鸭圆环病毒与鸭Ⅰ型肝炎病毒二重 PCR 检测方法的建立

目的：建立一种同时检测鸭圆环病毒（DuCV）和鸭I型肝炎病毒（DHV）病原体的二重PCR技术。方法：根据DuCV和DHV的基因文库,分别设计了2对与DuCV和DHV某段基因序列互补的引物,用这2对引物对同一样品中DuCV和DHV模板进行二重PCR扩增。结果与结论：用建立的方法均同时得到了2条特异性的大小与实验设计相符（DuCV：245bp;DHV：569bp）的二重PCR扩增带,而且对其他禽病病原的PCR扩增结果均为阴性,能同时检出56Pg的DHVRNA模板和6Pg的DuCVDNA模板。     

Microsatellite markers for two stifftail ducks: the white‐headed duck,Oxyura leucocephala,and the ruddy duck,O. jamaicensis

Hybridization with a close relative, the North American ruddy duck (Oxyura jamaicensis), is a major problem for the conservation of the endangered white‐headed duck (Oxyura leucocephala). We report the development of 11 microsatellite markers that can facilitate the identification of hybrids as well as the study of the population structure of both species across their distributions. These markers were tested in 63 white‐headed ducks and 50 ruddy ducks and show a larger diversity in the latter species.     

鸭呼肠孤病毒强毒株致鸭胚原代成纤维细胞凋亡的研究

通过光镜、电镜、DNA Ladder法、流式细胞术、荧光染色对鸭呼肠孤病毒(DRV)诱导鸭胚原代成纤维细胞(DEF)凋亡情况进行检测.结果显示,光镜可见细胞形态学上出现细胞皱缩,染色质浓染边移;电镜观察到细胞胞浆浓缩,细胞核染色质凝聚、部分形成凋亡小体;荧光染色结果显示,在感染后24h有激发绿色荧光的凋亡细胞出现,随着时间的推移,激发红色荧光的死亡细胞数量增多;DNA Ladder检测到感染后24～144h的DNA样品呈梯形条带;流式细胞术于感染后24h检测到凋亡细胞,其数量在72～96h达到高峰,144h开始下降.研究结果表明,DRV在DEF增殖的过程中具有诱导宿主细胞凋亡的作用.     

氧化苦参碱在鸭原代肝细胞中抗鸭乙肝病毒(DHBV)作用的研究

通过建立鸭原代肝细胞-DHBV感染模型研究氧化苦参碱抗DHBV的作用。分别在DHBV感染前、感染同时以及感染后给药,利用打点杂交、Southern印迹核酸杂交和荧光定量PCR方法分别检测培养细胞上清及细胞内病毒核酸,观察氧化苦参碱在病毒感染的各个环节所起的抗病毒作用。实验结果显示:1mg/mL氧化苦参碱处理细胞后,鸭原代肝细胞培养上清及细胞内的DHBV核酸明显低于病毒感染对照组,病毒抑制率达91.6%;在病毒感染同时加药对病毒的抑制率可达98.5%;感染后持续用药能使不同培养天数的鸭肝细胞内的DHBV核酸降低60.5%~96.6%;氧化苦参碱与DHBV共孵育后,可以使病毒感染力下降69.6%。结果说明氧化苦参碱可以在DHBV感染鸭原代肝细胞的多个环节,包括病毒吸附、进入细胞及细胞内复制等方面发挥抗病毒作用。     

Species‐specific habitat use of wing‐moulting waterbirds in response to temporary flightlessness

The choice of the moulting habitat is of paramount importance for wing‐moulting waterbirds that have to cope with a flightless period of several weeks. However, some species might have more restricted habitat requirements during moult than others, for example due to a highly specialized feeding ecology. The moult‐related habitat use of five species (Gadwall Anas strepera, Red‐crested Pochard Netta rufina, Common Pochard Aythya ferina, Tufted Duck Aythya fuligula, Coot Fulica atra) was compared at a European inland moulting site that offered a variety of water bodies characterized by different levels of nutrient concentration, water depth, shoreline vegetation density and disturbance. To determine location‐ and species‐specific densities, birds were regularly counted throughout the moulting seasons of 2010 and 2011. In 2011, additional data on Gadwalls were used to assess differences in requirements between the flightless phase of moult and the periods before and after. Furthermore, habitat choice of 38 tagged Gadwalls was compared among two to four successive years. During the moulting season, all species showed clear preferences for specific levels of nutrient content, suggesting an active choice of suitable food sources in both food specialists and generalists. Species showing the strongest attachment to shallow water (Gadwall and Coot) were most sensitive to human disturbance and increasing water depths, and species averse to diving (Gadwall) used ponds with dense shore vegetation while flightless. For Gadwalls, habitat conditions rather than nutrient supply became increasingly important during the flightless phase. Average return rates of 59 and 54% were recorded for male and female Gadwalls, respectively, and the repeated use of familiar locations could be demonstrated in the majority of returning birds (65%). Familiarity with the habitat apparently plays an important role and may enable individuals to compensate for suboptimal conditions at the moulting site.     

