血管内皮生长因子蛋白在大鼠睾丸和附睾的表达和定位研究

为探讨血管内皮生长因子(VEGF)在雄性生殖系精子发生发育和成熟过程中的调控作用,应用免疫组化、Periodic acid-Schiff(PAS)染色及蛋白质免疫印迹技术,检测VEGF蛋白在成年大鼠睾丸和附睾的表达和定位情况。Western-blots显示,在大鼠睾丸和附睾内均有VEGF蛋白(约45kD)的表达;免疫组化显示,睾丸内VEGF见于圆形和长形精子细胞、Sertoli细胞和Leydig细胞,免疫阳性产物位于细胞质内。精子细胞的VEGF表达伴随精子细胞顶体发育的全过程,精子残余体呈强阳性。附睾内VEGF表达于附睾管上皮,且有区域和细胞特异性。附睾起始段的所有上皮主细胞内都有VEGF阳性颗粒;头、体、尾各段的VEGF阳性细胞多数与含PAS阳性颗粒的细胞重合,证明为亮细胞;近端附睾的管腔内可见精子头部呈VEGF阳性染色。睾丸、附睾间质血管内皮为VEGF阴性。上述结果表明,VEGF蛋白可由生殖细胞和附睾管上皮细胞直接产生,它可能以自分泌和/或旁分泌的形式共同作用于睾丸和附睾的生殖细胞和血管内皮,直接或间接影响精子的发生、发育和成熟过程,特别是精子顶体的形成过程,并可能与精子在附睾内的成熟有关。     

小鼠精子表面Con A结合糖复合物的形成与变化

用辣根过氧化物酶标记的ＣｏｎＡ（伴刀豆素Ａ）对小鼠睾丸与附睾切片,以及对取自附睾和子宫（交配后）内的精子涂片进行了标记,旨在认识精子在发生、成熟和获能过程中表面糖复合物的形成与变化。本研究表明,睾丸内的生精细胞和支持细胞均呈ＣｏｎＡ标记阳性。附睾的输出小管和附睾管上皮细胞,ＣｏｎＡ标记呈中度至强阳性,有部位的差别。附睾头和附睾尾内精子表面的标记无明显差别,标记位置均主要在顶体区和尾部。精子在子宫内存留１．５小时后,顶体后区出现中度阳性标记,但存留３小时和６小时后,顶体和顶体后区的标记均减弱或消失。这些结果提示,（１）精子发生期即可合成ＣｏｎＡ结合糖复合物,（２）精子在附睾成熟过程中表面的ＣｏｎＡ结合糖复合物无明显变化,（３）精子获能后顶体后区出现的ＣｏｎＡ结合糖复合物可能与受精能力有关。     

血管内皮生长因子蛋白在大鼠睾丸和附睾的表达和定位研究

为探讨血管内皮生长因子(VEGF)在雄性生殖系精子发生发育和成熟过程中的调控作用,应用免疫组化、Periodic acid-Schiff(PAS)染色及蛋白质免疫印迹技术,检测VEGF蛋白在成年大鼠睾丸和附睾的表达和定位情况。Western-blots显示,在大鼠睾丸和附睾内均有VEGF蛋白(约45kD)的表达;免疫组化显示,睾丸内VEGF见于圆形和长形精子细胞、Sertoli细胞和Leydig细胞,免疫阳性产物位于细胞质内。精子细胞的VEGF表达伴随精子细胞项体发育的全过程,精子残余体呈强阳性。附睾内VEGF表达于附睾管上皮,且有区域和细胞特异性。附睾起始段的所有上皮主细胞内都有VEGF阳性颗粒;头、体、尾各段的VEGF阳性细胞多数与含PAS阳性颗粒的细胞重合,证明为亮细胞;近端附睾的管腔内可见精子头部呈VEGF阳性染色。睾丸、附睾间质血管内皮为VEGF阴性。上述结果表明,VEGF蛋白可由生殖细胞和附睾管上皮细胞直接产生,它可能以自分泌和／或旁分泌的形式共同作用于睾丸和附睾的生殖细胞和血管内皮,直接或间接影响精子的发生、发育和成熟过程,特别是精子顶体的形成过程,并可能与精子在附睾内的成熟有关。     

