SELEX法体外筛选胃癌细胞适配子方法的建立

目的:建立SELEX技术筛选胃癌细胞SGC-7901适配子的方法,并初步鉴定获得的SGC-790 1细胞适配子.方法:体外合成全长88bp中间含52bp随机序列的ssDNA文库 ,通过优化PCR扩 增条件,利用地高辛-抗地高辛抗体-碱性磷酸酶系统测定亲和力,经SELEX反复筛选获得胃 癌SGC-7901细胞的特异性适配子.将最后一轮筛选产物克隆、测序并用相关软件分析适配子 序列的一级结构和二级结构.结果:经12轮SELEX筛选,ssDNA文库与SGC- 7901细胞的亲和力由0.16上升至1.14,表明特异性适配子得到逐步富集.22个克隆子测序, 有4个序列完全一致,二级结构预测茎环可能是适配子与胃癌细胞作用的结构基础.结论:成功建立了SELEX技术体外筛选胃癌细胞SGC-7901高亲和性适配子的方法.     

肝脏去唾液酸糖蛋白受体特异性RNA适配子的SELEX筛选与鉴定

目的获得能够特异性高亲和力结合肝脏特异性去唾液酸糖蛋白受体（asialoglycoprotein receptor,ASGPR）的RNA适配子,为开发诊断和治疗肝脏疾病的靶向性试剂和药物奠定基础。方法合成一个长度为115nt含有25个随机序列的单链DNA随机文库,通过体外转录构建出单链RNA适配子随机文库,以肝脏ASGPR大亚基为靶蛋白,采用SELEX（systematic evolution of ligands by exponential enrichment）技术筛选具有高亲和力的AsGPR特异性RNA适配子;通过膜结合测定实验、凝胶阻滞实验鉴定筛选适配子对靶蛋白的特异性和亲和力。结果经过12轮筛选获得了具有高亲和力的肝脏ASGPR特异性RNA适配子。结论成功地筛选出了具有离亲和力的肝脏ASGPR特异性RNA适配子库。     

cell-SELEX筛选的适配子在肿瘤诊断和治疗中的应用

抗肿瘤治疗发展迅速,但仍然存在许多问题,例如早期诊断困难及化疗的副反应.为解决这些问题,适配子、包括单链DNA或RNA寡核苷酸受到越来越多的关注.适配子具有高度选择性、亲和力及稳定性.通过指数富集细胞配体系统进化技术(cell-SELEX)筛选到的寡核苷酸在识别病变细胞方面具有很大优势,因此,它具有应用于诊断和治疗的巨大潜力.该文综述了适配子在生物标记物的发现、肿瘤细胞富集和检测、靶向肿瘤治疗中的作用.     

细胞酶联反应法 (cell-ELA) 测定特异结合U87-EGFRvⅢ细胞的适配子的亲和力

通过细胞-指数级富集的配基系统进化(Cell based systematic evolution of ligands by exponentialenrichment,cell-SELEX)方法从随机文库中筛选得到与稳定过表达人表皮生长因子受体Ⅲ型突变体(Epidermal growth factor receptor variantⅢ,EGFRvⅢ)的胶质瘤细胞U87细胞株(U87-EGFRvⅢ)特异结合的DNA适配子。以U87-EGFRvⅢ细胞作为检测对象,筛选到的适配子A15作为检测分子,建立一种细胞酶联反应(Cell enzyme-linked assay,cell-ELA)方法测定适配子的亲和力,并用EGFR抗体作为对照来比较此种DNA适配子的亲和力。结果显示,所测定的DNA适配子A15的解离平衡常数(Equilibrium dissociation constants,Kd)小于100 nmol/L,对U87-EGFRvⅢ细胞的结合能力与抗体相似。Cell-ELA法可较方便地用于cell-SELEX中适配子亲和力的测定。     

哈维氏弧菌适配子的SELEX筛选及其亲和特异性研究

哈维氏弧菌是水产养殖中的重要条件致病菌,对其进行快速、准确地检测和鉴定是相关病害防治的基础和关键.适配子具有亲和力高、特异性强、稳定性好等优点,在微生物的检测和鉴定方面呈现出广泛的应用前景.本研究以哈维氏弧菌为靶目标,采用SELEX技术,即指数级富集配体的系统进化技术,筛选其特异性适配子.经15轮筛选后,随机ssDNA文库的亲和力从3.51上升到58.95,提高了15.8倍.筛选出的适配子富集库经克隆、测序后得到52条不同序列,根据同源性将这些序列分成8个家族,其中第1和第2家族的适配子数量最多,超过总数的50%.通过深入分析,筛选出6个对哈维氏弧菌有显著亲和特异性(P0.01)的高频适配子,其中5个高频适配子(S1、S25、S26、S27、S35)对哈维氏弧菌有较高的亲和力,相应的亲和常数Kd值分别为(32.6±7.1)、(45.3±10.1)、(24.7±5.8)、(34.8±5.6)、(12.9±4.0)nmol/L.本文还对高频适配子的产生机制及其应用价值进行了探讨.本文首次筛选出了对哈维氏弧菌具有较高亲和特异性的适配子,为后续利用适配子进行哈维氏弧菌的检测和鉴定奠定了基础.     

