Clustered Regularly Interspaced Short Palindromic Repeats(CRISPR):A critical overview on the most promising applications of molecular scissors in oral medicine

The scientific community is continuously working to translate the novel biomedical techniques into effective medical treatments.CRISPR-Cas9 system(Clustered Regularly Interspaced Short Palindromic Repeats-9),commonly known as the“molecular scissor”,represents a recently developed biotechnology able to improve the quality and the efficacy of traditional treatments,related to several human diseases,such as chronic diseases,neurodegenerative pathologies and,interestingly,oral diseases.Of course,dental medicine has notably increased the use of biotechnologies to ensure modern and conservative approaches:in this landscape,the use of CRISPR-Cas9 system may speed and personalize the traditional therapies,ensuring a good predictability of clinical results.The aim of this critical overview is to provide evidence on CRISPR efficacy,taking into specific account its applications in oral medicine.

Genome engineering using the CRISPR/Cas system

Recently, an epoch-making genome engineering technology using clustered regularly at interspaced short palindromic repeats(CRISPR) and CRISPR associated(Cas) nucleases, was developed. Previous technologies for genome manipulation require the time-consuming design and construction of genome-engineered nucleases for each target and have, therefore, not been widely used in mouse research where standard techniques based on homologous recombination are commonly used. The CRISPR/Cas system only requires the design of sequences complementary to a target locus, making this technology fast and straightforward. In addition, CRISPR/Cas can be used to generate mice carrying mutations in multiple genes in a single step, an achievement not possible using other methods. Here, we review the uses of this technology in genetic analysis and manipulation, including achievements made possible to date and the prospects for future therapeutic applications.

Combination of CRISPR/Cas9 System and CAR-T Cell Therapy:A New Era for Refractory and Relapsed Hematological Malignancies

Chimeric antigen receptor T(CAR-T)cell therapy is the novel treatment strategy for hematological malignancies such as acute lymphoblastic leukemia(ALL),lymphoma and multiple myeloma.However,treatment-related toxicities such as cytokine release syndrome(CRS)and immune effector cell-associated neurotoxicity syndrome(ICANS)have become significant hurdles to CAR-T treatment.Multiple strategies were established to alter the CAR structure on the genomic level to improve efficacy and reduce toxicities.Recently,the innovative gene-editing technology-clustered regularly interspaced short palindromic repeats(CRISPR)/CRISPR-associated nuclease9(Cas9)system,which particularly exhibits preponderance in knock-in and knockout at specific sites,is widely utilized to manufacture CAR-T products.The application of CRISPR/Cas9 to CAR-T cell therapy has shown promising clinical results with minimal toxicity.In this review,we summarized the past achievements of CRISPR/Cas9 in CAR-T therapy and focused on the potential CAR-T targets.

应用于食品检测领域的分子即时检测技术研究进展

食品安全问题关系人类民生。为有效预防和控制食品安全风险,减少食品安全经济损失,迫切需要开发出针对食源性病原体、食物掺假、转基因作物的高特异性、高敏感性、快速的核酸检测技术。即时检测(point-of-care testing,POCT)作为一种新兴的快速检测手段,由于其检测速度快、操作简单、现场检查等特点,在食品检测领域应用广泛。本文首先介绍了POCT技术的发展历史,而后根据食品安全事件的特点,从食源性致病菌、食物掺假、转基因作物3个方向分析了食品检测的主要对象,阐述了分子POCT技术在食品检测领域的应用现状,最后对应用于食品检测领域的分子POCT技术存在的问题和解决办法进行了分析总结,对食品检测分子POCT技术的发展方向进行了展望。本文有助于进一步了解分子POCT技术在食品检测中的应用,并为分子POCT技术在食品快速检测中的研究和应用提供参考。

基于RAA-CRISPR/Cas12a技术的桃成分单管一体化快速检测方法

通过设计特异性的桃重组酶介导的等温扩增(recombinase-aided amplification,RAA)和CRISPR RNA(crRNA)引物,建立RAA技术结合CRISPR/Cas12a系统的单管一体化桃成分快速检测方法,并分析该方法的特异性、灵敏度和检出限,同时对市售样品进行检测。结果显示,该方法不依赖大型仪器设备,在30 min内即可完成桃成分的快速检测;与其他常见水果物种之间无交叉污染,表现出良好的特异性;该方法的灵敏度为1.0×10-1 ng/μL;检出限为1%;通过对20份市售样品检测,结果显示本方法与实时聚合酶链式反应法检测结果一致。因此,本研究建立的RAA-CRISPR/Cas12a单管一体化桃成分快速检测方法具有特异性好、灵敏度高的优点,为桃成分快速检测提供了一种新的技术。

