Exploring the potential of CRISPR/Cas genome editing for vegetable crop improvement: An overview of challenges and approaches

Vegetables provide many nutrients in the form of fiber, vitamins, and minerals, which make them an important part of our diet. Numerous biotic and abiotic stresses can affect crop growth, quality, and yield. Traditional and modern breeding strategies to improve plant traits are slow and resource intensive. Therefore, it is necessary to find new approaches for crop improvement. Clustered regularly interspaced short palindromic repeats/CRISPR associated 9 (CRISPR/Cas9) is a genome editing tool that can be used to modify targeted genes for desirable traits with greater efficiency and accuracy. By using CRISPR/Cas9 editing to precisely mutate key genes, it is possible to rapidly generate new germplasm resources for the promotion of important agronomic traits. This is made possible by the availability of whole genome sequencing data and information on the function of genes responsible for important traits. In addition, CRISPR/Cas9 systems have revolutionized agriculture, making genome editing more versatile. Currently, genome editing of vegetable crops is limited to a few vegetable varieties (tomato, sweet potato, potato, carrot, squash, eggplant, etc.) due to lack of regeneration protocols and sufficient genome sequencing data. In this article, we summarize recent studies on the application of CRISPR/Cas9 in improving vegetable trait development and the potential for future improvement.     

基于CRISPR/Cas原理的转基因产品检测技术研究进展

随着转基因产品商业化种植面积不断增加、国际贸易日趋频繁,对转基因生物安全管理提出了更高的要求。转基因产品检测技术作为安全评价的关键环节,逐渐引起了各国政府的关注。目前,针对转基因产品的快速检测方法层出不穷,但这些检测方法对于设备、试剂和专业的实验人员均有较高的要求。因此,为了有效支撑转基因相关产业的发展和管理,亟需建立一种高灵敏度、高特异性及高效的转基因检测技术。基因组编辑技术是近年来迅速发展的一类遗传修饰技术,其代表技术——CRISPR/Cas技术,更是极大地推动了生物技术的发展。CRISPR/Cas技术除了被应用于基因编辑领域,也逐渐被应用于核酸分子检测领域。基于此,以转基因产品检测技术为立足点,从CRISPR/Cas的检测原理、检测效果等技术层面分析了CRISPR/Cas检测技术发展的必然性,并对其在转基因产品检测上的应用前景进行展望,旨在为我国转基因产品快速检测和有效监管工作提供资料,对于保障我国转基因产品贸易的顺利进行具有重要意义。     

CRISPR/Cas9系统在基因组DNA片段编辑中的应用

源于细菌和古菌的Ⅱ型成簇规律间隔短回文重复系统[Clustered regularly interspaced short palindromic repeats (CRISPR)/CRISPR-associated nuclease 9 (Cas9),CRISPR/Cas9]近年被改造成为基因组定点编辑的新技术。由于它具有设计简单、操作方便、费用低廉等巨大优势,给遗传操作领域带来了一场革命性的改变。本文重点介绍了CRISPR/Cas9系统在基因组DNA片段靶向编辑方面的研究和应用,主要包括DNA片段的删除、反转、重复、插入和易位,这一有效的DNA片段编辑方法为研究基因功能、调控元件、组织发育和疾病发生发展提供了有力手段。本文最后展望了Ⅱ型CRISPR/Cas9系统的应用前景和其他类型CRISPR系统的应用潜力,为开展利用基因组DNA片段靶向编辑进行基因调控和功能研究提供参考。     

基于CRISPR/Cas系统的多重基因编辑与调控技术

规律成簇的间隔短回文重复序列(clustered regularly interspaced short palindromic repeats, CRISPR)及其相关Cas蛋白所构建的CRISPR/Cas系统是古细菌或细菌中特有的一种获得性免疫系统。研究人员将其开发成基因编辑工具之后,凭借其高效、精准和通用性强等优点迅速成为合成生物学领域的热门研究方向,在生命科学、生物工程技术、食品科学及农作物育种等多个领域引发了革命性的影响。目前基于CRISPR/Cas系统单基因编辑与调控技术日益完善,但在多重基因编辑和调控方面仍存在挑战。本文聚焦基于CRISPR/Cas系统的多重基因编辑与调控技术开发及应用,针对单个细胞内实现多位点基因编辑或调控和细胞群体内实现多位点基因编辑或调控技术,依据作用原理对其进行了系统总结和阐述,包括基于CRISPR/Cas系统的双链断裂、单链断裂以及多重基因调控技术等。这些工作丰富了多重基因编辑与调控的工具,为CRISPR/Cas系统在多领域的应用作出了贡献。     

