Independent regulation of mouse VL30 retrotransposon expression in response to serum and oncogenic cell transformation

doi:10.1093/nar/18.8.2069

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Nucleic Acids Research, 1990, Vol. 18, No. 8 2069-2077
© 1990

MOLECULAR BIOLOGY

Independent regulation of mouse VL30 retrotransposon expression in response to serum and oncogenic cell transformation

Lynne Eaton and John D. Norton^*

Department of Haematology, Royal Free Hospital School of Medicine Pond Street, London NW3 2QG, UK

^* To whom correspondence should be addressed

Received December 20, 1989. Revised March 26, 1990. Accepted March 26, 1990.

The nucleotide sequence of the long terminal repeats (LTRs)of retrovirus-transmissible mouse VL30 cDNA clones, NVL-1 andNVL-2 were determined and compared with that of the prototypeNVL-3. Both shared the typical U3 R U5 structure together withunusual features of redundancy in the tRNA^gty primer bindingsite and adjacent inverted repeat. NVL-1 and NVL-2 LTRs werealmost identical and differed from the NVL-3 LTR in the U3 domainharbouring transcriptional regulatory determinants. S1 nucleaseanalysis of cellular and virus-encapsidated RNA suggested thatNVL-1/2 and NVL-3 elements retrotranspose with comparable efficiencybut that in contrast to transformation-regulated VL30 expressionwhich affects all types of NVL element, only NVL-1/2 elementswere found to be serum responsive. Both modes of VL30 regulationwere found to be coupled through protein kinase C-independentpathways. Expression of N-ras transactivated U3 enhancer determinantsin all classes of LTR. However the same region of NVL-1/2 LTRdid not confer serum responsiveness implying that cis regulatorydeterminants of VL30 elements mediating growth factor responsivenessare at least in part dissociable from those responsible forcell transformation-regulated expression.

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