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Plant Physiol, February 2001, Vol. 125, pp. 673-682 Hydrophobic Interactions of the Structural Protein GRP1.8 in the Cell Wall of Protoxylem Elements1Institute of Plant Biology, University of Zurich, 8008 Zurich, Switzerland
The glycine-rich structural protein GRP1.8 of French bean
(Phaseolus vulgaris) is specifically localized in the
modified primary cell walls of protoxylem elements. Continuous
deposition of GRP1.8 into the cell walls during elongation growth of
the plant suggests that GRP1.8 is part of a repair mechanism to
strengthen the protoxylem. In this work, a reporter-protein system was
developed to study the interaction of GRP1.8 with the extracellular
matrix. Fusion proteins of a highly soluble chitinase with different
domains of GRP1.8 were expressed in the vascular tissue of tobacco
(Nicotiana tabacum), and the chemical nature of the
interaction of these fusion proteins in the cell wall compartment was
analyzed. In contrast with chitinase that required only low-salt
conditions for complete extraction, the different chitinase/GRP1.8
fusion proteins were completely extracted only by a nonionic or ionic detergent, indicating hydrophobic interactions of GRP1.8. The same
interactions were found with the endogenous GRP1.8 in bean hypocotyls.
In addition, in vitro experiments indicate that oxidative cross-linking
of tyrosines might account for the insolubilization of GRP1.8 observed
in later stages of protoxylem development. Our data suggest that GRP1.8
forms a hydrophobic protein-layer in the cell wall of protoxylem vessels.
1 This work was supported by the Swiss National Science Foundation (grant nos. 31-33612.92 and 31-51055.97). 2 Present address: Promotion Software, Karlstrasse 3, 72072 Tuebingen, Germany. * Corresponding author; e-mail bkeller{at}botinst.unizh.ch; fax 41-1-634-82-04. © 2001 American Society of Plant Physiologists This article has been cited by other articles:
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