基于重组酶介导等温扩增-CRISPR/Cas12a的青鱼物种快速鉴定研究

目的 建立一种快速、特异、灵敏地鉴定青鱼物种的方法。方法 以青鱼线粒体16SrRNA基因的保守序列设计特异性crRNA,并根据crRNA设计重组酶介导等温扩增(recombinase-mediatedisothermal amplification,RAA)引物;建立青鱼的RAA-CRISPR/Cas12a快速鉴定方法,并对该方法的检测时间进行优化;同时,评估该方法的特异性和灵敏度,并对青鱼及其近缘物种的市售样品进行检测。结果 该方法仅需25 min完成检测;对青鱼物种的鉴定表现出显著的特异性,并对其近缘物种如草鱼、赤眼鳟、鳡鱼、倒刺鲃的检测结果均呈阴性;方法灵敏度为1.0×10-3ng/μL(以基因组DNA计);与DNA条形码技术相比,该方法在市售样品的检测结果上表现一致。结论 建立了青鱼物种的RAA-CRISPR/Cas12a现场快速检测方法,该方法具备快速、特异、灵敏的特点,为水产市场或野外环境中快速检测青鱼物种提供了技术手段。

利用CRISPR/Cas9系统制备斑马鱼cbsb敲除模型

目的 采用成簇的规律性间隔的短回文重复序列(CRISPR)/Cas9系统对斑马鱼胱硫醚-β-合成酶b基因(cbsb)进行编辑,并制备稳定的斑马鱼cbsb敲除品系。方法 使用ClustalX软件分析斑马鱼cbsb编码蛋白(Cbsb)的保守结构域,利用生物信息学选取向导RNA(gRNA)靶点,体外合成并纯化gRNA和密码子优化的Cas9 mRNA,在刚受精的斑马鱼胚胎(1-cell期)中显微注射混合的gRNA和Cas9 mRNA,提取受精后3 d的斑马鱼幼鱼基因组,通过PCR扩增并测序分析靶点的切割效率,通过基因组扩增和测序筛选并获得cbsb敲除的稳定品系。结果 斑马鱼Cbsb与人、小鼠胱硫醚-β-合成酶(CBS)高度同源。在斑马鱼Cbsb保守结构域的编码序列处设计4个靶点,其中4#靶点具有高效的切割效率,利用该靶点制备并筛选获得多个cbsb敲除斑马鱼,选取-3+13 bps和-228 bps移码突变的两种品系,进一步筛选获得稳定的cbsb敲除品系。结论 利用CRISPR/Cas9系统成功制备了两种斑马鱼cbsb敲除的稳定品系,为进一步在斑马鱼活体中研究Cbsb的功能奠定了基础。

重组酶介导的等温扩增结合CRISPR/Cas12a检测志贺氏菌和克罗诺杆菌

目的应用重组酶介导的等温扩增技术(recombinase-aided amplification,RAA)结合成簇规则的间隔短回文重复序列(clustered regularly interspaced short palindromic repeats,CRISPR),建立志贺氏菌和克罗诺杆菌的快速检测方法。方法通过筛选志贺氏菌和克罗诺杆菌特异性基因,设计特异扩增引物、CRISPR脱氧核糖核酸(CRISPR deoxyribonucleic acid,crDNA)和探针,将靶标进行RAA扩增后,建立CRISPR检测方法。对方法的灵敏度、特异性和应用性进行评价,并与国标检测方法进行对比。结果本研究对志贺氏菌和克罗诺杆菌纯菌液DNA最低检出限分别为4.9×10^(3) CFU/mL、4.4×10^(4) CFU/mL,基因组DNA最低检出限为6.8×10^(‒3) ng/μL、5.7×10^(‒3 )ng/μL,特异性好,与其他病原菌无交叉反应。同时,该方法成功检测出加标猪肉样品和人工污染奶粉中的志贺氏菌和克罗诺杆菌,比国家标准检出限更低。结论本研究建立的RAA-CRISPR方法可有效应用于志贺氏菌和克罗诺杆菌的检测,这为快速筛查食品中是否污染这两种病原菌提供重要价值。

