Nitrogen Utilization in <i>Lemna</i>

Ingemarsson, Björn

doi:10.1104/pp.85.3.856

Cited by 34 publications

(16 citation statements)

References 25 publications

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“…The fact that protease inhibitors had no effect in the present study does not necessarily refute this idea because the effectiveness of the tested protease inhibitors varies with the species, and proteases resistant to the particular inhibitors used in this study may have been present. For example, lcupeptin is effective against NRspecific proteases found in Lemna (Ingemarsson 1987), while PMSF is not. The effectiveness of BSA has also been noted by Ingemarsson ( 1987), but in these cases casein was also effective; this was not true in the present study (data not shown).…”

Section: Discussionmentioning

confidence: 99%

“…For example, lcupeptin is effective against NRspecific proteases found in Lemna (Ingemarsson 1987), while PMSF is not. The effectiveness of BSA has also been noted by Ingemarsson ( 1987), but in these cases casein was also effective; this was not true in the present study (data not shown). BSA may act by providing a protein in higher concentration that the proteases can degrade in preference to NR, but there may be other effects.…”

Section: Discussionmentioning

confidence: 99%

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Nitrate reductase activity quantitatively predicts the rate of nitrate incorporation under steady state light limitation: A revised assay and characterization of the enzyme in three species of marine phytoplankton

Berges

Harrison

1995

Limnology & Oceanography

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The enzyme nitrate reductase (NR) has been proposed as an index of nitrate incorporation rates in marine phytoplankton, but it has proven difficult to interpret NR measurements in field settings because many previous NR assays have been poorly optimized and NR activity in phytoplankton has been poorly characterized under steady state conditions. An NR assay was developed for the diatom Thalassiosira pseudonana using an extraction in phosphate buffer with Triton X-100, EDTA, dithiothreitol, polyvinyl pyrrolidone, and bovine serum albumin. NR activity in homogenates was stable for up to 1 h, but filtered samples could be stored for 96 h in liquid nitrogen without significant loss of activity. Addition of FAD to crude extracts of T. pseudonana had no effect, whereas the effect on desalted extracts or crude extracts from other species, varied from decreases in NR activity to over 250% increases. Half-saturation constants (K,) varied between species; high levels of NADH or nitrate were found to be inhibitory in some cases. These results indicate a wide diversity of forms of NR in marine phytoplankton.Under continuous, light-limited growth, NR activity was quantitatively related to calculated rates of nitrate incorporation (pN) in T. pseudonana, Skeletonema costatum, and three other diatom species examined. The relationship differed for 10 other species; NR activity was equal to bN in some cases, but higher or lower in others. In dinoflagellates, in particular, NR activity was highly correlated with pN, but accounted for ~20% of hN in Amphidinium carterae.The importance of nitrogen metabolism in general, and nitrate metabolism in particular, in the marine environment is based not only on the frequent identification of nitrogen as a nutrient limiting primary production, but also because of the important differences between the fate of production depending on whether newly available nitrogen (e.g. nitrate) or regenerated forms (e.g. ammonium) are used (Dugdale and Goering 1967;Platt et al. 1992). Thus, measurements of rates of nitrate incorporation (sensu Wheeler 1983, i.e. the combination of inorganic nitrogen into large macromolecules such as proteins and nucleic acids) by marine phytoplankton are critical to understanding rates of primary production and biogeochemical cycling in many areas of the oceans.Current methods of estimating rates of nitrate incorporation are based largely on incubation techniques with the stable isotope 15N as a tracer (Dugdale and Wilkerson 1986). It is appreciated that there are problems with this

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Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Nitrate reductase activity quantitatively predicts the rate of nitrate incorporation under steady state light limitation: A revised assay and characterization of the enzyme in three species of marine phytoplankton

Berges

Harrison

1995

Limnology & Oceanography

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“…ii) realização do ensaio sob condições ótimas de atividade, que são espécies-específi cas (Lobban & Harrison 1994) e requerem condições apropriadas como pH, temperatura e concentração de substrato (Berges 1997, Granbom et al 2004, Chow et al 2007. A adição de albumina sérica bovina (BSA) no tampão de extração pode ajudar a preservar a proteína e a atividade da NR, uma vez que este composto atua como substrato preferencial para as proteases endógenas e liga-se aos compostos fenólicos (Ingemarsson 1987.…”

Section: Introductionunclassified

Ensaio in vitro da enzima nitrato redutase e efeito da disponibilidade de nitrato e fosfato em variantes pigmentares de Hypnea musciformis (Wulfen) J. V. Lamour. (Gigartinales, Rhodophyta)

Martins¹,

Chow²,

Yokoya³

2009

Rev. bras. Bot.

