He-Ne激光对大鼠离体颈上神经节后神经元膜电导的影响

应用细胞内生物电记录技术 ,观测不同功率、不同照射时间的 He- Ne激光 (脉冲频率 1Hz)对大鼠离体颈上神经节后神经元快兴奋性突触后电位 (f- EPSP)期间膜电导的影响。功率密度为 2 m W/ cm2 的 He- Ne激光在照射初期 (1min～ 2 min)引起快兴奋性突触后电位 (f- EPSP)幅值增大 ,同时膜电导增大 ;而在激光照射后期 (后 3m in～8m in)引起节后神经元膜电导减少。功率密度为 5 m W/ cm2 的 He- Ne激光照射期膜电导无明显变化 .结果表明 :功率密度为 2 m W/ cm2 的 He- Ne激光照射初期引起膜电导 (Gl=34.6± 5 .4 n S)较照射前 (Gf=2 6 .8± 6 .2 n S)有明显增大 (P<0 .0 5 ) ,照射后期膜电导减少。提示 :He- Ne激光照射可能是通过两时相效应改变节后神经元膜电导来影响交感神经节内兴奋传递过程。这可能是低功率激光对神经细胞的一种作用机制。     

大鼠大脑皮层神经元上的延迟整流型钾离子单通道

延迟整流型钾通道在动作电位的复极化和时程控制以及绝对不应期的形成中充当重要角色.本文用细胞贴附式和内面向外式膜片箝技术研究了急性分离的SD大鼠大脑皮层神经元上延迟整流型钾通道的特性和阻断剂对其的作用,对推动钾通道的研究,了解皮层神经元电活动的规律有重要意义.     

青霉素致痫大鼠海马神经元单位放电特征分析

目的:观察青霉素致痫大鼠海马神经元单位放电特征。方法:24只Wistar雄性健康大鼠,随机分为正常对照组、癫痫模型组各12只。癫痫模型组用青霉素钠按6×106U/kg腹腔注射,观察癫痫发作级别,记录海马神经元单位放电。结果:正常对照组大鼠共记录到24个单位海马神经元放电,放电频率以中低频放电为主,放电形式以单个不均匀放电为主;癫痫模型组共记录到78个单位海马神经元放电,放电频率以高频放电为主,放电形式则以混合型放电为主,癫痫发作程度强。癫痫模型组与正常对照组比较,海马神经元单位放电数、放电频率以及放电形式均有显著性差异(P0.01);结论:青霉素诱导的癫痫模型,海马神经元单位放电数明显增多,放电频率高,并以混合型爆发放电为主。     

新生SD大鼠皮质神经元的体外培养和鉴定

目的：建立高纯度的新生SD大鼠皮质神经元原代培养方法。方法：取24h内的新生SD大鼠皮质,用木瓜酶和DNaseⅠ共同消化,5％胎牛血清终止消化,吹打分离组织获得单细胞悬液,进行细胞计数,用无血清DMEM／F12种植培养,4h后换成用无血清Neurobasal配制的维持培养液继续培养,尼氏小体染色和免疫荧光法鉴定神经元的纯度。结果：培养第10d,神经元胞体饱满,结构清晰完整,光晕明显,折光性强,可见粗长的树突和轴突,相邻细胞形成紧密网状联系,神经元纯度达到96％以上。结论：经改良和优化,无须添加阿糖胞苷抑制胶质细胞的生长即能够获得生长状态良好、高纯度的神经元。     

经验改变大鼠听皮层神经元的特征频率

应用常规电生理学技术,以神经元的特征频率和频率调谐曲线为指标,研究大鼠听皮层神经元特征频率的可塑性. 结果表明,在给予的条件刺激频率和神经元特征频率相差1.0 kHz范围内,条件刺激可诱导50%以上神经元特征频率发生完全偏移,并可分为向频率调谐曲线的低频端偏移、高频端偏移,或两侧均可偏移三种类型. 其中,神经元的特征频率高、Q₁₀-dB值大和频率调谐曲线对称指数大于零的神经元,其特征频率偏向频率调谐曲线高频端的概率更高. 结果提示,经验可改变大鼠听皮层神经元的特征频率,为深入研究中枢神经元功能活动可塑性的机制提供了重要实验资料.     

