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三功能偶联试剂。含有生物素和放射性金属螯合部分的试剂,用于体外亲和吸附放射性标记抗体。

Trifunctional conjugation reagents. Reagents that contain a biotin and a radiometal chelation moiety for application to extracorporeal affinity adsorption of radiolabeled antibodies.

作者信息

Wilbur D Scott, Chyan Ming-Kuan, Hamlin Donald K, Kegley Brian B, Nilsson Rune, Sandberg Bengt E B, Brechbiel Martin

机构信息

Department of Radiation Oncology, University of Washington, Seattle, Washington 98195-9103, USA.

出版信息

Bioconjug Chem. 2002 Sep-Oct;13(5):1079-92. doi: 10.1021/bc025535r.

Abstract

A method of removing radiolabeled monoclonal antibodies (mAbs) from blood using a device external to the body, termed extracorporeal affinity-adsorption (EAA), is being evaluated as a means of decreasing irradiation of noncancerous tissues in therapy protocols. The EAA device uses an avidin column to capture biotinylated-radiolabeled mAbs from circulated blood. In this investigation, three trifunctional reagents have been developed to minimize the potential deleterious effect on antigen binding brought about by the combination of radiolabeling and biotinylation of mAbs required in the EAA approach. The studies focused on radiolabeling with (111)In and (90)Y, so the chelates CHX-A' '-DTPA and DOTA, which form stable attachments to these radionuclides, were incorporated in the trifunctional reagents. The first trifunctional reagent prepared did not incorporate a group to block the biotin cleaving enzyme biotinidase, but the two subsequent reagents coupled aspartic acid to the biotin carboxylate for that purpose. All three reagents used 4,7,10-trioxa-1,13-tridecanediamine as water-soluble spacers between an aminoisophthalate core and the biotin or chelation group. The mAb conjugates were radioiodinated to evaluate cell binding as a function of substitution. Radioiodination was used so that a direct comparison with unmodified mAb could be made. Evaluation of the number of conjugates per antibody versus cell binding immunoreactivities indicated that minimizing the number of conjugates was best. Interestingly, a decrease of radioiodination yield as a function of the number of isothiocyanate containing conjugates per mAb was noted. The decreased yields were presumably due to the presence of thiourea functionality formed in the conjugation reaction. Radiolabeling with (111)In and (90)Y was facile at room temperature for conjugates containing the CHX-A' ', but elevated temperature (e.g., 45 degrees C) was required to obtain good yields with the DOTA chelate. Stability of (90)Y labeled mAb in serum, and when challenged with 10 mM EDTA, was high. However, challenging the (90)Y labeled mAb with 10 mM DTPA demonstrated high stability for the DOTA containing conjugate, but low stability for the CHX-A' ' containing conjugate. Thus, the choice between these two chelating moieties might be made on requirements for facile and gentle labeling versus very high in vivo stability. Application of the trifunctional biotinylation reagents to the blood clearance of labeled antibodies in EAA is under investigation. The new reagents may also be useful for other applications.

摘要

一种使用体外装置从血液中去除放射性标记单克隆抗体(mAb)的方法,称为体外亲和吸附(EAA),正在作为一种减少治疗方案中非癌组织辐射的手段进行评估。EAA装置使用抗生物素蛋白柱从循环血液中捕获生物素化的放射性标记mAb。在本研究中,已开发出三种三功能试剂,以尽量减少EAA方法中所需的mAb放射性标记和生物素化组合对抗原结合的潜在有害影响。研究集中于用(111)铟和(90)钇进行放射性标记,因此,与这些放射性核素形成稳定连接的螯合剂CHX - A'' - DTPA和DOTA被纳入三功能试剂中。制备的第一种三功能试剂未包含用于阻断生物素裂解酶生物素酶的基团,但随后的两种试剂为此目的将天冬氨酸与生物素羧酸盐偶联。所有三种试剂都使用4,7,10 - 三氧杂 - 1,13 - 十三烷二胺作为异邻苯二甲酸酰胺核心与生物素或螯合基团之间的水溶性间隔物。mAb缀合物进行放射性碘化以评估作为取代函数的细胞结合。使用放射性碘化以便能够与未修饰的mAb进行直接比较。评估每个抗体的缀合物数量与细胞结合免疫反应性表明,使缀合物数量最小化是最佳的。有趣的是,注意到放射性碘化产率随着每个mAb含异硫氰酸酯缀合物数量的增加而降低。产率降低可能是由于缀合反应中形成的硫脲官能团的存在。对于含有CHX - A''的缀合物,在室温下用(111)铟和(90)钇进行放射性标记很容易,但对于DOTA螯合物,需要升高温度(例如45℃)才能获得良好的产率。(90)钇标记的mAb在血清中以及用10 mM乙二胺四乙酸(EDTA)挑战时的稳定性很高。然而,用10 mM二乙三胺五乙酸(DTPA)挑战(90)钇标记的mAb表明,含DOTA的缀合物具有高稳定性,而含CHX - A''的缀合物稳定性低。因此,这两种螯合部分之间的选择可以根据简便温和标记的要求与非常高的体内稳定性来进行。三功能生物素化试剂在EAA中对标记抗体血液清除的应用正在研究中。这些新试剂也可能用于其他应用。

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