In vivo antibody labeling route and fluorophore dictate labeling efficiency, sensitivity, and longevity

Natalie B Hagan, Charles Inaku, Nikesh Kunder, Tayleur White, Thierry Iraguha, Anna Meyer, Kristen Pauken, Jason Matthew Schenkel
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Abstract

Leukocytes migrate through the blood and extravasate into organs to surveil the host for infection or cancer. Recently, we demonstrated that intravenous (IV) anti-CD45.2 antibody labeling allowed for precise tracking of leukocyte migration. However, the narrow labeling window can make this approach challenging for tracking rare migration events. Here, we show that altering antibody administration route and fluorophore can significantly extend the antibody active labeling time. We found that while both IV and intraperitoneal (IP) anti-CD45.2 antibody labeled circulating leukocytes after injection, they had different kinetic properties that impacted labeling time and intensity. Quantification of circulating antibody revealed that while unbound IV anti-CD45.2 antibody rapidly decreased, unbound IP anti-CD45.2 antibody increased over one hour. Using in vitro and in vivo serial dilution assays, we found that Alexa Fluor 647 (AF647) and Brilliant Blue 700 (BB700) dyes had the greatest labeling sensitivity compared to other fluorophores. However, IP antibody injection with anti-CD45.2 BB700, but not AF647, resulted in continuous blood leukocyte labeling for over 6 hours. Finally, we leveraged IP anti-CD45.2 BB700 antibody to track slower migrating leukocytes into tumors. We found that IP anti-CD45.2 antibody injection allowed for the identification of ~seven times as many tumor-specific CD8+ T cells that had recently migrated from blood into tumors. Our results demonstrate how different injection routes and fluorophores affect anti-CD45.2 antibody leukocyte labeling and highlight the utility of this approach for defining leukocyte migration in the context of homeostasis and cancer.
体内抗体标记途径和荧光团决定标记效率、灵敏度和寿命
白细胞通过血液迁移并渗入器官,以监测宿主的感染或癌症情况。最近,我们证明了静脉注射抗 CD45.2 抗体可精确追踪白细胞迁移。然而,由于标记窗口较窄,这种方法对于追踪罕见的迁移事件具有挑战性。在此,我们展示了改变抗体给药途径和荧光基团可显著延长抗体的活性标记时间。我们发现,虽然静脉注射和腹腔注射(IP)的抗-CD45.2抗体在注射后都能标记循环白细胞,但它们具有不同的动力学特性,会影响标记时间和标记强度。循环抗体定量显示,未结合的 IV 抗 CD45.2 抗体迅速减少,而未结合的 IP 抗 CD45.2 抗体在一小时内增加。通过体外和体内系列稀释试验,我们发现与其他荧光团相比,Alexa Fluor 647(AF647)和亮蓝 700(BB700)染料的标记灵敏度最高。然而,IP 抗体注射抗 CD45.2 BB700(而非 AF647)可持续标记血液白细胞超过 6 小时。最后,我们利用 IP 抗 CD45.2 BB700 抗体追踪进入肿瘤的迁移速度较慢的白细胞。我们发现,注射 IP 抗 CD45.2 抗体可识别出七倍于最近从血液迁移到肿瘤的肿瘤特异性 CD8+ T 细胞。我们的研究结果表明了不同的注射途径和荧光团对抗CD45.2抗体白细胞标记的影响,并强调了这种方法在平衡和癌症背景下定义白细胞迁移的实用性。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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