电针对庆大霉素耳毒性的预防作用

目的和方法 :本实验用耳廓反射 (PR)、脑干听觉诱发电位 (BAEP)、组织化学方法 ,观察电针疗法对豚鼠庆大霉素 (GE)耳毒性的防治作用 ,并探讨其机制。结果 :电针疗法能降低GE引起的PR阈值和BAEP反应阈的上移幅度及BAEP波峰潜伏期和波峰间期的延长 ,能维持毛细胞溶酶体的完整 ,防止毛细胞的自溶性破坏。结论 :电针疗法有对抗GE耳毒性作用。维持耳蜗毛细胞内溶酶体完整 ,防止溶酶体内水解酶的逸出而发生细胞自溶 ,可能是电针疗法的作用机制之一。     

豚鼠庆大霉素耳中毒后诱发的耳蜗热休克反应

目的：探讨热休克蛋白（HSP）70在庆大霉素（GM）耳中毒中的意义。方法：应用SABC免疫组化技术及图像分析技术并结合听脑干反应（ABR）测试。观察庆大霉素耳中毒后热休克蛋白70在豚鼠耳蜗中表达及其与听阈的关系。结果：实验组耳蜗Corti‘s器、血管纹、螺旋韧带、螺旋缘、螺旋神经节细胞HSP70表达呈强阳性。且ABP阈值变化与HSP70表达的变化高度相关（｜γ｜＞0．8,P＜0．01）。结论：庆大霉素耳中毒后能够诱发耳蜗热休克反应,增加HSP70在豚鼠耳蜗的表达,保护听力。     

脑细胞生长肽对GM耳毒性的预防作用

目的：观察脑细胞生长肽（cerebral cell growth peptide,CCGP)对庆大霉素（gentamicin,GM)引起的豚鼠耳中毒的预防作用）。方法：用脑干听觉诱发电位（brainstem auditory evoked potential,BAEP)和组织化学方法分别检测动物听阀的变化和耳蜗毛细胞线粒体内琥珀酸脱氢酶（succinate dehydrogenase,SDH)及溶酶体内的酸性磷酸酶（acid phosphatase,ACP)活性变化,并在三组动物进行耳蜗受损毛细胞计数。结果：CCGP能降低GM引起的BAEP反应阈的上升幅度,保护耳蜗毛细胞SDH和维持溶酶体的完整性,减轻毛细胞的损伤。结论：CCGP能降低GM的中毒性;保护耳蜗毛细胞SDH,维持毛细胞的能量代谢,减少溶酶体损伤,降低溶酶体内水解酶逸出引起的毛细胞自溶性损伤,可能是CCGP预防GM耳毒性的机制之一。     

丹参注射液对庆大霉素耳中毒豚鼠耳蜗氧自由基生成的影响

目的:研究丹参注射液(SM)对庆大霉素(GM)耳中毒豚鼠耳蜗氧自由基生成的影响,探讨SM对GM耳毒性损伤的保护作用及其机制.方法:检测豚鼠耳蜗组织中超氧化物歧化酶(SOD)活力和丙二醛(MDA)含量,结合听性脑干反应(ABR)测试及透射电镜技术.结果:经GM处理的耳蜗组织中SOD活力明显下降,MDA含量则明显增加(P＜0.01),且与ABR阈值升高高度相关(|r|＞0.8,P＜0.05).同时接受SM的动物,其耳蜗组织中SOD活力明显升高(P＜0.01),MDA含量则明显减少(P＜0.05),且听功能显著改善.电镜观察显示耳蜗形态学改变与听力变化相一致.结论:氧自由基及其引发的脂质过氧化参与了GM耳中毒过程,SM可通过提高耳蜗组织中SOD活力,防止脂质过氧化,减轻GM的耳蜗毒性,改善听功能.     

丹参注射液对庆大霉素耳中毒豚鼠耳蜗NOS异构体表达的影响

目的：研究丹参注射液（SM）对庆大霉素（GM）耳中毒豚鼠耳蜗一氧化氮合酶（NOS）异构体表达的影响,探讨SM对GM耳毒性的防护机制。方法：40只豚鼠随机分成对照组、GM组、SM组和GM＋SM组,应用SABC免疫组织化学方法及显微图像分析技术,观察NOS三型异构体在豚鼠耳蜗的表达;同时结合听脑干反应（ABR）测试,观察用药前后豚鼠听阈的变化。结果：GM＋SM组豚鼠耳蜗诱导型NOS（iNOS/NOSⅡ）表达和ABR阈值均明显低于GM组（P〈0.01）;且iNOS表达变化与ABR阈值改变高度相关（｜r｜〉0.7,P〈0.01）;而各组豚鼠耳蜗神经元型NOS（nNOS/NOSⅠ）和内皮型NOS（eNOS/NOSⅢ）表达均无显著性差异。结论：SM对GM耳中毒后豚鼠耳蜗nNOS和eNOS表达无影响,但可通过抑制GM所致iNOS高表达,以减少NO的过量生成,从而对GM的耳毒性损伤发挥防护作用。     