CRISPR/Cas12a技术在动物疫病检测方面的应用

CRISPR/Cas系统是由簇状规则间隔的短回文重复序列(CRISPR)和CRISPR相关蛋白(Cas)组成的一种基因编辑技术,可以特异地切割和识别靶标核酸基因。该技术具有检测速度快、灵敏度高和特异性强的优势,因此被广泛应用于动物疫病检测领域。本文就CRISPR/Cas12a结合等温核酸扩增技术和可视化技术在动物疫病检测中的应用进行综述,并对其应用前景进行展望,以期为我国的养殖业和进境动物疫病的监测提供技术支撑。

CRISPR/Cas系统中工程化gRNA技术的研究和应用

CRISPR/Cas是原核生物在进化过程中获得的一种免疫防御系统,用于抵抗外来遗传物质的入侵,近年来被开发成为高效的基因编辑、基因调控以及分子诊断工具。其可编程靶向机制揭开了利用该系统进行基因组操作的序幕,并允许在活性范围内实现动态调节和控制基因表达。作为现有基因修饰手段中灵活性最强和成本最低的技术之一,已被广泛应用于临床疾病治疗、工农业生产、可持续染料开发和化学品加工等领域。随着对CRISPR/Cas系统的不断深入挖掘和探索,大量研究报道了gRNA工程改造及优化方法,包括改变间隔序列长度、调节恒定区和可变区的结构、向末端或中间延伸添加额外功能序列及化学合成修饰等,以期降低脱靶突变率,提高作用效率,充分激发CRISPR基因操纵工具在生物医学方面的潜力。基于此,本综述将介绍CRISPR/Cas9和CRISPR/Cas12系统中gRNA工程化设计方法及应用研究的最新进展,分析探讨了当前工程化gRNA技术面临的机遇和挑战,旨在为获得性能更加优异的gRNA提供思路和方向,从而提高利用CRISPR/Cas系统探测人类细胞基因组的能力,进一步为可编程生物学带来更多可能性。

Overexpression of proteasome 26S subunit non-ATPase 6 protein and its clinicopathological significance in intrahepatic cholangiocarcinoma

BACKGROUND Currently,intrahepatic cholangiocarcinoma(ICC)poses a continuing,significant health challenge,but the relationship has yet to be established between ICC and the proteasome 26S subunit non-ATPase 6(PSMD6).AIM To investigate the protein expression and clinicopathological significance of PSMD6 in ICC.METHODS The potential impact of the PSMD6 gene on the growth of ICC cell lines was analyzed using clustered regularly interspaced short palindromic repeat knockout screening technology.Forty-two paired specimens of ICC and adjacent noncancerous tissues were collected.PSMD6 protein expression was determined by immunohistochemistry.Receiver operating characteristic curve analysis was performed to validate PSMD6 expression level,and its association with ICC patients’various clinicopathological characteristics was investigated.RESULTS The PSMD6 gene was found to be essential for the growth of ICC cell lines.PSMD6 protein was significantly overexpressed in ICC tissues(P<0.001),but showed no significant association with patient age,gender,pathological grade,or tumor-node-metastasis stage(P>0.05).CONCLUSION PSMD6 can promote the growth of ICC cells,thus playing a pro-oncogenic role.

CRISPR/Cas核酸检测系统的研究进展和未来挑战

成簇规律间隔短回文重复序列(CRISPR)/成簇规律间隔短回文重复序列相关蛋白(Cas)系统是一种新兴的分子诊断技术,具有检测速度快、操作简单、特异性高等优势,目前已成为分子诊断领域的研究热点。基于CRISPR/Cas系统构建的核酸检测系统中有一部分已得到临床验证,并获得预期的结果,有望成为一种理想的核酸分子诊断技术,但其在临床大规模应用前尚有一系列问题需要解决。文章对已建立的CRISPR/Cas核酸检测系统的原理、特点和存在的问题进行综述,以期为CRISPR/Cas核酸检测系统的临床应用提供依据。

CRISPR-Cas13a系统在病原体检测应用中的最新研究进展

规律成簇的间隔短回文重复序列及相关蛋白(CRISPR-Cas)系统已作为近年来兴起的新一代分子诊断工具,被广泛应用于基因编辑、核酸检测等领域,其中Cas13a亚型因其在核酸检测中高特异度、高灵敏度、无需昂贵设备、操作简单、费用低廉等特点,在病原体检测领域展现出巨大的潜力。该文综述了CRISPR-Cas13a的作用机制、在病原体检测中的应用以及相关检测方法,并对Cas13a应用前景进行了展望。以期为CRISPR-Cas13a系统的进一步研究及其在病原体检测中的应用提供借鉴和参考。

