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Using RNA-sequencing to detect novel splice variants related to drug resistance in in vitro cancer models

Articolo
Data di Pubblicazione:
2016
Abstract:
Drug resistance remains a major problem in the treatment of cancer for both hematological malignancies and solid tumors. Intrinsic or acquired resistance can be caused by a range of mechanisms, including increased drug elimination, decreased drug uptake, drug inactivation and alterations of drug targets. Recent data showed that other than by well-known genetic (mutation, amplification) and epigenetic (DNA hypermethylation, histone post-translational modification) modifications, drug resistance mechanisms might also be regulated by splicing aberrations. This is a rapidly growing field of investigation that deserves future attention in order to plan more effective therapeutic approaches. The protocol described in this paper is aimed at investigating the impact of aberrant splicing on drug resistance in solid tumors and hematological malignancies. To this goal, we analyzed the transcriptomic profiles of several in vitro models through RNA-seq and established a qRT-PCR based method to validate candidate genes. In particular, we evaluated the differential splicing of DDX5 and PKM transcripts. The aberrant splicing detected by the computational tool MATS was validated in leukemic cells, showing that different DDX5 splice variants are expressed in the parental vs. resistant cells. In these cells, we also observed a higher PKM2/PKM1 ratio, which was not detected in the Panc-1 gemcitabineresistant counterpart compared to parental Panc-1 cells, suggesting a different mechanism of drug-resistance induced by gemcitabine exposure.
Tipologia CRIS:
01.01 Articolo in rivista
Keywords:
Alternative splicing; Cancer research; Chemotherapy; Cytotoxicity; Issue 118; Resistance; RNA-seq; Transcriptomics
Elenco autori:
Giovannetti, Elisa
Link alla scheda completa:
https://iris.cnr.it/handle/20.500.14243/329108
Pubblicato in:
JOURNAL OF VISUALIZED EXPERIMENTS
Journal
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http://www.scopus.com/inward/record.url?eid=2-s2.0-85008653882&partnerID=q2rCbXpz
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