首页> 外文期刊>Bioconjugate Chemistry >An Efficient Method for Labeling Single Domain Antibody Fragments with F-18 Using Tetrazine-Trans-Cyclooctene Ligation and a Renal Brush Border Enzyme-Cleavable Linker
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An Efficient Method for Labeling Single Domain Antibody Fragments with F-18 Using Tetrazine-Trans-Cyclooctene Ligation and a Renal Brush Border Enzyme-Cleavable Linker

机译:使用四嗪 - 反式环辛烯连接和肾刷边界酶可切割接头用F-18标记单结构域抗体片段的有效方法

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Single domain antibody fragments (sdAbs) labeled with F-18 have shown promise for assessing the status of oncological targets such as the human epidermal growth factor receptor 2 (HER2) by positron emission tomography (PET). Earlier, we evaluated two residualizing prosthetic agents for F-18-labeling of anti-HER2 sdAbs; however, these methods resulted in poor labeling yields and high uptake of F-18 activity in the kidneys. To potentially mitigate these limitations, we have now developed an F-18 labeling method that utilizes the trans-cyclooctene (TCO)-tetrazine (Tz)-based inverse-electron demand Diels Alder reaction (IEDDAR) in tandem with a renal brush border enzyme-cleavable glycine-lysine (GK) linker in the prosthetic moiety. The HER2-targeted sdAb 2Rs15d was derivatized with TCO-GK-PEG(4)-NHS or TCO-PEG(4)-NHS, which lacks the cleavable linker. As an additional control, the non HER2-specific sdAb R3B23 was derivatized with TCO-GK-PEG(4)-NHS. The resultant sdAb conjugates were labeled with F-18 by IEDDAR using [F-18]AlF-NOTA-PEG(4)- methyltetrazine. As a positive control, the 2Rs15d sdAb was radioiodinated using the well-characterized residualizing prosthetic agent, N-succinimidyl 4-guanidinomethy1-3-[I-125]iodobenzoate ([I-125]SGMIB). Synthesis of [F-18]AlF-NOTA-Tz-TCO-GK-2Rs15d was achieved with an overall radiochemical yield (RCY) of 17.8 +/- 1.5% (n = 5) in 90 min, a significant improvement over prior methods (3-4% in 2-3 h). In vitro assays indicated that [F-18]AlF-NOTA-Tz-TCO-GK-2Rs15d bound with high affinity and immunoreactivity to HER2. In normal mice, when normalized to coinjected [I-125]SGMIB-2Rs15d, the kidney uptake of [F-18]AlF-NOTA-Tz-TCO-GK-2Rs15d was 15- and 28-fold lower (P 0.001) than that seen for the noncleavable control ([F-18]A1F-NOTA-Tz-TCO-2Rs15d) at 1 and 3 h, respectively. Uptake of [F-18]AlF-NOTA-Tz-TCO-GK-2Rs15d in HER2-expressing SKOV-3 ovarian carcinoma xenografts implanted in athymic mice was about 80% of that seen for coinjected [I-125]SGMIB-2Rs15d. On the other hand, kidney uptake was 5-6-fold lower, and as a result, tumor-to-kidney ratios were 4-fold higher for [F-18]A1F-NOTA-Tz-TCO-GK-2Rs15d than those for [I-125]SGMIB-2Rs15d. SKOV-3 xenografts were clearly delineated even at 1 h after administration of [F-18]AlF-NOTA-Tz-TCO-GK-2Rs15d by Micro-PET/CT imaging with even higher contrast observed thereafter. In conclusion, this strategy warrants further evaluation for labeling small proteins such as sdAbs because it offers the benefits of good radiochemical yields and enhanced tumor-to-normal tissue ratios, particularly in the kidney.
机译:用F-18标记的单结构域抗体片段(Sdabs)已经显示了通过正电子发射断层扫描(PET)评估人体表皮生长因子受体2(HER2)等肿瘤学靶标的状态。早些时候,我们评估了抗HER2 SDAB的F-18标记的两种残留的假体试剂;然而,这些方法导致肾脏中的标记差和高吸收的F-18活性。为了潜在地减轻这些限制,我们现在开发了一种F-18标记方法,其利用反式环辛烯(TCO) - 基于逆电子需求DIES桤木反应(IEDDAR)与肾刷边界酶串联 - 在假体部分中可生活的甘氨酸 - 赖氨酸(GK)接头。 HER2靶向SDAB 2RS15D用TCO-GK-PEG(4)-NHS或TCO-PEG(4)-NHS衍生,其缺乏可切割的接头。作为另外的控制,将非HER2特异性SDAB R3B23用TCO-GK-PEG(4)-NHS衍生化。使用[F-18] Alf-Nota-peg(4) - 甲基四苯胺,通过Ieddar用F-18标记所得的SDAB缀合物。作为阳性对照,2RS15DSDAB使用良好表征的残留假体,N-琥珀酰亚胺酰亚甲基甲酸钠([I-125] SGMIB)。通过90分钟内的整体放射化学产率(Rcy)为17.8 +/- 1.5%(n = 5)的整体放射化学产率(Rcy)来实现[F-18] Alf-Nota-TCO-TCO-GK-2RS15d,对现有方法显着改善(2-3小时3-4%)。体外测定表明[F-18] ALF-NOTA-TCO-GK-2RS15D与HER2的高亲和力和免疫反应结合。在正常小鼠中,当归一化以掺入[I-125] SGMIB-2RS15D时,[F-18] ALF-NOTA-TZ-TCO-TCO-GK-2RS15D的肾摄取为15-和28倍(P <0.001 )在1和3 h分别看见不可脱离对照([F-18] A1F-NOTA-TZ-TCO-2RS15D)。在植入胸腺小鼠中植入的HER2表达的SKOV-3卵巢癌异种移植物中的[F-18] ALF-NOTA-TCO-TCO-GK-2RS15D为互联[I-125] SGMIB-2RS15D的约80%。另一方面,肾脏摄取为5-6倍,结果,对于[F-18] A1F-NOTA-TZ-TCO-GK-2RS15D肿瘤至肾比值为4倍对于[I-125] SGMIB-2RS15D。在通过微宠物/ CT成像在施用[F-18] ALF-NOTA-TZ-TCO-TCO-GK-2RS15D之后,SKOV-3异种移植物显然描除了甚至在此后观察到更高的对比度。总之,该策略需要进一步评估标记SDAB等小蛋白质,因为它提供了良好的放射化学产量和增强的肿瘤至正常组织比,特别是在肾脏中的益处。

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