环磷酰胺对大鼠睾丸生精细胞凋亡的影响

观察环磷酰胺对大鼠睾丸组织学变化和生精细胞凋亡影响。用清洁级性成熟的15周龄雄性sD大鼠16只,体重300-350g。大鼠随机分为对照组和实验组,每组8只,实验组大鼠腹腔注射环磷酰胺,每天一次20mg／（kg·体重）,连续5d,对照组注射等量生理盐水;用药后两个月,以3％戊巴比妥钠（30mg／kg）麻醉,摘取一侧睾丸称重,4％多聚甲醛固定24h;     

海参精囊提取物对环磷酰胺诱导生殖系统受损小鼠 生精功能的影响*海参精囊提取物对环磷酰胺诱导生殖系统受损小鼠 生精功能的影响*

目的：本文旨在探讨海参精囊提取物对环磷酰胺诱导的生殖系统受损小鼠生精功能的保护作用。方法：昆明小白鼠随机分组,除正常组用生理盐水外其他各组均腹腔注射环磷酰胺（CP,28mg／kg）,每天1次,连续5天,复制生殖系统受损、雄激素部分缺乏模型;同时治疗组每天灌胃不同剂量的药物1次,连续4周,记录小鼠的体重并观察其精神状态。计算精子总数、运动率、畸形率及睾丸组织中T-S0D酶活力,并与模型组进行比较。结果：相较于模型组小鼠,虽海参精囊提取物高低剂量间无明显差异（P〉0．05）,但治疗组小鼠的精子总数、运动率、畸形率和T-SOD酶活力均有明显的改善（P〈0．01）,甚至接近或高于正常水平。结论：海参精囊提取物对环磷酰胺导致的生殖系统受损小鼠的生精功能具有一定的保护作用。     

镉对小鼠精子和生精细胞超微结构及生精细胞bcl-2、bax基因表达的影响

研究镉暴露对小鼠附睾精子和睾丸生精细胞超微结构的变化以及镉对生精细胞凋亡相关基因bcl-2、bax表达水平的影响。采用24只雄性ICR小鼠随机分为4组,每组6只,分别以0.183、0.915、1.83mg/kg氯化镉腹腔注射,每天1次,连续5次,设阴性对照生理盐水组。于第6天透射电镜观察附睾精子超微结构、睾丸生精细胞核和线粒体超微结构的变化,免疫组化方法检测生精细胞Bcl-2、Bax表达水平。透射电镜观察显示,0.183mg/kg组精子超微结构无显著性变化,0.915mg/kg组精子头部两侧膜与头部胞质间隙轻微扩大,线粒体嵴间腔扩大且轻度空泡化,但与对照组相比无统计学意义(P>0.05)。1.83mg/kg组头部两侧膜与胞质间隙扩大,与对照组相比有显著性差异(P<0.05),尾部线粒体嵴间腔扩大且轻度空泡化,与对照组相比有显著性差异(P<0.05)。3种剂量处理组睾丸生精细胞核超微结构异常发生率显著高于对照组(P<0.05),且随着处理浓度的升高异常发生率升高;1.83mg/kg组线粒体肿胀空泡化发生率显著高于对照组(P<0.05)。3种剂量实验组生精细胞Bcl-2表达水平(吸光度)显著低于对照组(P<0.01),0.915mg/kg组Bax表达水平显著高于对照组和0.183、1.83mg/kg组(P<0.01)。3种剂量实验组Bcl-2/Bax吸光度比值显著低于对照组(P<0.01);0.915mg/kg组Bcl-2/Bax比值显著低于1.83mg/kg组(P<0.01)。上述结果提示:高浓度镉诱导附睾精子超微结构改变,高中低浓度镉致睾丸生精细胞超微结构的改变,生精细胞超微结构发生凋亡现象。镉对Bcl-2、Bax表达水平的改变可能是生精细胞凋亡的分子机制之一。     