阿糖胞苷对大鼠海马神经元原代培养的影响

目的：探讨在大鼠海马神经元原代培养过程中,阿糖胞苷对培养神经元的影响。方法：将新生24 h大鼠,分离出海马组织,进行原代海马神经元培养,再将细胞分为阿糖胞苷组和对照组,阿糖胞苷组加入1μmol/L阿糖胞苷,通过检测神经元特异性标志物微管相关蛋白-2（Map-2）计算培养神经元的数量,通过台盼蓝染色法观察细胞的存活率。结果：培养第7天,阿糖胞苷组神经元数量为（11±3）个,对照组为（10±4）个,两组无明显差异;阿糖胞苷组神经元细胞在培养第14天时存活率为74%,培养第21天时存活率为49%,而对照组神经元14天时存活率为96%,21天存活率为88%,两组神经元存活率差异明显。结论：原代培养海马神经元时,阿糖胞苷对神经元产量及形态影响不明显,但是由于阿糖胞苷的毒性作用,明显缩短神经元的存活时间,影响长期培养神经元的存活率。     

谷氨酸促进大鼠海马神经元的内钙升高

谷氨酸能影响大鼠海马神经元胞内钙信号的变化,进而影响海马神经元神经冲动的发放和学习记忆过程。运用荧光测钙技术实时监测了大鼠海马神经元内钙信号的动态变化,同时分析了谷氨酸对其胞内钙信号的影响。试验表明：谷氨酸能够显著提高胞内游离钙离子的浓度;细胞外钙离子的存在、谷氨酸刺激时间及刺激频率的增加都能引起胞内钙信号不同程度的升高;但谷氨酸的过度刺激会引起钙离子浓度的超负荷,从而导致神经元结构和功能的损坏。     

“缺血”对大鼠大脑皮层神经元钙通道的影响

在急性分离的大鼠大脑皮层神经元上,用细胞贴附式膜片钳技术研究了在缺血状态下,膜Ｌ－和Ｎ－型钙通道的开关动力学变化。与对照组相比,在缺血状态下,Ｌ－型钙通道开放时间常数τ２由２．４７ｍｓ增加至１０．８１ｍｓ,关闭时间常数τ２由５０．７４ｍｓ缩短到１８．４２ｍｓ,开放概率由０．０６１增加到０．１８６（Ｐ均＜０．００１）,Ｎ－型钙通道开放时间常数τ２由１．７６ｍｓ增加到４．１３ｍｓ,关闭时间常数τ１和τ２分别由１．９６ｍｓ和５８．１７ｍｓ缩短到０．６１ｍｓ和９．５０ｍｓ,开放概率由０．０５３增加到０．１９３（Ｐ＜０．０１和０．００１）。钙通道的长时间开放可能对脑缺血胞内钙聚集起重要作用,加重缺血神经元的损伤     

大鼠海马神经元突触超微结构的增龄变化

目的为研究脑老化过程中学习、记忆功能减退的神经结构基础提供实验依据。方法应用透射电子显微镜,观察比较从出生1 d至24月龄（1 d、1月龄、3月龄、6月龄、18月龄、24月龄）的Sprague Dawley大鼠海马神经元突触超微结构的随增龄变化,同时观察与脑老化密切相关的指标脂褐素沉积。结果在大鼠6月龄之前,随着月龄的增加,海马神经元突触超微结构的发育逐渐完善,至6月龄大鼠突触数量明显增多;此后突触数量逐渐减少,至24月龄大鼠神经元突触数量最少。从1月龄开始海马神经元内即可见少量脂褐素颗粒沉积,随着月龄的逐渐增加,至24月龄时脂褐素颗粒沉积显著。结论青年期大鼠的海马神经元突触发育最好,进入老年期后,突触结构受损,老年期损伤最为严重,同时伴有大量的脂褐素颗粒沉积。     

