鲤鱼早期发育过程中免疫相关器官的发生

参与鱼类免疫应答的主要组织和器官有肾(特别是头肾)、脾、胸腺、血液和淋巴等。近30年来,随着鱼类免疫学的迅速发展,国内外许多学者在鱼类免疫相关组织和器官的结构、功能及免疫机理方面作了不少工作,但在鱼类免疫相关器官的发生方面所作工作很少。本文以正常鲤鱼的受精卵及不同发育阶段的幼鱼为材料,以Bouin‘s液固定,常规石蜡包埋,连续切片,然后利用酸性条件下的阿新兰染色和过碘酸——雪夫氏试剂反应相接合的方法(AB—PAS染色)处理切片,对鲤鱼早期发育过程中免疫相关器官的发生作了初步研究。结果表明,肾脏是出现最早的免疫器官,孵化前第一天(受精后第五天)就已经发现肾小管(Fig．1),孵化后第二天,在两个大的心窭之上出现网状的头肾组织,两条主要的,肾小管向后延伸在接近肛门处联合。在这个时期,骨小管之间分布有许多未分化的造血干细胞(Fig.2)和成熟的红细胞(Fig.3)。孵化后第五天,肾小管盘绕卷曲,肾小管之间的血细胞数目也有增加,出现体积较小的淋巴细胞(Fig．4)。孵化后第九天,造血组织同发育中的淋巴细胞数量大大增加,至孵化后30天,头肾、中肾、小管已很少,大部分被造血组织所充满。脾脏于孵化当天出现,位于肝胰脏之左后侧的肠背系膜上,含有红细胞和造血干细胞(Fig．5)。孵化三天后,脾脏生长速度加快,出现网状细胞、结缔组织和淋巴组织。肝脏与胰腺几乎同时出现于孵化当天,最初,两个腺体相互独立(Fig.6),孵化两天后,胰腺开始侵入肝组织中(Fig．7)。未发现造血组织和淋巴细胞存在于早期的肝组织中。胸腺于孵化后第三天,在第二鳃弓和第三鳃弓上方出现（Fig．8）。至第五天,胸腺中的细胞开始出现分化(Fig.9)以上结果比Botham等人报道的鲤鱼免疫相关器官的发生时间有所提前。     

斜带石斑鱼淋巴器官个体发育的组织学

本文应用连续组织切片技术和组织学观察,对出膜后1～60天的斜带石斑鱼(Epinephelus coioides)各期仔鱼、稚鱼和幼鱼的淋巴器官组织进行了研究,描述了淋巴器官的个体发育过程和组织学结构特征。研究表明：实验水温为22．0～27．8℃时,孵化后第10天出现头肾原基。头肾原基由未分化的造血干细胞组成。随着鱼体的生长,头肾原基的造血干细胞很快分化成不同类型的细胞;头肾主要由网状内皮系统支持下的淋巴造血组织构成。第11天出现脾脏原基。脾脏原基由造血细胞组成,淋巴化速度相对较慢。脾脏在整个发育过程中,红细胞和类红细胞占优势,没有红髓和白髓之分。第13天出现胸腺原基。胸腺发育速度较快,是明显的淋巴器官。胸腺主要由胸腺细胞(淋巴细胞)和上皮细胞组成,外区和内区没有明显的界限,但很容易区分。胸腺外被单层的上皮细胞层与咽腔相隔,保持浅表的位置,并且在整个发育过程中,胸腺与头肾是独立分开的。免疫器官原基出现顺序是头肾、脾脏和胸腺;而免疫器官淋巴化的顺序是胸腺,头肾和脾脏。和其它硬骨鱼类一样,斜带石斑鱼在早期发育阶段,淋巴器官的发育较迟,出现相对滞后的现象[动物学报49(6)：819～828,2003]。     

