转植酸酶基因家蚕的制作及表达检测

家蚕Bombyx mori丝腺具有高效合成蛋白质的特性,开发在丝腺特异表达外源蛋白质的生物反应器具有重要的意义。本研究利用piggyBac来源的两种载体pPIGA3GFP和pBac{3×P3-EGFPaf},建立了稳定的家蚕转基因技术体系; 然后,利用一株黑曲霉来源的植酸酶基因,构建了在家蚕后部丝腺特异表达的融合表达载体pBac [3×P3-EGFP+ FibLphyADsRed],注射蚕卵后,在53个G1蛾区中检测到3个有荧光蚕的蛾区。经Southern blot和反向PCR验证,转基因表达盒整合到家蚕染色体上。RT-PCR结果显示,植酸酶基因特异性地在后部丝腺表达,其表达模式与家蚕轻链丝素基因一致。结果表明我们成功获得了在后部丝腺特异表达植酸酶融合蛋白的转基因蚕,这为进一步开发家蚕生物反应器,利用转基因蚕生产各种重组蛋白具有积极的促进作用。     

即时浸酸显著提高滞育性家蚕卵辅酶Ⅰ和Ⅱ含量

即时浸酸在阻止家蚕Bombyx mori卵滞育发动的同时, 提高了其呼吸耗氧量, 抑制了山梨醇积累。本研究利用HPLC法测定了家蚕滞育卵和5 min即时浸酸滞育性卵中辅酶Ⅰ和Ⅱ含量。结果表明： 产下后24-72 h, 家蚕滞育卵中NAD, NADH, NADP和NADPH含量分别下降了30%, 37%, 50%和4%; 而即时浸酸滞育性卵中分别增加了77%, 46%, 142%和241%。不过, 即时浸酸并未显著改变滞育性家蚕卵中NADH/NAD和NADPH/NADP比值。据此推测, 即时浸酸提高滞育性家蚕卵辅酶Ⅰ含量与其呼吸耗氧量增加有关; 即时浸酸显著提高辅酶Ⅱ含量与山梨醇积累抑制无关, 而主要与生物合成加强有关。     

琥珀蚕孵化酶基因AaHE的克隆及启动子活性分析

【目的】琥珀蚕Antheraea assama具有典型的野蚕特征,蚕卵孵化不齐,严重影响琥珀蚕的室内规模化饲养。本研究旨在探究对琥珀蚕卵孵化起关键作用的孵化酶(hatching enzyme)基因及其启动子序列特征,为进一步选择合适的抑制剂或促进剂调节琥珀蚕卵的孵化奠定基础。【方法】采用RACE技术克隆琥珀蚕孵化酶基因的cDNA全长序列,对基因序列进行生物信息学分析;采用qRT-PCR检测琥珀蚕孵化酶基因在琥珀蚕不同发育天数卵中及5龄第3和4天幼虫不同组织(丝腺、马氏管、头、中肠、脂肪体、表皮、血液、精巢和卵巢)中的表达情况;采用染色体步移克隆琥珀蚕孵化酶基因的启动子序列,构建昆虫细胞重组表达载体转染家蚕Bombyx mori BmN细胞,检测琥珀蚕孵化酶基因启动子活性。【结果】获得了琥珀蚕孵化酶基因AaHE(GenBank登录号： KT336227.1)全长cDNA序列,长993 bp,编码294个氨基酸,预测蛋白质分子质量为33.7 kD,理论等电点为5.17。AaHE氨基酸序列含有一个信号肽和一个ZnMc结构域,AaHE是一种含有HExxH锌结合位点的锌依赖性蛋白水解酶,该类酶既是肽酶,同时又是一种消化酶。AaHE在琥珀蚕孵化前的卵及5龄幼虫中肠中特异性高表达,分别与AaHE的肽酶和消化酶的属性相吻合。AaHE启动子核心区存在多个转录因子结合位点,这可能与转录因子参与调节AaHE的表达有关。启动子活性分析表明,AaHE启动子在家蚕BmN细胞中能够启动EGFP基因的表达,具有明显的启动子活性。【结论】AaHE是锌依赖性蛋白水解酶,其启动子核心区存在多个转录因子结合位点。本研究为选择合适的抑制剂或促进剂调节琥珀蚕卵的孵化率提供了参考。     