基于CRISPR-Cas12a系统的鼠伤寒沙门氏菌可视化检测方法的建立

为了建立一种特异性强、灵敏度高的鼠伤寒沙门氏菌可视化检测方法,试验将聚合酶链式反应(PCR)与成簇的有规律间隔的短回文重复序列及其相关蛋白(clustered regularly interspaced short palindromic repeats-CRISPR-associated, CRISPR-Cas)系统相结合,首先根据鼠伤寒沙门氏菌的spy基因序列3′末端的保守区设计crRNA及靶标序列扩增引物,根据可视化检测原理设计单链DNA(single-stranded DNA, ssDNA)荧光报告探针;然后对靶标序列进行PCR扩增,将扩增产物加入CRISPR-Cas12a系统,在蓝光下通过肉眼观察是否产生绿色荧光实现对靶标的检测;最后进行特异性试验和灵敏度试验。结果表明:建立的方法仅能检测到鼠伤寒沙门氏菌,检测不到除鼠伤寒沙门氏菌外其他血清型的沙门氏菌及大肠杆菌、巴氏杆菌、鸭疫里默氏杆菌,能检测到循环数为14个的PCR产物和0.53 copies/μL的重组质粒,灵敏度优于常规PCR方法和实时荧光定量PCR方法。说明本试验建立的方法可以实现鼠伤寒沙门氏菌的可视化检测,具有特异性强、灵敏度高的特点。

基于293T-Cas9细胞株构建ICP34.5基因敲除的oHSV-1/Ecfp病毒

目的构建稳定表达Cas9蛋白的工具细胞,并利用短回文重复序列/相关蛋白9(CRISPR/Cas9)编辑技术改造1型单纯疱疹病毒(HSV-1),获得ICP34.5基因敲除的oHSV-1/Ecfp重组病毒。方法利用慢病毒包装体系,将包装Cas9表达质粒的病毒感染HEK293T细胞,然后经嘌呤霉素筛选获得稳定表达Cas9蛋白的293T-Cas9细胞株,通过聚合酶链式反应(PCR)及蛋白质免疫印迹技术检测Cas9基因及蛋白表达情况;利用分子克隆技术构建HSV-1病毒ICP34.5基因敲除的基因编辑质粒(pU6-Ecfp);pU6-Ecfp转染293T-Cas9细胞后感染野生型HSV-1病毒,在胞内通过CRISPR/Cas9技术敲除HSV-1病毒中ICP34.5基因,再利用增强型青色荧光(Ecfp)示踪及极限稀释法进行病毒富集纯化,通过PCR法进行oHSV-1/Ecfp病毒鉴定。结果PCR扩增、核酸电泳及蛋白质免疫印迹技术结果显示,细胞株293T-Cas9高转录Cas9基因及高表达Cas9蛋白;通过PCR鉴定及荧光示踪结果显示,基因编辑质粒pU6-Ecfp构建成功;Ecfp荧光示踪、PCR扩增及核酸电泳结果显示,Ecfp成功插入ICP34.5基因敲除位点,获得oHSV-1/Ecfp重组病毒。结论稳定表达Cas9蛋白的293T-Cas9细胞可作为CRISPR/Cas9基因编辑的工具细胞,构建的HSV-1/Ecfp病毒实现了ICP34.5基因敲除及Ecfp示踪蛋白的敲入。