砷对大鼠生精细胞凋亡的影响

砷是已肯定的生殖毒物之一,但关于砷对雄（男）性生殖系统的毒性作用的分子机制尚不清楚。本实验通过检测慢性砷中毒大鼠睾丸脏器系数、精子头数、每日精子生成量（DSP）及生精细胞凋亡情况,探讨砷对精子发生的影响,为进一步探讨砷致雄（男）性生殖毒性机制提供基础资料。结果显示,随染砷剂量的增加,大鼠出现睾丸生精上皮结构变疏松,生精上皮细胞层次紊乱,甚至部分生精小管基膜溶解、管腔中成熟精子减少、小管间隙增宽、细胞体积缩小、间质出现水肿、渗出等病理改变;睾丸精子头计数及DSP逐渐减少,中、高剂量组变化尤其明显。     

肾虚育精方对肾精亏虚小鼠模型生殖激素及氧化应激水平的影响

目的:研究肾虚育精方对肾精亏虚小鼠模型生殖激素及氧化应激水平的影响。方法:选择6周龄雄性健康级SD小鼠60只纳入本次研究。根据随机数字法将小鼠分成3组,分别为观察组、模型组及对照组,每组各20只。观察组及模型组的小鼠通过"房劳和惊恐复合伤肾法"建立肾精亏虚模型,对照组小鼠不建模。建模完成后观察组小鼠每日给予肾虚育精方的浓缩液干预,模型组及对照组则予以等量的生理盐水灌胃。干预21d后对比各组小鼠睾丸组织有关指标,包括Johnsen 10级积分、生精小管的直径及生精上皮厚度,小鼠生殖激素水平,包括血清卵泡刺激素(FSH)及睾酮(TEST),氧化应激指标水平,包括丙二醛(MDA)、过氧化物歧化酶(SOD)及总抗氧化能力(T-AOC)。结果:对照组与观察组的Johnsen 10级积分高于模型组,生精小管的直径及生精上皮厚度大于模型组,差异均有统计学意义(P0.05);观察组的生精上皮厚度明显大于对照组,差异有统计学意义(P0.05)。对照组与观察组小鼠的FSH及TEST水平均明显高于模型组,差异均有统计学意义(均P0.05)。对照组与观察组的MDA和SOD水平明显低于模型组,T-AOC水平明显高于模型组,差异均有统计学意义(P0.05)。结论:肾虚育精方能够提升肾精亏虚小鼠模型的生殖激素水平,并降低氧化应激水平,可将肾虚育精方应用于临床治疗。     

细胞松弛素E对大鼠生精细胞发育的影响

本文采用微丝抑制剂——细胞松弛素E对大鼠生精细胞发育的影响作了形态学观察,特别对支持细胞骨架复合体的作用进行了较为详细的研究。结果表明睾丸内注射0.1ml,1000μmol/L～2000μmol/L,细胞松弛素E,6-14小时后,光镜下可见曲细精管上皮排列疏松,组合紊乱,有的生精上皮基底部出现双核和三核的圆形细胞和多核巨精子细胞,管腔内出现未成熟的精子;在第ⅤⅢ～Ⅸ期曲细精管上皮中,有许多第8、第9期的精子细胞顶体不指向基底方向,属定向不正的精子。电镜下,实验组动物可见一些面向第8-18期精子细胞顶体的支持细胞骨架复合体出现不同程度的缺如,有的断裂成小段;有的破坏仅发生在顶体上方;有的几乎全部丢失,并有类管球复合体的形成。另外,在高渗液处理下,可见精子细胞顶体和支持细胞间的间隙扩大。最后对微丝在精子发育中的作用进行了讨论。     

