抗胃癌鼠单抗3Gg轻链可变区基因的克隆和序列分析

本文报导了用ＰＣＲ方法（Ｐｏｌｙｍｅｒａｓｅ Ｃｈａｉｎ Ｒｅａｃｔｉｏｎ）从抗胃癌单抗３Ｇｇ杂交瘤细胞的基因组ＤＮＡ中,扩增出３３３ｂｐ的轻链可变区基因,克隆至ｐＢｌｕｅｓｃｒｉｐｔ Ⅱｋｓ ＋／－载体上,筛选到阳性克隆。核苷酸序列分析表明：有５３％的核苷酸序列与抗体基因库中的一般序列相符。证明已获得抗胃癌单抗轻链可变区基因。     

抗D－双聚体单抗轻链可变区基因的克隆

以分泌小鼠抗人纤维蛋白降解产物D－双聚体单克隆抗体杂交瘤细胞株的mRNA为模板,用小鼠免疫球蛋白轻链可变区基因的通用引物,通过RT－PCR扩增基因,与载体重组后,经酶切鉴定和核苷酸序列分析,证明克隆含抗D－双聚体单抗的轻链可变区基因,长度为330 bp．     

抗人CD3单抗重、轻链可变区基因的体外扩增、克隆和序列分析

根据免疫球蛋白重链和轻链可变区基因５’端序列和Ｊ区序列,化学合成适合于体外扩增抗体重、轻链可变区基因的二对引物。从体外培养的ＯＫＴ３杂交瘤细胞中提取总ＲＮＡ,反转录生成ｃＤＮＡ,以ｃＤＮＡ为模板,分别加入合成的重、轻链可变区引物进行ＰＣＲ,扩增出抗体重、轻链可变区基因片段。将扩增产物分别插入ｐＵＣ１９质粒,筛选出阳性克隆,用链终止法进行ＤＮＡ序列测定。所测重链可变区基因全长３５７ｂｐ,编码１１９个氨基酸,轻链可变区基因全长３２１ｂｐ,编码１０７个氨基酸。     

抗人CD3单抗重,轻链可变区基因的体外扩增,克隆和序列分析

根据免疫球蛋白重链和轻链可变区基因５＇端序列和Ｊ区序列,化学合成适合于体外扩增抗体重、轻链可变区基因的二对引物。从体外培养的ＯＫＴ３杂交瘤细胞中提取总ＲＮＡ,反转录生成ｃＤＮＡ,以ｃＤＮＡ为模板,分别加入合成的重、轻链可变区引物进行ＰＣＲ,扩增出抗体重、轻链可变区基因片段。将扩增产物分别插入ｐＵＣ１９质粒,筛选出阳性克隆,用链终止法进行ＤＮＡ序列测定。所测重链可变区基因全长３５７ｂｐ,编码１１９个     

抗HFRSV人单抗可变区基因克隆及其序列测定

从杂交瘤细胞株87—2提取细胞总RNA．反转录合成cDNA链,进行PCR反应。其中扩增重链可变区一对引物分别与人免疫球蛋白重链v区基因5＇端和J区基因3＇端互补;扩增人λ轻链可变区引物与人免疫球蛋白λ轻链v区基因5＇端和J区基因3＇端互补。将重、轻链可变区基因的PCR扩增产物分别插入M13噬菌体．经转化筛选分别获得重组克隆。双脱氧法测定其序列,所得核苷酸序列经计算机分析,轻、重链可变区基因长度分别为309bp和405pb,编码103个氨基酸和135个氨基酸,有明显抗体可变区特征,具有骨架区和抗原互补区。     

