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Anti-Thy 1.2 monoclonal antibody linked to ricin is a potent cell-type-specific toxin.

机译:与蓖麻毒素连接的抗Thy 1.2单克隆抗体是一种有效的细胞类型特异性毒素。

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摘要

The cell-type specificity of the toxin ricin, which ordinarily binds, enters, and kills cells through receptors containing galactose, has been altered by covalently binding it to a monoclonal antibody and by reversibly binding it to lactose. The antibody, a monoclonal rat IgG2b directed against the Thy 1.2 antigen, provides ricin with a new binding site for the murine thymus cell surface. Addition of lactose saturates the galactose-binding site on ricin and inhibits ricin from binding and killing cells via the galactose-containing receptors. The antibody-ricin hybrid protein, anti-Thy 1.2-ricin, formed with a thioether linkage, has been purified by size exclusion and affinity chromatography. When assayed by inhibition of protein synthesis of EL-4 cells, which express the Thy 1.2 antigen anti-Thy 1.2-ricin is equally as toxic as ricin on a molar basis. The hybrid protein toxicity is unchanged in the presence of 100 mM lactose, whereas unmodified ricin toxicity is reduced to 1% of its toxicity in the absence of lactose. This demonstrates the altered receptor specificity of the ricin hybrid. The cell-type specificity of the anti-Thy 1.2-ricin inhibition of protein synthesis correlates with the presence of the Thy 1.2 antigen. Anti-Thy 1.2-ricin at 4 microgram/ml in the presence of lactose inhibits protein synthesis within 3.5 hr by 60-80% in EL-4 cells but does not affect Thy 1.1 alloantigen and HeLa cells that lack the Thy 1 antigen. Anti-Thy 1.2-ricin in the presence of lactose selectively kills EL-4 cells at concentrations that do not kill AKR-K36 cells. This selectivity, expressed as the ratio of anti-Thy 1.2-ricin concentrations required to kill 40% of both cell types, is 700. Ricin-monoclonal antibody hybrids of this type combine a high degree of cell-type selectivity and toxicity and may have pharmacologic utility as antitumor reagents.
机译:毒素蓖麻毒蛋白通常通过含半乳糖的受体结合,进入并杀死细胞的细胞类型特异性已通过与单克隆抗体共价结合并与乳糖可逆结合而改变。该抗体是针对Thy 1.2抗原的单克隆大鼠IgG2b,可为蓖麻毒蛋白提供鼠胸腺细胞表面的新结合位点。乳糖的添加使蓖麻蛋白上的半乳糖结合位点饱和,并抑制蓖麻毒蛋白通过含半乳糖的受体结合并杀死细胞。已通过大小排阻和亲和色谱法纯化了具有硫醚键的抗体-蓖麻毒蛋白杂合蛋白抗-Thy 1.2-蓖麻毒蛋白。通过抑制表达Thy 1.2抗原的EL-4细胞的蛋白质合成进行分析时,抗Thy 1.2-蓖麻毒蛋白的毒性与蓖麻毒蛋白的摩尔数相同。在100 mM乳糖的存在下,杂合蛋白的毒性没有变化,而在没有乳糖的情况下,未修饰的蓖麻毒蛋白的毒性降低到其毒性的1%。这证明蓖麻毒蛋白杂种的受体特异性改变。抗Thy 1.2蓖麻毒蛋白抑制蛋白质合成的细胞类型特异性与Thy 1.2抗原的存在有关。在乳糖存在下以4微克/毫升的抗Thy 1.2-蓖麻毒蛋白在EL-4细胞中3.5小时内可抑制蛋白质合成60-80%,但不影响Thy 1.1抗原和缺乏Thy 1抗原的HeLa细胞。乳糖存在下的抗Thy 1.2-蓖麻毒蛋白选择性地杀死EL-4细胞,其浓度不会杀死AKR-K36细胞。这种选择性以杀死两种细胞类型的40%所需的抗Thy 1.2-蓖麻毒蛋白浓度的比率表示,为700。这种类型的蓖麻毒素-单克隆抗体杂种结合了高度的细胞类型选择性和毒性,可能具有用作抗肿瘤药的药理学用途。

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  • 作者

    Youle, R J; Neville, D M;

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  • 年度 1980
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  • 正文语种 en
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