To determine if 12-h sleep deprivation disrupts neural plasticity, we compared long-term potentiation (LTP) in five sleep-deprived and five control rats. Thirty minutes after tetanus population spike amplitude increased 101 +/- 15% in 16 slices from sleep deprived rats and 139 +/- 14% in 14 slices from control rats. This significant (P < 0.05) reduction of LTP, the first demonstration that the sleep deprivation protocol impairs plasticity in adult rats, may be due to several factors. Reduced LTP may indicate that sleep provides a period of recuperation for cellular processes underlying neural plasticity. Alternatively, the stress of sleep deprivation, as indicated by elevated blood corticosterone levels, or other non-sleep-specific factors of deprivation may contribute to the LTP reduction.
Three experiments were carried out to evaluate the effects of varying levels of mineral and iodine supplements when offered to ewes in late pregnancy on lamb serum immunoglobulin G (IgG) concentrations. In experiment 1, 44 individually housed ewes were allocated to one of four treatments (no. = 11) and offered a basal diet of grass silage ad libitum which was supplemented with 500 g/day of a concentrate (190 g/kg of crude protein (CP)), in addition to mineral/vitamin fortification at the rate of 0 g (C), 17.3 g (LM), 34.6 g (MM) or 52.0 g (HM) per day for the final 7 weeks of pregnancy. The mineral/vitamin supplement contained Ca, P, Na, Mg, Mn, Se, I, Co, Mn and vitamin E. The ewes were milked at 1 h, 10 h and 18 h post partum and measured quantities of colostrum, proportional to lamb birth weight, were fed back to the lambs via a stomach tube. Treatment had no effect on total colostrum yield or total IgG yield to 18 h post partum (P > 0.05). There was a linear decrease in serum IgG concentration and IgG absorption efficiency as mineral supplementation increased (P < 0.001). In experiment 2, which was carried out in conjunction with experiment 1, 44 ewes were allocated to four treatments (no. = 11) and offered the same basal silage/concentrate diet as in experiment 1, in addition to receiving one of the following supplements : (C) control, as in experiment 1; (HM), as in experiment 1; (−I), ewes offered the same mineral/vitamin supplement as HM but with iodine excluded; (I0), ewes offered a daily mineral supplement of iodine only at a level of 40 mg per ewe, equivalent to the iodine inclusion in the 52 g of minerals offered in HM. The iodine-supplemented progeny (HM and IO) had lower (P < 0.001) serum IgG concentrations and higher soil scores (P < 0.05) than the C and −I progeny. In experiment 3, the effects of varying levels of iodine supplementation when offered to ewes during the final 6 weeks of pregnancy on lamb serum IgG values were examined. Forty-eight individually housed ewes were allocated to one of four treatments (no. = 12) and offered grass silage ad libitum, which was supplemented initially with 500 g of a concentrate (140 g/kg of CP) from days 99 to 130 of gestation and then replaced with 700 g/day of a concentrate (180 g/kg of CP) from day 131 of gestation until lambing. In addition, the diet of each ewe was supplemented on a daily basis with iodine at the rate of 0 mg (C), 8.9 mg (LI), 17.7 mg (MI) or 26.6 mg (HI). There was a negative linear reduction in serum IgG concentration and IgG absorption efficiency as maternal dietary iodine supplementation increased (P < 0.001). We conclude that supplementation of the ewe's diet in late pregnancy with 17.3 g of a mineral supplement as formulated in the current experiment lowers the lamb's ability to absorb colostral IgG, and offering only the iodine component of this mineral supplement, at a level which approximates to about one third of currently quoted toxicity levels, will result in reduced serum IgG concentration in the lamb. These findings suggest the need to re-examine current toxicity values for iodine.
The dorsal root origins of cutaneous nerves supplying the feline pelvic limb were determined electrophysiologically in 11 cats. Cutaneous nerves were surgically exposed and the presence or absence of an evoked potential in response to stimulation of individual dorsal roots was noted. The dorsal cutaneous branches of L3-L5 and S3, and the lateral cutaneous branch of L3 each arose solely from their parent spinal nerves. The L7, S1, and S2 dorsal cutaneous branches had multiple dorsal root origins. The lateral cutaneous femoral nerve originated from L3-L6 dorsal roots in 4 patterns of origin, and the saphenous nerve originated from L4-L6 dorsal roots in 2 patterns of origin. The lateral and caudal cutaneous sural nerves originated from L6-S1 roots in 2 and 3 patterns, respectively. The lateral and medial plantar nerves arose from L6-S2 roots in 4 and 2 patterns, respectively. The superficial and deep peroneal nerves originated from L6-S1 roots in 2 and 3 patterns, respectively. The caudal cutaneous femoral nerve or its branches arose from L7-S3 in 8 origin patterns. The dorsal nerve of the penis and the superficial perineal nerve arose from L7-S3 and S1-S3 roots, respectively, each in 4 patterns. A subtle correlation between plexus type and dorsal root origins of the cutaneous nerves was noted.
Cladophora is a genus of branched filamentous green algae (Ulvophyceae). It contains many species that are challenging to differentiate based on morphology because of the scarcity of diagnostic characters and extensive phenotypic plasticity. Within the past five years, Cladophora blooms have been observed on the ropes of green-lipped mussel farms in the Marlborough Sounds, New Zealand. When Cladophora reaches high biomass, it can clog mussel-harvesting equipment; thus, it is considered a nuisance organism in the region. This study used morphological and molecular techniques to identify the species responsible for the blooms, and to investigate whether this might be a recent incursion. Cladophora samples (n = 21) were collected from nine mussel farms, one salmon farm, and a marina. Morphological and phylogenetic analyses (partial large subunit and internally transcribed spacer regions 1 and 2 of the nuclear ribosomal cistron), revealed the identity of the bloom forming species as Cladophora ruchingeri (C.Agardh) Kützing, 1845. This represents the first report of this species in the Southern Hemisphere and Pacific region. Given the distinct morphology of C. ruchingeri (when mature), its absence from previous surveys of macro-algae from this region, and increasing reports of blooms, our findings suggest that this species has only recently been introduced to New Zealand. This study provides a robust taxonomic identification and initial baseline data. Further directed studies on Cladophora are required to advance knowledge on its ecology and distribution in New Zealand, and assist in the development of mitigation strategies.
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