Localization and abundance analysis of human lncRNAs at single-cell and single-molecule resolution

Cabili, Moran N.; Dunagin, Margaret C.; McClanahan, Patrick D.; Biaesch, Andrew G.; Padovan-Merhar, Olivia; Regev, Aviv; Rinn, John L.; Raj, Arjun

doi:10.1186/s13059-015-0586-4

Cited by 612 publications

(582 citation statements)

References 76 publications

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“…Briefly, the data were preprocessed with the read trimming and cropping tool Trimmomatic v.0.30 (83) (85) with the command line parameters: −no-coverage-search-b2-sensitive (Dataset S2). Uniquely mapped reads were counted with htseq-count v.0.6.1p1 and GTF transcriptome annotation file downloaded from GEO accession GSE57049 (86). Gene expression levels were calculated in FPKM, considering gene length as a sum of all exonic nonoverlapping sequences of all isoforms of a given gene.…”

Section: Methodsmentioning

confidence: 99%

Vulnerability of primitive human placental trophoblast to Zika virus

Sheridan

Yunusov

Balaraman

et al. 2017

Proc. Natl. Acad. Sci. U.S.A.

157

155

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Infection of pregnant women by Asian lineage strains of Zika virus (ZIKV) has been linked to brain abnormalities in their infants, yet it is uncertain when during pregnancy the human conceptus is most vulnerable to the virus. We have examined two models to study susceptibility of human placental trophoblast to ZIKV: cytotrophoblast and syncytiotrophoblast derived from placental villi at term and colonies of trophoblast differentiated from embryonic stem cells (ESC). The latter appear to be analogous to the primitive placenta formed during implantation. The cells from term placentas, which resist infection, do not express genes encoding most attachment factors implicated in ZIKV entry but do express many genes associated with antiviral defense. By contrast, the ESC-derived trophoblasts possess a wide range of attachment factors for ZIKV entry and lack components of a robust antiviral response system. These cells, particularly areas of syncytiotrophoblast within the colonies, quickly become infected, produce infectious virus and undergo lysis within 48 h after exposure to low titers (multiplicity of infection > 0.07) of an African lineage strain (MR766 Uganda: ZIKVU) considered to be benign with regards to effects on fetal development. Unexpectedly, lytic effects required significantly higher titers of the presumed more virulent FSS13025 Cambodia (ZIKVC). Our data suggest that the developing fetus might be most vulnerable to ZIKV early in the first trimester before a protective zone of mature villous trophoblast has been established. Additionally, MR766 is highly trophic toward primitive trophoblast, which may put the early conceptus of an infected mother at high risk for destruction.

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Section: Methodsmentioning

confidence: 99%

Vulnerability of primitive human placental trophoblast to Zika virus

Sheridan

Yunusov

Balaraman

et al. 2017

Proc. Natl. Acad. Sci. U.S.A.

157

155

View full text Add to dashboard Cite

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“…Cabili et al ., made use of two pools of probes labelled with different fluorophores and co‐localizing the signals obtained using the two probe sets. If the signals co‐localize, then they are construed as true ones indicating the lncRNA localizations, otherwise at least some of the signals are considered to be due to off‐target hybridizations 46 (Table 1). …”

Section: Methods Used To Localize Lncrnas Inside the Cellmentioning

confidence: 99%

State of the art technologies to explore long non‐coding RNAs in cancer

Salehi

Taheri

Azarpira

et al. 2017

J Cellular Molecular Medi

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Long non‐coding RNAs (lncRNAs) comprise a vast repertoire of RNAs playing a wide variety of crucial roles in tissue physiology in a cell‐specific manner. Despite being engaged in myriads of regulatory mechanisms, many lncRNAs have still remained to be assigned any functions. A constellation of experimental techniques including single‐molecule RNA in situ hybridization (sm‐RNA FISH), cross‐linking and immunoprecipitation (CLIP), RNA interference (RNAi), Clustered regularly interspaced short palindromic repeats (CRISPR) and so forth has been employed to shed light on lncRNA cellular localization, structure, interaction networks and functions. Here, we review these and other experimental approaches in common use for identification and characterization of lncRNAs, particularly those involved in different types of cancer, with focus on merits and demerits of each technique.

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“…This approach targets individual transcripts by up to 40 different oligonucleotides, which are directly conjugated to fluorophores. While a recent study achieved to monitor 61 different ncRNAs, it had to restrict itself to "a few dozen cells … due to limited imaging throughput" [12]. Possibly, this reflects the lower signal-to-noise ratio of single fluorescent spots of o-nuc sm-FISH and their need for a 600 times longer illumination time [4].…”

Section: Alternative Methods For Rna Detection In Imagingmentioning

confidence: 99%

Computer vision for image-based transcriptomics

Stoeger

Battich

Herrmann

et al. 2015

Methods

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Single-cell transcriptomics has recently emerged as one of the most promising tools for understanding the diversity of the transcriptome among single cells. Image-based transcriptomics is unique compared to other methods as it does not require conversion of RNA to cDNA prior to signal amplification and transcript quantification. Thus, its efficiency in transcript detection is unmatched by other methods. In addition, image-based transcriptomics allows the study of the spatial organization of the transcriptome in single cells at single-molecule, and, when combined with superresolution microscopy, nanometer resolution. However, in order to unlock the full power of image-based transcriptomics, robust computer vision of single molecules and cells is required. Here, we shortly discuss the setup of the experimental pipeline for image-based transcriptomics, and then describe in detail the algorithms that we developed to extract, at high-throughput, robust multivariate feature sets of transcript molecule abundance, localization and patterning in tens of thousands of single cells across the transcriptome. These computer vision algorithms and pipelines can be downloaded from: https://github.com/pelkmanslab/ImageBasedTranscriptomics. AbstractSingle-cell transcriptomics has recently emerged as one of the most promising tools for

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Localization and abundance analysis of human lncRNAs at single-cell and single-molecule resolution

Cited by 612 publications

References 76 publications

Vulnerability of primitive human placental trophoblast to Zika virus

Vulnerability of primitive human placental trophoblast to Zika virus

State of the art technologies to explore long non‐coding RNAs in cancer

Computer vision for image-based transcriptomics

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