Abstract

While the mature central nervous system has an overall diminished capacity for regrowth compared to an embryonic nervous system, axonal regeneration of some populations is possible when they are provided with a potently growth-permissive environment, such as one conferred by a peripheral nerve graft (PNG). Still, axons that are capable of regenerating into the graft fail to grow beyond the PNG to reinnervate spinal cord, at least partly because of the presence of the inhibitory glial scar that is present at the graft-host interface. Digesting the inhibitory extracellular matrix within the scar with chondroitinase ABC (ChABC) allows some axons to traverse the distal interface, synapse upon distal neurons, and mediate some behavioral recovery. Nonetheless, most of the axons remain in the graft. Thus it is important to develop strategies that enhance the ability of axons to regenerate out of a graft in order to increase their potential to improve function. We have preliminary data indicating that expressing constitutively active Rheb (caRheb) - a GTPase that is a critical regulatory component of protein synthesis - in adult neurons results in robust axonal outgrowth in an in vitro glial scar model and in vivo after SCI.
In Aim 1, we will test the hypothesis that expressing caRheb after SCI will enhance regeneration into and beyond a PNG. We will use histological, physiological, and behavioral analyses to examine if caRheb augments axonal regeneration - especially following ChABC treatment of the distal graft interface - and if these regenerated axons form functional synapses that facilitate behavioral recovery. Any regeneration is irrelevant if these axons do not integrate into circuits. Though ChABC enhances plasticity, ChABC-induced sprouted/regenerated fibers do not always form synapses to impact function. Thus, it is also important to devise strategies to improve integration of these axons (i.. synaptogenesis) in order to exploit regrowth that we encourage. We recently demonstrated the proof-of-principle that providing a single exogenous factor enhances the integration of axons that regenerate out of a PNG. Recent work indicates that secreted glypican is sufficient to promote functional, excitatory synapse formation in vitro and behavioral recovery in a cerebral ischemia model in vivo.
In Aim 2, we will test the hypothesis that providing exogenous glypican will enhance synaptogenesis of regenerated axons following SCI. We will graft a PNG into a SCI site that has been treated with ChABC to promote axonal regeneration. We will determine if infusing exogenous glypican into tissue surrounding the SCI site enhances synaptogenesis of these regenerated axons upon neurons distal to the PNG. We will gauge improvements in functional synapse formation physiologically and histologically by examining the colocalization of pre- and postsynaptic markers. We will also assess if enhanced synapse formation correlates with behavioral recovery. Because the strategies to be tested in Aims 1 and 2 take different approaches - enhancing the growth response and synaptogenesis, respectively - to promote functional repair after SCI, it is possible that even if the results in the previous Aims are incremental, combining the two approaches will lead to greater recovery than either alone.
In Aim 3, we will use a novel, multipronged strategy to fill the lesion cavity with a growth-promoting substrate (PNG), enhance the growth response (caRheb), modulate the inhibitory properties of the glial scar (ChABC) and promote synaptogenesis (glypican). We will use histological and physiological analyses to examine if glypican enhances the functional integration of axonal regeneration beyond a ChABC-treated PNG interface that is induced by expressing caRheb and if this results in more robust behavioral recovery than what occurs with either caRheb or glypican treatment separately. These data will identify new therapeutic strategies that may eventually be translated to clinical use to improve the quality of life of persons with SCI.

Public Health Relevance

Spinal cord injury (SCI) affects 1.3 million Americans. Because adult central nervous system axons fail to regenerate following injury, severed axons are permanently disconnected from their target neurons, resulting in the lasting loss of motor and/or sensory function. The proposed experiments in this application are relevant to public health because they will test whether a unique multi-faceted approach that simultaneously provides a growth-permissive substrate, mitigates the hostile inhibitory environment of the glial scar, enhances the axonal growth response, and promotes synaptogenesis facilitates functional axonal regeneration. The strategies have the potential to be translated to clinical application to improve the quality of life for persons who sustained SCI.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Neurological Disorders and Stroke (NINDS)
Type
Research Project (R01)
Project #
5R01NS085426-03
Application #
9057394
Study Section
Clinical Neuroplasticity and Neurotransmitters Study Section (CNNT)
Program Officer
Jakeman, Lyn B
Project Start
2014-05-01
Project End
2019-04-30
Budget Start
2016-05-01
Budget End
2017-04-30
Support Year
3
Fiscal Year
2016
Total Cost
Indirect Cost

  Institution

Name
Drexel University
Department
Anatomy/Cell Biology
Type
Schools of Medicine
DUNS #
002604817
City
Philadelphia
State
PA
Country
United States
Zip Code
19102

  Publications

Hou, Shaoping; Saltos, Tatiana M; Iredia, Idiata W et al. (2018) Surgical techniques influence local environment of injured spinal cord and cause various grafted cell survival and integration. J Neurosci Methods 293:144-150
Ahn, Jemin; Saltos, Tatiana M; Tom, Veronica J et al. (2018) Transsynaptic tracing to dissect supraspinal serotonergic input regulating the bladder reflex in rats. Neurourol Urodyn 37:2487-2494
Mironets, Eugene; Osei-Owusu, Patrick; Bracchi-Ricard, Valerie et al. (2018) Soluble TNF? Signaling within the Spinal Cord Contributes to the Development of Autonomic Dysreflexia and Ensuing Vascular and Immune Dysfunction after Spinal Cord Injury. J Neurosci 38:4146-4162
Wu, Di; Klaw, Michelle C; Connors, Theresa et al. (2017) Combining Constitutively Active Rheb Expression and Chondroitinase Promotes Functional Axonal Regeneration after Cervical Spinal Cord Injury. Mol Ther 25:2715-2726
Mironets, Eugene; Wu, Di; Tom, Veronica J (2016) Manipulating extrinsic and intrinsic obstacles to axonal regeneration after spinal cord injury. Neural Regen Res 11:224-5
Wu, Di; Klaw, Michelle C; Kholodilov, Nikolai et al. (2016) Expressing Constitutively Active Rheb in Adult Dorsal Root Ganglion Neurons Enhances the Integration of Sensory Axons that Regenerate Across a Chondroitinase-Treated Dorsal Root Entry Zone Following Dorsal Root Crush. Front Mol Neurosci 9:49
Hou, Shaoping; Carson, David M; Wu, Di et al. (2016) Dopamine is produced in the rat spinal cord and regulates micturition reflex after spinal cord injury. Exp Neurol 285:136-146
Partida, Elizabeth; Mironets, Eugene; Hou, Shaoping et al. (2016) Cardiovascular dysfunction following spinal cord injury. Neural Regen Res 11:189-94
Wu, Di; Klaw, Michelle C; Connors, Theresa et al. (2015) Expressing Constitutively Active Rheb in Adult Neurons after a Complete Spinal Cord Injury Enhances Axonal Regeneration beyond a Chondroitinase-Treated Glial Scar. J Neurosci 35:11068-80
Xu, Chen; Klaw, Michelle C; Lemay, Michel A et al. (2015) Pharmacologically inhibiting kinesin-5 activity with monastrol promotes axonal regeneration following spinal cord injury. Exp Neurol 263:172-6