首页 | 本学科首页   官方微博 | 高级检索  
相似文献
 共查询到20条相似文献,搜索用时 171 毫秒
1.
抗CD20嵌合抗体片段Fab′突变体的表达和活性研究   总被引:6,自引:2,他引:4  
利用PCR方法从抗CD20单链抗体(ScFv)表达载体上扩增抗CD20抗体轻链可变区基因(VL)、重链可变区基因(VH),同时在抗体的可变区引入突变,然后将VH、VL基因重组到Fab′表达载体pYZF1中,构建抗CD20嵌合抗体Fab′片段表达载体,并在大肠杆菌16c9中进行高效可溶性分泌表达。经大量的筛选,获得一个产量和活性均有所提高的突变克隆。其突变位点在轻链可变区的CDR1区,即G77→A(Ser→Asn)。突变的抗体的表达量为每克干菌3.8 mg,而未突变抗体的表达量为每克干菌1.3 mg。突变体的亲和力常数Ka为2.2×109 L/mol,约为突变前的2倍。竞争性免疫荧光抑制实验表明,突变的Fab′片段能竞争性抑制鼠源性抗CD20抗体HI47和CD20表达细胞Raji细胞的结合,使HI47的结合阳性率由98%下降至37.55%,体外细胞生长抑制试验亦证明突变的Fab′片段的抑制活性明显高于未突变的抗体。  相似文献   

2.
鼠源单克隆抗体MA18/7是特异识别乙型肝炎病毒 (HBV)pre S1抗原的中和抗体。为表达MA18/7的小分子抗体 ,将MA18/7的重链可变区基因(VH)和轻链可变区(VL)基因分别克隆到原核表达载体pTO-T7进行原核表达。结果VH和VL均以包涵体的形式高效表达 ,包涵体经过变性、复性及金属离子亲和纯化后获得纯度>90%的重组抗体片段。生物传感器、竞争ELISA和间接ELISA测定均显示 ,VH 或VL 均不能结合相应抗原 ,但二者体外混合后可迅速非共价结合形成具有良好活性的可变区抗体Fv,表明MA18/7的抗原结合活性区由重链可变区和轻链可变区共同组成.  相似文献   

3.
抗CEA单链抗体与链亲和素融合基因的表达   总被引:1,自引:0,他引:1  
克隆分泌CEA杂交瘤细胞重链可变区(VH)和轻链可变区(VL),以Linker连接VH及VL构建抗CEA单链抗体.同时以Spacer连接单链抗体和链亲和素,构建成功单链抗体和链亲和素融合基因,克隆该融合基因至原核表达载体,pET21a(+),经IPTG诱导表达出该双特异性融合蛋白.活性鉴定表明该融合蛋白具有结合CEA及生物素的双特异性.该融合蛋白在生物领域中有较广阔的应用前景.  相似文献   

4.
构建抗人乳腺癌细胞MCF 7的噬菌体单链抗体库 ,从中筛选MCF 7细胞特异性单链抗体。用MCF-7细胞免疫BALB C小鼠 ,取脾脏 ,提取总RNA ,用RT-PCR技术扩增小鼠抗体重链 (VH)和轻链 (VL)可变区基因 ,经重叠PCR(SOE-PCR) ,在体外将VH和VL连接成单链抗体 (scFv)基因 ,并克隆到噬菌粒载体pCANTAB5E中 ,电转化至大肠杆菌TG1,经辅助噬菌体超感染 ,构建噬菌体单链抗体库。从该抗体库中筛选特异性识别MCF-7细胞的噬菌体单链抗体 ,将表面展示单链抗体的单克隆噬菌体转化大肠杆菌TOP10进行可溶性表达。成功地构建了库容为12×106 的抗MCF-7乳腺癌细胞的单链抗体库 ,初步筛选到了与MCF 7细胞特异性结合的scFv,Westernblot检测表明 ,在大肠杆菌TOP10中实现了单链抗体可溶性表达  相似文献   

