表达抗α毒素单链抗体基因工程菌株的构建

将 2种抗A型产气荚膜梭菌α毒素单链抗体 (ScFv)基因ScFv 2E3和ScFv 1A8分别克隆至表达质粒pUC119,pET 2 0b ,pET 2 8a和pHOG2 1中 ,构建了重组质粒 ,分别转化至相应的受体菌JM10 5 ,BL2 1(DE3)和XL1 BLUE中 ,得到表达ScFv的重组菌株。ELISA和SDS PAGE分析检测表明 :经IPTG诱导后所表达的ScFv目的蛋白主要形成了包含体的形式 ,但也有少量ScFv存在于重组菌株的培养上清和胞周质中。经薄层扫描分析 :重组菌株XL1 BLUE (pHOG 2E3)的蛋白表达产物分别占菌体可溶性蛋白的 4% ,重组菌株XL1 BLUE (pHOG 2E3)的蛋白表达产物占菌体总蛋白的相对含量为 2 2 % ,其相对分子量约为 31ku。表达的ScFv蛋白不但具有中和卵磷脂酶的活性 ,而且能够对致死性腹腔攻击α毒素的小鼠产生良好的被动保护作用     

抗A型产气荚膜梭菌α毒素单链抗体基因的克隆和表达

应用RT PCR技术 ,从分泌具有中和活性的抗A型产气荚膜梭菌α毒素单克隆抗体的杂交瘤细胞中 ,扩增出抗体V_H 和V_L 基因 ,连接成ScFv基因 ,并将其克隆至pGEM T载体中构建了重组质粒pXScFv 2E3。经序列分析证实 ,V_H 和V_L 基因及linker基因拼接正确 ,基因全长为 726bp ,编码 242个氨基酸。随后将其定向克隆于表达载体pHOG21,转化至大肠杆菌XL1 BLUE筛选出表达菌株XL1 BLUE(pHOG 2E3)。经ELISA和SDS PAGE分析表明 ,在20℃用IPTG诱导培养时 ,表达的ScFv蛋白占菌体总蛋白的 25 %。并且ScFv基因表达产物能够中和α毒素的磷酯酶C活性     

不同培养条件对抗a毒素ScFv基因表达的影响

将ScFv基因片段与pHOG21载体连接后,转化至受体菌XL1-Blue中,得到重组菌株XL1-Blue（pHOG2E3）。随后研究了培养基中无机盐成分、温度、诱导时间、IPTG和蔗糖浓度对SvFv基因表达的影响。经SDS-PAGE分析表明,重组菌株XL1-Blue(pHOG2E3）在LB培养基中加入0.5mmol/L IPTG和0.4mol/L蔗糖。37℃诱导6h,其目的蛋白 表达量较高,表达的ScFv蛋白主要以包含体的形式存在,分子量在31,000D,在重组菌株的培养上清和菌体裂解上清液中,通过ELISA法也检测到了ScFv的存在,且具有中和a毒素的活性。     

不同培养条件对抗α毒素ScFv基因表达的影响

将ScFv基因片段与pHOG21载体连接后,转化至受体菌XL1-Blue中,得到重组菌株XL1-Blue（pHOG2E3）。随后研究了培养基中无机盐成分、温度、诱导时间、IPTG和蔗糖浓度对ScFv基因表达的影响。经SDS-PAGE分析表明,重组菌株XL1-Blue（pHOG2E3）在LB培养基中加入0.5mmol/L IPTG和 0.4 mol/L蔗糖,37℃诱导6h,其目的蛋白的表达量较高,表达的ScFv蛋白主要以包含体的形式存在,分子量为31,000D,在重组菌株的培养上清和菌体裂解上清液中,通过E     

表达抗α毒素单链缺本基因工程菌株的构建

将2种抗A型产气荚膜梭菌α毒素单链抗体（ScFv)基因ScFv-2E3和ScFv-1A8分别克隆至表达质粒pUC119,pET-20b,pET-28a和pHOC21中,构建了重组质粒,分别转化至相应的受体菌JM105,BL21（DE3）和XL1-BLUE中,得到表达ScFv的重组菌株,ELISA和SDS-PAGE分析检测表明：经IPTG诱导后所表达的ScFv目的蛋白主要形成了包含体的形式,但也有少量ScFv存在于重组菌株的培养上清和胞周质中,经薄层扫描分析;重组菌株XL1-BLUE（pHOG-2E3)的蛋白表达产物分别占菌体可溶性蛋白的4%,重组菌株XL1-BLUE（pHOG-2E3)的蛋白表达产物占菌体总蛋白的相对含量为22%,其相对分子量约为31ku。表达的ScFv蛋白不但具有中和卵磷脂酶的活性,而且能够对致死性腹腔攻击α毒素的小鼠产生良好的被动保护作用。     