即时浸酸显著降低滞育家蚕卵的还原型与氧化型谷胱甘肽比值

即时浸酸在阻止家蚕Bombyx mori卵滞育发动的同时, 显著提高了家蚕卵H₂O₂含量。还原型谷胱甘肽（reduced glutathione, GSH）与氧化型谷胱甘肽（oxidized glutathione, GSSG）的比值是一种氧化胁迫状态的动态指标。为了调查即时浸酸是否造成滞育家蚕卵氧化胁迫, 本研究利用分光光度法分别测定了滞育家蚕卵和5 min即时浸酸滞育家蚕卵中GSH和GSSG含量以及谷胱甘肽转移酶（glutathione-S-transferase, GST）活性。结果表明: 处理后24 h, 即时浸酸处理家蚕卵的总谷胱甘肽（GSH+2GSSG）含量、 GSH含量、 GSSG含量、 GSH/GSSG比值和GST活性分别相当于同期滞育家蚕卵的204%, 78%, 550%, 14%和97%。据此推测, 即时浸酸在阻止滞育发动的同时, 可能通过促进GSH氧化为GSSG, 而显著降低了GSH/GSSG比值, 使家蚕卵处于过氧化状态。     

一个新的家蚕油蚕白卵系BH863的基因型研究

家蚕卵色正常型为黑褐色,其突变种类丰富,其中白色卵系列不失为一特色。迄今研究报道的家蚕白卵突变基因有１２种之多（向仲怀,１９９４;江口正治等,１９８６;Ｆｕｊｉｉ,１９９８;Ｃｈｉｓｈｕｓｈｉ,１９７２;Ｋｉｎｇ,１９７６）。本研究室发现１９９４年由广东省农科院蚕业所移送西南农业大学家蚕基因库保存和鉴定的ＢＨ８６３系是一种新的油蚕白卵突变。ＢＨ８６３系是以家蚕品种湖２０４（♀）为受体,蓖麻蚕品种斑马（♂）为供体,经人工授精产生的子代中的家蚕变异品系（陈元霖等,１９９３）。其主要性状特征为：浆液膜…     

家蚕β-呋喃果糖苷酶基因BmSuc1的CRISPR敲除载体的构建与导入

【目的】CRISPR/Cas9是近些年报道较多的基因编辑新工具,具有简便高效、特异性强等优势。BmSuc1是从鳞翅目经济昆虫家蚕Bombyx mori体内发现的编码β-呋喃果糖苷酶(β-fructofuranosidase,β-FFase)的基因,也是首个被克隆和鉴定的动物型β-FFase编码基因。β-FFase是作用于果糖基的蔗糖水解酶,BmSUC1可能与家蚕防御桑叶生物碱的生理过程有关,但目前其发挥作用的分子机制尚不清晰。为了解析BmSuc1在蚕体的作用途径及其生理功能,本研究基于CRISPR/Cas9基因编辑系统构建表达双元sgRNA的CRISPR载体,用于敲除家蚕基因组中的BmSuc1基因。【方法】根据目的基因BmSuc1的ORF序列设计2条sgRNA,通过同源重组的方法分别插入CRISPR载体的Sal I和Nhe I酶切位点。进而利用转基因显微注射技术将该编辑载体注入G_0代蚕卵,经催青孵化饲养家蚕并自交制备G_1代蚕种。【结果】PCR验证及测序结果均表明CRISPR编辑载体构建成功。根据Ds Red2红色蛋白的荧光标记,从G_1代家蚕幼虫中成功筛选出阳性转基因个体。【结论】本文详细介绍了表达双元sgRNA的CRISPR载体的构建方法,所获得的阳性转基因家蚕对于下一步探讨BmSuc1在家蚕糖类营养的吸收与利用途径中的作用奠定了重要的实验基础,有助于阐明蚕-桑相互选择和适应的分子机制。     

