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海马内注射破伤风毒素诱导的大鼠原发性和继发性慢性癫痫病灶中的突触抑制

Synaptic inhibition in primary and secondary chronic epileptic foci induced by intrahippocampal tetanus toxin in the rat.

作者信息

Empson R M, Jefferys J G

机构信息

Department of Physiology and Biophysics, St Mary's Hospital Medical School, Imperial College, London.

出版信息

J Physiol. 1993 Jun;465:595-614. doi: 10.1113/jphysiol.1993.sp019695.

Abstract
  1. Injecting twelve mouse minimum lethal doses of tetanus toxin into one hippocampus of a rat leads to the development of chronic epileptic foci in both hippocampi. These generate intermittent epileptic discharges for 6-8 weeks. Here we compare GABAergic inhibition, 10-18 days after injection, in slices prepared from the injected and contralateral hippocampi (respectively the primary and the secondary or 'mirror' foci), using both neurochemical and electrophysiological methods. 2. Epileptic activity was recorded from slices of both hippocampi from all tetanus toxin-injected rats. Evoked epileptic discharges were similar on the two sides, but spontaneous epileptic discharges were more common contralaterally. 3. Ca(2+)-dependent, K(+)-stimulated (synaptic) release of radiolabelled GABA was depressed in slices from the injected hippocampus, compared with vehicle-injected controls. In contrast, slices from the contralateral hippocampus had normal levels of Ca(2+)-dependent, K(+)-stimulated GABA release, even though adjacent slices were epileptogenic. 4. Intracellular recordings revealed that both fast and slow stimulus-evoked inhibitory postsynaptic potentials (IPSPs) were abolished in CA3 pyramidal cells in the primary focus. In the secondary focus, however, fast IPSPs were seen in seven of twenty-five cells, and slow IPSPs were seen in all cells if the stimulus was strong enough. 5. Monosynaptic IPSPs were isolated pharmacologically by blocking glutamatergic excitatory postsynaptic potentials (EPSPs) with 6-cyano-7-nitroquinoxaline-2,3-dione (CNQX) and D(-)-2-amino-5-phosphopentanoic acid (AP-5). No monosynaptic IPSPs were uncovered in cells from the primary focus at any stimulus strength. Monosynaptic IPSPs were evoked in all cells from both the secondary focus and control slices. The estimated conductances of monosynaptic fast IPSPs were similar in cells from the secondary focus and from the controls, although the former required twice the stimulus strength. 6. Slow IPSPs were found in the secondary focus and in controls, but not in the primary focus. They were sensitive to 3-amino-2-(4-chlorophenyl)-2-hydroxy-propylsulphonic acid (2-OH saclofen). The estimated conductances of slow IPSPs evoked by weak stimuli in the secondary focus were much smaller than in the controls. However, stimuli that could trigger epileptic discharges in the secondary focus, evoked 2-OH saclofen-sensitive slow IPSPs with estimated conductances approaching the controls. This marked increase in the slow IPSP did not occur when EPSPs, and epileptic bursts, were blocked with CNQX and AP-5, suggesting that a strong barrage of excitation is needed to generate full-sized slow IPSPs in the secondary focus.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 向大鼠一侧海马注射12个小鼠最小致死剂量的破伤风毒素,会导致双侧海马出现慢性癫痫病灶。这些病灶会产生间歇性癫痫放电,持续6 - 8周。在此,我们在注射后10 - 18天,使用神经化学和电生理方法,比较从注射侧海马和对侧海马(分别为原发性和继发性或“镜像”病灶)制备的脑片中的γ-氨基丁酸(GABA)能抑制作用。2. 记录了所有注射破伤风毒素大鼠双侧海马脑片的癫痫活动。两侧诱发的癫痫放电相似,但对侧自发性癫痫放电更为常见。3. 与注射赋形剂的对照组相比,注射侧海马脑片中放射性标记的GABA的钙依赖性、钾离子刺激(突触性)释放受到抑制。相比之下,对侧海马脑片的钙依赖性、钾离子刺激的GABA释放水平正常,尽管相邻脑片具有致痫性。4. 细胞内记录显示,原发性病灶中CA3锥体细胞的快速和慢速刺激诱发的抑制性突触后电位(IPSPs)均消失。然而,在继发性病灶中,25个细胞中有7个出现了快速IPSPs,并且如果刺激足够强,所有细胞中都能观察到慢速IPSPs。5. 通过用6 - 氰基 - 7 - 硝基喹喔啉 - 2,3 - 二酮(CNQX)和D -(-)- 2 - 氨基 - 5 - 磷酸戊酸(AP - 5)阻断谷氨酸能兴奋性突触后电位(EPSPs),从药理学上分离出单突触IPSPs。在原发性病灶的细胞中,无论刺激强度如何,均未发现单突触IPSPs。继发性病灶和对照脑片的所有细胞中均可诱发出单突触IPSPs。继发性病灶细胞和对照细胞中,单突触快速IPSPs的估计电导相似,尽管前者所需刺激强度是后者的两倍。6. 在继发性病灶和对照中发现了慢速IPSPs,但在原发性病灶中未发现。它们对3 - 氨基 - 2 -(4 - 氯苯基)- 2 - 羟基 - 丙基磺酸(2 - 羟基舒氯芬)敏感。继发性病灶中由弱刺激诱发的慢速IPSPs的估计电导远小于对照。然而,能在继发性病灶中触发癫痫放电的刺激,诱发了2 - 羟基舒氯芬敏感的慢速IPSPs,其估计电导接近对照。当用CNQX和AP - 5阻断EPSPs和癫痫爆发时,这种慢速IPSPs的显著增加并未发生,这表明在继发性病灶中需要强烈的兴奋性刺激才能产生全尺寸的慢速IPSPs。(摘要截取自400字)
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/54d6/1175448/49c618b4c652/jphysiol00417-0595-a.jpg

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