enhancer trap line
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2021 ◽  
Author(s):  
Annalie Martin ◽  
Anne Babbitt ◽  
Allison G Pickens ◽  
Brett E Pickett ◽  
Jonathon T Hill ◽  
...  

The optic tectum (OT) is a multilaminated midbrain structure that acts as the primary retinorecipient in the zebrafish brain. Homologous to the mammalian superior colliculus, the OT is responsible for the reception and integration of stimuli, followed by elicitation of salient behavioral responses. While the OT has been the focus of functional experiments for decades, less is known concerning specific cell types, microcircuitry, and their individual functions within the OT. Recent efforts have contributed substantially to the knowledge of tectal cell types; however, a comprehensive cell catalog is incomplete. Here we contribute to this growing effort by applying single-cell RNA-sequencing (scRNA-seq) to characterize the transcriptomic profiles of tectal cells labeled by the transgenic enhancer trap line y304Et(cfos:Gal4;UAS:Kaede). We sequenced 13,320 cells, a 4X cellular coverage, and identified 25 putative OT cell populations. Within those cells, we identified several mature and developing neuronal populations, as well as non-neuronal cell types including oligodendrocytes, microglia, and radial glia. Although most mature neurons demonstrate GABAergic activity, several glutamatergic populations are present, as well as one glycinergic population. We also conducted Gene Ontology analysis to identify enriched biological processes, and computed RNA velocity to infer current and future transcriptional cell states. Finally, we conducted in situ hybridization to validate our bioinformatic analyses and spatially map select clusters. In conclusion, the larval zebrafish OT is a complex structure containing at least 25 transcriptionally distinct cell populations. To our knowledge, this is the first time scRNA-seq has been applied to explore the OT alone and in depth.


Author(s):  
Hiroki Yagi ◽  
Atsushi J Nagano ◽  
Jaewook Kim ◽  
Kentaro Tamura ◽  
Nobuyoshi Mochizuki ◽  
...  

Abstract Hydathodes are typically found at leaf teeth in vascular plants and are involved in water release to the outside. Although morphological and physiological analysis of hydathodes has been performed in various plants, little is known about the genes involved in hydathode function. In this study, we performed fluorescent protein-based imaging and tissue-specific RNA-seq analysis in Arabidopsis hydathodes. We used the enhancer trap line E325, which has been reported to express green fluorescent protein (GFP) at its hydathodes. We found that E325-GFP was expressed in small cells found inside the hydathodes (named E cells) that were distributed between the water pores and xylem ends. No fluorescence of the phloem markers pSUC2:GFP and pSEOR1:SEOR1-YFP was observed in the hydathodes. These observations indicate that Arabidopsis hydathodes are composed of three major components: water pores, xylem ends, and E cells. In addition, we performed transcriptome analysis of the hydathode using the E325-GFP line. Microsamples were collected from GFP-positive or -negative regions of E325 leaf margins with a needle-based device (~130 µm in diameter). RNA-seq was performed with each single microsample using a high-throughput library preparation method called Lasy-Seq. We identified 72 differentially expressed genes. Among them, 68 genes showed significantly higher and four genes showed significantly lower expression in the hydathode. Our results provide new insights into the molecular basis for hydathode physiology and development.


eLife ◽  
2019 ◽  
Vol 8 ◽  
Author(s):  
Bicheng He ◽  
Marita Buescher ◽  
Max Stephen Farnworth ◽  
Frederic Strobl ◽  
Ernst HK Stelzer ◽  
...  

The genetic control of anterior brain development is highly conserved throughout animals. For instance, a conserved anterior gene regulatory network specifies the ancestral neuroendocrine center of animals and the apical organ of marine organisms. However, its contribution to the brain in non-marine animals has remained elusive. Here, we study the function of the Tc-foxQ2 forkhead transcription factor, a key regulator of the anterior gene regulatory network of insects. We characterized four distinct types of Tc-foxQ2 positive neural progenitor cells based on differential co-expression with Tc-six3/optix, Tc-six4, Tc-chx/vsx, Tc-nkx2.1/scro, Tc-ey, Tc-rx and Tc-fez1. An enhancer trap line built by genome editing marked Tc-foxQ2 positive neurons, which projected through the primary brain commissure and later through a subset of commissural fascicles. Eventually, they contributed to the central complex. Strikingly, in Tc-foxQ2 RNAi knock-down embryos the primary brain commissure did not split and subsequent development of midline brain structures stalled. Our work establishes foxQ2 as a key regulator of brain midline structures, which distinguish the protocerebrum from segmental ganglia. Unexpectedly, our data suggest that the central complex evolved by integrating neural cells from an ancestral anterior neuroendocrine center.