乙烯利对青春期大鼠睾丸组织病理及生精细胞凋亡的影响

目的:探讨乙烯利对青春期大鼠睾丸组织病理及生精细胞凋亡的影响。方法:青春期雄性25日龄SD大鼠,分别以乙烯利浓度为2000 mg/kg、1000 mg/kg、500 mg/kg和生理盐水连续灌胃14和21天,分别取睾丸固定、包埋,以HE染色、末端转移酶标记技术(TUNE法)光镜观察睾丸的组织形态学变化、检测生精细胞凋亡情况。结果:低剂量组较对照组相比生精小管萎缩,生精细胞排列紊乱;中剂量和高剂量组较低剂量组相比,生精小管更加萎缩,生精细胞排列明显紊乱;接触乙烯利14天后高剂量组生精细胞凋亡指数与低剂量、对照组相比具有显著统计学差异(P0.01);高剂量与中剂量组相比无统计学差异(P0.05);中剂量和低剂量与对照组相比有显著统计学差异(P0.01);接触乙烯利21天后各组间比较均具有显著性差异(P0.01)。结论:乙烯利可导致大鼠生精细胞凋亡增加,生精能力下降,这可能是导致青年不育的原因之一。     

双酚A对中国林蛙生精细胞凋亡和Bax、Bcl-2表达的影响

为探讨双酚A(BPA)对两栖动物生精细胞凋亡及相关蛋白Bax和Bcl-2表达的影响.将雄性中国林蛙(Rana chensinensis)分别暴露于10-7、10-6、10-5 mol/L BPA水体中持续3 d、5 d、7 d,取其精巢组织.用原位末端转移酶法(TUNEL)和甲基绿-派诺宁法(Methyl Green-Pyronine)检测生精细胞凋亡,用免疫组织化学方法检测生精细胞的Bax和Bcl-2表达.结果显示,各BPA处理组中国林蛙生精细胞凋亡指数(Apoptotic index,AI)均显著高于对照组,10-6 mol/L与10-7 mol/L BPA处理组生精细胞的AI差异不显著,10-5 mol/L BPA处理组生精细胞的AI与前两组相比显著增高;在同一BPA浓度处理组,生精细胞AI随处理时间的延长而增高.与对照组相比,各BPA处理组Bax表达上调,Bcl-2表达下调,差异均显著;生精细胞AI与Bax/Bcl-2表达呈正相关.这些结果提示,BPA可导致中国林蛙的生精细胞凋亡,而生精细胞凋亡的发生与Bax/Bcl-2表达比值的变化密切相关.     

精子特异性钙通道CatSper1 对精子线粒体呼吸与能量代谢的影响

目的:应用Cat Sper1单克隆抗体抑制Cat Sper1的功能,检测精子线粒体呼吸功能及能量合成能力,观察Cat Sper1对精子线粒体呼吸与能量代谢的影响。方法:健康志愿者20例,检测精液均符合WHO健康标准。手淫法获取精液,经过上游法处理后每份精液分为A、B两组,分别与Earles液以及50μg/m L抗Cat Sper1多克隆抗体共孵育。在1 h,2 h,4 h后分别检测两组精子精液参数、细胞线粒体呼吸控制率RCR及精子细胞ATP含量。结果:与A组比较,B组精子各时间点a+b(%)尤其是a(%)均明显下降,差异具有统计学意义(P0.01);1 h后B组精子a(%)即明显下降,2 h,4 h后精子下降缓慢,与1 h相比无明显差异,无统计学意义(P0.05)。与A组比较,B组精子各时间点态3值、呼吸控制率RCR以及精子细胞ATP含量均明显下降,差异具有统计学意义(P0.01);B组精子中,2 h、4 h节点精子态3值、呼吸控制率RCR以及精子细胞ATP含量与1 h无明显差异,无统计学意义(P0.05)。结论:阻断精子特异性钙通道Cat Sper1,可降低精子细胞线粒体呼吸功能,减少精子生成ATP的能力,从而使精子活力降低。为精索静脉曲张引起精子Cat Sper1表达下降,从而导致不育的机制寻找可能的理论依据。     