5.
抗人CD3单链抗体与改形单域抗体的表达   总被引:4,自引:0,他引:4  
设计并化学合成含有适当酶切位点及连接肽的寡核苷酸序列,与一定的背景载体连接并改造成适用于单链抗体表达的载体:外分泌型pWAI80和融合蛋白型pROH80从分泌抗人CD3单克隆抗体的杂交瘤细胞UCHT1中,经PCR扩增出轻、重链可变区基因VH和VK,并插入上述表达载体中构建成单链抗体基因.通过对鼠OKT3结合位点的结构模拟,并比较人、鼠抗体家族性保守序列,设计出改形OKT3的基因序列.化学法部分合成8个寡核苷酸片段,应用重叠PCR技术扩增出完整改形重链基因VH,并克隆、酶切和测序鉴定.将所克隆VH基因插入表达载体pCOMB3和 pGEX-4T-1中进行表达.经 IPTG诱导表达,对表达产物进行SDS-PAGE和 Western blot分析以及 ELISA检测,结果发现分泌型表达产物及 M13基因Ⅲ-VH改形单域抗体融合蛋白具有与CD3单抗竞争抑制的活性;而融合型单链抗体及改形单域抗体表达产物主要以包涵体形式存在,占细菌总蛋白的 30%左右.  相似文献   

6.
应用RT-PCR技术从分泌抗人黑色素瘤单克隆抗体的杂交瘤细胞HB8760中克隆了抗体轻、重链可变区基因,用(Gly4Ser)3连接肽基因将VH、VL连接成ScFv基因,并进行了序列测定。ScFv基因全长927bp,其中VH基因长360bp,编码120个氨基酸,VL基因长324bp,编码108个氨基酸。在大肠杆菌融合表达载体pGEX-4T-1中表达了GST-ScFv融合蛋白,表达产量占菌体总蛋白的29%。凝血酶消化后的产物具有黑色素瘤细胞结合活性。  相似文献   

7.
基因工程二硫键抗体   总被引:1,自引:0,他引:1  
二硫键抗体(dsFv)的概念最早出现于1990年,它是将抗体重链可变区(VH)和轻链可变区(VL)的各一个氨基酸残基突变为半胱氨酸,通过链间二硫键连接抗体可变区(Fv)的片段抗体.通用的突变位点是重链的44位和轻链的100位或重链的105位和轻链的43位.dsFv最显著的优点是生化性质稳定,能够耐受环境条件的剧烈作用,在血液中的半衰期长达14 d以上,符合临床给药要求.动物实验显示,dsFv-毒素在不对动物造成毒副作用的情况下,可完全抑制肿瘤生长.  相似文献   

8.
抗人CD19单链抗体基因的构建、表达及功能测定   总被引:7,自引:0,他引:7  
采用RT-PCR方法从分泌抗人类白细胞表面分化抗原CD19单克隆抗体的杂交瘤细胞中克隆出VH和VL可变区基因,再通过重叠延伸拼接(spliceoverlap extension)PCR方法在VH和VL可变区基因之间引入连接肽(Gly4Ser)3,体外构建抗人CD19单链抗体(抗CD19-ScFv)基因。将其克隆至表达载体PET28a并在大肠杆菌中表达。SDS-PAGE和Westernblot分析结果表明,抗CD19-ScFv在BL21(DE3)菌中获得表达,重组蛋白的相对分子量为27kD,表达产物以不溶性包涵体形式存在,经过溶解包涵体,镍柱亲和层析纯化和体外复性过程,获得了高纯度的单链抗体片段。流式细胞分析结果证实抗CD19ScFv可与人类白细胞表面的分化抗原CD19结合,保留了鼠源性单抗与CD19结合活性。抗人CD19-ScFv的构建与表达,为下一步针对B淋巴系统恶性肿瘤的靶向治疗奠定了基础。  相似文献   

