加工产品中转基因玉米Bt11成分实时荧光PCR定量(性)检测

实验在玉米自身基因和外源基因的边界序列之间设计了具有品种和品系特异性的引物和探针 ,并以实时荧光PCR技术 ,建立了加工产品中转基因玉米Bt1 1成分品系鉴定检测和定量检测的方法。实验对加热条件和时间对检测转基因成分的影响作了探讨 ,并检测了部分市售食品和饲料。检测结果发现 ,加热时间温度越高、时间越长 ,对转基因成分定量检测的影响越大 ;在所检测的样品中可以检测出转基因玉米Bt1 1成分 ,有些样品还同时检出其他转基因成分。本研究实验建立的方法 ,可以用于加工产品中转基因成分的定量检测 ,也可以用于定性检测 ,或作为常规PCR定性检测后的确证实验方法。     

转基因水稻“科丰6号”实时荧光PCR定性定量检测方法研究

旨在建立转基因水稻"科丰6号"外源基因和边界序列的实时荧光PCR检测方法,为科丰6号定性定量检测提供技术支持。根据外源基因和边界序列信息,设计实时荧光PCR探针引物,优化体系,对不同转基因产品和不同转基因含量的"科丰6号"水稻进行检测。结果显示,所设计的引物探针具有很好的特异性,与其他转基因水稻品系、转基因玉米、转基因棉花、转基因番茄和非转基因水稻均无非特异性反应,对转基因水稻"科丰6号"的检测灵敏度达到0.01%。建立的科丰6号实时荧光PCR检测方法重复性好、灵敏度高,能够达到目前国际上转基因产品定量检测的标准,为该水稻品系的定性定量检测提供技术支持。     

应用实时荧光PCR技术定性定量检测改良品质的转基因小麦

目的:对转入高分子量谷蛋白亚基的小麦中转基因成分进行实时荧光PCR定性定量检测。方法:针对转基因小麦品系中通用的ubiquitin启动子,NOS终止子以及标记基因bar基因进行定性筛选检测,同时用已知为单拷贝的Wx012基因作为小麦物种内源特异参照基因,用单粒B73转基因小麦提取基因组DNA建立内源基因和外源基因的标准曲线,对转基因小麦样品A进行定量检测,同时优化实时荧光PCR条件反应条件。定量检测结果为5.35%。结果:研究的实时荧光PCR技术对转基因小麦中转基因成分能够快速准确地进行定性定量检测。     

研发动态

<正>农业部发布16项转基因检测标准农业部近日发布公告,根据《中华人民共和国农业转基因生物安全管理条例》规定,经专家审定通过了转基因动物及其产品成分检测、转基因植物及其产品成分检测的16项标准,并批准发布为中华人民共和国国家标准,自2014年8月1日起实施。具体包括:转基因动物及其产品成分检测:猪内标准基因定性PCR方法、羊内标准基因定性PCR方法;转基因植物及其     

转基因大豆、玉米、油菜和水稻品系特异性检测质粒标准分子的快速构建及应用

本文采用重叠延伸PCR技术快速构建了转基因大豆GTS40-3-2、玉米NK603、油菜RT73和水稻TT51-1的4种品系作物的质粒标准分子.经快速PCR鉴定及测序分析验证后,将构建的阳性质粒标准分子应用于实时荧光定量PCR标准曲线的构建,并建立其相应的荧光定量PCR检测体系,同时对该体系的扩增效率、精确度、灵敏度等指标进行了评估. 结果显示,建立的实时荧光定量PCR检测体系中,目标序列的扩增效率均在97.434%~101.479%正常范围内（R2≥0.995）,定量极限为20 copies,表明我们已成功构建了这4种转基因作物的品系质粒标准分子,并能有效应用于实时荧光定量PCR标准曲线的构建.     

