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Radioiodination of proteins using prosthetic group: a convenient way to produce labelled proteins with in vivo stability.

机译:使用修复基团对蛋白质进行放射性碘标记:一种生产具有体内稳定性的标记蛋白质的便捷方法。

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摘要

Radiolabelled peptides can provide new approaches for radiopharmaceutical development. Several prosthetic groups have been developed for radioiodination of proteins in order to minimize in vivo dehalogenation. In this work, the prosthetic group N-succinimidyl 4-[131I]iodobenzoate ([131I]SIB) was obtained by an alternative procedure that employs Cu(I) assisted radioiododebromination to produce p-[131I]iodobenzoic acid with a radiochemical yield of 92.73 +/- 1.51% (N = 6), followed by the reaction with TSTU (O-(N-succinimidyl)-N,N,N'N'-tetramethyluronium) in alkaline medium. The HPLC profile of the final product, revealed that [131I]SIB was obtained with a radiochemical purity of 98.19 +/- 1.14% (N = 6 Swiss mices (normal group) and animals with inflammation focus developed on the right thigh by tupertine injection) were injected with human immunoglobulin (IgG) radioiodinated with [131I]SIB and by direct method (Iodogen). The comparison of results showed a fast blood clearance, better target organ/background relation and low uptake in thyroid and stomach (p < 0.01) for the protein labelled with [131I]SIB, what suggests a greater in vivo stability.
机译:放射性标记的肽可以为放射性药物开发提供新的方法。为了使体内脱卤最小化,已经开发了几种用于蛋白质放射性碘化的修复基团。在这项工作中,通过另一种程序获得了人工取代的N-琥珀酰亚胺基4- [131I]碘代苯甲酸酯基团[[131I] SIB),该程序采用Cu(I)辅助放射性碘代溴化生产对位[131I]碘代苯甲酸,放射化学收率为92.73 +/- 1.51%(N = 6),然后与TSTU(O-(N-琥珀酰亚胺基)-N,N,N'N'-四甲基尿鎓)反应。最终产品的HPLC图谱显示,获得的[131I] SIB的放射化学纯度为98.19 +/- 1.14%(N = 6只瑞士小鼠(正常组)),并且通过古柏汀注射液使炎症集中在右大腿上的动物)注射的人免疫球蛋白(IgG)用[131I] SIB放射性碘标记,并通过直接方法(Iodogen)注射。结果比较显示,用[131I] SIB标记的蛋白具有更快的血液清除速度,更好的靶器官/背景关系以及甲状腺和胃的低摄取(p <0.01),这表明其体内稳定性更高。

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