体细胞介导制备转基因动物的新途径

体细胞介导制备转基因动物的技术路线是在核移植技术的基础上建立起来的。它的问世不过只有四五年时间 ,但显示了其具有广泛的应用前景。本综述比较了不同制备转基因动物技术的优缺点 ,介绍了体细胞介导制备转基因动物的基本技术路线 ,着重阐述了体细胞转染和整合细胞的克隆 ,以及体细胞介导的转基因技术的局限性和应用前景     

哺乳动物体细胞克隆及在动物转基因中的应用

哺乳动物体细胞克隆及转基因技术,近些年发展迅速。尤其1997年‘多利’羊的诞生,对推动哺乳动物克隆及转基因技术的发展具有里程碑式的意义。本文介绍了哺乳动物体细胞克隆的方法,存在的问题和体细胞克隆的机理研究。对这些方法和研究理论进行了讨论,并探讨如何利用克隆技术进行转基因动物的制备。     

动物基因敲除研究的现状与展望

基因打靶技术是建立在胚胎干细胞和同源重组技术之上,可对基因组进行定位修饰的实验方法,尤其可以在转基因动物的遗传性状修饰中起到巨大的作用。本文简述了转基因、体细胞克隆和基因打靶的研究历史,以及这些技术对转基因动物制备的影响和展望。     

制备动物乳腺生物反应器的问题和对策

动物乳腺是理想的用于生产复杂的生物活性蛋白的生物反应器。目前,显微注射仍然是制备大型转基因动物的主要方法,但外源基因整合效率低下和位置效应还需要解决。要解决这两个问题,人们探索了几种策略。尽管使用转染的体细胞和基因打靶的体细胞作为核移植的供体的动物克隆技术还在改善中,但是这一技术是有应用前景的转基因牲畜的方法。在转基因载体中使用LCR和MAR序列可显著提高表达水平和转基因效率。YAC、BAC作为理想的转基因载体可能因为它们能容纳基因座的所有元件。虽然这些技术和方法还存在不完善之处,但其发展将极大地提高动物乳腺生物反应器的整合率和表达水平。     

体细胞基因打靶-核移植技术研究进展

转基因效率与外源基因表达水平低的现状一直是制约动物生物反应器研究与产业化的主要技术瓶颈。体细胞克隆动物的成功和胚胎干细胞基因打靶技术的逐步完善使得体细胞基因打靶与核移植技术的结合使用成为可能,这就为生产遗传修饰家畜提供了一种新的手段,为动物生物反应器的成功研制提供了新的技术途径。从体细胞基因打靶的载体设计、转染系统的建立、中靶细胞的筛选和鉴定以及培养体细胞寿命等方面阐述了体细胞基因打靶—核移植技术体系的最新研究进展,并对其在异种器官移植、建立动物疾病模型、提高家畜生长性能以及生产药用蛋白等各个领域中的应用前景作了展望 。     

制作转基因动物的显微注射技术

转基因动物(Transgenic animals)是指体细胞和生殖细胞的基因组内,含有用实验方法导入的外源目的基因的动物。转基因动物的获得,大大地丰富了基因工程的研究内容,它为研究高等动物基因表达调控的分子机理提供了有效的途径。由于这种系统不仅可以表达多肽和蛋白质的产物作为医疗药物的生产途径,     

哺乳动物体细胞克隆技术的研究进展

尽管与已有十几年发展史的哺乳动物胚胎细胞克隆技术相比,其体细胞克隆技术的研究仅有不到三年的时间;然而,鉴于哺乳动物体细胞克隆技术在供核效率等方面所具备的明显优势,其应用价值远高于胚胎细胞克隆技术。随着对哺乳动物体细胞克隆技术基本机理的进一步广泛深入的研究,它将在大量克隆优良种畜、扩大同基因型实验动物种群、培育转基因动物和保护濒危野生动物遗传资源等方面发挥巨大作用。     

哺乳动物体细胞克隆技术的研究进展

尽管与已有十几年发展史的哺乳动物胚胎细胞克隆技术相比,其体细胞克隆技术的研究仅有不到三年的时间;然而,鉴于哺乳动物体细胞克隆技术在供核效率等方面所具备的明显优势,其应用价值远高于胚胎细胞克隆技术。随着对哺乳动物体细胞克隆技术基本机理的进一步广泛深入的研究,它将在大量克隆优良种畜、扩大同基因型实验动物种群、培育转基因动物和保护濒危野生动物遗传资源等方面发挥巨大作用。     