丹参注射液对庆大霉素耳中毒豚鼠耳蜗血管纹NOS活性的影响

目的：研究丹参注射液（SM）对庆大霉素（GM）耳中毒豚鼠耳蜗血管纹一氧化氮合酶（NOS）活性的影响及其与听阈的关系,探讨SM对GM耳毒性损伤的保护作用。方法：应用NADPH－黄递酶（NADPH-d）组织化学染色以及图象分析技术,并结合听性脑干反应（ABR）测试。结果：SM－GM组耳蜗血管纹NOS活性和ABR阈值均明显低于GM组（P＜0.01）;且各组NOS活性变化与ABR阈移高庆相关（rcontrol=-0.9464;rGM=-0.9117;rSM GM=-0.8958,P＜0.01）。结论：SM可通过降低耳蜗血管纹NOS活性以减轻GM的耳毒性损伤,从而改善听功能。     

豚鼠庆大霉素耳中毒后HSP70 mRNA的表达

为探讨热休克蛋白(heatshockprotein,HSP)70mRNA在庆大霉素(gentamicin,GM)耳中毒中的意义,本实验选用耳廓反射灵敏的健康白色红目豚鼠(200~250g)20只,雌雄不拘,随机分成两组,每组10只。实验组动物每日腹腔注射GM100mg/kg;对照组动物每日腹腔注射与GM等量的生理盐水2.5ml/kg。两组动物混合饲养,均连续用药10d。在用药前1天和停药后第1天进行听脑干反应(auditorybrainstemresponse,ABR)测试。各组豚鼠在行第二次ABR检测后,应用原位杂交及图像分析技术观察GM耳中毒后HSP70mRNA在豚鼠耳蜗中表达。结果显示:实验组耳蜗ABR阈值明显高于对照组,有显著性差异(P<0.01);实验组豚鼠耳蜗血管纹、螺旋韧带、螺旋神经节细胞HSP70mRNA表达呈强阳性,其平均灰度值较正常对照组明显减小(P<0.001),即GM能显著增强耳蜗HSP70mRNA的表达。结果提示,GM中毒后,动物可能通过增加HSP70mRNA在耳蜗的表达,起保护听力的作用。     

抗癌药顺铂耳毒性机制及防治方法的研究进展

顺铂是目前临床上常用的广谱抗癌药之一,但它具有较强的肾及耳毒性,限制了它的大剂量应用及更好地发挥疗效。对于顺铂的肾毒性,目前已有了较好的防护措施。因此,顺铂耳毒性的产生机制及防护办法就成为当前人们关心的热点。从目前国内外的研究资料来看,在顺铂耳毒性的防护措施方面,虽也找到了一些能显著改善其毒性的药物,但其毒性很可能是多途径作用的结果,因此,应选用不同拮抗机制的多种药物联合应用,以达到最佳的防治效果。     

ATP抗庆大霉素耳毒性效果的研究

伴随着氨基糖甙类抗生素的问世及其在临床的广泛应用,人们就几乎同时开始了对其毒性尤其是耳毒性的研究。过去一直认为内耳毛细胞作为一种高度分化的感觉上皮细胞受到损伤后会造成永久的不可逆的听力损失。但随后的研究发现由氨基糖甙类抗生素所造成的听力损伤是可以改善甚至恢复的。近年有资料提示,鸟类甚至哺乳类动物的毛细胞是可以再生的。因此,究竟是何种因素在毛细胞损伤的过程中具有保护作用,并促进受损毛细胞听觉功能的恢复便日益引起研究者们的广泛重视。ＡＴＰ这一影响,许多重要生理功能的高能化合物自被发现并提取以来,便是生命科…     

庆大霉素对豚鼠耳蜗一氧化氮合酶活性的影响

目的：研究庆大霉素（ＧＭ） 致聋豚鼠耳蜗一氧化氮合酶（ＮＯＳ） 的分布及其变化,探讨一氧化氮（ＮＯ） 与ＧＭ 耳毒机制的关系。方法：ＮＡＤＰＨｄ 酶组化方法及显微图像分析技术。结果：ＧＭ 致聋后,ＮＯＳ 阳性反应物密度在血管纹、内毛细胞、外毛细胞、螺旋神经节、听神经纤维的分布均比对照组明显增高（ Ｐ＜ ０ ．００１）;上述部位的ＮＯＳ平均灰度值降低与对照组相比有显著差异（ Ｐ＜ ０ ．００１）;ＡＢＲ 听阈变化与ＮＯＳ平均密度及灰度值变化高度相关（ 上述各部位ｒ 值范围,ｒ密度听阈：０ ．９１４０～０．８６９８;ｒ灰度听阈：－０ ．７８９２ ～－ ０．９３４７;Ｐ＜ ０．０１）。结论：①ＮＯ 可能与ＧＭ的耳毒作用机制有关,是耳毒作用的重要因素之一;②ＧＭ 耳毒作用部位不仅发生在血管纹和外毛细胞,而且还涉及到内毛细胞、螺旋神经节及听神经纤维     

