Spatial and temporal single-cell profiling of RNA compartmentalization in neurons with nanotweezers

Annie Sahota; Binoy Paulose Nadappuram; Zoe Kwan; Flavie Lesept; Jack H. Howden; Suzanne Claxton; Josef T. Kittler; Michael J. Devine; Joshua B. Edel; Aleksandar P. Ivanov

doi:10.1021/acsnano.5c02056

Spatial and temporal single-cell profiling of RNA compartmentalization in neurons with nanotweezers

Annie Sahota, Binoy Paulose Nadappuram, Zoe Kwan, Flavie Lesept, Jack H. Howden, Suzanne Claxton, Josef T. Kittler, Michael J. Devine, Joshua B. Edel, Aleksandar P. Ivanov^*

^*Corresponding author for this work

Pure And Applied Chemistry

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Abstract

Emerging techniques for mapping mRNAs within the subcellular compartments of live cells hold great promise for advancing our understanding of the spatial distribution of transcripts and enabling the study of single-cell dynamics in health and disease. This is particularly critical for polarized cells, such as neurons, where mRNA compartmentalization is essential for regulating gene expression, and defects in these localization mechanisms are linked to numerous neurological disorders. However, many subcellular analysis techniques require a compromise between subcellular precision, live-cell measurements, and nondestructive access to single cells in their native microenvironment. To overcome these challenges, we employ a single-cell technology that we have recently developed, the nanotweezer, which features a nanoscale footprint (∼100 nm), avoids cytoplasmic fluid aspiration, and enables rapid RNA isolation from living cells with minimal invasiveness. Using this tool, we investigate single-cell mRNA compartmentalization in the soma and dendrites of hippocampal neurons at different stages of neuronal development. By combining precise targeting with sequential sampling, we track changes in mRNA abundance at dendritic spine regions of the same neuron, both before and after stimulation. This minimally invasive approach enables time-resolved, subcellular gene expression profiling of the same single cell. This could provide critical insights into polarized cells and advance our understanding of biological processes and complex diseases.

Original language	English
Pages (from-to)	18522-18533
Number of pages	12
Journal	ACS Nano
Volume	19
Issue number	19
Early online date	6 May 2025
DOIs	https://doi.org/10.1021/acsnano.5c02056
Publication status	Published - 20 May 2025

Funding

A.S. was supported by a scholarship from the EPSRC CDT in Chemical Biology and acknowledge support from UKRI/ Wellcome grant EP/T022000/1−PoLNET3. A.P.I. and J.B.E. acknowledge support from EPSRC grant EP/V049070/1. This project has also received funding from the European Research Council (ERC) under the European Union’s Horizon 2020research and innovation program (grant agreement nos.724300 and 875525). M.J.D. was supported by the Francis Crick Institute, which receives its core funding from Cancer Research U.K. (CC2206), the U.K. Medical Research Council(CC2206), and the Wellcome Trust (CC2206). B.P.N. acknowledges support from the Analytical Chemistry Trust Fund and Community for Analytical Measurement Science fellowship (Ref. No. 600310/21/07) and Academy of Medical Sciences Springboard (SBF008\1179).

Keywords

RNA
nanobiopsy
nanotweezer
neuron
single-cell
synaptic plasticity

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10.1021/acsnano.5c02056Licence: CC BY 4.0

Sahota-etal-ACSN-2025-Spatial-and-temporal-single-cell-profiling-of-RNA-compartmentalizationFinal published version, 10 MBLicence: CC BY 4.0