磁处理水对家兔生殖影响的研究

目的:探讨磁处理水对家免睾丸、附睾重量以及精子活力、沃纱、密度的影响。方法:新西兰雄性大白免36只,随机分为实验组和对照组。对照组饮用自来水,实验组饮用磁处理水,磁处理水每天更换,实验进行90天。光镜下检测每只家免附睾尾精子密度,精子活力,精子活率,最后将睾丸、附睾称重。结果:实验组与对照组比较,其睾丸附睾重量明显增加,精子密度增加14 % ,精子活力增加8% ,精子活率增加11% ,两组差异有显著性(P <0 .0 5 )。结论:实验结果提示饮用磁处理水能显著提高家免的生殖能力。     

精子和卵母细胞质量控制对山羊卵胞质内精子注射(ICSI)受精的影响

以体外成熟卵母细胞为材料研究了精子来源及制动处理方法、卵母细胞质量及注射后激活等因素对山羊ICSI效果的影响.结果说明,附睾头、体和尾精子ICSI后的受精率、卵裂率和桑椹胚/囊胚发育率与射出的鲜精精子都没有明显差异(p＞0.05),但带下注射时附睾头和体精子的受精和发育率显著低于附睾尾和射精精子.在以4种不同方法致死的精子中,室温保存24h的死精子ICSI受精、卵裂和桑椹/囊胚率虽然低于对照组,但是明显高于其它方式致死的精子;5℃保存15天的死精子受精和发育效果最差.0.0005%Triton X-100处理精子的受精率、卵裂率和桑椹/囊胚率显著(p＜0.05)高于制动对照组、不制动对照组和其它浓度组.经高渗处理法检测质量好的卵母细胞ICSI受精和胚胎发育效果显著好于质量差的卵母细胞.与对照组相比,A23187和Ionomycin/6-DMAP激活处理均显著(p＜0.05)提高ICSI的受精率、卵裂率和桑椹/囊胚发育率.因此,精子在附睾内的成熟过程主要与其获得与卵质膜融合能力有关;精液保存方法对精子受精能力的损伤程度有很大差异;适当浓度的Triton X-100处理可模仿精子制动;卵母细胞质量是影响ICSI效果的重要因素;注射精子后激活卵母细胞能保证山羊ICSI的受精效果.     

小鼠和豚鼠精子在附睾成熟过程中Ca~(2 )分布变化规律的研究

小鼠附睾头精子,其头部Ca~(2 )在顶体前区顶体外膜内侧结合最多,Ca~(2 )沉淀反应颗粒于该处呈连续层状。附睾头豚鼠精子其头部结合Ca~(2 )含量很少,且主要结合于顶体前区腹面顶体外膜内侧。小鼠附睾体和附睾尾精子Ca~(2 )的分布特征基本上和附睾头精子相同。但豚鼠附睾尾精子顶体外膜内侧无Ca~(2 )结合。和附睾头、附睾尾的附睾液相比,附睾体附睾液基质内具有大量Ca~(2 )存在。附睾体柱状上皮细胞的微绒毛切面上也具有Ca~(2 )沉淀反应颗粒,微绒毛可能与附睾液Ca~(2 )含量的调节有关。精子尾部Ca~(2 )主要分布于线粒体内,在质膜内、外两侧和线粒体外膜外侧也结合有少量的Ca~(2 )。和小鼠精子相比,豚鼠精子尾部线粒体内具有大量的Ca~(2 )。     

夹竹桃麻素对双酚a诱导的成年雄性小鼠精子损伤作用的实验研究

目的:研究NADPH氧化酶抑制剂夹竹桃麻素(Apocynin)对双酚a(Bisphenol a,BPA)诱导的成年雄性小鼠精子损伤过程中的作用。方法:成年雄性小鼠给以BPA刺激,给以Apocynin(1 mg/kg/day和10 mg/kg/day,分别处理7 day)进行治疗,观察其对BPA诱导的成年雄性小鼠精子损伤的作用。结果:BPA处理组小鼠附睾精子数目和活力明显降低,血清中睾酮和黄体生成素水平明显减少;Apocynin治疗明显增加BPA处理组小鼠附睾中精子数目和活力,但是对血清中睾酮和黄体生成素水平没有明显影响。另外,BPA处理组小鼠睾丸中丙二醛(Malonaldehyde,MDA)水平明显增加;Apocynin治疗明显抑制了BPA处理组小鼠睾丸中MDA水平。结论:NADPH氧化酶抑制剂Apocynin减轻BPA诱导的成年雄性小鼠精子损伤。     

