HIM_(1) AND HIM4, TWO MONOCLONAL ANTIBODIES POTENTIALLY USEFUL FOR AUTOLOGOUS BONE MARROW TRANSPLANTATION IN CHRONIC MYELOGENOUS LEUKEMIA

We developed two complement-fixing MoAbsHIMand HIM(murine)that were specifically reac-tive with chronic myelogenous leukemia (CML) cells.They were capable of fixing human or rabbit com-plement and suitable for CML cells purging of re-mission marrow from CML patients.HIMreactedwith majority leukemic cells form 7 out of 10 CMLpatients by complement-mediated cytotoxicity(C’MC)assay(positive cells 80%—90%),HIMreacted withmajority CML cells from 4 out of 5 CML by C’MCassay(positive cells 80%—90%).Treatment withHIMor HIMand human C’was capable of lysing97% of K562,U937,HL-60 and CML cells in a 20fold excess of unrelated cells by indirect FITC+EBstain.Using limited dilution culture,incubation withHIMand C’produced 1.5 logs inhibition of growthin K562 cells,and 1.9 logs in U937 cells,and withHIMand C’produced 2.9 logs inhibition in HL-60cells and 3.0 logs in U937 cells.Both MoAbs cocktailwas shown 1.8 logs in K562 cells and 3.2 logs in U937cells.They were no suppression on the growth o

THE USE OF ANTI-HUMAN GLIOMA MONOCLONAL ANTIBODIES FOR TARGETING CHEMOTHERAPY OF BRAIN GLIOMAS(PREPARATION AND CYTOTOXIC PROPERTIES OF ANTIBODY-ADRIAMYCIN IMMUNOCONJUGATES)

Immunoconjugates are antibody-drug hybrid molecules which combine the exquisite selectivity or monoclonal antibodies with the potent toxicity of anticancer agents. A monoclonal antibody SZ39 against human brain gliomas was used as a drug carrier. Adriamycin (ADR) was bound covalently to SZ39 to form a SZ39-ADR conjugate. The cytotoxic activity of the SZ39-ADR conjugate was tested in vitro and demonstrated potent and specific killing of cells derived from a human malignant glioma. 50% inhibitory concentration (IC50) for SZ39-ADR to 'target' cells was 8.14×10-9 M. An index of specificity between 'target' and 'non-target' cells was calculated to be 88-fold. These data suggest that the SZ39-ADR may use as a potent and cell type-specific agent and is a likely candidate for the targeting chemotherapy of malignant gliotnas.

THE USE OF ANTIHUMAN GLIOMA MONOCLONAL ANTIBODIES FOR TARGETING CHEMOTHERAPY OF BRAIN GLIOMAS(POTENT SUPPRESSION OF MALIGNANT GLIOMA GROWTH WITH IMMUNOCONJUGATES IN VIVO)

Athymic nude mice bearing subcutaneous and intracerebral human glioma xenografts were used to assess the therapeutic efficacy of monoclonal anti-body-adriamycin immunoconjugates against malignant gliomas in vivo. Immunoconjugates showed a significantly stronger antitumor effect with a T/C (treated/ control tumor volume) of 30% as compared with free drug (T/C of 84%). The targeting treatment with immunoconjugates significantly prolonged 54% of median survival time of nude mice. Side effects of immunoconjugates on the normal bone marrow and small intestines were much slighter than those of the free drug. The results of this study indicate that the use of monoclonal antibodies as carriers of anti-tumor agents may have many therapeutic advantages and potential for the treatment of brain gliomas.

