scholarly journals Single Cell Viewer (SCV): An interactive visualization data portal for single cell RNA sequence data

2019 ◽  
Author(s):  
Shuoguo Wang ◽  
Constance Brett ◽  
Mohan Bolisetty ◽  
Ryan Golhar ◽  
Isaac Neuhaus ◽  
...  
Keyword(s):  
Single Cell ◽  
Sequence Data ◽  
Single Cells ◽  
Link Type ◽  
Technological Advances ◽  
R Shiny ◽  
Data Volume ◽  
Exploratory Data ◽  
Cell Data ◽  
Shiny Application

AbstractMotivationThanks to technological advances made in the last few years, we are now able to study transcriptomes from thousands of single cells. These have been applied widely to study various aspects of Biology. Nevertheless, comprehending and inferring meaningful biological insights from these large datasets is still a challenge. Although tools are being developed to deal with the data complexity and data volume, we do not have yet an effective visualizations and comparative analysis tools to realize the full value of these datasets.ResultsIn order to address this gap, we implemented a single cell data visualization portal called Single Cell Viewer (SCV). SCV is an R shiny application that offers users rich visualization and exploratory data analysis options for single cell datasets.AvailabilitySource code for the application is available online at GitHub (http://www.github.com/neuhausi/single-cell-viewer) and there is a hosted exploration application using the same example dataset as this publication at http://periscopeapps.org/[email protected]; [email protected]

scholarly journals CIM-seq

2021 ◽  
Author(s):  
Nathanael Andrews ◽  
Martin Enge
Keyword(s):  
Single Cell ◽  
Single Cells ◽  
Likelihood Estimation ◽  
Cell Types ◽  
Data Sets ◽  
Target Tissue ◽  
Data Set ◽  
Rnaseq Data ◽  
The Given ◽  
Cell Data

Abstract CIM-seq is a tool for deconvoluting RNA-seq data from cell multiplets (clusters of two or more cells) in order to identify physically interacting cell in a given tissue. The method requires two RNAseq data sets from the same tissue: one of single cells to be used as a reference, and one of cell multiplets to be deconvoluted. CIM-seq is compatible with both droplet based sequencing methods, such as Chromium Single Cell 3′ Kits from 10x genomics; and plate based methods, such as Smartseq2. The pipeline consists of three parts: 1) Dissociation of the target tissue, FACS sorting of single cells and multiplets, and conventional scRNA-seq 2) Feature selection and clustering of cell types in the single cell data set - generating a blueprint of transcriptional profiles in the given tissue 3) Computational deconvolution of multiplets through a maximum likelihood estimation (MLE) to determine the most likely cell type constituents of each multiplet.

scholarly journals metaCOVID: An R-Shiny application for living meta-analyses of COVID-19 trials

2021 ◽  
Author(s):  
Theodoros Evrenoglou ◽  
Isabelle Boutron ◽  
Anna Chaimani
Keyword(s):  
Evidence Synthesis ◽  
Source Code ◽  
Decision Makers ◽  
Sensitivity Analyses ◽  
Preventive Interventions ◽  
Primary Interest ◽  
Link Type ◽  
R Shiny ◽  
Meta Analyses ◽  
Shiny Application

Abstract“Living” evidence synthesis is of primary interest for decision-makers to overcome the COVID-19 pandemic. The COVID-NMA provides open-access living meta-analyses assessing different therapeutic and preventive interventions. Data are posted on a platform (https://covid-nma.com/) and analyses are updated every week. However, guideline developers and other stakeholders also need to investigate the data and perform their own analyses. This requires resources, time, statistical expertise, and software knowledge. To assist them, we created the “metaCOVID” application which, based on automation processes, facilitates the fast exploration of the data and the conduct of analyses tailored to end-users needs. metaCOVID has been created in R and is freely available as an R-Shiny application. The application conducts living meta-analyses for every outcome. Several options are available for subgroup and sensitivity analyses. The results are presented in downloadable forest plots. metaCOVID is freely available from https://covid-nma.com/metacovid/ and the source code from https://github.com/TEvrenoglou/metaCovid.

