Marked inhibition of glioblastoma target cell tumorigenicity in vitro by retrovirus-mediated transfer of a hairpin ribozyme against deletion-mutant epidermal growth factor receptor messenger RNA

The goal of this study was to evaluate the activity of certain hairpin ribozymes against deletion-mutant epidermal growth factor receptor (deltaEGFR) messenger (m)RNA in glioblastomas multiforme (GBMs). A distinct 801-bp deletion mutation associated with amplification of the EGFR gene is present in...

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Published in:	Journal of neurosurgery Vol. 92; no. 2; pp. 297 - 305
Main Authors:	HALATSCH, M.-E, SCHMIDT, U, BÖTEFÜR, I. C, HOLLAND, J. F, OHNUMA, T
Format:	Journal Article
Language:	English
Published:	Park Ridge, IL American Association of Neurological Surgeons 01-02-2000
Subjects:	Base Sequence Biological and medical sciences Brain Neoplasms - genetics Brain Neoplasms - therapy Cell Transformation, Neoplastic - genetics Chromosome Deletion DNA Mutational Analysis Genetic Therapy - methods Genetic Vectors - genetics Glioblastoma - genetics Glioblastoma - therapy Humans In Vitro Techniques Medical sciences Molecular Sequence Data Moloney murine leukemia virus - genetics Neurology Polymerase Chain Reaction Receptor, Epidermal Growth Factor - genetics RNA, Catalytic - genetics RNA, Messenger - genetics Tumor Cells, Cultured Tumor Stem Cell Assay Tumors of the nervous system. Phacomatoses Human Nervous system diseases Ribozyme Cytokine Exploration Receiver Malignant tumor Gene expression Glioblastoma multiforme Malignant glioma Epidermal growth factor Cell line Messenger RNA Polypeptide Central nervous system disease Growth factor
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Summary:	The goal of this study was to evaluate the activity of certain hairpin ribozymes against deletion-mutant epidermal growth factor receptor (deltaEGFR) messenger (m)RNA in glioblastomas multiforme (GBMs). A distinct 801-bp deletion mutation associated with amplification of the EGFR gene is present in a large subgroup of primary GBMs and confers enhanced tumorigenicity in vivo. As a result of the deletion mutation, the fusion junction of the gene is created directly upstream of a GTA triplet, which is subsequently transcribed into a ribozyme target codon (GUA). In attempts to intercept deltaEGFR gene expression at the mRNA level, the authors designed three different hairpin ribozymes derived from the negative strands of satellite RNAs in tobacco ringspot virus, chicory yellow mottle virus (sCYMV1), and arabis mosaic virus against this target and evaluated their efficiency and specificity in a cell-free system. The sCYMV1, identified as the most active anti-deltaEGFR hairpin ribozyme motif, was cloned into the retroviral plasmid N2A+tRNAi(met). High-titer recombinant retrovirus-containing supernatants (> 10(5) colony-forming units/ml) derived from an amphotropic GP+envAM 12 packaging cell line transfected with the N2A+tRNAi(met)-anti-deltaEGFR-sCYMV1 construct were used to introduce the sCYMV1 hairpin ribozyme into U-87MG.deltaEGFR glioblastoma cells, which overexpress exogenous deltaEGFR. Using a virus/target cell ratio of 40:1 in the absence of drug selection, the ribozyme transfer resulted in a greater than 90% reduction of deltaEGFR mRNA levels, a 69% inhibition of deltaEGFR-mediated proliferation advantage, and a greater than 95% decrease of colony formation in soft agar under relative serum starvation conditions in vitro; transfer of a control mutant ribozyme that was rendered incapable of cleaving its target yielded none of these effects. These findings indicate that the anti-deltaEGFR-sCYMV1 hairpin ribozyme is capable of specifically inhibiting the expression of deltaEGFR and reversing the deltaEGFR-associated malignant phenotype of GBM cells. This strategy may constitute a promising gene therapy approach for a molecularly defined subgroup of GBMs.
Bibliography:	ObjectType-Article-1 SourceType-Scholarly Journals-1 ObjectType-Feature-2 content type line 23
ISSN:	0022-3085 1933-0693
DOI:	10.3171/jns.2000.92.2.0297