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[
International C. elegans Meeting,
2001]
Early-onset torsion dystonia is a human neurological movement disorder caused by a deletion of single codon in the TOR1A (DYT-1) gene encoding a protein termed torsin A. We have utilized the C. elegans genome sequence database to identify 3 predicted open-reading frames that share high amino acid sequence identity to the human torsin A protein. Our focus has been on two of these genes, that we have named
tor-2 and
tor-1 , which share the highest identity to torsin A and lie a putative operon on Chr. IV of C. elegans. We are examining the function of these proteins using a combination of reverse genetic and functional genomic methods. As an initial step toward characterizing this protein family, we have generated a GFP reporter gene fusion to C. elegans
tor-2 and examined its expression in vivo. Like its human counterpart, the worm torsin A homolog is expressed in neurons. Fluorescence is detected in early larvae and persists through adulthood in neuronal processes of the head and tail. We are currently confirming this expression and determining the localization of this protein using affinity-purified antisera we have generated vs. worm TOR-2. We have also isolated a full-length cDNA for C. elegans
tor-2 , created a deletion of a corresponding codon designed to mimic the dominant human defect in this protein, and are studying the effect of overexpression of this construct in transgenic animals. Complementary phenotypic analyses by RNAi are also in progress. Torsin proteins share distant similarity to members of the Hsp100/Clp family of heat-shock proteins that have exhibited an ability to prevent polyglutamine aggregation. We are also investigating the possibility that worm TOR-2 and TOR-1 may function in a similar capacity. Elegant studies from the Morimoto and Kramer labs (PNAS, 97:5750-55) have shown that worms containing a transgenic array coding for 82 polyglutamine-repeats fused to GFP form aggregates when expressed in body wall muscle. We have placed the C. elegans
tor-2 gene under the control of the
unc-54 promoter and have co-expressed it with either Q82-GFP and Q19-GFP constructs. Preliminary results from this analysis indicate that TOR-2 may act as a molecular chaperone in that it exhibits an ability to reproducibly reduce polyglutamine-induced GFP aggregation. We are determining if this effect is either diminished by the substitution of wild-type TOR-2 with mutant TOR-2 or is further ameliorated by co-expression of TOR-1 in this assay. It is our hope that these studies will provide novel insights into torsin protein function towards gaining a more complete understanding of dystonia at the molecular level.
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[
Worm Breeder's Gazette,
2000]
WormBase (www.wormbase.org) is an international consortium of biologists and computer scientists dedicated to providing the research community with accurate, current, accessible information concerning the genetics, genomics and biology of C. elegans and some related nematodes. WormBase builds upon the existing ACeDB database of the C. elegans genome by providing curation from the literature, an expanded range of content and a user friendly web interface. The team that developed and maintained ACeDB (Richard Durbin, Jean Thierry-Mieg) remains an important part of WormBase. Lincoln Stein and colleagues at Cold Spring Harbor are leading the effort to develop the user interface, including visualization tools for the genome and genetic map. Teams at Sanger Centre (led by Richard Durbin) and the Genome Sequencing Center at Washington University, St. Louis (led by John Spieth) continue to curate the genomic sequence. Jean and Danielle Thierry-Mieg at NCBI spearhead importation of large-scale data sets from other projects. Paul Sternberg and colleagues at Caltech will curate new data including cell function in development, behavior and physiology, gene expression at a cellular level; and gene interactions. Paul Sternberg assumes overall responsibility for WormBase, and is delighted to hear feedback of any sort. WormBase has recently received major funding from the National Human Genome Research Institute at the US National Institutes of Health, and also receives support from the National Library of Medicine/NCBI and the British Medical Research Council. WormBase is an expansion of existing efforts, and as such continues to need you help and feedback. Even with the increased scope and funding, all past contributors to ACeDB remain involved. The Caenorhabditis Genetics Center (Jonathan Hodgkin and Sylvia Martinelli) collaborate with WormBase to curate the genetic map and related topics. Ian Hope and colleagues continue to supply expression data to WormBase. Leon Avery will continue his superb website and serves as one advisor to WormBase. While the major means of access to WormBase is via the world wide web, downloadable versions of WormBase as well as the acedb software engine will continue to be available.
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Zhen, Mei, Kasthuri, Bobby, Shalek, Richard, Lichtman, Jeff, Samuel, Aravi, Pfister, Hanspeter, Laskova, Valeriya, Kaynig-Fittkau, Verena, Wen, Quan, Berger, Daniel, Guan, Asuka
[
International Worm Meeting,
2013]
To investigate the poorly understood mechanisms of development and function of the nervous system, connections between neurons must be deciphered first. The adult nervous system of C. elegans was mapped to near completion by Dr. John White and his colleagues in 1970s. However, neuronal wiring in C. elegans larvae differs from that of an adult, since it undergoes multiple rounds of neuronal birth, apoptosis and rewiring during development. We utilize an Automatic Tape-Collecting Ultramicrotome (ATUM) to section an entire L1 stage animal into thousands cross-sections, followed by the automated imaging with a scanning electron microscope (SEM) to map an entire neuronal wiring diagram with synaptic resolution. The acquired wiring diagram will guide and be validated by calcium imaging to map the functional connection of the juvenile motor circuit.
