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1.
Plants of the C4 tree species, Euphorbia forbesii, Sherff and the C3 tree species, Claoxylon sandwicense Muell-Arg., were grown in a full sun and a shade environment designed to simulate the understory of their native Hawiian forest habitat. When grown under shade conditions, both species exhibited a photosynthetic light response typical of shade plants with low light compensation points and low dark respiration rates. E. forbesii, however, exhibited greater acclimation of light saturated photosynthetic rates and no evidence of photoinhibition in high light. In contrast, quantum yields for CO2 uptake and chlorophyll contents were reduced in the high-light as compared to the low-light grown C. sandwicense plants. Both species exhibited similar changes in the intercellular CO2 response curves and chloroplast whole-chain electron transport capacities, suggesting that the underlying mechanisms of light acclimation are similar. Chloroplasts of E. forbesii exhibited large changes in ultrastructure, with much greater thylakoid membrane development in low than high light. In contrast, C. sandwicense exhibited different starch contents, but otherwise similar membrane development in high and low light. The results show that E. forbesii possesses a very flexible photosynthetic apparatus which may account for its ability to survive in the understory of shaded forests.Abbreviations gs =
stomatal conductance
- HL =
high light
- LL =
low light
- Pi =
intercellular CO2 partial pressure
- PFD =
photon flux density 相似文献
2.
Respiratory responses to temperature and hypoxia in relation to burrowing depth were determined for winter- (W-C) and summer-conditioned (S-C) individuals of , , and . These bivalves occur sympatrically on sand-flats but display different sediment burrowing depths (. , <2 cm; . , 3–8 cm; . , 5–20 cm). A range depths over which daily temperature variation and O2 concentration decline rapidly from surface values. Species thermal tolerance limits were found to decrease and to be more greatly temperature compensated with burrowing depth. Oxygen consumption rate (VO2 increased with temperature to 25°C in . , but was, thereafter, regulated (Q10 1.0) up to 40°C while VO2 increased with temperature in . and . until thermally streased at 25° to 30°C. The deposit feeding . does not acclimate VO2 to temperature while . and . , both suspension feeders, show “reverse” acclimation [VO2 (W-C) < VO2 (S-C)] that conserves overwintering energy stores. The shallow burrowing . and deposit feeding . rarely experience hypoxia and are poor to non-regulators of VO2 in reduced O2 concentrations. In contrast, when winter-conditioned, . is a moderate regulator of VO2, the degree of regulation increasing in S-C individuals which are exposed to higher levels of hypoxia. 相似文献
3.
Zolmitriptan is a novel and highly selective 5-HT(1B/1D) receptor agonist used as an acute oral treatment for migraine. There are few reports regarding the in vitro metabolism of zolmitriptan. Previous studies indicated zolmitriptan was metabolized via CYP1A2 in human hepatic microsomes. In order to study the enzyme kinetics and drug interaction, the metabolism of zolmitriptan and possible drug-drug interactions were investigated in rat hepatic microsomes induced with different inducers. An active metabolite, N-demethylzolmitriptan, was detected and another minor, inactive metabolite that was reported in human hepatic microsomes was not detected in this study. The enzyme kinetics for the formation of N-demethylzolmitriptan from zolmitriptan in rat liver microsomes pretreated with BNF were 96+/-22 microM (K(m)), 11+/-3 pmol min(-1)mg protein(-1) (V(max)), and 0.12+/-0.02 microl min(-1)mg protein(-1) (CL(int)). Fluvoxamine and diphenytriazol inhibited zolmitriptan N-demethylase activity catalyzed by CYP1A2 (K(i)=3.8+/-0.3 and 3.2+/-0.1 microM, respectively). Diazepam and propranolol elicited a slight inhibitory effect on the metabolism of zolmitriptan (K(i)=70+/-11 and 90+/-18 microM, respectively). Cimetidine and moclobemide produced no significant effect on the metabolism of zolmitriptan. Fluvoxamine yielded a k(inactivation) value of 0.16 min(-1), and K(i) of 57 microM. The results suggest that rat hepatic microsomes are a reasonable model to study the metabolism of zolmitriptan, although there is a difference in the amount of minor, inactive metabolites between human hepatic microsomes and rat liver microsomes. The results of the inhibition experiments provided information for the interactions between zolmitriptan and drugs co-administrated in clinic, and it is helpful to explain the drug-drug interactions of clinical relevance on enzyme level. This study aso demonstrated that fluvoxamine may be a mechanism-based inactivator of CYP1A2. 相似文献