Roush W (1996) Science "Regulating G protein signaling."

Roush W

[Science, 1996]

As anyone who has ever slept with a snorer, studied in a college dormitory, or lived next door to a pianist knows, tuning out one's surroundings can be a sanity-preserving skill. This ability isn't just limited to humans. Even the simplest cells can mute their own internal communication lines to tune out the racket of chemical noise made by hormones, neurotransmitters, growth factors, and other cell regulators, allowing them to damp down their responses to such stimuli after prolonged exposure. Exactly how cells achieve this "desensitization" is unclear, but in a spate of recent studies, researchers in several laboratories have closed in on one volume control for a key intracellular communication line: the "G proteins" that serve as intermediaries carrying signals from numerous hormones and neurotransmitters to the cell interior. Over the past year, the work has uncovered a large and growing family of proteins that seem to regulate the sensitivity of G protein signaling pathways in organisms ranging from yeast and nematodes to rats and even

Roush W (1997) Science "Worm longevity gene cloned."

Roush W

[Science, 1997]

A gene that helps control the life-span of the nematode C. elegans encodes the worm version of the insulin receptor, thereby providing a possible link between aging and glucose metabolism.

Roush W (1996) Science "Sperm protein makes its mark upon the worm embryo."

Roush W

[Science, 1996]

In creatures from worms to people, it takes two sexes to reproduce, but it's often the female who gets stuck with the real work of childbearing. This division of labor is even mirrored in sperm and eggs. The unfertilized eggs of fruit flies, for example, already contain the molecular signals needed to direct one of the first events in embryonic growth, the creation of distinct body segments. The paternal contribution to early development, in contrast, seems paltry. Sperm carries nuclear material and organelles called centrosomes - organizing sites for cell division - that come into play later on, but no biochemical factors that guide early embryogenesis have been traced back to the father. In the January issue of the journal Development, however, molecular biologist Heidi Browning of the University of Colorado and developmental geneticist Susan Strome of Indiana University report that SPE-11, a protein produced only in the sperm of the nematode Caenorhabditis elegans, may play a crucial role during the first few minutes after the embryo is fertilized.

Roush W (1996) Science "Divide and confer: how worm embryo cells specialize."

Roush W

[Science, 1996]

The one-cell animal embryo, or zygote, faces a daunting engineering task: implementing the architectural plans inscribed in its DNS for building a complex, multicelled body. So, like any sensible construction supervisor, the zygote swiftly divides the project into manageable chunks, assigning some of its progeny to build only gut, for example, and other to make only muscle or skin. Just how each early embryonic cell gets its orders is understood only for the fruit fly Drosophila melanogaster-an achievement that helped win 1995's Nobel Prize in medicine for three developmental biologists. Now, however, the communication lines governing embryonic development are emerging in another animal beloved of developmental researchers: the tiny worm known as Caenorhabditis elegans.

K Omata et al. (1999) International C. elegans Meeting "Characterization of the neural circuit of C. elegans: model analysis of the touch response"

F Yonezawa, K Omata, K Kawamura

[International C. elegans Meeting, 1999]

In order to characterize the neural circuit of C. elagans, we construct a simple model by making use of the data table completed recently by Oshio et al . [1]. We assume that the signal of a neuron is calculated by the product of the signals from the neighboring neurons, and we investigate the touch sensitivity to continuous stimuli described by sinusoidal functions as defined in the rage from 0.0 to 1.0. We calculate the responses of the motor neurons by changing the frequencies of the stimuli. In our calculations, we change only the frequency w PLM for the input signal to the sensory neuron PLM, while the frequency for the other sensory neurons ALM, AVM and PVM is fixed to be a same value w 0 . We show that the output signals from the motor neurons A and B oscillate in time. We measure the minima of the oscillation for each w PLM value. The plot of the minima versus w PLM shows different hehaviors for the case of the neuron A and B. As for the signals from the neuron A, the values of the minima are widely distributed between 0.0 and 1.0 for all w PLM . As for the signals from the neuron B, on the other hand, the features are different for different w PLM values. (a) In the high frequency region of w PLM / w 0 0.4, the oscillation is simple harmonic and there exists only one minimum value (I min = 0.0). (b) As w PLM / w 0 is decreased, another minimum appears at a certain frequency, and the bifurcation takes place discontinuously. This behavior is different from usual continuous bifurcation observed in nonlinear systems. After a few discontinuous branching occur, signals with five periods can be seen in the intermediate frequency region of 0.3 w PLM / w 0 w PLM / w 0 [1] K. Oshio et al. ; C. elegans synaptic connectivity data'', Technical Report, CCEP, Keio Future No.1 (1998).

Wang C et al. (2018) Nat Commun "Author Correction: Small-molecule TFEB pathway agonists that ameliorate metabolic syndrome in mice and extend C. elegans lifespan."

Zhao T, Oswald NW, Li Y, Lin R, Wang C, Jaramillo J, Zhou A, McMillan EA, Douglas PM, MacMillan JB, Huang G, Luo M, Gao J, Mendiratta S, Lin Z, Wang Z, Niederstrasser H, Posner BA, Brekken RA, White MA

[Nat Commun, 2018]

The originally published version of this Article contained an error in the spelling of the author Nathaniel W. Oswald, which was incorrectly given as Nathaniel W. Olswald. This has now been corrected inboth the PDF and HTML versions of the Article.

Nawa Y et al. (1985) Parasite Immunol "Defective protective capacity of W/Wv mice against Strongyloides ratti infection and its reconstitution with bone marrow cells."

