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由麦谷蛋白膜形成的排列肌肉层和脂肪层培育肉。

Cultivated Meat from Aligned Muscle Layers and Adipose Layers Formed from Glutenin Films.

作者信息

Yao Ya, Yuen John S K, Sylvia Ryan, Fennelly Colin, Cera Luca, Zhang Kevin Lin, Li Chunmei, Kaplan David L

机构信息

Department of Biomedical Engineering, Tufts University, 4 Colby Street, Medford, Massachusetts 02155, United States.

MilliporeSigma, Inc., 400 Summit Drive, Burlington, Massachusetts 01803, United States.

出版信息

ACS Biomater Sci Eng. 2024 Feb 12;10(2):814-824. doi: 10.1021/acsbiomaterials.3c01500. Epub 2024 Jan 16.

Abstract

Cultivated meat production is a promising technology to generate meat while reducing the reliance on traditional animal farming. Biomaterial scaffolds are critical components in cultivated meat production, enabling cell adhesion, proliferation, differentiation, and orientation. In the present work, naturally derived glutenin was fabricated into films with and without surface patterning and in the absence of toxic cross-linking or stabilizing agents for cell culture related to cultivated meat goals. The films were stable in culture media for at least 28 days, and the surface patterns induced cell alignment and guided myoblast organization (C2C12s) and served as a substrate for 3T3-L1 adipose cells. The films supported adhesion, proliferation, and differentiation with mass balance considerations (films, cells, and matrix production). Freeze-thaw cycles were applied to remove cells from glutenin films and monitor changes in glutenin mass with respect to culture duration. Extracellular matrix (ECM) extraction was utilized to quantify matrix deposition and changes in the original biomaterial mass over time during cell cultivation. Glutenin films with C2C12s showed mass increases with time due to cell growth and new collagen-based ECM expression during proliferation and differentiation. All mass balances were compared among cell and noncell systems as controls, along with gelatin control films, with time-dependent changes in the relative content of film, matrix deposition, and cell biomass. These data provide a foundation for cell/biomaterial/matrix ratios related to time in culture as well as nutritional and textural features.

摘要

培养肉生产是一种很有前景的技术,既能生产肉类,又能减少对传统畜牧业的依赖。生物材料支架是培养肉生产中的关键组成部分,能够实现细胞黏附、增殖、分化和定向排列。在本研究中,将天然来源的麦谷蛋白制成有无表面图案的薄膜,且在与培养肉目标相关的细胞培养过程中不使用有毒的交联剂或稳定剂。这些薄膜在培养基中至少稳定28天,表面图案可诱导细胞排列并引导成肌细胞组织(C2C12细胞),并作为3T3-L1脂肪细胞的底物。这些薄膜在考虑质量平衡(薄膜、细胞和基质生成)的情况下支持细胞黏附、增殖和分化。应用冻融循环从麦谷蛋白薄膜中去除细胞,并监测麦谷蛋白质量随培养时间的变化。利用细胞外基质(ECM)提取来量化细胞培养过程中基质沉积和原始生物材料质量随时间的变化。含有C2C12细胞的麦谷蛋白薄膜由于细胞生长以及增殖和分化过程中新的基于胶原蛋白的ECM表达而随时间显示质量增加。将所有质量平衡在作为对照的细胞和无细胞系统以及明胶对照薄膜之间进行比较,同时比较薄膜、基质沉积和细胞生物量相对含量随时间的变化。这些数据为与培养时间相关的细胞/生物材料/基质比例以及营养和质地特征提供了基础。

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