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The Journal of biological chemistry, 1996-04, Vol.271 (16), p.9764-9770
1996
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Autor(en) / Beteiligte
Titel
Evidence for the Direct Interaction of the nifW Gene Product with the MoFe Protein
Ist Teil von
  • The Journal of biological chemistry, 1996-04, Vol.271 (16), p.9764-9770
Ort / Verlag
United States: Elsevier Inc
Erscheinungsjahr
1996
Quelle
MEDLINE
Beschreibungen/Notizen
  • The Azotobacter vinelandii nifW gene, under control of the nifH promoter, was subcloned into the broad host range multicopy plasmid pKT230 for overexpression in both wild-type and delta nifW strains of A. vinelandii. Unlike the parent delta nifW strain, which grows slowly relative to wild-type under N2-fixing conditions, both overproduction strains grow at the same rate showing that the overexpressed nifW product is functional in vivo. The approximately 40-fold overexpressed protein was purified, and sequence analysis confirmed its identity. During purification it was observed that NifW in crude extracts ran above the predicted molecular weight on denaturing gels and that as the purification proceeded lower molecular weight forms appeared. Mass spectrometry and studies with protease inhibitors revealed that this abnormal behavior was due to proteolysis. Native molecular weight determinations demonstrate that NifW is a homomultimer, most likely a trimer. Native gel electrophoresis analysis shows that the behavior of wild-type and overexpressed NifW are identical and that when extracts are prepared anaerobically only the homomultimeric forms of NifW are observed. When extracts are exposed to oxygen, however, NifW becomes part of a very high molecular weight complex. Immunoprecipitation with NifW antibodies demonstrate that under those conditions NifW specifically associates with the MoFe protein. These data are consistent with a model whereby NifW is not involved in the initial assembly of an active MoFe protein but rather is part of a system design to protect the MoFe protein from O2 damage

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