AI Article Synopsis

  • The main olfactory system in mice uses approximately 1,100 odorant receptor genes to help millions of olfactory sensory neurons communicate scents, which converge into around 3,600 glomeruli in the olfactory bulb.
  • The study involved counting all fluorescently tagged olfactory sensory neurons across 15 gene-targeted strains to better understand their distribution, resulting in a total cell count of 685,673 across 56 mice.
  • The researchers found significant variability in olfactory sensory neuron numbers among different odorant receptor genes and established a strong link between the number of olfactory sensory neurons and the total volume of the glomeruli formed by their axons, suggesting volume measurement could serve as a proxy for estimating these neuron counts.

Article Abstract

Chemosensory specificity in the main olfactory system of the mouse relies on the expression of ∼1,100 odorant receptor (OR) genes across millions of olfactory sensory neurons (OSNs) in the main olfactory epithelium (MOE), and on the coalescence of OSN axons into ∼3,600 glomeruli in the olfactory bulb. A traditional approach for visualizing OSNs and their axons consists of tagging an OR gene genetically with an axonal marker that is cotranslated with the OR by virtue of an internal ribosome entry site (IRES). Here we report full cell counts for 15 gene-targeted strains of the OR-IRES-marker design coexpressing a fluorescent protein. These strains represent 11 targeted OR genes, a 1% sample of the OR gene repertoire. We took an empirical, "count every cell" strategy: we counted all fluorescent cell profiles with a nuclear profile within the cytoplasm, on all serial coronal sections under a confocal microscope, a total of 685,673 cells in 56 mice at postnatal day 21. We then applied a strain-specific Abercrombie correction to these OSN counts in order to obtain a closer approximation of the true OSN numbers. We found a 17-fold range in the average (corrected) OSN number across these 11 OR genes. In the same series of coronal sections, we then determined the total volume of the glomeruli (TGV) formed by coalescence of the fluorescent axons. We found a strong linear correlation between OSN number and TGV, suggesting that TGV can be used as a surrogate measurement for estimating OSN numbers in these gene-targeted strains.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC4758392PMC
http://dx.doi.org/10.1002/cne.23835DOI Listing

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