Tumoricidal activation of murine resident peritoneal macrophages on pancreatic carcinoma by interleukin-2 and monoclonal antibodies

INTRODUCTIONMacrophages play an important role in tumor lysisand growth inhibition.They can be activated to atumoricidal state by a variety of agents such asIFNr,TNFα or IL2.The killing machanisms ofactivated macrophages have been extensivelyinvestigated.Recently,it has been proved thatantibody dependent cellular cytotoxicity (ADCC) isone of the potent arms to lyse tumor cells

DETECTION OF CANCER-ASSOCIATED ANTIGEN IN FECES USING MONOCLONAL ANTIBODIES IN THE DIAGNOSIS OF COLON CARCINOMA

Monoclonal antibodies against colon and pancreatic cancer, CL-2, CL-3, PS-9, PS-10, were used to detect the associated antigens in feces of patients with gastrointestinal carcinoma and non-cancer diseases. Binding inhibition test by SABC-ELISA method were performed for the measurement of the antigen level. Results showed that the associated antigen detected in feces of patients with colon cancer were significantly higher than that of non-cancer disease or normal subjects. The positive rates were 61.1% as detected with CL-2; 53.4% with CL-3; 55.0%, PS-9; and 53.3% PS-10 in cancer patients while that in normal subjects were 7%; 9%; 8%; and 8% respectively. When 'cocktail' of CL-2, PS-9 and PS-10 were used, the positive rates were 92.5% in colon cancer and 14% in normal subjects. In seven out of the sixty patients with colon cancer studied who were graded as Dukes A, the results were all positive. The results seem superior to the serologic detection and may provide a promising new approach in the early diagnosis of colon cancer.

关于抗Aβ单克隆抗体的临床应用建议(2024版)

最新研发的抗Aβ单克隆抗体陆续在国内外获批上市,并逐渐应用于我国临床实践。为促进抗Aβ单克隆抗体在我国阿尔茨海默病治疗中更合理、安全的应用,本文结合抗Aβ单克隆抗体现有临床试验证据及阿杜卡单抗在上海交通大学医学院附属瑞金医院海南医院的临床应用经验,总结抗Aβ单克隆抗体的临床应用建议,包括临床用药指征、用药前评估及准备、用药时医嘱及注意事项、用药后临床监测,旨在为临床医师提供翔实的用药指导和建议。

体外检测试剂盒阻断剂的制备方法及特性分析

目的探讨体外检测试剂盒阻断剂的制备方法及特性。方法采用6周龄BALB/c小鼠进行抗原免疫,构建杂交瘤细胞并克隆。采用动物体内诱导单克隆抗体的方法大量制备单克隆抗体,分别采用G柱亲和层析、蓝胶+Q柱离子交换层析两种方法进行纯化,核酸蛋白检测仪记录波长280 nm下的光密度(optical density,OD),紫外分光光度计测量成品浓度。采用十二烷基硫酸钠-聚丙烯酰胺凝胶电泳(sodium dodecylsulfate-polyacrylamide gel electrophoresis,SDS-PAGE)检测抗体纯度。采用酶联免疫吸附试验(enzyme-linked immunosorbent assay,ELISA)双抗体夹心法检测该阻断剂(CN302)对假阳性样本的阻断能力。结果G柱亲和层析法提取阻断剂的收率(3个批次分别为6.49、6.12、6.27 g/L)高于蓝胶+Q柱离子交换层析法(3个批次分别为1.78、1.68、1.61 g/L)。两种纯化方法的纯度均高达95%以上。G柱亲和层析法、蓝胶+Q柱离子交换层析法所得阻断剂的活性分别为106.54%、92.45%;与空白组相比,两种纯化方式所得阻断剂CN302对假阳性样本的检出率均降低,其OD值均小于0.2,与基准阻断剂大致相同。G柱亲和层析法所得阻断剂CN302未冻融的活性为99.86%,冻融5次后活性为99.83%。无阻断剂存在时,对假阳性样本检测的OD值约为2.5,最高可达到4.0;加入阻断剂后,OD值明显降低;阻断剂CN302对假阳性样本检测的OD值低于其他阻断剂。结论本研究所得阻断剂能显著消除样本内源性干扰,且活性几乎全部保留。G柱亲和层析法提取抗体的收率和阻断能力均高于蓝胶+Q柱离子交换层析法。

