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缺氧对体外舌下神经元细胞内和细胞外钾活性的影响。

Effect of anoxia on intracellular and extracellular potassium activity in hypoglossal neurons in vitro.

作者信息

Jiang C, Haddad G G

机构信息

Department of Pediatrics, Yale University School of Medicine, New Haven, Connecticut 06510.

出版信息

J Neurophysiol. 1991 Jul;66(1):103-11. doi: 10.1152/jn.1991.66.1.103.

DOI:10.1152/jn.1991.66.1.103
PMID:1919660
Abstract
  1. A brain slice preparation was used to study the hypoglossal (XII) neuronal response to anoxia. Both intra- and extracellular potassium activities (K+i,K+o) were measured by the use of ion-selective microelectrodes, and K+ flux was assessed by the use of pharmacologic blockers. 2. Extracellular recordings showed that a short period of anoxia (4 min) induced an increase in K+o of 26.4 +/- 7.5 mM (mean +/- SD, n = 20) in the XII nucleus of adult rats. 3. Intracellular recordings (n = 31) in XII neurons showed a substantial decrease in K+i during anoxia. Fourteen neurons were analyzed in detail and these showed that XII neurons depolarized to -25.3 +/- 7.7 mV, whereas K+i dropped from 93.6 +/- 14.9 to 32 +/- 9.0 mM. These results strongly suggested that K+ is lost from XII neurons during anoxia. 4. Although the extracellular space (ECS) shrank by approximately 50% during anoxia, the possibility that the increase in K+o and decrease in K+i were mainly caused by shrinkage of the ECS and swelling of intraneuronal space was excluded to a great degree because the changes in K+i and K+o during anoxia were relatively very large. 5. To study the mechanisms by which K+ is lost from XII neurons, we used several pharmacologic blockers. High concentration of ouabain (10 mM) and strophanthidin (80 microM) increased K+o from baseline (3-4 mM) to 40.9 +/- 2.5 mM (n = 6) but did not abolish an additional anoxia-induced increase in K+o, suggesting that mechanisms other than Na(+)-K(+)-adenosine triphosphatase inhibition were also responsible for the anoxia-induced K+ leakage.(ABSTRACT TRUNCATED AT 250 WORDS)
摘要
  1. 采用脑片制备技术研究舌下神经(XII)神经元对缺氧的反应。使用离子选择性微电极测量细胞内和细胞外钾离子活性(K+i、K+o),并使用药理学阻滞剂评估钾离子通量。2. 细胞外记录显示,短时间缺氧(4分钟)可使成年大鼠XII核中的K+o增加26.4±7.5 mM(平均值±标准差,n = 20)。3. XII神经元的细胞内记录(n = 31)显示,缺氧期间K+i显著降低。对14个神经元进行了详细分析,结果表明XII神经元去极化至-25.3±7.7 mV,而K+i从93.6±14.9 mM降至32±9.0 mM。这些结果强烈表明,缺氧期间钾离子从XII神经元丢失。4. 尽管缺氧期间细胞外间隙(ECS)缩小了约50%,但由于缺氧期间K+i和K+o的变化相对非常大,因此在很大程度上排除了K+o增加和K+i降低主要由ECS收缩和神经内空间肿胀引起的可能性。5. 为了研究钾离子从XII神经元丢失的机制,我们使用了几种药理学阻滞剂。高浓度的哇巴因(10 mM)和毒毛花苷(80 microM)可使K+o从基线水平(3 - 4 mM)增加到40.9±2.5 mM(n = 6),但并未消除缺氧诱导的K+o进一步增加,这表明除了抑制钠钾ATP酶之外的其他机制也导致了缺氧诱导的钾离子泄漏。(摘要截短于250字)

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