适于转基因油菜RT73品系特异性检测的标准分子构建及其适用性鉴定

针对目前转基因产品检测标准物质缺乏的难题,构建适于转基因油菜RT73品系特异性检测的标准分子pEASY-RT73.其包含转基因油菜RT73品系3'端侧翼序列,油菜内标准基因HMG和PEP片段.对其在定性和定量检测中的适用性进行了实验室内部验证,结果表明,标准分子pEASY-RT173高度特异于转基因油菜RT73品系.以标准分子为标准品的普通PCR扩增中,3个目标片段的检测下限(LOD)均为10拷贝.实时荧光PCR检测的LOD均为25拷贝,定量下限(LOQ)均为50拷贝.以标准分子为标准品构建的标准曲线反应效率介于0.96-1.02间,相关系数均大于0.999.分别以PEP和HMG为内标准基因对5个盲样的测试结果显示,测量值与设定值间偏差(Bias)介于-14.13%-14.29%间,SD小于0.20,RSD小于18.0%.因此,标准分子pEASY-RT73可很好地替代植物来源阳性标准品用于转基因油菜Rt73及其来源产品品系特异性检测.     

转基因植物的应用研究及基因产品的安全性

报道了水稻、油菜、棉花、番茄、马铃薯等植物通过基因工程的方法,在作物品质改良、抗病虫、抗除草剂、杂种优势利用等方面的研究进展,并对转基因产品的安全性进行了阐述。     

5种转基因油菜转化体特异性多重PCR检测方法

【目的】全球转基因植物及其产品的数量和种类越来越多,迫切需要可同时精准高效检测多个转化载体的检测方法。【方法】针对RF1、MS8、Topas19/2、Oxy235和RF3等5个转基因油菜品系的侧翼序列及油菜内源基因cruciferin A(Cru A)序列设计多重聚合酶链式反应特异性引物,通过对转基因油菜、转基因大豆、转基因玉米、转基因水稻、转基因棉花等不同作物进行PCR扩增来测试所选择的引物特异性,优化多重PCR反应引物的浓度,用所建立的检测体系对不同混合比例的转基因油菜进行多重PCR扩增来测试所建立的检测方法的灵敏度。【结果】通过测试,仅在含有目标样品中检测出阳性结果,灵敏度达0.05%,表明所建立的6重PCR检测方法可同时精准检测RF1、MS8、Topas19/2、Oxy235和RF3等5种转基因油菜转化载体。【结论】所建立的6重转基因油菜转化体特异性PCR检测方法通量高、特异性好、灵敏度高,符合有关转基因产品检测的要求,可作为转基因油菜检测的有效方法。     

转基因植物与近缘种之间基因流的研究进展

随着转基因植物的大面积种植,转基因植物的生态风险受到广泛关注,其中主要的风险是转基因植物与近缘物种之间的基因流及其影响。本文综述了目前商业化种植的转基因作物油菜、棉花、玉米和大豆,以及未商业化种植的水稻、小麦的基因流研究进展;分析了不同转基因作物与其近缘种之间发生基因流的频率和最远发生距离;介绍了降低基因流发生的方法。基因流频率受物种亲缘关系、花期重叠时间、风速风向等因素的影响,最远发生距离受气候条件、传粉媒介、地理条件等因素的影响。转基因作物与其近缘种之间的基因流频率与距花粉源的距离呈负相关关系(y=-0.59x-0.46,R²=0.25,P<0.01),亲缘关系近的基因流频率高。为了降低转基因植物与其近缘物种之间的基因流风险,建议采取“分区管理”的策略,并加强基因流发生之后的生态风险评价研究。     

基于焦磷酸测序技术建立基因编辑水稻检测方法

基因编辑技术发展迅速,但对应的检测方法较少。为寻找创建基因编辑作物适用的检测方法,以 PL3 基因编辑水稻编辑位点为靶标,有效设计了焦磷酸测序的扩增引物及测序引物,并进行有效性检测,分别利用Sequence to Analyze等程序以及SNP和AQ两种模式完成了对PL3 基因的定性和定量检测试验,建立了 PL3 基因编辑水稻编辑位点焦磷酸测序检测方法。结果表明,基于焦磷酸测序技术可以通过检测编辑位点从而将基因编辑型水稻与野生型水稻进行区分。与常规的转基因检测方法相比,该检测方法具有较好的准确性、高效性及高灵敏度等优点,在基因编辑型水稻编辑位点定性和定量检测分析方面具有很好的应用前景。     

