scholarly journals Machine Learning-Assisted Identification of Factors Contributing to the Technical Variability Between Bulk and Single-Cell RNA-Seq Experiments

2022 ◽  
Author(s):  
Sofya Lipnitskaya ◽  
Yang Shen ◽  
Stefan Legewie ◽  
Holger Klein ◽  
Kolja Becker
Keyword(s):  
Gene Expression ◽  
Machine Learning ◽  
Single Cell ◽  
Rna Sequencing ◽  
Quantitative Difference ◽  
Rna Seq ◽  
Sequencing Data ◽  
Factors Affecting ◽  
Expression Variability ◽  
Technical Variability

Abstract Background: Recent studies in the area of transcriptomics performed on single-cell and population levels reveal noticeable variability in gene expression measurements provided by different RNA sequencing technologies. Due to increased noise and complexity of single-cell RNA-Seq (scRNA-Seq) data over the bulk experiment, there is a substantial number of variably-expressed genes and so-called dropouts, challenging the subsequent computational analysis and potentially leading to false positive discoveries. In order to investigate factors affecting technical variability between RNA sequencing experiments of different technologies, we performed a systematic assessment of single-cell and bulk RNA-Seq data, which have undergone the same pre-processing and sample preparation procedures. Results: Our analysis indicates that variability between gene expression measurements as well as dropout events are not exclusively caused by biological variability, low expression levels, or random variation. Furthermore, we propose FAVSeq, a machine learning-assisted pipeline for detection of factors contributing to gene expression variability in matched RNA-Seq data provided by two technologies. Based on the analysis of the matched bulk and single-cell dataset, we found the 3'-UTR and transcript lengths as the most relevant effectors of the observed variation between RNA-Seq experiments, while the same factors together with cellular compartments were shown to be associated with dropouts. Conclusions: Here, we investigated the sources of variation in RNA-Seq profiles of matched single-cell and bulk experiments. In addition, we proposed the FAVSeq pipeline for analyzing multimodal RNA sequencing data, which allowed to identify factors affecting quantitative difference in gene expression measurements as well as the presence of dropouts. Hereby, the derived knowledge can be employed further in order to improve the interpretation of RNA-Seq data and identify genes that can be affected by assay-based deviations. Source code is available under the MIT license at https://github.com/slipnitskaya/FAVSeq.

scholarly journals Machine learning-assisted identification of factors contributing to the technical variability between bulk and single-cell RNA-seq experiments

2022 ◽  
Author(s):  
Sofya Lipnitskaya ◽  
Yang Shen ◽  
Stefan Legewie ◽  
Holger Klein ◽  
Kolja Becker
Keyword(s):  
Gene Expression ◽  
Machine Learning ◽  
Single Cell ◽  
Rna Sequencing ◽  
Quantitative Difference ◽  
Rna Seq ◽  
Sequencing Data ◽  
Factors Affecting ◽  
Expression Variability ◽  
Technical Variability

Background: Recent studies in the area of transcriptomics performed on single-cell and population levels reveal noticeable variability in gene expression measurements provided by different RNA sequencing technologies. Due to increased noise and complexity of single-cell RNA-Seq (scRNA-Seq) data over the bulk experiment, there is a substantial number of variably-expressed genes and so-called dropouts, challenging the subsequent computational analysis and potentially leading to false positive discoveries. In order to investigate factors affecting technical variability between RNA sequencing experiments of different technologies, we performed a systematic assessment of single-cell and bulk RNA-Seq data, which have undergone the same pre-processing and sample preparation procedures. Results: Our analysis indicates that variability between gene expression measurements as well as dropout events are not exclusively caused by biological variability, low expression levels, or random variation. Furthermore, we propose FAVSeq, a machine learning-assisted pipeline for detection of factors contributing to gene expression variability in matched RNA-Seq data provided by two technologies. Based on the analysis of the matched bulk and single-cell dataset, we found the 3'-UTR and transcript lengths as the most relevant effectors of the observed variation between RNA-Seq experiments, while the same factors together with cellular compartments were shown to be associated with dropouts. Conclusions: Here, we investigated the sources of variation in RNA-Seq profiles of matched single-cell and bulk experiments. In addition, we proposed the FAVSeq pipeline for analyzing multimodal RNA sequencing data, which allowed to identify factors affecting quantitative difference in gene expression measurements as well as the presence of dropouts. Hereby, the derived knowledge can be employed further in order to improve the interpretation of RNA-Seq data and identify genes that can be affected by assay-based deviations. Source code is available under the MIT license at https://github.com/slipnitskaya/FAVSeq.

scholarly journals SPsimSeq: semi-parametric simulation of bulk and single cell RNA sequencing data

2019 ◽  
Author(s):  
Alemu Takele Assefa ◽  
Jo Vandesompele ◽  
Olivier Thas
Keyword(s):  
Gene Expression ◽  
Single Cell ◽  
Rna Sequencing ◽  
Empirical Distribution ◽  
Supplementary Information ◽  
Rna Seq ◽  
Sequencing Data ◽  
Actual Distribution ◽  
Wide Range ◽  
Single Cell Rna Sequencing

