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PLANT PHYSIOLOGY , Vol 102, Issue 3 881-889, Copyright © 1993 by American Society of Plant Biologists
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METABOLISM AND ENZYMOLOGY |
Cellular Localization of Protoporphyrinogen-Oxidizing Activities of Etiolated Barley (Hordeum vulgare L.) Leaves (Relationship to Mechanism of Action of Protoporphyrinogen Oxidase-Inhibiting Herbicides)
H. J. Lee, M. V. Duke and S. O. Duke
United States Department of Agriculture/Agricultural Research Service, Southern Weed Science Laboratory, Stoneville, Mississippi 38776
Seven-day-old, etiolated barley (Hordeum vulgare L. var Post) leaves were
fractionated into crude and purified etioplast, microsomal, and plasma
membrane (PM) fractions. Protoporphyrinogen oxidase (Protox) specific
activities of crude etioplast, purified etioplast, microsome, and PM
fractions were approximately 29, 26, 23, and 12 nmol h-1 mg-1 of protein,
respectively. The herbicide acifluorfen-methyl (AFM), at 1 [mu]M, inhibited
Protox activity from crude etioplasts, purified etioplasts, microsomes, and
PM by 58, 59, 23, and 0% in the absence of reductants. Reductants
(ascorbate, glutathione [GSH], dithiothreitol [DTT], and NADPH)
individually reduced the Protox activity of all fractions, except that
microsomal Protox activity was slightly stimulated by NADPH. Ascorbate,
GSH, or a combination of the two reductants enhanced Protox inhibition by
AFM, and AFM inhibition of Protox was greatest in all fractions with DTT.
NADPH enhanced AFM inhibition significantly only in etioplast fractions.
Uroporphyrinogen I (Urogen I) and coproporphyrinogen I (Coprogen I) oxidase
activities were found in all fractions; however, etioplast fractions had
significantly more substrate specificity for protoporphyrinogen IX
(Protogen IX) than the other fractions. Urogen I and Coprogen I oxidase
activities were unaffected by AFM in all fractions, and 2 mM DTT almost
completely inhibited these activities from all fractions.
Diethyldithiocarbamate inhibited PM Protox activity by 62% but had less
effect on microsome and little or no effect on etioplast Protox. Juglone
and duroquinone stimulated microsomal and PM Protox activity, whereas the
lesser effect of these quinones on etioplast Protox activity was judged to
be due to PM and/or microsomal contaminants. These data indicate that there
are microsomal and PM Protogen IX-oxidizing activities that are not the
same as those associated with the etioplast and that these activities are
not inhibited in vivo by AFM. In summary, these data support the view that
the primary source of high protoporphyrin IX concentrations in AFM-treated
plant tissues is from Protogen IX exported by plastids and oxidized by
AFM-resistant extraorganellar oxidases.
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