Adrian Shajkofci scite author profile

Because the complexity of metabolism cannot be intuitively understood or analyzed, computational methods are indispensable for studying biochemistry and deepening our understanding of cellular metabolism to promote new discoveries. We used the computational framework BNICE.ch along with cheminformatic tools to assemble the whole theoretical reactome from the known metabolome through expansion of the known biochemistry presented in the Kyoto Encyclopedia of Genes and Genomes (KEGG) database. We constructed the ATLAS of Biochemistry, a database of all theoretical biochemical reactions based on known biochemical principles and compounds. ATLAS includes more than 130 000 hypothetical enzymatic reactions that connect two or more KEGG metabolites through novel enzymatic reactions that have never been reported to occur in living organisms. Moreover, ATLAS reactions integrate 42% of KEGG metabolites that are not currently present in any KEGG reaction into one or more novel enzymatic reactions. The generated repository of information is organized in a Web-based database ( http://lcsb-databases.epfl.ch/atlas/ ) that allows the user to search for all possible routes from any substrate compound to any product. The resulting pathways involve known and novel enzymatic steps that may indicate unidentified enzymatic activities and provide potential targets for protein engineering. Our approach of introducing novel biochemistry into pathway design and associated databases will be important for synthetic biology and metabolic engineering.

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ASAP: a web-based platform for the analysis and interactive visualization of single-cell RNA-seq data

Gardeux

David

Shajkofci

et al. 2017

117

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MotivationSingle-cell RNA-sequencing (scRNA-seq) allows whole transcriptome profiling of thousands of individual cells, enabling the molecular exploration of tissues at the cellular level. Such analytical capacity is of great interest to many research groups in the world, yet these groups often lack the expertise to handle complex scRNA-seq datasets.ResultsWe developed a fully integrated, web-based platform aimed at the complete analysis of scRNA-seq data post genome alignment: from the parsing, filtering and normalization of the input count data files, to the visual representation of the data, identification of cell clusters, differentially expressed genes (including cluster-specific marker genes), and functional gene set enrichment. This Automated Single-cell Analysis Pipeline (ASAP) combines a wide range of commonly used algorithms with sophisticated visualization tools. Compared with existing scRNA-seq analysis platforms, researchers (including those lacking computational expertise) are able to interact with the data in a straightforward fashion and in real time. Furthermore, given the overlap between scRNA-seq and bulk RNA-seq analysis workflows, ASAP should conceptually be broadly applicable to any RNA-seq dataset. As a validation, we demonstrate how we can use ASAP to simply reproduce the results from a single-cell study of 91 mouse cells involving five distinct cell types.Availability and implementationThe tool is freely available at asap.epfl.ch and R/Python scripts are available at github.com/DeplanckeLab/ASAP.Supplementary information Supplementary data are available at Bioinformatics online.

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Semi-Blind Spatially-Variant Deconvolution in Optical Microscopy with Local Point Spread Function Estimation by Use of Convolutional Neural Networks

Shajkofci

Liebling

2018

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We present a semi-blind, spatially-variant deconvolution technique aimed at optical microscopy that combines a local estimation step of the point spread function (PSF) and deconvolution using a spatially variant, regularized Richardson-Lucy algorithm [1]. To find the local PSF map in a computationally tractable way, we train a convolutional neural network to perform regression of an optical parametric model on synthetically blurred image patches. We deconvolved both synthetic and experimentally-acquired data, and achieved an improvement of image SNR of 1.00 dB on average, compared to other deconvolution algorithms.

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Spatially-Variant CNN-Based Point Spread Function Estimation for Blind Deconvolution and Depth Estimation in Optical Microscopy

Shajkofci

Liebling

2020

IEEE Trans. on Image Process.

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Optical microscopy is an essential tool in biology and medicine. Imaging thin, yet non-flat objects in a single shot (without relying on more sophisticated sectioning setups) remains challenging as the shallow depth of field that comes with highresolution microscopes leads to unsharp image regions and makes depth localization and quantitative image interpretation difficult. Here, we present a method that improves the resolution of light microscopy images of such objects by locally estimating image distortion while jointly estimating object distance to the focal plane. Specifically, we estimate the parameters of a spatiallyvariant Point Spread Function (PSF) model using a Convolutional Neural Network (CNN), which does not require instrument-or object-specific calibration. Our method recovers PSF parameters from the image itself with up to a squared Pearson correlation coefficient of 0.99 in ideal conditions, while remaining robust to object rotation, illumination variations, or photon noise. When the recovered PSFs are used with a spatially-variant and regularized Richardson-Lucy (RL) deconvolution algorithm, we observed up to 2.1 dB better Signal-to-Noise Ratio (SNR) compared to other Blind Deconvolution (BD) techniques. Following microscope-specific calibration, we further demonstrate that the recovered PSF model parameters permit estimating surface depth with a precision of 2 micrometers and over an extended range when using engineered PSFs. Our method opens up multiple possibilities for enhancing images of non-flat objects with minimal need for a priori knowledge about the optical setup.

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