鳜鱼头肾的组织发生及成鱼头肾B淋巴细胞的分布

通过整体连续切片,研究了鳜鱼不同发育时期的头肾结构,并利用原位PCR方法检测了B淋巴细胞在鳜鱼头肾中的分布。在孵化后第1d观察到了肾组织,主要由肾小管组成。尔后头肾的发育经历了三个结构和功能的转变。第一个阶段为孵化后第1d到第7d,头肾作为滤过性器官存在,由肾小管及少量淋巴细胞组成。第二个阶段从第8d到第36d,是一个功能混合型阶段,头肾中既有肾小管,又有造血组织;随时间推移,肾小管数量减少,淋巴细胞数量剧增。紧接着进入第三个阶段：肾小管完全消失,头肾中开始出现大量的嗜铬细胞,头肾作为淋巴-肾上腺组织而存在。肾上腺首先出现在头肾前端,随发育成熟,集中分布于头肾门静脉周围。IgM在鳜头肾中大量表达,IgM分泌细胞分布于整个头肾组织,在血管周围有集中趋势[动物学报51(3)：440—446,20051。     

火炬松成熟合子胚离体培养过程中诱导不定芽的影响因素研究(英文)

火炬松（ＰｉｎｕｓｔａｅｄＬ）界南方松中最重要的针叶树种之一,在环境保护,园林绿化和林业生产中有重要应用价值。有关火炬松未成熟胚的体细胞胚胎发生和器官发生的研究报道不多,其成熟合子胚的愈伤组织器官发生则未见报道。本文以取自湖南省邵阳市林场的火炬松成熟种胚为外植体,在诱导其愈伤组织器官发生的基础上,系统地研究了ＢＡ浓度,基本培养基（ＴＥ）浓度和不同碳源等对愈伤组织上不定芽的发生和发育的影响,优化了火炬松离体再生的培养条件,为火炬松的无性繁殖技术应用于实际生产奠定了基础。研究结果表明：不同的浓度条件下,４ｍｇ／ＬＢＡ培养基上的不定芽诱导频率和每个胚上的芽平均数最高,分别是７６．３％和３．４。火炬松器官发生愈伤组织（Ｆｉｇ．１）上的不定芽形成于愈伤组织表面（Ｆｉｇ．２）。不定芽的发生常不同步（Ｆｉｇ．３）。不定芽在低浓度ＢＡ（１～２ｍｇ／Ｌ）条件下发育较好（Ｆｉｇ．４）,在高浓度ＢＡ（８～１６ｍｇ／Ｌ）条件下发育减慢（Ｆｉｇ．５）,在１ｍｇ／ＬＢＡ条件下伸长生长较快（Ｆｉｇ．６）;不同浓度基本培养基的实验结果表明,当基本培养基浓度为１．２５ＴＥ时,不定芽诱导频率（７３．５％）和每个胚上的芽平均数（３．９）最高。当     

中华鳖造血和免疫器官的个体发育

采用常规孵化的中华鳖胚胎为材料,对不同发育时期造血和免疫器官进行了组织学研究,描述了卵黄囊、胸腺、肝、脾、肾以及骨髓的形态结构变化。发现胚胎期首先出现的造血器官是卵黄囊。此后,卵黄囊的造血干细胞出现在胚体的血循环中,造血功能相继在胚胎胸腺、肝、脾、骨髓(可能还包括肾)中产生。胸腺是中华鳖免疫系统发育的第一个淋巴器官,来自卵黄囊的干细胞在此先分化成小淋巴细胞,然后再迁移至脾脏。脾脏发育中首先出现各发育阶段的红细胞、嗜酸性的细胞和少量粒细胞,淋巴细胞出现较晚,未发现淋巴小结。在胚胎期肝脏发育过程中可见不同发育时期的红细胞和嗜酸性的细胞。在肾的发育过程中,尚可观察到嗜酸性的细胞和类似头肾组织的细胞团。直至出壳前,骨髓内方可见各发育阶段的各系细胞[动物学报49(2)：238—247,2003]。     

乙型脑炎减毒活疫苗（SA14—14—2）在豚鼠体内保护作用的免疫…

本实验将乙脑减毒活疫苗ＳＡ１４－１４－２株以不同疫苗病毒量（３．８７ＰＦＵ／ｍｌ和５．８７ＰＦＵ／ｍｌ）分别一次免疫豚鼠,观察其对强毒攻击后抑制毒血症和抗体形成的能力。结果显示疫苗（５．８７ＰＦＵ／ｍｌ）免疫组豚鼠攻击前虽然中和抗体阴性或很低,但经攻击感染后不同时间内均未出现病毒血症,对照组豚鼠则于第２,３,４天全部出现病毒血症。表明一次活疫苗免疫后能有效地抑制病毒血症的产生。免疫后３０天虽然免疫     