抗TNF-α单链抗体的表达及其纯化

克隆抗人肿瘤坏死因子(TNF-α)鼠源单抗的可变区基因以构建其单链抗体(ScFv)表达载体,实现在大肠杆菌的表达,并进行ScFv的可溶性纯化与鉴定。采用RT-PCR技术,以前导肽序列的引物从1个分泌抗人TNF-α的鼠单抗杂交瘤细胞系中克隆抗体轻链、重链可变区基因(VL,VH),构建ScFv基因,将ScFv基因片段与pGEX-4T-1表达载体连接,在大肠杆菌中表达并采用十二烷基肌氨酸钠(Sarkosyl)进行可溶性纯化,最后鉴定其生物活性。结果显示,得到了功能性重排的轻、重链可变区基因,分别构建了VH和VL不同连接顺序的HLL(VH-Linker-VL)和LLH(VL-Linker-VH)两种ScFv,LLH的表达量较HLL的高,但亲和力不及HLL。采用Sarkosyl溶解包涵体,对目的蛋白进行可溶性纯化,蛋白纯度达到90%,纯化后的蛋白经ELISA和WB证明ScFv维持了亲本抗体与TNF-α特异性结合的能力,且具有细胞毒中和活性。实验中研究探索了一种新颖的,操作简单,省时的裂解、纯化方案,实现了单链抗体经原核系统的表达后得以可溶性纯化。     

抗乙型肝炎表面抗原单链抗体(ScFv)的原核表达、纯化及鉴定

从抗HBsAg鼠单抗的杂交瘤细胞提取RNA,经反转录得到cDNA,进一步扩增得到鼠重链可变区基因(VH)和轻链可变区基因(VL),按VH-linker-VL的结构将VH、VL基因拼接成单链抗体(scFv)基因;经测序正确后进一步构建了表达重组体p26HBSc并在E.coli中表达,得到一约30kD的外源蛋白;纯化后经ELISA检测与HBsAg有较高的亲和力活性,为下一步的人源化改造奠定了基础。     

Ⅱ型志贺毒素单克隆抗体可变区基因克隆及单链抗体的表达和功能鉴定

目的从分泌抗肠出血性大肠埃希菌Ⅱ型志贺毒素中和单克隆抗体杂交瘤细胞株S2C4中克隆抗体可变区基因,构建单链抗体（ScFv）,进行原核表达,并对其功能进行鉴定。方法从杂交瘤细胞株S2C4中提取总RNA,逆转录成cDNA。在cDNA3’-OH末端添加poly．G。PCR扩增包括5’非翻译区和信号肽序列在内的抗体重、轻链可变区基因VH和VL,PCR产物装入T—A载体测序。根据测序结果,设计引物分别扩增VH和VL编码区,再通过重叠PCR,在VH和VL．编码区基因之间引入连接链,构建Scn基因,并克隆到表达载体pComb3xSS中。重组载体导入E．coliTop10F’进行表达,重组蛋白经纯化后,分别用ELISA和动物保护性实验鉴定其生物学活性。结果VH和VL编码区基因全长分别为396bp和378bp,ScFv基因能在大肠埃希菌中高效表达,表达产物的分子量为34000,用NiSO4亲和层析柱成功纯化。功能性实验表明纯化的重组蛋白可以与Stx2毒素有效结合,能保护动物抵御毒素分子的攻击。结论成功地克隆S2C4单抗可变区基因,并构建、表达其单链抗体ScFv,为下一步进行该抗体人源化奠定实验基础。     

抗犬细小病毒VP2蛋白单链抗体的制备与中和活性研究

为了减轻鼠源单克隆抗体(McAb)异源性引起的宿主免疫排斥反应,同时克服生产McAb成本高及费时费力等缺点,利用原核表达制备具有抗犬细小病毒(CPV)鼠源抗体可变区基因的单链抗体(single chain antibody fragment,ScFv)。提取实验室前期制备筛选的分泌具有良好中和活性抗CPV VP2蛋白McAb的杂交瘤细胞株总RNA,从反转录cDNA中扩增抗体重链可变区(VH)基因和轻链可变区(VL)基因并克隆到表达载体中,构建重组质粒p OPE101-ScFv;将重组质粒转化大肠杆菌进行诱导表达,通过蛋白免疫印迹(Western blot)实验、酶联免疫吸附试验(enzyme linked immunosorbent assay,ELISA)和间接免疫荧光试验(indirect immunofluorescence assay,IFA)证明,利用大肠杆菌表达系统获得的ScFv具有和CPV特异性结合的能力,且具有中和活性,效价为1:20(0. 028μg/ml),为CPV的临床免疫治疗提供基础。     

