PLOS Pathogens Staff (2014) PLoS Pathog "Correction: Ubiquitin-Mediated Response to Microsporidia and Virus Infection in C. elegans."

PLOS Pathogens Staff

[PLoS Pathog, 2014]

The fourth author's name is spelled incorrectly. The correct name is: Tiffany L. Dunbar. The correct citation is: Bakowski MA, Desjardins CA, Smelkinson MG, Dunbar TL, Lopez-Moyado IF, et al. (2014) Ubiquitin-Mediated Response to Microsporidia and Virus Infection in C. elegans. PLoS Pathog 10(6): e1004200. doi:10.1371/journal.ppat.1004200

Shao X et al. (2019) Mol Biol Cell "The adhesion modulation domain of C. elegans -catenin regulates actin binding during morphogenesis."

Strauch J, Hardin J, Lucas B, Shao X

[Mol Biol Cell, 2019]

Maintaining tissue integrity during epidermal morphogenesis depends on -catenin, which connects the cadherin complex to F-actin. We show that the adhesion modulation domain (AMD) of <i>C. elegans</i> HMP-1/-catenin regulates its F-actin binding activity and organization of junctional proximal actin <i>in vivo</i>. Deleting the AMD increases F-actin binding <i>in vitro</i> and leads to excess actin recruitment to adherens junctions <i>in vivo</i>. Reducing actin binding through a compensatory mutation in the C terminus leads to improved function. Based on the effects of phosphomimetic and non-phosphorylatable mutations phosphorylation of S509, within the AMD, may regulate F-actin binding. Taken together, these data establish a novel role for the AMD in regulating the actin binding ability of an -catenin and its proper function during epithelial morphogenesis.

Shimizu T et al. (2021) J Neurosci "Caenorhabditis elegans F-box protein promotes axon regeneration by inducing degradation of the Mad transcription factor."

Shimizu T, Hisamoto N, Todoroki Y, Matsumoto K, Hanafusa H, Sakai Y, Pastuhov SI

[J Neurosci, 2021]

In <i>Caenorhabditis elegans</i>, axon regeneration is activated by a signaling cascade through the receptor tyrosine kinase (RTK) SVH-2. Axonal injury induces <i>svh-2</i> gene expression by degradation of the Mad-like transcription factor MDL-1. In this study, we identify the <i>svh-24</i>/<i>sdz-33</i> gene encoding a protein containing F-box and F-box associated domains as a regulator of axon regeneration in motor neurons. We find that <i>sdz-33</i> is required for axon injury-induced <i>svh-2</i> expression. SDZ-33 targets MDL-1 for poly-ubiquitylation and degradation. Furthermore, we demonstrate that SDZ-33 promotes axotomy-induced nuclear degradation of MDL-1, resulting in the activation of <i>svh-2</i> expression in animals. These results suggest that the F-box protein is required for RTK signaling in the control of axon regeneration.<b>SIGNIFICANCE STATEMENT:</b>In <i>C. elegans</i>, axon regeneration is positively regulated by the growth factor SVH-1 and its receptor tyrosine kinase SVH-2. Expression of the <i>svh-2</i> gene is induced by axonal injury via the Ets-like transcription factor ETS-4, whose transcriptional activity is inhibited by the Mad-like transcription factor MDL-1. Axon injury leads to the degradation of MDL-1, and this is linked to the activation of ETS-4 transcriptional activity. In this study, we identify the <i>sdz-33</i> gene encoding a protein containing an F-box domain as a regulator of axon regeneration. We demonstrate that MDL-1 is poly-ubiquitylated and degraded through the SDZ-33-mediated 26S proteasome pathway. These results reveal that an F-box protein promotes axon regeneration by degrading the Mad transcription factor.

Pilotte N et al. (2019) Gates Open Res "Laboratory evaluation of molecular xenomonitoring using mosquito and tsetse fly excreta/feces to amplify Plasmodium, Brugia, and Trypanosoma DNA."

