妊娠期血清微量元素的变化

目的探讨妊娠期血清微量元素的变化规律。方法以原子吸收分光光度法分别测定421例孕妇和128例正常对照妇女血清铜(Cu)、锌(Zn)、铁(Fe)等微量元素浓度和血清镁(Mg)、钙(Ca)浓度。结果血清铜(Cu)在整个孕期内无显著性变化,P>0.05;血清锌(Zn)、铁(Fe)、镁(Mg)、钙(Ca)随孕期的增加而降低,P均<0.05。结论孕妇在妊娠期内应根据不同孕期,合理补充微量元素。     

Electrical behaviour in a line of anterior pituitary cells (GH cells) and the influence of the hypothalamic peptide, thyrotrophin releasing factor

Anterior pituitary cells of the GH line, which secrete prolactin spontaneously, showed spontaneous action potential activity. Thyrotrophin releasing factor, which increases secretion in these cells, caused a prompt increase of action potential frequency. Potassium, another secretagogue, depolarized the cells and sometimes initiated a burst of action potentials at the onset of this effect. The action potentials persisted in tetrodotoxin-containing and Na-free media, but were suppressed by the Ca-channel blocker, methoxyverapamil. Moreover, elevating the extracellular Ca²⁺ concentration increased the amplitude of the action potentials. These action potentials therefore have a prominent Ca component. This endows them with a particular interest since secretory activity of these cells is known to be dependent on extracellular Ca²⁺. Ba²⁺, which can substitute for Ca²⁺ in maintaining secretion, also substituted for Ca²⁺ in the maintenance of the action potentials. In addition, Ba²⁺ prolonged action potentials remarkably: tetraethylammonium was less effective in this regard.The several parallels between known secretory behaviour and electrical phenomena encourage the view that analysis of electrical activity in anterior pituitary cells may provide useful clues to events involved in stimulus-secretion coupling and in the secretory control exerted by the brain.     

Bestimmung der enteralen Resorption hoher Calciumdosen mittels stabiler Isotope

Zusammenfassung Bei 8 gesunden Versuchspersonen (Durchschnittsalter 25,6 Jahre) wurde nach oraler Applikation von 500 mg und 1000 mg Calcium die Calcium-Resorption bestimmt. Hierzu wurde ein Doppelisotopenverfahren mit angereicherten stabilen Calciumisotopen verwendet, das, da im Gegensatz zu Radiotracermethoden jegliche Strahlenbelastung vermieden wird, uneingeschränkt anwendbar ist. Die oral verabreichten Calciumsalze wurden mit⁴⁸Ca, das intravenös injizierte CaCl₂ mit⁴⁶Ca markiert. Die Bestimmung der beiden Isotope in Serum- und Urinproben erfolgte mit Hilfe der Neutronenaktivierungsanalyse. Für die Resorptionsquote wurde, unabhängig von der Calcium-Dosis, ein Wert von 30% gefunden. Aus dem⁴⁶Ca-Gehalt im Serum wurde für das in 24 h ausgetauschte Körper-Calcium ein mittlerer Wert von 6,4±1,0 g Calcium oder 98,8±15,4 mg Ca/kg Körpergewicht berechnet.     

Decay kinetics of calcium currents in rat sensory neurones: analysis at two internal free calcium concentrations

The patch-clamp technique in whole-cell configuration was, used to investigate the kinetics of decay of calcium currents in rat sensory neurones. Whole-cell recording permitted control of the internal medium, particularly of the internal free calcium concentration, which was maintained at either 10^–9 M or 10^–6 M using a high concentration of Ca buffer. The inactivation decay of the total Ca current elicited above –10 mV was found to be faster at pCa 6 than at pCa 9. The total current contained three exponential components which were tentatively identified as the three types of Ca currents (ICa_T, ICa_N and ICa_S). Kinetic analyses indicated that the control of the inactivation process by internal Ca results from an effect on both high-threshold Ca currents, ICa_N, and ICa_S. The inactivation kinetics reported in the literature presents a large variability depending on the cell type. We propose that this variability may result from differences in the capacity of those cells to control their internal Ca.     

