Deep imaging flow cytometry

被引:26
|
作者
Huang, Kangrui [1 ]
Matsumura, Hiroki [1 ]
Zhao, Yaqi [1 ]
Herbig, Maik [1 ]
Yuan, Dan [1 ]
Mineharu, Yohei [2 ,3 ]
Harmon, Jeffrey [1 ]
Findinier, Justin [4 ]
Yamagishi, Mai [5 ]
Ohnuki, Shinsuke [6 ]
Nitta, Nao [7 ]
Grossman, Arthur R. [4 ,8 ]
Ohya, Yoshikazu [6 ,9 ]
Mikami, Hideharu [1 ,10 ]
Isozaki, Akihiro [1 ]
Goda, Keisuke [1 ,11 ,12 ]
机构
[1] Univ Tokyo, Dept Chem, Tokyo 1130033, Japan
[2] Kyoto Univ, Dept Neurosurg, Kyoto 6068507, Japan
[3] Kyoto Univ, Dept Artificial Intelligence Healthcare & Med, Grad Sch Med, Kyoto 6068507, Japan
[4] Carnegie Inst Sci, Dept Plant Biol, Stanford, CA 94305 USA
[5] Univ Tokyo, Dept Biol Sci, Tokyo 1130033, Japan
[6] Univ Tokyo, Grad Sch Frontier Sci, Dept Integrated Biosci, Chiba 2778562, Japan
[7] CYBO, Tokyo 1010022, Japan
[8] Stanford Univ, Dept Biol, Stanford, CA 94305 USA
[9] Univ Tokyo, Collaborat Res Inst Innovat Microbiol, Tokyo 1138654, Japan
[10] Japan Sci & Technol Agcy, PRESTO, Kawaguchi, Saitama 3320012, Japan
[11] Univ Calif Los Angeles, Dept Bioengn, Los Angeles, CA 90095 USA
[12] Wuhan Univ, Inst Technol Sci, Wuhan 430072, Hubei, Peoples R China
关键词
MICROSCOPY; IMAGES;
D O I
10.1039/d1lc01043c
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Imaging flow cytometry (IFC) has become a powerful tool for diverse biomedical applications by virtue of its ability to image single cells in a high-throughput manner. However, there remains a challenge posed by the fundamental trade-off between throughput, sensitivity, and spatial resolution. Here we present deep-learning-enhanced imaging flow cytometry (dIFC) that circumvents this trade-off by implementing an image restoration algorithm on a virtual-freezing fluorescence imaging (VIFFI) flow cytometry platform, enabling higher throughput without sacrificing sensitivity and spatial resolution. A key component of dIFC is a high-resolution (HR) image generator that synthesizes "virtual" HR images from the corresponding low-resolution (LR) images acquired with a low-magnification lens (10x/0.4-NA). For IFC, a low-magnification lens is favorable because of reduced image blur of cells flowing at a higher speed, which allows higher throughput. We trained and developed the HR image generator with an architecture containing two generative adversarial networks (GANs). Furthermore, we developed dIFC as a method by combining the trained generator and IFC. We characterized dIFC using Chlamydomonas reinhardtii cell images, fluorescence in situ hybridization (FISH) images of Jurkat cells, and Saccharomyces cerevisiae (budding yeast) cell images, showing high similarities of dIFC images to images obtained with a high-magnification lens (40x/0.95-NA), at a high flow speed of 2 m s(-1). We lastly employed dIFC to show enhancements in the accuracy of FISH-spot counting and neck-width measurement of budding yeast cells. These results pave the way for statistical analysis of cells with high-dimensional spatial information.
引用
收藏
页码:876 / 889
页数:15
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