scholarly journals Extrinsic noise prevents the independent tuning of gene expression noise and protein mean abundance in bacteria

2020 ◽  
Vol 6 (41) ◽  
pp. eabc3478
Author(s):  
A. Deloupy ◽  
V. Sauveplane ◽  
J. Robert ◽  
S. Aymerich ◽  
M. Jules ◽  
...  
Keyword(s):  
Gene Expression ◽  
Fluorescent Protein ◽  
Biological Engineering ◽  
Translation Control ◽  
Extrinsic Noise ◽  
Translation Rate ◽  
Gene Expression Noise ◽  
Expression Noise ◽  
Noise Optimization ◽  
Custom Made

It is generally accepted that prokaryotes can tune gene expression noise independently of protein mean abundance by varying the relative levels of transcription and translation. Here, we address this question quantitatively, using a custom-made library of 40 Bacillus subtilis strains expressing a fluorescent protein under the control of different transcription and translation control elements. We quantify noise and mean protein abundance by fluorescence microscopy and show that for most of the natural transcription range of B. subtilis, expression noise is equally sensitive to variations in the transcription or translation rate because of the prevalence of extrinsic noise. In agreement, analysis of whole-genome transcriptomic and proteomic datasets suggests that noise optimization through transcription and translation tuning during evolution may only occur in a regime of weak transcription. Therefore, independent control of mean abundance and noise can rarely be achieved, which has strong implications for both genome evolution and biological engineering.

scholarly journals Plasmids for Independently Tunable, Low-Noise Expression of Two Genes

mSphere ◽  
2019 ◽  
Vol 4 (3) ◽  
Author(s):  
João P. N. Silva ◽  
Soraia Vidigal Lopes ◽  
Diogo J. Grilo ◽  
Zach Hensel
Keyword(s):  
Gene Expression ◽  
Protein Expression ◽  
Low Noise ◽  
Expression Systems ◽  
Extrinsic Noise ◽  
Gene Expression Noise ◽  
Expression Noise ◽  
Foreign Proteins ◽  
Noise Limit ◽  
Cell Variation

ABSTRACTSome microbiology experiments and biotechnology applications can be improved if it is possible to tune the expression of two different genes at the same time with cell-to-cell variation at or below the level of genes constitutively expressed from the chromosome (the “extrinsic noise limit”). This was recently achieved for a single gene by exploiting negative autoregulation by the tetracycline repressor (TetR) and bicistronic gene expression to reduce gene expression noise. We report new plasmids that use the same principles to achieve simultaneous, low-noise expression for two genes inEscherichia coli. The TetR system was moved to a compatible plasmid backbone, and a system based on thelacrepressor (LacI) was found to also exhibit gene expression noise below the extrinsic noise limit. We characterized gene expression mean and noise across the range of induction levels for these plasmids, applied the LacI system to tune expression for single-molecule mRNA detection under two different growth conditions, and showed that two plasmids can be cotransformed to independently tune expression of two different genes.IMPORTANCEMicrobiologists often express foreign proteins in bacteria in order study them or to use bacteria as a microbial factory. Usually, this requires controlling the number of foreign proteins expressed in each cell, but for many common protein expression systems, it is difficult to “tune” protein expression without large cell-to-cell variation in expression levels (called “noise” in protein expression). This work describes two protein expression systems that can be combined in the same cell, with tunable expression levels and very low protein expression noise. One new system was used to detect single mRNA molecules by fluorescence microscopy, and the two systems were shown to be independent of each other. These protein expression systems may be useful in any experiment or biotechnology application that can be improved with low protein expression noise.

scholarly journals Plasmids for independently tunable, low-noise expression of two genes

2019 ◽  
Author(s):  
João P. N. Silva ◽  
Soraia Vidigal Lopes ◽  
Diogo J. Grilo ◽  
Zach Hensel
Keyword(s):  
Gene Expression ◽  
Single Molecule ◽  
Single Gene ◽  
Growth Conditions ◽  
Low Noise ◽  
Extrinsic Noise ◽  
Gene Expression Noise ◽  
Expression Noise ◽  
Compatible Plasmid ◽  
Noise Limit

