Origin and maintenance of large ribosomal RNA gene repeat size in mammals

Author:

Macdonald Emma1,Whibley Annabel12,Waters Paul D3,Patel Hardip4,Edwards Richard J35,Ganley Austen R D16ORCID

Affiliation:

1. School of Biological Sciences, University of Auckland , Private Bag 92019, Auckland 1142 , New Zealand

2. Grapevine Improvement, Bragato Research Institute, RFH Building, Engineering Drive, Lincoln University , Lincoln 7647 , New Zealand

3. School of Biotechnology and Biomolecular Sciences, UNSW Sydney, Chancellery Walk , Kensington, NSW 2033 , Australia

4. John Curtin School of Medical Research, Australian National University , 131 Garran Rd, Acton, ACT 2601 , Australia

5. Minderoo OceanOmics Centre at UWA, UWA Oceans Institute, University of Western Australia , Crawley WA 6009 , Australia

6. Digital Life Institute, University of Auckland , Private Bag 92019, Auckland 1142 , New Zealand

Abstract

Abstract The genes encoding ribosomal RNA are highly conserved across life and in almost all eukaryotes are present in large tandem repeat arrays called the rDNA. rDNA repeat unit size is conserved across most eukaryotes but has expanded dramatically in mammals, principally through the expansion of the intergenic spacer region that separates adjacent rRNA coding regions. Here, we used long-read sequence data from representatives of the major amniote lineages to determine where in amniote evolution rDNA unit size increased. We find that amniote rDNA unit sizes fall into two narrow size classes: “normal” (∼11–20 kb) in all amniotes except monotreme, marsupial, and eutherian mammals, which have “large” (∼35–45 kb) sizes. We confirm that increases in intergenic spacer length explain much of this mammalian size increase. However, in stark contrast to the uniformity of mammalian rDNA unit size, mammalian intergenic spacers differ greatly in sequence. These results suggest a large increase in intergenic spacer size occurred in a mammalian ancestor and has been maintained despite substantial sequence changes over the course of mammalian evolution. This points to a previously unrecognized constraint on the length of the intergenic spacer, a region that was thought to be largely neutral. We finish by speculating on possible causes of this constraint.

Funder

New Zealand Marsden Fund

Medical Research Futures Fund

MRFF

National Health and Medical Research Council

Australian Research Council Discovery Projects

Genomics Aotearoa High Quality Genomes and Population Genomics Project

Publisher

Oxford University Press (OUP)

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