Title
Molecular organization of the early stages of nucleosome phase separation visualized by cryo-electron tomography
Date Issued
18 August 2022
Access level
open access
Resource Type
journal article
Author(s)
Zhang M.
Díaz-Celis C.
Onoa B.
Cañari-Chumpitaz C.
Requejo K.I.
Liu J.
Vien M.
Nogales E.
Ren G.
University of California
Publisher(s)
Cell Press
Abstract
It has been proposed that the intrinsic property of nucleosome arrays to undergo liquid-liquid phase separation (LLPS) in vitro is responsible for chromatin domain organization in vivo. However, understanding nucleosomal LLPS has been hindered by the challenge to characterize the structure of the resulting heterogeneous condensates. We used cryo-electron tomography and deep-learning-based 3D reconstruction/segmentation to determine the molecular organization of condensates at various stages of LLPS. We show that nucleosomal LLPS involves a two-step process: a spinodal decomposition process yielding irregular condensates, followed by their unfavorable conversion into more compact, spherical nuclei that grow into larger spherical aggregates through accretion of spinodal materials or by fusion with other spherical condensates. Histone H1 catalyzes more than 10-fold the spinodal-to-spherical conversion. We propose that this transition involves exposure of nucleosome hydrophobic surfaces causing modified inter-nucleosome interactions. These results suggest a physical mechanism by which chromatin may transition from interphase to metaphase structures.
Start page
3000
End page
3014.e9
Volume
82
Issue
16
Language
English
OCDE Knowledge area
Física atómica, molecular y química
Bioquímica, Biología molecular
Subjects
Scopus EID
2-s2.0-85136837091
PubMed ID
Source
Molecular Cell
ISSN of the container
10972765
Sponsor(s)
We thank Professor Geeta Narlikar for providing the expression vectors of X. laevis histones and Dr. Hataichanok “Mam” Scherman for providing linker histone H1. We thank Professor Daniel Fletcher and Dr. Aymeric Chorlay for their help with FRAP experiments. We thank Professor David Limmer and Alex Tong for helpful discussions. Data were collected at the Cal-Cryo facility, Berkeley QB3 Institute. This research was supported by the Nanomachine program (KC1203) funded by the Office of Basic Energy Sciences of the US Department of Energy (DOE) contract no. DE-AC02-05CH11231 (C.B.). The work was also partially supported by grants from the US National Institutes of Health (R01HL115153, R01GM104427, and R01MH077303; R01DK042667 to G.R.; R35GM127018 to E.N.; and R01GM032543 to C.B.). C.B. and E.N. are Howard Hughes Medical Institute investigators. C.B. M.Z. and C.D.-C. conceived the study, and C.B. M.Z. G.R. and E.N. designed the research. C.D.-C. and M.V. purified and labeled histones, reconstituted and purified tetranucleosome and dodecamer samples. C.C.-C. and C.D.-C. performed the fluorescence microscopy imaging, and B.O. collected the AFM images. M.Z. prepared EM specimens. M.Z. and J.L. collected the EM data. M.Z. and G.R. designed the cryo-ET workflow. M.Z. conducted the 3D reconstruction, modeling, and statistical analyses. M.Z. interpreted the data and prepared the EM-related figures and videos. M.Z. and C.B. wrote the original draft, and C.D.-C. E.N. G.R. B.O. K.I.R. C.C.-C. and M.V. edited the manuscript. K.I.R. supplemented the theory section. C.B. and G.R. supervised the work. The authors declare no competing interests.
Sources of information:
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