薄荷油对雄性小鼠的抗生育作用研究

目的探讨薄荷油对雄性小鼠的抗生育作用。方法将60只健康的雄性性成熟昆明小鼠随机分成3个试验组和1个对照组,各试验组小鼠灌胃0.135 g/(kg·d),0.27 g/(kg·d)和0.54 g/(kg·d)的薄荷油0.5%羧甲基纤维素钠(sodium carboxymethylcellulose,CMC)混悬液,对照组灌胃0.5%羧甲基纤维素钠溶液,灌胃1周后按雌雄比2∶1合笼,继续对雄鼠灌胃至19 d,采集雄性小鼠的血液并测定血液生化指标,剖检灌胃雌雄小鼠,统计雌性小鼠的怀孕率,测定雄性小鼠睾丸与附睾的脏器系数及附睾精子活力,并固定睾丸和附睾,研究其组织学变化。结果与对照组相比较,雄性小鼠灌胃薄荷油后,导致雌性小鼠的怀孕率降低,睾丸脏器系数和附睾精子活率极显著降低(P<0.01),精子畸形率极显著升高(P<0.01)。光学显微镜下,试验组小鼠睾丸和附睾均有一定程度的损伤,睾丸间质减少,睾丸各级生精细胞排列疏松,曲细精管内有多核巨噬细胞浸润。附睾具正常的管腔结构,但能明显观察到管腔内精子减少。结论薄荷油对雄性小鼠具有抗生育作用,且主要通过影响精子的生成及破坏生精组织而达到,具有实际应用价值,可进一步开发成环境友好型鼠类抗生育药剂。     

合欢皮总皂苷对雄性小鼠的抗生育作用研究

目的探讨合欢皮总皂苷对雄性小鼠的抗生育作用。方法将60只健康的雄性性成熟昆明小鼠随机分成3个试验组和1个对照组,各试验组小鼠灌胃540 mg·(kg·d)-1,270 mg·(kg·d)-1和135 mg·(kg·d)-1的合欢皮总皂苷水溶液,对照组自由饮水,灌胃1周后按雌雄比2∶1合笼,继续对雄鼠灌胃至19 d,采集雄性小鼠的血液并测定血液生化指标,剖检灌胃雌性小鼠,统计雌性小鼠的怀孕率,测定雄性小鼠睾丸与附睾的脏器系数及附睾精子活力,并固定睾丸和附睾,研究其组织学变化。结果与对照组相比较,雄性小鼠灌胃合欢皮总皂苷后,导致雌性小鼠的怀孕率降低,睾丸脏器系数和附睾精子活率极显著降低(P<0.01),精子畸形率极显著升高(P<0.01)。光学显微镜下,试验组小鼠睾丸和附睾均有一定程度的损失,睾丸生精细胞排列疏松,间质减少,可见曲细精管内有多核巨噬细胞浸润,各级生精细胞脱落。附睾具正常的管腔结构,但能明显观察到管腔内精子几乎消失。结论合欢皮总皂苷对雄性小鼠具有抗生育作用,主要通过影响精子的生成及破坏生精组织而达到。     

雄性裸鼹鼠可育个体与不可育个体生殖系统结构与功能差异初探

目的观察和分析雄性裸鼹鼠中可育个体和不可育个体生殖系统结构和功能的差异,初步探索雄性不可育个体不能繁育后代的原因。方法雄性裸鼹鼠可育个体和不可育个体各5只,先采集一侧睾丸和附睾组织,称重后换算脏器系数;再采集另一侧睾丸组织,用中性甲醛溶液进行固定后制备组织切片;取另一侧附睾用作精子计数、精子活动度的测定;采集血清测定血清中黄体生成素(LH)和睾酮(T)浓度。结果与可育个体组相比较,不可育个体组的睾丸重量下降(P0.05),附睾重量显著下降(P0.01),且睾丸系数和附睾系数均显著下降(P0.01);精子数量显著减少(P0.01),精子活动度也显著减弱(P0.01);血清黄体生成素和睾酮水平均显著降低(P0.01);睾丸组织切片观察显示,不可育个体各级生精细胞严重脱落,排列混乱无序,支持细胞和间质细胞均有减少。结论雄性裸鼹鼠不可育个体生殖系统存在睾丸和附睾萎缩、生精功能下降和性激素分泌减少等现象。     