Capture and Mortality Rates of Ducks in Selected Trap Types

ABSTRACT We evaluated different trap styles and related mortality of trapped ducks (Anas spp.) for 3 field seasons as part of the United States-Canada Cooperative Waterfowl Banding Program. During 2002, we evaluated 4 trap designs and caught 10,966 ducks. Trap style affected capture rates (P = 0.018, F₅ = 9.02), with Benning II and oval traps catching more ducks than cloverleaf and star traps. In 2003, we tested 3 trap styles and caught 10,849 ducks. Trap style affected duck capture rates (P < 0.01, F₅ = 15.16), with oval traps with 6-m lead panels catching more ducks than Benning II traps and cloverleaf traps. During 2004, we tested 3 trap styles and caught 11,737 ducks. Trap style affected capture rates (P < 0.01, F₅ = 11.23), with oval traps with 6-m leads catching more ducks than either the oval trap without leads or Benning II traps. Trap style affected mortality rates of ducks, but overall mortality of trapped ducks was low with a rate of 1.16% in 2002, 0.32% in 2003, and 0.17% in 2004; mortality was not a major problem in our study. Waterfowl managers may be able to catch more ducks using oval traps with leads without increasing mortality of captured ducks.     

番鸭呼肠孤病毒的鉴定

从以软脚为主要临床症状,以肝、脾表面有多量灰白色坏死点,肾肿大及出血为主要病变的病番鸭肝、脾组织中分离到5株病毒(MW9710、MW9803、MW9806、MW9809和MW9810).雏番鸭和雏鹅经人工感染后出现与自然病例相同的临床症状和病理变化,并能回收到病毒.樱桃谷鸭、麻鸭和鸡人工感染不发病.经电镜观察,病毒呈球形,正二十面体,立体对称,无囊膜,有双层衣壳,直径为60nm～73nm,病毒粒子在胞浆中增殖.病毒对乙醚、氯仿、胰蛋白酶、50℃处理1h和3%甲醛处理不敏感.对pH3处理2h、60℃处理30min和紫外线照射敏感.1mol/L Mg-Cl2不能增强病毒的感染力.病毒核酸型为dsRNA,病毒核酸具有禽呼肠孤病毒的特征:有10条带,按其大小可分为三类:大片段(L1～L3)、中片段(M1～M3)和小片段(S1～S4).但是MW9710株的M2和S1～S4片段的迁移率明显不同于鸡关节炎病毒(ARV)S1133株,而与番鸭呼肠孤病毒法国株(89330、89026株)的核酸电泳图谱极为相似.在血清中和试验中,ARV S1133和MW9710株互不交叉.并且,以针对ARV S1基因的特异性引物XZ11、XZ12对MW9710株等进行RT-PCR扩增,只能从ARV中扩增出特异性条带;而以MDRV89026株S1基因的特异引物HP11、HP12进行RT-PCR扩增,只能从MW9710等分离毒株中扩增出特异性条带.上述结果表明,MW9710株等5株病毒是上述疫病(番鸭"肝白点病")的病原,属呼肠孤病毒科正呼肠孤病毒属番鸭呼肠孤病毒.     

圈养条件下鸳鸯的自然繁殖

本文对成都动物园圈养条件下鸳鸯的自然繁殖和行为进行了观察,结果表明：巢箱要求放置不是太高,只要光线较暗或比较隐蔽即可;声音对圈养条件下鸳鸯的繁殖干扰不大;在发情和育雏期间应适当增加动物性蛋白饲料;断翅后的鸳鸯受精率略低于未断翅鸳鸯.     

