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J. Biol. Chem., Vol. 266, Issue 12, 7393-7399, 04, 1991
H Macdonald, AM Jones and PJ King
The photoaffinity labeling agent azido-IAA (5-N3-[7-3H]indole-3-acetic
acid), a biologically active analogue of the endogenous auxin indole-3-
acetic acid, was used to search for auxin-binding proteins in the soluble
fraction of Hyoscyamus muticus cells. Azido-IAA became covalently attached
to three polypeptides with a high specific activity. The labeling was
specific for IAA and not due to random tagging. Two polypeptides with
molecular masses of 31 and 24 kDa in the 0-30% ammonium sulfate fraction
were labeled after UV photolysis at 0 degree C but not at -196 degrees C,
and appeared to have a high affinity indole-binding site(s) for which
active, non-indole auxins were not good ligands. A third polypeptide with a
molecular mass of 25 kDa present in the 50-60% ammonium sulfate fraction
labeled exclusively at -196 degrees C and had a significant affinity for
active auxins but not for inactive indoles. The azido-IAA labeling pattern,
pI, competition results, and immunoprecipitation all indicate that the 31-
and 24-kDa polypeptides are related to the basic form of endo-1,3-beta-
glucanase (EC 3.2.1.39). Azido-IAA labeling polypeptides equivalent to the
31- and 24-kDa species were apparently also present in the cell wall. The
low pH optimum for binding of azido-IAA to the 25-kDa polypeptide suggests
the location of the active protein in a compartment such as the vacuole or
a transport vesicle rather than in the cytosol.
Photoaffinity labeling of soluble auxin-binding proteins
Friedrich Miescher-Institut, Basel, Switzerland.
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