Journal of Isotopes (Dec 2024)

SPECT Imaging of PD-L1 Expression of MDA-MB-231 Tumor Xenograft Mice with 125I-labeled Monoclonal Antibody

  • Shuhua HE,
  • Yang WANG,
  • Xiaobei ZHENG,
  • Yuxia LIU,
  • Lina JIA,
  • Lan ZHANG

DOI
https://doi.org/10.7538/tws.2024.youxian.008
Journal volume & issue
Vol. 37, no. 6
pp. 568 – 574

Abstract

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125I-Atezolizumab was synthesized with Iodogen method for monitoring the expression level of PD-L1 in tumors. The influence of reaction time on 125I-labeling efficiency and the stability of 125I-Atezolizumab in PBS and fetal bovine serum were studied. The pharmacokinetics of 125I-Atezolizumab was evaluated in rats. Binding specificity to PD-L1 was determined using cellular uptake experiment of breast cancer cell line MDA-MB-231 in vitro and SPECT imaging of mice bearing MDA-MB-231 xenografts in vivo. The results indicated that the labeling yield of 125I-Atezolizumab was over 98% after 5 minutes reaction at room temperature. The radiochemical purity was more than 90% after 48 h incubation in PBS and fetal bovine serum. The elimination half-life of 125I-Atezolizumab in rats was (12.1±1.9) h. The immunological activity of 125I-Atezolizumab was well maintained (IF=52%) and high affinity was demonstrated in breast cancer cell line. SPECT/CT imaging of MDA-MB-231 tumor-bearing mice showed high radioactivity uptake in the tumor. Tumor uptake of 125I-Atezolizumab was blocked in the presence of Atezolizumab,confirming target specificity. The preliminary results suggested that 125I-Atezolizumab exhibited specificity for PD-L1 imaging using a simple and efficient labeling method,and demonstrated relatively good in vitro stability. It is potential to monitor the expression levels of PD-L1 in tumors by 125I-Atezolizumab SPECT imaging and is worthy of further research.

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