2010
DOI: 10.1073/pnas.1003438107
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Human ISWI chromatin-remodeling complexes sample nucleosomes via transient binding reactions and become immobilized at active sites

Abstract: Chromatin remodeling complexes can translocate nucleosomes along the DNA in an ATP-dependent manner. Here, we studied autofluorescent protein constructs of the human ISWI family members Snf2H, Snf2L, the catalytically inactive Snf2L+13 splice variant, and the accessory Acf1 subunit in living human and mouse cells by fluorescence microscopy/spectroscopy. Except for Snf2L, which was not detected in the U2OS cell line, the endogenous ISWI proteins were abundant at nuclear concentrations between 0.14 and 0.83 μM. … Show more

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Cited by 93 publications
(131 citation statements)
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References 44 publications
(61 reference statements)
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“…Accordingly, the average residence time of ISWI remodelers increased to seconds and minutes at these sites. 1 This change in binding activity is in line with a 'release mechanism' proposed previously based on in vitro experiments: 2 Nucleosomes that are to be translocated by a given chromatin remodeling complex display a higher binding affinity than those at positions reached at the end points of the remodeling reaction.…”
Section: Snf2h Snf2l and Acf1 Are Rapidly Recruited To Dna Damage Sitessupporting
confidence: 55%
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“…Accordingly, the average residence time of ISWI remodelers increased to seconds and minutes at these sites. 1 This change in binding activity is in line with a 'release mechanism' proposed previously based on in vitro experiments: 2 Nucleosomes that are to be translocated by a given chromatin remodeling complex display a higher binding affinity than those at positions reached at the end points of the remodeling reaction.…”
Section: Snf2h Snf2l and Acf1 Are Rapidly Recruited To Dna Damage Sitessupporting
confidence: 55%
“…The slow PCNA component is unlikely to represent chromatin dynamics since the diffusion coefficient was too large and the anomaly parameter was α ≈ 0.7 (for confined diffusion of chromatin fibers, an anomaly parameter larger than 1 is expected in the FCS fit of the data as observed for Snf2H with α = 2.1 ± 0.2, 1,21 ). We conclude that the equilibrium density of bound PCNA molecules along the chromatin fiber is insufficient to be detected in the correlation function.…”
Section: Pcna and Snf2h Are Not Detected In Soluble Complexesmentioning
confidence: 99%
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