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DNA 酶触发水凝胶的溶胶-凝胶-溶胶转变可实现靶细胞的富集。

DNAzyme-Triggered Sol-Gel-Sol Transition of a Hydrogel Allows Target Cell Enrichment.

机构信息

College of Biology, Hunan University, Changsha 410082, China.

State Key Laboratory of Chemo/Biosensing and Chemometrics, College of Chemistry and Chemical Engineering, Hunan University, Changsha 410082, China.

出版信息

ACS Appl Mater Interfaces. 2021 Apr 7;13(13):15031-15039. doi: 10.1021/acsami.1c02262. Epub 2021 Mar 25.

Abstract

Enrichment of rare cancer cells from various cell mixtures for subsequent analysis or culture is essential for understanding cancer formation and progression. In particular, maintaining the viability of captured cancer cells and gently releasing them for relevant applications remain challenging for many reported methods. Here, a physically cross-linked deoxyribozyme (DNAzyme)-based hydrogel strategy was developed for the specific envelopment and release of targeted cancer cells, allowing the aptamer-guided capture, 3D envelopment, and Zn-dependent release of viable cancer cells. The DNAzyme hydrogel is constructed through the intertwinement and hybridization of two complementary DNAzyme strands located on two rolling circle amplification-synthesized ultralong DNA chains. The enveloping and separation of target cells were achieved during the formation of the DNAzyme hydrogel (sol-gel transition). Triggered by Zn, the encapsulated cells can be gently released from the dissociated DNAzyme hydrogel with high viability (gel-sol transition). Successful isolations of target cells from cancer cell mixtures and peripheral blood mononuclear cells (PBMC) were demonstrated. This method offers an attractive approach for the separation of target cancer cells for various downstream applications that require viable cells.

摘要

从各种细胞混合物中富集稀有癌细胞,以便随后进行分析或培养,这对于理解癌症的形成和发展至关重要。特别是,对于许多已报道的方法来说,保持捕获的癌细胞的活力并温和地释放它们用于相关应用仍然具有挑战性。在这里,开发了一种基于物理交联脱氧核酶 (DNAzyme) 的水凝胶策略,用于靶向癌细胞的特异性包裹和释放,允许适体引导捕获、3D 包裹和 Zn 依赖性释放有活力的癌细胞。DNAzyme 水凝胶是通过位于两个滚环扩增合成的超长 DNA 链上的两条互补 DNAzyme 链的交织和杂交构建的。在 DNAzyme 水凝胶的形成过程中(溶胶-凝胶转变)实现了目标细胞的包裹和分离。在 Zn 的触发下,被包裹的细胞可以从解离的 DNAzyme 水凝胶中温和释放,具有高活力(凝胶-溶胶转变)。成功地从癌细胞混合物和外周血单核细胞 (PBMC) 中分离出了目标细胞。该方法为各种需要有活力细胞的下游应用的目标癌细胞分离提供了一种有吸引力的方法。

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