Single-cell transcriptomics defines Dot1L interacting partners and downstream target genes in the mouse molar dental pulp

Authors

Rosa Guzzo
Badam Enkhmandakh
Timothy Becker
Pujan Joshi
Paul Robson, The Jackson LaboratoryFollow
Anushree Vijaykumar
Mina Mina
Dong-Guk Shin
Dashzeveg Bayarsaihan

Document Type

Article

Publication Date

1-1-2022

Publication Title

The International journal of developmental biology

Keywords

JGM

JAX Source

Int J Dev Biol . 2022;66(7-8-9):391-400.

Volume

66

Issue

2009-07-08

First Page

391

Last Page

400

PMID

36942693

DOI

10.1387/ijdb.220141db

Grant

This project was funded by the grant REP-401754-20144-20 from the University of Connecticut to DB. We thank all members of the mm, RG and DB laboratories.

Abstract

Although histone methyltransferases are implicated in many key developmental processes, the contribution of individual chromatin modifiers in dental tissues is not well understood. Using single-cell RNA sequencing, we examined the expression profiles of the disruptor of telomeric silencing 1-like (Dot1L) gene in the postnatal day 5 mouse molar dental pulp. Dot1L is the only known enzyme that methylates histone 3 on lysine 79, a modification associated with gene expression. Our research revealed 15 distinct clusters representing different populations of mesenchymal stromal cells (MSCs), immune cells, pericytes, ameloblasts and endothelial cells. We documented heterogeneity in gene expression across different subpopulations of MSCs, a good indicator that these stromal progenitors undergo different phases of osteogenic differentiation. Interestingly, although Dot1L was broadly expressed across all cell clusters within the molar dental pulp, our analyses indicated specific enrichment of Dot1L within two clusters of MSCs, as well as cell clusters characterized as ameloblasts and endothelial cells. Moreover, we detected Dot1L co-expression with protein interactors involved in epigenetic activation such as Setd2, Sirt1, Brd4, Isw1, Bptf and Suv39h1. In addition, Dot1L was co-expressed with Eed2, Cbx3 and Dnmt1, which encode epigenetic factors associated with gene silencing and heterochromatin formation. Dot1l was co-expressed with downstream targets of the insulin growth factor and WNT signaling pathways, as well as genes involved in cell cycle progression. Collectively, our results suggest that Dot1L may play key roles in orchestrating lineage-specific gene expression during MSC differentiation.

Recommended Citation

Guzzo R, Enkhmandakh B, Becker T, Joshi P, Robson P, Vijaykumar A, Mina M, Shin D, Bayarsaihan D. Single-cell transcriptomics defines Dot1L interacting partners and downstream target genes in the mouse molar dental pulp Int J Dev Biol . 2022;66(7-8-9):391-400.