Reimer LJ, Cook DAN, Williams SA, Minetti C, Zulch MF, Pilotte N, Pryce J

[Gates Open Res, 2019]

<b>Background:</b> Results from an increasing number of studies suggest that mosquito excreta/feces (E/F) testing has considerable potential to serve as a supplement for traditional molecular xenomonitoring techniques. However, as the catalogue of possible use-cases for this methodology expands, and the list of amenable pathogens grows, a number of fundamental methods-based questions remain. Answering these questions is critical to maximizing the utility of this approach and to facilitating its successful implementation as an effective tool for molecular xenomonitoring. <b>Methods:</b> Utilizing E/F produced by mosquitoes or tsetse flies experimentally exposed to <i>Brugia malayi</i>, <i>Plasmodium falciparum</i>, or <i>Trypanosoma brucei brucei</i>, factors such as limits of detection, throughput of testing, adaptability to use with competent and incompetent vector species, and effects of additional blood feedings post parasite-exposure were evaluated. Two platforms for the detection of pathogen signal (quantitative real-time PCR and digital PCR (dPCR)) were also compared, with strengths and weaknesses examined for each. <b>Results:</b> Experimental results indicated that high throughput testing is possible when evaluating mosquito E/F for the presence of either <i>B. malayi</i> or <i>P. falciparum</i> from both competent and incompetent vector mosquito species. Furthermore, following exposure to pathogen, providing mosquitoes with a second, uninfected bloodmeal did not expand the temporal window for E/F collection during which pathogen detection was possible. However, this collection window did appear longer in E/F collected from tsetse flies following exposure to <i>T. b. brucei</i>. Testing also suggested that dPCR may facilitate detection through its increased sensitivity. Unfortunately, logistical obstacles will likely make the large-scale use of dPCR impractical for this purpose. <b>Conclusions:</b> By examining many E/F testing variables, expansion of this technology to a field-ready platform has become increasingly feasible. However, translation of this methodology from the lab to the field will first require field-based pilot studies aimed at assessing the efficacy of E/F screening.

Kipreos ET et al. (2000) Genome Biol "The F-box protein family."

Kipreos ET, Pagano M

[Genome Biol, 2000]

SUMMARY: The F-box is a protein motif of approximately 50 amino acids that functions as a site of protein-protein interaction. F-box proteins were first characterized as components of SCF ubiquitin-ligase complexes (named after their main components, Skp I, Cullin, and an F-box protein), in which they bind substrates for ubiquitin-mediated proteolysis. The F-box motif links the F-box protein to other components of the SCF complex by binding the core SCF component Skp I. F-box proteins have more recently been discovered to function in non-SCF protein complexes in a variety of cellular functions. There are 11 F-box proteins in budding yeast, 326 predicted in Caenorhabditis elegans, 22 in Drosophila, and at least 38 in humans. F-box proteins often include additional carboxy-terminal motifs capable of protein-protein interaction; the most common secondary motifs in yeast and human F-box proteins are WD repeats and leucine-rich repeats, both of which have been found to bind phosphorylated substrates to the SCF complex. The majority of F-box proteins have other associated motifs, and the functions of most of these proteins have not yet been defined.

Hsu HW et al. (2020) Development "C. elegans flamingo FMI-1 controls dendrite self-avoidance through F-actin assembly."

Syu RT, Hsu HW, Pan CL, Chiang YC, Liao CP

[Development, 2020]

Self-avoidance is a conserved mechanism that prevents crossover between sister dendrites from the same neuron, ensuring proper functioning of the neuronal circuits. Several adhesion molecules are known to be important for dendrite self-avoidance, but the underlying molecular mechanisms are incompletely defined. Here we show that FMI-1/Flamingo, an atypical cadherin, is required autonomously for self-avoidance in the multidendritic PVD neuron of <i>C. elegans</i> The <i>fmi-1</i> mutant shows increased crossover between sister PVD dendrites. Our genetic analysis suggests that FMI-1 promotes transient F-actin assembly at the tips of contacting sister dendrites to facilitate their efficient retraction during self-avoidance events, likely by interacting with WSP-1/N-WASP. Mutations of <i>vang-1</i>, which encodes the planar cell polarity protein Vangl2 previously shown to inhibit F-actin assembly, suppress self-avoidance defects of the <i>fmi-1</i> mutant. FMI-1 downregulates VANG-1 level likely through forming protein complexes. Our study identifies molecular links between Flamingo and the F-actin cytoskeleton for efficient dendrite self-avoidance.

