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  Identification of regeneration-associated genes after central and peripheral nerve injury in the adult rat

Schmitt, A. B., Breuer, S., Liman, J., Buss, A., Schlangen, C., Pech, K., et al. (2003). Identification of regeneration-associated genes after central and peripheral nerve injury in the adult rat. BMC Neuroscience, 4: 8. doi:0.1186/1471-2202-4-8.

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1471-2202-4-8[1].pdf (Any fulltext), 648KB
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Schmitt, A. B.1, Author
Breuer, S.1, Author
Liman, J.1, Author
Buss, A.1, Author
Schlangen, C.1, Author
Pech, K.1, Author
Hol, E. M.1, Author
Brook, G. A.1, Author
Noth, J.1, Author
Schwaiger, F. W.2, Author           
Affiliations:
1Univ Aachen, Sch Med, Dept Neurol, D-52057 Aachen, Germany.; Netherlands Inst Brain Res, NL-1105 AZ Amsterdam, Netherlands., ou_persistent22              
2Emeritus Group: Neuromorphology / Kreutzberg, MPI of Neurobiology, Max Planck Society, ou_1113551              

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 Abstract: Background: It is well known that neurons of the peripheral nervous system have the capacity to regenerate a severed axon leading to functional recovery, whereas neurons of the central nervous system do not regenerate successfully after injury. The underlying molecular programs initiated by axotomized peripheral and central nervous system neurons are not yet fully understood.Results: To gain insight into the molecular mechanisms underlying the process of regeneration in the nervous system, differential display polymerase chain reaction has been used to identify differentially expressed genes following axotomy of peripheral and central nerve fibers. For this purpose, axotomy induced changes of regenerating facial nucleus neurons, and non-regenerating red nucleus and Clarke's nucleus neurons have been analyzed in an intra-animal side-to-side comparison. One hundred and thirty five gene fragments have been isolated, of which 69 correspond to known genes encoding for a number of different functional classes of proteins such as transcription factors, signaling molecules, homeobox-genes, receptors and proteins involved in metabolism. Sixty gene fragments correspond to genomic mouse sequences without known function. In situ-hybridization has been used to confirm differential expression and to analyze the cellular localization of these gene fragments. Twenty one genes (similar to 15%) have been demonstrated to be differentially expressed.Conclusions: The detailed analysis of differentially expressed genes in different lesion paradigms provides new insights into the molecular mechanisms underlying the process of regeneration and may lead to the identification of genes which play key roles in functional repair of central nervous tissues.

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Language(s): eng - English
 Dates: 2003-05-19
 Publication Status: Issued
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 Identifiers: eDoc: 127675
ISI: 000185761400001
DOI: 0.1186/1471-2202-4-8
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Title: BMC Neuroscience
Source Genre: Journal
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Publ. Info: BioMed Central
Pages: - Volume / Issue: 4 Sequence Number: 8 Start / End Page: - Identifier: ISSN: 1471-2202
CoNE: https://pure.mpg.de/cone/journals/resource/111000136905018