AbstractSome microbiology experiments and biotechnology applications can be improved if it is possible to tune the expression of two different genes at the same time with cell-to-cell variation at or below the level of genes constitutively expressed from the chromosome (the “extrinsic noise limit”). This was recently achieved for a single gene by exploiting negative autoregulation by the tetracycline repressor (TetR) and bicistronic gene expression to reduce gene expression noise. We report new plasmids that use the same principles to achieve simultaneous, low-noise expression for two genes. The TetR system was moved to a compatible plasmid backbone, and a system based on the lac repressor (LacI) was found to also exhibit gene expression noise below the extrinsic noise limit. We characterize gene expression mean and noise across the range of induction levels for these plasmids, apply the LacI system to tune expression for single-molecule mRNA detection in two different growth conditions, and show that two plasmids can be co-transformed to independently tune expression of two different genes.

scholarly journals Coordination of gene expression noise with cell size: analytical results for agent-based models of growing cell populations

2021 ◽  
Vol 18 (178) ◽  
pp. 20210274
Author(s):  
Philipp Thomas ◽  
Vahid Shahrezaei
Keyword(s):  
Gene Expression ◽  
Master Equation ◽  
Cell Size ◽  
Chemical Master Equation ◽  
Gillespie Algorithm ◽  
Agent Based Models ◽  
Extrinsic Noise ◽  
Gene Expression Noise ◽  
Agent Based ◽  
Expression Noise

The chemical master equation and the Gillespie algorithm are widely used to model the reaction kinetics inside living cells. It is thereby assumed that cell growth and division can be modelled through effective dilution reactions and extrinsic noise sources. We here re-examine these paradigms through developing an analytical agent-based framework of growing and dividing cells accompanied by an exact simulation algorithm, which allows us to quantify the dynamics of virtually any intracellular reaction network affected by stochastic cell size control and division noise. We find that the solution of the chemical master equation—including static extrinsic noise—exactly agrees with the agent-based formulation when the network under study exhibits stochastic concentration homeostasis , a novel condition that generalizes concentration homeostasis in deterministic systems to higher order moments and distributions. We illustrate stochastic concentration homeostasis for a range of common gene expression networks. When this condition is not met, we demonstrate by extending the linear noise approximation to agent-based models that the dependence of gene expression noise on cell size can qualitatively deviate from the chemical master equation. Surprisingly, the total noise of the agent-based approach can still be well approximated by extrinsic noise models.

scholarly journals Uncoupling gene expression noise along the central dogma using genome engineered human cell lines

2020 ◽  
Vol 48 (16) ◽  
pp. 9406-9413 ◽  
Author(s):  
Tyler Quarton ◽  
Taek Kang ◽  
Vasileios Papakis ◽  
Khai Nguyen ◽  
Chance Nowak ◽  
...  
Keyword(s):  
Gene Expression ◽  
Protein Synthesis ◽  
Reporter System ◽  
Extrinsic Noise ◽  
Cell Content ◽  
Gene Expression Noise ◽  
Central Dogma ◽  
Expression Noise ◽  
Global Correlation ◽  
Noise In Gene Expression

Abstract Eukaryotic protein synthesis is an inherently stochastic process. This stochasticity stems not only from variations in cell content between cells but also from thermodynamic fluctuations in a single cell. Ultimately, these inherently stochastic processes manifest as noise in gene expression, where even genetically identical cells in the same environment exhibit variation in their protein abundances. In order to elucidate the underlying sources that contribute to gene expression noise, we quantify the contribution of each step within the process of protein synthesis along the central dogma. We uncouple gene expression at the transcriptional, translational, and post-translational level using custom engineered circuits stably integrated in human cells using CRISPR. We provide a generalized framework to approximate intrinsic and extrinsic noise in a population of cells expressing an unbalanced two-reporter system. Our decomposition shows that the majority of intrinsic fluctuations stem from transcription and that coupling the two genes along the central dogma forces the fluctuations to propagate and accumulate along the same path, resulting in increased observed global correlation between the products.

scholarly journals Coordination of gene expression noise with cell size: extrinsic noise versus agent-based models of growing cell populations

2020 ◽  
Author(s):  
Philipp Thomas ◽  
Vahid Shahrezaei
Keyword(s):  
Gene Expression ◽  
Master Equation ◽  
Cell Size ◽  
Chemical Master Equation ◽  
Simulation Algorithm ◽  
Agent Based Models ◽  
Extrinsic Noise ◽  
Gene Expression Noise ◽  
Agent Based ◽  
Expression Noise

