4.4 Article

Viral Vector-Based Evaluation of Regulatory Regions in the Neuron-Specific Enolase (NSE) Promoter in Mouse Cerebellum In Vivo

期刊

CEREBELLUM
卷 16, 期 5-6, 页码 913-922

出版社

SPRINGER
DOI: 10.1007/s12311-017-0866-5

关键词

Neuron-specific enolase; Promoter; AAV vector; Viral vector; Purkinje cell; Interneuron

资金

  1. Ministry of Education, Culture, and Sports Science (MEXT)
  2. Japan Agency for Medical Research and Development (AMED)
  3. Gunma University Initiative for Advanced Research (GIAR)
  4. JSPS KAKENHI [15K18330]
  5. Grants-in-Aid for Scientific Research [15K18330, 16K15477] Funding Source: KAKEN

向作者/读者索取更多资源

We investigated the neuron-specific enolase (NSE) promoter in terms of its promoter strength and neuronal specificity in the cerebellum in vivo. The 1.8 kb rat NSE promoter was divided into three regions, A (0.8 kb), B (0.7 kb), and C (0.3 kb), starting from the 5' side. Then, we made various deletion constructs and assessed them by virally expressing GFP under the control of one of the deleted promoters. Removing region A reduced GFP expression to similar to 6% of that of the original 1.8 kb promoter. Further deletion of region B (presence of region C alone) did not influence the promoter strength, but removing region B from the original 1.8 kb promoter reduced the GFP expression to similar to 6% of the original level, similar to the level observed after deletion of region A. Immunohistochemistry showed robust GFP expression in Purkinje cells and modest expression in interneurons by the original promoter. Removing region A and/or region B abolished the GFP expression in Purkinje cells in most cerebellar lobules, with the expression in interneurons almost unchanged. These results suggest that region C, which is a proximal 0.3 kb sequence, contains cis-acting elements that drive transcription predominantly in interneurons. The addition of either region A or B onto region C does not alter the promoter properties; however, the addition of both regions A and B to region C drastically enhanced the promoter activity in Purkinje cells, suggesting the synergistic action of cis-acting regulatory elements in regions A and B for strong activation in Purkinje cells.

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