影响火炬松胚性悬浮细胞原生质体的胚胎发生的因素(英文)

火炬松（ＰｉｎｕｓｔａｅｄａＬ．）是我国亚热带和部分热带地区最重要的绿化和造林树种。它的生长周期长,杂合程度高,难以用常规的杂交方法进行品种改良。建立火炬松的原生质体胚胎发生体系,有可能、进而以遗传转化为基础进行火炬松等针叶树的品种改良。本研究以湖南省绍阳市的火炬松成熟种子为材料,建立胚性细胞悬浮系。将其培养至对数生长期,用１％ＲＳ、２．５％Ｒ１０和０．２％Ｙ２３的酶混和液分离原生质体,活力达９０％以上（Ｆｉｇ．１）。纯化原生质体,在再生培养基上培养２天后,细胞壁再生（Ｆｉｇ．２）;;６天后,６５％的原生质体第１次分裂（Ｆｉｇ．３）;培养３周后,形成小细胞团（Ｆｉｇ．４）;６周后,形成大细胞团（Ｆｉｇ．５）;８周后,形成胚性胚柄细胞团（ＥＳＭ）（Ｆｉｇ．６）;１０周后,形成早期体细胞胚（ＥＳＥ）（Ｆｉｇ．７）;１２周后,形成后期体细胞胚（ＬＳＥ）（Ｆｉｇ．８）火炬松原生质体胚形成过程中的关键结构是ＥＳＭ,ＥＳＥ和ＬＳＥ。它们形成的最佳基本培养基是１．２５ＬＰ培养基。再生培养基中高浓度的ＢＡ和低浓度的肌醇有利于ＥＳＭ的形成,但不利于ＥＳＥ和ＬＳＥ的形成。反之,低浓度的ＢＡ和高浓度的肌醇不利于ＥＳＭ的形成,     

用RAPD法研究火炬松愈伤组织发生的遗传特性(英文)

体外培养对于植物的快速繁殖是非常有效的。和其它一些松果类硬木植物一样,火炬松的体外培养成功率却一直很低。本工作研究了不同的基本培养基和低温条件对于火炬松Ｊ－５６, Ｓ－１００３, ａｎｄ Ｅ－４４０等三个品系的成熟合子胚形成愈伤组织、分化出芽、成苗的影响。在不同的基本培养基条件下芽分化的程度差异很大。合子胚经过９－１２周培养,开始分化,形成具有器官发生的愈伤组织（Ｆｉｇ．２ａ）。分化后３周,开始诱导出芽（Ｆｉｇ．２ｂ）,芽的生长快慢不同（Ｆｉｇ．２ｃ,ｄ）。同一个愈伤组织上会生出几个芽来（Ｆｉｇ．２ｅ）。在添加有ＩＢＡ和ＢＡ的ＴＥ培养基上芽生长最快（Ｆｉｇ．１）。低温条件持续 １５天,能增加芽的数量和分化的程度（Ｔａｂｌｅ１）。上述培养基中增加ＧＡ３时表明,ＧＡ３对于根的诱导有决定性的作用。将９８株再生苗转移到特殊的混合土壤上;成活了７５株苗（Ｆｉｇ．２ｆ）。以这三种火炬松的再生苗尖为材料制备ＤＮＡ。用２０个引物进行ＲＡＰＤ分析,结果表明：这三种火炬松苗的扩增产物是相同的（Ｆｉｇ．２ｇ,ｈ＆ｉ）。这说明：用愈伤组织克隆植株的过程中没有引起植物遗传变异。     

杂交柑桔的胚胎发育(英文)