羊精子表面的凝集素标记特征

用辣根过氧化物酶标记的蓖麻凝集素和伴刀豆素Ａ,对绵羊精子表面的凝集素标记特征进行了观察。蓖麻凝集素在睾丸内精子的顶体区有中等强度标记,尾部有弱标记,在附睾内成熟时,顶体区标记逐渐增强,尾部的标记消失,获能后标记强度则明显减弱。伴刀豆素Ａ的标记在睾丸内的精子仅限于顶体区,随着在附睾内成熟,顶体区的标记增强,尾部也出现弱的标记,获能后有部分精子的标记强度有所增加。实验结果表明,羊精子在成熟过程和获能过程表面糖复合物发生明显修饰。     

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.     

VEGF、VEGFR2在青春期大鼠睾丸、附睾及附睾精子上的表达

目的通过对血管内皮生长因子(VEGF)及其受体VEGFR2在青春期大鼠睾丸及附睾表达的研究,探讨其在雄性生殖器官中的作用。方法采用免疫组化法检测VEGF、VEGFR2在SD大鼠睾丸和附睾的表达定位,用免疫荧光法检测它们在大鼠附睾精子上的表达定位。结果VEGF及VEGFR2在青春期大鼠睾丸和附睾组织中均有表达。在睾丸中,VEGF主要表达于精原细胞胞质、精子细胞发育中的顶体、Sertoli细胞胞质及精子残余体内,Leydig细胞胞质也有阳性表达;VEGFR2主要表达于精子细胞发育中的顶体和间质细胞胞质。在附睾中,VEGF表达于附睾管上皮所有主细胞胞质内;而VEGFR2表达于附睾管头段和尾段上皮主细胞胞质内,体段免疫染色阴性。免疫荧光显示,VEGF与VEGFR2都与精子头部顶体、尾部颈段、中段和主段相结合,末段未见阳性荧光。结论VEGF及VEGFR2在大鼠的睾丸和附睾中均有表达,其表达定位具有细胞特异性和区域特异性,提示其可能在大鼠睾丸精子发生和附睾精子成熟中发挥重要作用。     

甘肃张掖黑河湿地黑鹳繁殖和迁徙习性

黑鹳(Ciconia nigra)属国家Ⅰ级保护野生动物.2010至2018年,通过样线、样带和固定样点调查的方法对张掖黑河湿地国家级自然保护区的黑鹳种群进行了监测,黑鹳最大种群数量均出现在每年的9月下旬,数量120～430只不等,年均308只.春季迁徙季节,黑鹳于3至4月到达保护区,部分个体会在此繁殖,其他个体会继续...     

黑麂Y染色体的鉴别和Sry基因的克隆及定位

以流式细胞仪分离小麂(Muntiacus reevesi)Y染色体和黑麂(Muntiacus crinifrons)Y1,Y2,X+4和1号染色体,利用DOP-PCR技术富集了分离的各单条染色体。然后,将小麂的Y染色体的DOP-PCR产物经Cy3标记后直接作为涂染探针,应用染色体涂染技术与雌雄黑麂的核型标本进行杂交,确认了黑麂真正的Y染色体为Y2染色体。再以黑麂的Y1,Y2,X+4和1号染色体的DOP-PCR产物为模板,用人的特异性的SRY（sex determining region of the Y chromosome）基因引物对其进行扩增,结果表明黑麂只有Y2染色体出现了SRY扩增片段。然后扩增产物克隆和测序,比较它与人的同源性,初步把黑麂的Sry基因定位在Y2染色体上。最后提取雄性黑麂的基因组DNA,并用同一对引物对其进行扩增,亦得到Sry基因的片段,对此扩增片段进行克隆,测序,结果表明其与Y2染色体得到的Sry基因片段完全一样,与人SRY基因的同源性均为83%。 Abstract：The single Y chromosome of Muntiacus reevesi and Y1,Y2 ,X+4,1 chromosome of Muntiacus crinifrons were obtained by flow-sorting ,then they were amplified through DOP-PCR . After that, the metaphase karyotype of Muntiacus crinifrons were painted by using the product of the DOP-PCR of the Y chromosome of Muntiacus reevesi as a special probe and the result showed that Y2 chromosome was the real Y chromosome of Muntiacus crinifrons. Secondly the product of the DOP-PCR of Y1,Y2,X+4,1 chromosome of Muntiacus crinifrons were used as the templates of the next amplification using the special primer devised according to the human SRY gene .One band was obtained only from Y2 chromosome, then it was cloned to the T-vector and sequenced. The Sry gene sequence of Muntiacus crinifrons was acquired and the conclution was that there are 83% homology between the human and Muntiacus crinifrons. It was testified that in all mammal Sry gene is consertive. On the other side the Sry gene was located to the Y2 chromosome of the Muntiacus crinifrons.     