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[
European Worm Meeting,
2006]
Gary Williams1, Paul Davis1, Anthony Rogers1, Philip Ozersky2, John Spieth2, Tamberlyn Bieri2, Darin Blasiar2. WormBase is an international consortium of biologists and computer scientists from Caltech (USA), Cold Spring Harbor Laboratory (USA), Wellcome Trust Sanger Institute (UK) and the Genome Sequencing Center at Washington University (USA).. WormBase is dedicated to providing the research community with accurate, current, accessible information concerning the genetics, genomics and biology of C. elegans, and some related nematodes. WormBase can be freely accessed at www.wormbase.org, and is also available for download at ftp://ftp.wormbase.org/pub/wormbase A new data release is produced every three weeks. Recently some new datasets have been added to the database to aid curation.The protein products from automated gene prediction in C. remanei have been mapped to the C. elegans genome; InterPro motifs are no longer taken from SwissProt annotations, but are directly predicted from the C. elegans proteins; contigs of ESTs from other nematode species produced by the NEMBASE and Nematode.net projects have been mapped to the genome and a new set of TEC-REDs have been mapped to the genome resulting in 3,325 new trans-spliced sites which mark the 5'' ends of genes or isoforms. Work is underway to classify and curate transposons and we intend to add Mass-Spec data from several sources to improve coding sequence validation.. Over the last year the curated coding sequences have increased from 19,854 to 20,060 and alternately spliced isoforms have increased from 2,772 to 2,883. The number of genes where every base of every exon is confirmed by EST evidence has increased from 6,427 to 6,584. In the C. elegans proteins there have been 630 modified entries, 440 deleted entries, 709 new entries and 64 reappeared entries.. WormBase is supported by a grant from the National Human Genome Research Institute at the US National Institute of Health #P41 HG02223 and the British Medical Research Council.
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[
Neuronal Development, Synaptic Function, and Behavior Meeting,
2006]
The networks of nerves and muscles responsible for forward and backward movements in C. elegans offer unique advantages for investigating the functional relationships among cells in integrated cellular networks. The first advantage is that John Sulston and his colleagues identified the interneurons, motor neurons and muscle cells that compose the networks (Sulston, et al., 1983). Second, John White and colleagues determined the synaptic patterns that interconnect the network (White et al., 1986). Finally, the C. elegans community has generated mutations that cause specific alterations in the cellular networks. A model based on the connectivity pattern and laser ablation results suggests that distinct sets of interneurons and excitatory motor neurons are dedicated to forward and backward movement, respectively. These two circuits converge upon two classes of inhibitory motor neurons and four longitudinal strands of body wall muscles and create antiphasic contractile muscular waves that travel along the dorsal and ventral axes of the body. We will report results from the analysis of movies showing locomotion patterns of animals. These movies allows us to quantitatively characterize the traveling wave in terms of amplitudes, dorsal and ventral deflections, frequency and velocity of the wave progression and the forward and backward velocity of the animal's progression. We will compare wild-type locomotion characteristics with those exhibited by three uncoordinated mutants (
unc-4,
unc-55, and
cnd-1) that are known to make specific alterations in the network that result in movement defects that are predicted by the model. The connectivity model can also be used to predict epistatic relationships for double mutant combinations (for example
unc-55 mutants exhibit a ventral asymmetric pattern of backward movement, whereas
unc-4 exhibits a dorsal asymmetric pattern of backward movement). We find that
unc-4 masks the defect of
unc-55 mutants, which is predicted by the model neural circuit. However the model's predictions for forward movement are not as accurate. We will discuss possible explanations for the resiliency of forward movement and the vulnerability of backward movement to genetic perturbations.
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[
West Coast Worm Meeting,
2000]
We briefly describe the current status and plans for WormBase, initially an extension of the existing ACeDB database with a new user interface. The WormBase consortium includes the team that developed ACeDB (Richard Durbin and colleagues at the Sanger Centre; Jean Thierry-Mieg and colleagues at Montpellier); Lincoln Stein and colleagues at Cold Spring Harbor, who developed the current web interface for WormBase; and John Spieth and colleagues at the Genome Sequencing Center at Washington University, who along with the Sanger Centre team, continue to annotate the genomic sequence. The Caltech group will curate new data including cell function in development, behavior and physiology, gene expression at a cellular level, and gene interactions. Data will be extracted from the literature, as well as by community submission. We look forward to providing the C. elegans and broader research community easy access to vast quantities of high quality data on C. elegans. Also, we welcome your suggestions and criticism at any time. WormBase can be accessed at www.wormbase.org.