柑桔类珠心胚现象对研究其进化和种质保存方面有着重要意义,但是给其有性杂交育种工作造成相当大的麻烦：它不仅使杂交后代难于区分合子苗和珠心苗,而且会使合子胚发育中途天折。解决的途径是适时分离合子胚进行单独培养。为此,本工作于柑桔胚胎发育的不同时期取样、固定、观察,研究其合子胚发育规律,确定珠心胚侵入胚囊的时期。结果表明：一般情况下,授粉后３０ｄ,合于处于单细胞状态（Ｆｉｇ．１Ａ）;授粉后４０ｄ;合子开始分裂（Ｆｉｇ．１Ｂ）;授粉后４５ｄ,合子胚形成８－１６个细胞,珠心胚开始分裂（Ｆｉｇ．１Ｃ）;授粉后５０ｄ,合子形成球形胚,珠心胚尚未侵入胚囊（Ｆｉｇ．１Ｄ＆Ｅ）;授粉后５５ｄ,合子胚为球形胚或早心形胚,开始有少数珠心胚侵入胚囊（Ｆｉｇ．１Ｄ＆Ｅ）;授粉后６０ｄ,合子胚为心形胚（Ｆｉｇ．１Ｇ）。授粉后８０ｄ,合子胚为晚心形,珠心胚巨大量侵入并迅速发育（Ｆｉｇ．１Ｈ）。杂交的组合对合子,胚珠及果实发育均有一定影响,主要取决于杂交亲本。与种间杂交相比,属间杂交其合子分裂较迟,合子胚发育较慢,珠心胚侵入时期也较迟（Ｔａｂｌｅｌ,Ｆｉｇ．２）。这种发育速度的差异,引起所产生的合子胚的大小（Ｔａｂｌｅ２）珠心胚侵率（Ｔａｂ     

HSP_(70)基因表达对高粱育性的影响(英文)

高粱细胞质雄性不育系３１９７Ａ（３Ａ）在常温条件下是不育的（Ｆｉｇｓ．１１＆２）,经热激（４５℃）诱导不同程度地恢复了育性（Ｆｉｇｓ．１３＆４）,为研究其不育机理提供了线索。热激２ｈ后,３Ａ中即可产生一类线粒体热激蛋白（ＨＳＰｓ）。其中,分子量为７０ｋＤ的ＨＳＰ７０含量最高,也最为稳定。不过,３Ａ中ＨＳＰｓ的稳定性弱于保持系３１９７Ｂ（３Ｂ）（Ｆｉｇ．２,Ｐａｎｅｌｓ１～４）。放线菌素Ｄ抑制ＨＳＰｓ的合成,而氯霉素无此作用（Ｆｉｇ．２,Ｐａｎｅｌｓ５＆６）,表明：ＨＳＰｓ是由核基因编码、在细胞质中合成、再跨膜转运到线粒体中的。３Ａ幼穗经热激后,线粒体的总蛋白量猛增了２．７倍（Ｆｉｇ．３）,达到３Ｂ的水平,育性亦变为可育的。Ｆｉｇ．４表明：ＨＳＰ７０反义链ｃＤＮＡ（Ｒ１）能进入到３Ｂ花药细胞中,并与靶ＲＮＡ（ＨＳＣ７０ｍＲＮＡ）结合,而对照、正义链ｃＤＮＡ（Ｄ）链无此反应。由此、再增加一个通用保守序列的反义链ｃＤＮＡ（Ｒ２）、共两个探针（Ｒ１、Ｒ２）,可以检测到：３Ａ在常温下没有能力合成ＨＳＣ７０ｍＲＮＡ（Ｆｉｇ．５）,而在热激条件下,转变为有能力（Ｆｉｇ．６）。启示：３Ａ在热激条件下由不育转变为可育     

鲤稚幼早期发育过程中粘液细胞的发生和变化

利用酸性条件下的阿新蓝染色和过碘酸－雪夫氏试剂反应相接合的方法（AB－PAS染色）,对鲤早期发育过程中粘液细胞的变化作了初步研究。结果表明,鲤的粘中液细胞在受精卵孵化前一天出现,密度随个体的而增大,成分随发育过程的进行而趋于复杂,鲤的粘液细胞可分为四种类型,Ⅰ型和Ⅱ型含单一成分,为幼稚型,Ⅲ型和Ⅳ型含复合成分,为成熟型,鲤粘液细胞在不同组织器官中的分布是不均匀的,其主要分布区是皮肤、口腔、鳃、消化道等部位。     

Ontogeny of IgM-producing cells in the lymphoid organs of rainbow trout, Salmo gairdneri Richardson: an immuno- and enzyme-histochemical study