Off-label use of targeted therapies in oncology

Off-label use is defined by the prescription of a marketed drug outside the conditions described in the summary of product characteristics.In oncology,off-label prescribing of targeted therapies may occur in patients with other tumor types expressing the same target.Agents associated to phenotypic approaches such as therapies against the tumoral vasculature(anti-angiogenic drugs) and new immunotherapies(checkpoint inhibitors) also carry the potential of alternative indications or combinations.Off-label use of targeted therapies is little documented and appears to be in the same range than that regarding older drugs with wide variations among agents.When compared with older agents,off-label use of targeted therapies is probably more rational through tumoral genotyping but is faced with a limited clinical support,reimbursement challenges related to the very high pricing and the cost of genotyping or molecular profiling,when applicable.

鸡传染性法氏囊病单抗快速诊断试剂盒的研制及初步应用

以感染传染性法氏囊病病毒 ( IBDV)的鸡法氏囊组织制备免疫抗原 ,免疫 BALB/c系小鼠 ,取其脾细胞与 NS0浆细胞进行细胞融合 ;以 AC-ELISA筛选阳性细胞克隆 ,经 3次有限稀释克隆化及鉴定 ,获得 2株识别 IBDV不同抗原决定簇的高亲和力单克隆抗体株。以该 2株单克隆抗体制备快速诊断试剂 ,组装了鸡传染性法氏囊病快速诊断试剂盒。该试剂盒由若干 4 0孔酶标板 ,1号酶标液 ( HRP标记 IBDV单抗 )、2号洗涤液、3号显色液 ( TMD显色底物 )、4号显色液 (供氢体 )等反应液 ,0 .0 1 mol/L PBS( p H7.2 )阴性对照、IBDV阳性对照 (提取的 IBDV蛋白 )组成 ,并对试剂盒特异性、敏感性、重复性及稳定性等进行了鉴定。应用该快速诊断试剂盒对来源于不同地区的临床诊断疑似 IBD的法氏囊病料各 2 0份进行了检测 ,并与琼扩试验、常规ELISA检测结果作了比较 ,结果表明 ,该快速诊断试剂盒的检测结果与常规 ELISA的检测结果相似 ,操作程序简便 ,可在 1 0～ 1 5min内完成 。

CA_(125)、CA_(199)及CA_(153)联合检测对肺癌的诊断价值

目的 :评价血清 CA12 5、CA199、CA153联合检测对肺癌诊断及分期的临床价值。方法 :用免疫放射分析法测定 72例不同类型及分期的肺癌患者 ,46例肺良性疾病患者及 38例健康体检者血清 CA12 5、CA199、CA153水平的变化。结果 :肺癌组血清 CA12 5、CA199、CA153水平均高于正常对照组及肺良性疾病患者 ,有显著性差异 ,且 TNM分期越晚 ,其水平越高。 3项肿瘤标志联合检测可提高敏感性及准确性。结论 :CA12 5、CA199、CA153联合检测可以为肺癌的诊断及分期提供有价值的实验室依据。

三聚氰胺单克隆抗体制备与鉴定

目的制备高度特异的三聚氰胺单克隆抗体,经酶联免疫吸附试验鉴定并制备胶体金试剂盒。方法以牛血清白蛋白交联的三聚氰胺为抗原,免疫BALB/c小鼠,通过传统杂交瘤融合和筛选技术制备抗三聚氰胺单克隆抗体,经纯化制备腹水,采用酶联免疫吸附实验(enzyme linked immune sorbent assay, ELISA)对抗体进行效价测定、亚类测定、交叉鉴定和蛋白质免疫印迹试验(westernblot)特异性鉴定后制备胶体金试剂盒。结果筛选出1株抗三聚氰胺单抗,制备的三聚氰胺胶体金试剂盒敏感值能达到30μg/L。结论获得了高度特异的且能稳定分泌三聚氰胺抗体的细胞株。

