Abstract
Microfluidics in vitro assays recapitulate a blood vessel microenvironment using surface-immobilized agonists under biofluidic flows. However, these assays do not quantify intrathrombus mass and activities of adhesive platelets at the agonist margin and use fluorescence labeling, therefore limiting clinical translation potential. Here, we describe a label-free multimodal quantitative imaging flow assay that combines rotating optical coherent scattering microscopy and quantitative phase microscopy. The combined imaging platform enables real-time evaluation of membrane fluctuations of adhesive-only platelets and total intrathrombus mass under physiological flow rates in vitro. We call this multimodal quantitative imaging flow assay coherent optical scattering and phase interferometry (COSI). COSI records intrathrombus mass to picogram accuracy and shape changes to a platelet membrane with high spatial-temporal resolution (0.4 μm/s) under physiological and pathophysiological fluid shear stress (1800 and 7500 s−1). With COSI, we generate an axial slice of 4 μm from the coverslip surface, approximately equivalent to the thickness of a single platelet, which permits nanoscale quantification of membrane fluctuation (activity) of adhesive platelets during initial adhesion, spreading, and recruitment into a developing thrombus (mass). Under fluid shear, pretreatment with a broad range metalloproteinase inhibitor (250 μM GM6001) blocked shedding of platelet adhesion receptors that shown elevated adhesive platelet activity at average of 42.1 μm/s and minimal change in intrathrombus mass.
Original language | English |
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Pages (from-to) | 791-804 |
Number of pages | 14 |
Journal | Biophysical Journal |
Volume | 120 |
Issue number | 5 |
Early online date | 26 Jan 2021 |
DOIs | |
Publication status | Published - 2 Mar 2021 |
Bibliographical note
Funding Information:The authors acknowledge the initial technical advice from Dr. Yuanqing Ma on setting up COSI system. We thank Ms. Samina Nazir, Ms. Sarah Hicks, and Ms. Simone Brysland for providing the washed platelets sample. This work was supported by grants from the Australian Research Council (DP200100364, DP190100039, and DE160100843) and ANU Major Equipment grant (15MEC36 and 16MEC26).
Publisher Copyright:
© 2021 Biophysical Society
ASJC Scopus subject areas
- Biophysics