Department of Bioengineering and Molecular Engineering and Sciences Institute, University of Washington, Seattle, WA 98195, United States.
Theranostics. 2016 Jun 15;6(9):1403-14. doi: 10.7150/thno.15394. eCollection 2016.
Tumor associated macrophages (TAMs) are a major stromal component of the tumor microenvironment in several cancers. TAMs are a potential target for adjuvant cancer therapies due to their established roles in promoting proliferation of cancer cells, angiogenesis, and metastasis. We previously discovered an M2 macrophage-targeting peptide (M2pep) which was successfully used to target and deliver a pro-apoptotic KLA peptide to M2-like TAMs in a CT-26 colon carcinoma model. However, the effectiveness of in vivo TAM-targeting using M2pep is limited by its poor serum stability and low binding affinity. In this study, we synthesized M2pep derivatives with the goals of increasing serum stability and binding affinity. Serum stability evaluation of M2pepBiotin confirmed its rapid degradation attributed to exolytic cleavage from the N-terminus and endolytic cleavages at the W10/W11 and S16/K17 sites. N-terminal acetylation of M2pepBiotin protected the peptide against the exolytic degradation while W10w and K(17,18,19)k substitutions were able to effectively protect endolytic degradation at their respective cleavage sites. However, no tested amino acid changes at the W10 position resulted in both protease resistance at that site and retention of binding activity. Therefore, cyclization of M2pep was investigated. Cyclized M2pep better resisted serum degradation without compromising binding activity to M2 macrophages. During the serum stability optimization process, we also discovered that K9R and W10Y substitutions significantly enhanced binding affinity of M2pep. In an in vitro binding study of different M2pep analogs pre-incubated in mouse serum, cyclic M2pep with K9R and W10Y modifications (cyclic M2pep(RY)) retained the highest binding activity to M2 macrophages over time due to its improved serum stability. Finally, we evaluated the in vivo accumulation of sulfo-Cy5-labeled M2pep and cyclic M2pep(RY) in both the CT-26 and 4T1 breast carcinoma models. Cyclic M2pep(RY) outperformed M2pep in both tumor localization and selective accumulation in M2-like TAMs. In conclusion, we report cyclic M2pep(RY) as our lead M2pep analog with improved serum stability and M2 macrophage-binding activity. Its enhanced utility as an in vivo M2-like-TAM-targeting agent was demonstrated in two tumor models, and is expected to be applicable for other tumor models or in models of M2 macrophage-related diseases.
肿瘤相关巨噬细胞(TAMs)是多种癌症肿瘤微环境中的主要基质成分。由于 TAMs 在促进癌细胞增殖、血管生成和转移方面的作用已得到确立,因此它们是辅助癌症治疗的潜在靶点。我们之前发现了一种 M2 巨噬细胞靶向肽(M2pep),它已成功用于将促凋亡的 KLA 肽靶向 CT-26 结肠癌细胞模型中的 M2 样 TAMs 并进行递送。然而,M2pep 对体内 TAM 靶向的有效性受到其血清稳定性差和结合亲和力低的限制。在这项研究中,我们合成了 M2pep 的衍生物,旨在提高其血清稳定性和结合亲和力。M2pepBiotin 的血清稳定性评估证实,其由于从 N 端的外切降解以及 W10/W11 和 S16/K17 位点的内切降解而迅速降解。M2pepBiotin 的 N 端乙酰化保护肽免受外切降解,而 W10w 和 K(17,18,19)k 取代能够有效地保护各自裂解位点的内切降解。然而,在 W10 位置测试的任何氨基酸变化都没有导致该位点的蛋白酶抗性和结合活性的保留。因此,我们研究了 M2pep 的环化。环化的 M2pep 在不影响与 M2 巨噬细胞结合活性的情况下,更好地抵抗血清降解。在血清稳定性优化过程中,我们还发现 K9R 和 W10Y 取代可显著增强 M2pep 的结合亲和力。在不同 M2pep 类似物与小鼠血清预孵育的体外结合研究中,由于其血清稳定性提高,具有 K9R 和 W10Y 修饰的环化 M2pep(环化 M2pep(RY))在较长时间内保持对 M2 巨噬细胞的最高结合活性。最后,我们评估了 sulfo-Cy5 标记的 M2pep 和环化 M2pep(RY)在 CT-26 和 4T1 乳腺癌模型中的体内积累。环化 M2pep(RY)在肿瘤定位和 M2 样 TAMs 中的选择性积累方面均优于 M2pep。总之,我们报告了具有改进的血清稳定性和 M2 巨噬细胞结合活性的环化 M2pep(RY)作为我们的主导 M2pep 类似物。其作为体内 M2 样-TAM 靶向剂的增强实用性已在两种肿瘤模型中得到证明,并有望适用于其他肿瘤模型或 M2 巨噬细胞相关疾病模型。
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