Literature DB >> 2987925

Isolation of a gene enhancer within an amplified inverted duplication after "expression selection".

M Ford, B Davies, M Griffiths, J Wilson, M Fried.   

Abstract

We have attempted to isolate and identify cellular expression sequences from F9 teratocarcinoma DNA by utilizing their ability to reactivate a selectable gene devoid of its own expression sequences (expression selection). Restriction nuclease-digested F9 cellular DNA was ligated to a polyoma virus (Py) DNA fragment which contains an intact transforming region but is incapable of inducing transformation because it lacks the viral 5' enhancer sequence. The ligation mixture was used to transfect Rat-1 cells and a transformed cell line, 3B, was isolated. The 3B cell line contained a single type of Py DNA insert, which was molecularly cloned as an 18-kilobase BglII fragment. A weak cellular enhancer was identified in a 4.7-kilobase BamHI fragment upstream from the Py sequences. Both the Py DNA and the enhancer sequences were found to be present in an inverted duplication in the 3B clone. The presence of this structure in 3B genomic DNA was confirmed by the analysis of selectively isolated inverted duplicated sequences, and the structure was found to be at least 22 kilobases long. In the 3B cell line, the inverted duplicated sequences containing the Py and enhancer sequences are quite stable and are amplified 20- to 40-fold. The strongly transformed phenotype of the 3B cells may be a result of this amplification. The formation of inverted duplications as a part of the amplification mechanism as well as a general strategy for the cloning of inverted duplicated (amplified) sequences is discussed.

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Year:  1985        PMID: 2987925      PMCID: PMC397777          DOI: 10.1073/pnas.82.10.3370

Source DB:  PubMed          Journal:  Proc Natl Acad Sci U S A        ISSN: 0027-8424            Impact factor:   11.205


  10 in total

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Authors:  M Fried; M Griffiths; B Davies; G Bjursell; G La Mantia; L Lania
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8.  The isolation of structural genes from libraries of eucaryotic DNA.

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9.  A small segment of polyoma virus DNA enhances the expression of a cloned beta-globin gene over a distance of 1400 base pairs.

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  10 in total
  23 in total

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2.  Formation of large palindromic DNA by homologous recombination of short inverted repeat sequences in Saccharomyces cerevisiae.

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3.  The use of 5-azacytidine to increase cleavage of methylation sensitive rare cutting restriction enzymes sites in amplified DNA.

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Review 4.  Mechanisms of gene duplication and amplification.

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5.  Large inverted duplications in amplified DNA of mammalian cells form hairpins in vitro upon DNA extraction but not in vivo.

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7.  Gene activation properties of a mouse DNA sequence isolated by expression selection.

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8.  Charomids: cosmid vectors for efficient cloning and mapping of large or small restriction fragments.

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9.  Hairpin structures are the primary amplification products: a novel mechanism for generation of inverted repeats during gene amplification.

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10.  MYCN is retained in single copy at chromosome 2 band p23-24 during amplification in human neuroblastoma cells.

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