Novel MtCEP1 peptides produced in vivo differentially regulate root development in Medicago truncatula

Nadiatul A Mohd-Radzman; Steve Binos; Thy T Truong; Nijat Imin; Michael Mariani; Michael A Djordjevic

doi:10.1093/jxb/erv008

Novel MtCEP1 peptides produced in vivo differentially regulate root development in Medicago truncatula

J Exp Bot. 2015 Aug;66(17):5289-300. doi: 10.1093/jxb/erv008. Epub 2015 Feb 22.

Authors

Nadiatul A Mohd-Radzman¹, Steve Binos², Thy T Truong³, Nijat Imin¹, Michael Mariani², Michael A Djordjevic⁴

Affiliations

¹ Division of Plant Sciences, Research School of Biology, College of Medicine, Biology and Environment, The Australian National University, Canberra ACT 0200, Australia.
² Thermo Fisher Scientific Pty Ltd, 5 Caribbean Drive, Scoresby, VIC 3179, Australia.
³ Mass Spectrometry Facility, Research School of Biology, College of Medicine, Biology and Environment, The Australian National University, Canberra ACT 0200, Australia.
⁴ Division of Plant Sciences, Research School of Biology, College of Medicine, Biology and Environment, The Australian National University, Canberra ACT 0200, Australia michael.djordjevic@anu.edu.au.

Abstract

Small, post-translationally modified and secreted peptides regulate diverse plant developmental processes. Due to low natural abundance, it is difficult to isolate and identify these peptides. Using an improved peptide isolation protocol and Orbitrap mass spectrometry, nine 15-amino-acid CEP peptides were identified that corresponded to the two domains encoded by Medicago truncatula CEP1 (MtCEP1). Novel arabinosylated and hydroxylated peptides were identified in root cultures overexpressing MtCEP1. The five most abundant CEP peptides were hydroxylated and these species were detected also in low amounts in vector control samples. Synthetic peptides with different hydroxylation patterns differentially affected root development. Notably, the domain 1 peptide hydroxylated at Pro4 and Pro11 (D1:HyP4,11) imparted the strongest inhibition of lateral root emergence when grown with 5mM KNO3 and stimulated the highest increase in nodule number when grown with 0mM KNO3. Inhibition of lateral root emergence by D1:HyP4,11 was not alleviated by removing peptide exposure. In contrast, the domain 2 peptide hydroxylated at Pro11 (D2:HyP11) increased stage III-IV lateral root primordium numbers by 6-fold (P < 0.001) which failed to emerge. Auxin addition at levels which stimulated lateral root formation in wild-type plants had little or no ameliorating effect on CEP peptide-mediated inhibition of lateral root formation or emergence. Both peptides increased and altered the root staining pattern of the auxin-responsive reporter GH3:GUS suggesting CEPs alter auxin sensitivity or distribution. The results showed that CEP primary sequence and post-translational modifications influence peptide activities and the improved isolation procedure effectively and reproducibly identifies and characterises CEPs.

Keywords: Legume root development; mass spectrometry; nodulation; peptide isolation; peptide signaling; post-translational modification; secreted peptides..

Publication types

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

MeSH terms

Amino Acid Sequence
Gene Expression Regulation, Plant*
Indoleacetic Acids / pharmacology*
Medicago truncatula / genetics*
Medicago truncatula / growth & development
Medicago truncatula / metabolism
Naphthaleneacetic Acids / pharmacology*
Plant Growth Regulators / pharmacology*
Plant Proteins / chemistry
Plant Proteins / genetics*
Plant Proteins / metabolism
Plant Roots / growth & development
Plant Roots / metabolism
Plants, Genetically Modified / genetics
Plants, Genetically Modified / metabolism
Tandem Mass Spectrometry

Substances

Indoleacetic Acids
Naphthaleneacetic Acids
Plant Growth Regulators
Plant Proteins
1-naphthaleneacetic acid