Project description:BackgroundTime series single-cell RNA sequencing (scRNA-seq) data are emerging. However, the analysis of time series scRNA-seq data could be compromised by 1) distortion created by assorted sources of data collection and generation across time samples and 2) inheritance of cell-to-cell variations by stochastic dynamic patterns of gene expression. This calls for the development of an algorithm able to visualize time series scRNA-seq data in order to reveal latent structures and uncover dynamic transition processes.ResultsIn this study, we propose an algorithm, termed time series elastic embedding (TSEE), by incorporating experimental temporal information into the elastic embedding (EE) method, in order to visualize time series scRNA-seq data. TSEE extends the EE algorithm by penalizing the proximal placement of latent points that correspond to data points otherwise separated by experimental time intervals. TSEE is herein used to visualize time series scRNA-seq datasets of embryonic developmental processed in human and zebrafish. We demonstrate that TSEE outperforms existing methods (e.g. PCA, tSNE and EE) in preserving local and global structures as well as enhancing the temporal resolution of samples. Meanwhile, TSEE reveals the dynamic oscillation patterns of gene expression waves during zebrafish embryogenesis.ConclusionsTSEE can efficiently visualize time series scRNA-seq data by diluting the distortions of assorted sources of data variation across time stages and achieve the temporal resolution enhancement by preserving temporal order and structure. TSEE uncovers the subtle dynamic structures of gene expression patterns, facilitating further downstream dynamic modeling and analysis of gene expression processes. The computational framework of TSEE is generalizable by allowing the incorporation of other sources of information.

Project description:Clustering is a critical step in single cell-based studies. Most existing methods support unsupervised clustering without the a priori exploitation of any domain knowledge. When confronted by the high dimensionality and pervasive dropout events of scRNA-Seq data, purely unsupervised clustering methods may not produce biologically interpretable clusters, which complicates cell type assignment. In such cases, the only recourse is for the user to manually and repeatedly tweak clustering parameters until acceptable clusters are found. Consequently, the path to obtaining biologically meaningful clusters can be ad hoc and laborious. Here we report a principled clustering method named scDCC, that integrates domain knowledge into the clustering step. Experiments on various scRNA-seq datasets from thousands to tens of thousands of cells show that scDCC can significantly improve clustering performance, facilitating the interpretability of clusters and downstream analyses, such as cell type assignment.

Project description:Gene expression over time is, biologically, a continuous process and can thus be represented by a continuous function, i.e. a curve. Individual genes often share similar expression patterns (functional forms). However, the shape of each function, the number of such functions, and the genes that share similar functional forms are typically unknown. Here we introduce an approach that allows direct discovery of related patterns of gene expression and their underlying functions (curves) from data without a priori specification of either cluster number or functional form. Smoothing spline clustering (SSC) models natural properties of gene expression over time, taking into account natural differences in gene expression within a cluster of similarly expressed genes, the effects of experimental measurement error, and missing data. Furthermore, SSC provides a visual summary of each cluster's gene expression function and goodness-of-fit by way of a 'mean curve' construct and its associated confidence bands. We apply this method to gene expression data over the life-cycle of Drosophila melanogaster and Caenorhabditis elegans to discover 17 and 16 unique patterns of gene expression in each species, respectively. New and previously described expression patterns in both species are discovered, the majority of which are biologically meaningful and exhibit statistically significant gene function enrichment. Software and source code implementing the algorithm, SSClust, is freely available (http://genemerge.bioteam.net/SSClust.html).

Project description:Analyzing single-cell RNA sequencing (scRNA-seq) data remains a challenge due to its high dimensionality, sparsity and technical noise. Recognizing the benefits of dimensionality reduction in simplifying complexity and enhancing the signal-to-noise ratio, we introduce scBiG, a novel graph node embedding method designed for representation learning in scRNA-seq data. scBiG establishes a bipartite graph connecting cells and expressed genes, and then constructs a multilayer graph convolutional network to learn cell and gene embeddings. Through a series of extensive experiments, we demonstrate that scBiG surpasses commonly used dimensionality reduction techniques in various analytical tasks. Downstream tasks encompass unsupervised cell clustering, cell trajectory inference, gene expression reconstruction and gene co-expression analysis. Additionally, scBiG exhibits notable computational efficiency and scalability. In summary, scBiG offers a useful graph neural network framework for representation learning in scRNA-seq data, empowering a diverse array of downstream analyses.

Project description:MotivationSingle-cell chromatin accessibility sequencing (scCAS) technology provides an epigenomic perspective to characterize gene regulatory mechanisms at single-cell resolution. With an increasing number of computational methods proposed for analyzing scCAS data, a powerful simulation framework is desirable for evaluation and validation of these methods. However, existing simulators generate synthetic data by sampling reads from real data or mimicking existing cell states, which is inadequate to provide credible ground-truth labels for method evaluation.ResultsWe present simCAS, an embedding-based simulator, for generating high-fidelity scCAS data from both cell- and peak-wise embeddings. We demonstrate simCAS outperforms existing simulators in resembling real data and show that simCAS can generate cells of different states with user-defined cell populations and differentiation trajectories. Additionally, simCAS can simulate data from different batches and encode user-specified interactions of chromatin regions in the synthetic data, which provides ground-truth labels more than cell states. We systematically demonstrate that simCAS facilitates the benchmarking of four core tasks in downstream analysis: cell clustering, trajectory inference, data integration, and cis-regulatory interaction inference. We anticipate simCAS will be a reliable and flexible simulator for evaluating the ongoing computational methods applied on scCAS data.Availability and implementationsimCAS is freely available at https://github.com/Chen-Li-17/simCAS.