μ and δ opioid receptor activation inhibits ω-conotoxin-sensitive calcium channels in a voltage- and time-dependent mode in the human neuroblastoma cell line SH-SY5Y

 Ca²⁺ channel modulation by the μ opioid agonist [d-Ala², N-Me-Phe⁴, Gly⁵-ol]-enkephalin (DAGO) and the δ opiate agonists [d-Pen², d-Pen⁵]-enkephalin (DPDPE) and [d-Ala², d-Leu⁵]-enkephalin (DADLE) in cultured human neuroblastoma SH-SY5Y cells was investigated using the whole-cell variant of the patch-clamp technique. In SH-SY5Y cells, differentiated in vitro with retinoic acid, all agonists reversibly decreased high-voltage-activated, ω-conotoxin-sensitive Ba²⁺ currents in a concentration-dependent way. Inhibition was maximal with a 1 μM concentration of opiate agonists (76% with DAGO and 63% with δ agonists, when measured at 0 mV) and was characterized by a clear slow down of Ba²⁺ current activation at low test potentials. Both inhibition and slow down of activation were attenuated at more positive potentials, and could be partially relieved by strong conditioning depolarizations. Current suppression operated by both μ and δ agonists was prevented by pre-treatment of the cells with pertussis toxin. No sign of additivity was observed when δ agonists were applied to cells that were maximally activated by DAGO, suggesting that a common mechanism, involving the same type of modulating molecule, is responsible for Ca²⁺ channel inhibition promoted by activation of μ and δ opioid receptors in SH-SY5Y cells. Received: 10 October 1996 / Received after revision and accepted: 18 November 1996     

β-淀粉样蛋白对培养神经细胞的毒性作用及神经节苷脂的保护作用

向培养液中加入15mmol／L的β-AP1-40，48h后，发现原代培养的海马细胞内Ca2+的浓度明显增高，对照组为23．9±3．6（n=51）而β-AP组为36．5±15．8（n=30），两组比较P＜0．001，有非常显著性的差别。对照组的乳酸脱氢酶没有明显变化，而β－AP组在加β－AP1－4048h后乳酸脱氢酶明显增加，从52iu／L增加到105iu／L，实增加了101％。实验结果表明，β－AP1-40对培养的神经细胞有明显的毒性作用，但没有发现形态学的变化和对细胞的特异性。如在培养液中加β－AP1-40的同时再加25mg／ml的神经节苷脂（GAs）可明显减弱β-AP1-40引发的胞内Ca2+浓度和培养液中LDH浓度的升高。β-AP＋GAs组胞内Ca2+浓度为27.7±5.58，与β-AP组比较，有显著性差异（P＜0．01）。β-AP组海马细胞培养液中乳酸脱氢酶的浓度增高为101％，而β-AP-GAs组培养液中乳酸脱氢酶的浓度增高仅为67％。在NG108－15细胞上也获得了相同的结果。单唾液酸神经节苷脂虽有与GAs类似的作用，但较弱。这些实验结果指出，神经节苷脂和单唾液酸神经节苷脂均能拮抗β-AP1-40的毒性作用，从而对细胞可起到保护作用。     

Whole-cell currents from the cloned canine cardiac Na+/Ca2+ exchanger NCX1 overexpressed in a fibroblast cell CCL39

 A conventional patch-clamp technique was used to record the whole-cell current from the cloned canine cardiac Na⁺/Ca²⁺ exchanger NCX1 overexpressed in a fibroblast cell. Ca²⁺ was extracellularly applied to the Na⁺-loaded cell to activate the outward current by operating the reverse mode of NCX1. No measurable outward current was ever elicited from the nontransfected cell. Na⁺/Ca²⁺ exchange blocker 5 mM Ni²⁺ or 3 μM KB-R7943 that was applied extracellularly abolished the outward current. With 140 mM external Li⁺ (replacing Na⁺), the outward current was transient during the Ca²⁺ application. In contrast, with 140 mM external Na⁺, the outward current was maintained without any inactivation during the Ca²⁺ application. I–V relations predicted from the whole-cell clamp protocols used were obtained both before and during the Ca²⁺ application. The exchanger whole-cell currents are thus successfully detectable from NCX1 which is overexpressed in this stable transfectant system. Received: 28 February 1997 / Accepted: 9 April 1997     

Q-type Ca2+ channels are located closer to secretory sites than L-type channels: functional evidence in chromaffin cells

