Hawgood B J, Smith J W
Br J Pharmacol. 1977 Dec;61(4):597-606. doi: 10.1111/j.1476-5381.1977.tb07553.x.
1 Phospholipase A(2)-crotapotin complex (P-C complex) isolated from the venom of Crotalus durissus terrificus induced an irreversible blockade of neuromuscular transmission when twitch tension was measured in the mouse phrenic nerve-hemidiaphragm preparation in vitro at 37 degrees C.2 A similar concentration of the phospholipase A(2) (10 mug/ml) alone did not affect neuromuscular transmission and no priming action was detected on later addition of crotapotin.3 The rate of neuromuscular blockade induced by P-C complex (15 mug/ml) was not altered by raising the frequency of nerve stimulation. Lower temperatures markedly increased the time of onset and reduced the rate of blockade (Q(10) (27-37 degrees C) of 4.4) whilst replacement of Ca by Sr in the medium prevented this activity. These latter results suggest that enzymatic activity is important in the neurotoxicity of the complex.4 A myotoxic action was shown by 30 mug/ml P-C complex and 30 mug/ml phospholipase A(2).5 P-C complex (150 mug) was injected into the tail vein of mice and the intoxicated hemidiaphragm preparation removed for intracellular recording at 25 degrees C.6 In fully intoxicated hemidiaphragms, resting membrane potentials were unaltered and endplate potentials (e.p.ps) varied in average amplitude from zero to less than 3 mV.7 Miniature endplate potential (m.e.p.p.) frequency was lower at fully poisoned endplates than at controls; the frequency rose during a 50 Hz tetanus but was unaffected by either raising external K or the application of the Ca-ionophore A23187.8 E.p.ps were recorded in partially intoxicated hemidiaphragms with (+)-tubocurarine (0.5-1.0 mug/ml) added to prevent contraction. Evoked release was abnormal as 50 Hz tetanus elicited e.p.ps of very variable amplitude, no facilitation of response was shown to paired stimuli, and tetraethylammonium (0.5 mM) failed to increase e.p.p. amplitudes.9 M.e.p.ps and e.p.ps were recorded at partially poisoned endplates in low Ca-high Mg solution. A reduction in the quantal content of evoked transmitter release was observed in comparison with controls.10 M.e.p.ps recorded at partially and at fully intoxicated endplates showed an altered amplitude distribution with a higher proportion of large potentials.11 It is concluded that P-C complex has a presynaptic site of action and may interfere with depolarization-secretion coupling at the motor nerve terminals.
1 从剧毒南美响尾蛇毒液中分离出的磷脂酶A(2)-响尾蛇毒素复合物(P-C复合物),在37℃体外小鼠膈神经-半膈肌标本中测量抽搐张力时,可诱导神经肌肉传递的不可逆阻滞。2 单独使用类似浓度的磷脂酶A(2)(10微克/毫升)不影响神经肌肉传递,且在随后添加响尾蛇毒素时未检测到引发作用。3 提高神经刺激频率不会改变P-C复合物(15微克/毫升)诱导的神经肌肉阻滞速率。较低温度显著延长了起效时间并降低了阻滞速率(27 - 37℃时的Q(10)为4.4),而用Sr替代培养基中的Ca可阻止这种活性。后一结果表明酶活性在该复合物的神经毒性中起重要作用。4 30微克/毫升的P-C复合物和30微克/毫升的磷脂酶A(2)表现出肌毒性作用。5 将P-C复合物(150微克)注入小鼠尾静脉,并在25℃下取出中毒的半膈肌标本进行细胞内记录。6 在完全中毒的半膈肌中,静息膜电位未改变,终板电位(e.p.ps)的平均幅度从零变化到小于3毫伏。7 在完全中毒的终板处,微小终板电位(m.e.p.p.)频率低于对照组;在50赫兹强直刺激期间频率升高,但不受提高细胞外K浓度或应用钙离子载体A23187的影响。8 在部分中毒的半膈肌中添加(+)-筒箭毒碱(0.5 - 1.0微克/毫升)以防止收缩,记录e.p.ps。诱发释放异常,因为50赫兹强直刺激引发的e.p.ps幅度变化很大,对成对刺激未显示反应易化,且四乙铵(0.5毫摩尔)未能增加e.p.p.幅度。9 在低Ca - 高Mg溶液中,在部分中毒的终板处记录m.e.p.ps和e.p.ps。与对照组相比,观察到诱发递质释放的量子含量减少。10 在部分和完全中毒的终板处记录的m.e.p.ps显示幅度分布改变,大电位的比例更高。11 得出结论,P-C复合物具有突触前作用位点,可能干扰运动神经末梢的去极化-分泌偶联。