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-(In vitro assay of nitrate reductase enzyme and effect of nitrate and phosphate availability in colour strains of Hypnea musciformis (Wulfen) J. V. Lamour. (Gigartinales, Rhodophyta)). The enzyme nitrate reductase (NR) catalyzes the reduction of nitrate to nitrite and controls the rate of nitrate assimilation. The in vitro assay of NR was optimized for the wild strain (brown, MA), and the phycoerythrin-defi cient strain (light-green, VC) of Hypnea musciformis. Both strains were cultured at temperature of 23 ± 2 °C, photoperiod of 14 h, irradiance of 60-90 μmol photons m -2 s -1 , with medium composed by sterilized seawater (salinity 30 psu) with 50% von Stosch's enrichment solution (VSES/2). The optimal conditions for in vitro assay of NR were: 40 μM of NADH; 10 min of incubation of crude extracts (EB), and 100 μL of EB to both strains. Optimal activity of NR occurred at 4 and 2 mM of nitrate to the VC and MA strains, respectively. The VC and MA strains showed, respectively, Michaelis-Menten constants (K M ) for NADH of 0.2068 and 0.0837 μM, and K M for nitrate of 0.0492 and 0.0294 mM. The results indicate that the NR of MA strain has higher affi nity by the substrate than the NR of VC strain of H. musciformis. Experiments on the effects of availabilities of nitrate (5 to 105 μM) and nitrate and phosphate (0.5 to 25.5 μM, with a N:P relation of 4:1) showed that NR activity of VC and MA strain did not increase with the addition of nitrate to the medium, what can be related with their nutritional state. The NR activity was higher in treatments with phosphate addition than those with only nitrate addition, indicating that this nutrient is important to metabolic processes related to the NR activity.Key words -colour strain, Hypnea, nitrate, nitrate reductase, phosphate RESUMO -(Ensaio in vitro da enzima nitrato redutase e efeito da disponibilidade de nitrato e fosfato em variantes pigmentares de Hypnea musciformis (Wulfen) J. V. Lamour. (Gigartinales, Rhodophyta)). A enzima nitrato redutase (NR) catalisa a redução do nitrato a nitrito e controla a taxa de assimilação do nitrato. O ensaio in vitro da nitrato redutase foi otimizado para a linhagem selvagem (marrom, MA) e para a linhagem defi ciente em fi coeritrina (verde-clara, VC) de Hypnea musciformis. As duas linhagens foram cultivadas em temperatura de 23 ± 2 °C, fotoperíodo de 14 horas, irradiância de 60-90 μmol fótons m -2 s -1 , e meio composto por água do mar esterilizada (30 ups) enriquecida com a solução de von Stosch na concentração de 50% (VSES/2). As condições ótimas de ensaio para ambas as linhagens foram: 40 μM de NADH; 10 min de incubação do extrato bruto (EB) e 100 μL de EB. A atividade ótima da NR ocorreu em 4 e 2 mM de nitrato para a linhagem VC e MA, respectivamente. As linhagens VC e MA apresentaram, respectivamente, constante aparente de Michaelis-Menten (K M ) para NADH de 0,2068 e 0,0837 μM, e K M para nitrato de 0,0492 e 0,0294 mM. Os resultados indicam que a NR da linhagem MA tem maior afi nidade pelo substrato do que a NR da linha...

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“…The activity of the enzyme is usually determined by colorometric assay of nitrite formation in cell-free extracts (Morris & Syrett 1965, Eppley et al 1969; the sensitivity of this assay is low unless incubations are relatively long (tens of minutes). NR activity is labile in vitro, and susceptible to proteolysis unless precautions are taken (Ingemarsson 1987). Consequently, low levels of enzyme activity are difficult to detect and preserve.…”

Section: Introductionmentioning

confidence: 99%

Rapid incorporation of 13N03 by NH4- limited phytoplankton

Zehr¹,

Capone²,

Falkowski³

1989

Mar. Ecol. Prog. Ser.

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Nitrate reductase, the enzyme which catalyzes the reduction of nitrate to nitrite, is repressed by ammonium and induced by the presence of nitrate. In oligotrophic oceans, inorganic nitrogen concentrations are low and it is believed that phytoplankton primarily use regenerated ammonium. Under these conditions, nitrate reductase activity should be reduced. We investigated the metabolism of nitrate in ammonium-limited chemostats of marine phytoplankton using the short-lived radiotracer '=N. We found that nitrate is rapidly taken up, reduced and incorporated into protein by ammonium-limited phytoplankton due to the constitutive activity of nitrate reductase. These results provide a mechanism for the utilization of episodic pulses of nitrate, which have been suggested to be responsible for a significant fraction of nitrate-based production in the open ocean.

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Nitrogen Utilization in Lemna

Cited by 34 publications

References 25 publications

Nitrate reductase activity quantitatively predicts the rate of nitrate incorporation under steady state light limitation: A revised assay and characterization of the enzyme in three species of marine phytoplankton

Nitrate reductase activity quantitatively predicts the rate of nitrate incorporation under steady state light limitation: A revised assay and characterization of the enzyme in three species of marine phytoplankton

Ensaio in vitro da enzima nitrato redutase e efeito da disponibilidade de nitrato e fosfato em variantes pigmentares de Hypnea musciformis (Wulfen) J. V. Lamour. (Gigartinales, Rhodophyta)

Rapid incorporation of 13N03 by NH4- limited phytoplankton

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