scholarly journals SPRING: a kinetic interface for visualizing high dimensional single-cell expression data

2016 ◽  
Author(s):  
Caleb Weinreb ◽  
Samuel Wolock ◽  
Allon Klein
Keyword(s):  
Gene Expression ◽  
Single Cell ◽  
Nearest Neighbor ◽  
High Dimensional ◽  
K Nearest Neighbor ◽  
Link Type ◽  
Cell Gene Expression ◽  
Graph Layouts ◽  
Cell Expression ◽  
Cell Data

MotivationSingle-cell gene expression profiling technologies can map the cell states in a tissue or organism. As these technologies become more common, there is a need for computational tools to explore the data they produce. In particular, existing data visualization approaches are imperfect for studying continuous gene expression topologies.ResultsForce-directed layouts of k-nearest-neighbor graphs can visualize continuous gene expression topologies in a manner that preserves high-dimensional relationships and allows manually exploration of different stable two-dimensional representations of the same data. We implemented an interactive web-tool to visualize single-cell data using force-directed graph layouts, called SPRING. SPRING reveals more detailed biological relationships than existing approaches when applied to branching gene expression trajectories from hematopoietic progenitor cells. Visualizations from SPRING are also more reproducible than those of stochastic visualization methods such as tSNE, a state-of-the-art tool.Availabilityhttps://kleintools.hms.harvard.edu/tools/spring.html,https://github.com/AllonKleinLab/SPRING/[email protected], [email protected]

scholarly journals Accurate sub-population detection and mapping across single cell experiments with PopCorn

2018 ◽  
Author(s):  
Yijie Wang ◽  
Jan Hoinka ◽  
Teresa M Przytycka
Keyword(s):  
Comparative Analysis ◽  
Single Cell ◽  
Single Cells ◽  
Novel Method ◽  
Cell Data

The identification of sub-populations of cells present in a sample and the comparison of such sub-populations across samples are among the most frequently performed analyzes of single-cell data. Current tools for these kinds of data, however, fall short in their ability to adequately perform these tasks. We introduce a novel method, PopCorn (single cell sub-Populations Comparison), allowing for the identification of sub-populations of cells present within individual experiments while simultaneously performing sub-populations mapping across these experiments. PopCorn utilizes several novel algorithmic solutions enabling the execution of these tasks with unprecedented precision. As such, PopCorn provides a much-needed tool for comparative analysis of populations of single cells.

scholarly journals GPseudoClust: deconvolution of shared pseudo-profiles at single-cell resolution

2019 ◽  
Author(s):  
Magdalena E Strauss ◽  
Paul DW Kirk ◽  
John E Reid ◽  
Lorenz Wernisch
Keyword(s):  
Single Cell ◽  
Time Course ◽  
Gene Clusters ◽  
Supplementary Information ◽  
Clustering Methods ◽  
Link Type ◽  
Novel Approach ◽  
Broad Array ◽  
Recent Method ◽  
Cell Data

AbstractMotivationMany methods have been developed to cluster genes on the basis of their changes in mRNA expression over time, using bulk RNA-seq or microarray data. However, single-cell data may present a particular challenge for these algorithms, since the temporal ordering of cells is not directly observed. One way to address this is to first use pseudotime methods to order the cells, and then apply clustering techniques for time course data. However, pseudotime estimates are subject to high levels of uncertainty, and failing to account for this uncertainty is liable to lead to erroneous and/or over-confident gene clusters.ResultsThe proposed method, GPseudoClust, is a novel approach that jointly infers pseudotem-poral ordering and gene clusters, and quantifies the uncertainty in both. GPseudoClust combines a recent method for pseudotime inference with nonparametric Bayesian clustering methods, efficient MCMC sampling, and novel subsampling strategies which aid computation. We consider a broad array of simulated and experimental datasets to demonstrate the effectiveness of GPseudoClust in a range of settings.AvailabilityAn implementation is available on GitHub: https://github.com/magStra/nonparametricSummaryPSM and https://github.com/magStra/[email protected] informationSupplementary materials are available.

scholarly journals Single cell network analysis with a mixture of Nested Effects Models

