Literature DB >> 10854414

The 10q25 neocentromere and its inactive progenitor have identical primary nucleotide sequence: further evidence for epigenetic modification.

A E Barry1, M Bateman, E V Howman, M R Cancilla, K M Tainton, D V Irvine, R Saffery, K H Choo.   

Abstract

We have previously localized the core centromere protein-binding domain of a 10q25.2-derived neocentromere to an 80-kb genomic region. Detailed analysis has indicated that the 80-kb neocentromere (NC) DNA has a similar overall organization to the corresponding region on a normal chromosome 10 (HC) DNA, derived from a genetically unrelated CEPH individual. Here we report sequencing of the HC DNA and its comparison to the NC sequence. Single-base differences were observed at a maximum rate of 4.6 per kb; however, no deletions, insertions, or other structural rearrangements were detected. To investigate whether the observed changes, or subsets of these, might be de novo mutations involved in neocentromerization (i.e., in committing a region of a chromosome to neocentromere formation), the progenitor DNA (PnC) from which the NC DNA descended, was cloned and sequenced. Direct comparison of the PnC and NC sequences revealed 100% identity, suggesting that the differences between NC and HC DNA are single nucleotide polymorphisms (SNPs) and that formation of the 10q25.2 NC did not involve a change in DNA sequence in the core centromere protein-binding NC region. This is the first study in which a cloned NC DNA has been compared directly with its inactive progenitor DNA at the primary sequence level. The results form the basis for future sequence comparison outside the core protein-binding domain, and provide direct support for the involvement of an epigenetic mechanism in neocentromerization.

Mesh:

Year:  2000        PMID: 10854414      PMCID: PMC310875          DOI: 10.1101/gr.10.6.832

Source DB:  PubMed          Journal:  Genome Res        ISSN: 1088-9051            Impact factor:   9.043


  28 in total

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9.  Human centromeres and neocentromeres show identical distribution patterns of >20 functionally important kinetochore-associated proteins.

Authors:  R Saffery; D V Irvine; B Griffiths; P Kalitsis; L Wordeman; K H Choo
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10.  A novel epigenetic effect can alter centromere function in fission yeast.

Authors:  N C Steiner; L Clarke
Journal:  Cell       Date:  1994-12-02       Impact factor: 41.582

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  12 in total

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5.  Adaptive evolution of Cid, a centromere-specific histone in Drosophila.

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8.  Centromeric chromatin pliability and memory at a human neocentromere.

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10.  LINE retrotransposon RNA is an essential structural and functional epigenetic component of a core neocentromeric chromatin.

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