Nascent Ribo-Seq measures ribosomal loading time and reveals kinetic impact on ribosome density

Johanna Schott; Sonja Reitter; Doris Lindner; Jan Grosser; Marius Bruer; Anjana Shenoy; Tamar Geiger; Arthur Mathes; Gergana Dobreva; Georg Stoecklin

doi:10.1038/s41592-021-01250-z

Nascent Ribo-Seq measures ribosomal loading time and reveals kinetic impact on ribosome density

Nat Methods. 2021 Sep;18(9):1068-1074. doi: 10.1038/s41592-021-01250-z. Epub 2021 Sep 3.

Authors

Johanna Schott^{1

2}, Sonja Reitter^{3

4}, Doris Lindner^{3

4}, Jan Grosser^{3

4}, Marius Bruer^{3

4}, Anjana Shenoy⁵, Tamar Geiger⁵, Arthur Mathes^{6

7}, Gergana Dobreva^{6

7}, Georg Stoecklin^{3

4}

Affiliations

¹ Mannheim Institute for Innate Immunoscience (MI3), Medical Faculty Mannheim, Heidelberg University, Mannheim, Germany. johanna.schott@medma.uni-heidelberg.de.
² Center for Molecular Biology of Heidelberg University (ZMBH), German Cancer Research Center (DKFZ)-ZMBH Alliance, Heidelberg, Germany. johanna.schott@medma.uni-heidelberg.de.
³ Mannheim Institute for Innate Immunoscience (MI3), Medical Faculty Mannheim, Heidelberg University, Mannheim, Germany.
⁴ Center for Molecular Biology of Heidelberg University (ZMBH), German Cancer Research Center (DKFZ)-ZMBH Alliance, Heidelberg, Germany.
⁵ Sackler Faculty of Medicine, Tel Aviv University, Tel Aviv, Israel.
⁶ Department of Anatomy and Developmental Biology, European Center for Angioscience (ECAS), Medical Faculty Mannheim, Heidelberg University, Mannheim, Germany.
⁷ German Center for Cardiovascular Research (DZHK), Heidelberg, Germany.

PMID: 34480152
DOI: 10.1038/s41592-021-01250-z

Abstract

In general, mRNAs are assumed to be loaded with ribosomes instantly upon entry into the cytoplasm. To measure ribosome density (RD) on nascent mRNA, we developed nascent Ribo-Seq by combining Ribo-Seq with progressive 4-thiouridine labeling. In mouse macrophages, we determined experimentally the lag between the appearance of nascent mRNA and its association with ribosomes, which was calculated to be 20-22 min for bulk mRNA. In mouse embryonic stem cells, nRibo-Seq revealed an even stronger lag of 35-38 min in ribosome loading. After stimulation of macrophages with lipopolysaccharide, the lag between cytoplasmic and translated mRNA leads to uncoupling between input and ribosome-protected fragments, which gives rise to distorted RD measurements under conditions where mRNA amounts are far from steady-state expression. As a result, we demonstrate that transcriptional changes affect RD in a passive way.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Cytoplasm / genetics
Kinetics
Lipopolysaccharides / pharmacology
Mice
Mouse Embryonic Stem Cells / cytology
Mouse Embryonic Stem Cells / physiology
Protein Biosynthesis*
RAW 264.7 Cells
RNA, Messenger / genetics
Ribosomal Proteins / biosynthesis
Ribosomal Proteins / genetics
Ribosomes / drug effects
Ribosomes / genetics*
Ribosomes / metabolism*
Sequence Analysis, RNA / methods*
Time Factors

Substances

Lipopolysaccharides
RNA, Messenger
Ribosomal Proteins