抗肠炎沙门氏菌单链抗体制备及其特异性分析

目的:利用基因工程技术制备抗肠炎沙门氏菌的单链抗体.方法:从抗肠炎沙门氏菌单克隆抗体的杂交瘤细胞中纯化RNA,反转录后扩增出抗体的重链可变区(VH)和轻链可变区(VL)基因片段,采用重叠延伸的方法,用柔性多肽Linker接头(Gly4 Ser)3按VL-Linker-VH方式将VH基因和VL基因拼接成单链抗体基因片段后,连接到pGEX-4T-1载体上,进行重组转化.挑取阳性克隆,经IPTG诱导后,通过GST柱进行亲和层析,最后利用ELISA检测抗体的活性.结果:成功构建了表达抗肠炎沙门氏菌单链抗体的基因工程菌株,经SDS-PAGE和ELISA检测结果表明,诱导表达的单链抗体scFv分子量约为60 kDa,其能特异与肠炎沙门氏菌结合,但与副甲伤寒沙门氏菌、鸭沙门氏菌、鼠伤寒沙门氏菌有轻度交叉反应.结论:成功构建了抗肠炎沙门氏菌单链抗体的表达菌株,表达的单链抗体scFv可作为沙门氏菌的检测的候选抗体分子.     

抗破伤风类毒素单抗可变区基因的克隆及在大肠杆菌中表达的三种工程抗体

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。     

抗破伤风类毒素单抗可变区基因的克隆及在大肠杆菌中表达的三种工程抗体

The heavy and light chain variable region genes of anti-tetanus toxoid (TT) antibody and the heavy chain Fd genes were amplified and cloned through RT-PCR from mouse hybridoma cells. The sequences of VH and VK were determined. Fd gene fragments were expressed in E. coli. The ELISA results indicated that the expressed Fd showed antigen binding activity but was nonspecific. Furthermore, through SOE and PCR techniques, the VH and VK gene fragments together with ScFv linker were assembled into single chain antibody (ScFv) gene fragment. While together with human heavy chain CH 1 gene fragment and Fab linker, they were assembled into chimeric Fab gene fragment. The two assembled gene fragments were separately inserted into phagemid pHEN 1, which was a fd-based vector containing gene 3 encoding the minor coat protein. In presence of helper phage M 13-VCS the anti-TT phage-ScFv or phage-Fab were displayed on the surface of phage particles respectively. Results from phage-ELISA indicated that both phage antibodies were TT-specific.     

Cloning and complete nucleotide sequence of mouse immunoglobulin gamma 1 chain gene.

The 6.6 kb DNA fragment coding for the immunoglobulin γ1 chain was cloned from newborn mouse DNA using λgtWES·λB as the EK2 vector. The complete nucleotide sequence (1823 bases) of the γ1 chain gene was determined. The cloned gene contained the entire constant region gene sequence as well as the poly(A) addition site, but not the variable region gene. The results indicate that the variable and constant region genes of immunoglobulin heavy chain are separated in newborn mouse DNA. The constant region genes of other gamma chains (that is, γ2a, γ2b and γ3) are not present in the cloned DNA fragment. The sequence demonstrates that the γ1 chain gene is interrupted by three intervening sequences at the junction of the domains and the hinge region, as previously shown in the γ2b and α chain genes and in the γ1 chain gene cloned from myeloma. The results suggest that the intervening sequence was introduced into the heavy chain gene before divergence of the heavy chain classes, and also support the hypothesis that the splicing mechanism has facilitated the evolution of eucaryotic genes by linking duplicated domains or prototype peptides not directly adjacent to one another. Comparison of the nucleotide sequence of the γ1 chain gene around the boundaries of the coding and intervening sequences with those of other mouse genes revealed extensive divergence, although short prevalent sequences of AG-GTCAG at the 5′ border of the intervening sequence and TCTGCAG-GC at the 3′ border were deduced. A limited homology of nucleotide sequences was found among domains and between the hinge region and the 5′ portion of the CH2 domain. Comparison of 3′ untranslated sequences from the γ1 and γ2b chain genes and the mouse major β-globin gene shows significant homology and a palindrome sequence surrounding the poly(A) addition site.     

Evolution of human immunoglobulin kappa J region genes

Immunoglobulin kappa chain variable region genes are assembled from two discontinuous DNA segments, a V and a J gene. The J region genes, in addition to encoding amino acid positions 96-108 of the kappa polypeptide chain, also provide sequences required for both DNA and RNA splicing reactions. For purposes of evolutionary comparison and to establish the complexity of the kappa J region locus in man, we have determined an approximately 3000 basepair nucleotide sequence in a cloned human DNA fragment that encodes the germline distinct J region segments. Significant blocks of homology have been tightly maintained between this region and an analogous segment of the mouse genome. In particular, the short sequences, GGTTTTTGT and CACTGTG, thought to be involved in V-J recombination, are the most highly conserved regions (97% homology). In addition, from heteroduplex data and computer analysis of the nucleotide sequences, it is clear that the mouse J3 sequence, a pseudogene, is not present in the human cluster. This can be explained by a duplication event in the mouse J region gene cluster that may have been the result of unequal crossing over between homologous chromosomes.     