雷公藤制剂对雄性长爪沙鼠繁殖功能的影响

为了检测雷公藤制剂对长爪沙鼠繁殖功能的影响,根据预实验结果,将40只雄性长爪沙鼠分为40 mg/kg连续用药4周组(n=16)、100 mg/kg一次给药组(n=10)和1%CMC灌胃对照组(n=14)处理,6周后剖检,比较睾丸、附睾的脏器系数、精子密度、精子活力、精子形态和繁殖率等指标.结果表明40 mg/kg连续用药组鼠的睾丸、附睾脏器系数与对照组比较差异显著;精子密度、精子活力和活精子百分率显著下降;精子畸形率显著上升;繁殖率显著下降(df=1,P<0.05).100 mg/kg一次给药组除附睾脏器系数显著下降、精子畸形率显著上升外,其它指标与对照组无明显差异.该药对长爪沙鼠连续作用4周后不育效果明显,并且具有致畸性,在药物有效范围内,高浓度一次性给药方式不如较低浓度连续多次给药效果显著.     

恒定磁场对小鼠精子毒性作用的实验研究

观察不同强度恒定磁场对雄鼠睾丸、附睾重量、精子数量、精子活动度及精子形态的影响. 结果显示睾丸与附睾重量各组无显著差异, 精子数量在实验组与对照组中亦无明显改变. 在 0.12T磁场环境暴露下, 雄鼠精子畸形率增加及活动率下降, 与对照组相比有显著差异. (P< 0.01), 提示磁场对小鼠精子有一定毒性, 并且毒性与其强度有关.     

炔雌醚对雄性长爪沙鼠不育效果及其可逆性

为探讨炔雌醚对雄性长爪沙鼠生殖器官及繁殖的影响,将试鼠随机分为多剂量组、单剂量组和对照组.多剂量组以每次3.5 m/kg·BW(5次/周,2周)、单剂量组以35 mg/kg·BW炔雌醚灌胃.处理后15 d、30 d、60d、90d剖检,观察性腺系数、精子质量和繁殖率等指标,H·E染色观察附睾组织病理学变化.结果表明:与对照相比,炔雌醚处理后15 d、30 d给药组试鼠睾丸、附睾及精囊腺极度萎缩(P＜0.01),精子密度、精子活力和活精子百分率明显下降(P＜0.01),精子畸形率显著上升(P＜0.01),附睾管腔内充满大量发育异常的精子细胞,繁殖率显著下降;与单次给药相比,多次连续给药对试鼠生殖器官影响更严重.处理后60d,除多剂量组附睾外,各组性腺基本恢复至对照水平,单剂量组、多剂量组精子质量及繁殖率与对照仍有极显著差异(P＜0.01).90d后试鼠各项指标及繁殖率均恢复正常,表现为可逆性.结果表明:该药对长爪沙鼠不育效果明显;多次低剂量给药较单次高剂量给药不育效果更好;90d后,炔雌醚对生殖器官和繁殖的影响能够恢复正常.     

EP-1对雄性中华姬鼠和黑线姬鼠繁殖力的影响

为了检测左炔诺孕酮-炔雌醚（EP-1）对雄性中华姬鼠和黑线姬鼠的不育效果, 将32只雄性中华姬鼠和30只雄性黑线姬鼠分为 30mg/kg 单剂量组、30mg/kg多剂量组和对照组, 15d 和 45d 后剖检, 比较睾丸、附睾、储精囊、精子密度、睾酮含量及睾丸组织形态的变化。结果发现：给药后第 15 天,两种试鼠的睾丸、附睾、储精囊的重量较对照组明显降低; 精子密度、睾酮含量显著下降; 曲细精管结构破坏明显。给药后第45天,处理组各生理指标继续下降,但与第15天相比差别不显著;单剂量组和多剂量组在两个时间点的差别并不显著。结果表明,EP-1对雄性中华姬鼠和黑线姬鼠的繁殖器官有显著抑制效果,单次给药与多次给药的不育效果差别不大。     

关养密度和成年雄鼠填充物的气味对黄毛鼠(Rattus rattoides)的发育和性成熟的影响(英文)