巨噬细胞抑制因子-1单克隆抗体的研制及血清检测系统的建立

目的研制巨噬细胞抑制因子-1(MIC-1)单克隆抗体并建立MIC-1血清检测方法。方法应用自主研制的MIC-1抗原免疫BALB/C雌鼠,通过杂交瘤技术获得分泌抗MIC-1单克隆抗体的杂交瘤细胞株,通过ELISA方法构建MIC-1血清检测体系并对性能进行鉴定。结果成功获得了32株抗MIC-1单克隆抗体,选用其中2株高亲和力单克隆抗体建立了双夹心ELISA MIC-1血清快速检测方法。性能鉴定结果表明所建立的方法线性关系良好(R2值大于0.999);试验内变异系数为5.15%,试验间变异系数为9.51%;平均回收率为98.9%;37℃保存3天和4℃保存6个月稳定性良好。结论所制备的MIC-1检测方法各项指标均达到SFDA相关要求,能够满足科学研究和临床检测的技术需要,并进入产业化程序。

临床诊断试剂及其诊断方法研究进展

本文结合作者工作，综述了现代临床化学所用诊断试剂，以及诊断方法学研究的某些进展与发展趋向。内容包括：免疫层析诊断试条将替代ＥＬＩＳＡ法和点印渍法诊断药盒的理由；可在室温长期储存诊断试剂的玻璃化技术研究进展；单表位单抗能提高诊断试剂选择性的依据，以及广谱恶性肿瘤早期诊断试剂研制现状。

抗家蚕浓核症病毒单克隆抗体实用化研究

制备了家蚕浓核症诊断试剂盒,将单克隆抗体与双向免疫技术相结合,用于家蚕浓核症的诊断.采用此试剂盒,对家蚕浓核症的最早检出时间为感染病毒后48小时.若将此单克隆抗体与免疫酶技术或萤光抗体技术结合,则能在感染病毒后12～16小时的家蚕中肠组织内检测到病毒抗原.配制的单克隆抗体应用液效价稳定,在37℃下放置一个月,室温下放置两个月仍然有效.单克隆抗体能代替常规抗血清用于家蚕浓核症的诊断.

抗胃肠癌单克隆抗体对胃肠癌普查1801例结果分析

以抗结肠癌及胃癌单克隆抗体组合应用对１８０１例进行胃肠癌普查。普查结果：３２例胃肠癌肿瘤相关抗原阳性，阳性率为１．８％，部分进行胃及肠镜检查，其中１２例做肠镜，３０例做胃镜，结果证实：早期胃癌１例。癌前病变１９例，其中大肠腺瘤５例，伴不典型增生２例，萎缩性胃炎１２例，伴不典型增生７例，浅表性胃炎伴不典型增生１例，老年多发性肠憩室１例。此外，非癌前病变７例，包括浅表性胃炎、急性胃、肠炎等。１７５０例阴性者随访１年以上，尚未发现胃、肠癌，本法假阳性率低，０．３％。且方法较简便、价低。用于胃肠癌普查及诊断将有一定意义。

大便隐血单克隆抗体检查方法的优化

目的 了解增强液 (改进稀释液 )是否优于 DH2 O(原法稀释液 ) ,从而提高实验的灵敏度。方法 通过改进反应介质 ,选择抗原抗体反应最适浓度。患者样本采用两种方法进行随机对比分析。结果 经 STAT医学统计软件包处理 ,其χ2 =6 7.2 8,P<0 .0 5 ,显示两法的检验效能不一致。结论 采用增强液做抗原抗体反应介质检测大便隐血优于用 DH2