环磷酰胺诱导小鼠血小板减少症模型的建立(英文）

比较由环磷酰胺两种不同给药方式诱导小鼠血小板减少症模型的效果,并对效果较稳定的一种给药方式进行最佳造模剂量摸索,以期确定一个造模效果较好,毒副作用较低,利于观察治疗药物疗效的血小板减少症模型。模型A组,第1天尾静脉注射环磷酰胺200 mg/kg,然后连续6 d,每天1次以维持剂量30 mg/kg腹腔注射环磷酰胺。模型B组,按150 mg/kg皮下注射环磷酰胺,每天1次,连续3 d。结果显示模型B组造模效果较好,故以模型B组给药方法进行剂量摸索实验。由第7天的血小板计数可知环磷酰胺低（100 mg/kg）、中（120 mg/kg）、高（140 mg/kg）剂量均可引起血小板减少症,而低剂量组与其他组比较有高效低毒的特点,更有利于观察治疗药物的作用,可用于具有升血小板作用药物的药效学研究     

环磷酰胺诱导小鼠血小板减少症模型的建立(英文)

比较由环磷酰胺两种不同给药方式诱导小鼠血小板减少症模型的效果,并对效果较稳定的一种给药方式进行最佳造模剂量摸索,以期确定一个造模效果较好,毒副作用较低,利于观察治疗药物疗效的血小板减少症模型.模型A组,第1天尾静脉注射环磷酰胺200 mg/kg,然后连续6 d,每天1次以维持剂量30 mg/kg腹腔注射环磷酰胺.模型B组,按150 mg/kg皮下注射环磷酰胺,每天1次,连续3 d.结果显示模型B组造模效果较好,故以模型B组给药方法进行剂量摸索实验.由第7天的血小板计数可知环磷酰胺低(100 mg/kg)、中(120mg/kg)、高(140 mg/kg)剂量均可引起血小板减少症,而低剂量组与其他组比较有高效低毒的特点,更有利于观察治疗药物的作用,可用于具有升血小板作用药物的药效学研究.     

Expression Profiling and Identification of Novel SNPs in CatSper2 Gene and Their Influence on Sperm Motility Parameters in Bovines

122 randomly selected Vrindavani cattle were studied to detect polymorphism in four fragments of the CatSper2 gene that were comprised of exon 2, 4, 5, and 6 with flanking regions. Using PCR-SSCP and sequencing analysis, three SNPs (T157C, C273A, and A274C) in the first fragment, one SNP (C30G) in the second fragment, and two SNPs (T86G and T292C) in the fourth fragment were identified. The third fragment did not reveal any polymorphism. The SNPs were used for construction of haplotypes and three haplotypes were found. The least square analysis of variance revealed a significant (P?G or C>T SNPs may not play a role in sperm motility. However, when the comparison was made between haplotype I and II, it can be inferred that C>T SNP may have a role in sperm motility, as haplotype II has better motility parameters. Expression profiling of Catper2 gene revealed nonsignificant down regulation of CatSper2 gene in poor motility sperm compared to good motility sperm.     

少弱精子症患者精子候选差异蛋白Trx 2、TrxR 1的验证及在少精、弱精子症中的表达研究

目的:根据TMT技术筛选少弱精子症患者精子差异蛋白的结果,选取硫氧还蛋白2(thioredoxin 2,Trx 2)、硫氧还蛋白还原酶1(thioredoxin reductase 1,TrxR 1)进行验证,探讨二者在少精、弱精和少弱精子症中的表达变化及其意义。方法:收集105例少精子症组(O组)、150例弱精子症组(A组)、50例少弱精子症组(OA组)和106例正常精液男性(N组)精液,分离出精子,对少弱精子症进行串联质谱标签(Tandem Mass Tag,TMT)技术蛋白质组学分析,根据少弱精子症组的精子差异蛋白结果选取Trx 2、TrxR 1,通过免疫荧光和免疫印迹方法检测其在O组、A组、OA组的表达情况。结果:TMT技术蛋白质组学结果显示Trx 2为上调差异蛋白(为N组的1.31倍),TrxR 1为下调差异蛋白(为N组的0.82倍)。免疫荧光和免疫印迹结果显示O组、A组、OA组Trx 2表达显著高于N组(P0.05),O组、OA组TrxR 1的表达显著低于N组(P0.05)。二者在OA组的结果与蛋白质组学结果一致。结论:Trx 2、TrxR 1可能在少精、弱精及少弱精子症的发生中起着重要的作用,并有望成为少弱精子症患者精子的候选标志物及治疗靶点。     