Reeves' Muntjac Muntiacus reevesi in Britain: their history, spread, habitat selection, and the role of human intervention in accelerating their dispersal

The origins, early history, captive populations, spread and habitat preferences of Reeves' Muntjac in Britain are reviewed. It is suggested that much of the published information on the history of Muntjac in Britain is based on misconceptions, and that each subsequent report has continued to promulgate a false impression on the origins, time-scale and pattern of spread of the species in Britain. Indian and Reeves' Muntjac were introduced to Woburn Park in Bedfordshire within a year of each other, and it appears that the Indian Muntjac did not thrive, at least in the decade following their introduction. How long they survived as a free-living species in Britain is unclear, but it was probably only a few years. However, there is some evidence to suggest that they might have persisted within the Park at Woburn until 1930. Following the first releases from Woburn in 1901, the numbers of free-living Reeves' Muntjac in Britain remained low until the 1920s, when populations were largely confined to the woods around Woburn, and possibly also around Tring in Hertfordshire. However, in the 1930s and 1940s there were further deliberate introductions in selected areas some distance from Woburn. As a consequence, the subsequent spread of Reeves' Muntjac was from several main foci, i.e. from the vicinity of Woburn, the Norfolk/Suffolk border, three sites in Northamptonshire, two sites in Oxfordshire and two in Warwickshire. The spread in the second half of this century has been aided by further deliberate and accidental releases, and by these means new populations continue to be established outside the main range. Thus the natural spread has been much less impressive than previously assumed; even in areas with established populations it takes a long time for Muntjac to colonize all the available habitat. Data from a number of areas in Britain suggest that the natural rate of spread is about 1 km a year, which is comparable to other species of deer in Britain. The many introductions have complicated an analysis of the habitat preferences of Reeves' Muntjac, and no clear trends could be found. It would appear that Reeves' Muntjac are less dependent on specific types of habitat than previously believed. Examination of the land-class preferences using resource selection indices showed that arable land classes were predominantly selected for, and that marginal upland land classes tended to be avoided. Subsequent logistic regression models based on the land classes selected (and to a lesser extent avoided) by Muntjac were able to predict accurately the current distribution of Reeves' Muntjac in Britain, and one of these, together with our knowledge of their history and spread, was used to infer those areas most likely to be colonized by Muntjac in the near future. The greatest potential for range expansion is in Kent and Sussex, and to a lesser extent north into Lincolnshire, Nottinghamshire and south Yorkshire, and west into Cheshire and north Shropshire. However, long-established populations in areas such as Betws-y-Coed in Wales show that Muntjac may persist in low numbers in atypical habitats. Future habitat changes, such as the planting of new woodlands, and continued deliberate and accidental releases, are likely to lead to population changes in addition to those predicted by the logistic regression model.     

麂属(Muntiacus)动物线粒体12S rRNA、细胞色素b基因和多药耐药基因序列分析及其分子进化关系

对麂属（Muntiacus)中的3种动物：赤麂（M.muntjak)(2n=6♀,7♂）,小麂（M.reevesi)(2n=46),黑麂（M.cri.nifrons)(2n=8♀,9♂）线粒体DNA 12S rRNA和细胞色素b基因784bp左右的片段和核基因－多药耐药基因（multidrug resistance,MDR1)的728bp左右的片段进行了序列分析,并根据序列信息建立了分子系统树,同时探讨了这3种动物的起源,分类地位及进化关系。     

小麂、赤麂、黑麂mtDNA序列变异性及反映的进化关系

利用已测定的鹿科麂亚科动物小麂、赤麂、黑麂的线粒体全基因组序列,统计它们各自连接在一起的13个蛋白编码基因、22个tRNA基因、2个rRNA基因和1个控制区序列的碱基长度和组成,计算rRNA基因遗传距离,估算分歧时间,比较蛋白编码基因的碱基水平和氨基酸水平上的差异,基于连接在一起的13个氨基酸序列,以羊为外群,通过邻位相连法和最大简约性法构建进化树,探讨小麂、赤麂、黑麂的进化关系。结果表明,小麂是较原始的物种,赤麂和黑麂较为近缘,是从类似小麂的祖先演化而来。     