Cite this

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title = "Spatial and temporal single-cell profiling of RNA compartmentalization in neurons with nanotweezers",

abstract = "Emerging techniques for mapping mRNAs within the subcellular compartments of live cells hold great promise for advancing our understanding of the spatial distribution of transcripts and enabling the study of single-cell dynamics in health and disease. This is particularly critical for polarized cells, such as neurons, where mRNA compartmentalization is essential for regulating gene expression, and defects in these localization mechanisms are linked to numerous neurological disorders. However, many subcellular analysis techniques require a compromise between subcellular precision, live-cell measurements, and nondestructive access to single cells in their native microenvironment. To overcome these challenges, we employ a single-cell technology that we have recently developed, the nanotweezer, which features a nanoscale footprint (∼100 nm), avoids cytoplasmic fluid aspiration, and enables rapid RNA isolation from living cells with minimal invasiveness. Using this tool, we investigate single-cell mRNA compartmentalization in the soma and dendrites of hippocampal neurons at different stages of neuronal development. By combining precise targeting with sequential sampling, we track changes in mRNA abundance at dendritic spine regions of the same neuron, both before and after stimulation. This minimally invasive approach enables time-resolved, subcellular gene expression profiling of the same single cell. This could provide critical insights into polarized cells and advance our understanding of biological processes and complex diseases.",

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author = "Annie Sahota and \{Paulose Nadappuram\}, Binoy and Zoe Kwan and Flavie Lesept and Howden, \{Jack H.\} and Suzanne Claxton and Kittler, \{Josef T.\} and Devine, \{Michael J.\} and Edel, \{Joshua B.\} and Ivanov, \{Aleksandar P.\}",

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AU - Sahota, Annie

AU - Paulose Nadappuram, Binoy

AU - Kwan, Zoe

AU - Lesept, Flavie

AU - Howden, Jack H.

AU - Claxton, Suzanne

AU - Kittler, Josef T.

AU - Devine, Michael J.

AU - Edel, Joshua B.

AU - Ivanov, Aleksandar P.

PY - 2025/5/20

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N2 - Emerging techniques for mapping mRNAs within the subcellular compartments of live cells hold great promise for advancing our understanding of the spatial distribution of transcripts and enabling the study of single-cell dynamics in health and disease. This is particularly critical for polarized cells, such as neurons, where mRNA compartmentalization is essential for regulating gene expression, and defects in these localization mechanisms are linked to numerous neurological disorders. However, many subcellular analysis techniques require a compromise between subcellular precision, live-cell measurements, and nondestructive access to single cells in their native microenvironment. To overcome these challenges, we employ a single-cell technology that we have recently developed, the nanotweezer, which features a nanoscale footprint (∼100 nm), avoids cytoplasmic fluid aspiration, and enables rapid RNA isolation from living cells with minimal invasiveness. Using this tool, we investigate single-cell mRNA compartmentalization in the soma and dendrites of hippocampal neurons at different stages of neuronal development. By combining precise targeting with sequential sampling, we track changes in mRNA abundance at dendritic spine regions of the same neuron, both before and after stimulation. This minimally invasive approach enables time-resolved, subcellular gene expression profiling of the same single cell. This could provide critical insights into polarized cells and advance our understanding of biological processes and complex diseases.

AB - Emerging techniques for mapping mRNAs within the subcellular compartments of live cells hold great promise for advancing our understanding of the spatial distribution of transcripts and enabling the study of single-cell dynamics in health and disease. This is particularly critical for polarized cells, such as neurons, where mRNA compartmentalization is essential for regulating gene expression, and defects in these localization mechanisms are linked to numerous neurological disorders. However, many subcellular analysis techniques require a compromise between subcellular precision, live-cell measurements, and nondestructive access to single cells in their native microenvironment. To overcome these challenges, we employ a single-cell technology that we have recently developed, the nanotweezer, which features a nanoscale footprint (∼100 nm), avoids cytoplasmic fluid aspiration, and enables rapid RNA isolation from living cells with minimal invasiveness. Using this tool, we investigate single-cell mRNA compartmentalization in the soma and dendrites of hippocampal neurons at different stages of neuronal development. By combining precise targeting with sequential sampling, we track changes in mRNA abundance at dendritic spine regions of the same neuron, both before and after stimulation. This minimally invasive approach enables time-resolved, subcellular gene expression profiling of the same single cell. This could provide critical insights into polarized cells and advance our understanding of biological processes and complex diseases.

KW - RNA

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KW - synaptic plasticity

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ER -

Spatial and temporal single-cell profiling of RNA compartmentalization in neurons with nanotweezers

Abstract

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Keywords

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