Abstract
Inspite of being embedded in a dense meshwork of nuclear chromatin, gene loci and large nuclear components are highly dynamic at C. To understand this apparent unfettered movement in an overdense environment, we study the dynamics of a passive micron size bead in live cell nuclei at two different temperatures ( and C) with and without external force. In the absence of a force, the beads are caged over large time scales. On application of a threshold uniaxial force (about 10 pN), the passive beads appear to hop between cages; this large scale movement is absent upon ATP-depletion, inhibition of chromatin remodeling enzymes and RNAi of lamin B1 proteins. Our results suggest that the nucleus behaves like an active solid with a finite yield stress when probed at a micron scale. Spatial analysis of histone fluorescence anisotropy (a measure of local chromatin compaction, defined as the volume fraction of tightly bound chromatin) shows that the bead movement correlates with regions of low chromatin compaction. This suggests that the physical mechanism of the observed yielding is the active opening of free-volume in the nuclear solid via chromatin remodeling. Enriched transcription sites at C also show caging in the absence of the applied force and directed movement beyond a yield stress, in striking contrast with the large scale movement of transcription loci at C in the absence of a force. This suggests that at physiological temperatures, the loci behave as active particles which remodel the nuclear mesh and reduce the local yield stress.
Highlights
The 3D spatial assembly of nuclear chromatin is believed to be crucial for the specific patterning of in-vivo gene expression [1]
Experiments on the dynamics of transcription compartments (TCs) [5], cajal bodies [6], PML bodies [7], and gene loci [12], have reported large scale directed movements at physiological temperatures, which are influenced by ATP-dependent chromatin remodeling, while similar studies on the dynamics of TCs at lower temperatures (250C) reveal a near absence of any large scale movement [5]
By analyzing the diffusion of micron size beads, we probe the microrheology of the fluctuating nuclear medium on scales of order q{1*1mm, the size of the bead
Summary
The 3D spatial assembly of nuclear chromatin is believed to be crucial for the specific patterning of in-vivo gene expression [1]. Biophysical measurements have shown that nuclear chromatin is organized as a heterogeneous mesh [2] with a typical mesh size of about 300nm [3], and is dynamically remodeled by a variety of chromatin remodeling proteins [4]. To maintain this precise 3D architecture over interphase, mobile transcription elements should be able to move in a directed and regulated manner through this dense nuclear meshwork. Experiments on the dynamics of transcription compartments (TCs) [5], cajal bodies [6], PML bodies [7], and gene loci [12], have reported large scale directed movements at physiological temperatures, which are influenced by ATP-dependent chromatin remodeling, while similar studies on the dynamics of TCs at lower temperatures (250C) reveal a near absence of any large scale movement [5]
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