鼠抗HFRSV衣壳蛋白McAb F3株可变区基因的获取及特性分析

培养鼠抗肾综合征出血热病毒衣壳蛋白Ｆ３杂交瘤细胞株,提取总ＲＮＡ,根据鼠源ＩｇＧ抗体基因家族可变区基因碱基序列的特点,设计简并引物,通过逆转录聚合酶链反应,获得抗体轻链可变区和重链可变区基因。分别将其克隆入载体ＰＴ７ＢｌｕｅＴ Ｖｅｃｔｏｒ,选取阳性重组克隆各两个,分别测定了所载重链可变区和轻链可变区基因的碱基序列,比较了不同克隆轻链可变区基因之间和重链可变区基因之间碱基序列的差异;分析了各自的氨基酸框架及其对应蛋白的亲水性。结果显示,两个重链可变区基因碱基序列有４处不同,同源性为９７９％;其中重组克隆ＺＧ３６４ ５Ｆ所载重链可变区基因有完整的开放阅读框架,对应的蛋白含有丰富的亲水基因,第１１２氨基酸处亲水性最高;另一重组克隆ＺＧ３６４ ４Ｆ所载重链可变区基因不能通读。两个轻链基因碱基序列有４处不同,同源性为９９１％,重组克隆ＺＧ３６５ ５Ｆ和ＺＧ３６５ ７Ｆ所载轻链可变区基因均有完整的开放阅读框架,对应的蛋白均含有丰富的亲水基因,ＺＧ３６５ ５Ｆ所载基因对应蛋白第６７氨基酸亲水性最高,ＺＧ３６５ ７Ｆ所载基因对应蛋白第３４氨基酸亲水性最高。     

抗甜菜坏死黄脉病毒单链抗体表达载体的构建及其表达

用ＰＣＲ方法以分泌抗甜菜坏死黄脉病毒（ＢＮＹＶＶ）单克隆抗体的杂交瘤细胞的基因组为模板,扩增了编码ＢＮＹＶＶ单抗的重链可变区（ＶＨ）基因。测序表明,该ＶＨ序列属于小鼠ＩＩ（Ａ）亚类,全长为３６０ｂｐ,编码１２０个氨基酸。将其和先前克隆的轻链基因分别插入到一个含有连接ＶＨ和ＶＬ基因的连接序列的质粒之中,构建成单链抗体（ｓｃＦｖ）基因的表达载体ｐＴＣｓｃＦｖ。将质粒在大肠杆菌中表达,ＥＬＩＳＡ法检测出     

抗人CD8单抗κ轻链可变区基因的克隆和序列测定

OK T8杂交瘤细胞株从American typecuhure collection(ATCC)获得,产生抗人CD8分子的单克隆抗体IgG2a(γ2a,κ),为了对这一鼠源性单抗进行基因工程改造,我们首先克隆了该单抗的κ轻链可变区基因,并测定了其碱基序列,现将结果报道如下: 通过计算机查找并分析了已发表的几十株抗体的轻链可变区基因序列,经比较其5’端保守序列和J区序列,设计了一对DNA引物:GTGAATTCATGGACATCCAGATGACCCA-     

甲型H1N1流感病毒血凝素单克隆抗体轻链和重链可变区基因的巢式PCR扩增及序列分析

目的：采用巢式PCR对甲型H1N1流感病毒血凝素单克隆抗体的轻链和重链基因进行扩增,对获得的基因进行序列分析,并找出克隆鼠Igκ轻链和重链可变区基因的通用方法。方法：设计22对扩增鼠Igκ轻链可变区和重链可变区基因的引物,对6株鼠抗人甲型H1N1流感病毒血凝素单克隆抗体的轻链和重链可变区基因进行克隆并测序,与NCBI公布的鼠免疫球蛋白序列比对分析。结果：巢式PCR方法可以有效避免单克隆抗体克隆过程的假基因,并且得到的单克隆抗体的氨基酸序列均符合鼠免疫球蛋白可变区特征。结论：建立了克隆鼠免疫球蛋白轻链和重链可变区基因的通用方法,为后期克隆鼠源性单克隆抗体的可变区基因提供了基础,并为研究甲型H1N1流感病毒血凝素与抗体的结合位点提供了实验数据。     

一株乙酰胆碱受体单克隆抗体的序列分析

探讨重症肌无力自身抗体分子结构及其在发病机制中的作用。利用PCR从分泌乙酰胆碱受体（AChR）单抗A49的杂交瘤细胞株扩增抗体可变区（V）基因,经转化大肠杆菌DH5α克隆后,进行核苷酸序列分析。A49的重性V区基因由小鼠VHNP族基因编码,轻链V区基因由小鼠VK2组基因编码。与致病性AChR抗体V区比较,其同源性均在70％以下。A49的分子结构与致病性AChR抗体不同。     

Germ line maintenance of the pseudogene donor pool for somatic immunoglobulin gene conversion in chickens.