黄毛鼠（Ｒａｔｔｕｓ ｒａｔｔｉｄｅｓ）在群居（４只／笼）时体重及性器官,如睾丸和附睾的增长都受到了极大的抑制;血清中睾酮含量的迅速上升以及成熟精子在附睾的曲细精管中出现的时间也比单独关养的晚。成年雄鼠的笼填充物的气味能够诱导幼年雄鼠体重,睾丸的总量和长度以及血清中睾酮的含量的增加。     

前列腺素与雄性生殖生理

小剂量前列腺素(PGs)作用于下丘脑,增加LHRH释放,后者促使垂体分泌LH、FSH,从而刺激睾酮分泌。睾丸间质细胞的功能还直接受PGs的调节,睾酮也显著影响雄性生殖道中PGs水平。PGs可增加大鼠睾丸重量,刺激生精过程,增加精子细胞数目,提高精子活力,维持生殖道中平滑肌的收缩,参与射精过程,促进精子在雌体生殖道内的运行,故利于受精。大剂量PGs抑制雄性生殖,使血中LH、FSH、睾酮水平下降,使睾丸动脉收缩,导致睾丸萎缩,减少睾丸及副性腺的重量,抑制生精作用,降低附睾精子活力,增加畸精率。     

免不1号和2号治疗免疫性不育雄鼠的组织学和免疫组织化学研究

用中药复方免不1号,免不2号治疗免疫性不育雄鼠,观察睾丸,附睾组织学和免疫组化的变化。用精子抗原免疫昆明种雄性小白鼠,建立免疫性不育动物模型。同时分别饲喂中药复方免不1号,免不2号,醋酸强的松,生理盐水;从组织学和免疫组化等方面观察免疫性不育症的变化。结果显示免疫性不育雄鼠血清,精囊液抗精子抗体高,睾丸间质,睾丸曲细精管界膜,精原细胞,附睾管上皮细胞免疫复合物沉积多,睾丸每曲细精管精子和晚期精子细胞减少,中药免不1号和2号能降低抗精子抗体,清除免疫复合物的沉积,恢复曲细精管精子和晚期精子细胞数。结果表明：免不1号和2号通过调节全身免疫系统,清除循环和局部的抗精子抗体,免疫复合物,提高精子和精子细胞数,从而提高小鼠的受孕率。     

Effects of PNU157706, a dual 5alpha-reductase inhibitor, on rat epididymal sperm maturation and fertility

Sperm entering the epididymis gain progressive motility and fertilizing ability in a process termed maturation. The functional dependence of the epididymis on dihydrotestosterone (DHT) is well established, yet few studies have examined the consequences on the epididymis of inhibiting DHT formation. We have shown that inhibition of both isoforms of 5alpha-reductase (types 1 and 2), the enzyme that converts testosterone to DHT, has pronounced effects on epididymal gene expression. In the present study, we investigate whether inhibiting 5alpha-reductase has consequences on epididymal sperm maturation. Rats were treated with vehicle or 10 mg/kg/day PNU157706, a dual-type inhibitor, for 28 days. Fertility and several key facets of sperm maturation were analyzed. Changes in sperm motility were assessed by computer-assisted sperm analysis (CASA). Changes in sperm morphology were assessed by CASA and electron microscopy. The motility of spermatozoa from the cauda epididymidis of treated animals showed a significant decrease in both the percentage of motile and progressively motile sperm as well as altered motion parameters. The morphology of cauda epididymal spermatozoa was also adversely affected by the treatment; the most prominent effect was a markedly elevated proportion of sperm that retained their cytoplasmic droplet. Matings with treated males resulted in fewer successful pregnancies and a higher rate of preimplantation loss. Progeny outcome was unaffected. The compromised sperm motility and morphology likely contribute to the subfertility of inhibitor-treated rats. Our results indicate a role for dual 5alpha-reductase inhibitors in further studies of epididymal physiology and as a potential component of a male contraceptive.     

The effects of long-term administration of either a crude inhibin preparation or an antiserum to FSH on serum hormone levels, testicular function and fertility of adult male rats.

Adult male rats were given either daily injections of ram rete testis fluid for periods of up to 70 days or injections of an antiserum against FSH every 3 days for 90 days. Compared with the control groups, the rats injected with ram rete testis fluid had lowered serum FSH levels, but only at treatment periods of 30 days and less. The levels of LH and testosterone in serum, testicular fluid secretion, sperm counts, testis weights and fertility were not affected by rete testis fluid treatment. The rats injected with anti-FSH serum exhibited an impairment of fertility which was never complete and evident only after 49 days of treatment. After 90 days of anti-FSH treatment, testis weight and free serum FSH were reduced, but sperm counts, testicular fluid secretion and serum levels of LH and testosterone were not affected.     

