Determinants of minor satellite RNA function in chromosome segregation in mouse embryonic stem cells

Author:

Chen Yung-Li1ORCID,Jones Alisha N.2ORCID,Crawford Amy3ORCID,Sattler Michael24ORCID,Ettinger Andreas1ORCID,Torres-Padilla Maria-Elena15ORCID

Affiliation:

1. Institute of Epigenetics and Stem Cells (IES), Helmholtz Munich 1 , München, Germany

2. Institute of Structural Biology, Molecular Targets and Therapeutics Center, Helmholtz Munich 2 , Neuherberg, Germany

3. New York University 3 Department of Chemistry, , New York, NY, USA

4. Bavarian NMR Center, School of Natural Sciences, Technical University of Munich 4 Department of Bioscience, , Garching, Germany

5. Faculty of Biology, Ludwig-Maximilians Universität 5 , München, Germany

Abstract

The centromere is a fundamental higher-order structure in chromosomes ensuring their faithful segregation upon cell division. Centromeric transcripts have been described in several species and suggested to participate in centromere function. However, low sequence conservation of centromeric repeats appears inconsistent with a role in recruiting highly conserved centromeric proteins. Here, we hypothesized that centromeric transcripts may function through a secondary structure rather than sequence conservation. Using mouse embryonic stem cells (ESCs), we show that an imbalance in the levels of forward or reverse minor satellite (MinSat) transcripts leads to severe chromosome segregation defects. We further show that MinSat RNA adopts a stem-loop secondary structure, which is conserved in human α-satellite transcripts. We identify an RNA binding region in CENPC and demonstrate that MinSat transcripts function through the structured region of the RNA. Importantly, mutants that disrupt MinSat secondary structure do not cause segregation defects. We propose that the conserved role of centromeric transcripts relies on their secondary RNA structure.

Funder

German Research Foundation

Helmholtz Association

Publisher

Rockefeller University Press

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