从噬菌体抗体库中淘选血纤维蛋白特异的单链抗体

为构建小鼠噬菌体抗体库 ,以获得对人血纤维蛋白特异的抗体 ,由小鼠脾脏提取 m RNA,经反转录 PCR扩增出抗体重链、轻链可变区基因片段 ,将二者和一段编码十五肽 (Gly4 Ser) 3的 DNA接头借助重组 PCR组装成为单链抗体 (single- chain antibody,Sc Ab)基因 .将单链抗体基因插入噬菌体展示载体 p CANTAB- 5E,通过电击法转化大肠杆菌 TG1细胞 ,用辅助噬菌体 M1 3K0 7超感染 ,构建了库容量在 1 0 8以上的噬菌体单链抗体库 .利用亲和选择方法 (淘选 ) ,从噬菌体抗体库中选得血纤维蛋白特异的单链抗体 .模拟抗体成熟过程 ,用 DNA改组 (DNA shuffling)技术使抗体基因重新组合 ,构建新的改组抗体库 ,并从中选择到提高了亲和力的噬菌体单链抗体 .抗体基因在大肠杆菌中表达 ,表达蛋白经 Sephadex G- 75柱层析分离 ,得到初步纯化的单链抗体蛋白 .     

鼠源抗HFRSV衣壳蛋白McAbF3株单链抗体基因克隆构建及表达

为了获得原抗ＨＦＲＳＶ衣壳蛋白ＭｃＡｂＦ３＾１株轻链可变区基因,由连接肽体外连接获得单链抗体基因,在大肠杆菌中表达,从鼠源抗ＨＦＲＳＶ衣壳蛋白ＭｃＡｂＦ３株细胞中分离总ＲＮＡ,以ｏｌｉｇｏ（ｄＴ）１８为引物逆转录成ｃＤＮＡ,通过ＰＣＲ扩增出抗体的轻链（ＶＬ）和重链可变区（Ｖ１１）基因,由连接本外连接获得单链抗体（ＳｅＦｖ）基因。将此单链抗体（ＳｅＦｖ）基因插入原核表达载体ＰＥＴ２８ａ,经大肠杆菌（     

抗CD5单链抗体基因克隆和表达

以分泌抗CD5单克隆抗体的杂交瘤细胞poly(A) mRNA为模板,通过RTPCR扩增出抗CD5单克隆抗体的重链可变区(VH)和轻链可变区(VL) cDNA片段组装出抗CD5单链抗体(ScFv) cDNA片段。该ScFv片段被克隆到pCANTAB 5E载体上,以E.coli TG1为宿主,进行噬菌体表面呈现。通过Molt4细胞表面分子CD抗原,对噬菌体表面呈现的ScFv进行免疫亲和富集筛选。经细胞ELISA鉴定,得到4株高亲和力克隆。DNA序列分析得知,单链抗体全长732碱基,其中VH为339碱基,VL为300碱基。抗CD5 ScFv在E.coli HB2151中以可溶形式分泌表达,产物主要分布于周质之中,占周质中总蛋白的20%。     

Single-chain antibody against human lipocalin-type prostaglandin D synthase: Construction, expression, purification, and activity assay

An active form of single-chain antibody (ScFv) from murine monoclonal antibody 4A7, which is specific for lipocalin-type prostaglandin D synthase (L-PGDS), was produced in Escherichia coli. The complementary DNA fragments encoding the variable regions of heavy chain (VH) and light chain (VL), which amplified from hybridoma 4A7 producing a monoclonal antibody (IgG1) against L-PGDS, were connected by a (Gly4Ser)3 linker using an assembly polymerase chain reaction. The resultant ScFv were cloned into the vector pGEM and expressed in E. coli as inclusion bodies. The expressed ScFv fusion proteins were purified by Ni2+-nitrilotriacetic acid chromatography. The purity and activity of purified ScFv were confirmed by SDS-PAGE and ELISA. The result revealed that 4A7 ScFv conserved the same characteristics of specific recognition and binding to sperm as the parental 4A7 monoclonal antibody.     

抗人CD19单链抗体基因的构建、表达及功能测定

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V_H和V_L可变区基因,再通过重叠延伸拼接（spliceoverlap extension）PCR方法在V_H和V_L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。