First published online June 20, 2002; 10.1104/pp.002592
Plant Physiol, July 2002, Vol. 129, pp. 1391-1397
Transfer Specificity of Detergent-Solubilized Fenugreek
Galactomannan Galactosyltransferase
Mary E.
Edwards,
Elaine
Marshall,1
Michael J.
Gidley, and
J.S. Grant
Reid*
Department of Biological Sciences, University of Stirling, Stirling
FK9 4LA, Scotland (M.E.E., E.M., J.S.G.R.); and Unilever Research
Laboratory, Colworth House, Sharnbrook, Bedford MK44 1LQ, United
Kingdom (M.J.G.)
The current experimental model for galactomannan
biosynthesis in membrane-bound enzyme systems from developing
legume-seed endosperms involves functional interaction between a
GDP-mannose (Man) mannan synthase and a UDP-galactose (Gal)
galactosyltransferase. The transfer specificity of the
galactosyltransferase to the elongating mannan chain is critical in
regulating the distribution and the degree of Gal substitution of the
mannan backbone of the primary biosynthetic product. Detergent
solubilization of the galactosyltransferase of fenugreek
(Trigonella foenum-graecum) with retention of activity permitted the partial purification of the enzyme and the cloning and
sequencing of the corresponding cDNA with proof of functional identity.
We now document the positional specificity of transfer of
(14C)Gal from UDP-(14C)Gal to
manno-oligosaccharide acceptors, chain lengths 5 to 8, catalyzed by the
detergent-solubilized galactosyltransferase. Enzymatic fragmentation
analyses of the labeled products showed that a single Gal residue was
transferred per acceptor molecule, that the linkage was (1 6)- ,
and that there was transfer to alternative Man residues within the
acceptor molecules. Analysis of the relative frequencies of transfer to
alternative Man residues within acceptor oligosaccharides of different
chain length allowed the deduction of the substrate subsite recognition
requirement of the galactosyltransferase. The enzyme has a principal
recognition sequence of six Man residues, with transfer of Gal to the
third Man residue from the nonreducing end of the sequence. These
observations are incorporated into a refined model for enzyme
interaction in galactomannan biosynthesis.
1
Present address: Roslin Institute, Roslin,
Midlothian EH25 9PS, Scotland.
*
Corresponding author; e-mail j.s.g.reid{at}stir.ac.uk; fax
44-1786-464994.
© 2002 American Society of Plant Physiologists
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