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Inhibition of human dyskerin as a new approach to target ribosome biogenesis

Academic Article
Publication Date:
2014
abstract:
The product of the DKC1 gene, dyskerin, is required for both ribosome biogenesis and telomerase complex stabilization. Targeting these cellular processes has been explored for the development of drugs to selectively or preferentially kill cancer cells. Presently, intense research is conducted involving the identification of new biological targets whose modulation may simultaneously interfere with multiple cellular functions that are known to be hyper-activated by neoplastic transformations. Here, we report, for the first time, the computational identification of small molecules able to inhibit dyskerin catalytic activity. Different in silico techniques were applied to select compounds and analyze the binding modes and the interaction patterns of ligands in the human dyskerin catalytic site. We also describe a newly developed and optimized fast real-time PCR assay that was used to detect dyskerin pseudouridylation activity in vitro. The identification of new dyskerin inhibitors constitutes the first proof of principle that the pseudouridylation activity can be modulated by means of small molecule agents. Therefore, the presented results, obtained through the usage of computational tools and experimental validation, indicate an alternative therapeutic strategy to target ribosome biogenesis pathway. © 2014 Rocchi et al.
Iris type:
01.01 Articolo in rivista
List of contributors:
DEL RIO, Alberto; Zamboni, Roberto
Handle:
https://iris.cnr.it/handle/20.500.14243/224437
Published in:
PLOS ONE
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http://www.scopus.com/record/display.url?eid=2-s2.0-84904268446&origin=inward
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