9.
以本室研制的一株抗肿瘤血管单克隆抗体AA98为基础,采用PCR扩增抗体AA98基因的重链可变区(VH)和轻链(L),以重链恒定区1(CH1)5′端12个氨基酸的序列作为连接肽,并将连接肽中的Lys突变为Ser,构建VH连接肽-L三结构域单链抗体。重组VH/L单链抗体在大肠杆菌中得到了高效表达,其表达量占菌体总蛋白质的20%。表达的蛋白质在菌内形成包含体,经凝胶过滤法复性,获得了有抗原结合活性的VH/L。该三结构域单链抗体的成功构建和复性,为重组抗体片段的研制提供了借鉴。  相似文献   

10.
为构建能同时表达抗人CD28嵌合重链和嵌合轻链基因的双启动子杆状病毒转移载体,利用PCR法扩增出抗人CD28鼠源性单抗的可变区基因和人IgG1的恒定区基因,再采用一种不需要限制性核酸内切酶和连接酶的新方法——三引物PCR(TP-PCR)法将两者拼接后分别插入杆状病毒转移载体pAcUW3的php10启动子后,并通过酶切、电泳、PCR扩增和测序对重组体进行了鉴定。研究结果表明,TP-PCR法快速、方便、准确,无需设计外源的DNA序列,就能构建完好的融合表达基因。该转移载体的构建成功为嵌合抗体基因在昆虫细胞中的表达奠定了基础。  相似文献   

11.
Cassette vectors have been constructed for mammalian expression of complete immunoglobulin heavy and light chain genes whose variable regions are produced by the polymerase chain reaction (PCR). The light and heavy chain vectors have promoter, leader, partial intron, enhancer and constant region segments within modified pSV2-gpt and pSV2-neo plasmids, respectively. Variable (V) regions are obtained by PCR using a two step process: 1) the V gene is amplified from genomic or cDNA, cloned into an intermediate vector and sequenced; 2) the first PCR product serves as the template for a second amplification in which restriction enzyme recognition sites and limited flanking intron sequence are added. The second PCR product is inserted into the expression vector, which is then transfected into mouse myeloma cells. These vectors contain human constant regions and may be used to express chimeric, humanized or human Ig genes. This report describes the design of these vectors and their application for the expression of chimeric 60.3, an anti-CD18 antibody.  相似文献   

12.
采用基因工程技术 ,将小鼠 6C6单克隆抗体可变区基因与人抗体恒定区基因连接 ,构建了鼠 人 6C6嵌合抗体基因 ,并在CHO细胞中高效表达 .利用ProteinA亲和层析柱从细胞培养上清中分离纯化 6C6嵌合抗体 ,得到电泳纯度大于 98%的 6C6嵌合抗体 ,其重链 (5 5kD)和轻链 (2 4kD)符合IgG相对分子质量的理论值 .Western印迹、细胞免疫荧光和免疫组织化学实验结果均呈阳性 .表明6C6嵌合抗体可识别人乳腺癌细胞表面上的肿瘤相关抗原 ,保持了 6C6单克隆抗体的特性 ,为后续的研究工作奠定了基础  相似文献   

13.
Production and application of therapeutic monoclonal antibodies are second only to vaccines in the world pharmaceutical market. The most common therapeutic antibodies are monoclonal antibodies (mAbs) of the IgG isotype that are produced in eukaryotic CHO cells. In recent years, there has been a considerable interest in developing treatment medications based on IgA antibodies, which can have a wide range of effector functions on human mucous membranes. To study the expression level of immunoglobulin A (IgA) in mammal cells, we designed a set of bipromoter (CMV and EF1α) vectors. The vectors contain gene fragments that encode the heavy chain variable domain (VH) and the light chain variable domain (VL) of the human monoclonal antibody FI6v3 against the hemagglutinin of influenza virus A. They also contain gene fragments that encode the light chain (kappa type) constant domain and the heavy chain constant domain of the human antibody IgA1. The expression vectors differed in the orientation of the promoters and the presence or absence of introns. Two variants of the full-length light and heavy chains were cloned into a eukaryotic expression vector in head-to-head and head-to-tail orientations. The resulting plasmids were transfected into CHO-DG44 and HEK-293T cells. The antibody expression level for the stable transfection of CHO-DG44 and HEK-293T cell cultures was determined by ELISA. The results of the experiments showed that the expression of FI6v3-IgA1 antibodies significantly increased when eukaryotic cells were transfected with the plasmid pBiPr-ABIgA1FI6-Iht in which the heavy chain of IgA1 contains introns and the promoters are arranged head-to-tail.  相似文献   

