
Production of multiple plant hormones from a single polyprotein precursor
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ABSTRACT Some animal and yeast hormone genes produce prohormone polypeptides that are proteolytically processed to produce multiple copies of hormones with the same or different functions1.
In plants, four polypeptides have been identified that can be classed as hormones2,3,4,5 (intercellular chemical messengers6) but none are known to be produced as multiple copies from a
single precursor. Here we describe a polyprotein hormone precursor, present in tobacco plants, that gives rise to two polypeptide hormones, as often found in animals and yeast. The tobacco
polypeptides activate the synthesis of defensive proteinase-inhibitor proteins in a manner similar to that of systemin, an 18-amino-acid polypeptide found in tomato plants2. The two tobacco
polypeptides are derived from each end of a 165-amino-acid precursor that bears no homology to tomato prosystemin. The data show that structurally diverse polypeptide hormones in different
plant species can serve similar signalling roles, a condition not found in animals or yeast. Access through your institution Buy or subscribe This is a preview of subscription content,
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OPTIONS: * Log in * Learn about institutional subscriptions * Read our FAQs * Contact customer support SIMILAR CONTENT BEING VIEWED BY OTHERS DEVELOPMENTAL TIMING IN PLANTS Article Open
access 27 March 2024 REROUTING PLANT TERPENE BIOSYNTHESIS ENABLES MOMILACTONE PATHWAY ELUCIDATION Article 26 October 2020 SPATIOTEMPORAL FORMATION OF GLANDS IN PLANTS IS MODULATED BY
MYB-LIKE TRANSCRIPTION FACTORS Article Open access 15 March 2024 ACCESSION CODES ACCESSIONS GENBANK/EMBL/DDBJ * AY033148 * AY033149 DATA DEPOSITS The GenBank accession number for tobacco
systemin precursor pro-TobSys-A is AY033148, and for pro-TobSys-B is AY033149. REFERENCES * Niall, H. D. The evolution of peptide hormones. _Ann. Rev. Physiol._ 44, 615– 624 (1982). Article
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research was supported by the College of Agriculture and Home Economics and by the National Science Foundation. We thank S. Vogtman for growing plants; G. Munske for amino-acid sequence
analyses; and W. Siems for MALDI mass spectroscopic analyses. AUTHOR INFORMATION Author notes * Johannes Stratmann Present address: Department of Biological Sciences, University of South
Carolina, Columbia, South Carolina, 29208, USA * Clarence A. Ryan: Correspondence and requests for materials should be addressed to C.A.R. AUTHORS AND AFFILIATIONS * Institute of Biological
Chemistry, Washington State University, Pullman, 99164-6340, Washington, USA Gregory Pearce, Daniel S. Moura, Johannes Stratmann & Clarence A. Ryan Authors * Gregory Pearce View author
publications You can also search for this author inPubMed Google Scholar * Daniel S. Moura View author publications You can also search for this author inPubMed Google Scholar * Johannes
Stratmann View author publications You can also search for this author inPubMed Google Scholar * Clarence A. Ryan View author publications You can also search for this author inPubMed Google
Scholar CORRESPONDING AUTHOR Correspondence to Clarence A. Ryan. SUPPLEMENTARY INFORMATION SUPPLEMENT 1. (DOC 23 KB) Protocol for the purification of tobacco systemins SUPPLEMENT 2. (JPG 17
KB) Alkalinization of the medium of suspension cultured tobacco cells in response to increasing concentrations of the ‘crude polypeptide extract’ from leaves as described in the Methods
SUPPLEMENT 3. (PPT 378 KB) The changes in molecular masses of Tob Sys I and II during the hydrolysis of 100 pmoles of each in 100 mL 1% trifluoroacetic acid at 80 °C. At the intervals shown,
10 μL aliquots were removed for MALDI-MS analysis. A ladder of fragments duffering by 132 mass units (indicative of pentoses) were produced as the carbohydrate moieties were removed from
the polypeptides. a. 0 min. b. 15 min. c. 30 min d. 60 min. e. 180 min. SUPPLEMENT 4. (JPG 38 KB) Alkalinization assays of synthetic Tob Sys I and II backbone polypeptides using tobacco
suspension cultured cells. The change in pH of the culture medium was measured 15 min after addition of the polypeptides. Half maximal activity of each polypeptide is about 2 μM, as compared
to 200 pM of the native polypeptides (cf. Figure 2a). SUPPLEMENT 5. (JPG 67 KB) Alignment of the two deduced tobacco systemin precursor proteins (pro-TobSys-A and pro-TobSys-B). The
alignment was made using the Genetics Computer Guoup (GCG-Wisconsin Package Version 10, Madison, WI) programs "translate", "pilieup") (default values) and
"prettybox". SUPPLEMENT 6. (PPT 706 KB) Southern Blots of 5 µg of genomic DNA from tobacco leaves, digested using XbaI SacI NdeI, HindIII, HaeII, EcorRI, and ClaI restriction
enzymes. Digested DNA was separted in agarose gels, salt transferred to nylon membranes and probed using Tobacco preproprotein cDNA. Molecular markers anre indicated on the left (Kb).
Und=undigested. SUPPLEMENT 7. (PPT 187 KB) Gel blot analyses of tobacco prosystemin mRNA in leaves of young tobacco plants exposed to either air or air containing methyl jasmonate vapors.
Following methyl jasmonate treatment for 6 h, RNA extraction and gel blot analyses were performed as described in Bergey et al (1999). RIGHTS AND PERMISSIONS Reprints and permissions ABOUT
THIS ARTICLE CITE THIS ARTICLE Pearce, G., Moura, D., Stratmann, J. _et al._ Production of multiple plant hormones from a single polyprotein precursor. _Nature_ 411, 817–820 (2001).
https://doi.org/10.1038/35081107 Download citation * Received: 05 December 2000 * Accepted: 30 April 2001 * Issue Date: 14 June 2001 * DOI: https://doi.org/10.1038/35081107 SHARE THIS
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