Qiu Z et al. (2019) Front Cell Dev Biol "A Novel Mutation in an NPXY Motif of Integrin Reveals Phenotypes Similar to him-4/hemicentin."

Qiu Z, Lee M, Ahn JH, Yu EJ, Sheesley P

[Front Cell Dev Biol, 2019]

Integrin, an heterodimeric cell surface receptor for the extracellular matrix (ECM), carries two tyrosine phosphorylation motifs in the cytoplasmic tail of the subunit. NPXY (Asn-Pro-x-Tyr) is a conserved tyrosine phosphorylation motif that binds to the phospho-tyrosine binding (PTB) domain. We generated a tyrosine to glutamic acid (E) mutation to modify tyrosine (Y) into a negatively charged amino NPXY in the <i>pat-3</i> integrin of <i>Caenorhabditis elegans</i>. The transgenic rescue animal displayed defects in gonad migration and tail morphology. Also, the mutant animals produced a high number of males, suggesting that the Y to E mutation in <i>pat-3</i> integrin causes a phenotype similar to that of Him mutant. Further analyses revealed that males of <i>pat-3(Y804E)</i> and <i>him-4/</i>hemicentin share additional phenotypes such as abnormal gonad and unsuccessful mating. A <i>pat-3</i> transgenic rescue mutant with a non-polar phenylalanine (F) in NPXY, <i>pat-3(Y792/804F)</i>, suppressed the high male number, defective mating, inviable zygote, and the abnormal gonad of <i>him-4</i> mutants, indicating that Y to F mutation in both NPXY motifs suppressed the <i>him-4</i> phenotypes. This finding supports the idea that the ECM determines the activation state in integrin NPXY motifs; <i>him-4/</i>hemicentin may directly or indirectly interact with integrins and maintain the NPXY non-charged. Our findings provide new insight into a suppressive role of an ECM molecule in integrin NPXY phosphorylation.

Azimi Hashemi N et al. (2019) Proc Natl Acad Sci U S A "Rhodopsin-based voltage imaging tools for use in muscles and neurons of Caenorhabditis elegans."

Liewald JF, Bach M, Azimi Hashemi N, Bergs ACF, Schuler C, Gottschalk A, Scheiwe AR, Steuer Costa W

[Proc Natl Acad Sci U S A, 2019]

Genetically encoded voltage indicators (GEVIs) based on microbial rhodopsins utilize the voltage-sensitive fluorescence of all-<i>trans</i> retinal (ATR), while in electrochromic FRET (eFRET) sensors, donor fluorescence drops when the rhodopsin acts as depolarization-sensitive acceptor. In recent years, such tools have become widely used in mammalian cells but are less commonly used in invertebrate systems, mostly due to low fluorescence yields. We systematically assessed Arch(D95N), Archon, QuasAr, and the eFRET sensors MacQ-mCitrine and QuasAr-mOrange, in the nematode <i>Caenorhabditis elegans</i> ATR-bearing rhodopsins reported on voltage changes in body wall muscles (BWMs), in the pharynx, the feeding organ [where Arch(D95N) showed approximately 128% F/F increase per 100 mV], and in neurons, integrating circuit activity. ATR fluorescence is very dim, yet, using the retinal analog dimethylaminoretinal, it was boosted 250-fold. eFRET sensors provided sensitivities of 45 to 78% F/F per 100 mV, induced by BWM action potentials, and in pharyngeal muscle, measured in simultaneous optical and sharp electrode recordings, MacQ-mCitrine showed approximately 20% F/F per 100 mV. All sensors reported differences in muscle depolarization induced by a voltage-gated Ca²⁺-channel mutant. Optogenetically evoked de- or hyperpolarization of motor neurons increased or eliminated action potential activity and caused a rise or drop in BWM sensor fluorescence. Finally, we analyzed voltage dynamics across the entire pharynx, showing uniform depolarization but compartmentalized repolarization of anterior and posterior parts. Our work establishes all-optical, noninvasive electrophysiology in live, intact <i>C. elegans</i>.