2018 ◽  
Author(s):  
Martin Pirkl ◽  
Niko Beerenwinkel
Keyword(s):  
Single Cell ◽  
New Technologies ◽  
Single Cells ◽  
R Package ◽  
Supplementary Information ◽  
Data Sets ◽  
Cell Network ◽  
A Cell ◽  
Supplementary Material ◽  
Cell Data

AbstractMotivationNew technologies allow for the elaborate measurement of different traits of single cells. These data promise to elucidate intra-cellular networks in unprecedented detail and further help to improve treatment of diseases like cancer. However, cell populations can be very heterogeneous.ResultsWe developed a mixture of Nested Effects Models (M&NEM) for single-cell data to simultaneously identify different cellular sub-populations and their corresponding causal networks to explain the heterogeneity in a cell population. For inference, we assign each cell to a network with a certain probability and iteratively update the optimal networks and cell probabilities in an Expectation Maximization scheme. We validate our method in the controlled setting of a simulation study and apply it to three data sets of pooled CRISPR screens generated previously by two novel experimental techniques, namely Crop-Seq and Perturb-Seq.AvailabilityThe mixture Nested Effects Model (M&NEM) is available as the R-package mnem at https://github.com/cbgethz/mnem/[email protected], [email protected] informationSupplementary data are available.online.

scholarly journals starmapVR: immersive visualisation of single cell spatial omic data

2020 ◽  
Author(s):  
Andrian Yang ◽  
Yu Yao ◽  
Xiunan Fang ◽  
Jianfu Li ◽  
Yongyan Xia ◽  
...  
Keyword(s):  
Single Cell ◽  
Low Cost ◽  
Single Cells ◽  
Three Dimensional ◽  
Supplementary Information ◽  
Phenotypic Properties ◽  
Histological Image ◽  
Link Type ◽  
Molecular Expression ◽  
Omic Data

AbstractMotivationAdvances in high throughput single-cell and spatial omic technologies have enabled the profiling of molecular expression and phenotypic properties of hundreds of thousands of individual cells in the context of their two dimensional (2D) or three dimensional (3D) spatial endogenous arrangement. However, current visualisation techniques do not allow for effective display and exploration of the single cell data in their spatial context. With the widespread availability of low-cost virtual reality (VR) gadgets, such as Google Cardboard, we propose that an immersive visualisation strategy is useful.ResultsWe present starmapVR, a light-weight, cross-platform, web-based tool for visualising single-cell and spatial omic data. starmapVR supports a number of interaction methods, such as keyboard, mouse, wireless controller and voice control. The tool visualises single cells in a 3D space and each cell can be represented by a star plot (for molecular expression, phenotypic properties) or image (for single cell imaging). For spatial transcriptomic data, the 2D single cell expression data can be visualised alongside the histological image in a 2.5D format. The application of starmapVR is demonstrated through a series of case studies. Its scalability has been carefully evaluated across different platforms.Availability and implementationstarmapVR is freely accessible at https://holab-hku.github.io/starmapVR, with the corresponding source code available at https://github.com/holab-hku/starmapVR under the open source MIT license.Supplementary InformationSupplementary data are available at Bioinformatics online.

scholarly journals Cellsnp-lite: an efficient tool for genotyping single cells

2021 ◽  
Author(s):  
Xianjie Huang ◽  
Yuanhua Huang
Keyword(s):  
Single Cell ◽  
Single Cells ◽  
Basic Research ◽  
Substantial Improvement ◽  
Data Sets ◽  
Sequencing Data ◽  
Single Cell Sequencing ◽  
Memory Efficiency ◽  
Computational Speed ◽  
Cell Data

AbstractSummarySingle-cell sequencing is an increasingly used technology and has promising applications in basic research and clinical translations. However, genotyping methods developed for bulk sequencing data have not been well adapted for single-cell data, in terms of both computational parallelization and simplified user interface. Here we introduce a software, cellsnp-lite, implemented in C/C++ and based on well supported package htslib, for genotyping in single-cell sequencing data for both droplet and well based platforms. On various experimental data sets, it shows substantial improvement in computational speed and memory efficiency with retaining highly concordant results compared to existing methods. Cellsnp-lite therefore lightens the genetic analysis for increasingly large single-cell data.AvailabilityThe source code is freely available at https://github.com/single-cell-genetics/[email protected]

scholarly journals Modeling latent flows on single-cell data using the Hodge decomposition

