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Hormone release from isolated nerve endings of the rat neurohypophysis.

机译:激素从大鼠神经垂体的孤立神经末梢释放。

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摘要

1. Isolated neurosecretory nerve endings were prepared from rat neurohypophyses. The amount of vasopressin (AVP) and oxytocin released was measured by radioimmunoassay. 2. The amount of hormone release under resting conditions was not affected by external calcium (Ca2+o). Secretion decreased by ca. 50% when external sodium (Na+o) was replaced by choline or sucrose. 3. Ouabain did not modify the basal AVP release. 4. The Na+ ionophore monensin increased the release of AVP only in the presence of Na+o. This increase was maintained during prolonged exposure to the ionophore and occurred in the presence of Ca2+o only. 5. In the presence of Ca2+o, the amount of evoked hormone release was dependent on the external K+ concentration. Half-maximal activation was achieved with ca. 40 mM-K+. The K+-induced secretion was potentiated in Na+-free solution. 6. Prolonged 100 mM-K+-induced depolarization in the presence of Ca2+o gave rise to a large increase in hormone secretion which decreased with time (t1/2 = 2.5 min). The release could be reactivated after permeabilization of the nerve terminals in the presence of micromolar concentrations of Ca2+. 7. A stepwise paradigm in which Ko+ is incrementally increased to 25, 50, 75 and then 100 mM released more AVP than a prolonged exposure to 100 mM-K+. 8. Veratridine increased the amount of AVP released. This effect was considerably reduced in the absence of Nao+ and abolished in the presence of D600. 9. The depolarization-induced AVP release was blocked by different Ca2+-antagonists. Their effectiveness was nitrendipine = nicardipine greater than Cd2+ greater than Gd3+ greater than Co2+ = Mn2+. 10. The dihydropyridine Bay K 8644 potentiated both the basal and the K+-evoked AVP release. Its maximal effect was obtained with 25-50 mM-Ko+. 11. In conclusion, the isolated neurohypophysial terminals which have both Na+ and Ca2+ channels and release AVP and oxytocin upon depolarization might be an excellent system to study further the mechanisms leading to secretion of neurohormones.
机译:1.从大鼠神经垂体组织中分离出神经分泌神经末梢。通过放射免疫测定法测定释放的加压素(AVP)和催产素的量。 2.休息条件下激素释放的量不受外部钙(Ca2 + o)的影响。分泌减少约。当外部钠(Na + o)被胆碱或蔗糖代替时为50%。 3. Ouabain并未修改基本AVP版本。 4. Na +离子载体莫能菌素仅在Na + o存在下才增加AVP的释放。这种增加在长时间暴露于离子载体中得以维持,并且仅在Ca2 + o的存在下发生。 5.在Ca2 + o存在下,诱发的激素释放量取决于外部K +浓度。约半激活达到约。 40 mM-K +。在无Na +的溶液中增强了K +诱导的分泌。 6.在Ca 2+存在下,延长的100 mM-K +引起的去极化导致激素分泌的大量增加,激素分泌随时间而减少(t1 / 2 = 2.5分钟)。在存在微摩尔浓度的Ca2 +的情况下,神经末梢通透后,释放可以重新激活。 7.逐步范式,其中Ko +逐渐增加到25、50、75,然后100 mM释放的AVP高于长时间暴露于100 mM-K +。 8.藜芦定增加了AVP的释放量。在没有Nao +的情况下,这种作用会大大降低,在D600的存在下,这种作用会消失。 9.去极化诱导的AVP释放被不同的Ca 2+拮抗剂阻断。他们的效果是硝苯地平=尼卡地平大于Cd2 +大于Gd3 +大于Co2 + = Mn2 +。 10.二氢吡啶Bay K 8644增强了基础释放和K +诱发的AVP释放。用25-50 mM-Ko +可获得最大效果。 11.总之,具有Na +和Ca2 +通道并且在去极化时释放AVP和催产素的孤立的神经垂体末梢可能是进一步研究导致神经激素分泌的机制的一个极好的系统。

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