大鼠海马触液神经元的分布特征及其纤维联系

本文应用ＨＲＰ追踪与电镜结合的方法研究了大白鼠海马接触脑脊液神经元的分布特征和皮质内联系。光镜观察在海马的多形细胞层和锥体细胞层等处可见散在的神经元被标记,而在室管膜层标记的细胞较多,它们分布于交织成网的阳性纤维中。透射电镜可见海马室管膜层的ＨＲＰ反应阳性的神经细胞、树突末稍及神经胶质细胞。在海马室管膜上也见到了被标记的神经纤维。同时在海马室管膜层内还发现未标记的阴性轴突与被ＨＲＰ标记的阳性树突构成的轴－树突触。上述结果提示海马为接触脑脊液神经元存在的部位之一,其接触脑脊液神经元并受到其它神经元的突触调控     

Transmission pathways in the rat superior cervical ganglion

On isolated preparations of the superior cervical ganglion (SCG, n = 8) taken from 21-day-old rats, we studied the intraganglion pathways and mechanisms underlying generation of synaptic responses of SCG neurons to antidromic stimulation. One of the three nerves connected with the SCG was stimulated, and compound action potentials were recorded simultaneously from the other two nerves; then, the order of stimulated and recorded nerves was changed. Orthodromic stimulation of the cervical sympathetic nerve (CSN) evoked responses in the internal carotid nerve (ICN), which could be completely blocked by hexamethonium, and responses in the external carotid nerve (ECN), which contained a component that was not blocked by this of the ECN caused responses in the CSN, which were not blocked by hexamethonium. Effects of superfusion of the SCG with a Ca²⁺-free solution allowed us to conclude that the hexamethonium-insensitive component of the responses in the CSN and ECN and ECN-CSN conduction can be explained by the presence of direct fibers going from the CSN to the ECN with no synaptic relay. Possible mechanisms underlying antidromic stimulation-induced synaptic responses in SCG neurons are discussed. Neirofiziologiya/Neurophysiology, Vol. 39, Nos. 4/5, pp. 396–399, July–October, 2007.     

Changes in the intracellular calcium concentration upon activation of rat superior cervical ganglion neurons

Changes in the intracellular calcium concentration induced by activation of neurons of the isolated intact rat superior cervical ganglion were recorded. It is concluded that stimulation within the physiological range of frequencies can effectively increase the intracellular calcium concentration in these neurons. Neirofiziologiya/Neurophysiology, Vol. 39, Nos. 4/5, pp. 400–402, July–October, 2007.     

Expression of vitamin D receptors in the superior cervical ganglia of rats

We investigated the role of vitamin D in the sympathetic nervous system including the distribution of vitamin D receptors (VDR), 1α-hydroxylase and 24-hydroxylase (CYP24) in neuronal subpopulations and satellite glia in the superior cervical ganglia (SCGs) of rats using immunohistochemistry. VDR immunoreactivity was observed in the cytoplasm and nucleus of nearly all neurons in the SCG. Intensity of VDR fluorescence was significantly greater in the cytoplasm of neuropeptide Y (NPY) negative somata compared to NPY positive neurons. Immunoreactivity for 1α-hydroxylase also was observed in the cytoplasm of all neurons of the SCG, but the intensity of fluorescence was less in the nuclei. To the contrary, the immunoreactivity for CYP24 was stronger in the nuclei, although it was present at lower intensity also in the cytoplasm of neurons. VDR and 1α-hydroxylase immunofluorescence was observed in many non-neuron cells, except satellite glial cells, which exhibited weak CYP24 immunofluorescence. Expression of VDRs and key metabolizing enzymes indicated the importance of vitamin D in the autonomic nervous system and the ability of sympathetic neurons to activate and deactivate vitamin D for its autocrine and paracrine roles.     