Sterility due to inhibition of sperm motility by oral administration of benzene chromatographic fraction of the chloroform extract of the seeds of Carica papaya in rats.

The contraceptive effects of benzene chromatographic fraction of the chloroform extract of the seeds of Carica papaya have been reported in male albino rats at the dose regimens 5 and 10 mg/animal/day; oral for 150 days. The body weight, weight of testis, epididymis, seminal vesicle and ventral prostate remained unaltered during the entire course of the investigation. Total suppression of cauda epididymal sperm motility coincided with a decrease in sperm count, viability and an increase in per cent abnormal spermatozoa during 60-150 days observation period. Minor changes in the germ cell proliferations in the testis and vacuolization and pyknotic nuclei in the few epithelial cells of the cauda epididymis were observed. Histology and biochemical composition of testis and accessory sex organs, haematology and serum clinical biochemistry and serum testosterone levels remained unchanged throughout the course of the investigation. Test for estrogenicity indicated mild estrogenicity. Monthly fertility test showed negative fertility. All the altered parameters returned to normal level following 60 days withdrawal of the treatment. The results suggest that the benzene chromatographic fraction of the chloroform extract of the seeds of Carica papaya exerts antifertility effects in rats without adverse toxicity and that the effects may be directly rendered on the spermatozoa.     

Diethylstilbestrol-treated adult rats with altered epididymal sperm numbers and sperm motility parameters, but without alterations in sperm production and sperm morphology

In this study, we characterized estrogenic effects of diethylstilbestrol (DES) on reproductive parameters in male rats to identify a minimal dose level that alters epididymal and sperm functions but has little or no effect on sperm production and/or spermatogenesis. Adult rats (five animals/group) received s.c. injections of 0.2 ml of corn oil containing DES at a rate of 1.0 mg, 200 microg, 40 microg, 8 microg, 1.6 microg, or 320 ng x rat(-1) x day(-1) for 12 days. The control group received corn oil only. DES effects were similar in the 8-microg group and higher dose groups and included significant (P < or = 0.05) reductions in 1) absolute and relative weights of the head and body of the epididymis (EP), tail of the EP, and seminal vesicle, 2) numbers of sperm in both regions of the EP, and 3) motility characteristics in sperm collected from the tail of the EP. Conversely, no significant changes were observed in relative testis weight, daily sperm production, spermatogenesis, seminiferous epithelial height in stage VII, and sperm morphology. All of the above parameters in the 1.6-microg group (except seminal vesicle weight) and 320-ng group were comparable to those of controls. Plasma testosterone (T) level was reduced to an almost undetectable level in the > or = 8-microg groups and to a very low level in the 1.6-microg group (0.35 vs. 2.36 ng/ml in controls or 320-ng group), but LH level was unaltered. In a parallel fertility study, males received DES at a rate of 40, 8, or 1.6 microg x rat(-1) x day(-1) for 12 days prior to and 12 days during cohabitation (1:1) with untreated females. Of the 15 females cohabited with treated males (5 females/dose), none in the 40-microg and 8-microg groups and 1 in the 1.6-microg group formed a copulatory plug and delivered 8 pups, in contrast to 5/5 copulatory plugs and 13-15 pups/litter in the controls. DES at a rate of 8 microg x rat(-1) x day(-1) for 12 days reduced EP weights, sperm numbers in the EP, and sperm motility patterns but caused minimal to no alterations in daily sperm production, spermatogenesis, or sperm morphology. Factors other than T, or in addition to lower T, may be responsible for DES-induced reproductive disorders (despite lower T, sperm contents and sperm motility patterns in the EP were normal in the 1.6-microg group). Deficits in EP sperm functions and/or sexual behavior (as evident from absence of copulatory plugs) probably accounted for reduced fertility in treated males.     