SummarySPsimSeq is a semi-parametric simulation method for bulk and single cell RNA sequencing data. It simulates data from a good estimate of the actual distribution of a given real RNA-seq dataset. In contrast to existing approaches that assume a particular data distribution, our method constructs an empirical distribution of gene expression data from a given source RNA-seq experiment to faithfully capture the data characteristics of real data. Importantly, our method can be used to simulate a wide range of scenarios, such as single or multiple biological groups, systematic variations (e.g. confounding batch effects), and different sample sizes. It can also be used to simulate different gene expression units resulting from different library preparation protocols, such as read counts or UMI counts.Availability and implementationThe R package and associated documentation is available from https://github.com/CenterForStatistics-UGent/SPsimSeq.Supplementary informationSupplementary data are available at bioRχiv online.

scholarly journals CCSN: Single Cell RNA Sequencing Data Analysis by Conditional Cell-specific Network

2020 ◽  
Author(s):  
Lin Li ◽  
Hao Dai ◽  
Zhaoyuan Fang ◽  
Luonan Chen
Keyword(s):  
Gene Expression ◽  
Single Cell ◽  
Rna Sequencing ◽  
Network Flow ◽  
Single Cells ◽  
Cellular Heterogeneity ◽  
Rna Seq ◽  
Sequencing Data ◽  
Cell Clustering ◽  
A Cell

AbstractThe rapid advancement of single cell technologies has shed new light on the complex mechanisms of cellular heterogeneity. However, compared with bulk RNA sequencing (RNA-seq), single-cell RNA-seq (scRNA-seq) suffers from higher noise and lower coverage, which brings new computational difficulties. Based on statistical independence, cell-specific network (CSN) is able to quantify the overall associations between genes for each cell, yet suffering from a problem of overestimation related to indirect effects. To overcome this problem, we propose the “conditional cell-specific network” (CCSN) method, which can measure the direct associations between genes by eliminating the indirect associations. CCSN can be used for cell clustering and dimension reduction on a network basis of single cells. Intuitively, each CCSN can be viewed as the transformation from less “reliable” gene expression to more “reliable” gene-gene associations in a cell. Based on CCSN, we further design network flow entropy (NFE) to estimate the differentiation potency of a single cell. A number of scRNA-seq datasets were used to demonstrate the advantages of our approach: (1) one direct association network for one cell; (2) most existing scRNA-seq methods designed for gene expression matrices are also applicable to CCSN-transformed degree matrices; (3) CCSN-based NFE helps resolving the direction of differentiation trajectories by quantifying the potency of each cell. CCSN is publicly available at http://sysbio.sibcb.ac.cn/cb/chenlab/soft/CCSN.zip.

scholarly journals QUBIC2: A novel biclustering algorithm for large-scale bulk RNA-sequencing and single-cell RNA-sequencing data analysis

2018 ◽  
Author(s):  
Juan Xie ◽  
Anjun Ma ◽  
Yu Zhang ◽  
Bingqiang Liu ◽  
Changlin Wan ◽  
...  
Keyword(s):  
Gene Expression ◽  
Transcriptional Regulation ◽  
Single Cell ◽  
Rna Sequencing ◽  
Spatial Data ◽  
Large Scale ◽  
Biological Information ◽  
Superior Performance ◽  
Rna Seq ◽  
Sequencing Data

ABSTRACTThe combination of biclustering and large-scale gene expression data holds a promising potential for inference of the condition specific functional pathways/networks. However, existing biclustering tools do not have satisfied performance on high-resolution RNA-sequencing (RNA-Seq) data, majorly due to the lack of (i) a consideration of high sparsity of RNA-Seq data, e.g., the massive zeros or lowly expressed genes in the data, especially for single-cell RNA-Seq (scRNA-Seq) data, and (ii) an understanding of the underlying transcriptional regulation signals of the observed gene expression values. Here we presented a novel biclustering algorithm namely QUBIC2, for the analysis of large-scale bulk RNA-Seq and scRNA-Seq data. Key novelties of the algorithm include (i) used a truncated model to handle the unreliable quantification of genes with low or moderate expression, (ii) adopted the mixture Gaussian distribution and an information-divergency objective function to capture shared transcriptional regulation signals among a set of genes, (iii) utilized a Core-Dual strategy to identify biclusters and optimize relevant parameters, and (iv) developed a size-based P-value framework to evaluate the statistical significances of all the identified biclusters. Our method validation on comprehensive data sets of bulk and single cell RNA-seq data suggests that QUBIC2 had superior performance in functional modules detection and cell type classification compared with the other five widely-used biclustering tools. In addition, the applications of temporal and spatial data demonstrated that QUBIC2 can derive meaningful biological information from scRNA-Seq data. The source code for QUBIC2 can be freely accessed at https://github.com/maqin2001/qubic2.