Contributions of extracellular and intracellular Ca2+ to regulation of sperm motility: Release of intracellular stores can hyperactivate CatSper1 and CatSper2 null sperm

In order to fertilize, mammalian sperm must hyperactivate. Hyperactivation is triggered by increased flagellar Ca(2+), which switches flagellar beating from a symmetrical to an asymmetrical pattern by increasing bending to one side. Thimerosal, which releases Ca(2+) from internal stores, induced hyperactivation in mouse sperm within seconds, even when extracellular Ca(2+) was buffered with BAPTA to approximately 30 nM. In sperm from CatSper1 or CatSper2 null mice, which lack functional flagellar alkaline-activated calcium currents, 50 microM thimerosal raised the flagellar bend amplitudes from abnormally low levels to normal pre-hyperactivated levels and, in 20-40% of sperm, induced hyperactivation. Addition of 1 mM Ni(2+) diminished the response. This suggests that intracellular Ca(2+) is abnormally low in the null sperm flagella. When intracellular Ca(2+) was reduced by BAPTA-AM in wild-type sperm, they exhibited flagellar beat patterns more closely resembling those of null sperm. Altogether, these results indicate that extracellular Ca(2+) is required to supplement store-released Ca(2+) to produce maximal and sustained hyperactivation and that CatSper1 and CatSper2 are key elements of the major Ca(2+) entry pathways that support not only hyperactivated motility but possibly also normal pre-hyperactivated motility.     

Ca2+ Signals Generated by CatSper and Ca2+ Stores Regulate Different Behaviors in Human Sperm

[Ca²⁺]_i signaling regulates sperm motility, enabling switching between functionally different behaviors that the sperm must employ as it ascends the female tract and fertilizes the oocyte. We report that different behaviors in human sperm are recruited according to the Ca²⁺ signaling pathway used. Activation of CatSper (by raising pH_i or stimulating with progesterone) caused sustained [Ca²⁺]_i elevation but did not induce hyperactivation, the whiplash-like behavior required for progression along the oviduct and penetration of the zona pellucida. In contrast, penetration into methylcellulose (mimicking penetration into cervical mucus or cumulus matrix) was enhanced by activation of CatSper. NNC55-0396, which abolishes CatSper currents in human sperm, inhibited this effect. Treatment with 5 μm thimerosal to mobilize stored Ca²⁺ caused sustained [Ca²⁺]_i elevation and induced strong, sustained hyperactivation that was completely insensitive to NNC55-0396. Thimerosal had no effect on penetration into methylcellulose. 4-Aminopyridine, a powerful modulator of sperm motility, both raised pH_i and mobilized Ca²⁺ stored in sperm (and from microsomal membrane preparations). 4-Aminopyridine-induced hyperactivation even in cells suspended in Ca²⁺-depleted medium and also potentiated penetration into methylcellulose. The latter effect was sensitive to NNC55-039, but induction of hyperactivation was not. We conclude that these two components of the [Ca²⁺]_i signaling apparatus have strikingly different effects on sperm motility. Furthermore, since stored Ca²⁺ at the sperm neck can be mobilized by Ca²⁺-induced Ca²⁺ release, we propose that CatSper activation can elicit functionally different behaviors according to the sensitivity of the Ca²⁺ store, which may be regulated by capacitation and NO from the cumulus.     