Souza ACR et al. (2018) Genes (Basel) "Pathogenesis of the Candida parapsilosis Complex in the Model Host Caenorhabditis elegans."

Colombo AL, Fuchs BB, Jayamani E, Mylonakis E, Souza ACR, Alves VS

[Genes (Basel), 2018]

<i>Caenorhabditis</i><i>elegans</i> is a valuable tool as an infection model toward the study of <i>Candida</i> species. In this work, we endeavored to develop a <i>C</i>. <i>elegans</i>-<i>Candida</i><i>parapsilosis</i> infection model by using the fungi as a food source. Three species of the C. parapsilosis complex (<i>C.</i><i>parapsilosis</i> (<i>sensu</i><i>stricto</i>), <i>Candida</i><i>orthopsilosis</i> and <i>Candida</i><i>metapsilosis</i>) caused infection resulting in <i>C. elegans</i> killing. All three strains that comprised the complex significantly diminished the nematode lifespan, indicating the virulence of the pathogens against the host. The infection process included invasion of the intestine and vulva which resulted in organ protrusion and hyphae formation. Importantly, hyphae formation at the vulva opening was not previously reported in <i>C</i>. <i>elegans</i>-<i>Candida</i> infections. Fungal infected worms in the liquid assay were susceptible to fluconazole and caspofungin and could be found to mount an immune response mediated through increased expression of <i>cnc</i>-<i>4</i>, <i>cnc</i>-<i>7</i>, and <i>fipr</i><i>-</i><i>22</i>/<i>23</i>. Overall, the <i>C</i>. <i>elegans</i>-<i>C</i>. <i>parapsilosis</i> infection model can be used to model <i>C</i>. <i>parapsilosis</i> host-pathogen interactions.

Wamucho A et al. (2023) Int J Mol Sci "Global DNA Adenine Methylation in Caenorhabditis elegans after Multigenerational Exposure to Silver Nanoparticles and Silver Nitrate."

Tsyusko O, May J, Unrine J, Wamucho A

[Int J Mol Sci, 2023]

Multigenerational and transgenerational reproductive toxicity in a model nematode <i>Caenorhabditis elegans</i> has been shown previously after exposure to silver nanoparticles (Ag-NPs) and silver ions (AgNO₃). However, there is a limited understanding on the transfer mechanism of the increased reproductive sensitivity to subsequent generations. This study examines changes in DNA methylation at epigenetic mark N6-methyl-2'-deoxyadenosine (6mdA) after multigenerational exposure of <i>C. elegans</i> to pristine and transformed-via-sulfidation Ag-NPs and AgNO₃. Levels of 6mdA were measured as 6mdA/dA ratios prior to <i>C. elegans</i> exposure (F₀) after two generations of exposure (F₂) and two generations of rescue (F₄) using high-performance liquid chromatography with tandem mass spectrometry (LC-MS/MS). Although both AgNO₃ and Ag-NPs induced multigenerational reproductive toxicity, only AgNO₃ exposure caused a significant increase in global 6mdA levels after exposures (F₂). However, after two generations of rescue (F₄), the 6mdA levels in AgNO₃ treatment returned to F₀ levels, suggesting other epigenetic modifications may be also involved. No significant changes in global DNA methylation levels were observed after exposure to pristine and sulfidized sAg-NPs. This study demonstrates the involvement of an epigenetic mark in AgNO₃ reproductive toxicity and suggests that AgNO₃ and Ag-NPs may have different toxicity mechanisms.