scholarly journals Single-Cell Transcriptome Analysis Reveals Dynamic Cell Populations and Differential Gene Expression Patterns in Control and Aneurysmal Human Aortic Tissue

Circulation ◽  
2020 ◽  
Vol 142 (14) ◽  
pp. 1374-1388
Author(s):  
Yanming Li ◽  
Pingping Ren ◽  
Ashley Dawson ◽  
Hernan G. Vasquez ◽  
Waleed Ageedi ◽  
...  
Keyword(s):  
Gene Expression ◽  
Single Cell ◽  
Rna Sequencing ◽  
Aortic Wall ◽  
Genome Wide Association ◽  
Aortic Tissue ◽  
Sequencing Data ◽  
Genome Wide ◽  
Single Cell Rna Sequencing ◽  
Differential Gene

Background: Ascending thoracic aortic aneurysm (ATAA) is caused by the progressive weakening and dilatation of the aortic wall and can lead to aortic dissection, rupture, and other life-threatening complications. To improve our understanding of ATAA pathogenesis, we aimed to comprehensively characterize the cellular composition of the ascending aortic wall and to identify molecular alterations in each cell population of human ATAA tissues. Methods: We performed single-cell RNA sequencing analysis of ascending aortic tissues from 11 study participants, including 8 patients with ATAA (4 women and 4 men) and 3 control subjects (2 women and 1 man). Cells extracted from aortic tissue were analyzed and categorized with single-cell RNA sequencing data to perform cluster identification. ATAA-related changes were then examined by comparing the proportions of each cell type and the gene expression profiles between ATAA and control tissues. We also examined which genes may be critical for ATAA by performing the integrative analysis of our single-cell RNA sequencing data with publicly available data from genome-wide association studies. Results: We identified 11 major cell types in human ascending aortic tissue; the high-resolution reclustering of these cells further divided them into 40 subtypes. Multiple subtypes were observed for smooth muscle cells, macrophages, and T lymphocytes, suggesting that these cells have multiple functional populations in the aortic wall. In general, ATAA tissues had fewer nonimmune cells and more immune cells, especially T lymphocytes, than control tissues did. Differential gene expression data suggested the presence of extensive mitochondrial dysfunction in ATAA tissues. In addition, integrative analysis of our single-cell RNA sequencing data with public genome-wide association study data and promoter capture Hi-C data suggested that the erythroblast transformation-specific related gene( ERG ) exerts an important role in maintaining normal aortic wall function. Conclusions: Our study provides a comprehensive evaluation of the cellular composition of the ascending aortic wall and reveals how the gene expression landscape is altered in human ATAA tissue. The information from this study makes important contributions to our understanding of ATAA formation and progression.

scholarly journals SSCC: a novel computational framework for rapid and accurate clustering large single cell RNA-seq data

2018 ◽  
Author(s):  
Xianwen Ren ◽  
Liangtao Zheng ◽  
Zemin Zhang
Keyword(s):  
Single Cell ◽  
Rna Sequencing ◽  
Large Scale ◽  
Random Projection ◽  
Rna Seq ◽  
Sequencing Data ◽  
Computational Framework ◽  
Human Blood Cells ◽  
Single Cell Rna Sequencing ◽  
Data Volume

ABSTRACTClustering is a prevalent analytical means to analyze single cell RNA sequencing data but the rapidly expanding data volume can make this process computational challenging. New methods for both accurate and efficient clustering are of pressing needs. Here we proposed a new clustering framework based on random projection and feature construction for large scale single-cell RNA sequencing data, which greatly improves clustering accuracy, robustness and computational efficacy for various state-of-the-art algorithms benchmarked on multiple real datasets. On a dataset with 68,578 human blood cells, our method reached 20% improvements for clustering accuracy and 50-fold acceleration but only consumed 66% memory usage compared to the widely-used software package SC3. Compared to k-means, the accuracy improvement can reach 3-fold depending on the concrete dataset. An R implementation of the framework is available from https://github.com/Japrin/sscClust.

scholarly journals Splatter: simulation of single-cell RNA sequencing data

2017 ◽  
Author(s):  
Luke Zappia ◽  
Belinda Phipson ◽  
Alicia Oshlack
Keyword(s):  
Single Cell ◽  
Rna Sequencing ◽  
Real Data ◽  
Cell Types ◽  
Rna Seq ◽  
Sequencing Data ◽  
Sequencing Technologies ◽  
Simulation Based ◽  
Single Cell Rna Sequencing ◽  
Multiple Cell

AbstractAs single-cell RNA sequencing technologies have rapidly developed, so have analysis methods. Many methods have been tested, developed and validated using simulated datasets. Unfortunately, current simulations are often poorly documented, their similarity to real data is not demonstrated, or reproducible code is not available.Here we present the Splatter Bioconductor package for simple, reproducible and well-documented simulation of single-cell RNA-seq data. Splatter provides an interface to multiple simulation methods including Splat, our own simulation, based on a gamma-Poisson distribution. Splat can simulate single populations of cells, populations with multiple cell types or differentiation paths.

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