家蚕转基因载体pBacA3EG的构建及其表达

以家蚕Bombyx mori肌动蛋白A3(actin 3)启动子、增强性绿色荧光蛋白(enhanced green fluorescent protein, EGFP)基因及SV40的多聚腺苷酸识别序列为元件,经多次克隆,将其插入到piggyBac转座载体中。经PCR、酶切鉴定及测序表明各元件已按正确的方式插入到piggyBac载体中。将构建好的piggyBac表达载体显微注射到胚盘形成前期的蚕卵中,在胚胎早期发育的第3天,通过体视荧光显微镜检测到蚕卵内发出较强的绿色荧光。结果表明该载体构建正确且能在蚕卵中进行表达。家蚕转基因载体的体外瞬时表达不但是成功进行家蚕转基因所必需的第一步,而且其自身也可以应用于基因的功能研究,为家蚕后基因组研究奠定了基础。     

高低温催青温度敏感期家蚕卵的差异蛋白筛查

滞育（Diapause）是昆虫发育停滞或减缓的生理状态,家蚕Bombyx mori作为卵滞育的代表,其滞育过程已得到广泛研究,但诱导滞育发生的分子机制尚不清楚。二化性家蚕滞育性由遗传和母系在胚胎期所处的环境条件决定,25℃催青蚕卵孵化后的家蚕产滞育卵,15℃低温催青则诱导家蚕产下非滞育卵。本研究分别用25℃和15℃催青蚕卵,在发生滞育诱导的温度敏感期取样,抽提蛋白质通过非标（Label-free）蛋白质组定量技术进行质谱测序。筛选出具有明显表达差异的蛋白104个,其中56个蛋白上调,48个蛋白下调。通过生物信息学对差异蛋白进行GO分类和KEGG功能富集分析,结果显示差异蛋白主要参与生长发育、物质代谢和胁迫应答等生物过程;同时差异蛋白主要参与胰岛素信号通路、乙醛酸和二羧酸代谢等相关途径。分别选取上调基因和下调基因进行qRT-PCR验证,其趋势与蛋白组学结果一致。该研究将为进一步解析家蚕滞育诱导发生机制提供靶标蛋白和数据参考。     

非转座子载体介导的转基因家蚕表达hIL-28A

为了探讨非转座子载体介导转基因家蚕表达外源基因的可能性,将hIL-28A克隆进昆虫细胞表达载体pIZT/V5-His,构建了重组载体pIZT/V5-His-hIL-28A.利用精子介导法将该重组载体导入家蚕卵,通过绿色荧光筛选并结合PCR、DNA杂交等分子鉴定,证实成功获得了转基因家蚕.Western blotting结果显示,转基因家蚕表达重组hIL-28A的分子质量为25 ku,ELISA检测结果显示,hIL-28A在G3代转基因蚕、后部丝腺、脂肪组织冻干粉中的含量分别为0.198、0.320和0.238 ng/g.表明通过非转座子载体介导可以将外源基因导入家蚕基因组并实现外源基因的表达.     

家蚕转基因技术中若干因素对转基因效率的影响

建立高效、稳定的家蚕Bombyx mori转基因技术对于推进家蚕功能基因组研究, 解决蚕丝产业重大问题以及向非绢丝产业拓展等具有重要意义。本文在已建立的基于piggyBac的家蚕转基因技术基础上, 探索了多个影响转基因效率的因素。结果显示：以家蚕品种大造 (P50) 为供试材料、pBac［GOI］为供体质粒、pHA4PIG为辅助质粒, 以眼睛和神经组织特异启动子3×p3启动的红色荧光蛋白基因DsRed为报告基因, 在蚕卵产下后2～3 h进行注射,综合效果最佳, 孵化率和转化率分别达到62.7%和34.8%;荧光筛选的最佳时期在胚胎发育第5到第8天;在2 000～8 000 bp之间时, 外源片段的长度对转化率并无太大影响。本研究建立的技术体系, 有望为家蚕功能基因研究、品种分子改良和家蚕生物反应器的开发奠定基础, 并为其他鳞翅目昆虫转基因技术的建立提供参考。     