体细胞基因打靶制备动物乳腺生物反应器的策略与应用

在转基因动物研究中,由于基因表达调控元件的人工拼接和外源基因在动物基因组中随机整合所带来的“位置效应”,致使转基因动物外源基因的表达水平不高并且差异较大。为此,利用定位整合优势,对以基因同源重组为基础的基因打靶技术进行了大量研究。介绍了就利用体细胞基因打靶和核移植技术制备动物乳腺生物反应器的策略和应用情况做一综述,并对提高基因打靶效率的各种策略,打靶细胞的选择,转基因细胞核移植的低融合事件以及基因打靶制备乳腺生物反应器的优越性进行分析。     

动物乳腺生物反应器的现状和趋势

利用转基因家畜的乳腺生产人类重组蛋白,可以高效获得安全、足量的药用蛋白。本文针对乳腺生物反应器的成功研制,从目的基因的选择、载体构建、转基因技术等方面探讨了动物乳腺生物反应器的研究现状。分析了提高转基因效率和外源蛋白表达水平的技术途径,提出了降低总体成本的战略措施。特别探讨了利用Cre-loxP系统发展“体细胞打靶体细胞核移植技术体系”,高效生产乳腺生物反应器动物的可能性。     

两种不同终止子在转基因鲤鱼中的促生长效应

转基因构建体中启动子的选择会直接影响转植基因的活性, 近年来有研究表明转基因构建体中终止子的选择会一定程度地影响转植基因的活性。为了更好地筛选转基因构建体和培育快速生长的转“全鱼”生长激素(Growth hormone, GH)基因鱼, 文章用鲤鱼β-actin基因终止子和生长激素基因终止子分别构建了转基因构建体, 显微注射得到转“全鱼”GH基因鱼P0代养殖群体, 比较两种不同终止子构建体的活性。统计分析发现, 生长激素基因终止子构建体的养殖群体的体重频率呈正态分布且平均体重显著高于β-actin基因终止子构建体的养殖群体, β-actin基因终止子构建体的养殖群体的体重频率呈右倾趋势的非正态分布。值得一提的是在混合养殖组中得到一条生长最为快速的鲤鱼证实为转基因阳性且为生长激素基因终止子构建体的转基因鲤鱼。该结果表明转“全鱼”生长激素基因鲤鱼可快速生长, 并能将转植基因向下代遗传。实验结果提示生长激素基因终止子构建体比β-actin基因终止子构建体表现的促生长活性要强。     

转CpTI-Bt基因棉和转Bt基因棉对棉铃虫幼虫存活、生长及营养利用的影响

2000年7月中旬和8月中旬, 分别测定了采自田间的转CpTI-Bt基因双价抗虫棉（SGK321, 以下简称CpTI-Bt棉）和转Bt基因抗虫棉（中30,以下简称Bt棉）对棉铃虫Helicoverpa armigera幼虫存活、生长的影响。结果表明：7月中旬两种转基因抗虫棉抗虫效果均较好,尤其是CpTI-Bt棉棉叶和花瓣对4龄幼虫3天内致死率为92%以上;8月中旬两种转基因棉的抗虫活性均明显降低,且Bt棉的杀虫活性显著低于CpTI-Bt棉,其幼虫死亡率与对照受体棉中16的死亡率之间无显著差异,仅显著抑制了幼虫的生长;石远321(SGK321受体品系)的花瓣具有一定的抗虫活性,可显著降低取食幼虫的体重,甚至造成部分幼虫死亡; CpTI-Bt棉中,花瓣和棉叶的抗虫性明显高于蕾和铃心。对5龄幼虫取食棉铃1日后的营养指标测定结果显示： 两种转基因抗虫棉处理的幼虫相对生长率和相对取食量均显著低于石远321,但两者之间无显著差异; CpTI-Bt棉处理的幼虫近似消化率显著低于石远321和Bt棉,但其食物利用率显著高于石远321和Bt棉。     

Age-specific bioassays and fecundity of Phthorimaea operculella (Lepidoptera: Gelechiidae) reared on cry1Ac -transgenic potato plants

Variation in the susceptibility of lepidopterous pest larvae of different ages to transgenic crops and the potential for survivors to reproduce could have important consequences for the development of resistance in such pests. Experiments were undertaken in the laboratory to determine if larvae of the potato tuber moth, Phthorimaea operculella, of different ages (0 (< 1 day old), 3, 5, 7 days) varied in their susceptibility to cry1Ac9–transgenic potato (Solanum tuberosum) foliage grown in the glasshouse or field. The survival and fecundity of larvae reared on transgenic tubers was also determined in the laboratory. There were no apparent differences in susceptibility of larvae of different ages to transgenic foliage. Larvae fed glasshouse or field‐grown non‐transgenic foliage had significantly larger relative growth indices and more larvae pupated, than those fed transgenic foliage, regardless of larval age. Eggs from a laboratory colony were placed on transgenic or non‐transgenic tubers to measure survival and fecundity. Between 6% and 15% of eggs placed on transgenic tubers developed into pupae for three of the four transgenic potato lines tested. On one transgenic line, only six adults emerged from 1300 eggs. In contrast, between 71% and 97% of the eggs placed on non‐transgenic tubers developed into pupae. Male and female pupae from transgenic lines weighed less than those from non‐transgenic lines. The fecundity of females from two of four transgenic lines was lower than from the non‐transgenic parent cultivar. Although larvae of different ages did not exhibit any overall age‐dependent pattern of increasing or decreasing susceptibility to transgenic foliage of glasshouse or field‐grown plants, the ability of larvae to survive and reproduce on transgenic tubers suggests this pest has the ability to evolve resistance to the transgenic plants used in the present study.     

