An approach for the intracellular delivery of IgG via enzymatic ligation with a cell-permeable attenuated cationic amphiphilic lytic peptide

IF 4.3 3区 材料科学 Q1 ENGINEERING, ELECTRICAL & ELECTRONIC ACS Applied Electronic Materials Pub Date : 2024-07-24 DOI:10.1016/j.bmc.2024.117835
Yoshimasa Kawaguchi, Sakahiro Terada, Shiroh Futaki
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Abstract

Achieving effective intracellular delivery of therapeutic molecules such as antibodies (IgG) is a challenge in biomedical research and pharmaceutical development. Conjugation of IgG with a cell-penetrating peptide is a rational approach. Here, not only the efficacy of the conjugates in internalizing into cells, but also the physicochemical property of the conjugates allowing their solubilized states in solution without forming aggregates are critical. In this study, we have shown that the first requirement can be addressed using a cell-permeable attenuated cationic amphiphilic lytic (CP-ACAL) peptide, L17ER4. The second requirement can be addressed by ligation of IgG to L17ER4 using sortase A, where the use of a linker of appropriate chain length is also important. For evaluation, the intracellular delivery efficacy was studied using conjugate structures with different orientations and conjugation modes of L17ER4 in ligation to a model protein, green fluorescent protein fused to a nuclear localization signal (NLS-EGFP). The effect of tetraarginine positioning in the L17ER4 sequence was also investigated. Following these studies, an optimized peptide sequence containing L17ER4 was ligated to an anti-green fluorescent protein (GFP) IgG bearing a sortase A recognition sequence. Treatment of the cells with the conjugate of anti-GFP IgG and L17ER4 resulted in a high efficiency of cytosolic translocation of the conjugate and the binding to the target protein in the cell without significant aggregate formation. The feasibility of the d-form of L17ER4 as a CP-ACAL was also confirmed.

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通过与细胞渗透性减弱的阳离子两亲性裂解肽进行酶连接,在细胞内输送 IgG 的方法。
实现治疗分子(如抗体(IgG))的有效细胞内递送是生物医学研究和药物开发中的一项挑战。将 IgG 与细胞穿透肽共轭是一种合理的方法。在这里,不仅共轭物在细胞内化方面的功效至关重要,共轭物在溶液中的溶解状态而不形成聚集体的理化性质也至关重要。在这项研究中,我们发现使用一种细胞渗透性减弱的阳离子两亲性裂解(CP-ACAL)肽 L17ER4 可以满足第一个要求。第二个要求可通过使用分选酶 A 将 IgG 与 L17ER4 连接来实现,其中使用链长适当的连接体也很重要。为了进行评估,我们利用 L17ER4 与模型蛋白--融合了核定位信号的绿色荧光蛋白(NLS-EGFP)--连接时的不同方向和连接模式的共轭结构研究了细胞内递送功效。此外,还研究了 L17ER4 序列中四精氨酸定位的影响。在这些研究之后,将含有 L17ER4 的优化肽序列连接到带有分选酶 A 识别序列的抗绿色荧光蛋白(GFP)IgG 上。用抗绿色荧光蛋白(GFP)IgG 和 L17ER4 的共轭物处理细胞后,共轭物在细胞内的转运效率很高,并能与细胞内的目标蛋白结合,而不会形成明显的聚集体。L17ER4 的 d-形式作为 CP-ACAL 的可行性也得到了证实。
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CiteScore
7.20
自引率
4.30%
发文量
567
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