核酸层析法转基因快速检测体系的建立及应用

随着我国转基因研究及产业化进程提速,转基因检测的重要性日益凸显,因而快速、高效的分子检测新方法的研发具有重要的生产实践及科研意义。在转基因检测中,常规PCR技术具有检测范围广的特点,但较为费时费力,且对实验条件要求较高;而胶体金蛋白试纸法检测方便、快捷,但可检范围窄。基于此,建立了一套基于核酸层析法快速转基因检测的方法体系。将经液氨研磨后的样品通过一管法提取DNA后直接进行PCR扩增,再将PCR扩增产物滴加到胶体金检测卡上,通过直接观察胶体金卡条显色状况进行结果判别。此方法最终检验出玉米内参基因ZSSⅡB及Zein、大豆内参基因SPS、水稻内参基因Lectin,转基因元件启动子CaMV35S及终止子NOS,以及抗虫基因Cry1Ab/1Ac、抗除草剂基因Bar、Pat、CP4-EPSPS及选择标记基因NPTⅡ、Pmi等外源基因;并成功检出特异性转基因事件Mir604及Bt11。研究获得的核酸层析检测方法具有灵敏度高、省时省力且对检测条件要求低等优点,集PCR法与蛋白试纸检测法二者优势于一身,可广泛应用于转基因产品的精确快速检测,为我国转基因生物安全监管提供了良好的技术支撑。     

Identification of genetically modified vegetable sources in food and feed using hydrogel oligonucleotide microchip

A method of multiplex polymerase chain reaction (PCR) followed by the hybridization on a hydrogel oligonucleotide biochip was developed for simultaneous identification of ten different transgenic elements of plant DNA in feed and food products. The biochip contained 22 immobilized probes intended for (i) detection of plant DNA; (ii) plant species determination (soybean, maize, potato, rice); (iii) identification of transgenic elements, including 35S CaMV, 35S FMV, rice actine gene promoters, nos, 35S CaMV, ocs, pea rbcS1 gene terminators, and bar, gus, nptII marker genes. The limit of detection was 0.5% of genetically modified (GM) soybean and maize in analyzed samples. Identification of transgenic DNA in food and feed products using either the developed approach or real-time PCR led to virtually identical results. The assay can be used for selection of GM samples by screening food and feed products for subsequent quantitative determination of the GM component based on the identified transgene.     

Identification of plant-derived genetically modified organisms in food and feed using a hydrogel oligonucleotide microchip

A method of multiplex polymerase chain reaction (PCR) followed by hybridization on a hydrogel oligonucleotide biochip was developed for simultaneous identification of ten different transgenic elements of plant DNA in food and feed products. The biochip contained 22 immobilized oligonucleotide probes that were intended for (1) detection of plant DNA, (2) determination of plant species (soybean, maize, potato, and rice), and (3) identification of transgenic elements, including sequences of 35S CaMV, 35S FMV, rice actin gene promoters, nos, 35S CaMV, ocs, pea rbcS1 gene terminators, and bar, gus, and nptII marker genes. The limit of detection was 0.5% for genetically modified (GM) soybean and maize in the analyzed samples. The tests on food and feed products using the developed approach and real-time PCR showed full agreement in determination of transgenic DNA in the samples. The proposed assay can be used for selection of GM samples by screening food and feed products for subsequent quantitative determination of GM component based on the identified transgene.     