Feeding behaviour of Helicoverpa armigera larvae on insect-resistant transgenic cotton and non-transgenic cotton

Abstract: Feeding behaviour of Helicoverpa armigera Hübner (Lep.; Noctuidae) larvae on non‐transgenic Bacillus thuringiensis (Bt) cotton (Gossypium hirsutum L.), Zhong 30, and transgenic cowpea trypsin inhibitor (CpTI)‐Bt cotton, SGK 321, and non‐transgenic cotton, Shiyuan 321, was investigated in both choice tests and no‐choice tests. The results of choice tests suggested that neonates have the ability to detect and avoid transgenic cotton. In the choice tests of neonates with both transgenic and non‐transgenic cotton leaves, a significantly greater proportion of larvae and higher consumption were observed on non‐transgenic cotton than on the transgenic Bt or CpTI‐Bt cotton. In the choice tests with leaves of two transgenic cotton lines, the proportion of neonates on leaf discs of the two lines was not significantly different, but there was significantly higher consumption on CpTI‐Bt transgenic cotton than that on Bt transgenic cotton. In addition, significantly more neonates were found away from the leaf discs, lower consumption and higher mortality were achieved in the choice test with two transgenic cotton leaves than in the choice tests containing non‐transgenic cotton leaves. Leaves and buds were examined in choice tests of fourth instars. It appeared that fourth instars were found in equal numbers on transgenic and non‐transgenic cotton, except when larvae were exposed to leaves for 3 h. However, the total consumption on transgenic cotton was lower than that of the non‐transgenic cotton, so fourth instars may still have the capacity to detect transgenic cotton and reduce feeding on it, although they showed no preference on either transgenic or non‐transgenic cotton. More larvae were found off diet in the treatments with leaves than that of buds, and the number of injured leaf discs by per fourth instar was significantly higher than that of buds in choice tests, suggesting that leaf is a less preferred organ for H. armigera larvae, elicited more larval movements. Similarly, in no‐choice tests of fifth instars, significantly fewer feeding time and more moving time occurred on leaf than that of bud, boll and petal. When cotton line was considered, compared with non‐transgenic cotton, significantly lower feeding time and higher resting time occurred on the two transgenic cottons. Overall, H. armigera larvae have the ability to detect the transgenic Bt and CpTI‐Bt cottons or the less preferred organs and selectively feed more on the non‐transgenic cotton or the preferred organs, especially the neonates, which have a high capacity for avoiding transgenic cotton.     

转基因植物环境监测进展

近20年来,转基因植物的商业化应用规模越来越大,而转基因生物安全问题依然是转基因植物产业进一步发展的最主要制约因素。转基因植物在商业化应用之前虽然预先进行了风险评估,但是,包括环境监测在内的风险管理措施是确保转基因植物安全应用的必要手段。在转基因作物大规模应用近20年之后,其在靶标生物抗性、对生物多样性的影响、基因漂移、在生态系统中的长期存留等方面产生的环境风险已经渐渐显现出来,表明风险评估无法为转基因植物应用提供足够的安全保障,还必须通过开展系统而长期的环境监测,明确转基因植物在生产应用后的实际环境影响。联合国环境规划署和欧盟等已经制定了转基因植物环境监测的法规和技术指南,一些国家实施了系统的转基因植物环境监测。对转基因植物所产生的环境风险以及环境监测应包括的内容进行了综述。     

A pre-breeding screening program for transgenic boars based on fluorescence in situ hybridization assay

For efficient transgenic herd expansion, only the transgenic animals that possess the ability to transmit transgene into next generation are considered for breeding. However, for transgenic pig, practically lacking a pre-breeding screening program, time, labor and money is always wasted to maintain non-transgenic pigs, low or null transgenic transmission pigs and the related fruitless gestations. Developing a pre-breeding screening program would make the transgenic herd expansion more economical and efficient. In this technical report, we proposed a three-step pre-breeding screening program for transgenic boars simply through combining the fluorescence in situ hybridization (FISH) assay with the common pre-breeding screening workflow. In the first step of screening, combined with general transgenic phenotype analysis, FISH is used to identify transgenic boars. In the second step of screening, combined with conventional semen test, FISH is used to detect transgenic sperm, thus to identify the individuals producing high quality semen and transgenic sperm. In the third step of screening, FISH is used to assess the in vitro fertilization embryos, thus finally to identify the individuals with the ability to produce transgenic embryos. By this three-step screening, the non-transgenic boars and boars with no ability to produce transgenic sperm or transgenic embryos would be eliminated; therefore only those boars could produce transgenic offspring are maintained and used for breeding and herd expansion. It is the first time a systematic pre-breeding screening program is proposed for transgenic pigs. This program might also be applied in other transgenic large animals, and provide an economical and efficient strategy for herd expansion.     