Project description:Single-cell RNA-sequencing (scRNA-seq) provides new opportunities to gain a mechanistic understanding of many biological processes. Current approaches for single cell clustering are often sensitive to the input parameters and have difficulty dealing with cell types with different densities. Here, we present Panoramic View (PanoView), an iterative method integrated with a novel density-based clustering, Ordering Local Maximum by Convex hull (OLMC), that uses a heuristic approach to estimate the required parameters based on the input data structures. In each iteration, PanoView will identify the most confident cell clusters and repeat the clustering with the remaining cells in a new PCA space. Without adjusting any parameter in PanoView, we demonstrated that PanoView was able to detect major and rare cell types simultaneously and outperformed other existing methods in both simulated datasets and published single-cell RNA-sequencing datasets. Finally, we conducted scRNA-Seq analysis of embryonic mouse hypothalamus, and PanoView was able to reveal known cell types and several rare cell subpopulations.

Project description:MotivationGenetic intra-tumor heterogeneity (ITH) characterizes the differences in genomic variations between tumor clones, and accurately unmasking ITH is important for personalized cancer therapy. Single-cell DNA sequencing now emerges as a powerful means for deciphering underlying ITH based on point mutations of single cells. However, detecting tumor clones from single-cell mutation data remains challenging due to the error-prone and discrete nature of the data.ResultsWe introduce bmVAE, a bioinformatics tool for learning low-dimensional latent representation of single cell based on a variational autoencoder and then clustering cells into subpopulations in the latent space. bmVAE takes single-cell binary mutation data as inputs, and outputs inferred cell subpopulations as well as their genotypes. To achieve this, the bmVAE framework is designed to consist of three modules including dimensionality reduction, cell clustering and genotype estimation. We assess the method on various synthetic datasets where different factors including false negative rate, data size and data heterogeneity are considered in simulation, and further demonstrate its effectiveness on two real datasets. The results suggest bmVAE is highly effective in reasoning ITH, and performs competitive to existing methods.Availability and implementationbmVAE is freely available at https://github.com/zhyu-lab/bmvae.Supplementary informationSupplementary data are available at Bioinformatics online.

Project description:Single-cell RNA sequencing technologies have enabled us to study tissue heterogeneity at cellular resolution. Fast-developing sequencing platforms like droplet-based sequencing make it feasible to parallel process thousands of single cells effectively. Although a unique molecular identifier (UMI) can remove bias from amplification noise to a certain extent, clustering for such sparse and high-dimensional large-scale discrete data remains intractable and challenging. Most existing deep learning-based clustering methods utilize the mean square error or negative binomial distribution with or without zero inflation to denoise single-cell UMI count data, which may underfit or overfit the gene expression profiles. In addition, neglecting the molecule sampling mechanism and extracting representation by simple linear dimension reduction with a hard clustering algorithm may distort data structure and lead to spurious analytical results. In this paper, we combined the deep autoencoder technique with statistical modeling and developed a novel and effective clustering method, scDMFK, for single-cell transcriptome UMI count data. ScDMFK utilizes multinomial distribution to characterize data structure and draw support from neural network to facilitate model parameter estimation. In the learned low-dimensional latent space, we proposed an adaptive fuzzy k-means algorithm with entropy regularization to perform soft clustering. Various simulation scenarios and the analysis of 10 real datasets have shown that scDMFK outperforms other state-of-the-art methods with respect to data modeling and clustering algorithms. Besides, scDMFK has excellent scalability for large-scale single-cell datasets.

Project description:Gene clustering is one of the important techniques to identify co-expressed gene groups from gene expression data, which provides a powerful tool for investigating functional relationships of genes in biological process. Self-training is a kind of important semi-supervised learning method and has exhibited good performance on gene clustering problem. However, the self-training process inevitably suffers from mislabeling, the accumulation of which will lead to the degradation of semi-supervised learning performance of gene expression data. To solve the problem, this paper proposes a self-training subspace clustering algorithm based on adaptive confidence for gene expression data (SSCAC), which combines the low-rank representation of gene expression data and adaptive adjustment of label confidence to better guide the partition of unlabeled data. The superiority of the proposed SSCAC algorithm is mainly reflected in the following aspects. 1) In order to improve the discriminative property of gene expression data, the low-rank representation with distance penalty is used to mine the potential subspace structure of data. 2) Considering the problem of mislabeling in self-training, a semi-supervised clustering objective function with label confidence is proposed, and a self-training subspace clustering framework is constructed on this basis. 3) In order to mitigate the negative impact of mislabeled data, an adaptive adjustment strategy based on gravitational search algorithm is proposed for label confidence. Compared with a variety of state-of-the-art unsupervised and semi-supervised learning algorithms, the SSCAC algorithm has demonstrated its superiority through extensive experiments on two benchmark gene expression datasets.

Project description:Single-cell multimodal sequencing technologies are developed to simultaneously profile different modalities of data in the same cell. It provides a unique opportunity to jointly analyze multimodal data at the single-cell level for the identification of distinct cell types. A correct clustering result is essential for the downstream complex biological functional studies. However, combining different data sources for clustering analysis of single-cell multimodal data remains a statistical and computational challenge. Here, we develop a novel multimodal deep learning method, scMDC, for single-cell multi-omics data clustering analysis. scMDC is an end-to-end deep model that explicitly characterizes different data sources and jointly learns latent features of deep embedding for clustering analysis. Extensive simulation and real-data experiments reveal that scMDC outperforms existing single-cell single-modal and multimodal clustering methods on different single-cell multimodal datasets. The linear scalability of running time makes scMDC a promising method for analyzing large multimodal datasets.