Strain-Dependent Differences in the Efficiency of Transgenic Mouse Production

Transgenic mouse production via pronuclear microinjection is a complex process consisting of a number of sequential steps. Many different factors contribute to the effectiveness of each step and thus influence the overall efficiency of transgenic mouse production. The response of egg donor females to superovulation, the fertilization rate, egg survival after injection, ability of manipulated embryos to implant and develop to term, and concentration and purity of the injected DNA all contribute to transgenic production efficiency. We evaluated and compared the efficiency of transgenic mouse production using four different egg donor mouse strains: B6D2/F1 hybrids, Swiss Webster (SW) outbred, and inbred FVB/N and C57BL/6. The data included experiments involving 350 DNA transgene constructs performed by a high capacity core transgenic mouse facility. Significant influences of particular genetic backgrounds on the efficiency of different steps of the production process were found. Except for egg production, FVB/N mice consistently produced the highest efficiency of transgenic mouse production at each step of the process. B6D2/F2 hybrid eggs are also quite efficient, but lyze more frequently than FVB/N eggs after DNA microinjection. SW eggs on the other hand block at the 1-cell stage more often than eggs from the other strains. Finally, using C57BL/6 eggs the main limiting factor is that the fetuses derived from injected eggs do not develop to term as often as the other strains. Based on our studies, the procedure for transgenic mouse production can be modified for each egg donor strain in order to overcome any deficiencies, and thus to increase the overall efficiency of transgenic mouse production.     

Efficient strategies for changing the diapause character of silkworm eggs and for the germline transformation of diapause silkworm strains

Abstract To overcome the disadvantages of current silkworm Bombyx mori transgenic technology, such as costly and time‐consuming to maintain non‐diapause transgenic silkworms, we report here on the development of treatments for the germline transformation of diapause silkworm strains. Our results showed that HCl treatment within 3 h of oviposition was able to prevent the diapause of eggs from Japanese lineage diapause silkworm strains and was also suitable for germline transformation of the same strains. By incubating developing mother eggs from Chinese lineage diapause silkworm strains at 15°C (15°C‐IME), we were able to prevent the diapause of their daughter eggs; a similar strategy (15°C‐IMES) for the germline transformation of the same strains was that the mother eggs were incubated at 15°C, and the daughter eggs were then microinjected according to the conventional microinjection methods used for non‐diapause eggs. By combining temperature and light controls, the improved 15°C‐IMES strategy prevented diapause in daughter eggs, and also enabled the germline transformation of both Japanese and Chinese lineage diapause silkworm strains. Although each of the strategies developed here has advantages and disadvantages, we suggest that the 15°C‐IMES strategy is a good reference for the establishment of germline transformation technologies of other egg diapause insects. These new strategies for the efficient germline transformation of diapause silkworm strains are likely to improve the practical use of silkworm transgenic lines in sericulture and also highlight silkworm functional genomics research and its modeling.     

Production of hyperdorsal larvae by exposing uncleaved Xenopus eggs to a centrifugal force directed from the animal pole to the vegetal pole

Exposure of uncleaved Xenopus eggs to a centrifugal force directed from the animal pole to the vegetal pole produces larvae with enhanced dorsal structures, which resemble 'hyperdorso-anterior' larvae produced by D₂O-treatment at 0.3 normalized time (NT). Optimal conditions are 70 g for 6 min at 20% of the first cell cycle (0.2 NT). Exposure before removal of vegetal pole cortical cytoplasm, which we find has an effect of eliminating dorsal structures, protects eggs from losing their ability to form dorsal axial structures upon removal. In contrast, exposure after a slight ultraviolet (UV)-irradiation, which has virtually no effect on dorsal development, produces larvae with heavily reduced dorsal structures, which resemble 'ventralized' larvae produced by heavy UV-irradiation. Interestingly, none of these treatments prevents cortical rotation. Morphological and histological examinations reveal that exposure to the force causes displacement of both cortical and deep egg components from around the vegetal pole to subequatorial regions. We conclude that exposure to the centrifugal force enhances dorsal structures by displacing dorsal determinants from around the vegetal pole to subequatorial regions broader than normal. This is the first experiment in which displacement of egg components, by methods independent of the rotation, are shown to perturb larval body pattern.     