丙型肝炎病毒 NS3 螺旋酶寡核苷酸 适配子的筛选与鉴定

为筛选和鉴定抗丙型肝炎病毒 (HCV) NS3 螺旋酶 (NS3h) 的寡核苷酸适配子 (aptamers). 利用 SELEX 技术,以 HCV NS3h 为靶分子,从体外合成的 81 bp 随机单链 DNA 文库中筛选与 HCV NS3h 特异结合的寡核苷酸适配子 . 克隆测序后,进行了解离常数 (K_d) 测定和 Clustal W 软件包分析适配子一级结构 . 经过 8 轮循环筛选,随机 ssDNA 库与 HCV NS3h 的结合率从 0.45% 上升到 29.5%. 所有的一级结构没有共同的同源序列,但可分 5 个家族,其中 4 个家族具有共同的保守序列 . 解离常数测定表明,寡核苷酸适配子 H2 与 HCV NS3h 特异结合的亲和力最高,K_d值为 140 nmol/L. 适配子 H2 (10 μmol/L) 在体外对 HCV NS3h 的活性具有一定的抑制作用,抑制率达 44%. 利用随机寡核苷酸文库获得了抗 HCV NS3h 的寡核苷酸适配子 .     

抑制肿瘤坏死因子-α的DNA适配子的筛选与鉴定

应用SELEX技术筛选能与TNF结合的DNA适配子。化学合成随机寡聚DNA库,以TNF为靶蛋白,经过12轮SELEX筛选,将所得产物克隆、测序。根据所测序列化学合成寡聚DNA适配子,用生物素_亲和素_辣根过氧化物酶显色系统检测适配子与TNF的结合活性;用鼠L929细胞检测适配子拮抗TNF活性。结果显示,所筛选到的寡聚DNA能与TNF-α高亲和力结合,并能在细胞培养中拮抗TNF-α的细胞毒活性。     

与细胞因子特异结合的寡聚核苷酸适配子及其在诊断和治疗中的应用

寡聚核苷酸适配子（Aptamer）是用指数富集式配基系统进化方法（SELEX）筛选出的寡聚核苷酸,它能与靶分子特异性结合,具有识别和抑制靶物质生物学活性的作用。将体外筛选到的寡聚核苷酸适配子作为在动物或人体内应用的药剂,还需要进行化学修饰来提高它的生物利用度和在血浆中的稳定性。2氟、2′烷氧基或2′氨基修饰可以提高适配子的稳定性,使适配子的体外半衰期延长;5′端交联一个高分子量的PEG分子或脂质体分子,可以使它的血浆清除率由1小时提高到几小时至1天。修饰后仍保持生物学活性的适配子可用于治疗相应靶细胞因子引起的疾病。目前,国内外已经筛选到了十几种细胞因子的适配子,其中血管内皮生长因子已经用于临床疾病的治疗。除了用于临床治疗外,适配子还可以用于细胞因子的诊断,凡是涉及抗体的诊断领域,几乎都可以用寡聚核苷酸适配子代替。应用大规模机械化筛选技术,可以在短期内筛选到大量的高特异性、高亲和力适配子,这将有力推动临床诊断和治疗的发展。     

抑制RANKL诱导破骨细胞分化的DNA适配子的筛选

目的:筛选能高特异性、高亲和力结合RANKL蛋白并有效抑制RANKL对破骨细胞诱导分化作用的DNA适配子。方法:首先,采用原核系统表达并纯化RANKL蛋白,通过SELEX(Systematic evolution of ligands by exponential)技术从人工合成的单链随机寡核苷酸文库中筛选能高特异性、高亲和力结合RANKL蛋白的DNA适配子。然后,用RNAfolding sever software分析适配子空间结构,以ELISA检测DNA适配子和RANKL亲和力大小并筛选出亲和力最高的一组DNA适配子用以验证DNA适配子对RANKL诱导破骨细胞分化的抑制作用。结果:(1)成功在原核系统表达并纯化RANKL蛋白;(2)筛选出能高特异性、高亲和力结合RANKL蛋白的12个DNA适配子。(3)与对照组相比,不同浓度DNA适配子能明显抑制TRAP阳性破骨细胞数量(P0.05),且浓度越高抑制效果越明显。结论:成功筛选出的DNA适配子能特异性结合RANKL蛋白并有效抑制RANKL对破骨细胞的诱导分化功能。     