Transformation of Acinetobacter sp. BD413 with DNA from commercially available genetically modified potato and papaya

AIM: To estimate the likelihood of transfer of kanamycin-resistance gene (nptII) from commercially available genetically modified (GM) plants. METHODS AND RESULTS: Acinetobacter sp. BD413 carrying a plasmid containing an inactivated nptII gene was treated with DNA derived from GM potato and GM papaya. Kanamycin-resistant transformants were obtained at a frequency of 10-30 microg(-1) DNA. Calculation of the results suggested that 6-9 x 10(4) molecules of genomic DNA from GM plants were needed to obtain one transformant. However, such transformation events were not detectable in the absence of the plasmid in the host strain. CONCLUSIONS: Acinetobacter sp. BD413 was transformed with DNA derived from GM potato and GM papaya, in the presence of an inactivated nptII gene on a plasmid. However, the frequency of such events in the natural environment on wild-type strains, while evidently low, remains unknown. SIGNIFICANCE AND IMPACT OF THE STUDY: Our results may help to evaluate potential risks associated with the use of antibiotic-resistance determinants as genetic markers in GM plants. Complete risk assessment must consider factors other than transformation frequency alone, including the natural background of antibiotic resistance present in bacterial populations, and the spectrum and clinical use of the antimicrobial agents in question.     

关于加强我国生物安全工作若干问题的思考

随着现代化生物技术,特别是基因工程技术的兴起和迅速发展,生物安全问题农渐成为全球社会普遍关注的热点,它既是一个科学问题,又是一个管理问题,需要从健全法律法规体系,理顺管理机构体系,支持鼓励科学研究,重视科学宣传普及,加强相关国际合作等方面,大力加强我国的生物安全工作,达到保障安全,促进发展的目标。     

转基因农作物检测技术及其应用与发展

常用的转基因检测方法可分为两个方向,一是以检测外源基因为目标,如多聚酶链式反应分析法(PCR),二是以检测外源蛋白为目标,如酶联免疫分析法(ELISA)。此外,近年来,随着世界各国对转基因生物安全问题的日益关注,还涌现出了一批新的检测方法,如微阵列分析法(microarray),色谱分析法(chroma-tography),表面等离子共振(surfaceplasmonresonance,SPR)生物传感器分析法以及近红外线光谱分析法(nearinfraredspectroscopy,NIR)等。将对各种转基因检测方法的原理、特点及研究现状做一个扼要介绍。     

限制性内切酶策略鉴定CRISPR/Cas9介导的Chrm3基因敲除小鼠

CRISPR/Cas9技术是近年发展起来的快速基因编辑技术。通过该技术已对多种生物的基因组进行了编辑。由此产生的基因编辑动物的建系与鉴定是随之而来较为繁琐的工作。单导向RNA(single-guide RNA, sgRNA)靶序列的设计和确定不仅影响后续靶向基因组的效率,还可作为优化鉴定、筛选方法的参考。本研究在选取sgRNA靶序列时,不仅依据软件的评分,还分析了sgRNA靶序列是否含有酶切位点,以便对后续纯合子/杂合子进行鉴定。结果显示,以特异引物扩增的野生型小鼠Chrm3基因片段可被限制性内切酶BanⅡ切为两个片段;而纯合子小鼠“丢失”该酶切位点,其PCR产物不能被切开;杂合子小鼠PCR产物被不完全切开,凝胶电泳结果可见三条带。本研究结果提示该策略可有效简化基因编辑动物建系鉴定工作,提高鉴定效率及改善阳性动物辨识效果。     

CRISPR/Cas基因编辑技术研究进展及其在斑马鱼中的应用

规律成簇间隔的短回文序列(Clustered regularly interspaced short palindromic repeats,CRISPR)是细菌和古菌中的获得性免疫系统,利用该系统能定点进行基因编辑。最近,科学家发现了新的CRISPR-associated (Cas)蛋白,其中由Cas12a介导的基因编辑能显著降低脱靶率。文中对CRISPR/Cas系统的发现历史、组成和分类、工作原理进行概述,并总结了该系统的最新研究进展及在斑马鱼Danio rerio中的应用。     

