Exploring the changing landscape of cell-to-cell variation after CTCF knockdown via single cell RNA-seq

Exploring the changing landscape of cell-to-cell variation after CTCF knockdown via single cell RNA-seq

Abstract Background CCCTC-Binding Factor (CTCF), also known as 11-zinc finger protein, participates in many cellular processes, including insulator activity, transcriptional regulation and organization of chromatin architecture. Based on single cell flow cytometry and single cell RNA-FISH analyses,...

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Main Authors: Wei Wang, Gang Ren, Ni Hong, Wenfei Jin
Format: Article
Language:English
Published: BMC 2019-12-01
Series:BMC Genomics
Subjects:
Single cell RNA-seq
Cell-to-cell variation
CTCF
Change of cellular variation
CTCF knockdown
Online Access:https://doi.org/10.1186/s12864-019-6379-5
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spelling doaj-7dbd09e366bf48128d58609b907cdfd12020-12-27T12:08:34ZengBMCBMC Genomics1471-21642019-12-012011910.1186/s12864-019-6379-5Exploring the changing landscape of cell-to-cell variation after CTCF knockdown via single cell RNA-seqWei Wang0Gang Ren1Ni Hong2Wenfei Jin3Department of Biology, Southern University of Science and TechnologySystems Biology Center, Division of Intramural Research, National Heart, Lung and Blood Institute, National Institutes of HealthDepartment of Biology, Southern University of Science and TechnologyDepartment of Biology, Southern University of Science and TechnologyAbstract Background CCCTC-Binding Factor (CTCF), also known as 11-zinc finger protein, participates in many cellular processes, including insulator activity, transcriptional regulation and organization of chromatin architecture. Based on single cell flow cytometry and single cell RNA-FISH analyses, our previous study showed that deletion of CTCF binding site led to a significantly increase of cellular variation of its target gene. However, the effect of CTCF on genome-wide landscape of cell-to-cell variation remains unclear. Results We knocked down CTCF in EL4 cells using shRNA, and conducted single cell RNA-seq on both wild type (WT) cells and CTCF-Knockdown (CTCF-KD) cells using Fluidigm C1 system. Principal component analysis of single cell RNA-seq data showed that WT and CTCF-KD cells concentrated in two different clusters on PC1, indicating that gene expression profiles of WT and CTCF-KD cells were systematically different. Interestingly, GO terms including regulation of transcription, DNA binding, zinc finger and transcription factor binding were significantly enriched in CTCF-KD-specific highly variable genes, implying tissue-specific genes such as transcription factors were highly sensitive to CTCF level. The dysregulation of transcription factors potentially explains why knockdown of CTCF leads to systematic change of gene expression. In contrast, housekeeping genes such as rRNA processing, DNA repair and tRNA processing were significantly enriched in WT-specific highly variable genes, potentially due to a higher cellular variation of cell activity in WT cells compared to CTCF-KD cells. We further found that cellular variation-increased genes were significantly enriched in down-regulated genes, indicating CTCF knockdown simultaneously reduced the expression levels and increased the expression noise of its regulated genes. Conclusions To our knowledge, this is the first attempt to explore genome-wide landscape of cellular variation after CTCF knockdown. Our study not only advances our understanding of CTCF function in maintaining gene expression and reducing expression noise, but also provides a framework for examining gene function.https://doi.org/10.1186/s12864-019-6379-5Single cell RNA-seqCell-to-cell variationCTCFChange of cellular variationCTCF knockdown
collection DOAJ
language English
format Article
sources DOAJ
author Wei Wang
Gang Ren
Ni Hong
Wenfei Jin
spellingShingle Wei Wang
Gang Ren
Ni Hong
Wenfei Jin
Exploring the changing landscape of cell-to-cell variation after CTCF knockdown via single cell RNA-seq
BMC Genomics
Single cell RNA-seq
Cell-to-cell variation
CTCF
Change of cellular variation
CTCF knockdown
author_facet Wei Wang
Gang Ren
Ni Hong
Wenfei Jin
author_sort Wei Wang
title Exploring the changing landscape of cell-to-cell variation after CTCF knockdown via single cell RNA-seq
title_short Exploring the changing landscape of cell-to-cell variation after CTCF knockdown via single cell RNA-seq
title_full Exploring the changing landscape of cell-to-cell variation after CTCF knockdown via single cell RNA-seq
title_fullStr Exploring the changing landscape of cell-to-cell variation after CTCF knockdown via single cell RNA-seq
title_full_unstemmed Exploring the changing landscape of cell-to-cell variation after CTCF knockdown via single cell RNA-seq
title_sort exploring the changing landscape of cell-to-cell variation after ctcf knockdown via single cell rna-seq
publisher BMC
series BMC Genomics
issn 1471-2164
publishDate 2019-12-01
description Abstract Background CCCTC-Binding Factor (CTCF), also known as 11-zinc finger protein, participates in many cellular processes, including insulator activity, transcriptional regulation and organization of chromatin architecture. Based on single cell flow cytometry and single cell RNA-FISH analyses, our previous study showed that deletion of CTCF binding site led to a significantly increase of cellular variation of its target gene. However, the effect of CTCF on genome-wide landscape of cell-to-cell variation remains unclear. Results We knocked down CTCF in EL4 cells using shRNA, and conducted single cell RNA-seq on both wild type (WT) cells and CTCF-Knockdown (CTCF-KD) cells using Fluidigm C1 system. Principal component analysis of single cell RNA-seq data showed that WT and CTCF-KD cells concentrated in two different clusters on PC1, indicating that gene expression profiles of WT and CTCF-KD cells were systematically different. Interestingly, GO terms including regulation of transcription, DNA binding, zinc finger and transcription factor binding were significantly enriched in CTCF-KD-specific highly variable genes, implying tissue-specific genes such as transcription factors were highly sensitive to CTCF level. The dysregulation of transcription factors potentially explains why knockdown of CTCF leads to systematic change of gene expression. In contrast, housekeeping genes such as rRNA processing, DNA repair and tRNA processing were significantly enriched in WT-specific highly variable genes, potentially due to a higher cellular variation of cell activity in WT cells compared to CTCF-KD cells. We further found that cellular variation-increased genes were significantly enriched in down-regulated genes, indicating CTCF knockdown simultaneously reduced the expression levels and increased the expression noise of its regulated genes. Conclusions To our knowledge, this is the first attempt to explore genome-wide landscape of cellular variation after CTCF knockdown. Our study not only advances our understanding of CTCF function in maintaining gene expression and reducing expression noise, but also provides a framework for examining gene function.
topic Single cell RNA-seq
Cell-to-cell variation
CTCF
Change of cellular variation
CTCF knockdown
url https://doi.org/10.1186/s12864-019-6379-5
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