刺五加注射液对豚鼠庆大霉素耳毒性拮抗作用的实验研究

目的：探讨中药刺五加注射液（ASS）对庆大霉素（GM）耳毒性作用的影响及其机制。方法：豚鼠随机分成对照组、GM组、ASS4-GM组和ASS组。采用听性脑干反应（ABR）、透射电镜技术（TEM）、Western blot方法观察用药前后豚鼠的ABR阈值、形态学变化及caspase-3的表达情况。结果：用药后GM组ABR阈值明显升高;ASS组ABR阈值与对照组相比无显著性差异,与GM组和ASS4-GM组相比明显降低。透射电镜观察用药后GM组毛细胞损伤严重,出现了凋亡的形态学特征,而ASS4-GM组损伤较轻。Western blot结果表明用药后GM组豚鼠caspase-3表达明显增加;ASS4-GM组caspase-3的表达稍有升高。结论：刺五加注射液对庆大霉素耳毒性具有拮抗作用,其机制可能是通过抑制caspase-3的表达来实现的。     

Protective effect of alpha-linolenic acid on gentamicin-induced ototoxicity in mice

Alpha-linolenic acid is one of the fatty acids known as omega 3. Previous studies have shown the antioxidant and anti-inflammatory effects of alpha-linolenic acid, which prevented cell damage by inhibiting apoptotic pathway. Also, it is known that gentamicin activates apoptotic mediators and causes necrosis in the kidney. Due to this reason, we planned a study to evaluate the protective effects of alpha-linolenic acid on gentamicin induced ototoxicity by evaluating inflammation and apoptotic mediators. For this purpose, 100?mg/kg gentamicin (i.p; intraperitoneally) and 200?mg/kg alpha-linolenic acid (gavage) are administered to mice for 9?days. On 9th and 10th days, rotarod performance was assessed to test the effect of gentamicin and alpha-linolenic acid treatment on the motor coordination of mice. Gentamicin treatment decreased fall latency of mice and gentamicin treatment together with alpha-linolenic acid increased fall latency of mice. Gentamicin treatment also increased expression of phospholipase A2(plA2), cyclooxygenase-2(COX-2) and inducible nitric oxide syntheses (iNOS). Furthermore, it increased Bax and caspase-3, which are proapoptotic proteins and decreased bcl-2 that is an antiapoptotic protein. Gentamicin treatment together alpha-linolenic acid recovered the change of expression of these enzymes. In conclusion, this study showed that alpha-linolenic acid will be useful to prevent gentamicin-induced ototoxicity by inhibiting apoptosis and inflammation.     

Antiradiation effects of leucynferon on dogs and guinea pigs

In experiments with two species of animals (dogs, guinea pigs) irradiated with sublethal and lethal doses of gamma-rays, it was observed, that leucynferon had antiradiation effect. Course of injections: dogs--8 injections subcutaneus: 2.0 ml (1, 3, 5, 8, 12, 14, 21, 34 days after irradiation); guinea pigs--14 injections subcutaneus, 0.2 ml (1-14 days after irradiation). Therapeutical effect was explained by capacity of the preparation to defend the hemopoietic organs from the radiation and to stimulate hemopoiesis. Leucynferon hindered the development of acute radiation sickness symptoms. Immunoreactivity of dogs and guinea pigs in experimental group was more complete and restored faster. The growth of the automicroflora on the skin was restrained. Production of interferon-gamma (which is a function of T-lymphocytes) was restored faster.     

