunit straightjacket (stj). Mice mutant for the stj ortholog CACNA2D3 (α2δ3) also exhibit impaired behavioral heat pain sensitivity. In addition, in humans, α2δ3 SNP variants associate with reduced sensitivity to acute noxious heat and chronic back pain. Functional imaging in α2δ3 mutant mice revealed impaired transmission of thermal pain-evoked signals from the thalamus to higher-order pain centers. Intriguingly, in α2δ3 mutant mice, thermal pain and tactile stimulation triggered strong cross-activation, or synesthesia, of brain regions involved in vision, olfaction, and hearing.
Screen detailsStable Id:
GR00135-A-1
Screen title:
Heat nociception (1)
Assay:
Noxious heat avoidance and viability
Method:
Fly count
Scope:
Genome-wide
Screen type:
in vivo
Species:
Drosophila melanogaster
Biosource:
Organism
Biomodel:
elav-GAL4
Library:
VDRC, np
Reagent type:
UAS-IR construct
Score type:
Z-score
Cutoff:
> 1.65
Notes:
Additional information about secondary screens (geotactic, phototaxis, and temperature sensitivity)
|
| Akt-TOR pathway negative feedback regulation | FBgn0004607
| zfh2 | | -2.4 |
none
| no |
ReferenceDynamic switch of negative feedback regulation in Drosophila Akt-TOR signaling. Kockel et al.,
2010
Akt represents a nodal point between the Insulin receptor and TOR signaling, and its activation by phosphorylation controls cell proliferation, cell size, and metabolism. The activity of Akt must be carefully balanced, as increased Akt signaling is frequently associated with cancer and as insufficient Akt signaling is linked to metabolic disease and diabetes mellitus. Using a genome-wide RNAi screen in Drosophila cells in culture, and in vivo analyses in the third instar wing imaginal disc, we studied the regulatory circuitries that define dAkt activation. We provide evidence that negative feedback regulation of dAkt occurs during normal Drosophila development in vivo. Whereas in cell culture dAkt is regulated by S6 Kinase (S6K)-dependent negative feedback, this feedback inhibition only plays a minor role in vivo. In contrast, dAkt activation under wild-type conditions is defined by feedback inhibition that depends on TOR Complex 1 (TORC1), but is S6K-independent. This feedback inhibition is switched from TORC1 to S6K only in the context of enhanced TORC1 activity, as triggered by mutations in tsc2. These results illustrate how the Akt-TOR pathway dynamically adapts the routing of negative feedback in response to the activity load of its signaling circuit in vivo.
Screen detailsStable Id:
GR00169-A
Screen title:
Akt-TOR pathway negative feedback regulation
Assay:
dAkt phosphorylation
Method:
Fluorescence
Scope:
Genome-wide
Screen type:
Cell-based
Species:
Drosophila melanogaster
Biosource:
Cell line
Biomodel:
Kc167
Library:
Custom-made, Custom-made
Reagent type:
dsRNA
Score type:
Z-score
Cutoff:
< -2.5 OR > 2.5
Notes:
|
| Notch pathway regulation (4) | CG1449
| | | sp |
Completely lethal (pupal)
| no |
ReferenceGenome-wide analysis of Notch signalling in Drosophila by transgenic RNAi. Mummery-Widmer et al.,
2009
Genome-wide RNA interference (RNAi) screens have identified near-complete sets of genes involved in cellular processes. However, this methodology has not yet been used to study complex developmental processes in a tissue-specific manner. Here we report the use of a library of Drosophila strains expressing inducible hairpin RNAi constructs to study the Notch signalling pathway during external sensory organ development. We assigned putative loss-of-function phenotypes to 21.2% of the protein-coding Drosophila genes. Using secondary assays, we identified 6 new genes involved in asymmetric cell division and 23 novel genes regulating the Notch signalling pathway. By integrating our phenotypic results with protein interaction data, we constructed a genome-wide, functionally validated interaction network governing Notch signalling and asymmetric cell division. We used clustering algorithms to identify nuclear import pathways and the COP9 signallosome as Notch regulators. Our results show that complex developmental processes can be analysed on a genome-wide level and provide a unique resource for functional annotation of the Drosophila genome.
Screen detailsStable Id:
GR00144-A-4
Screen title:
Notch pathway regulation (4)
Assay:
External sensory organ morphology and viability
Method:
Visual inspection
Scope:
Genome-wide
Screen type:
in vivo
Species:
Drosophila melanogaster
Biosource:
Tissue
Biomodel:
pnr-GAL4
Library:
VDRC, np
Reagent type:
UAS-IR construct
Score type:
Phenotype strength
Cutoff:
np
Notes:
|