小麂、黑麂、赤麂精母细胞联会复合体的比较研究

本工作以界面铺张——硝酸银染色技术,对小麂(Muntiacus reeuesi)、黑麂(M.crinifrons)和赤麂(M.muntjak)的精母细胞联会复合体(Syna ptonemal complex,SC)进行亚显微结构的比较研究。结果表明: 1.SC的平均相对长度和臂比指数同有丝分裂细胞相应染色体的数值有很好的一致性。根据SC的相对长度和臂比指数绘制了三种麂的SC组型图。雄性黑麂减数分裂前期形成一个复杂的易位多价体,意味着其核型的演化过程涉及两次染色体易位和一次臂间倒位。 2.在减数分裂前期,性染色体的形态和行为同常染色体的有明显差异,如性染色体嗜银性较强,配对延迟等。XY的配对起始于早粗线期,在中粗线期,Y的全长均同X配对;XY-SC开始解体于晚粗线期。 3.在粗线期,X染色体未配对区域出现自身折叠,形成“发夹”状结构。这种“发夹”结构的形成,可能是在性染色体的进化过程中,X染色体通过不对称易位得到的重复片段在减数分裂前期同源配对的一种细胞学表现。     

麂属(Muntiacus)动物MDR-1基因序列分析及其分子进化关系

对麂属（Muntiacus)中的3种动物：赤麂（M.muntjak)(2n-6♀,7♂）,小麂（M.reevesi)(2n=46),黑麂（M.crinifrons(2n=8♀,9♂）MDR－1基因（multidrug resistance,多药耐药基因）726bp左右的片段进行了序列分析并根据序列信息建立分子系统树,同时探讨了这3种动物的起源,分类地位及进化关系。     

麂属(Muntiacus)动物线粒体12SrRNA和细胞色素B基因序列分析及其分子进化关系

对麂属（Muntiacus)中的3种动物;赤麂（M.muntjak)（2n=6♀,7♂）,小麂（M.reevesi)(2n=46）,黑（M.crinifrons(2♀,9♂）线粒体DNA12SrRNA和细胞色素B783bp左右的片段进行序列分析,并根据序列信息建立分子系统树,同时探讨了这3种动物的起源,分类地位及进化关系。     

High-density comparative BAC mapping in the black muntjac (Muntiacus crinifrons): molecular cytogenetic dissection of the origin of MCR 1p+4 in the X1X2Y1Y2Y3 sex chromosome system

The black muntjac (Muntiacus crinifrons, 2n = 8[female symbol]/9[male symbol]) is a critically endangered mammalian species that is confined to a narrow region of southeastern China. Male black muntjacs have an astonishing X1X2Y1Y2Y3 sex chromosome system, unparalleled in eutherian mammals, involving approximately half of the entire genome. A high-resolution comparative map between the black muntjac (M. crinifrons) and the Chinese muntjac (M. reevesi, 2n = 46) has been constructed based on the chromosomal localization of 304 clones from a genomic BAC (bacterial artificial chromosome) library of the Indian muntjac (M. muntjak vaginalis, 2n = 6[female symbol]/7[male symbol]). In addition to validating the chromosomal homologies between M. reevesi and M. crinifrons defined previously by chromosome painting, the comparative BAC map demonstrates that all tandem fusions that have occurred in the karyotypic evolution of M. crinifrons are centromere-telomere fusions. The map also allows for a more detailed reconstruction of the chromosomal rearrangements leading to this unique and complex sex chromosome system. Furthermore, we have identified 46 BAC clones that could be used to study the molecular evolution of the unique sex chromosomes of the male black muntjacs.     

Isolation and characterization of microsatellite markers in black muntjac (Muntiacus crinifrons)

The black muntjac (Muntiacus crinifrons) is a vulnerable species found in the mountains of eastern China, about which little is known. Here we develop 11 polymorphic microsatellite loci from a (CA)(n) -enrichment library for the animal. In the analyses of 25 individuals sampled, unbiased expected heterozygosity levels varied from 0.686 to 0.876 and the number of alleles per locus varied from five to nine. Results that 11 microsatellite loci were highly polymorphic indicated that these markers are sufficiently powerful to address such questions as parentage, mating system and population genetic structure of M. crinifrons.