单克隆抗体夹心斑点免疫金银染色法诊断恶性疟的初步研究

用单克隆抗体(McAb)夹心斑点免疫金银染色法(Dot-IGSSA),对采自海南省的30价原虫血症范围为0.015-0.58％的恶性疟病人血和30份正常人血进行了检测。当用McAb 11G_5、13A_2、13A_1分别与金标记McAb 14D_9夹心时,其阳性检出率分别为96.7％、93.3％和93.3％,假阳性反应约为3.3％,最低可检测出约0.0001％的疟原虫血症。其中11G_5、13A_1分别与金标记14D_9夹心时,对体外培养的云南和安徽的恶性疟红内期抗原呈阳性反应,但其McAb与诺氏疟原虫和伯氏疟原虫均无交叉反应。McAb 13A_1与14D_9夹心时,对食蟹猴疟原虫和间日疟病人感染血中的疟原虫抗原有部分交叉反应。

免疫筛选恶性疟原虫cDNA克隆

目的 :获取恶性疟原虫 (海南株 )抗原的 c DNA克隆并进行初步鉴定。方法 :采用 dot-EL ISA,以兔免疫血清对恶性疟原虫 c DNA表达文库约 80万个重组噬斑进行筛选 ,并用 2 0株单克隆抗体和恶性疟患者血清对强阳性克隆进行再筛选。 PCR初步鉴定 17个强阳性克隆。结果 :兔免疫血清确定了 17个强阳性克隆 ,患者血清检测到 11个阳性克隆 (含 8个强阳性 ) ,11株单抗与 9个 c DNA克隆呈阳性反应。 17个强阳性克隆均能扩增出大小在 30 0 bp- 2 .5kb左右的条带。结论 :已筛选到能与抗恶性疟原虫兔血清、单克隆抗体及患者血清产生特异性免疫反应的 c DNA克隆。

亲本瘤和杂交瘤细胞在无血清培养基内生长特性的动态观察

我们研制了一种适用于瘤细胞长期传代培养、冷冻复苏、克隆化生长和细胞融合的无血清培养基(DMI)。在此基础上,本文进一步报告了亲本瘤和杂交瘤细胞在DMI内的生长特性。6株瘤细胞中,2株生长曲线的迟缓期稍延长,5株对数生长期历时较长,提示DMI尚缺少有益于细胞生长的、存在于小牛血清中的某种或某些因子;6株瘤细胞稳定期显著延长,提示细胞密度达高峰的维持时间较长,有助于分泌较多的单克隆抗体。SP_2/0、P_3U_1、983和13F_3在DMI内的倍增时间长于在含15％小牛血清培养基内的倍增时间,653和32B_5在两种培养基中的倍增时间相近。

用斑点酶联免疫吸附试验筛选抗恶性疟原虫单克隆抗体及检测恶性疟抗原

以往筛选抗恶性疟原虫(Pf)单克隆抗体(McAb)常用间接免疫荧光(IFA)或ELISA,以培养的原虫为检测抗原。所得McAb检测培养的Pf抗原效果较好,但检测病人血中Pf抗原时阳性率较低。抗原分析显示这些McAbs多是针对滋养体、裂殖体或裂殖子抗原。为了得到能用于诊断的抗环状体期McAb,我们直接以病人血中Pf为检测抗原,用斑点酶联免疫吸附试验(DotELISA)进行筛选,结果如下。

抗恶性疟McAb的筛选与恶性疟免疫诊断研究

用单克隆抗体(McAb)夹心斑点免疫金银染色法(Dot-IGSSA)对11株抗恶性疟McAbs和4株抗食蟹猴疟原虫McAbs进行了筛选,其中McAbs11G5、13A2、13A1可包被到硝酸纤维素膜(NcF)上作为捕获抗体,McAb14D9可用于胶体金探针的标记。此外,为增加胶体金的标记效果和胶体金标记McAb14D9探针的敏感性,还对McAb14D9的等电点(pI)进行了测定,其pI为6.35。同时用筛选出的最佳McAbs对10份恶性疟病人感染血和10份健康人血样品进行了检测,并对这几株McAbs的交叉反应性进行了测定,结果表明McAbs11G5、13A1与14D9夹心时,对云南株和安微株恶性疟原虫红内期抗原呈现交叉反应,而且McAb13A1与14D9夹心时还可以用于检测间日疟抗原。