14.
目的构建含F/2A序列的抗P185^erbB2人鼠嵌合抗体慢病毒表达载体,观察其在293T细胞中的表达。方法用具有自我剪切能力的弗林蛋白酶(Furin)/口蹄疫病毒2A多肽(F/2A)连接人鼠嵌合抗体的重链和轻链,形成一个开放阅读框(ORF),插入慢病毒表达载体pWPI,构建重组抗P185神睨全长人鼠嵌合抗体表达载体pWPI/H-F2A—L。以已构建的慢病毒表达载体pWPI/H-IRES-L为对照质粒。应用磷酸钙沉淀法将慢病毒载体3质粒系统共转染入293T细胞进行包装,测定病毒滴度。再感染293T细胞,荧光显微镜下观察GFP的表达和转染效率,RT—PER、ELISA方法分别检测嵌合抗体mRNA和蛋白的表达。结果经测序鉴定,pWPI/H—F2A—L与预期设计一致;pWPI/H—F2A—L组的病毒滴度为4.3×10^5TU/ml,而pWPI/H—IRES—L组的病毒滴度为3.5×10^5TU/ml;两组重组慢病毒的转染效率分别为87.68%和79.08%;两组重组慢病毒感染293T细胞后,都有嵌合重链和嵌合轻链的表达,由F/2A介导的嵌合抗体的表达水平要高于由IRES介导的嵌合抗体。结论成功构建了含F/2A序列的抗P185^erbB2人鼠嵌合抗体慢病毒表达载体,为今后抗P185^erbB2工程抗体的研究奠定了基础。  相似文献   

15.
Mouse‐human chimeric monoclonal antibodies that could neutralize botulinum neurotoxins were developed and an attempt was made to establish mouse hybridoma cell clones that produced monoclonal antibodies that neutralized botulinum neurotoxin serotype A (BoNT/A). Four clones (2–4, 2–5, 9–4 and B1) were selected for chimerization on the basis of their neutralizing activity against BoNT/A and the cDNA of the variable regions of their heavy (VH) and light chains (VL) were fused with the upstream regions of the constant counterparts of human kappa light and gamma 1 heavy chain genes, respectively. CHO‐DG44 cells were transfected with these plasmids and mouse‐human chimeric antibodies (AC24, AC25, AC94 and ACB1) purified to examine their binding and neutralizing activities. Each chimeric antibody exhibited almost the same capability as each parent mouse mAb to bind and neutralize activities against BoNT/A. From the chimeric antibodies against BoNT/A, shuffling chimeric antibodies designed with replacement of their VH or VL domains were constructed. A shuffling antibody (AC2494) that derived its VH and VL domains from chimeric antibodies AC24 and AC94, respectively, showed much higher neutralizing activity than did other shuffling antibodies and parent counterparts. This result indicates that it is possible to build high‐potency neutralizing chimeric antibodies by selecting and shuffling VH and VL domains from a variety of repertoires. A shuffling chimeric antibody might be the best candidate for replacing horse antitoxin for inducing passive immunotherapy against botulism.  相似文献   