Somatic immunoglobulin diversity is generated in avian species by sequential gene conversion of variable (V) gene segments of the immunoglobulin heavy- and light-chain loci during B-cell development. The germ line pools of donor sequence information for somatic V-region gene conversion are found in families of V pseudogenes, located 5' of the single functional V gene of each locus. The sequence relationships among the pseudogenes (psi VL) and functional VL1 gene of the chicken light-chain alleles in three inbred strains were compared to determine the extent of diversity within the germ line pseudogene cluster. Numerous differences were observed. For example, compared with the previously reported CB allele and the G4 allele, the S3 allele contains two intact pseudogenes between psi VL16 and psi VL18. These two adjacent psi VL gene segments (psi VL17a and psi VL17b) could have given rise to the psi VL17 segment of the G4 and CB alleles by homologous recombination. The majority of other sequence polymorphisms among the psi VL alleles appear to be the result of meiotic gene conversion. The incidence of untemplated mutations within psi VL segments is significantly lower than the incidence of mutation within the pseudogene flanking regions. Together with the observations that most psi VL segments have open reading frames and lack stop codons, these data support the hypothesis that the psi VL cluster resembles a functional multigene family maintained by evolutionary selection for its functional role in generating somatic antibody diversity. Meiotic gene conversion events within the psi VL cluster serve both to introduce diversity by the exchange of short segments between family members and to prevent the accumulation of random mutations.     

Rates of lipogenesis and plasma insulin concentrations in inbred lines of mice differing in fatness

Rates of lipogenesis de novo and plasma concentrations of insulin were compared during post-natal growth in two inbred lines of mice (VL/fDk (VL) and SWR/fNIMR (SWR] in which differences in growth and fatness are probably due to multiple not single gene effects. Irrespective of sex, the lipogenic rate/g was higher in the fatter VL mice in the liver and all other tissues except the head, where it was lower, and the gonadal fat pad, where it was not different. Adult mice in general had lower lipogenic rates than those measured soon after weaning. In both lines the lipogenic rate/g of tissue was higher in males in the liver and in females in the gonadal fat pad. Plasma insulin concentrations were higher in VL mice and tended to rise with age. These results demonstrate that metabolic differences associated with differences in fatness in inbred lines of mice in which fatness is controlled by more than one gene, are qualitatively but not quantitatively similar to those observed by other workers in lines of mice differing in fatness due to a single gene mutation.     

Cloning and Sequencing of VL Gene of Monoclonal Antibody Against Beet Necrotic Yellow Vein Virus

The results showed that PCR product was 318 bp VL gene of monoclonal antibody against beet necrotic yellow vein virus, code 106 amino acids. VL gene belongs to a k chain subclass Ⅱ of mouse, frame region had 85 % homogenous with the published sequencing of VL gene of mouse and was in accord with structural characteristics of VL of mouse.     

狂犬病人源二硫键稳定单链抗体融合蛋白的构建及活性检测

【目的】构建、表达人源二硫键稳定单链抗体(scdsFv),检测其生物活性,以获得对狂犬病病毒有特异结合能力及中和活性的scdsFv蛋白。【方法】从GenBank上获得RV单抗SO57重链可变区VH和轻链可变区VL序列,在VH44和VL100位各突变一个氨基酸为半胱氨酸,用linker连接形成scdsFv,人工合成此序列,克隆入表达载体pET22b(+),在大肠杆菌中表达目的蛋白,镍柱亲和层析法纯化,并进行SDS-PAGE、Westernblot鉴定。ELISA法和鼠脑组织抹片方法检测scdsFv对RV的特异结合活性;硫氰酸盐洗脱法测定scdsFv蛋白对RV的相对亲和力指数;分别用荧光抗体病毒中和试验(FAVN)和小鼠体内中和试验测定scdsFv的体外和体内中和活性。【结果】成功获得RV人源二硫键稳定单链抗体序列,大肠杆菌中表达得到scdsFv蛋白;分子量约为30.0kDa,Western blot表明此蛋白能与抗His单克隆抗体发生特异性反应。scdsFv能与RVVero疫苗特异结合,且结合力随抗原浓度降低而降低;scdsFv能与鼠脑组织中的RV结合。FAVN法测得scdsFv的中和效价为41IU/mL;小鼠体内中和试验表明scdsFv能保护55.6%鼠耐过强毒攻击。【结论】获得的scdsFv,具有良好的RV结合活性和体内外中和活性,有可能被用于暴露后狂犬病的预防。     

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。     

Analyses of chicken immunoglobulin light chain cDNA clones indicate a few germline V lambda genes and allotypes of the C lambda locus.

