Cell type-specific regulatory sequences control expression of theDrosophila FMRF-NH2 neuropeptide gene

Benveniste, Ronald J.; Taghert, Paul H.

doi:10.1002/(sici)1097-4695(199903)38:4<507::aid-neu7>3.0.co;2-x

Cited by 40 publications

(33 citation statements)

References 53 publications

(49 reference statements)

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“…A Drosophila ddc::GFP construct containing this fragment was relatively strongly expressed in most pharyngeal muscle cells, a single amphid neuron, a single head interneuron (likely RICL or RIAL) and in PVT, but not in catecholaminergic neurons. Finally, Drosophila FMRF::GFP construct contained a 3.6 kb fragment upstream of the translation initiation site of Drosophila FMRFamide gene which was previously shown to be expressed in nearly all FMRFergic neurons in the fly (Benveniste and Taghert, 1999). We detected consistent expression of this fusion gene in most muscle cells in the pharynx, a single head interneuron (RMDDL, RMDL, RMF, or RMH) and three to five neurons in the ventral cord (DA or VA).…”

Section: Resultsmentioning

confidence: 68%

Functional tests of enhancer conservation between distantly related species

Ruvinsky

Ruvkun

2003

Development

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Expression patterns of orthologous genes are often conserved, even between distantly related organisms, suggesting that once established, developmental programs can be stably maintained over long periods of evolutionary time. Because many orthologous transcription factors are also functionally conserved, one possible model to account for homologous gene expression patterns, is conservation of specific binding sites within cis-regulatory elements of orthologous genes. If this model is correct, a cis-regulatory element from one organism would be expected to function in a distantly related organism. To test this hypothesis, we fused the green fluorescent protein gene to neuronal and muscular enhancer elements from a variety of Drosophila melanogaster genes, and tested whether these would activate expression in the homologous cell types in Caenorhabditis elegans. Regulatory elements from several genes directed appropriate expression in homologous tissue types, suggesting conservation of regulatory sites. However, enhancers of most Drosophila genes tested were not properly recognized in C. elegans, implying that over this evolutionary distance enough changes occurred in cis-regulatory sequences and/or transcription factors to prevent proper recognition of heterospecific enhancers. Comparisons of enhancer elements of orthologous genes between C. elegans and C. briggsae revealed extensive conservation, as well as specific instances of functional divergence. Our results indicate that functional changes in cis-regulatory sequences accumulate on timescales much shorter than the divergence of arthropods and nematodes, and that mechanisms other than conservation of individual binding sites within enhancer elements are responsible for the conservation of expression patterns of homologous genes between distantly related species.

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Section: Resultsmentioning

confidence: 68%

Functional tests of enhancer conservation between distantly related species

Ruvinsky

Ruvkun

2003

Development

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“…1 (compare A with B), we find that in crawling third instar wit mutants there is a specific disruption in the accumulation of FaRPs in the Tv neurons and the neurohemal organ. Other FaRP-positive cells such as the subesophageal neurons (SE2) (Benveniste and Taghert, 1999) in the ventral ganglia and several neurons in the brain appear to express FaRPs normally or are only moderately affected. It is important to note that the NHO is composed of two components: the two or three NHO cells and the large varicosities formed by the Tv neurons axons that terminate on the NHO cells.…”

Section: Results Wit Mutants Eliminate Expression Of Fmrfa In Tv Neuronsmentioning

confidence: 99%

“…As the FMRFa gene is known to be strongly expressed in the Tv neurons that innervate the NHO Schneider et al, 1993a;Schneider et al, 1993b), we examined the effect of wit mutations on the expression of a FMRFa/lacZ transgene. The regulatory region of FMRFa comprises several different enhancers, including one that produces strong expression in the Tv neurons (Benveniste and Taghert, 1999). As shown in Fig.…”

Section: Results Wit Mutants Eliminate Expression Of Fmrfa In Tv Neuronsmentioning

confidence: 99%

“…Although several families are recognized on the basis of conserved sequences, among the most broadly distributed are FMRFamide-related peptides (FaRPs) (Geary et al, 1999;Grimmelikhuijzen et al, 1989;Hinuma et al, 2000;Yang et al, 1985). These peptides share a common C-terminal RFamide sequence and in Drosophila are produced from at least five genes, dromyosuppressin, drosulfakinin, two neuropeptide F-like genes and FMRFa (reviewed by Benveniste and Taghert, 1999;Merte and Nichols, 2002). Some of these loci can produce several different peptides exhibiting unique N-terminal sequences by selective proteolytic processing of a proprotein.…”

