Efficient characterization of red blood cell rheological properties using a multichannel microfluidic chip and optical tweezers

光学镊子 微流控 表征(材料科学) 流变学 镊子 材料科学 微流控芯片 实验室晶片 纳米技术 光电子学 光学 物理 复合材料
作者
Ying Liu,Hongtao Rao,Hongliang Zhang,Meng Wang,Yinglian Wu,Ying Wu,Caiqin Han,Changchun Yan,Le Zhang,Wei Chen,Jingjing Wang
出处
期刊:Materials today advances [Elsevier BV]
卷期号:24: 100545-100545 被引量:6
标识
DOI:10.1016/j.mtadv.2024.100545
摘要

The rheological properties of red blood cells (RBCs) are crucial for human health. Combining optical tweezers with microfluidics provides a non-contact, sensitive, and high-throughput method for studying RBC rheology. However, the limited trapping capacity of optical tweezers restricts RBC flow within microchannels, reducing individual RBC capture efficiency. To address this, we developed a multichannel microfluidic chip with a pressure relief structure. Integrating this with optical tweezers using time-division multiplexing enabled simultaneous capture of RBCs across multiple microchannels. This method not only enhances sample throughput during optical tweezer measurements but also allows individual capture and analysis of multiple flowing RBCs in the same timeframe. Image recognition analysis of RBCs captured by optical tweezers revealed distinct morphological differences between normal and diseased RBCs, consistent with finite element method simulations of RBC rheological behavior. This approach provides quantitative characterization of RBC rheology and enables effective detection. Microfluidic chip structure and multichannel erythrocyte capture. (a) Chip assembly; (b) Center capture channel of the chip; (c) Multichannel capture of erythrocytes. • Designed a multichannel optical capture microfluidic chip to address low efficiency. • Integrated a pressure relief channel into the chip to regulate flow rates in the capture channel center. • Combined the setup with image analysis to extract binarized eigenvalues of rheological images. • Measured deformation areas and lengths of erythrocytes in fluid environments. • The proposed assay efficiently quantifies changes in single erythrocyte rheological behavior.
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