The ontogenetic development of IgM-containing cells is described as demonstrated by immunoperoxidase staining with a mouse anti-trout IgM monoclonal antibody and the differentiation of enzyme-histochemical markers in the non-lymphoid cells forming the stroma of the thymus, spleen and kidney of the rainbow trout. The first lymphoid cells staining with the monoclonal antibody occurred at day 4-5 after hatching in the renal lympho-haemopoietic tissue. By 1 month after hatching IgM-positive cells also appeared in the spleen and thymus. Enzyme-histochemical demonstration of the alkaline and acid phosphatase and non-specific σ-naphthyl acetate esterase enzymatic activities in the non-lymphoid cells indicated that a certain degree of maturation of the cellular stroma of the developing lymphoid organs of trout was reached before or at the time when IgM-expressing cells could be observed. The relationships of the stromal components of the various lymphoid organs to the development of IgM-positive cells, and the possible role of the renal lympho-haemopoietic tissue as a primary lymphoid organ for B-cell differentiation in the trout are discussed.     

Expression of the polymeric Immunoglobulin Receptor (pIgR) in mucosal tissues of common carp (Cyprinus carpio L.)

The mucosal immune system seems to be an important defence mechanism for fish but the binding of IgM in mucosal organs is poorly described in fish. In this study the gene encoding the polymeric Immunoglobulin Receptor (pIgR) in carp has been isolated and sequenced from a liver cDNA-library and aligned with other species. The pIgR of carp consists of 2 Ig domains, a transmembrane and an intracellular region, together 327 amino acids. In situ hybridisations with sense and anti-sense DIG-labelled pIgR RNA probes were performed on liver, gut and skin of common carp (Cyprinus carpio L.) and in these organs only anti-sense probes were found to hybridise. In liver the majority of hepatocytes was stained around the nucleus. In gut and skin, staining could be detected around the nucleus of the epithelial cells, but in gut also a subpopulation of lymphoid cells was stained in epithelium and lamina propria. The specific in situ hybridisation of the epithelia and hepatocytes coincides with the in situ binding of FITC-labelled carp IgM to the same cells. RT-PCR results indicate the expression of the pIgR gene in all lymphoid organs of carp, but not in muscle. Macrophages/neutrophils enriched by adherence or sorted B cells (MACS) did not show expression of the pIgR gene and are excluded as the pIgR expressing lymphoid cells in the intestine. The relevance of pIgR staining and gene expression in mucosal organs is discussed.     

Short-term storage of ova of common carp and tench in extenders

In a study of the effect of short-term storage on the hatching rate of common carp Cyprinus carpio and tench Tinca tinca ova in vitro in various extenders at 21° C under aerobic conditions, the best extender for 30 min storage for common carp appeared to be Dettlaff 1. This gave the same hatching rate as controls without extender (55% v. 56%). For 60 min storage of ova, the best extenders were Dettlaff 2 (24% hatching rate) and Dettlaff 3 (30%), but hatching was significantly lower than in the control (58%). In carp ovarian artificial fluid (CAF) extender, the hatching rate of common carp ova was also high after 10 min, but decreased to 12% after 30 min. In tench, the hatching rate of ova increased after 10 min storage in Dettlaff 5 extender (44%) compared to the control (41%) without extender. However, it was significantly lower after storage in Dettlaff 1, 2, 3, 4, 5 and CAF extenders for 20, 30 and 60 min, compared to controls. Malformations (10–50%) were observed in the tench second control groups without extender after 10, 20 and 30 min storage of ova.     

Development, during ontogenetic development of gymnotids, of substance p expression in tuberous organs (electroreceptors)]

The evolution of the neuropeptidic expression of Substance P has been investigated with immunohistochemistry in the cutaneous electroreceptors, tuberous organs, during ontogenetic development of Apteronotus leptorhynchus. In the present data, antiSP antiserum has been applied to serial sections of Apteronotus leptorhynchus larvae obtained from several egg layings. Larvae were taken during development from hatching up to one hundred days old. SP immunoreactivity appeared just after hatching, in the epidermal zones which give rise to cutaneous sense organs. Four days after hatching, the tuberous organs are differentiated and immunoreactivity was observed in these organs, in both sensory cells and accessory cells. From day 30 after hatching, there was a regular decrease in the number of tuberous organs showing labelled accessory cells, and one hundred days later only 8% of tuberous organs had immunoreactive accessory cells. The adult accessory cells were no longer labelled with anti-SP antiserum. The results showed that in Apteronotus leptorhynchus, the epidermal structures which give rise to the cutaneous sensory organs were immunoreactive at a very early stage of development; this suggests that SP could have an effect upon their differentiation.     

