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重编程锚定依赖性以开发用于重组蛋白表达的细胞系。

Reprogramming anchorage dependency to develop cell lines for recombinant protein expression.

出版信息

Biotechnol J. 2024 May;19(5):e2400104. doi: 10.1002/biot.202400104.

Abstract

As the biopharmaceutical industry continues to mature in its cost-effectiveness and productivity, many companies have begun employing larger-scale biomanufacturing and bioprocessing protocols. While many of these protocols require cells with anchorage-independent growth, it remains challenging to induce the necessary suspension adaptations in many different cell types. In addition, although transfection efficiency is an important consideration for all cells, especially for therapeutic protein production, cells in suspension are generally more difficult to transfect than adherent cells. Thus, much of the biomanufacturing industry is focused on the development of new human cell lines with properties that can support more efficient biopharmaceutical production. With this in mind, we identified a set of "Adherent-to-Suspension Transition" (AST) factors, IKZF1, BTG2 and KLF1, the expression of which induces adherent cells to acquire anchorage-independent growth. Working from the HEK293A cell line, we established 293-AST cells and 293-AST-TetR cells for inducible and reversible reprogramming of anchorage dependency. Surprisingly, we found that the AST-TetR system induces the necessary suspension adaptations with an accompanying increase in transfection efficiency and protein expression rate. Our AST-TetR system therefore represents a novel technological platform for the development of cell lines used for generating therapeutic proteins.

摘要

随着生物制药行业在成本效益和生产力方面的不断成熟,许多公司已经开始采用更大规模的生物制造和生物加工方案。虽然这些方案中的许多都需要具有无锚定依赖性生长的细胞,但在许多不同的细胞类型中诱导必要的悬浮适应仍然具有挑战性。此外,尽管转染效率是所有细胞的重要考虑因素,尤其是对于治疗性蛋白质生产,但悬浮细胞通常比贴壁细胞更难转染。因此,生物制造行业的大部分都专注于开发具有支持更高效生物制药生产能力的新人类细胞系。考虑到这一点,我们确定了一组“贴壁-悬浮过渡”(AST)因子,包括 IKZF1、BTG2 和 KLF1,它们的表达诱导贴壁细胞获得无锚定依赖性生长。从 HEK293A 细胞系开始,我们建立了 293-AST 细胞和 293-AST-TetR 细胞,用于诱导和可逆重编程锚定依赖性。令人惊讶的是,我们发现 AST-TetR 系统诱导了必要的悬浮适应,同时提高了转染效率和蛋白质表达率。因此,我们的 AST-TetR 系统代表了一种用于生成治疗性蛋白质的细胞系开发的新型技术平台。

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