Abstract
Tomographic phase microscopy (TPM) in flow cytometry is one of the most promising computational imaging techniques for the quantitative 3-dimensional (3D) analysis of unstained single cells. Continuous cells’ flow, combined with the stain-free mode, can assure the high-throughput collection of quantitative and informative 3D data. TPM promises to allow rapid cells’ screening by a nondestructive technique and with statistically relevant data. The current leading-edge research aimed at developing TPM systems in flow cytometry has already demonstrated the possibility of acquiring thousands of single-cell tomograms. Nevertheless, a key unsolved problem exists about the efficient storage and easy handling of such a huge amount of 3D data that prevents rapid analysis for cell diagnosis. Here, we show, for the first time, an effective encoding strategy of single-cell tomograms that can completely overcome this critical bottleneck. Essentially, by using the 3D version of Zernike polynomials, we demonstrate that the 3D refractive index distribution of a cell can be straightforwardly encoded in 1D with negligible information loss (<1%), thus greatly streamlining the data handling and storage. The performance analysis of the proposed method has been first assessed on simulated tomographic cell phantom, while the experimental validation has been extensively proofed on tomographic data from experiments with different cell lines. The results achieved here imply an intriguing breakthrough for TPM that promises to unlock computational pipelines for analyzing 3D data that were unattainable until now.
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