抗霍乱弧菌O1群单克隆抗体的制备及初步鉴定

目的制备抗霍乱弧菌O1群特异性单克隆抗体(McAb),并进行鉴定。方法以福尔马林灭活的O1群霍乱弧菌免疫BALB/c小鼠,应用细胞融合技术建立分泌抗O1群霍乱弧菌McAb的杂交瘤细胞株。对配对较好的6个细胞株分泌的McAb进行腹水效价、免疫球蛋白类及亚类、抗体亲和常数测定及凝集试验和稳定性试验。与细菌培养法对比检测208份临床标本。结果6个细胞株分泌的McAb腹水效价均为105,均为IgM;抗体亲和常数为1.84×105～5.38×107;且均与O1群霍乱弧菌菌株发生凝集反应,与霍乱弧菌O139群、大肠杆菌、出血性大肠杆菌O157∶H7、副溶血弧菌、麦弧菌、河弧菌、结肠炎耶尔森菌、普通变形杆菌、痢疾杆菌、伤寒杆菌及各型副伤寒杆菌均不发生凝集反应。6个分泌McAb的细胞株连续培养15周,经液氮冻存12个月后复苏,仍能稳定分泌抗体;与细菌培养法对比检测208份临床标本,特异性和灵敏度均达100%。结论制备的McAb具有较高的特异性,有可能用于开发霍乱弧菌O1群的检测试剂。

McAb-Dot-ELISA检测血吸虫循环抗原的现场查病应用

将 McAb-Dot-ELlSA 检测循环抗原法应用于血吸虫病疫区现场查病125例。结果:居民循环抗原阳性率为44.0%,较粪检虫卵阳生率26.4%高(P<0.01),两者符合率为83.3%;治疗后3个月循环抗原阴转率为63.6%,较抗体阴转率10.9%高(P<0.01)。提示:McAb-Dot-ELISA 检测循环抗原法较粪检法检出率高,与 IHA 检测抗体法比较具有近期疗效考核价值。

沙门氏菌单克隆抗体研究 Ⅰ.杂交瘤细胞系的建立

用沙门氏菌O,H,Vi抗原免疫BALB/c小鼠,采用细胞融合技术,获得分泌抗沙门氏茵0-2,4,7,8,9,3,10,11和H-a,b,c,d,i及Vi抗原的单克隆抗体杂交瘤细胞系29株。所产生的抗体17株属IgM,7株为IgG3,3株为IgG1,1株为IgG_(2a),1株未测;轻链除3株为λ链外,其余为κ链。将杂交瘤细胞所诱生的腹水,组成一套(11种)沙门氏菌诊断用单克隆抗体试剂,经用沙门氏菌属和其它肠道菌属的代表菌株作鉴定,证明具有良好的特异性和敏感性、可供初步诊断伤寒,副伤寒和鼠伤寒用。与目前常规生产的家兔诊断血清相比,具有简化生产过程,节约家兔与培养基及省时省力等优点,值得在生产上和使用上推广。

艰难梭菌A毒素单克隆抗体酶标诊断试剂盒的研制

目的制备艰难梭菌A毒素的单克隆抗体酶标诊断试剂。方法采用夹心ELISA方法,用纯化的抗艰难梭菌A毒素的兔单特异血清包板,10%BSA-PBST封闭,加入检测样品,洗涤后加入辣根过氧化物酶标记的单克隆抗体,用底物TMP显色,2MH2SO4终止反应,测定OD450。结果对2株艰难梭菌产毒株、2株艰难梭菌非产毒株、26株大肠杆菌、2株痢疾杆菌、1株双歧杆菌、5株霍乱弧菌、2株伤寒沙门氏菌、7株肉毒梭菌、1株索氏梭菌、1株酪酸梭菌的培养滤液进行检测,该ELISA试剂具有很高的特异度和灵敏度,最低可检出艰难梭菌A毒素0.1ng。结论这种艰难梭菌A毒素的单克隆抗体酶标诊断试剂盒具有较高的特异度和灵敏度,适合临床推广应用。