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Ablation of central nervous system progenitor cells in transgenic rats using bacterial nitroreductase system

โœ Scribed by Seung P. Kwak; Jessica E. Malberg; David S. Howland; Ke-Yi Cheng; Jianying Su; Yin She; Myles Fennell; Afshin Ghavami


Publisher
John Wiley and Sons
Year
2007
Tongue
English
Weight
503 KB
Volume
85
Category
Article
ISSN
0360-4012

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โœฆ Synopsis


Abstract

Specific ablation of central nervous system (CNS) progenitor cells in the brain of live animals is a powerful method to determine the functions of these cells and to reveal novel avenues for the treatment of several CNSโ€related disorders. To achieve this goal, we generated a line of transgenic rats expressing a bacterial enzyme, Escherichia coli nitroreductase gene (NTR), under control of the nestin promoter. In this system, NTR^+^ cells are selectively eliminated upon application of prodrug CB1954, through activation of programmed cell death machineries. At 5 days of age, which is a time when cerebellar development is occurring, transgenic rats bearing the nestinโ€NTR/green fluorescent protein (GFP) gene are overtly normal and express NTR/GFP in neuronal stem cells, without any toxicity in these cells. The functional consequence of progenitor cell ablation was demonstrated by administering prodrug CB1954 into the cerebellum at this 5โ€day time point. Stem cell ablation in these neonates resulted in sensorimotor abnormalities, cerebellar degeneration, overall reduction in cerebellar seize, and manifestation of ataxia. In adult rats, GFP expression was not seen in the hippocampal progenitor cells and seen only at very low levels in the lateral ventricles, indicating a different NTR/GFP expression pattern between neonates and adults. In addition, application of CB1954 by intraventricular delivery reduced the number of 5โ€bromoโ€2โ€ฒโ€deoxyuridineโ€labeled proliferating cells in the lateral ventricle but not hippocampus of NTR/GFP rats. These findings shows that targeted expression of NTR under a specific promoter might be of significant value in addressing the function of distinct cell population in vivo. ยฉ 2007 Wileyโ€Liss, Inc.


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