The transcriptional diversity of 25 <i>Drosophila</i> cell lines

Cherbas, Lucy; Willingham, Aarron; Zhang, Dayu; Yang, Li; Zou, Yi; Eads, Brian D.; Carlson, Joseph W.; Landolin, Jane M.; Kapranov, Philipp; Dumais, Jacqueline; Samsonova, Anastasia; Choi, Jeong-Hyeon; Roberts, Johnny; Davis, Carrie A.; Tang, Haixu; Baren, Marijke J. van; Ghosh, Srinka; Dobin, Alexander; Bell, Kimberly; Lin, Wei; Langton, Laura; Duff, Michael O.; Tenney, Aaron; Zaleski, Chris; Brent, Michael R.; Hoskins, Roger A.; Kaufman, Thomas C.; Andrews, Justen; Graveley, Brenton R.; Perrimon, Norbert; Celniker, S; Gingeras, T; Cherbas, Peter

doi:10.1101/gr.112961.110

Cited by 239 publications

(331 citation statements)

References 66 publications

Supporting

Mentioning

304

Contrasting

Order By: Relevance

“…Abl stimulates Eya tyrosine phosphorylation and cytoplasmic accumulation (Xiong et al 2009 and Figure 6, A vs. B, quantified in N) and thus should enhance SH2/PTB-pY-Eya interactions. Abl is expressed endogenously in S2 cells (Cherbas et al 2011), and some tyrosine phosphorylation of Eya can be detected in cells transfected with Eya alone (Tootle et al 2003), perhaps explaining the low levels of Socs36E and Socs44A CoIP detected when Abl was not supplied by cotransfection (Figure 5, C and D). The Abl independence of the Eya-Hop CoIP ( Figure 5A) suggests that either Hop phosphorylates Eya at different tyrosine residues, or that pY-SH2 interactions do not drive the CoIP.…”

Section: Mathey-prevot 2002;mentioning

confidence: 99%

Retinal Axon Guidance Requires Integration of Eya and the Jak/Stat Pathway into Phosphotyrosine-Based Signaling Circuitries in Drosophila

2016

View full text Add to dashboard Cite

The transcriptional coactivator and phosphatase eyes absent (Eya) is dynamically compartmentalized between the nucleus and cytoplasm. Although the nuclear transcriptional circuits within which Eya operates have been extensively characterized, understanding of its cytoplasmic functions and interactions remains limited. Our previous work showed that phosphorylation of Drosophila Eya by the Abelson tyrosine kinase can recruit Eya to the cytoplasm and that eya-abelson interactions are required for photoreceptor axons to project to correct layers in the brain. Based on these observations, we postulated that photoreceptor axon targeting might provide a suitable context for identifying the cytoplasmic signaling cascades with which Eya interacts. Using a dosesensitive eya misexpression background, we performed an RNA interference-based genetic screen to identify suppressors. Included among the top 10 hits were nonreceptor tyrosine kinases and multiple members of the Jak/Stat signaling network (hop, Stat92E, Socs36E, and Socs44A), a pathway not previously implicated in axon targeting. Individual loss-of-function phenotypes combined with analysis of axonal projections in Stat92E null clones confirmed the importance of photoreceptor autonomous Jak/Stat signaling. Experiments in cultured cells detected cytoplasmic complexes between Eya and Hop, Socs36E and Socs44A; the latter interaction required both the Src homology 2 motif in Socs44A and tyrosine phosphorylated Eya, suggesting direct binding and validating the premise of the screen. Taken together, our data provide new insight into the cytoplasmic phosphotyrosine signaling networks that operate during photoreceptor axon guidance and suggest specific points of interaction with Eya.KEYWORDS SH2; genetic screen; retinal determination network; eye development; Socs44A A remarkable feature of multicellular animal development is that the complexity and diversity in tissue type and patterning is achieved using fewer than a dozen signaling pathways, including Notch, receptor tyrosine kinase, Wnt, Hedgehog, TGFb, Jak/Stat, and Hippo. These cascades are repeatedly deployed in different contexts to regulate the majority of the critical proliferation, survival, specification, and differentiation decisions (reviewed in Voas and Rebay 2004;Housden and Perrimon 2014). One strategy to achieve context-specific developmental regulation is for proteins and pathways to function together in interconnected networks. Further, individual proteins within these networks may encode multiple independent functions that can be executed in distinct parts of the cell, cell types, or stages of development. In this way, even a modest number of individual proteins and core pathways can create vast combinatorial possibilities.Eyes absent (Eya), a protein conserved from plants to humans, presents an ideal model to study integration because its multifunctionality and dynamic subcellular localization provide opportunities for interaction with many signaling pathways (reviewed in Jemc andRebay 2007 an...