Rapid and improved method for windowing eggs accessing the stage X chicken embryo

The chick stage X blastoderm is routinely accessed through a small window in a freshly laid egg. However, windowing severely compromises embryo survival with hatch rates as low as a few percent. We previously reported a simple modification to the standard method that reduced introduction of air into the sealed egg and improved the hatchability to 32%. Here, we describe an even simpler and more rapid method for sealing a windowed egg using hot glue or paraffin in which the hatch rate increased to an average of 63% of the unwindowed control eggs. The primary reason for low hatchability can be attributed to air trapped within the egg during windowing and/or leakage during incubation, as shown by increased lethality by artificially introducing air into windowed and sealed eggs. Although the hatch rate was considerably improved, air can still enter the egg during incubation and is likely to account for less than 100% hatchability of the sealed eggs. The success of this new windowing method will facilitate high throughput for the production of transgenic birds and find use in developmental biology, toxicity testing, and avian disease research.     

Cytoplasmic Ca2+ release induced by microinjection of Ca2+ and effects of microinjected divalent cations on Ca2+ sequestration and exocytosis of cortical alveoli in the medaka egg

Intracellular release of Ca2+ by microinjection of Ca2+ was analyzed by measuring the luminescence of aequorin loaded in eggs of the medaka (Oryzias latipes). Microinjection of Ca2+ into the cortical cytoplasm induced propagative waves of cytoplasmic Ca2+ release and exocytosis of cortical alveoli initiated at the injection point. The Ca2+ wave was initiated with a time lag after some was sequestered at the region of the microinjection. Microinjection of Mg2+ or Mn2+ failed to trigger Ca2+ release and exocytosis. When the aequorin-loaded eggs were inseminated after microinjection of Mg2+, Mn2+, or Co2+ into a restricted region of the vegetal hemisphere, the wave of Ca release was propagated through the injected region toward the vegetal pole, but neither Ca sequestration (fall in Ca-aequorin luminescence) nor exocytosis occurred at the area of cortex where the eggs were injected with these divalent cations. These results suggest that a significant period is required to induce Ca2+ release from cytoplasmic stores by the increased Ca2+ concentration and that both the phenomena of Ca2+ release and Ca sequestration are involved in the process of exocytosis.     

温湿度对稻纵卷叶螟卵的联合作用

为了探讨温湿度在稻纵卷叶螟Cnaphalocrocis medinalis （Guenée）种群发展中的作用, 通过室内实验调查了不同温度和湿度组合下该蛾卵的发育历期、 胚胎发育情况、 孵化率和卵粒重量的变化。结果表明： 在相同温度下卵历期随相对湿度的增大而缩短, 孵化率随相对湿度的加大而提高。在22℃下低于46%的相对湿度显著降低了卵的孵化率, 而在25～34℃下低于66%的相对湿度会引起孵化率的显著降低, 37℃下卵无论在何种湿度中均不能孵化。在50%左右的低湿条件下, 温度高于28℃后卵也不能孵化。温度在22～31℃和相对湿度在77%～100%范围内, 卵的孵化率无显著差异, 这属于稻纵卷叶螟卵的适宜温湿度范围。稻纵卷叶螟卵的发育起点温度和有效积温分别为10.1±0.6℃和63.7±3.5日度。卵的孵化率（Y）与温湿系数（RH/T）间呈显著的逻辑斯蒂曲线关系Y=0.8662/[1+exp(17.4084-7.5714×RH/T)]。温湿系数在2.34以下时卵孵化率将低于50%, 而达到3.0左右时孵化率接近最高值。结论认为, 低湿造成的稻纵卷叶螟卵重量显著降低、 卵粒干瘪、 胚胎发育受阻是致死卵的主要原因。     