SELEX技术在神经系统疾病研究中的应用

配体指数级富集系统进化（systematic evolution of ligands by exponential enrichment,SELEX）技术是一种组合化学技术,可经过反复筛选扩增得到针对靶分子的高亲和力和高特异性的适配子.适配子通过识别、结合特定靶分子并对其进行功能调控从而达到对疾病诊断和治疗的目的 .近年来SELEX技术在神经系统功能和疾病研究中的应用越来越多.现已经筛选出针对朊蛋白、肌腱蛋白-C、β-淀粉样肽、乙酰胆碱受体的自身抗体等靶标的适配子,促进了对朊病毒病、脑肿瘤、阿茨海默病、重症肌无力等神经系统疾病的诊断和治疗研究,为这些疾病的诊治提供了新的研究工具.     

筛选环孢霉素A适体的SELEX技术的建立

体外合成一个全长78个核苷酸,中间含35个随机序列的随机单链寡核苷酸序列(ssDNA)文库,运用指数富集的配体系统进化(SELEX)技术,以环孢霉素A(CsA)为靶目标,以磁珠作为筛选介质,利用生物素 链酶抗生物素 辣根过氧化物酶系统,检测每轮ssDNA文库与CsA的亲和力,筛选并鉴定CsA特异性的适体.经过11轮的筛选,ssDNA文库与CsA的亲和力呈上升趋势.将第10轮筛选产物克隆测序并运用相关软件进行一级结构和二级结构分析.随机挑选的19个克隆适体,根据一级结构的同源性可分为5个家族,二级结构预测以茎环(发夹)为主,这可能是适体与CsA作用的部位. CsA特异性的适体将用于酶联法、免疫荧光法等对CsA进行检测.     

In vitro selection of a DNA aptamer targeted against Shigella dysenteriae

To identify DNA aptamers demonstrating binding specificity for Shigella dysenteriae, a whole-bacterium Systemic Evolution of Ligands by Exponential enrichment (SELEX) method was applied to a combinatorial library of single-stranded DNA (ssDNA) molecules. After several rounds of selection using S. dysenteriae as the target, the highly enriched oligonucleotide pool was sequenced and then grouped into different families based on primary sequence homologies and similarities in the secondary structures. Aptamer S 1, which showed particularly high binding affinity in preliminary studies, was chosen for further characterisation. This aptamer displayed a dissociation constant (K_d value) of 23.47 ± 2.48 nM. Binding assays to assess the specificity of aptamer S 1 showed high binding affinity for S. dysenteriae and low apparent binding affinity for other bacteria. The ssDNA aptamers generated may serve as a new type of molecular probe for microbial pathogens, as it has the potential to overcome the tedious isolation and purification requirements for complex targets.     

Development of an Efficient Targeted Cell-SELEX Procedure for DNA Aptamer Reagents

Background

DNA aptamers generated by cell-SELEX offer an attractive alternative to antibodies, but generating aptamers to specific, known membrane protein targets has proven challenging, and has severely limited the use of aptamers as affinity reagents for cell identification and purification.

Methodology

We modified the BJAB lymphoblastoma cell line to over-express the murine c-kit cell surface receptor. After six rounds of cell-SELEX, high-throughput sequencing and bioinformatics analysis, we identified aptamers that bound BJAB cells expressing c-kit but not wild-type BJAB controls. One of these aptamers also recognizes c-kit endogenously expressed by a mast cell line or hematopoietic progenitor cells, and specifically blocks binding of the c-kit ligand stem cell factor (SCF). This aptamer enables better separation by fluorescence-activated cell sorting (FACS) of c-kit⁺ hematopoietic progenitor cells from mixed bone marrow populations than a commercially available antibody, suggesting that this approach may be broadly useful for rapid isolation of affinity reagents suitable for purification of other specific cell types.

Conclusions/Significance

Here we describe a novel procedure for the efficient generation of DNA aptamers that bind to specific cell membrane proteins and can be used as high affinity reagents. We have named the procedure STACS (Specific TArget Cell-SELEX).     

Isolation of a new ssDNA aptamer against staphylococcal enterotoxin B based on CNBr‐activated sepharose‐4B affinity chromatography