A CRISPR/Cas9-based genome editing system for Rhodococcus ruber TH

Rhodococcus spp. are organic solvent-tolerant strains with strong adaptive abilities and diverse metabolic activities, and are therefore widely utilized in bioconversion, biosynthesis and bioremediation. However, due to the high GC-content of the genome (~70%), together with low transformation and recombination efficiency, the efficient genome editing of Rhodococcus remains challenging. In this study, we report for the first time the successful establishment of a CRISPR/Cas9-based genome editing system for R. ruber. With a bypass of the restriction-modification system, the transformation efficiency of R. ruber was enhanced by 89-fold, making it feasible to obtain enough colonies for screening of mutants. By introducing a pair of bacteriophage recombinases, Che9c60 and Che9c61, the editing efficiency was improved from 1% to 75%. A CRISPR/Cas9-mediated triple-plasmid recombineering system was developed with high efficiency of gene deletion, insertion and mutation. Finally, this new genome editing method was successfully applied to engineer R. ruber for the bio-production of acrylamide. By deletion of a byproduct-related gene and in-situ subsititution of the natural nitrile hydratase gene with a stable mutant, an engineered strain R. ruber THY was obtained with reduced byproduct formation and enhanced catalytic stability. Compared with the use of wild-type R. ruber TH, utilization of R. ruber THY as biocatalyst increased the acrylamide concentration from 405 g/L to 500 g/L, reduced the byproduct concentration from 2.54 g/L to 0.5 g/L, and enhanced the number of times that cells could be recycled from 1 batch to 4 batches.     

CRISPR基因编辑技术虚拟仿真教学软件的构建及应用

CRISPR基因编辑技术逐渐成为一个强有力的分子技术,已越来越广泛地应用于科学研究和临床试验.在高校教学实践中,为了解决该实验原理复杂、操作难度大、周期长、成本高等问题,构建了CRISPR基因编辑仿真教学软件.该软件包括原理演示和实训操作2个模块.原理部分通过3D技术呈现出每个分子的结构,并以动画的形式演绎CRISPR...     

Genetically modified organisms and risks of their introduction

The major goal of this review is to assess food risks of the introduction of genetically modified (GM) crops. The author analyzes the properties of the several classes of target proteins used in the transgenic constructions and discusses the problems that arise due to the pleiotropic action of transgenic proteins, the horizontal transfer of the transgenic constructions, primarily in bacteria, and their instability. Particular consideration is given to elevated risks of using the GM plant varieties for producing pharmaceutical preparations, due to the probability of uncontrolled cross-pollination between the GM plants and the plants grown for foodstuff production. The author emphasizes the requirement for assessing in detail all hypothetic risks in each particular case of cultivating GM varieties; as a control, such assessment must involve a comprehensive comparison with the conventional parental forms.Translated from Fiziologiya Rastenii, Vol. 52, No. 1, 2005, pp. 115–128.Original Russian Text Copyright © 2005 by Kulikov.     

CRISPR/Cas基因编辑系统在原核微生物细胞工厂构建中的开发与应用

随着能源和环境问题的日益突出,化学品以及燃料的合成方式正逐渐由传统的化学法合成转变为以细菌为基础的生物炼制过程,其中最关键问题是需要开发出合适的基因工程工具用于构建相应的产品生产菌株。成簇的规律间隔短回文重复序列(Clusteredregularlyinterspacedshortpalindromic repeats,CRISPR)/CRISPR相关蛋白(CRISPR-associated proteins,Cas)系统是一种存在于细菌和古细菌中的免疫系统,能够用于抵御病毒和外源质粒的入侵,近年来被开发成为一种高效、便捷、精确的基因编辑工具,显示出巨大的应用潜力。本文立足于CRISPR/Cas系统的原理与最新分类,结合实例综述了CRISPR/Cas基因编辑系统在原核微生物细胞工厂构建中的建立与优化策略,以及主要的应用方向,并探讨该系统所面临的主要问题并提出了一些可行的解决方案。     

出入境转基因产品及其分子检测现状与展望

随着转基因产品在全球的迅速推广,包括我国在内的很多国家都建立了转基因标识制度。各检验检疫口岸应转基因产品生产企业、食品制造商、消费者等多方面需要,相继开展了转基因产品的检测工作。准确可靠的转基因产品检测技术是各国检疫检疫单位的共同需求。转基因产品的检测主要有两大类方法,一类是DNA水平上的检测,另一类是蛋白质水平上的检测。多个发达国家也相继成立专门机构或部门,负责转基因产品生物检测技术标准化工作。国际上对转基因产品的检测工作有向委托鉴定方向发展的趋势。我们简要综述了出入境转基因产品及其分子检测现状。