Phenotypic Switching of Nonpeptidergic Cutaneous Sensory Neurons following Peripheral Nerve Injury

In adult mammals, the phenotype of half of all pain-sensing (nociceptive) sensory neurons is tonically modulated by growth factors in the glial cell line-derived neurotrophic factor (GDNF) family that includes GDNF, artemin (ARTN) and neurturin (NRTN). Each family member binds a distinct GFRα family co-receptor, such that GDNF, NRTN and ARTN bind GFRα1, -α2, and -α3, respectively. Previous studies revealed transcriptional regulation of all three receptors in following axotomy, possibly in response to changes in growth factor availability. Here, we examined changes in the expression of GFRα1-3 in response to injury in vivo and in vitro. We found that after dissociation of adult sensory ganglia, up to 27% of neurons die within 4 days (d) in culture and this can be prevented by nerve growth factor (NGF), GDNF and ARTN, but not NRTN. Moreover, up-regulation of ATF3 (a marker of neuronal injury) in vitro could be prevented by NGF and ARTN, but not by GDNF or NRTN. The lack of NRTN efficacy was correlated with rapid and near-complete loss of GFRα2 immunoreactivity. By retrogradely-labeling cutaneous afferents in vivo prior to nerve cut, we demonstrated that GFRα2-positive neurons switch phenotype following injury and begin to express GFRα3 as well as the capsaicin receptor, transient receptor potential vanilloid 1(TRPV1), an important transducer of noxious stimuli. This switch was correlated with down-regulation of Runt-related transcription factor 1 (Runx1), a transcription factor that controls expression of GFRα2 and TRPV1 during development. These studies show that NRTN-responsive neurons are unique with respect to their plasticity and response to injury, and suggest that Runx1 plays an ongoing modulatory role in the adult

The role of GDNF family ligand signalling in the differentiation of sympathetic and dorsal root ganglion neurons

The diversity of neurons in sympathetic ganglia and dorsal root ganglia (DRG) provides intriguing systems for the analysis of neuronal differentiation. Cell surface receptors for the GDNF family ligands (GFLs) glial cell-line-derived neurotrophic factor (GDNF), neurturin and artemin, are expressed in subpopulations of these neurons prompting the question regarding their involvement in neuronal subtype specification. Mutational analysis in mice has demonstrated the requirement for GFL signalling during embryonic development of cholinergic sympathetic neurons as shown by the loss of expression from the cholinergic gene locus in ganglia from mice deficient for ret, the signal transducing subunit of the GFL receptor complex. Analysis in mutant animals and transgenic mice overexpressing GFLs demonstrates an effect on sensitivity to thermal and mechanical stimuli in DRG neurons correlating at least partially with the altered expression of transient receptor potential ion channels and acid-sensitive cation channels. Persistence of targeted cells in mutant ganglia suggests that the alterations are caused by differentiation effects and not by cell loss. Because of the massive effect of GFLs on neurite outgrowth, it remains to be determined whether GFL signalling acts directly on neuronal specification or indirectly via altered target innervation and access to other growth factors. The data show that GFL signalling is required for the specification of subpopulations of sensory and autonomic neurons. In order to comprehend this process fully, the role of individual GFLs, the transduction of the GFL signals, and the interplay of GFL signalling with other regulatory pathways need to be deciphered

Long Non-coding RNAs in a Single-Cell Type: Function and Subcellular Localization

After the conclusion of the human genome project, the annotated genes varied among 26,000 and 39,000. However, this gene count is significantly smaller than what was observed later in 2012 when it was evidenced that most of the human genome is transcribed. The vast majority of the transcribed genome does not code for translated RNAs that are involved in the protein synthesis, but comprises non-coding RNAs. This is true not only for the human genome but also for most of the mammalian genomes. Among non-coding RNAs, the most abundant are long non-coding RNAs (lncRNAs). They are emerging as important players in the regulation of several aspects of cellular biology. For instance, they are involved in cell differentiation, normal functioning of differentiated cells, and also involved in the development of pathological conditions such as tumors. They present an expression that is more cell-specific than coding RNAs and for this reason, it is important to study them in single cells instead of using bulk tissues or a cell population. Recent improvements in techniques that allow genomic and transcriptomic analyses of single cells and those for fluorescence amplification have given a considerable boost in the comprehension of cell specificity, subcellular localization, and function of lncRNAs. The purpose of this chapter is to discuss different methods that are available to detect RNA expression using a single cell approach evidencing the advantages and disadvantages of each of them. We will consider how the analysis of single cells has contributed to the better comprehension of lncRNA functions and how it was involved in proposing new paradigms. To conclude the chapter, we will consider published databases to retrieve information on genomic and transcriptomic experiments on single cells