Studying the roundworm Caenorhabditis elegans using microfluidic chips

微流控 秀丽隐杆线虫 生物 模式生物 细胞生物学 高含量筛选 计算生物学 活体细胞成像 遗传筛选 表型 药物开发 纳米技术 遗传学 药品 基因 细胞 材料科学 药理学
作者
Martin A. M. Gijs
标识
DOI:10.1117/12.2513194
摘要

C. elegans is an attractive model organism in biology, as it shows genetic similarity with humans, facilitates microscopic observation due to its transparency, and has a short life cycle. Moreover, many mutants expressing fluorescent proteins in particular cell types exist, and these can be advantageously used for gene/protein expression studies. Nematodes are traditionally cultured on agar plates seeded with E. coli bacteria as food and well plate-based worm cultures using liquid media have enabled high-throughput drug screening. In addition to the well plate format, microfluidics promises precise spatio-temporal handling and dosing of biological reagents for more controlled manipulation and culture of worms and embryos on-chip. I will first discuss reversible worm immobilization protocols, like the use of mechanical clamping or the temperature-sensitive sol-gel transition of a Pluronic solution, for high-resolution on-chip imaging. In particular, we exploited the imaging potential offered by microfluidic chips for performing fluorescent protein aggregation studies to characterize progress of neurodegenerative disease and for mitochondrial morphology studies. We have also implemented worm bio-communication assays on-chip, and have proposed microfluidic chips for automated embryo arraying, phenotyping, and long-term live imaging, as well as for drug studies performed during early embryogenesis. Microfluidic chips thereby allowed studying worm populations at individual animal resolution level and permitted investigating multiple phenotypes at different time points during worm development. Thereby we could observe individualized multi-phenotypic responses to drugs and genetic cues.
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