Calsperin is a testis-specific chaperone required for sperm fertility

Calnexin (CANX) and calreticulin (CALR) are homologous lectin chaperones located in the endoplasmic reticulum and cooperate to mediate nascent glycoprotein folding. In the testis, calmegin (CLGN) and calsperin (CALR3) are expressed as germ cell-specific counterparts of CANX and CALR, respectively. Here, we show that Calr3(-/-) males produced apparently normal sperm but were infertile because of defective sperm migration from the uterus into the oviduct and defective binding to the zona pellucida. Whereas CLGN was required for ADAM1A/ADAM2 dimerization and subsequent maturation of ADAM3, a sperm membrane protein required for fertilization, we show that CALR3 is a lectin-deficient chaperone directly required for ADAM3 maturation. Our results establish the client specificity of CALR3 and demonstrate that the germ cell-specific CALR-like endoplasmic reticulum chaperones have contrasting functions in the development of male fertility. The identification and understanding of the maturation mechanisms of key sperm proteins will pave the way toward novel approaches for both contraception and treatment of unexplained male infertility.     

α‐Lipoic acid inhibits testicular and epididymal oxidative damage and improves fertility efficacy in arsenic‐intoxicated rats

The present study evaluates the protective effect of α‐lipoic acid (LA) against arsenic‐induced testicular and epididymal oxidative damage in rats. Arsenic caused significant reduction in the reproductive organ weights, serum testosterone levels, testicular daily sperm count, epididymal sperm count, sperm motility, sperm viability, and sperm membrane integrity. Significant reduction in the activity levels of superoxide dismutase, catalase, and glutathione levels with a concomitant increase in the lipid peroxidation and protein carbonyl content in the testis and the cauda epididymis of arsenic‐exposed rats. Arsenic intoxication also enhanced the testicular caspase‐3 mRNA levels, disorganization of testicular and cauda epididymal architecture as well as increased arsenic content in the testis and the cauda epididymis of rats. Arsenic exposure also deteriorated fertility ability in male rats over controls. Conversely, α‐LA negated the testicular and cauda epididymal oxidative stress and restored the male reproductive health in arsenic‐exposed rats.     

Ameliorative effect of ellagic acid and Vitamin C against malathion-induced toxicity in testis of adult Wistar rats

The pesticide malathion (MT), an organophosphate, is highly neurotoxic and causes cholinergic disorders as well as cytotoxicity, genotoxicity, mutagenicity, carcinogenicity and reproductive toxicity. Our purpose was to study the effect of ellagic acid (EA) and Vitamin C on the testis against MT-induced toxicity in the rats. Thirty-six adult Wistar rats were employed, separated into six groups and were given treatment for 14 days. The toxicity of MT on the testis was evaluated using a variety of physical parameters, such as mortality rate and body weight, as well as biochemical parameters, such as total protein, total cholesterol, serum glutamic-oxaloacetic transaminase and serum glutamic-pyruvic transaminase, and haematological parameters, such as counts of red blood cells, haemoglobin (Hb) and white blood cells, as well as mean corpuscular volume, mean corpuscular Hb, and mean corpuscular Hb concentration. At the end of the experiment, rats were killed and a histological examination of the testis was performed. A sperm count technique and an analysis of sperm motility were used to determine the sperm quality. Biochemical indicators, sperm count, motility, viability and morphology were significantly decreased with MT. When compared with MT and the control group, EA and Vitamin C administration significantly increased sperm motility and count (p < 0.05). After receiving EA and Vitamin C, biochemical indicators and histological characteristics are also intensified. The results of the current investigation show that EA and Vitamin C can both reduce increased levels of biochemical markers and improve pathological alterations in the testis brought on by MT treatment.     

Maturational changes in motility, acrosomal proteolytic activity, and penetrability of the inner perivitelline layer of fowl sperm, during their passage through the male genital tract

The objective was to examine, in vitro, the motility, acrosomal proteolytic activity (APA), and penetrating ability of fowl sperm recovered from the testis and epididymis, as well as the proximal, middle, and distal vas deferens, to assess the potential fertilizing ability of sperm as a function of maturation. A motile sperm separation technique was used to estimate sperm motility with Accudenz, a gelatin slide technique was used to measure the diameter of the halo around the acrosome of individual sperm as an indication of APA, and a sperm-inner perivitelline layer (IPL) interaction assay was done to estimate the number of hole formations as an indication of sperm penetration into the IPL. Sperm in the testis exhibited the least motility, produced the smallest halos, and created the least number of holes per 0.25 mm². Motility, diameter of the halo, and number of holes increased gradually (P < 0.05) from the epididymis to the distal vas deferens and were markedly different (P < 0.05) between testicular and deferent duct sperm. Based on these in vitro experimental findings, we inferred that fowl sperm undergo a gradual process of maturational changes in motility, APA, and penetrability as a means of acquiring potential fertility during their passage throughout the male genital tract.     

