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Ammonium-assimilating enzymes and their regulation in wild and NADP-glutamate dehydrogenase-deficient strains of the ectomycorrhizal fungus Hebeloma cylindrosporum
Authors:Michel Chalot  Annick Brun  Jean Claude Debaud  Bernard Botton
Affiliation:Laboratoire de Physiologie Végétale et Forestiére, Facultédes Sciences, Univ. de Nancy I, BP 239, F-54506 Vandoeuvre-lés-Nancy Cedex, France;Laboratoire de Mycologie, Univ. Claude Bernard, Lyon I, Institut de Chimie et Biologie Moléculaires et Cellulaires, F-69622 Villeurbanne Cedex, France.
Abstract:Hebeloma cylindrosporum strain h 17 was grown on media containing either glutamate or ammonium as nitrogen source. Growth tests and in vitro activity measurements revealed that both glutamine synthetase (GS. EC 6.3.1.2) and NADP-specific glutamate dehydrogenase (NADP-GDH, EC 1.4.1.4) are fully functional in wild type mycelia grown on glutamate or ammonium as sole nitrogen source. However, NADP-GDH appeared to be more active than GS in stationary growing mycelia. NADP-GDH is also able to sustain adequate ammonium assimilation in methionine sulfoximine (MSX)-treated mycelia since they grew as well as mycelia fed with ammonium alone. The NADP-GDH also appeared to be L-glutamate inducible whereas GS was repressed by ammonium. The NADP-GDH deficient strain, when transferred from a glutamate containing medium to an ammonium containing medium, exhibited a derepressed GS, although this enzyme did not fully substitute for the deficiency of NADP-GDH in ammonium assimilation. The low NADP-GDH activity of the mutant strain exhibited a reduced mobility on a 6% constant polyacrylamide gel. By contrast, the two enzymes had identical molecular weights, estimated to be ca 295 kDa on gradient polyacrylamide gel. The involvement of NADP-GDH and GS enzymes in nitrogen assimilation is discussed.
Keywords:Ectomycorrhizal fungus    glutamate dehydrogenase    glutamine synthetase    Hebeloma cylindrosporum    mutant    nitrogen metabolism
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