16.
为构建和表达抗人CD3单链抗体 (scFv) 人p5 3四聚功能域融合基因 ,选用人IgG3上游铰链区作为抗人CD3scFv和人p5 3四聚功能域之间连接的linker .利用递归PCR法扩增人IgG3上游铰链区与人p5 3四聚功能域融合基因 ,克隆入pUC18载体中构建pUC18 IgG3 p5 3克隆载体 .将抗人CD3scFv克隆入pUC18 IgG3 p5 3载体中 ,构建抗人CD3scFv 人p5 3四聚功能域融合基因 .经酶切鉴定及序列测定证实后 ,将融合基因克隆入真核表达载体pSecTag2 B中 ,转染HeLa细胞进行表达 ,表达产物纯化后利用流式细胞仪进行亲和活性测定 .获得了抗人CD3scFv 人p5 3四聚功能域融合基因 ,基因全长 882bp ,可编码 2 94个氨基酸 ,与已发表的抗人CD3scFv、人IgG3上游铰链区和人p5 3四聚功能域基因cDNA序列一致 .表达产物经SDS PAGE和Western印迹实验证实为约 35kD的特异蛋白条带 ,纯化后经流式细胞仪检测可以特异性地结合人外周血单个核细胞 (PBMC)细胞 ,亲和力高于scFv ,为进一步临床应用奠定基础  相似文献   

17.
我们采用RT-PCR,从小鼠杂交瘤细胞中扩增并克隆了抗破伤风类毒素(TT)抗体轻、重链可变区,重链Fd区基因,测定了其VH、Vk序列。并在大肠杆菌中表达了Fd片段,ELISA分析的结果表明Fd片段具有抗原结合的能力,但特异性很差。进一步采用SOE,和PCR技术,将VH、VK基因与ScFv连接片段组装成单链抗体(ScFv)基因片段,以及将人重链CH1和Fab基因连接片段组装成Fab基因片段。将它们分别插入含噬菌体fd外壳蛋白3基因的phagem-id pHEN 1中,在辅助噬菌体M 13-VCS作用下,噬菌体表面表达了抗TT的噬菌体单链抗体(phage-ScFv)与噬菌体Fab(phage-Fab),经ELISA检测,表明它们都能与TT特异结合。  相似文献   

18.
家蚕细胞和虫体产生抗人小细胞肺癌抗体   总被引:1,自引:0,他引:1  
用重组昆虫病毒表达系统,在家蚕细胞和虫体表达了抗人小细胞肺癌人-鼠嵌合抗体。重组病毒rNPVL2,rNPVH17及双重组病毒rNPVLH19感染的家蚕细胞和虫体血淋巴中都检测到抗体分子的表达。双重组病毒的双基因共表达部分产物可装配。ELISA分析表明抗体重轻链基因共表达产物具有比单基因表达产物高得多的与小细胞肺癌细胞免疫结合功能。  相似文献   

19.
  相似文献   

20.
G3(3) is a novel murine monoclonal antibody directed against the CD3 antigen of human T lymphocytes which could be used to analyze lymphoid malignancies. We have produced and characterized a recombinant colorimetric immunoconjugate with the antigen-binding specificity of antibody G3(3). A gene encoding a single-chain antibody variable fragment (scFv) was assembled using the original hybridoma cells as a source of antibody variable heavy (VH) and variable light (VL) chain genes. The chimeric gene was introduced into a prokaryotic expression vector in order to produce a soluble scFv fused to bacterial alkaline phosphatase. DNA sequencing and Western blotting analyses demonstrated the integrity of the soluble immunoconjugate recovered from induced recombinant bacteria. The scFv/AP protein was bifunctional and similar in immunoreactivity to the parent G3(3) antibody. Flow cytometry and immunostaining experiments confirmed that the activity of the scFv/AP protein compares favourably with that of the parent antibody. The scFv/AP conjugate was bound to CD3 antigen at the surface of T cells and was directly detected by its enzymatic activity. Thus this novel fusion protein has potential applications as an immunodiagnostic reagent.  相似文献   

设为首页 | 免责声明 | 关于勤云 | 加入收藏

Copyright©北京勤云科技发展有限公司  京ICP备09084417号