Neonatal estrogen exposure of male rats alters reproductive functions at adulthood

The effects of neonatal exposure to different doses of diethylstilbestrol (DES) on the reproductive functions of male rats at adulthood were evaluated. Sprague-Dawley rats (5-8/group) received sc injections of 25 microl olive oil containing DES (Sigma Chemical Co., St. Louis, MO) at a dose of 10 microg, 1 microg, 100 ng, 10 ng, or 1 ng per rat on alternate days from Postnatal Days 2-12. Control animals received olive oil only. All animals were allowed to develop until 83-91 days of age; however, when they were 70 to 80 days old, four male rats each from the 10 microg, 1 microg, 100 ng, and control groups were cohabited with untreated 60- to 70-day-old females (1:1) for 12 days. At the end of cohabitation, both mated and unmated male rats were weighed, and blood and tissue samples were collected and processed. Results revealed that although sperm motility patterns and sperm morphology were adversely affected in the 10- microg group, other reproductive parameters, including 1). daily sperm production (DSP)/testis; 2). absolute and relative weights of the testis, epididymis, and seminal vesicle; and 3). sperm numbers in both regions of the epididymis declined significantly in a dose-dependent manner in the 10- and 1- microg groups. Conversely, in the <1- microg groups, none of these parameters (except DSP/testis and weight of the epididymis in the 100-ng group, and sperm numbers in the epididymis of the 100- and 10-ng groups) was different from controls. Generally, plasma testosterone levels decreased in the 10- and 1- microg groups, FSH level increased in the 10-microg group, and prolactin and LH levels were unaltered. In the fertility study, although each male in the 1-microg, 100-ng, and control groups produced a copulatory plug and impregnated a female, none could do so in the 10-microg group. The mean number of pups per litter was reduced to eight in the 1-microg group, in contrast to 15 each in the 100-ng and control groups. In conclusion, exposure of neonatal male rats to DES altered sperm motility patterns, sperm fertility (as evident from the reduced number of pups in the 1-microg group), and sexual behavior (as evident from the absence of copulatory plugs in the 10-microg group) and reduced weights of reproductive organs, DSP/testis, and sperm numbers in the epididymis. Whether these alterations/reductions persist in older rats (6-8 mo of age) is under investigation.     

Protective Role of Cactus Cladodes Extract on Sodium Dichromate-Induced Testicular Injury and Oxidative Stress in Rats

Cactus (Opuntia ficus-indica) is a xerophyte plant that belongs to the Cactaceae family. The present study was designed to investigate the possible protective effects of cactus cladodes extract (CCE) on sodium dichromate-induced testis damage in adult male Wistar rats. For this purpose, CCE at a dose of 100 mg/kg was orally administrated, followed by 10 mg/kg sodium dichromate (intraperitoneal injection). After 40 days of treatment, the rats were sacrificed, and the testes were excised for histological, lipid peroxidation (LPO), and antioxidant enzyme analyses. Sodium dichromate treatment significantly (P?<?0.01) decreased the body, testis, and accessory sex organ weights, sperm count and motility, and serum testosterone level. In addition, histological analysis revealed pronounced morphological alterations with tubular necrosis and reduction in the number of gametes in the lumen of the seminiferous tubules of sodium dichromate-intoxicated rats. Furthermore, exposure to sodium dichromate significantly (P?<?0.01) increased LPO level and decreased superoxide dismutase (SOD), catalase (CAT), and glutathione peroxidase (GPx) activities in testis. Interestingly, pretreatment with CCE significantly (P?<?0.01) restored the serum testosterone level, sperm count, and motility to the levels of the control group. Moreover, CCE administration was capable of reducing the elevated level of LPO and significantly (P?<?0.01) increased SOD, CAT, and GPx activities in testis. Cactus cladodes supplementation minimized oxidative damage and reversed the impairment of spermatogenesis and testosterone production induced by sodium dichromate in the rat testis.