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1.
Nat Commun ; 15(1): 3104, 2024 Apr 10.
Article En | MEDLINE | ID: mdl-38600066

During embryonic development, pluripotent cells assume specialized identities by adopting particular gene expression profiles. However, systematically dissecting the relative contributions of mRNA transcription and degradation to shaping those profiles remains challenging, especially within embryos with diverse cellular identities. Here, we combine single-cell RNA-Seq and metabolic labeling to capture temporal cellular transcriptomes of zebrafish embryos where newly-transcribed (zygotic) and pre-existing (maternal) mRNA can be distinguished. We introduce kinetic models to quantify mRNA transcription and degradation rates within individual cell types during their specification. These models reveal highly varied regulatory rates across thousands of genes, coordinated transcription and destruction rates for many transcripts, and link differences in degradation to specific sequence elements. They also identify cell-type-specific differences in degradation, namely selective retention of maternal transcripts within primordial germ cells and enveloping layer cells, two of the earliest specified cell types. Our study provides a quantitative approach to study mRNA regulation during a dynamic spatio-temporal response.


Single-Cell Gene Expression Analysis , Zebrafish , Animals , Embryonic Development/genetics , Transcription, Genetic , RNA, Messenger/genetics , RNA, Messenger/metabolism , Gene Expression Regulation, Developmental
2.
STAR Protoc ; 4(3): 102534, 2023 Sep 15.
Article En | MEDLINE | ID: mdl-37656628

Data normalization is critical to the process of estimating RNA degradation by analyzing RNA levels when transcription is blocked. Here, we present a protocol for measuring mRNA degradation rates, optimized for mouse embryonic stem cells, using α-amanitin inhibitor. We describe steps for a time course α-amanitin treatment, RNA-seq, and alignment; we then detail procedures for analyzing data and sequence enrichment. Our method relies on large-scale normalization of stable transcripts in genomic RNA-seq measurements, providing reliable readouts. For complete details on the use and execution of this protocol, please refer to Viegas et al.1.


Alpha-Amanitin , Mouse Embryonic Stem Cells , Animals , Mice , Alpha-Amanitin/pharmacology , Genomics , RNA/genetics , RNA-Seq
3.
bioRxiv ; 2023 Apr 21.
Article En | MEDLINE | ID: mdl-37131717

During embryonic development, pluripotent cells assume specialized identities by adopting particular gene expression profiles. However, systematically dissecting the underlying regulation of mRNA transcription and degradation remains a challenge, especially within whole embryos with diverse cellular identities. Here, we collect temporal cellular transcriptomes of zebrafish embryos, and decompose them into their newly-transcribed (zygotic) and pre-existing (maternal) mRNA components by combining single-cell RNA-Seq and metabolic labeling. We introduce kinetic models capable of quantifying regulatory rates of mRNA transcription and degradation within individual cell types during their specification. These reveal different regulatory rates between thousands of genes, and sometimes between cell types, that shape spatio-temporal expression patterns. Transcription drives most cell-type restricted gene expression. However, selective retention of maternal transcripts helps to define the gene expression profiles of germ cells and enveloping layer cells, two of the earliest specified cell-types. Coordination between transcription and degradation restricts expression of maternal-zygotic genes to specific cell types or times, and allows the emergence of spatio-temporal patterns when overall mRNA levels are held relatively constant. Sequence-based analysis links differences in degradation to specific sequence motifs. Our study reveals mRNA transcription and degradation events that control embryonic gene expression, and provides a quantitative approach to study mRNA regulation during a dynamic spatio-temporal response.

4.
Dev Cell ; 57(24): 2731-2744.e5, 2022 12 19.
Article En | MEDLINE | ID: mdl-36495875

Embryonic stem cells (ESCs) are self-renewing and pluripotent. In recent years, factors that control pluripotency, mostly nuclear, have been identified. To identify non-nuclear regulators of ESCs, we screened an endogenously labeled fluorescent fusion-protein library in mouse ESCs. One of the more compelling hits was the cell-cycle-associated protein 1 (CAPRIN1). CAPRIN1 knockout had little effect in ESCs, but it significantly altered differentiation and gene expression programs. Using RIP-seq and SLAM-seq, we found that CAPRIN1 associates with, and promotes the degradation of, thousands of RNA transcripts. CAPRIN1 interactome identified XRN2 as the likely ribonuclease. Upon early ESC differentiation, XRN2 is located in the nucleus and colocalizes with CAPRIN1 in small RNA granules in a CAPRIN1-dependent manner. We propose that CAPRIN1 regulates an RNA degradation pathway operating during early ESC differentiation, thus eliminating undesired spuriously transcribed transcripts in ESCs.


Cell Cycle Proteins , Exoribonucleases , Mouse Embryonic Stem Cells , Animals , Mice , Cell Cycle , Cell Cycle Proteins/metabolism , Cell Differentiation , RNA Stability , Exoribonucleases/metabolism
5.
Mon Hefte Math ; 182(3): 577-618, 2017.
Article En | MEDLINE | ID: mdl-32269388

Simultaneous Diophantine approximation is concerned with the approximation of a point x ∈ R d by points r ∈ Q d , with a view towards jointly minimizing the quantities ‖ x - r ‖ and H ( r ) . Here H ( r ) is the so-called "standard height" of the rational point r . In this paper the authors ask: What changes if we replace the standard height function by a different one? As it turns out, this change leads to dramatic differences from the classical theory and requires the development of new methods. We discuss three examples of nonstandard height functions, computing their exponents of irrationality as well as giving more precise results. A list of open questions is also given.

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