分泌抗包虫囊液抗原McAb杂交瘤细胞株的建立

应用Oriel法制备的包虫囊液抗原经腹腔注入供实验的小鼠,作为脾细胞供体。此脾细胞与不能分泌的骨髓瘤细胞株SP2/0和P3u_1相融合,以生成杂交瘤细胞株。用ELISA法从这些混合细胞培养基中筛选出上清液,用稀释法将上清液克隆,再克隆化之后,生成能分泌单克隆抗体、抗包虫囊液活性的杂交瘤,其染色体数目在80～100范围之内。单克隆抗体类及亚类13Fs和31G_(12)分别是IgG_1和IgA。DD和ELISA用于鉴定它们的敏感性和特异性。应用ELISA法比较杂交瘤和绦虫囊尾蚴液等其它寄生虫抗原制备物,包虫囊液和Pf抗原,表明单克隆抗体对包虫囊寄生虫有很高的特异性。

提高抗恶性疟独特型单抗克隆出现频率的方法学探讨

用Protein A-Sepharose亲和层析法提纯McAb-IgG,皮下多点和腹腔免疫雄性Wistar大鼠,间隔两周共3次,融合前3天采用腹腔、尾静脉和脾内注射等三种加强免疫方法,以间接ELISA法和抗体竞争ELISA法筛选Anti-Id阳性克隆。结果显示:融合前大鼠血清抗小鼠IgG或抗免疫原McAb-IgG滴度,静脉组和脾内组比腹腔组高一个滴度;Anti-Id阳性克隆出现频率,腹腔组为0.9％和0.3％,静脉组为11.0％和13.3％,脾内组为16.4％和12.9％,静脉组和脾内组明显高于腹腔组(P<0.01);上述三种加强免疫方法对抗小鼠IgG阳性克隆出现频率无明显影响(P>0.05);与腹腔加强免疫组相比,静脉和脾内加强免疫组也可提高细胞融合效果(P<0.01).本实验结果提示,腹腔和皮下多点多次长程基础免疫结合静脉或脾内加强免疫是制备Anti-Id McAb比较好的免疫方案。

鼠类亲本瘤细胞体外生长时需要胆固醇

本文在无血清培养条件下,对长期在DMI中传代培养的大鼠亲本瘤细胞系IR983F及小鼠亲本瘤细胞系P3U1和653对胆固醇的需求进行了动态观察。结果显示,胆固醇对这些亲本瘤系体外增殖是绝对必需的,其理想浓度为5—15μg/ml;10μg/ml量的人低密度脂蛋白可完全代替所需的胆固醇。与亲本瘤细胞系相比,长期在DMI中传代培养的杂交瘤细胞和SP2/0癌细胞对胆固醇的需要不十分严格。

抗恶性疟单抗独特型决定簇之第二单克隆抗体的制备和鉴定

以分泌抗恶性疟红内期抗体的小鼠杂交瘤细胞系94D1诱生的腹水,通过Protein A-Sepharose CL-4B亲和层析法纯化IgG,并以此作为免疫原皮下多点免疫Wistar大鼠。加强免疫后3天取脾与小鼠SP^2/0瘤细胞进行异种间的细胞融合,经间接ELISA法检测筛选和5次克隆化,最终得到一株生长稳定、连续分泌特异抗体的异种杂交瘤细胞系41RF5。经过多次冷冻和复苏以及体外连续传代培养16个月,其稳定性与小鼠×小鼠杂交瘤细胞相近。选择8株单抗和SP2/0IgG作为包被抗原,用间接ELISA法对41RF5特异性进行鉴定.结果显示,41RF5单抗只与94D1呈阳性反应,与其余各种包被抗原均呈阴性反应,表明41RF5具有良好的抗94D1单抗独特型决定簇的特异性。41RF5培养上清中特异的抗体效价为1:1280。

长期无血清传代培养瘤细胞的某些生物学特性观察

本文对长期在无血清培养基内传代培养的亲本瘤和杂交瘤细胞的某些生物学特性进行了监测。结果显示,长期(三个月以上)在DMI传代的瘤细胞,贴壁能力明显减弱,个别瘤系完全呈悬浮型生长,但重新置回含血清常规培养基培养,贴壁能力大部分可恢复到原来状态:诱发BALB/c小鼠腹水和皮下实体瘤的能力保持不变;在HAT选择培养基中培养,瘤细胞的死亡时间在DMI和RPS15对照两种培养基内基本一致;4个亲本瘤系8-氮鸟嘌呤筛选结果与含血清培养的瘤细胞相似;经DMI长期传代的杂交瘤系分泌抗体的能力基本保持不变。

