Literature DB >> 1648753

Induction of chromosome damage by restriction enzymes during mitosis.

W F Morgan1, E R Valcarcel, E Abella Columna, R A Winegar, B L Yates.   

Abstract

Once electroporated into the nucleus of eukaryotic cells, restriction enzymes will bind at specific DNA sequences and cleave DNA to make double-strand breaks. These induced breaks can lead to chromosome aberrations and consequently offer one approach to determining the mechanism(s) of aberration formation. Because the higher-order structure of DNA in eukaryotic cells might influence the ability of restriction enzymes to locate their recognition sequence, bind, and cleave DNA, we have investigated whether enzymes will cut DNA during metaphase when the chromosomes are most condensed. Chinese hamster ovary cells synchronized in mitosis and treated with either AluI or Sau3AI showed few chromosome aberrations when held in mitosis for 1, 2, or 3 h after enzyme treatment. However, some disruption of chromosome morphology was seen, especially after exposure to Sau3AI. When cells were allowed to complete one cell cycle after enzyme treatment in the preceding mitosis, there was extensive chromosome damage, with the most abundant type of lesion being the interstitial deletion. It appears that restriction enzymes will cleave the highly condensed DNA in mitotic cells but that decondensation, DNA replication, and recondensation are required before the aberrations are manifested.

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Year:  1991        PMID: 1648753

Source DB:  PubMed          Journal:  Radiat Res        ISSN: 0033-7587            Impact factor:   2.841


  2 in total

1.  On the importance of DNA strand breaks as the first event to initiate sister chromatid exchange (SCE): experiments with restriction endonuclease BglI.

Authors:  T Ortiz; J Piñero; F Cortés
Journal:  Chromosome Res       Date:  1996-11       Impact factor: 5.239

2.  Noncomplementary DNA double-strand-break rejoining in bacterial and human cells.

Authors:  J S King; E R Valcarcel; J T Rufer; J W Phillips; W F Morgan
Journal:  Nucleic Acids Res       Date:  1993-03-11       Impact factor: 16.971

  2 in total

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