show abstract

Section: Mathey-prevot 2002;mentioning

confidence: 99%

Retinal Axon Guidance Requires Integration of Eya and the Jak/Stat Pathway into Phosphotyrosine-Based Signaling Circuitries in Drosophila

2016

View full text Add to dashboard Cite

show abstract

“…2). Kc cells, which are thought to be of hematopoietic origin (Echalier and Ohanessian 1969), do not express detectable levels of Snail, Twist, or Dorsal (data not shown), while the corepressors dCtBP and Ebi are present (Cherbas et al 2011). First, we tested the ability of Snail to repress the Dorsaldependent wntD-lacZ enhancer in this system (Zeitlinger et al 2007).…”

Section: Snail Positively Regulates Enhancer Activity In Collaboratiomentioning

confidence: 92%

A conserved role for Snail as a potentiator of active transcription

et al. 2014

View full text Add to dashboard Cite

The transcription factors of the Snail family are key regulators of epithelial–mesenchymal transitions, cell morphogenesis, and tumor metastasis. Since its discovery in Drosophila ∼25 years ago, Snail has been extensively studied for its role as a transcriptional repressor. Here we demonstrate that Drosophila Snail can positively modulate transcriptional activation. By combining information on in vivo occupancy with expression profiling of hand-selected, staged snail mutant embryos, we identified 106 genes that are potentially directly regulated by Snail during mesoderm development. In addition to the expected Snail-repressed genes, almost 50% of Snail targets showed an unanticipated activation. The majority of “Snail-activated” genes have enhancer elements cobound by Twist and are expressed in the mesoderm at the stages of Snail occupancy. Snail can potentiate Twist-mediated enhancer activation in vitro and is essential for enhancer activity in vivo. Using a machine learning approach, we show that differentially enriched motifs are sufficient to predict Snail's regulatory response. In silico mutagenesis revealed a likely causative motif, which we demonstrate is essential for enhancer activation. Taken together, these data indicate that Snail can potentiate enhancer activation by collaborating with different activators, providing a new mechanism by which Snail regulates development.

show abstract

“…Since Dmel2 cells express endogenous Brat and Pum (Cherbas et al 2011;Harris et al 2011;Weidmann and Goldstrohm 2012), we also performed knockdown experiments. As we lacked an antibody against endogenous Pum, we confirmed knockdown efficiency by the downregulation of coexpressed HA-tagged Pum (Fig.…”

Section: Repression Of Hb By Brat Is Independent Of Pummentioning

confidence: 99%

The NHL domain of BRAT is an RNA-binding domain that directly contacts the hunchback mRNA for regulation

et al. 2014

View full text Add to dashboard Cite

The Drosophila protein brain tumor (Brat) forms a complex with Pumilio (Pum) and Nanos (Nos) to repress hunchback (hb) mRNA translation at the posterior pole during early embryonic development. It is currently thought that complex formation is initiated by Pum, which directly binds the hb mRNA and subsequently recruits Nos and Brat. Here we report that, in addition to Pum, Brat also directly interacts with the hb mRNA. We identify Brat-binding sites distinct from the Pum consensus motif and show that RNA binding and translational repression by Brat do not require Pum, suggesting so far unrecognized Pum-independent Brat functions. Using various biochemical and biophysical methods, we also demonstrate that the NHL (NCL-1, HT2A, and LIN-41) domain of Brat, a domain previously believed to mediate protein-protein interactions, is a novel, sequence-specific ssRNA-binding domain. The Brat-NHL domain folds into a six-bladed b propeller, and we identify its positively charged top surface as the RNA-binding site. Brat belongs to the functional diverse TRIM (tripartite motif)-NHL protein family. Using structural homology modeling, we predict that the NHL domains of all TRIM-NHL proteins have the potential to bind RNA, indicating that Brat is part of a conserved family of RNA-binding proteins.

show abstract

The transcriptional diversity of 25 Drosophila cell lines

Cited by 239 publications

References 66 publications

Retinal Axon Guidance Requires Integration of Eya and the Jak/Stat Pathway into Phosphotyrosine-Based Signaling Circuitries in Drosophila

Retinal Axon Guidance Requires Integration of Eya and the Jak/Stat Pathway into Phosphotyrosine-Based Signaling Circuitries in Drosophila

A conserved role for Snail as a potentiator of active transcription

The NHL domain of BRAT is an RNA-binding domain that directly contacts the hunchback mRNA for regulation

Contact Info

Product

Resources

About