环磷酰胺对雄性大鼠生殖免疫功能的影响

目的观察环磷酰胺对大鼠睾丸及其细胞免疫的影响,探讨抗肿瘤药物在生殖免疫功能中的机制。方法选用16只15周龄SD大鼠,随机分为对照组和实验组,每组8只;实验组腹腔注射环磷酰胺20mg/kg/d,连续5天,用药两个月后,应用HE染色法研究大鼠睾丸远期组织学变化,用原位缺口末端标记法（TUNEL方法）检测生精小管中生殖细胞凋亡,放射免疫法检测血清睾酮（T）、卵泡刺激素（FSH）、黄体生成素（LH）,流式细胞术进行血液T淋巴细胞亚群分析。结果实验组睾丸生精小管直径缩小、间距增宽、生精上皮变薄、生殖细胞层次和数量减少、生精小管腔多未见精子形成,实验组睾丸生精小管直径、面积、生殖细胞数均显著低于对照组（P〈0.01）;实验组与对照组比较生殖细胞凋亡增多,差异显著（P〈0.01）;实验组与对照组比较血清T明显降低,差异显著（P〈0.01）,血清FSH、LH水平两组间差异无显著性;血液T淋巴细胞亚群分析,实验组与对照组比较CD3＋CD4＋、CD4＋/CD8＋明显降低（P〈0.01）,CD3＋CD8＋明显升高（P〈0.01）。结论环磷酰胺对大鼠睾丸远期损害明显,促进生殖细胞凋亡,降低睾酮的分泌,并抑制T淋巴细胞的免疫功能。     

Protective Effects of Caffeic Acid Phenethyl Ester on Cyclophosphamide‐Induced Hemorrhagic Cystitis in Rats

We investigated the protective effect of caffeic acid phenethyl ester (CAPE) on cyclophosphamide‐induced hemorrhagic cystitis in rats in comparison with 2‐mercaptoethane sulfonate (MESNA). Forty male rats were randomized into four groups: group 1 (control), group 2 (cyclophosphamide), group 3 (cyclophosphamide + MESNA), group 4 (cyclophosphamide + CAPE). Cyclophosphamide injection increased malondialdehyde levels indicating oxidative stress, whereas CAPE and MESNA ameliorated malondialdehyde levels in the bladder (p < 0.05). Only catalase activities were decreased significantly in both groups (cyclophosphamide + MESNA and cyclophosphamide + CAPE, p < 0.05). Pretreatment with CAPE (p < 0.01) resulted in a significant decrease in nitric oxide levels when compared with the cyclophosphamide group. When we consider the studies that show the critical importance of increased nitric oxide levels in pathogenesis of cyclophosphamide‐induced hemorrhagic cystitis, we suggest that it would be more beneficial to use MESNA with CAPE to prevent histological damage.     

一种环境激素联合冷应激大鼠模型阴茎组织中 Sprouty 2、ERK1/2表达的研究

目的:研究Sprouty 2(Spry 2)和细胞外调节蛋白激酶(ERK1/2)在环境激素联合冷应激大鼠模型阴茎组织中的表达,并观察伊木萨克片对二者表达的影响。方法:选用30只正常的雄性SD大鼠,其中10只为正常对照组(N组),余20只为造模组,采用富含环境雌激素饲料+寒冷环境的干预条件建立复合性应激大鼠模型(20 w),其中10只大鼠采用伊木萨克片干预2 w(Y组),剩余10只为模型组(M组)。采用免疫组化方法检测各组大鼠阴茎组织中Spry 2、ERK1/2的表达。结果:M组大鼠阴茎组织中Spry2表达低于N组(P0.05),Y组大鼠阴茎组织中Spry 2表达明显高于M组(P0.05)。三组大鼠阴茎组织中总ERK1/2(t-ERK1/2)的表达比较差异均无统计学意义(P0.05)。M组大鼠阴茎组织中磷酸化ERK1/2(p-ERK1/2)表达高于N组(P0.05),Y组大鼠阴茎组织中p-ERK1/2表达明显低于M组(P0.05)。结论:Spry 2表达下调和ERK1/2活化可能促进应激反应的发生发展,伊木萨克片可能通过上调Spry 2的表达和减少ERK1/2的活化发挥抗应激作用。