Imaging axon regeneration within synthetic nerve conduits

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作者
Barbara Fogli
Nikky Corthout
Axelle Kerstens
Frank Bosse
Lars Klimaschewski
Sebastian Munck
Rüdiger Schweigreiter
机构
[1] Innsbruck Medical University,
[2] Department of Anatomy,undefined
[3] Histology and Embryology,undefined
[4] Division of Neuroanatomy,undefined
[5] VIB-KU Leuven Center for Brain & Disease Research O&N 4,undefined
[6] Campus Gasthuisberg,undefined
[7] KU Leuven,undefined
[8] Department for Neuroscience,undefined
[9] Campus Gasthuisberg,undefined
[10] VIB Bio Imaging Core,undefined
[11] Campus Gasthuisberg,undefined
[12] Heinrich-Heine-University Düsseldorf,undefined
[13] Department of Neurology,undefined
[14] Molecular Neurobiology Laboratory,undefined
[15] Innsbruck Medical University,undefined
[16] Biocenter,undefined
[17] Division of Neurobiochemistry,undefined
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摘要
While axons within the central nervous system (CNS) do not regenerate following injury, those in the peripheral nervous system (PNS) do, although not in a clinically satisfactory manner as only a small proportion of axons exhibit long-distance regeneration. Moreover, functional recovery is hampered by excessive axonal sprouting and aberrant reinnervation of target tissue. In order to investigate the mechanisms governing the regrowth of axons following injury, previous studies have used lesion paradigms of peripheral nerves in rat or mouse models, and reagents or cells have been administered to the lesion site through nerve conduits, aiming to improve early-stage regeneration. Morphological analysis of such in vivo experiments has however been limited by the incompatibility of synthetic nerve conduits with existing tissue-clearing and imaging techniques. We present herein a novel experimental approach that allows high-resolution imaging of individual axons within nerve conduits, together with quantitative assessment of fiber growth. We used a GFP-expressing mouse strain in a lesion model of the sciatic nerve to describe a strategy that combines nerve clearing, chemical treatment of chitosan nerve conduits, and long working distance confocal microscopy with image processing and analysis. This novel experimental setup provides a means of documenting axon growth within the actual conduit during the critical initial stage of regeneration. This will greatly facilitate the development and evaluation of treatment regimens to improve axonal regeneration following nerve damage.
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