Cry1Ah蛋白标准物质候选物的制备与纯化（英文）

随着转基因技术的迅猛发展,转基因产品的安全性受到了广泛关注。转基因检测用有证标准物质在确保转基因产品定性、定量检测结果的可比性和可追溯性方面发挥着重要作用。但转基因蛋白质标准物质的开发相对缓慢,其中一个难点是制备高纯度的转基因蛋白质候选物。苏云金芽胞杆菌Bacillus thuringiensis cry1Ah1基因因其对亚洲玉米螟等鳞翅目害虫有很好的杀虫活性,已用于转基因抗虫作物的研制,并获得具有较好抗虫性状的转基因株系。为了研发Cry1Ah蛋白有证标准物质,亟需建立其制备及纯化体系。文中优化了利用Bt表达系统制备Cry1Ah蛋白的体系,利用离子交换色谱法和排阻色谱法逐级纯化的方法,获得了高纯度的Cry1Ah蛋白(排阻色谱纯度:99.6%)。生物活性测定结果表明,纯化的Cry1Ah蛋白与原毒素对小菜蛾Plutella xylostella的杀虫活性没有显著差异。最后使用Edman降解法和质谱法确定了Cry1Ah蛋白活化后的氨基酸序列。综上所述,获得的Cry1Ah纯蛋白可用于蛋白质标准物质的研制。     

Cry1Ah蛋白标准物质候选物的制备与纯化

随着转基因技术的迅猛发展,转基因产品的安全性受到了广泛关注。转基因检测用有证标准物质在确保转基因产品定性、定量检测结果的可比性和可追溯性方面发挥着重要作用。但转基因蛋白质标准物质的开发相对缓慢,其中一个难点是制备高纯度的转基因蛋白质候选物。苏云金芽胞杆菌Bacillus thuringiensis cry1Ah1基因因其对亚洲玉米螟等鳞翅目害虫有很好的杀虫活性,已用于转基因抗虫作物的研制,并获得具有较好抗虫性状的转基因株系。为了研发Cry1Ah蛋白有证标准物质,亟需建立其制备及纯化体系。文中优化了利用Bt表达系统制备Cry1Ah蛋白的体系,利用离子交换色谱法和排阻色谱法逐级纯化的方法,获得了高纯度的Cry1Ah蛋白 (排阻色谱纯度：99.6%)。生物活性测定结果表明,纯化的Cry1Ah蛋白与原毒素对小菜蛾Plutella xylostella的杀虫活性没有显著差异。最后使用Edman降解法和质谱法确定了Cry1Ah蛋白活化后的氨基酸序列。综上所述,获得的Cry1Ah纯蛋白可用于蛋白质标准物质的研制。     

双重数字PCR在转基因大豆检测中的应用

利用微滴式数字PCR(droplet digital PCR, ddPCR)平台建立针对MON87705、MON87769、DP356043三种转基因大豆中外源基因的双重PCR检测方法。利用双重数字PCR方法检测特异性、定量范围等参数,优化所用引物探针组合及实验体系程序,检测外源基因与内标准基因的拷贝数。结果表明,所用引物探针组合在数字PCR方法中仅对目标大豆品系有荧光信号,具有特异性,可用于转基因大豆品系的筛选与鉴别。检测了大豆的转基因成分含量,结果与材料标准品参数基本一致,并根据结果设定定量检测限为0.5%,定性检测限为0.05%,可满足低纯度样品检测的需求。双重数字PCR体系能够准确且稳定的满足实际检测需要,在实际应用上具有良好的发展前景。     

转基因玉米双抗12-5转化体特异性PCR方法验证结果分析

抗虫和耐除草剂玉米双抗12-5是我国自主研发的转基因品种,该品种于2020年1月21日获得农业转基因生物安全证书,具有广阔的应用前景。转化体特异性PCR方法是进行转基因生物安全监管的最有效的技术手段之一,可以对转基因产品进行身份鉴定。本研究组织8家实验室对研发单位提供的的双抗12-5转化体特异性定性、定量PCR方法进行了验证,验证结果显示定性与定量PCR检测方法均具有稳定性好、特异性强和灵敏度高的特点,定量PCR方法能精确地定量检测质量分数为5%和0.5%的双抗12-5样品,并且具有良好的重复性和再现性,符合相关标准的要求。本研究有助于后续标准方法的建立和完善,为我国转基因生物安全监管提供技术支撑和决策依据。     