Evidence for transsynaptic regulation of neuronal cell surface heparan sulfate proteoglycan in developing rat superior cervical ganglion

The effect of neonatal deafferentation on the expression of a neuronal cell surface heparan sulfate proteoglycan (HeS-PG) was investigated in the developing rat superior cervical ganglion. Two monoclonal antibodies, one directed against the core protein of HeS-PG, and one to a determinant associated with a heparan sulfate side-chain, were used to monitor postnatal increases of HeS-PG by radioimmunoassay. Following neonatal deafferentation by section of the cervical sympathetic trunk, total protein per ganglion was slightly reduced at survival times of 7, 14, and 30 days. Expression of the core protein determinant on HeS-PG was not altered in deafferented ganglia. In contrast, levels of side-chain determinant were significantly reduced at 14 and 30 days. These results suggest that processing of HeS-PG side-chains by principal ganglionic neurons is partially regulated by transsynaptic influences during development. Transsynaptic regulation of neuronal development may be a more general process than was believed previously, with effects not limited to molecules associated with synaptic development.     

Monoamine storage sites in the rat superior cervical ganglion following synthesis inhibition

Summary Monoamine storage sites in paraganglionic (PG-)cells of the rat superior cervical ganglion were investigated by electron and fluorescence microscopy following treatment with p-chlorophenylalanine (pCPA), disulfiram or guanethidine respectively.Dense core vesicles in PG-cells are significantly decreased (p< 0.001) in number following pCPA, and in the majority of these cells following disulfiram and guanethidine. However in a minor portion of PG-cells the latter agents cause an increase in number and in size of dense core vesicles, in parallel with structural alterations. In agreement with these electron microscopic findings fluorescence microscopic and cytophotometric evaluations reveal a general decrease in catecholamine content with few cells showing an increase.The findings provide a morphological basis for the assumption, that monoamine storage sites in PG-cells can be decreased by inhibition of monoamine synthesis, following administration of pCPA, disulfiram and guanethidine. However the two types of responses of PG-cells which occur after disulfiram and guanethidine demonstrate a functional heterogeneity of this cell system in the rat superior cervical ganglion which is discussed.Supported by Deutsche Forschungsgemeinschaft — Grant He 919/1.I like to thank Prof. Arnold, Tübingen, for the kind disposal of cytophotometric equipment.     

Appearance of retrogradely labeled neurons in the rat superior cervical ganglion after injection of wheat-germ agglutinin-horseradish peroxidase conjugate into the contralateral ganglion

Summary Injection of wheat-germ agglutinin-horseradish peroxidase conjugate (WGA-HRP) into the superior cervical ganglion (SCG) of the rat results in accumulation of WGA-HRP in sympathetic postganglionic neurons in the contralateral SCG. The sympathetic pathways involved and the mechanism underlying the labeling were investigated. The labeling in neurons in the contralateral SCG was apparent 6 h after injection and increased in intensity with longer survival times. The number of labeled neurons reached 1300 at 72 h after the injection. Transection of the external (ECN) or internal carotid nerves (ICN) resulted in considerable reduction in the number of labeled neurons. Combined transection of both ECN and ICN virtually eliminated labeling in the contralateral SCG. This provides strong evidence that these two nerves are the major pathways for WGA-HRP transport out of the SCG. No labeling was observed in the contralateral SCG following injection of horseradish peroxidase (HRP). Therefore, it seems unlikely that a direct nerve connection exists between the bilateral ganglia. Instead, the labeling of contralateral SCG neurons appears to depend on the transneuronal transport capacity of WGA-HRP, which conveys the marker in an anterograde direction along the postganglionic fibers to terminals in sympathetic target organs, and then delivers it transneuronally to contralateral SCG neurons. We suggest that the sympathetic nerve fibers originating in the bilateral SCGs run intermingled and are in close contact in their peripheral target organs.