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Efficient and Targeted siRNA Delivery to M2 Macrophages by Smart Polymer Blends for M1 Macrophage Repolarization as a Promising Strategy for Future Cancer Treatment

纳米载体 小干扰RNA 材料科学 内体 基因沉默 纳米技术 药物输送 甘露糖受体 癌细胞 癌症研究 细胞生物学 癌症 巨噬细胞 生物物理学 体外 转染 化学 细胞培养 生物 细胞内 生物化学 基因 遗传学
作者
David C. Jürgens,Benjamin Winkeljann,Miriam Kolog Gulko,Jinrong Yao,Judith Möller,Joshua Winkeljann,Sahana Sheshachala,A.M. Anger,Andreas Hörner,Nathan B. P. Adams,Nora Anne Urbanetz,Olivia M. Merkel
出处
期刊:ACS Biomaterials Science & Engineering [American Chemical Society]
卷期号:10 (1): 166-177 被引量:3
标识
DOI:10.1021/acsbiomaterials.3c01595
摘要

Cancer remains an issue on a global scale. It is estimated that nearly 10 million people succumbed to cancer worldwide in 2020. New treatment options are urgently needed. A promising approach is a conversion of tumor-promoting M2 tumor-associated macrophages (TAMs) as part of the tumor microenvironment to tumor-suppressive M1 TAMs by small interfering RNA (siRNA). In this work, we present a well-characterized polymeric nanocarrier system capable of targeting M2 TAMs by a ligand–receptor interaction. Therefore, we developed a blended PEI-based polymeric nanoparticle system conjugated with mannose, which is internalized after interaction with macrophage mannose receptors (MMRs), showing low cytotoxicity and negligible IL-6 activation. The PEI–PCL–PEI (5 kDa–5 kDa–5 kDa) and Man-PEG–PCL (2 kDa–2 kDa) blended siRNA delivery system was optimized for maximum targeting capability and efficient endosomal escape by evaluation of different polymer and N/P ratios. The nanoparticles were formulated by surface acoustic wave-assisted microfluidics, achieving a size of ∼80 nm and a zeta potential of approximately +10 mV. Special attention was given to the endosomal escape as the so-called bottleneck of RNA drug delivery. To estimate the endosomal escape capability of the nanocarrier system, we developed a prediction method by evaluating the particle stability via the inflection temperature. Our predictions were then verified in an in vitro setting by applying confocal microscopy. For cellular experiments, however, human THP-1 cells were polarized to M2 macrophages by cytokine treatment and validated through MMR expression. To show the efficiency of the nanoparticle system, GAPDH and IκBα knockdown was performed in the presence or absence of an MMR blocking excess of mannan. Cellular uptake, GAPDH knockdown, and NF-κB western blot confirmed efficient mannose targeting. Herein, we presented a well-characterized nanoparticle delivery system and a promising approach for targeting M2 macrophages by a mannose–MMR interaction.
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