Effects of Transgenic Petunia Expressing Bacillus thuringiensis Toxin on Selected Lepidopteran Pests

Toxicity of 11 transgenic petunia lines expressing the CryIA (c) insecticidal crystal protein of Bacillus thuringiensis subsp . kurstaki was investigated using lepidopteran neonates Spodoptera exigua, Trichoplusia ni and Manduca sexta. Mortality of S. exigua, T. ni and M. sexta varied within and among transgenic petunia lines . Bioassay results demonstrated that levels of CryIA (c) expression obtained in 7 out of the 11 transgenic petunia lines produced at least 50% mortality in S. exigua and T. ni, and all 11 transgenic lines produced more than 80% mortality in M. sexta. Demographic analysis of the biological impact of transgenic petunia on S. exigua revealed that sub - lethal feeding on transgenic petunia significantly reduced larval weight and prolonged larval and pupal development times . Continuous feeding on transgenic petunia significantly reduced lifetime fecundity , egg hatch and longevity in female and male moths . Compared with insects fed continuously on non - transgenic petunia , lifetime fecundity and net reproductive rate were reduced by 58 and 84% in insects fed continuously on transgenic petunia respectively . Mean generation time was 8 days longer for insects fed continuously on transgenic petunia than for insects fed on non - transgenic petunia . Ovipositional attractiveness of transgenic petunia to S. exigua with respect to non - transgenic tomato or lettuce plants was similar , suggesting that petunia / tomato and petunia / lettuce may not be effective trap - cropping combinations . The potential and implications of using transgenic petunia as trap plants interplanted with crop plants for management of lepidopteran pests in the field are discussed .     

转基因动物在生物制药工业中的应用

简要论述了转基因动物的概念、制作方法及应用领域,回顾了转基因动物技术的发展及现状,分析了转基因动物与克隆动物的区别.就转基因动物在制药工业和生物医药领域中的国内外研究与开发应用情况进行了阐述,同时展望了转基因动物制药的发展前景及对社会的影响.     

Selection of in vitro produced, transgenic embryos by nested PCR for efficient production of transgenic goats

The production of valuable pharmaceutical proteins using transgenic animals as bioreactors has become one of the goals of biotechnology. However, the efficiency of producing transgenic animals by means of pronuclear microinjection is low. This may be attributed in part to the low integration rate of foreign DNA. Therefore, a large number of recipients are required to produce transgenic animals. We recently developed a transgenic procedure that combined the techniques of goat oocyte in vitro maturation (IVM), in vitro fertilization (IVF), microinjection, preimplantation selection of the transgenic embryos with nested PCR and transferring the transgenic embryos into the recipient goat uterus to produce transgenic goats. Thirty-seven transgenic embryos determined by nested PCR were transferred to thirty-two recipient goats. In the end, four live-born kids were produced. As predicted, all the live kids were transgenic as identified by PCR as well as Southern blot hybridization, The integration rate was 100% (4/4) which was completely in accordance with the results of embryo preimplantation detection. The results showed a significant decrease in the number of recipients required as only 8 recipients (32/4) were needed to obtain one live transgenic goat. We suggest that the transgenic system described herein may provide an improved way to efficiently produce transgenic goats on a large scale.     

Distinguishing transgenic from non-transgenic Arabidopsis plants by 1H NMR-based metabolic fingerprinting

We have recently reported the construction of an nuclear magnetic resonance （NMR）-based metabonomics study platform, Automics. To examine the application of Automics in transgenic plants, we performed metabolic fingerprinting analysis, i.e., 1H NMR spectroscopy and multivariate analysis, on wild-type and transgenic Arabidopsis. We found that it was possible to distinguish wild-type from four transgenic plants by PLS-DA following application of orthogonal signal correction （OSC）. Scores plot following OSC clearly demonstrates significant variation between the transgenic and non-transgenic groups, suggesting that the metabolic changes among wild-type and transgenic lines are possibly associated with transgenic event, We also found that the major contributing metabolites were some specific amino acids （i.e., threonine and alanine）, which could correspond to the insertion of the selective marker BAR gene in the transgenic plants. Our data suggests that NMR-based metabonomics is an efficient method to distinguish fingerprinting difference between wild-type and transgenic plants, and can potentially be applied in the bio-safety assessment of transgenic plants.