鸭类mtDNA限制性酶切图谱的比较研究

本文报道了番鸭、建昌鸭、杂交鸭(♀建昌鸭×(?)番鸭)和北京鸭的mtDNA限制性酶切图谱。限制性内切酶HindⅢ、PsiⅠ、BamHⅠ和EcoRⅠ在番鸭mtDNA上分别有(?)、2、2和1个酶切位点。建昌鸭、杂交鸭和北京鸭的mtDNA限制性酶切图谱完全一致。以上4种内切酶在这3种鸭子mtDNA上分别有5、4、2和1个位点。比较研究4种限制性图谱,我们得到三点结论:(1)鸭类mtDN种间差异程度很高;(2)家鸭很可能不存在mtDNA种内异质现象;(3)鸭类mtDNA为母性遗传。     

麻鸭肠道无芽胞厌氧菌定性、定量和定位研究

本研究采用气、液相色谱分析法(Gas-Liquid Chromatography,GLC)分析细菌代谢产物,结合微生物学鉴定和微量快速生化反应,在我国首次定量测定了麻鸭小肠、大肠每克内容物4种厌氧菌的菌数,初次确定在小肠有卵形类杆菌、发酵乳杆菌、两歧双歧杆菌、空肠弯曲杆菌4个种;在大肠有卵形类杆菌、多形类杆菌、解脲类杆菌、发酵乳杆菌、干酪乳杆菌、植物乳杆菌、短双歧杆菌、空肠弯曲杆菌和粪弯曲杆菌9个种。类杆菌和乳杆菌等是麻鸭肠道正常微生物群。     

腺病毒载体介导的GFP基因在鸭胚成纤维细胞中的表达及RNA干扰

目的：建立在鸭胚成纤维细胞（DEF）中进行RNA干扰（RNAi）的技术平台,为鸭基因组功能的研究提供新的技术手段。方法：以绿色荧光蛋白（GFP）基因为报告基因,脂质体转染化学合成的GFP特异小干扰RNA（GFP-siRNA）,用流式细胞仪测定GFP-siRNA对重组腺病毒（Adv-GFP）介导的GFP基因在DEF中表达的干扰效果。结果：200MOI（感染复数）Adv-GFP介导的GFP基因在DEF中表达效率最高,为31．20％±3．1l％,对DEF的活力无明显影响;GFP-siRNA能有效干扰GFP基因在DEF中的表达,相对抑制率为98．56％。结论：在DEF中进行RNAi是可行的,Adv-GFP是介导外源基因在DEF中表达较为理想的载体;首次建立了在DEF中进行RNAi的技术平台,为鸭基因组的功能等研究提供了新的技术手段。     

AFLP analysis of genetic diversity and relationship among some Chinese domestic ducks and wild ducks

The amplified fragment length polymorphic (AFLP) technique was used to analyze the genome DNA polymorphism among 8 breeds of domestic ducks and 2 species of wild ducks. Nine of the 17 selected primers pairs gave reproducible polymorphic DNA amplification bands. The amplified bands ranged from 44 to 83 per primer pair. Of the 513 AFLP markers obtained, 498 were polymorphic. The proportion of polymorphic loci was 97.1%. The genetic distance (D) and similarity coefficients (GS) were calculated based on the polymorphic data. Between domestic ducks D ranged from 0.331 to 0.589, while between domestic ducks and the wild ducks, it ranged from 0.298 to 0.520 (vs. Anas Platyrhynchos) and from 0.316 to 0.522 (vs. A. Poecilorhyncha), respectively. The variance analysis showed no significant difference between the two groups of data, which indicated that both mallard and spot-billed ducks made contributions to domestic duck evolution. A dendrogram was constructed according to the D value. __________ Translated from Journal of Xiamen University (Natural Science), 2005, 44(5): 729–733 [译自: 厦门大学学报 (自然科学版), 2005, 44(5): 729–733]     

Origin and domestication history of Peking ducks deltermined through microsatellite and mitochondrial marker analysis

In order to elucidate the domestication history of Peking ducks, 190 blood samples from six Chinese indigenous duck breeds were collected with186 individualsgenotyped by 15 microsatellite markers. Both the F_ST and Nei’s standard genetic distances (D_s) from the microsatellite data indicated high genetic differentiation between Peking duck and other Chinese indigenous breeds. The haplotype network with mtDNA data showed that most of the Peking duck haplotypes were distinctly different from those of other domestic breeds. Although the H01 haplotype was shared by all domesticated duck breeds, Peking ducks displayed 12 specific domestic duck haplotypes, including four similar haplotypes H02, H04, H08 and H22, that formed a single haplogroup (A). Both H02 and H22 haplotypes were also shared by mallard and Peking ducks, indicating that Peking ducks originated from wild mallard ducks.     

