Human Molecular Genetics, Vol 8, 1417-1424, Copyright © 1999 by Oxford University Press
C Guiducci, F Ascenzioni, C Auriche, E Piccolella, AM Guerrini and P Donini
A natural human minichromosome (MC1) derived from human chromosome 1 was
shown to be linear and to have a size of 5.5 Mb. Human IL-2 cDNA and the
neo gene were co-transfected into a MC1-containing human-CHO hybrid cell
line. Integration of the foreign genes was directed to the pericentromeric
region of MC1 by co-transfection of chromosome 1- specific satellite 2 DNA.
A number of G418-resistant transfectants were obtained and expression of
IL-2 was determined. FISH analysis demonstrated co-localization in the
minichromosome of the IL-2 gene and of the satellite 2 DNA. An
IL-2-producing clone was used in cell fusion experiments with
IL-2-dependent murine CTLL cells to generate CTLL- human hybrids containing
the modified minichromosome (MC1- IL2 ). The hybrids were able to grow in
medium lacking IL-2 for 17 mean population doublings (MPD), indicating that
expression of the cytokine was sufficient to relieve the IL-2 dependence of
CTLL proliferation. Endogenous IL-2 production delayed the onset of
apoptosis in the IL-2- dependent CTLL cells. Mitotic stability was shown to
be 100% in the human-CHO hybrids and 97% per MPD in CTLL cells. These
results demonstrate that a natural human minichromosome can be utilized as
a cloning and expression vector for mammalian cells and that the MC1
minichromosome can be engineered to deliver IL-2 to two types of cells,
fibroblasts and lymphocytes.
ARTICLES
Use of a human minichromosome as a cloning and expression vector for mammalian cells
Istituto Pasteur-Fondazione Cenci Bolognetti, c/o Dipartimento di Biologia Cellulare e dello Sviluppo, Universita 'La Sapienza', Via degli Apuli 1, 00185 Roma, Italy.
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