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中枢阿片系统参与人α干扰素诱导的小鼠强迫游泳试验中的不动行为。

Involvement of central opioid systems in human interferon-alpha induced immobility in the mouse forced swimming test.

作者信息

Makino M, Kitano Y, Komiyama C, Hirohashi M, Takasuna K

机构信息

Drug Safety Research Laboratory, Daiichi Pharmaceutical Co., Ltd., Tokyo, Japan.

出版信息

Br J Pharmacol. 2000 Jul;130(6):1269-74. doi: 10.1038/sj.bjp.0703432.

Abstract
  1. We investigated the mechanism by which human interferon-alpha (IFN-alpha) increases the immobility time in a forced swimming test, an animal model of depression. 2. Central administration of IFN-alpha (0.05 - 50 IU per mouse, i.cist.) increased the immobility time in the forced swimming test in mice in a dose-dependent manner. 3. Neither IFN-beta nor -gamma possessed any effect under the same experimental conditions. 4. Pre-treatment with an opioid receptor antagonist, naloxone (1 mg kg(-1), s.c.) inhibited the prolonged immobility time induced by IFN-alpha (60 KIU kg(-1), i.v. or 50 IU per mouse. i.cist. ). 5. Peripheral administration of naloxone methiodide (1 mg kg(-1), s. c.), which does not pass the blood - brain barrier, failed to block the effect of IFN-alpha, while intracisternal administration of naloxone methiodide (1 nmol per mouse) completely blocked. 6. The effect of IFN-alpha was inhibited by a mu(1)-specific opioid receptor antagonist, naloxonazine (35 mg kg(-1), s.c.) and a mu(1)/mu(2) receptor antagonist, beta-FNA (40 mg kg(-1), s.c.). A selective delta-opioid receptor antagonist, naltrindole (3 mg kg(-1), s.c.) and a kappa-opioid receptor antagonist, nor-binaltorphimine (20 mg kg(-1), s.c.), both failed to inhibit the increasing effect of IFN-alpha. 7. These results suggest that the activator of the central opioid receptors of the mu(1)-subtype might be related to the prolonged immobility time of IFN-alpha, but delta and kappa-opioid receptors most likely are not involved.
摘要
  1. 我们研究了人类α干扰素(IFN-α)在强迫游泳试验(一种抑郁症动物模型)中增加不动时间的机制。2. 向小鼠脑室内注射IFN-α(每只小鼠0.05 - 50国际单位,脑室内注射),在强迫游泳试验中以剂量依赖方式增加了小鼠的不动时间。3. 在相同实验条件下,IFN-β和IFN-γ均无任何作用。4. 用阿片受体拮抗剂纳洛酮(1毫克/千克,皮下注射)预处理可抑制IFN-α(60千国际单位/千克,静脉注射或每只小鼠50国际单位,脑室内注射)诱导的延长的不动时间。5. 不能透过血脑屏障的甲基碘化纳洛酮外周给药(1毫克/千克,皮下注射)未能阻断IFN-α的作用,而甲基碘化纳洛酮脑室内给药(每只小鼠1纳摩尔)则完全阻断了该作用。6. IFN-α的作用被μ₁特异性阿片受体拮抗剂纳洛嗪(35毫克/千克,皮下注射)和μ₁/μ₂受体拮抗剂β-FNA(40毫克/千克,皮下注射)抑制。选择性δ阿片受体拮抗剂纳曲吲哚(3毫克/千克,皮下注射)和κ阿片受体拮抗剂去甲二氢吗啡酮(20毫克/千克,皮下注射)均未能抑制IFN-α的增加作用。7. 这些结果表明,μ₁亚型的中枢阿片受体激活剂可能与IFN-α延长的不动时间有关,但δ和κ阿片受体很可能未参与其中。

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