Histomorphology of the early yolk-sac larvae of the Atlantic halibut (Hippoglossus hippoglossus L.)—an indication of the timing of functionality

Halibut larvae hatch at a very immature stage, and the duration of the yolk-sac period is very long (up to 50 days). This paper describes the histomorphological development of organs of the yolk-sac larvae (6° C) by use of light and electron microscopy. Rudimentary branchial cavities were open from 2 days after hatching. Kidneys seemed functional 16 days after hatching and onwards, and primitive lamellae on the gill arches were beginning to form at this age. Pancreatic zymogen granules were first observed 20daysafter hatching. The liver was segmented into lobes between 20 and 23 days after hatching, and the gall bladder seemed functional from day 23. The hindgut became extensively folded from day 26, and branchial capillaries were first observed at this stage. The larvae were able to catch food particles 24 days after hatching. Judging from ultrastructural observations, it seemed that halibut larvae were able to digest food particles between day 24 and 26 after hatching (around 150 daydegrees and 50% yolk absorption).     

草鱼感染GCRV后血液中淋巴细胞变化及BCL10表达分析

为了研究草鱼BCL10基因在草鱼出血病中的应答机制, 文章克隆了BCL10基因, 并利用生物信息学、荧光定量和血涂片等技术对其进行了分析。生物信息学结果显示, BCL10基因开放阅读框为738 bp, 编码245个氨基酸。实时荧光定量PCR结果显示, 感染病毒后草鱼体内BCL10表达量持续上调, 在肝胰腺和中肾中第4天达到峰值, 第7天表达量开始下调。血涂片显微镜观察发现了血液中淋巴细胞在感染病毒后第1到第4天下降, 第7天时上升。肾脏的组织病理学观察也发现中肾中肾小管上皮细胞第1到第7天逐渐空泡化, 脱落坏死。以上结果表明, BCL10基因参与了草鱼应对草鱼呼肠孤病毒(GCRV)入侵的免疫应答。     

Effects of sodium chloride, formalin and iodine on the hatching success of common carp, Cyprinus carpio, eggs

Saprolegniales are ubiquitous in natural water supplies of fish hatcheries, and often cause serious disease problems. Sodium chloride, formalin and iodine, administered twice a day as a flush at different concentrations, were tested on infected eggs of common carp, Cyprinus carpio, to evaluate their antifungal activity and effect on hatching rates. Sodium chloride at 35 000 mg L^?1 and formalin at 400 mg L^?1 were found to be most effective in controlling Saprolegnia sp., with 85.4 and 91.8% hatching rates, respectively. Iodine increased the hatching rate by 27% at 200 mg L^?1 (P < 0.05). There were infections on eggs exposed to all levels of iodine, but not on eggs treated with sodium chloride and formalin. Sodium chloride and formalin were more effective than iodine in controlling Saprolegnia. Sodium chloride is a safe, efficacious and economical treatment of Saprolegniosis and is therefore recommended for treating common carp eggs.     

用直接注射法生产转基因鱼

本文报道了对鲤鱼、鲫鱼受精卵不加任何去膜处理,用显微操作器把外源基因直接注射到卵核附近,构建转基因鱼的方法。本法操作方便,孵化条件简单,成活率高。斑点杂交和Southern Blot杂交结果表明,外源基因的整合率与其它方法构建的转基因鱼的外源基因的整合率相近。从1988年至今,本组运用这个方法生产转基因鲤鱼、鲫鱼一万余尾。     

Multiple molecular forms of soluble esterases in the digestive system of the developing chicken

Soluble esterases in tissues of endodermic origin and of various developmental ages of Gallus gallus were analysed by polyacrylamide slab gel electrophoresis and characterized as carboxylesterases, acetylesterases and cholinesterases. Esterase bands were observed from day 9 in the liver and from day 6 in stomach, intestine and yolk sac. The electrophoretic profiles became more complex after hatching with concomitant increase in the staining intensity. On isoelectric focusing of liver extracts only a major form with pI 5.4 was observed. An eserine sensitive band designated EL-1 was found to be tissue (liver) and age (upon hatching) specific. EL-1-like isozymes were also observed in other species of the Galliformes order.