Literature DB >> 16100259

Compaction kinetics on single DNAs: purified nucleosome reconstitution systems versus crude extract.

Gaudeline Wagner1, Aurélien Bancaud, Jean-Pierre Quivy, Cédric Clapier, Geneviève Almouzni, Jean-Louis Viovy.   

Abstract

Kinetics of compaction on single DNA molecules are studied by fluorescence videomicroscopy in the presence of 1), Xenopus egg extracts and 2), purified nucleosome reconstitution systems using a combination of histones with either the histone chaperone Nucleosome Assembly Protein (NAP-1) or negatively charged macromolecules such as polyglutamic acid and RNA. The comparison shows that the compaction rates can differ by a factor of up to 1000 for the same amount of histones, depending on the system used and on the presence of histone tails, which can be subjected to post-translational modifications. Reactions with purified reconstitution systems follow a slow and sequential mechanism, compatible with the deposition of one (H3-H4)(2) tetramer followed by two (H2A-H2B) dimers. Addition of the histone chaperone NAP-1 increases both the rate of the reaction and the packing ratio of the final product. These stimulatory effects cannot be obtained with polyglutamic acid or RNA, suggesting that yNAP-1 impact on the reaction cannot simply be explained in terms of charge screening. Faster compaction kinetics and higher packing ratios are reproducibly reached with extracts, indicating a role of additional components present in this system. Data are discussed and models proposed to account for the kinetics obtained in our single-molecule assay.

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Year:  2005        PMID: 16100259      PMCID: PMC1366857          DOI: 10.1529/biophysj.105.062786

Source DB:  PubMed          Journal:  Biophys J        ISSN: 0006-3495            Impact factor:   4.033


  59 in total

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3.  Mechanical disruption of individual nucleosomes reveals a reversible multistage release of DNA.

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Journal:  Proc Natl Acad Sci U S A       Date:  2002-02-19       Impact factor: 11.205

4.  Chromatin fiber folding: requirement for the histone H4 N-terminal tail.

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5.  Functional analysis of nucleosome assembly protein, NAP-1. The negatively charged COOH-terminal region is not necessary for the intrinsic assembly activity.

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Journal:  J Biol Chem       Date:  1992-10-15       Impact factor: 5.157

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7.  Ribonucleic acid and other polyanions facilitate chromatin assembly in vitro.

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Authors:  A Ruiz-Carrillo; J L Jorcano; G Eder; R Lurz
Journal:  Proc Natl Acad Sci U S A       Date:  1979-07       Impact factor: 11.205

9.  Evidence for a shared structural role for HMG1 and linker histones B4 and H1 in organizing chromatin.

Authors:  K Nightingale; S Dimitrov; R Reeves; A P Wolffe
Journal:  EMBO J       Date:  1996-02-01       Impact factor: 11.598

10.  Assembly of SV40 chromatin in a cell-free system from Xenopus eggs.

Authors:  R A Laskey; A D Mills; N R Morris
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7.  Reconstituted TAD-size chromatin fibers feature heterogeneous nucleosome clusters.

Authors:  Nikolay Korolev; Anatoly Zinchenko; Aghil Soman; Qinming Chen; Sook Yi Wong; Nikolay V Berezhnoy; Rajib Basak; Johan R C van der Maarel; John van Noort; Lars Nordenskiöld
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8.  Organization of human replicon: singles or zipping couples?

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9.  Histone H1 compacts DNA under force and during chromatin assembly.

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  9 in total

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