Estimating the copy number of transgenes in transformed rice by real-time quantitative PCR

In transgenic plants, transgene copy number can greatly influence the expression level and genetic stability of the target gene, making estimation of transgene copy number an important area of genetically modified (GM) crop research. Transgene copy numbers are currently estimated by Southern analysis, which is laborious and time-consuming, requires relatively large amounts of plant materials and may involve hazardous radioisotopes. We report here the development of a sensitive, high-throughput real-time (RT)-PCR technique for estimating transgene copy number in GM rice. This system uses TaqMan quantitative RT-PCR and comparison to a novel rice endogenous reference gene coding for sucrose phosphate synthase (SPS) to determine the copy numbers of the exogenous beta-glucuronidase (GUS) and hygromycin phosphotransferase (HPT) genes in transgenic rice. The copy numbers of the GUS and HPT in primary rice transformants (T0) were calculated by comparing quantitative PCR results of the GUS and HPT genes with those of the internal standard, SPS. With optimized PCR conditions, we achieved significantly accurate estimates of one, two, three and four transgene copies in the T0 transformants. Furthermore, our copy number estimations of both the GUS reporter gene and the HPT selective marker gene showed that rearrangements of the T-DNA occurred more frequently than is generally believed in transgenic rice.     

Presence of potential allergy-related linear epitopes in novel proteins from conventional crops and the implication for the safety assessment of these crops with respect to the current testing of genetically modified crops

Mitochondria of cytoplasmic male sterile crop plants contain novel, chimeric open reading frames. In addition, a number of crops carry endogenous double-stranded ribonucleic acid (dsRNA). In this study, the novel proteins encoded by these genetic components were screened for the presence of potential binding sites (epitopes) of allergy-associated IgE antibodies, as was previously done with transgenic proteins from genetically modified crops. The procedure entails the identification of stretches of at least six contiguous amino acids that are shared by novel proteins and known allergenic proteins. These stretches are further checked for potential linear IgE-binding epitopes. Of the 16 novel protein sequences screened in this study, nine contained stretches of six or seven amino acids that were also present in allergenic proteins. Four cases of similarity are of special interest, given the predicted antigenicity of the identical stretch within the allergenic and novel protein, the IgE-binding by a peptide containing an identical stretch reported in literature, or the multiple incidence of identical stretches of the same allergen within a novel protein. These selected stretches are present in novel proteins derived from oilseed rape and radish (ORF138), rice (dsRNA), and fava bean (dsRNA), and warrant further clinical testing. The frequency of positive outcomes and the sizes of the identical stretches were comparable to those previously found for transgenic proteins in genetically modified crops. It is discussed whether novel proteins from conventional crops should be subject to an assessment of potential allergenicity, a procedure which is currently mandatory for transgenic proteins from genetically modified crops.     

Multiplex event-specific qualitative polymerase chain reaction for detecting three transgenic rice lines and application of a standard plasmid as a quantitative reference molecule

The three most well-known genetically modified (GM) rice lines in China are TT51-1, KMD1, and KF6. The purposes of this study were to establish a multiplex event-specific qualitative polymerase chain reaction (meqPCR) system for simultaneous detection of the three transgenic rice events and to construct a plasmid as the reference molecule for quantitative analysis. Event-specific primers for each event were selected or designed by focusing on the transgene borders between the inserted DNA and the flanking rice DNA. The developed meqPCR was anticipated to detect distinct amplicons as 454, 398, 301, and 250 bp from KF6, KMD1, TT51-1, and the rice endogenous reference gene, respectively. The robustness of the meqPCR was tested with different levels of the three transgenic rice genomic DNAs, and the sensitivity threshold of the meqPCR was at least 50 ng of 0.1% rice DNA for each event when the three transgenic rice events present and with other GM materials together. The constructed plasmid was evaluated using mixed samples with known GM contents in real-time quantitative PCR. The results indicated that the constructed plasmid was acceptable and suitable for GM rice quantitative analysis.