111InCl3在淋巴结转移肿瘤模型中的分布及摄取机制

M. De Sousa , A.M. Carroll , P.G. Herman , S. Kerr , J. Boulton , M.R. Zalutsky
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引用次数: 4

摘要

研究了注射氯化111In后大鼠H-4-II-E ACI肝癌肿瘤和引流淋巴结中111In活性的定位。在该肿瘤模型中,肿瘤仅在雄性大鼠中转移到区域淋巴结。进行了以下实验:(a) 111In的生物分布;(b) 111In摄取与[3H]胸苷的相关性;(c) γ相机成像;(d)放射自显影法;(e)铁竞争和(f) 131i -转铁蛋白与H-4-II-E细胞结合。注射24小时后,男性肿瘤与肌肉的比值为111In,原发肿瘤为4.9:1,转移淋巴结为9.1:1。在男性淋巴结转移中,111In摄取与[3H]胸腺嘧啶之间存在显著相关性(r = 0.737),提示转移灶中111In摄取与细胞增殖有关。在原发肿瘤(男性和女性)或女性的引流淋巴结中均未观察到这种相关性。男性的转移淋巴结可以在γ相机图像中检测到,而女性的引流淋巴结无法描绘。在111 - in给药前注射柠檬酸铁可显著减少肝脏、脾脏和肿瘤对111 - in的摄取,并增加肾脏恢复的活性。对131i标记的大鼠转铁蛋白与H-4-II-E细胞结合的测量表明,这些细胞显示转铁蛋白受体。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Distribution and mechanism of uptake of 111InCl3 in a tumor model for lymph node metastases

The localization of 111In activity in the tumor and draining lymph nodes of the H-4-II-E ACI rat hepatoma was investigated following the injection of 111In-chloride. In this tumor model, the tumors metastasize to the regional lymph nodes in male rats only. The following experiments were performed: (a) biodistribution of 111In; (b) correlation of 111In uptake with [3H]thymidine; (c) γ camera imaging; (d) autoradiography; (e) iron competition and (f) binding of 131I-transferrin to H-4-II-E cells. Tumor-to-muscle ratios of 111In in males were 4.9:1 in the primary tumor and 9.1:1 in the metastatic lymph nodes 24h post injection. In the lymph node metastases in the males, a significant correlation between 111In uptake and [3H]thymidine was observed (r = 0.737) suggesting that 111In uptake in the metastases is related to cellular proliferation. No such correlation was observed in either primary tumors (both male and female) or in the draining lymph nodes of the females. Metastatic lymph nodes in males could be detected in γ camera images while draining nodes in females could not be delineated. Injection of ferric citrate prior to 111In administration resulted in a significant reduction of 111In uptake in the liver, spleen and tumor and increased the amount of activity recovered from the kidney. Measurements of the binding of 131I-labeled rat transferrin to H-4-II-E cells in vitro suggest that these cells display transferrin receptors.

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