2019 ◽  
Author(s):  
Bicheng He ◽  
Marita Buescher ◽  
Max Stephen Farnworth ◽  
Frederic Strobl ◽  
Ernst Stelzer ◽  
...  

AbstractThe genetic control of anterior brain development is highly conserved throughout animals. For instance, a conserved anterior gene regulatory network specifies the ancestral neuroendocrine center of animals and the apical organ of marine organisms. However, its contribution to the brain in non-marine animals has remained elusive. Here, we study the function of theTc-foxQ2forkhead transcription factor, a key regulator of the anterior gene regulatory network of insects. We characterized four distinct types ofTc-foxQ2positive neural progenitor cells based on differential co-expression withTc-six3/optix, Tc-six4, Tc-chx/vsx, Tc-nkx2.1/scro, Tc-ey, Tc-rxandTc-fez1. An enhancer trap line built by genome editing markedTc-foxQ2positive neurons, which projected through the primary brain commissure and later through a subset of commissural fascicles. Eventually, they contributed to the central complex. Strikingly, inTc-foxQ2RNAi knock-down embryos the primary brain commissure did not split and subsequent development of midline brain structures stalled. Our work establishesfoxQ2as a key regulator of brain midline structures, which distinguish the protocerebrum from segmental ganglia. Unexpectedly, our data suggest that the central complex evolved by integrating neural cells from an ancestral anterior neuroendocrine center.Summary statementAn ancestral neuroendocrine center contributes to the evolution of the central complex.foxQ2is a gene required for the development of midline structures of the insect brain, which distinguish protocerebrum from segmental ganglia.


Plant Methods ◽  
2019 ◽  
Vol 15 (1) ◽  
Author(s):  
Lei Zhang ◽  
Li-Na Qin ◽  
Zi-Rui Zeng ◽  
Chang-Zheng Wu ◽  
Yuan-Yong Gong ◽  
...  

2018 ◽  
Vol 115 (4) ◽  
pp. E658-E667 ◽  
Author(s):  
David M. Linz ◽  
Yoshinori Tomoyasu

The origin of insect wings is still a highly debated mystery in biology, despite the importance of this evolutionary innovation. There are currently two prominent, but contrasting wing origin hypotheses (the tergal origin hypothesis and the pleural origin hypothesis). Through studies in the Tribolium beetle, we have previously obtained functional evidence supporting a third hypothesis, the dual origin hypothesis. Although this hypothesis can potentially unify the two competing hypotheses, it requires further testing from various fields. Here, we investigated the genetic regulation of the tissues serially homologous to wings in the abdomen, outside of the appendage-bearing segments, in Tribolium. We found that the formation of ectopic wings in the abdomen upon homeotic transformation relies not only on the previously identified abdominal wing serial homolog (gin-trap), but also on a secondary tissue in the pleural location. Using an enhancer trap line of nubbin (a wing lineage marker), we were able to visualize both of these two tissues (of tergal and pleural nature) contributing to form a complete wing. These results support the idea that the presence of two distinct sets of wing serial homologs per segment represents an ancestral state of the wing serial homologs, and can therefore further support a dual evolutionary origin of insect wings. Our analyses also uncovered detailed Hox regulation of abdominal wing serial homologs, which can be used as a foundation to elucidate the molecular mechanisms that have facilitated the evolution of bona fide insect wings, as well as the diversification of other wing serial homologs.


2015 ◽  
Vol 244 (12) ◽  
pp. 1574-1580 ◽  
Author(s):  
Hideaki Matsui ◽  
Alessandro Dorigo ◽  
Astrid Buchberger ◽  
Jennifer C. Hocking ◽  
Martin Distel ◽  
...  

2015 ◽  
Vol 19 (2) ◽  
pp. 96-100 ◽  
Author(s):  
Hee Jeong Kong ◽  
Jae-Ho Ryu ◽  
Woo-Jin Kim ◽  
Cheul Min An ◽  
Kyung-Eun Lim ◽  
...  

2012 ◽  
Vol 54 (2) ◽  
pp. 241-252 ◽  
Author(s):  
Naouel Gharbi ◽  
Xiao-Feng Zhao ◽  
Staale Ellingsen ◽  
Anders Fjose

2011 ◽  
Vol 11 (7) ◽  
pp. 409-414 ◽  
Author(s):  
Jane A. Cox ◽  
Anthony R. McAdow ◽  
Amy E. Dinitz ◽  
Andrew S. McCallion ◽  
Stephen L. Johnson ◽  
...  

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