Fertility and hatchability of eggs laid in the pullet-to-breeder transition period and in the initial production period

The initial eggs produced by broiler breeder hens are relatively small compared with later in the production cycle. An evaluation of indices related to hatchability is required when these eggs are to be used for the production of broiler chicks. Two experiments were conducted to evaluate characteristics related to the hatchability of eggs from pullet-to-breeder transition phase, at 25 and 27 weeks of age, and from the peak of production period and five weeks later, at 32 and 37 weeks of age. Eggs from birds 25 weeks had a lesser fertility in Experiment 1. Mortality occurred unevenly in early (1–5 days), middle (6–17 days) and late (18–21 days) incubation, and greater mortality was observed after the internal membrane was ruptured. The younger the hen, the lighter the egg, chick, and shell, and the longer the time required to complete the hatching process. In Experiment 2, greater mortalities were observed at the early period (1–5 days) and after “pipping” of the internal and external membranes. Embryos from heavy eggs of breeder hens 37 weeks of age took less time to complete the hatching process. Results indicated the larger the egg, the heavier the chick and shell, and the lesser the shell percentage. As breeder age advanced, characteristics related to egg fertility and hatchability improved.     

Changes in vitellin and other yolk proteins during embryonic development in the silkworm, Bombyx mori

Changes in the amounts of vitellin and other yolk proteins of the eggs of the silkworm, Bombyx mori were investigated during embryonic development using polyacrylamide gel electrophoresis and immunotitration techniques. In the newly laid eggs, soluble proteins were separated into at least nine bands after electrophoresis. The major band was identified as vitellin, accounting for about 40% of the total proteins. The four predominant bands including vitellin exhibited the same mobility as the proteins of haemolymph, but one other major band was specific to the eggs, accounting for about 20% of the proteins.During embryonic differentiation 6–7 days after oviposition, the total protein content did not decrease and the banding patterns and their relative concentrations remained unchanged as a whole. However the concentration of the egg specific protein steadily decreased. During subsequent larval differentiation until hatching, the total proteins were utilized to about 50% of the initial levels: the rapid degradation was observed in almost every species of proteins.An immunotitration experiment further demonstrated that vitellin was not utlilized during embryonic differentiation but was consumed markedly during larval differentiation. However, about 30% of initial level was reserved in the newly hatched larvae. Such a prolonged persistence of vitellin is discussed in relation to protein metabolism during embryonic development in silkworms.     

Egg size and composition in an ageing capital breeder – consequences for offspring performance

1. Egg size is often used as a proxy of egg quality although size and composition may vary, e.g. in insects egg size usually decreases as female ages. Whether this decrease in size reflects reduced concentrations of essential nutrients such as lipids and proteins of eggs laid by ageing females, or does reduced size per se explain often observed lower fitness of later laid eggs is poorly explored. 2. Egg properties were compared with fitness parameters of offspring laid on the first and fourth night during the oviposition period of a capital breeding moth, Cleorodes lichenaria (Hufnagel). The study aim was to explore whether decreased egg size is caused by decreased provisioning into later laid eggs measured as egg protein and lipid concentration, and whether it results in lower fitness of later laid offspring. 3. The fresh and dry weight of eggs decreased over the oviposition period, but the protein and lipid concentration remained constant. Survival of larvae was lower among the fourth night laid offspring on a low quality host Parmelia sulcata Taylor compared to a high quality host Ramalina fraxinea (L.) Ach. No differences were observed in egg fertility or hatchability, neonate survival without food and pupal mass between the offspring produced on different nights. 4. Decreased survival of offspring produced later was rather attributable to absolute provisioning (i.e. lower weight of eggs) than relative provisioning (i.e. decreased concentrations of nutrients in eggs). It is argued that lower survival of later laid smaller eggs on low quality diet is likely attributable to physical and chemical characteristics of host lichens and/or physical properties of tiny neonate larvae.