2019 ◽  
Author(s):  
Kazumitsu Maehara ◽  
Yasuyuki Ohkawa
Keyword(s):  
Diffusion Process ◽  
Single Cell ◽  
Trajectory Analysis ◽  
Single Cells ◽  
Hodge Decomposition ◽  
Biological Data ◽  
Graph Representation ◽  
Specific Cell ◽  
Sparse Graph ◽  
Cell Data

AbstractSingle-cell analysis is a powerful technique used to identify a specific cell population of interest during differentiation, aging, or oncogenesis. Individual cells occupy a particular transient state in the cell cycle, circadian rhythm, or during cell death. An appealing concept of pseudo-time trajectory analysis of single-cell RNA sequencing data was proposed in the software Monocle, and several methods of trajectory analysis have since been published to date. These aim to infer the ordering of cells and enable the tracing of gene expression profile trajectories in cell differentiation and reprogramming. However, the methods are restricted in terms of time structure because of the pre-specified structure of trajectories (linear, branched, tree or cyclic) which contrasts with the mixed state of single cells.Here, we propose a technique to extract underlying flows in single-cell data based on the Hodge decomposition (HD). HD is a theorem of vector fields on a manifold which guarantees that any given flow can decompose into three types of orthogonal component: gradient-flow (acyclic), curl-, and harmonic-flow (cyclic). HD is generalized on a simplicial complex (graph) and the discretized HD has only a weak assumption that the graph is directed. Therefore, in principle, HD can extract flows from any mixture of tree and cyclic time flows of observed cells. The decomposed flows provide intuitive interpretations about complex flow because of their linearity and orthogonality. Thus, each extracted flow can be focused on separately with no need to consider crosstalk.We developed ddhodge software, which aims to model the underlying flow structure that implies unobserved time or causal relations in the hodge-podge collection of data points. We demonstrated that the mathematical framework of HD is suitable to reconstruct a sparse graph representation of diffusion process as a candidate model of differentiation while preserving the divergence of the original fully-connected graph. The preserved divergence can be used as an indicator of the source and sink cells in the observed population. A sparse graph representation of the diffusion process transforms data analysis of the non-linear structure embedded in the high-dimensional space of single-cell data into inspection of the visible flow using graph algorithms. Hence, ddhodge is a suitable toolkit to visualize, inspect, and subsequently interpret large data sets including, but not limited to, high-throughput measurements of biological data.The beta version of ddhodge R package is available at:https://github.com/kazumits/ddhodge

scholarly journals Multiplexed Single-Cell in situ RNA Profiling

2021 ◽  
Vol 8 ◽  
Author(s):  
Yu-Sheng Wang ◽  
Jia Guo
Keyword(s):  
Single Cell ◽  
Single Cells ◽  
Disease Diagnosis ◽  
Tissue Architecture ◽  
Rna Profiling ◽  
Rna Analysis ◽  
Technological Advances ◽  
Health And Disease ◽  
Type Classification

The ability to quantify a large number of varied transcripts in single cells in their native spatial context is crucial to accelerate our understanding of health and disease. Bulk cell RNA analysis masks the heterogeneity in the cell population, while the conventional RNA imaging approaches suffer from low multiplexing capacity. Recent advances in multiplexed fluorescence in situ hybridization (FISH) methods enable comprehensive RNA profiling in individual cells in situ. These technologies will have wide applications in many biological and biomedical fields, including cell type classification, signaling network analysis, tissue architecture, disease diagnosis and patient stratification, etc. In this minireview, we will present the recent technological advances of multiplexed single-cell in situ RNA profiling assays, discuss their advantages and limitations, describe their biological applications, highlight the current challenges, and propose potential solutions.

Sign in / Sign up

Export Citation Format

Share Document