cDNA libraries of chicken spleen and Harder gland (a gland enriched with immunocytes) constructed in pBR322 were screened by differential hybridization and by mRNA hybrid-selected translation. Eleven L-chain cDNA clones were identified from which VL probes were prepared and each was annealed with kidney DNA restriction digests. All VL probes revealed the same set of bands, corresponding to about 15 germline VL genes of one subgroup. The nucleotide sequences of six VL clones showed greater than or equal to 85% homology, and the predicted amino acid sequences were identical or nearly identical to the major N-terminal sequence of L-chains in chicken serum. These findings, and the fact that the VL clones were randomly selected from normal lymphoid tissues, strongly indicate that the bulk of chicken L-chains is encoded by a few germline VL genes, probably much less than 15 since many of the VL genes are known to be pseudogenes. Therefore, it is likely that somatic mechanisms operating prior to specific triggering by antigen play a major role in the generation of antibody diversity in chicken. Analysis of the constant region locus (sequencing of CL gene and cDNAs) demonstrate a single CL isotype and suggest the presence of CL allotypes.     

'Solo' large terminal repeats (LTR) of an endogenous retrovirus-like gene family (VL30) in the mouse genome.

VL30 genetic elements constitute a murine multicopy gene family that is retrovirus-like, despite the lack of sequence homology with any known retrovirus. Over one hundred copies of VL30 units are dispersed throughout the mouse genome. We report here that the mouse genome also contains 'solo' VL30 long terminal repeats (LTRs). These are structures which contain the LTR detached from the rest of the VL30 sequences. The isolation of solo LTRs from a mouse embryonic gene library with the aid of sub-genomic VL30 probes is described. Direct DNA sequencing established that the solo LTR unit is grossly similar to a standard VL30 LTR and that the LTR is flanked by a 4-base pair duplication. The analogy to the occurrence of solitary LTR units of transposable elements is discussed.     

Coevolution of immunoglobulin heavy- and light-chain variable-region gene families

The gene families encoding the immunoglobulin variable regions of heavy (VH) and light (VL) chains in vertebrates are composed of many genes. However, the gene number and the extent of diversity among VH and VL gene copies vary with species. To examine the causes of this variation and the evolutionary forces for these multigene families, we conducted a phylogenetic analysis of VH and VL genes from the species of amniotes. The results of our analysis showed that for each species, VH and VL genes have the same pattern of clustering in the trees, and, according to this clustering pattern, the species can be divided into two groups. In the first group of species (humans and mice), VH and VL genes were extensively intermingled with genes from other organisms; in the second group of species (chickens, rabbits, cattle, sheep, swine, and horses), the genes tended to form clusters within the same group of organisms. These results suggest that the VH and VL multigene families have evolved in the same fashion: they have undergone coordinated contraction and expansion of gene repertoires such that each group of organisms is characterized by a certain level of diversity of VH and VL genes. The extent of diversity among copies of VH and VL genes in each species is related to the mechanism of generation of antibody variety. In humans and mice, DNA rearrangement of immunoglobulin variable, diversity, and joining-segment genes is a main source of antibody diversity, whereas in chickens, rabbits, cattle, sheep, swine, and horses, somatic hypermutation and somatic gene conversion play important roles. The evolutionary pattern of VH and VL multigene families is consistent with the birth-and-death model of evolution, yet different levels of diversifying selection seem to operate in the VH and VL genes of these two groups of species.      

Diverse long terminal repeats are associated with murine retroviruslike (VL30) elements.

The VL30 family is a retroviruslike gene family with no apparent nucleic acid homology to any known retrovirus. Over 100 copies of VL30 DNA elements are dispersed throughout the mouse genome. Sequence analysis of the VL30 long terminal repeat (LTR) units showed that, whereas the LTR units of a given VL30 DNA element were almost identical, the LTR units associated with distinct members of the family were very different from one another. Comparison of the LTR sequences possessed by two particular VL30 DNA elements revealed a pattern of extensively homologous DNA segments adjacent to only distantly related DNA sequences. With the aid of sub-LTR probes, it was shown that a certain LTR is composed of both U5 sequences that are abundantly present in all species of the genus Mus and a U3 region detected only in Mus musculus. In addition, we isolated a VL30 DNA element in which the LTR units were replaced by the LTR units of an apparently novel retroviruslike family. These findings suggest that recombinations have played a role in generating the diverse population of VL30-associated LTRs.