 This study uses a new strategy to investigate the hypothesis that, of the various Ca²⁺ channels expressed by a neurosecretory cell, a given channel subtype is coupled more tightly to the exocytotic apparatus than others. The approach is based on the prediction that the degree of inhibition of the secretory response by various Ca²⁺ channel blockers will differ at low (0.5 mM) and high (5 mM) extracellular Ca²⁺ concentrations ([Ca²⁺]_o). So, at low [Ca²⁺]_o the K⁺-evoked catecholamine release from superfused bovine chromaffin cells was depressed 60–70% by 2 μM ω-agatoxin IVA (P/Q-type Ca²⁺ channel blockade), by 3 μM ω-conotoxin MVIIC (N/P/Q-type Ca²⁺ channel blockade), or by 3 μM lubeluzole (N/P/Q-type Ca²⁺ channel blockade); in high [Ca²⁺]_o these blockers inhibited the responses by only 20–35%. At 1–3 μM ω-conotoxin GVIA (N-type Ca²⁺ channel blockade) or 3 μM furnidipine (L-type Ca²⁺ channel blockade), secretion was inhibited by 30 and 50%, respectively; such inhibitory effects were similar in low or high [Ca²⁺]o. Combined furnidipine plus ω-conotoxin MVIIC, ω-agatoxin IVA or ω-conotoxin GVIA exhibited additive blocking effects at both Ca²⁺ concentrations. The results suggest that Q-type Ca²⁺ channels are coupled more tightly to exocytotic active sites, as compared to L-type channels. This hypothesis if founded in the fact that external Ca²⁺ that enters the cell through a Ca²⁺ channel located near to chromaffin vesicles will saturate the K⁺ secretory response at both [Ca²⁺]_o, i.e. 0.5 mM and 5 mM. In contrast, Ca²⁺ ions entering through more distant channels will be sequestered by intracellular buffers and, thus, will not saturate the secretory machinery at lower [Ca²⁺]_o. Received: 23 September 1997 / Received after revision: 29 October 1997 / Accepted: 30 October 1997     

RNA阵列技术检测自发性高血压大鼠肌浆网Ca2+-ATP酶和受磷蛋白基因表达

目的:探讨肌浆网Ca²⁺-ATP酶(SERCA)和受磷蛋白(PLB)在原发性高血压发病过程中的变化特点及其相互关系。方法:提取2、4、6、8、10、12不同周龄雄性自发性高血压大鼠(SHR)和正常血压大鼠(WKY)的心室肌、血管平滑肌、肝脏和肾脏组织的总RNA,共294个样品,利用高通量RNA阵列技术(RNAarray)检测SERCA和PLB基因在不同周龄SHR和WKY中mRNA表达谱改变。结果:SHR在6、8、10、12周龄血压出现显著高于同周龄WKY(均P<0.01),10、12周龄心室肌重量／体重比出现显著增加(均P<0.01),心肌和血管平滑肌SERCA的表达在4、6、8、10、12周龄出现显著高于同周龄WKY(P<0.05或P<0.01)。PLB基因表达在两组间无显著差异(P>0.05)。心肌的SERCA与PLB表达量比值在6、8、10、12周龄出现显著大于同周龄WKY(P<0.05或P<0.01),而血管平滑肌的SERCA与PLB表达量比值在4、6、8、10、12周龄出现显著大于同周龄WKY(P<0.05或P<0.01)。结论:肌浆网SERCAmRNA表达改变及SERCA与PLB比例失常是高血压发生和发展过程中重要的分子生物学机制。     

Involvement of a Na−Ca exchange mechanism in contraction induced by low-Na solution in isolated guinea-pig aorta

The possibility of involvement of a Na–Ca exchange mechanism in the contractile responses induced by a reduction of external Na concentration ([Na]₀) has been studied in isolated guinea-pig aorta. Low-Na (11.9 mM) solution (Lisubstituted) produced a contraction in ouabain-treated muscles in the presence of phentolamine (10^–6 M). The magnitude of the contraction was dependent on the duration of the pretreatment with ouabain (2×10^–5 M). Ca-free solution, but not verapamil (10^–6 M), abolished the contraction induced by low-Na solution. The muscles were loaded with various amounts of Na by incubating the tissue with ouabain and varying [Na]₀ (11.9–148.7 mM) in the absence of Ca. The magnitude of the contractions induced in these muscles by low-Na solution containing Ca (2.5 mM) was dependent on the cellular Na content. Loss of cellular Na into low-Na solution followed a single exponential time course and the rate coefficient of Na-loss in the presence of external Ca was about twice as great as in the absence of Ca. Cellular⁴⁵Ca uptake in low-Na solution was significantly greater in Na-loaded tissues (pretreated with ouabain for 3 h) than in normal tissues. The⁴⁵Ca uptake in low-Na solution was not inhibited by verapamil. These results suggest that the contraction induced by low-Na solution is caused by a Ca influx which is dependent on internal Na (a Na–Ca exchange mechanism).