Glutamine synthetase activity of the endosperm, embryo and pedicel‐placento‐chalazal regions of developing maize ( Zea mays ) kernels

Glutamine synthetase (GS, EC 6.3.1.2) activity in homogenates of the maize ( Zea mays L. hybrid A619 X W64A) kernel pedicel‐placento‐chalazal (PPCh), endosperm regions was characterized in order to optimize assay (hydroxylamine‐dependent γ‐glutamyl hydroxymate formation) conditions for quantitating maize kernel GS in crude extracts. The GS activities of all three tissue extracts exhibited optima at pH 7.0 with ATP:Mg 2+ of 1:1.6. Assays of kernel tissue GS activity required relatively high concentrations of substrates to achieve saturation compared to GS from other plant tissue sources, a point which has not been considered in previous reports of maize kernel GS activity. When measured under optimal assay conditions. PPCh‐GS increased to a peak of 51 nmol γ‐glutamyl hydroxymate kernel −1 min −1 at 25 days after pollination and then declined throughout the remainder of kernel development. Embryo GS activity increased steadily throughout development to a maximum of 24 nmol γ‐glutamyl hydroxymate embryo −1 min −1 by 50 days after pollination. In contrast, endosperm GS activity, which was 25 nmol γ‐glutamyl hydroxymate endosperm −1 min −1 at 25 days after pollination, exhibited no discernable pattern of change during kernel development. These findings are discussed with respect to the possible roles PPCh, endosperm and embryo GS play in kernel development.