Staphylococcus aureus are potent human pathogens possessing arsenal of virulence factors. Staphylococcal food poisoning (SFP) and respiratory infections mediated by staphylococcal enterotoxin B (SEB) are common clinical manifestations. Many diagnostic techniques are based on serological detection and quantification of SEB in different food and clinical samples. Aptamers are known as new therapeutic and detection tools which are available in different ssDNA, dsDNA and protein structures. In this study, we used a new set of ssDNA aptamers against SEB. The methods used included preparation of a dsDNA library using standard SEB protein as the target analyte, affinity chromatography matrix in microfuge tubes, SELEX procedures to isolate specific ssDNA‐aptamer as an affinity ligand, aptamer purification using ethanol precipitation method, affinity binding assay using ELISA, aptamer cloning and specificity test. Among 12 readable sequences, three of them were selected as the most appropriate aptamer because of their affinity and specificity to SEB. This study presents a new set of ssDNA aptamer with favorable selectivity to SEB through 12 rounds of SELEX. Selected aptamers were used to detect SEB in infected serum samples. Results showed that SEB c1 aptamer (2 µg SEB/100 nM aptamer) had favorable specificity to SEB (k_d = 2.3 × 10^?11). In conclusion, aptamers can be considered as useful tools for detecting and evaluating SEB. The results showed that affinity chromatography was an affordable assay with acceptable accuracy to isolate sensitive and selective novel aptamers. Copyright © 2016 John Wiley & Sons, Ltd.     

Cell-SELEX based selection and characterization of DNA aptamer recognizing human hepatocarcinoma

Single-stranded DNA aptamers recognizing human hepatocarcinoma were isolated by means of a systematic evolution of ligands by exponential enrichment using whole cells as targets (cell-SELEX). After 11 rounds of cell-SELEX procedure using human hepatoma HepG2 cells as targets and human normal hepatocyte cells as counterparts, 12 independent DNA aptamer candidate sequences were obtained. The specific interaction between selected DNA aptamers and targeted cell was confirmed. Dissociation constants of the 12 sequences obtained were also estimated in the range of 19–450 nM. Moreover, the consensus secondary structure was found in the isolated aptamers, which was responsible to the recognition of HepG2 cells.     

金黄色葡萄球菌外毒素B特异性适体的筛选及其应用

目的:利用指数富集配基的系统进化(SELEX)技术,筛选能与金黄色葡萄球菌外毒素B(SEB)特异、高亲和力结合的单链DNA(ssDNA)适体,并将该适体应用于患者血清标本的检测。方法:从体外合成的96核苷酸随机ss-DNA文库中,以羧基磁珠作为筛选介质,经逐步PCR扩增、筛选,获得针对SEB的高亲和力、高特异性适体;利用荧光素标记适体测定筛选过程中各轮结合力;利用酶连接适体方法检测适体特异性和结合力。结果:经过13轮筛选,ssDNA文库与SEB的结合百分率从1.1%提高到39.8%,增加了36倍;获得的ssDNA适体(A11)针对SEB的特异性强,与金黄色葡萄球菌表面蛋白A(SPA)结合低,并能初步识别患者血清。结论:利用SELEX技术筛选获得了特异结合SEB的高亲和力的ssDNA适体,为金黄色葡萄球菌的临床诊断与治疗奠定了基础。     

早期胃癌血清特异标志物过氧化物酶4核酸适配体的筛选、鉴定与应用

胃癌是世界上死亡率第三的重大疾病,而在早期阶段却有着良好的治愈率和生存率。因此,找到针对早期胃癌的特异性标志物从而提高早期胃癌的检出率,是目前亟待解决的问题。在本实验室的早期研究中,发现过氧化物酶4（peroxiredoxin-4,PRDX4）有极大的潜能作为早期胃癌的特异性标志物,并且由于蛋白质结构的特殊性,能够分泌至血清中,为早期胃癌的无创化诊断提供了可能。本文为寻找血清中PRDX4蛋白的特异性适配体,通过消减-SELEX方法找到9种适配体。经特异性和亲和力分析后,证实其中Ap-EGACS-11在9种适配体中具有最高的特异性和亲和力。随后在适配体的验证研究中证实,相对于进展期胃癌病人血清、结直肠癌病人血清和正常人血清,Ap-EGACS-11对早期胃癌病人血清的检出率最高。该结果表明,PRDX4具有早期胃癌特异性血清标志物的潜能,且Ap-EGACS-11可直接作为早期胃癌的检测试剂。     

Dissection of the functional structure of aptamer17, which specifically recognizes differentiated PC12 cells

A specific single-stranded DNA (ssDNA) aptamer (aptamer17) that specifically recognizes differentiated PC12 cells had been previously obtained after 6 rounds of whole cell-based subtractive systematic evolution of ligands by exponential enrichment selection from a random ssDNA library. To further investigate the relationship between the structure and function of this aptamer, 3 truncated ssDNA aptamers were designed according to the predicted secondary structure of aptamer17. Our results show that the stem-loop is the core structure of the aptamers required for specific binding to differentiated PC12 cells, specifically loops I and II. Aptamer17 and the truncated aptamers with this basic structure could bind specifically to differentiated PC12 cells and identify these cells from a mixture of differentiated and undifferentiated PC12 cells. Therefore, truncated forms of aptamer17 may be useful in the clinic to identify undifferentiated and differentiated PC12 cells from a mixture of cells.