AFLP analysis of genetic diversity and relationship among some Chinese domestic ducks and wild ducks

The amplified fragment length polymorphic(AFLP)technique was used to analyze the genome DNA polymorphism among 8 breeds of domestic ducks and 2 species of wild ducks.Nine of the 17 selected primers pairs gave reproducible polymorphic DNA amplification bands.The amplified bands ranged from 44 to 83 per primer pair.Of the 513 AFLP markers obtained.498 were polymorphic.The proportion of polymorphic loci was 97.1%.The genetic distance(D)and similarity coefficients(GS)were calculated based on the polymorphic data.Between domestic ducks D ranged from 0.331 to 0.589,while between domestic ducks and the wild ducks,it ranged from 0.298 to 0.520(vs.Anas Platyrhynchos)and from 0.316 to 0.522(vs.A.Poecilorhyncha),respectively.The variance analysis showed no significant difference between the two groups of data,which indicated that both mallard and spot-billed ducks made contributions to domestic duck evolution.A dendrogram was constructed according to the D value.     

鸭胚成纤维细胞中鸭瘟强毒的增殖特性研究

通过细胞培养物光学显微观察、细胞超薄切片研究、定量PCR检测技术对鸭胚成纤维细胞中鸭瘟强毒的增殖特性进行了研究.结果表明:鸭瘟强毒接种鸭胚成纤维细胞后42 h,可使细胞培养物出现大量明显的蚀斑病变.细胞培养物的超薄切片电镜观察研究表明,病毒核酸在胞核内常集中分布,呈直径35～45 nm的圆形颗粒状;核衣壳在胞核和胞浆内都有分布,呈直径90～100 nm的网形颗粒状;成熟病毒位于胞浆空泡内,呈直径150～300 nm的圆形,有囊膜和皮层结构;病毒通过囊膜与胞膜融合入侵细胞,在核内生成核酸、装配核衣壳,在胞浆中得到皮层,出芽到胞浆空泡内获得囊膜,通过胞吐作用释放到胞外.定量PCR研究表明:鸭瘟强毒接种细胞后10 h开始明显复制,接毒后30 h时含量趋于稳定,接毒后22 h时开始向胞外释放,50 h时达最大值,细胞和上清中病毒含量的增幅均为103左右,病毒主要存在于细胞中,其含量为上清的102～103倍.     

Genetic signature of hybridization between Chinese spot-billed ducks and domesticated ducks

In this study, we analyzed 93 whole genomes from Chinese spot-billed ducks (CSB), meat-type ducks (MET), and egg and dual purpose-type ducks (EDT) to characterize the genetic material flowing between the CSB and modern ducks. Using a frequency of shared identical-by-descent method, approximately 10.9 Mb introgression segments containing 140 genes were identified showing the signatures of introgression between CSB and EDT. Meanwhile, nearly 10.6 M introgression regions containing 149 genes were identified between CSB and MET. Based on the haplotypes tree of each segment, we found that the introgression between CSB and domesticated ducks was asymmetric with a high level of gene flow from domestic to CSB and a low level of migration in the opposite direction. Moreover, we identified several genes that were introgressions from CSB and showed the signature of positive selection, which may contribute to the breeding of modern ducks. Our results provide new insight into the evolution and breeding history of domestic ducks and may be useful for the future management of wild and domestic duck populations.     

鸭肠炎病毒CHv强毒株超微结构研究

将鸭成纤维细胞培养的鸭肠炎病毒(DEV),经超声处理、高速冷冻差速离心后,采用酒石酸钾—甘油非线性密度梯度超速离心,收集病毒蛋白带,3%磷钨酸负染后观察病毒粒子形态。结果表明:病毒粒子主要集中在40%~50%酒石酸钾—甘油缓冲液交界层。电镜下,病毒粒子纯净,具有疱疹病毒典型形态结构,剖面六角,外观轮廓清楚。成熟病毒粒子直径约150~266nm,病毒囊膜、核衣壳和核心清晰可见;囊膜外层较内层着色略深,且可见尚未形成完整囊膜的柄状拖尾结构。多数病毒粒子以单核衣壳为主,一定数量的病毒具有双核衣壳,偶见三核衣壳,核衣壳直径为100~150nm,呈现致密圆形、半圆形或马蹄形等类型。在核衣壳外和囊膜之间可见明显的亮晕。核心DNA电子染色较深,集中分布,直径40~65nm。本文获得的清晰DEV负染超微结构照片,为该病毒结构生物学的研究提供了重要依据。