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Regulation of expression of glutamine synthetase in a symbiotic Nostoc strain associated with Anthoceros punctatus

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A characteristic of N2-fixing cyanobacteria in symbiotic associations appears to be release of N2-derived NH4+. The specific activity of the primary ammonium-assimilating enzyme, glutamine synthetase (GS), was found to be three- to fourfold lower in Nostoc sp. strain 7801 grown in symbiotic association with the bryophyte Anthoceros punctatus than in free-living Nostoc sp. strain 7801. Quantitative immunological assays with antisera against GS purified from Nostoc sp. strain 7801 and from Escherichia coli indicated that similar amounts of the GS protein were present in symbiotic (50 micrograms mg-1) and free-living (68 micrograms mg-1) cultures. The conclusion from these experiments is that GS is regulated by a posttranslational mechanism in Anthoceros-associated Nostoc sp. strain 7801. However, the results of comparative catalytic and immunological experiments between N2- and NH4+-grown free-living Nostoc sp. strain 7801 implied control of GS synthesis. A correlation was not observed between the level of GS expression and the extent of symbiotic heterocyst differentiation in Nostoc sp. strain 7801 associated with A. punctatus.
American Society for Microbiology
Title: Regulation of expression of glutamine synthetase in a symbiotic Nostoc strain associated with Anthoceros punctatus
Description:
A characteristic of N2-fixing cyanobacteria in symbiotic associations appears to be release of N2-derived NH4+.
The specific activity of the primary ammonium-assimilating enzyme, glutamine synthetase (GS), was found to be three- to fourfold lower in Nostoc sp.
strain 7801 grown in symbiotic association with the bryophyte Anthoceros punctatus than in free-living Nostoc sp.
strain 7801.
Quantitative immunological assays with antisera against GS purified from Nostoc sp.
strain 7801 and from Escherichia coli indicated that similar amounts of the GS protein were present in symbiotic (50 micrograms mg-1) and free-living (68 micrograms mg-1) cultures.
The conclusion from these experiments is that GS is regulated by a posttranslational mechanism in Anthoceros-associated Nostoc sp.
strain 7801.
However, the results of comparative catalytic and immunological experiments between N2- and NH4+-grown free-living Nostoc sp.
strain 7801 implied control of GS synthesis.
A correlation was not observed between the level of GS expression and the extent of symbiotic heterocyst differentiation in Nostoc sp.
strain 7801 associated with A.
punctatus.

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