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Berriman, Matt, Howe, Kevin, Kersey, Paul, Stein, Lincoln, Harris, Todd, Sternberg, Paul, Schedl, Tim
[
International Worm Meeting,
2015]
WormBase has existed for 15 years and has evolved in many ways. The new website is fully operational and has made the process of adding new data types, displays, and tools easier. Behind the scenes we are piloting an overhaul of the underlying database infrastructure to allow us to handle the ever increasing data, have the website perform faster, and allow more frequent updates of information. This is a critical time for the project, as we face considerable pressure from two directions. The first is that our funders really want us to do more with less. We are responding to this by leading the way in making curation (the process of extracting information from papers and data sets into computable form) more efficient using a new version of Textpresso (to be released later this calendar year); by discussing with other model organism information resources ways to work together to be more efficient and inter-connected; and by seeking additional sources of funding. The second, delightful, pressure is an increase in data and results generated by the C. elegans and nematode communities. While we are handling this increase by changes in our software for curation, the database infrastructure, and the website, we do need your help. Many of you have helped us over the last few years to identify data in your papers or by sending us data directly. We now need you to help with a few types of information by submitting the data via specially designed, user-friendly forms that ensure good quality and the use of standard terminology. In particular, we have a large backlog of uncurated information associating alleles with phenotypes. We pledge to make this process as painless as possible, and to improve WormBase's description of phenotypes with your feedback, starting at this meeting at the WormBase booth, workshops and posters. With your help, continual improvement of our efficiency, and additional sources of funding, we are optimistic that we can do much more with even somewhat less effort.Consortium: Paul Davis, Michael Paulini, Gary Williams, Bruce Bolt, Thomas Down, Jane Lomax, Todd Harris, Sibyl Gao, Scott Cain, Xiaodong Wang, Karen Yook, Juancarlos Chan, Wen Chen, Chris Grove, Mary Ann Tuli, Kimberly Van Auken, D. Wang, Ranjana Kishore, Raymond Lee, John DeModena, James Done, Yuling Li, H.-M. Mueller, Cecilia Nakamura, Daniela Raciti, Gary Schindelman.
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[
European Worm Meeting,
2006]
Rachel McMullan, Emma Hiley, Paul Morrison and Stephen J. Nurrish. Rho GTPases have important roles in neuronal development but their function in adult neurons is less well understood. We demonstrate that pre-synaptic changes in Rho activity at C.elegans neuromuscular junctions can radically change animal behaviour via modulation of two separate pathways. In one, pre-synaptic Rho increases acetylcholine (ACh) release by stimulating the accumulation of diacylglycerol (DAG) and the DAG-binding protein UNC-13 at sites of neurotransmitter release; this pathway requires binding of Rho to the DAG kinase DGK-1. A second DGK-1-independent mechanism is revealed by the ability of a Rho inhibitor (C3 transferase) to decrease levels of release even in the absence of DGK-1; this pathway is independent of UNC-13 accumulation at release sites. We do not detect any Rho induced changes in neuronal morphology or synapse number, thus Rho facilitates synaptic transmission by a novel mechanism. Surprisingly, many commonly available human RhoA constructs contain an uncharacterised mutation that severely reduces binding of RhoA to DAG kinase. Thus a role for RhoA in controlling DAG levels has not been previously appreciated.
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[
Japanese Worm Meeting,
2002]
The synaptic connectivity of C. elegans is well known from observations of the somatic system by White et al. and those of the pharyngeal system by Albertson et al. So far, three databases were constructed for computational usage by Achacoso et al. and Durbin, and recently in WormBase. However, they lack some data such as those in tables of White's paper and those in figures of Albertson's book. Our database (K. Oshio, S. Morita, Y. Osana and K. Oka: Technical Report of CCEP, Keio Future No.1, 1998) includes all data described in White's paper and Albertson's book. Unfortunately, some mistakes were found in the database through private communications with John White who is the author of White's paper and with the users of the database. Thus we have been proceeding with the revision to make it perfect one. We are planning to complete the revision in September 2002. The database should be worthwhile not only for neurophysiological studies, but also for post-genomic interests mediating genomes and behavior.
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[
International C. elegans Meeting,
1995]
During spermiogenesis, round nonmotile spermatids are rapidly transformed into asymmetrical crawling spermatozoa. In addition to
spe-8 and
spe-12, we found two new genes,
spe-27 and
spe-29, that when mutated, disrupt spermiogenesis in an identical manner: mutant hermaphrodites are self-sterile, while mutant males are fertile. Sperm from both sexes activate abnormally in vitro, suggesting that these gene products are expressed in both sperm, but only hermaphrodites require them for activation. The hermaphrodite's spermatids, however, can be activated by mating. This phenotype has been explained by a model that has two distinct pathways of activation, one for males and one for hermaphrodites (Shakes and Ward, 1989). The four genes are needed only for the hermaphrodite pathway.
spe-27 and
spe-12 have been cloned. Their mRNA is found exclusively in the germline during spermatogenesis. Their predicted protein sequences show no similarities to known proteins. We are currently cloning
spe-29. To further understand how these genes act during spermiogenesis we are determining the subcellular localization of their gene products. In addition, suppressor analysis is under way (see abstract by Paul Muhlrad and Samuel Ward) to look for other genes in this pathway and for interactions between these genes.