Kotani M, Nawa Y, Kiyota M, Korenaga M

[Parasite Immunol, 1985]

The susceptibility of congenitally anemic, and mast cell deficient W/Wv mice to infection with Strongyloides ratti was examined. After a primary infection, W/Wv mice showed greater and more persistent peak larval counts than did normal littermates. Worm expulsion was also slower in W/Wv mice than in +/+ mice. Furthermore, difference in susceptibility was expressed as early as 24 h after infection, suggesting not only that protective mechanisms of the gut but also of the connective tissue were defective in W/Wv mice. Reconstitution with bone marrow or spleen cells from +/+ mice was effective in restoring the protective response in W/Wv mice, whereas thymocytes or mesenteric lymph nodes had no effect. Both connective tissue and mucosal mast cells were repaired in W/Wv mice after marrow reconstitution and infection. Since relatively long incubation period was required for the expression of such reconstituting activities, bone marrow cells seem to contain precursor cells of the effector and/or regulator cells.

Casiraghi M et al. (2004) Int J Parasitol "Mapping the presence of Wolbachia pipientis on the phylogeny of filarial nematodes: evidence for symbiont loss during evolution."

Guerrero R, Bandi C, Franceschi A, Pocacqua V, Gardner SL, Casiraghi M, Martin C, Bain O

[Int J Parasitol, 2004]

Wolbachia pipientis is a bacterial endosymbiont associated with arthropods and filarial nematodes. In filarial nematodes, W. pipientis has been shown to play an important role in the biology of the host and in the immuno-pathology of filariasis. Several species of filariae, including the most important parasites of humans and animals (e.g. Onchocerca volvulus, Wuchereria bancrofti and Dirofilaria immitis) have been shown to harbour these bacteria. Other filarial species, including an important rodent species (Acanthocheilonema viteae), which has been used as a model for the study of filariasis, do not appear to harbour these symbionts. There are still several open questions about the distribution of W. pipientis in filarial nematodes. Firstly the number of species examined is still limited. Secondly, it is not clear whether the absence of W. pipientis in negative species could represent an ancestral characteristic or the result of a secondary loss. Thirdly, several aspects of the phylogeny of filarial nematodes are still unclear and it is thus difficult to overlay the presence/absence of W. pipientis on a tree representing filarial evolution. Here we present the results of a PCR screening for W. pipientis in 16 species of filariae and related nematodes, representing different families/subfamilies. Evidence for the presence of W. pipientis is reported for five species examined for the first time (representing the genera Litomosoides, Litomosa and Dipetalonema); original results on the absence of this bacterium are reported for nine species; for the remaining two species, we have confirmed the absence of W. pipientis recently reported by other authors. In the positive species, the infecting W. pipientis bacteria have been identified through 16S rDNA gene sequence analysis. In addition to the screening for W. pipientis in 16 species, we have generated phylogenetic reconstructions based on mitochondrial gene sequences (12S rDNA; COI), including a total of 28 filarial species and related spirurid nematodes. The mapping of the presence/absence of W. pipientis on the trees generated indicates that these bacteria have possibly been lost during evolution along some lineages of filarial nematodes.

Lewis JA (1981) Worm Breeder's Gazette "Modified Ficoll Method for Cleaning Worms"

Lewis JA

[Worm Breeder's Gazette, 1981]

I have made two modifications in the Ficoll method I originally described in WBG, vol. 3, #2. First, all Ficoll solutions are made 0. 1 M in NaCl to avoid shocking osmoticalIy sensitive worms like unc-29( e1072). Second, after sedimenting worms through 15% w/w Ficoll 400 ( 15', 300 x g), the worms are diluted with an equal volume of 0.1 M NaCl and floated on 35% w/w Ficoll (15', 300 x g) before washing 2x with 0.1 M NaCl. The Ficoll sedimentation removes dead or degenerated worms, cuticles, bacteria. The flotation removes crystalline debris sometimes occurring in worm cultures. We also find that special care to pipette out the last residue of bacterial medium (e.g. 3XD) before resuspending bacteria for worm growth is most conducive to obtaining uncontaminated worms.

Li Z et al. (2018) Pak J Pharm Sci "Cellulase-assisted extraction and anti-ultraviolet activity of polysaccharides from the root of Flammulina velutipes on Caenorhabditis elegans."

Chen M, Lin L, Zhang Y, Wang T, Cui H, Wang C, Li Z

[Pak J Pharm Sci, 2018]

We investigated the cellulase-assisted extraction and anti-ultraviolet activity of water-soluble polysaccharides from the root of Flammulina velutipes on Caenorhabditis elegans. A Box-Behnken design experiment with three factors and three levels, including enzymolysis temperature, microwave time, and microwave power, was designed on the basis of the results of single-factor experiments. For improving the polysaccharide yield of F. velutipes root, the following optimal extraction conditions were used: 52.67C enzymolysis temperature, 80s microwave time, and 144 W microwave power. Under optimal conditions, the actual measured value of the yield was 2.01% (w/w) and the predicted value was 2.06% (w/w). One fraction (FRP-2) was isolated and purified, and its characteristics were analyzed. The average mean molecular weight of FRP-2 was measured to be 2.60x10⁵ Da, and its monosaccharide composition is mainly glucose. The sugar units are present both in the -configuration and -configuration. Moreover, FRP-2 exhibited certain anti-ultraviolet activity to C. elegans when the polysaccharide concentration ranged between 0.05mg/mL and 0.20mg/mL.