氯离子通道阻断剂对豚鼠耳蜗螺旋动脉平滑肌细胞兴奋性接头电位的影响

血管平滑肌细胞膜上存在氯离子通道,不仅参与调节平滑肌细胞的肌原性紧张,而且参与多种血管床的神经平滑肌细胞之间的信息传递,但氯离子通道及其阻断剂对耳蜗螺旋动脉（spiral modiol arartery,SMA）平滑肌细胞兴奋性接头电位（excitatory junction potential,EJP）是否有影响,尚不清楚。本实验运用细胞内微电极记录技术,在豚鼠耳蜗SMA离体标本上,研究氯通道阻断剂（niflumic acid,NFA,indanyloxyacetic acid 94,IAA-94;disodium 4,4’-diisothiocyanatostilbene-2．2’-disulfonate,DIDS）对去甲肾上腺素（norepinephrine,NE）引起SMA平滑肌细胞去极化反应和平滑肌细胞EJP的影响。结果显示,多数SMA平滑肌细胞在适宜的刺激下,通过神经兴奋传递产生EJP（75％,n=49）。在联合使用α1（prazosin,0．1-1 μmol／L）,α2（idazoxan,0．3-1μmol／L）和P2x（PPADS,10-100μmol／L）受体拮抗剂时,所产生的EJP幅值仅有30％-80％被抑制。在使用上述拮抗剂的基础上,NFA（10-1000μmol/L）能进一步抑制EJP,而且缩短EJP的时程。减少细胞外氯离子浓度（由135．6mmol／L减少到60mmol／L）,在同样刺激强度下激起的EJP的幅度和时程均增加,低氯的这一作用可被IAA-94和DIDS所反转。NFA和IAA-94也可进一步抑制α1、α2和β受体拮抗剂联合使用不能消除的NE（1—50μmol／L）引起的去极化反应。结果提示：NE可能通过激活一类非α、非β肾上腺能受体（可能属于γ肾上腺能受体）引起氯离子通道开放,增加氯离子电导,调节耳蜗SMA平滑肌细胞的生理活动。     

Protein-mediated assembly of succinate dehydrogenase and its cofactors

Abstract

Succinate dehydrogenase (or complex II; SDH) is a heterotetrameric protein complex that links the tribarboxylic acid cycle with the electron transport chain. SDH is composed of four nuclear-encoded subunits that must translocate independently to the mitochondria and assemble into a mature protein complex embedded in the inner mitochondrial membrane. Recently, it has become clear that failure to assemble functional SDH complexes can result in cancer and neurodegenerative syndromes. The effort to thoroughly elucidate the SDH assembly pathway has resulted in the discovery of four subunit-specific assembly factors that aid in the maturation of individual subunits and support the assembly of the intact complex. This review will focus on these assembly factors and assess the contribution of each factor to the assembly of SDH. Finally, we propose a model of the SDH assembly pathway that incorporates all extant data.     

Mechanism of neurotensin-induced pressor effect and tachycardia in guinea pigs

Neurotensin (NT) was found to produce a dose-dependent increase of the systolic and diastolic blood pressure, and of the heart rate in anesthetized guinea pigs when injected intravenously (i.v.) as a bolus, or when infused i.v. over a 15 min period. In a small percentage (20%) of animals, bolus injections of NT evoked triphasic variations (e.g. increase followed by a decrease and a further increase) of the blood pressure associated with unpredictable changes of heart rate. The pressor effect of NT was consistently reduced by prior treatment of the animals with pentolinium, a ganglion blocking agent, a mixture of alpha and beta adrenergic receptor blocking drugs, reserpine, a drug known to deplete adrenergic neurons of their neurotransmitters, or guanethidine, a drug known to paralyse adrenergic neurons. NT-induced tachycardia was either unchanged or slightly potentiated following the administration of the latter autonomic blockers. Neither the pressor effect nor the tachycardia evoked by NT was affected by antihistaminics, antiangiotensin or by indomethacin, an inhibitor of prostaglandin synthesis. These results suggest that the pressor effect of NT in anesthetized guinea pigs is likely the result of an interaction (most likely an activation) between the peptide and the sympathetic nervous system. The increase of heart rate induced by NT appears to be due to a direct effect on the heart.     

Differential effects of tryptophan on glucose synthesis in rats and guinea pigs.

1. Tryptophan inhibition of gluconeogenesis in isolated rat liver cells is characterized by a 20 min lag period before linear rates of glucose output are attained. 2. Half-maximal inhibition of gluconeogenesis in isolated rat hepatocytes is produced by approx. 0.1 mM-tryptophan. 3. Tryptophan inhibits gluconeogenesis from all substrates giving rise to oxaloacetate, but stimulates glycerol-fuelled glucose production. 4. Gluconeogenesis in guinea-pig hepatocytes is insensitive to tryptophan. 5. Changes in metabolite concentrations in rat liver cells are consistent with a locus of inhibition at the step catalysed by phosphoenolpyruvate carboxykinase. 6. Inhibition of gluconeogenesis persists in cells from rats pretreated with tryptophan in vivo. 7. Tryptophan has no effect on urea production from alanine, but decreases [1-14C]palmitate oxidation to 14CO2 and is associated with an increased [hydroxybutyrate]/[acetoacetate] ratio. 8. These results are discussed with reference to the control of gluconeogenesis in various species.