恶性疟原虫免疫学特性与免疫诊断研究

本项研究是采用免疫学方法把流行区不同年龄不同感染者人群的免疫血清与体外长期传代培养的恶性疟原虫抗原进行免疫反应,以评价和探讨用体外长期培养的疟原虫免疫的BALB/C小鼠脾细胞与小鼠骨髓瘤细胞融合,克隆后所产生的单克隆抗体检测自然虫株感染的病人血中疟疾抗原的可能性,并通过改进免疫学诊断方法达到现场应用的效果。其主要研究结果如下:

适用于亲本瘤细胞和杂交瘤细胞生长的无血清培养基

以RPMI1640和DMEM-F12按1:1混合组成基础培养基(BM),再添加胰岛素等12种因子制成一种无血清培养基(SFM)。SP2/0等多种亲本瘤细胞以及异种、同种杂交瘤细胞均能在此SFM中适应生长,其细胞密度相当于含15%小牛血清的普通培养基的33%～120%。所有瘤细胞均能在SFM中长期传代培养,但贴壁性能有所降低,杂交瘤细胞能持续保持分泌单克隆抗体的能力。

Preparation and Identification of Rat Monoclonal Anti-idiotope Antibody to the Antibody against Erythrocytic Stages of Plasmodium Falciparum

A hybridoma cell line secreting monoclonal antibody to idiotope of the monoclonalantibody 94D1 specific for asexual erythrocytic stages of Plasmodium falciparum was established byfusion of SP2/0 mouse myeloma cells with spleen cells of Wistar rats immunized with monoclonalIgG of 94D1 purified from ascitic fluid of BALB/C mouse by affinity chromatography on ProteinA- Sepharose CL- 4B. Specificity of the anti - idiotope antibody (anti - Id), 41RF5, was deter-mined with indirect enzyme-linked immunosorbent assay (ELISA). The results showedthat 41RF5 reacted only with 94D1 IgG2b, not with normal mouse IgG and other seven mousemonoclonal antibodies - five specific for erythrocytic stages of P. falciparum, one for erythrocyticstages of P. inui, and one for Dengue fever virus type III, which indicates that 41RF5 does recognizespecifically the idiotope of 94D1 monoclonal antibody. In 41RF5 heterohybrid culture supernatant,anti-Id titre measured by ELISA was above 1:1 280. Up to the present, the heterohybrid cell linehas been cultured stably for 16 months.

Some biological characteristics of hybridomas and parental myelomas cultivated in serum-free medium for long-term period

It has been developed in this laboratory that a serum-free medium, designated asDMI,is adaptive for long-term culture,freezing and resurgence in liquid nitrogen,and cloningof hybridoma and parental myelomas as well as for cell fusions.In this report,it is describedthat the myeloma cells grown in DMI for more than 3 months maintained their biological charac-teristics such as induction of aseites and subcutaneous somatic tumor in BALB/c mice and toler-ance toward 8-azaguanine,ete..However,the ability of the tumor cells to attach to glass wallwas decreased.The selecting assay of these cells in HAT medium(medium containing hypoxan-thine,aminopterin and thymidine)showed that the death time in DMI was similar to that in theconventional 15％ newborn calf serum-supplemented medium(RPS15).The hybridoma cellsadapted in DMI secrete monoclonal antibodies in quantities comparable to those produced inRPS15.

Cholesterol requirement for growth of rodent parental myeloma cells in serum-free medium

Cholesterol,a major lipid component of plasma membrane,is thoughtto have profound effects on the structure and function of cells.Mostanimal tis-sues are capable of synthesizing cholesterol de novo from acetate;however,thereare relatively few mammalian cells in vitro expressing an absolute requirement foran exogenous source of cholesterol.In this paper,it was shown that IR983F(983)rat myeloma cells and P3X63-AgS-U1(P3U1)and P3X63-Ag8.653(653)mousemy eloma cells which had been cultivated in serum-free medium for more than 6months required cholesterol in vitro for growth in serum-free medium.Optimalgrowth of P3U1,653 and 983 occurred in cholesterol concentration of 5,10 and15μg/ml,respectively.Moreover,it was demonstrated that the cholesterol couldbe replaced by human low density lipoprotein in a concentration of 10μg/ml butnot by mevalonic acid lactone.In contrast to the parental myeloma cells,hybridoma cells derived from the mouse myeloma cells which had been cultivatedin serum-free medium for more than 6 months did not require cholesterol.