The chemical master equation and the stochastic simulation algorithm are widely used to model the reaction kinetics inside living cells. It is thereby assumed that cell growth and division can be modelled for through effective dilution reactions and extrinsic noise sources. We here re-examine these paradigms through developing an analytical agent-based framework of growing and dividing cells accompanied by an exact simulation algorithm, which allows us to quantify the dynamics of virtually any intracellular reaction network affected by stochastic cell size control and division noise in a growing population. We find that the solution of the chemical master equation – including static extrinsic noise – exactly agrees with the one of the agent-based formulation when a simple condition on the network’s topology is met. We illustrate this result for a range of common gene expression networks. When these conditions are not met, we demonstrate using analytical solutions of the agent-based models that the dependence of gene expression noise on cell size can qualitatively deviate from the effective master equation. Surprisingly, the latter distorts total noise in gene regulatory networks by at most 8% independently of network parameters. Our results highlight the accuracy of extrinsic noise modelling within the chemical master equation framework.

Reduction in gene expression noise by targeted increase in accessibility at gene loci

2021 ◽  
Vol 118 (42) ◽  
pp. e2018640118
Author(s):  
LaTasha C. R. Fraser ◽  
Ryan J. Dikdan ◽  
Supravat Dey ◽  
Abhyudai Singh ◽  
Sanjay Tyagi
Keyword(s):  
Gene Expression ◽  
Transcription Factors ◽  
Single Molecule ◽  
Single Cells ◽  
Global Changes ◽  
Messenger Rnas ◽  
Histone Acetyl Transferase ◽  
Gene Expression Noise ◽  
Expression Noise ◽  
Eukaryotic Genes

Many eukaryotic genes are expressed in randomly initiated bursts that are punctuated by periods of quiescence. Here, we show that the intermittent access of the promoters to transcription factors through relatively impervious chromatin contributes to this “noisy” transcription. We tethered a nuclease-deficient Cas9 fused to a histone acetyl transferase at the promoters of two endogenous genes in HeLa cells. An assay for transposase-accessible chromatin using sequencing showed that the activity of the histone acetyl transferase altered the chromatin architecture locally without introducing global changes in the nucleus and rendered the targeted promoters constitutively accessible. We measured the gene expression variability from the gene loci by performing single-molecule fluorescence in situ hybridization against mature messenger RNAs (mRNAs) and by imaging nascent mRNA molecules present at active gene loci in single cells. Because of the increased accessibility of the promoter to transcription factors, the transcription from two genes became less noisy, even when the average levels of expression did not change. In addition to providing evidence for chromatin accessibility as a determinant of the noise in gene expression, our study offers a mechanism for controlling gene expression noise which is otherwise unavoidable.

scholarly journals Enhancement of gene expression noise due to nonspecific transcription factor binding

2019 ◽  
Author(s):  
Supravat Dey ◽  
Mohammad Soltani ◽  
Abhyudai Singh
Keyword(s):  
Gene Expression ◽  
Stochastic Dynamics ◽  
Gene Expression Noise ◽  
Downstream Target ◽  
High Affinity ◽  
Expression Noise ◽  
Degradation Rates ◽  
Poisson Limit ◽  
Random Fluctuations

ABSTRACTThe genome contains several high-affinity non-functional binding sites for transcription factors (TFs) creating a hidden and unexplored layer of gene regulation. We investigate the role of such “decoy sites” in controlling noise (random fluctuations) in the level of a TF that is synthesized in stochastic bursts. Prior studies have assumed that decoy-bound TFs are protected from degradation, and in this case decoys function to buffer noise. Relaxing this assumption to consider arbitrary degradation rates for both bound/unbound TF states, we find rich noise behaviors. For low-affinity decoys, noise in the level of unbound TF always monotonically decreases to the Poisson limit with increasing decoy numbers. In contrast, for high affinity decoys, noise levels first increase with increasing decoy numbers, before decreasing back to the Poisson limit. Interestingly, while protection of bound TFs from degradation slows the time-scale of fluctuations in the unbound TF levels, decay of bounds TFs leads to faster fluctuations and smaller noise propagation to downstream target proteins. In summary, our analysis reveals stochastic dynamics emerging from nonspecific binding of TFs, and highlight the dual role of decoys as attenuators or amplifiers of gene expression noise depending on their binding affinity and stability of the bound TF.

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