转录因子HNF1A、HNF4A和FOXA2调节肝细胞蛋白质N-糖基化

Hepatocyte nuclear factor 1 alpha(HNF1A),hepatocyte nuclear factor 4 alpha(HNF4A),and forkhead box protein A2(FOXA2)are key transcription factors that regulate a complex gene network in the liver,cre-ating a regulatory transcriptional loop.The Encode and ChIP-Atlas databases identify the recognition sites of these transcription factors in many glycosyltransferase genes.Our in silico analysis of HNF1A,HNF4A.and FOXA2 binding to the ten candidate glyco-genes studied in this work confirms a significant enrich-ment of these transcription factors specifically in the liver.Our previous studies identified HNF1A as a master regulator of fucosylation,glycan branching,and galactosylation of plasma glycoproteins.Here,we aimed to functionally validate the role of the three transcription factors on downstream glyco-gene transcriptional expression and the possible effect on glycan phenotype.We used the state-of-the-art clus-tered regularly interspaced short palindromic repeats/dead Cas9(CRISPR/dCas9)molecular tool for the downregulation of the HNF1A,HNF4A,and FOXA2 genes in HepG2 cells-a human liver cancer cell line.The results show that the downregulation of all three genes individually and in pairs affects the transcrip-tional activity of many glyco-genes,although downregulation of glyco-genes was not always followed by an unambiguous change in the corresponding glycan structures.The effect is better seen as an overall change in the total HepG2 N-glycome,primarily due to the extension of biantennary glycans.We propose an alternative way to evaluate the N-glycome composition via estimating the overall complexity of the glycome by quantifying the number of monomers in each glycan structure.We also propose a model showing feedback loops with the mutual activation of HNF1A-FOXA2 and HNF4A-FOXA2 affecting glyco-genes and protein glycosylation in HepG2 cells.

The Applications of CRISPR Screening in Aging Research

The advancement of Clustered Regularly Interspaced Short Palindromic Repeats(CRISPR)gene editing technology has revolutionized the comprehension of human genome,propelling molecular and cellular biology research into unexplored realms and accelerating progress in life sciences and medicine.CRISPR-based gene screening,recognized for its efficiency and practicality,is widely utilized across diverse biological fields.Aging is a multifaceted process governed by a myriad of genetic and epigenetic factors.Unraveling the genes regulating aging holds promise for understanding this intricate phenomenon and devising strategies for its assessment and intervention.This review provides a comprehensive overview of the progress in CRISPR screening and its applications in aging research,while also offering insights into future directions.CRISPR-based genetic-manipulation tools are positioned as indispensable instruments for mitigating aging and managing age-related diseases.

Is 26S proteasome non-ATPase regulatory subunit 6 a potential molecular target for intrahepatic cholangiocarcinoma?

In this editorial we comment on the article by Tang et al published in the recent issue of World Journal of Hepatology.Drug therapy of intrahepatic cholangiocarcinoma(iCCA)poses an enormous challenge since only a small proportion of patients demonstrate beneficial responses to therapeutic agents.Thus,there has been a sustained search for novel molecular targets for iCCA.The study by Tang et al evaluated the role of 26S proteasome non-ATPase regulatory subunit 6(PSMD6),a 19S regulatory subunit of the proteasome,in human iCCA cells and specimens.The authors employed clustered regularly interspaced short palindromic repeat(CRISPR)knockout screening technology integrated with the computational CERES algorithm,and analyzed the human protein atlas(THPA)database and tissue microarrays.The results show that PSMD6 is a gene essential for the proliferation of 17 iCCA cell lines,and PSMD6 protein was overexpressed in iCCA tissues without a significant correlation with the clinicopathological parameters.The authors conclude that PSMD6 may play a promoting role in iCCA.The major limitations and defects of this study are the lack of detailed information of CRISPR knockout screening,in vivo experiments,and a discussion of plausible mechanistic cues,which,therefore,dampen the significance of the results.Further studies are required to verify PSMD6 as a molecular target for developing novel therapeutics for iCCA.In addition,the editorial article summarizes the latest advances in molecular targeted drugs and recently emerging immunotherapy in the clinical management of iCCA,development of proteasome inhibitors for cancer therapy,and advantages of CRISPR screening technology,computational methods,and THPA database as experimental tools for fighting cancer.We hope that these comments may provide some clues for those engaged in the field of basic and clinical research into iCCA.

基因编辑技术及其在糖生物学研究中的应用

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反式切割CRISPR/Cas技术在食源致病微生物检测方面的原理及应用

食源性致病微生物是食品安全的一大严重威胁,传统的生化检测手段面临着一系列挑战。近年来,随着成簇规律间隔短回文重复序列(clustered regularly interspaced short palindromic repeats,CRISPR)技术的逐步发展,具有反式切割活性的CRISPR/Cas体系受到了越来越多的关注。本文综述了具有反式切割活性的CRISPR/Cas体系的起源与分类,并详细介绍了具有反式切割活性的CRISPR/Cas体系的作用原理。同时,本文对反式切割CRISPR/Cas技术在食源性致病微生物领域的多方面应用进行了综述,并讨论了该技术的优劣和未来发展方向。