Section: Introductionmentioning

confidence: 99%

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Retrograde Gbb signaling through the Bmp type 2 receptor Wishful Thinking regulates systemic FMRFa expression inDrosophila

et al. 2003

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Amidated neuropeptides of the FMRFamide class regulate numerous physiological processes including synaptic efficacy at the Drosophilaneuromuscular junction (NMJ). We demonstrate here that mutations in wishful thinking (wit) a gene encoding a DrosophilaBmp type 2 receptor that is required for proper neurotransmitter release at the neuromuscular junction, also eliminates expression of FMRFa in that subset of neuroendocrine cells (Tv neurons) which provide the systemic supply of FMRFa peptides. We show that Gbb, a Bmp ligand expressed in the neurohemal organ provides a retrograde signal that helps specify the peptidergic phenotype of the Tv neurons. Finally, we show that supplying FMRFa in neurosecretory cells partially rescues the witlethal phenotype without rescuing the primary morphological or electrophysiological defects of wit mutants. We propose that Wit and Gbb globally regulate NMJ function by controlling both the growth and transmitter release properties of the synapse as well as the expression of systemic modulators of NMJ synaptic activity.

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“…The primers 5′-CAGATCTCGACGATTTTTGTTCAGCCAT-3′ (5′ UTR) and 5′-TGCGGCCGCAGAAACTCTCGAAAGGGCT-3′ (end of the ORF) were used to construct a 1236 bp fragment that was cloned into pBSK+ and then transferred to pP{UAST-Myc} at the BglII and NotI sites. Transgenic lines containing P{UAS-dimm::Myc} insertions were created using standard techniques (Benveniste and Taghert, 1999). UAS-dimm::Myc 2-A-3 , Rev8/CyO, Act-GFP flies were crossed to c127-Gal4, UAS-GFP; Rev4/CyO, Act-GFP, and first instar larvae were scored for Act-GFP-and c127-specific GFP labeling patterns.…”

Section: Uas-dimm Transgenementioning

confidence: 99%

The bHLH protein Dimmed controls neuroendocrine cell differentiation inDrosophila

et al. 2003

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Neuroendocrine cells are specialized to produce, maintain and release large stores of secretory peptides. We show that the Drosophila dimmed/Mist1 bHLH gene confers such a pro-secretory phenotype on neuroendocrine cells. dimmed is expressed selectively in central and peripheral neuroendocrine cells. In dimmed mutants, these cells survive, and adopt normal cell fates and morphology. However, they display greatly diminished levels of secretory peptide mRNAs, and of diverse peptides and proteins destined for regulated secretion. Secretory peptide levels are lowered even in the presence of artificially high secretory peptide mRNA levels. In addition, overexpression of dimmed in a wild-type background produces a complimentary phenotype: an increase in secretory peptide levels by neuroendocrine cells, and an increase in the number of cells displaying a neuroendocrine phenotype. We propose that dimmed encodes an integral component of a novel mechanism by which diverse neuroendocrine lineages differentiate and maintain the pro-secretory state. 1772 dimmed (dimm), with an expression pattern that corresponds precisely to the neuronal and endocrine cells that accumulate large amounts of secretory peptides. We present both loss-offunction and gain-of-function analyses to argue that dimm confers a pro-secretory phenotype within these diverse cells, and that its actions appear confined to that aspect of cellular differentiation. Thus, we propose a novel and general mechanism, of which dimm is an essential component, for the amplification of the regulated secretory pathway by dedicated secretory cells. MATERIALS AND METHODS StrainsFlies were cultured at 22-25°C on a standard cornmeal-yeast-agar medium. The molecular and genetic characterization of c929, R6 and Rev8 has been described previously (Hewes et al., 2000). Rev4 and Rev18 are X-ray revertants of P{PZ}l (2)k05106 S2a ) were obtained by transposase-mediated excision, and each line was characterized by PCR with primers flanking the original insertion site. Except as noted, all other strains are described elsewhere (Lindsley and Zimm, 1992;FlyBase, 1999) and were obtained from the Bloomington stock center, the BDGP Gene Disruption Project and other sources. Scoring of dimm larvaeEggs were collected on apple juice-agar plates supplemented with yeast paste. Larvae were collected from the plates, and heterozygotes (y* w* and balanced over CyO-y + ) were distinguished by mouthpart color. After scoring, size-matched pairs of y -and y + larvae were dissected and stained in parallel.

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Cell type-specific regulatory sequences control expression of theDrosophila FMRF-NH2 neuropeptide gene

Cited by 40 publications

References 53 publications

Functional tests of enhancer conservation between distantly related species

Functional tests of enhancer conservation between distantly related species

Retrograde Gbb signaling through the Bmp type 2 receptor Wishful Thinking regulates systemic FMRFa expression inDrosophila

The bHLH protein Dimmed controls neuroendocrine cell differentiation inDrosophila

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